Title of Invention	SOLID-PHASE OLIGOSACCHARIDE TAGGING: A TECHNIQUE FOR MANIPULATION OF IMMOBILIZED CARBOHYDRATES
Abstract	The invention relates to methods of manipulating immobilized carbohydrates by derivatisation. Depending on the nature of the derivatisation, the carbohydrate may thereby be more easily detected and/or identified or handled. In particular, the ivention relates to methods of preparing a reactive sugar comprising the steps of: i) providing a sample comprising a reducing sugar; (ii) providing a solid support covalently attached to a linker comprising a capture group comprising an - NH2 group, wherein said linker optionally is attached to said solid support via a spacer; iii) reacting said reducing sugar with said -NH2 group, thereby obtaining an immobilized sugar; iv) reacting free -NH2 groups with a capping agent, wherein the capping agent com-prises a reactive group capable of reacting with an -NH2 group; and v) reducing C=N bonds with a reducing agent, thereby obtaining an reactive sugar of the struc-ture SugarCHn- NH-linked to a solid support via linker and optionally a spacer, wherein n is 1 or 2.

Title of Invention

SOLID-PHASE OLIGOSACCHARIDE TAGGING: A TECHNIQUE FOR MANIPULATION OF IMMOBILIZED CARBOHYDRATES

Abstract

The invention relates to methods of manipulating immobilized carbohydrates by derivatisation. Depending on the nature of the derivatisation, the carbohydrate may thereby be more easily detected and/or identified or handled. In particular, the ivention relates to methods of preparing a reactive sugar comprising the steps of: i) providing a sample comprising a reducing sugar; (ii) providing a solid support covalently attached to a linker comprising a capture group comprising an - NH2 group, wherein said linker optionally is attached to said solid support via a spacer; iii) reacting said reducing sugar with said -NH2 group, thereby obtaining an immobilized sugar; iv) reacting free -NH2 groups with a capping agent, wherein the capping agent com-prises a reactive group capable of reacting with an -NH2 group; and v) reducing C=N bonds with a reducing agent, thereby obtaining an reactive sugar of the struc-ture SugarCHn- NH-linked to a solid support via linker and optionally a spacer, wherein n is 1 or 2.

Full Text	Solid-Phase Oligosaccharide Tagging: A technique for manipulation of immo- bilized carbohydrates. All patent and non-patent references cited herein are hereby incorporated by refer- ence. Field of invention The present invention relates to the field of carbohydrate manipulation. In particular, the invention relates to methods of manipulating immobilised carbohydrates by deri- vatisation. Depending on the nature of the derivatisation, the carbohydrate may thereby be more easily detected and/or identified or handled. Thus, in one aspect the invention relates to the field of carbohydrate detection and identification. Background of the invention Carbohydrates exist in many forms in nature. In animals including man, examples include free reducing sugars in solution (such as the monosaccharide glucose in serum), free oligosaccharides in solution (such as the disaccharide lactose in milk), they can be attached to peptides or proteins through covalent linkages to a variety of amino acids (such as asparagine, serine, threonine and others), covalently attached to lipids such as ceramide (as in gangliosides) or attached to membrane anchors via phosphatidylinositols. Sugars are also found attached to many small molecules in- cluding some involved in metabolism, such as glucuronides. In the above examples, the length of the sugar chains can vary from one to over 100 sugar residues. In lower organisms, including bacteria and plants, an even wider array of structures exists. The surface of bacterial cells can be covered by sugar polymers that are thousands of residues long, which can act as antigens in the detection of bacteria and as vaccines. Sugars are an integral part of bacterial cell walls. The sugars can themselves be antibiotics (such as the aminoglycoside antibiotics, for example streptomycin), or can be found as essential components of antibiotics (such as erythromycin and vancomycin), as enzyme inhibitors (as in Acarbose) or as anti- cancer agents (such as for example calicheamycin). One area of particular interest is the structure of the carbohydrate chains (glycans) found attached to glycoproteins and glycoiipids. The glycosylation pattern of glyco- proteins has been shown to be important for their biologlcal functions, including their bioavailablity, their targeting, and have even been directly correlated with the metas- tatic potential of tumor cells. The glycosylation pattern of human serum transferrin, for example, is being used as a diagnostic test for a series of genetic diseases termed Carbohydrate-Deficient Glycosylation Syndromes. Specific glycolipid se- quences have been shown to be involved in neuronal development and cell surface signalling, in diabetes, and are accumulated in certain specific metabolic diseases such as Tay-Sachs, for which they are diagnostic. The linkages between the sugar residues in the oligosaccharides and polysaccha- rides described above can have either the alpha or beta configurations, and the gly- cans can be multiply branched. The diversity of structures possible for glycan chains is therefore enormous and their structural characterization is therefore inherently complex. There is therefore a strong interest in methods for the detection, structural characterization, identification, quantitation, and chemical/enzymatic manipulation of carbohydrate and glycan structures, in research, in diagnostics, in monitoring the glycosylation of recombinant glycoproteins and in the development of new pharma- ceutical agents. Several methods are in current use for the analysis for carbohydrate structures, and these have recently been reviewed. Underivatized oligosaccharides and glycoiipids can be analyzed by NMR-spectroscopy, by mass-spectrometry, and by chromatog- raphy. For the much larger glycoproteins, mass spectrometry provides more limited information but analysis of their proteolytic digests, i.e. glycopeptides, has been ex- tensively used. Indirect structural information about underivatized oligosaccharides can also be deduced from their abilities to interact with carbohydrate-binding pro- teins such as lectins, antibodies or enzymes. Carbohydrates themselves have no characteristic chromophores, only N-acetyl groups, so monitoring their separation by optical or spectroscopic detection is not commonly used. Pulsed amperometric detection of the polyols has however been an important technique for detection in chromatography. The most widely used method for high-sensitivity detection of carbohydrates has been the labeling of the reducing ends (lactols, tautomers of hydroxyaidehydes and hydroxyketones) with either radioactive or fluorescent TAGs. Both chemical and enzymatic methods have been described that cleave carbohydrates from glycopro- teins and glycolipids, permitting the generation of the required reducing sugars from glycoproteins, glycolipds and other glycoconjugates. Most commonly, such reducing sugars are reacted with amino-containing derivatives of fluorescent molecules under conditions of reductive amination: i.e., where the initially formed imines (C=N) are reduced to amines (CH-NH) to produce a stable linkage. In most cases, the labeling reactions have been performed in solution using a large excess of labeling agent. This requires separation of the excess labeling agent and its by-products prior to or during analysis. Other TAGs of utility in mass-spectrometry have been added in the same manner, by either amination or reductive amination, the detection then being performed by the mass-spectrometer. Once the label has been added to permit specific detection, the carbohydrates de- scribed above can subsequently be subjected to separation and detec- tion/quantification. Additional structural information can be obtained by exposing the tagged carbohydrates to enzymes such as glycosidases. If specific glycosidases act on the tagged carbohydrates, they can cleave one or more sugar residues resulting in a change in chromatographic or electrophoretic mobility, as detected by, for ex- ample, a fluorescence detector in HPLC, CE or by a change in their mobility in SDS- PAGE, or a change in their mass as detected by a change in m/z value in a mass- spectrometer. Arrays of enzymes have been used to provide a higher throughput analysis. Below a short overview of prior art is glven: Gao et al. 2003 reviews suitable techniques for derivatisation of carbohydrates in solution. In solution carbohydrates may be derivatised by reductive amination. In general, -NH2 groups of amines may react with aidehyde or ketone group of reduc- ing sugars, thereby producing compounds of -C=N structure. Such compounds may further be reduced for example by NaCNBH3. Gao et al., 2003 does not disclose manipulation of immobilised carbohydrates. US5,100,778 describes a method for oligosaccharide sequencing comprising plac- ing an identifylng label on the reducing terminal residue of an oligosaccharide, divid- ing into a plurality of separate portions, treating each portion with for example spe- cific glycosidases, pooling product and analysing the pools obtained. The document does not describe immobilised oligosaccharides. US4,419,444 describes methods for chemically binding organic compounds contain- ing carbohydrate residues to a support bearing reactive -NH2 groups. The methods involve either the periodate oxidation of carbohydrate diols to produce reactive aide- hydes by cleaving of C-C bonds in the carbohydrate or oxidation of -CH2OH groups to -CHO groups enzymatically. Both oxidations will result in alteration of the struc- ture of the carbohydrate. The reactive aidehydes can be immobilised by reaction with the -NH2 groups. After immobilisation of the carbohydrate containing com- pound a reduction step (for example using NaBH4) may be performed to increase stability. The document describes neither the immobilization of a reducing sugar through its reducing end nor manipulation of immobilised altered carbohydrate con- taining compounds via the reduced amine bond. Furthermore, the chemical nature of the carbohydrate has been altered and this alteration may impair further modula- tions, such as specific enzymatic cleavage by glycosidases. The document also does not describe the addition of any chemical reagents to the immobilised oligo- saccharide that result in the addition of molecular structures to it. W092/719974 describes a method of sequencing oligosaccharides. The method involves immobilising oligosaccharides on a solid support and subsequent treatment with a variety of glycosidases. Prior to immoblisation, the oligosaccharide may be linked to a conjugate. The document does not describe modulation of immobilised oligosaccharides other than glycosidase treatment. The above describes the biologlcal importance and complexity of glycans, and summarizes some benefits of attaching TAGs to reducing sugars, such as mono- saccharides, as well as to the reducing sugar end of oligosaccharides. To date, such attachment has been performed in solution using large excesses of tagglng agent (and often additional chemical agents such as reducing agents), and thus require time consuming and frequently difficult separation techniques to be applied before either detection or further manipulation. Such separation techniques invariably result in losses of material, and dilution, thus considerably complicating and biasing the analysis. There is therefore a great need for simple methods that can install a TAG onto a carbohydrate structure and further manipulate the structure, without the need for complex and biased methods for separating reaction starting materials, reagents, by-products and sought after products. We describe herein such simple methods. Summary of the invention The present invention relates to methods of covalent attachment of reducing sugars, (which may be any of the reducing sugars mentioned herein below in the section "Reducing sugar") to a solid-support (which may be any of the solid supports de- scribed herein below in the section "Solid support") through reaction with an immobi- lized molecule consisting of an optional spacer (i.e. with or without spacer) and a linker (which can be cleavable) that incorporates a capture group containing an -NH2 functionality. The resulting immobilized sugar has an acyclic form with a C=N bond, which may be in equilibrium with it's cyclic glycosylamine tautomer. Free -NH2 groups on the solid support after immobilisation may be capped and the C=N bond can be reduced. This method is outlined in fig. 1 A+B^E. The figure shows an underivatised pyranose, which however is meant to represent any reduc- ing sugar. In a variation, the methods of the invention may comprise reduction of the immobi- lized sugar containing a C=N bond (exemplified by structure C, fig. 1) to CH-NH prior to capping free -NH2 groups, producing a compound of structure Cred (fig. 1). The - NH2 groups in Cred may then be capped at this stage to produce a compound of the same structure E as that produced by the sequence C to D to E described above and shown in fig. 1. Compounds of the structure E may thus be produced by either the sequence A+B goes to C goes to D goes to E, or A+B goes to C goes to Cred goes to E. It is therefore an object of the present invention to provide methods of preparing a reactive sugar, said method comprising the steps of i. Providing a sample comprising a reducing sugar (such as A in fig. 1) ii. Providing a solid support (e.g. solid in fig. 1) covalently attached to a linker comprising a capture group comprising an -NH2 group, wherein said linker optionally is attached to said solid support via a spacer (such as B in fig. 1) iii. Reacting said reducing sugar with said -NH2 group, thereby obtaining an immobilised sugar (such as C in fig. 1), iv. Reacting free -NH2 groups with a capping agent, wherein the capping agent comprises a reactive group capable of reacting with a -NH2 group v. Reducing C=N bonds with a reducing agent vi. thereby obtaining a reactive sugar containing the structure SugarCHn- NH- linked to a solid support via a linker and optionally a spacer, wherein n is 1 or 2 (such as compound E of fig. 1), wherein steps iv and v may be performed in any order. In embodiments of the invention wherein step iv is performed prior to step v, capping -NH2 groups in step iv will for example result in compound D of fig. 1, whereas the reduction performed in step v will for example result in compound E of fig. 1; In embodiments of the invention wherein step v is performed prior to step iv, then the reduction of the C=N bond (for example of compound C of fig. 1) will for example result in compound Cred of fig. 1. The capping of the -NH2 groups in step iv will for example produce the compounds of structure E, fig.1. It is comprised within the pre- sent invention that the sample comprising the reducing sugar may be incubated with the solid support and the reducing agent simultaneously. Thus, reduction of C=N bonds (step v) will be performed immediately following reaction of the reducing sugar with the -NH2 group of the solid support (step iii). In step iii), preferably, the reducing end of said reducing sugar is reacted with said - NH2 group. Thus preferably the aidehyde group or the hemiacetal of the reducing sugar is reacted with the -NH2 group. it is preferred that the methods further comprise the step of vii. Reacting the -NH- group of the reactive sugar (for example com- pound E of fig. 1) with a derivatising agent comprising a nitrogen- reactive functional group (X), thereby obtaining a sugar covalently at- tached to said agent. Said sugar covalently attached to said agent may for example be compound F of fig. 1 (when the derivatising agent is a TAG) or compound H of fig.1, when the derivatising agent is a tether linked to functional group. The term "TAG" in the present context, and in fig. 1 (vide infra) is meant to indicate any atom, molecule or entity that can become covalently attached to another mole- cule thereby labelling said another molecule as having undergone the covalent at- tachment. Brief Description of the drawings Fig. 1 illustrates an example of the method according to the invention. Fig. 1: A-E illustrates capture and manipulation of a reducing sugar on a solid support to glve a reactive sugar E. Fig. 1: E-G and J illustrates manipulation of a reactive sugar E on a solid support, and cleavage of a tagged sugar. The methods of the invention may comprise one or more of the steps illustrated in the fig. 1. In the fig. 1 the reducing sugar is exemplified with a pyranose, however any reducing sugar may be used with the method. The figure shows an example where the linker is linked to the solid sup- port via a spacer, however, the linker may also be directly linked to the solid support. The solid support is designated "Solid" in the figure, however it may be any of the solid supports mentioned herein below. Fig. 2. Structures 1 -10 of the reducing sugars, and mixtures thereof, used in the examples of the present invention. Fig. 3. Synthesis of a linker (14) and structure of a spacer (15). Fig. 4. Solution-phase synthesis of the TMR-tagged D-galactose derivative, GalCH2- N(R)-TMR (21), and description of nomenclature used for monosaccharide stan- dards. Fig. 5. Structures 21 - 28 of synthetic tagged derivatives of the eight common mammalian monosoaccharides of general structure SugarCH2-N(R)-TMR. Fig. 6. Structures of the four solid supports Bp, B°, B1 and B2. Fig. 7. Structures of some capping agents. Fig. 8. Structures of some nitrogen-reactive tagglng agents used, of general struc- ture TAG-X Fig. 9. Example of E goes to J (30) using the protected nitrogen-reactive agent 29 of general structure X-tether-YP. Fig. 10. Separation by CE of the eight TMR-labelled monosaccharide standards shown in Fig. 5. The order of elution is GainAc (27), Xyl (24), Man (23), Glc (22), GlcNAc (26), Fuc (25), Gal (21), and glcA (28). The top trace is an expansion. Fig. 11. CE of Gp3 (with LacNAc as the reducing sugar tagged using TRITC, section 4.2.1). Fig. 12. Eiectrospray mass-spectrum in the negative ion mode of Gp5 (with lacto-N- tetraose as the reducing sugar tagged using 4-bromophenylisothiocyanate, section 4.2.2). The inset is an expansion showing the two peaks corresponding to the major isotopes of Br. Fig. 13. CE of Gp6a (with monosaccharide mixture 6 tagged using TRITC, section 4.2.3). X denotes unidentified peaks. The order of elution is GainAc (27), Man (23) and Fuc (25). The lower trace is an expansion. Fig. 14. CE of Gp7a (with monosaccharide mixture 7 tagged using TRITC, section 4.2.4). X denotes unidentified peaks. The order of elution is GainAc (27), Man (23) and Fuc (25). The lower trace is an expansion. Fig. 15. CE of Gp9 (with the oligosaccharide mixture 9 tagged using FITC, section 4.2.5). The order of elution is G7 to G2 (Fig. 2). Fig. 16. CE of Gp10 (ribonuclease B oligosaccharides 10 tagged using FITC, section 4.2.6). Fig. 17. CE of G12 (with Gal 2 as the reducing sugar tagged using TRITC, section 4.3.1). Fig. 18. CE of G15 (with LNT 5 as the reducing sugar tagged using TRITC, section 4.3.2). Fig. 19. CE of G18 (with 8 as the reducing sugar mixture tagged using TRITC, sec- tion 4.3.3). The order of elution is LNT followed by Gal. Fig. 20. CE of the cleaved products G°5 (A), G15 (B) and G25 (C) after beta- galactosidase digestion of immobilized LNT (5), section 5.1.1). The TRITC-labelled LNT tetrasaccharide elutes first near 36 minutes. Loss of galactose ylelds the trisac- charide product eluting after 38 minutes. Fig. 21. CE of the cleaved product before (trace A) and after (trace B) incubation of F24 (maltotriose (G3) as the reducing sugar tagged using TRITC) with glucoamy- lase, section 5.1.2). A reference sample of tagged Glc (22, Fig. 5) was added to the sample prior to recording trace A. Fig. 22. CE of the cleaved products obtained after beta-galactosidase treatment of C25 (bearing LNT and free NH2 groups), followed by capture of the released galac- tose, reduction and tagglng using TRITC, section 5.2. The order of elution is LNT, the trisaccharide resulting from loss of galactose and galactose (21). Fig. 23. CE analysis of the cleaved products derived from C22 (immobilized galac- tose) after capping with various agents, reduction and labelling using TRITC, section 6.1). The capping agents were A (acetic anhydride), B (benzoic anhydride), C (tri- chloroacetic anhydride) and D (dibromoxylene). Tagged galactose (21) elutes near 17 minutes in all traces. Fig. 24. CE of the cleaved product obtained from processing galactose through the sequence C->Cred->G, section 6.2). The galactose 21 elutes at 17 minutes. Detalled description of the invention Methods of manipulating a reducing sugar. The present invention relates to methods of manipulating a reducing sugar. An ex- ample of the methods of the invention is outlined in fig. 1. It should be noted that the methods of the invention do not necessarily involve all of the steps illustrated in fig. 1. Thus the methods may comprise only some of the steps outlined in fig. 1. Pref- erably, the methods will comprise at least the steps A+B—>C, C->D and D->E, or the steps A+B->C, C—>Cred and Cred->E In fig, 1 the reducing sugar is exemplified by a pyranose, however any reducing sugar may be used with the invention, in particular any of the reducing sugars described herein below in the section "Reducing sugar". The -OH group dissecting the pyranose ring in fig. 1 is meant to indicate that the reducing sugar may bear one or more hydroxyl groups attached to it. Each of the steps of the methods of the invention are described herein below in more detall, wherein capital letters A to J and Cred refer to fig. 1 The identity of each of the compounds or intermediates of the present invention, for example of compounds A, B, C, Cred D, E, F, G, H, I or J may be verified by stan- dard techniques known to the skilled person, such as by NMR. A. Reducing sugar The term "reducing sugar" as used herein covers the classical definition of sugars that are capable of reducing Cu2+ to Cu+. Whether a sugar is reducing may for ex- ample be tested using Fehlings reagent. In more modem terminology, reducing sugars are sugars that comprise an aidehyde group or a hemiacetal of the formula R2C(OH)OR', wherein R' is not H. Preferably, a reducing sugar is a carbohydrate structure containing an aidehyde, which is in equilibrium with the cyclized form called a hemiacetal. D-glucose is a non-iimiting example of such a reducing sugar. The most abundant cyclic forms contain 5-membered rings, termed furanoses, and 6-membered rings termed pyranoses. (See rules of nomenclature). The term "sugar" as used herein covers monosaccharides, oligosaccharides, poly- saccharides, as well as compounds comprising monosaccharide, oligosaccharide, or polysaccharide. The terms "carbohydrate" and "sugar" are herein used inter- changeably. Oligosaccharides and polysaccharides are compounds consisting of monosaccha- rides linked glycosidically. in general polysaccharides comprise at least 10 mono- saccharide residues, whereas oligosaccharides in general comprise in the range of 2 to 10 monosaccharides. Oligosaccharides and polysaccharides may be linear or branched. A monosaccharide is defined as a polyhydroxy aidehyde H-(CHOH)n- CHO or polyhydroxyketone H-(CHOH)n-CO-(CHOH)m-H, wherein m and n are inte- gers. Preferred monosaccharides comprises in the range of 4 to 9 carbons, thus preferably for polyhydroxy aidehydes n is an integer in the range of 3 to 8 and for polyhydroxyketones n+m is an integer in the range of 3 to 8. Monosaccharides are compounds such as aidoses and ketoses and a wide variety of derivatives thereof. Derivation includes those obtained by oxidation, deoxygenation, replacement of one or more hydroxyl groups by preferably a hydrogen atom, an amino group or thiol group, as well as alkylation, acylation, sulfation or phosphorylation of hydroxy groups or amino groups. According to IUPAC nomenclature, carbohydrates are compounds of the stoichiometric formula Cn(H2O)n, such as aidoses and ketoses as well as substances derived from monosaccharides by reduction of the carbonyl group (aiditols), by oxidation of one or more terminal groups to carboxylic acids, or by replacement of one or more hydroxyl group(s) by a hydrogen atom, an amino group, thiol group or similar groups or derivatives of these compounds. In a preferred embodiment, the reducing sugar is a naturally occurring reducing sugar or a reducing sugar, which has been liberated from a naturally occurring or recombinantly produced compound comprising a carbohydrate, preferably without having been subject to furthermore modifications after liberation. In particular it is preferred that the reducing sugar, is a naturally occurring reducing sugar or a reduc- ing sugar liberated from a naturally occurring or recombinantly produced compound, wherein none of the alcohol groups of said naturally occurring sugar or said liber- ated sugar have been enzymatically transformed to an aidehyde or ketone by oxida- tion at the level of the oligosaccharide. It is also preferred that the reducing sugar, is a naturally occurring reducing sugar or a reducing sugar liberated from a naturally occurring or recombinantly produced compound, wherein said naturally occurring sugar or said liberated sugar have not been subjected to periodate treatment. It is thus generally preferred that no alcohol group of said naturally occurring sugar or said liberated sugar have been transformed to an aidehyde or ketone. In this context recombinantly produced compounds are compounds produced by a living organism with the aid of recombinant technologles, for example heterologous glycoproteins. Reducing sugars may be derived from a variety of sources. For example the reduc- ing sugar may be obtained from a living organism or part of a living organism, such as animals or plants or from one or more specific animal or plant tissues, from or- ganisms such as prokaryotic or eukaryotic cells, from viruses, from in vitro culti- vated mammalian cells, insect cells, plant cells, fungl, bacterial cells, yeast, or phages. For example the reducing sugar may be isolated from extracts of any of the aforementioned cells, microbial organisms or living organisms. Such extracts may comprise reducing sugars, such as free carbohydrates. Extracts may also comprise compounds comprising monosaccharide, oligosaccharide, polysaccharide or carbo- hydrate moieties, notably glycoproteins or glycolipids or small organic molecules to which carbohydrates are attached, which are generally referred to as glycosides. Glycoproteins are compounds in which a carbohydrate component is linked to a peptide, polypeptide or protein component. Thus as used herein the term glycopro- tein also cover proteoglycans and glycosaminoglycans. Glycolipids are compounds containing one or more monosaccharide, oligosaccharide, polysaccharide or carbo- hydrate moieties bound by a glycosidic linkage to a hydrophobic moiety such as an acylglycerol, a sphingoid, a ceramide (W-acylsphingoid) or a prenyl phosphate. Gly- cosides are meant to describe small (MWt 100 - 5000) organic molecule glycosidi- cally linked to one or more sugars via elther O, N or S. Reducing sugars may also be the products of chemical synthesis, or chemi- cal/enzymatic synthesis, such as oligosaccharides prepared in vitro by chemical synthesis in solution or on the solid phase. These same synthetic oligosaccharides may be further modified by enzymatic reaction, such as for example by the sulfation, phosphorylation or glycosylation. Thus the methods described herein may also be used for manipulation of synthetic or semi-synthetic oligosaccharides or oligosac- charide libraries. Preferably, the monosaccharide, oligosaccharide, polysaccharide or carbohydrate moiety is liberated from the glycoprotein, prior to performing the methods of the in- vention. This may be done by standard methods known to the skilled person, N- linked monosaccharides, oligosaccharides, polysaccharides or carbohydrates may be cleaved from glycoproteins by chemical or enzymatic methods. Enzymatic methods may for example involve use of glycosidases such as endoglycosidases H and F or N-glycanases such as PNGase-F.O-linked monosaccharides, oligosac- charides, polysaccharides or carbohydrates may be cleaved from glycoproteins by chemical methods, including hydrazinolysis or alkaline β-elimination or enzymatically using enzymes such as an O-glycosidase. Chemical methods useful for release of both N-linked and O-linked includes reactions with strong nucleophiles and/or strong bases such as hydrazine. Carbohydrates may be cleaved from small organic mole- cules using elther acidic or basic reactions, or by the action of glycosidases. In one embodiment of the invention a predetermined amount of a reference stan- dard is added to the sample comprising the reducing sugar. This may facilitate quantification of said reducing sugar after immobilisation or after immobilisation and release in embodiments of the invention wherein the linker is cleavable. The reference standard may be any compound capable of reacting with -NH2, for example any compound comprising one of the nitrogen reactive functional groups described herein below in the section "E->F. Adding TAGs". Preferably the refer- ence standard is an aidehyde or a ketone, more preferably a sugar. In another em- bodiment of the invention, the same or different reference standard is added to the solid support prior to contact with the solution containing the reducing sugar with or without the added reference standard included in the solution (see herein below in section "B. Solid support"). Thus two or more reference standards may be used, one (or more) added to the solid support prior to contact of the solid support with the solution comprising a reducing sugar, and one or more added to the solution con- taining the reducing sugar. One or more reference standards may also be added to to the solid support after contact with the reducing sugar, but preferably prior to capping. Thus for example the reference standard may be added to compound C or Cred of fig. 1, preferably after a washing step. In embodiments of the invention wherein the solid support is coupled to a reference standard (see herein below in section "B. Solid support") it is preferred that different reference standards are used. In one embodiment of the invention the methods comprises a step of pre-treatment of the sample to be used with the method. In particular, a sample comprising glyco- sidically-linked sugars such as a glycoproteins, glycolipids or glycosides may be pretreated with a scavenger resin prior to reaction with the solid support. The scav- enger resin is preferably a resin comprising a nucleophilic group capable of reacting with aidehydes and ketones, including reducing sugars, preferably the scavenger resin comprises an amino group or a hydrazine. Incubation of the sample with the scavenger resin will thus remove additional aidehydes, ketones and reducing sug- ars. After pre-treatment, such methods will in general further comprise the step of liberating reducing sugars from said glycosidically-linked sugars thereby obtaining a sample comprising reducing sugars. The vast majority of aidehydes and ketone within said sample will thus be reducing sugars released from glycosidically-linked sugars. Said reducing sugars may be liberated by a number of methods, including chemical or enzymatic methods, such as any of the methods described herein above in this section. Treatment of the pretreated sample with for example PNGaseF can cause the release of reducing oligosaccharides into solution for cap- ture and manipulation according to the methods of the invention. The oligosaccha- rides thus released will be essentially free of contaminating carbonyl compounds. Release of reducing carbohydrates may also be effected by other enzymes, such as glycosidases, or using chemical reactions, after scavenglng of contaminating car- bonyl compounds as described above. B. Solid support The methods according to the present invention involve immobilisation of a reducing sugar to a solid support. Solid phase chemistry offers a number of advantages, such as easy handling, purification and concentration of immobiiised compounds. How- ever, not all reactions doable in solution can be performed on solid phases. The attachment to a solid support practically confer infinite size to each molecular entity. This has the effect that the molecule reacts much more slowly in a bimolecular reac- tion than the same molecule would do in solution. Some reactions that may be car- ried out in solution with an acceptable yleld simply will not perform on solid support. The term "solid support" as used herein covers physical solids as well as insoluble polymers, insoluble particles, surfaces, membranes and resins, preferably the solid support is an insoluble polymer, an insoluble particle, a surface or a resin. Thus the "solid support" may be an insoluble inorganic matrix (such as glass), an insoluble polymer (such as a plastic, for example polystyrene), an insoluble matrix consisting of parts of both organic and inorganic components (e.g. some hybrid silicates, such as compounds of the structure R-Si-O-), organic polymers in common use in solid-phase synthesis (polystyrenes, PEGA resins, PEG resins, SPOCC res- ins and hybrids thereof), polyethylene glycol chains (which can be soluble in certain organic solvents and made insoluble by the addition of other solvents). The solid may also be a metal (such as gold), an alloy, or a composite such as for example indium-tin oxide or mica. Any of the above listed solid supports may additionally be coated with agents that have an affinity for carbohydrates, such as but not limited to aryl boronates or poly- mers thereof. Such coatings can increase the concentration of carbohydrate at the surface of the solid support, enhancing the rate and yleld of capture. Organic polymers used in solid-phase synthesis for example includes TentaGel (commercially available from Rapp polymere, Tubingen, Germany), Ar- goGel (commercially available from Argonaut Technologles Inc., San Carlos, CA), PEGA (commercially available from Polymer Laboratories, Amherst, MA), POEPOP (Renil et al., 1996, Tetrahedron Lett., 37; 6185-88; available from Versamatrix, Co- penhagen, Denmark) and SPOCC (Rademann et al, 1999, J. Am, Chem. Soc., 121: 5459-66; available from Versamatrix, Copenhagen, Denmark). In one embodiment of the invention the solid support is a sensor, such as a surface acoustic wave sensor (such as any of the sensors described in Samoyolov et al. 2002, J. Molec. Recognit. 15:197-203) or a surface plasmon resonance sensor (such as any of the sensors reviewed by Homola et at., 1999, Sensors and Actua- tors B, 54: 3-15). Such solid supports may be inorganic materials such as glass, metals such as gold, organic polymeric materials or hybrids thereof and may be covered various coatings such as proteins or polysaccharides, oligomers such as as dendrimers or polymers such as polyacrylamide or polyethylene glycol. In a preferred embodiment the solid support is glass or PEGA resins. In one embodiment of the present invention the solid support is coupled to a refer- ence standard, which may facilitate quantification of immobilised reducing sugar. In particular, it is preferred that said reference standard is attached to the solid support (elther directly or indirectly) by a cleavable linker, which could facilitate quantification of immobilised and released reducing sugar. In embodiments of the invention wherein the reducing sugar is immobilised to the solid support via a cleavable linker, it is preferred that the reference standard is immobilised to the solid support via an identical or similar cleavable linker. The reference standard may be any detectable compound, for example the refer- ence standard may or may not be a sugar, preferably however it is carbohydrate. The amount of reference standard may vary, in general the solid support may com- prise in the range of 20 to 500, preferably in the range of 50 to 200, such as in the range of 90 to 110 -NH2 groups per reference standard. B. Spacer According to the present invention the solid support is optionally coupled to a linker via a spacer. However, it is also comprised within the present invention that the solid support is directly coupled to the linker. A spacer is a chemical entity in the range of 1 to 1000 atoms long. Preferably, said spacer is a linear or branched chain and/or a ring structure. The nature of the spacer may be hydrophobic or hydrophilic or have a mixture of these two properties. The group of spacers comprises molecules in common use in solid phase synthesis and on-bead, in-well or on-slide assays involving the detection of molecules attached via spacers to solid-supports. The skilled person will readily be able to identify a useful spacer for a glven solid support. The spacer is preferably an alkyl chain (more preferably a C1 to C1000 alkyl chain), which optionally may be branched, wherein said alkyl chain optionally is substituted at one or more positions by groups containing one or more of B, O, N, S, P, Si, F, CI, Br or I. The spacer may also comprise one or more aryl residues which optionally may be branched or substituted in the same manner. In one preferred embodiment, the spacer is selected from the group consisting of amides and ethers. Thus the spacer may essentially consist of a chain containing one or more amide bonds (- CONH-), one more ethylene glycol units (-CH2-CH2-O-), or combinations of these units with the alkyl or aryl chains. In one embodiment of the invention, the spacer preferably does not comprise elther a primary or a secondary amine. In another embodiment of the invention any amines comprised within the spacer are capped. B. Linker The present invention relates to capture of reducing sugars onto solid supports co- valently attached to a linker comprising a capture group. The linker serves to link the capture group, terminating in -NH2, to the solid support optionally through a spacer. The linker may be any of a large variety of linkers such as those in common use in solid-phase organic synthesis. The linker may elther be a non-cleavable linker or a cleavable linker. Non-cleavable linkers may for example be alkyl, aryl, ethers or amides, wherein any of the aforementioned may optionally be substituted. For example any of the afore- mentioned may be substituted with heteroatoms or they may contain, 0-alkyl,alkyl, aryl or heteroatoms as branches. In one example the linker comprises or essentially consists of PEG and/or polyamide. The linker may comprise a site where a reaction can be made to occur to sever the part containing the capture group (including the molecules it has captured and which have been optionally further modified) from the spacer and the solid support. Such linkers are referred to as cleavable linkers, and are in wide use in solid phase or- ganic synthesis. Examples of cieavable linkers are known where the cleavage can be effected by electrophiles, nucleophiles, oxidizing agents, reducing agents, free radicals, acid, base, light, heat or enzymes. Cieavable linkers may for example be acid labile (for example, the Rink amide as described in Rink, 1987, Tetrahedron) Lett., 28: 387 and traceless silyl linkers as described in Plunkett et at., 1995, J. Org. Chew., 60: 6006-7), base labile (for exam- ple, HMBA as described in Atherton et al. 1981, J. Chem. Soc. Perkin Trans, 1: 538), or photolabile (for example, 2-nitrobenzyl type as described in Homles et al., 1995, J. Org. Chem., 60: 2318-2319). The linkers may be more specific and restric- tive of the type of chemistry performed, such as silyl linkers (for example, those cleaved with fluoride as described in Boehm et al., 1996, J. Org. Chem., 62: 6498- 99), allyl linkers (for example, Kunz et al., 1988, Angew. Chem. Int. Ed. Engl., 27: 711-713), and the safety catch sulfonamide linker (for example, as described in Kenner et al., 1971, Chem. Commun., 12: 636-7). Enzyme cieavable linkers may for example be any of the enzyme cieavable linkers described in Reents et al., 2002, Drug Discov. Today, 7: 71-76, or any functionalised derivatives of the enzyme-labile protecting groups described in the review by Waidmann et al., 2001, Chem. Rev. 101: 3367-3396. Heat labile linkers may for example be of the type described in Meng et al., 2004, Angew. Chem. Int. Ed., 43: 1255-1260. B. Capture group According to the present invention the linker comprises a capture group, wherein the capture group comprises at least one -NH2 group. In a favourable format, the cap- ture group terminates in an -NH2 group that is attached to the linker through an op- tional group R. Thus the capture group preferably is of the structure R-NH2. R may be a simple alkyl, aryl or substituted alkyl or aryl group. Preferably, R should contain a heteroatom directly attached to the -NH2 group, to produce structures of the type linker-M-NH2, wherein M is a heteroatom (i.e. not carbon), preferably M is selected from the group consisting of N, O and S. Especially favourable are compounds where M is a heteroatom, such as in the structures linker-O-NH2 linker-NH-NH2, linker-CO-NH-NH2, linker-NH-CO-NH-NH2, linker-S(O)2NH-NH2 and Iinker-S-NH2. A+B—>C, Methods of capture The capture of the reducing sugar is done by reacting the -NH2 group of the capture group with the reducing end of said reducing sugar, i.e. with the aidehyde or he- miacetal group. The reaction can occur at any pH values but is most favored in the range of pH 2 - 9. The methods may involve the addition of one or more additives, such as additives which may elther facilitate or favourably alter the equllibrium be- tween the open chain aidehyde form of the reducing sugar and the hemiacetal form of the reducing sugar (e.g. compound A, fig. 1), wherein the open chain aidehyde form is preferred. The additive may for example be metal ions, boronates or sili- cates. The capture produces a species attached to the solid support through a cova- lent double bond (shown as C=N) where the C is derived from the sugar moiety and N from the capture group. This immobilized sugar may also be in equllibrium with its cyclic ring form, in particular if the reducing sugar was a pyranose, then the immobi- lised sugar may be in equllibrium with its cyclic 6-membered ring form (see for ex- ample compounds C and C of fig. 1), but it may also be in equllibrium with its 5- membered ring form if the appropriate OH group on the sugar is unsubstituted. The capture reaction may be performed in any useful solvent. A person of ordinary skill in the art will readily be able to identify a useful solvent for any glven com- pounds A and B. The solvent may for example be selected from the group consist- ing of water, aqueous buffer, organic solvents and mixed aqueous and organic sol- vents. The solvent may also be any of the aforementioned comprising one or more additives such as acids, bases, salts, divalent metal cations, detergents, complex- ing agents including inclusion-complex-forming molecules such as cyclodextrins or calixarenes, chelating agents (for example EDTA), borates, boronates or silicates. In a preferred embodiment the amount of solid support (compound B of fig. 1) added to the reaction is adjusted so that a molar excess of capture groups are present in relation to the reducing sugar, preferably said excess is large, such as at least 2 times, preferably at least 5 times, more preferably at least 10 times, such as at least 50 times, for example at least 100 times or more. This excess will ensure a more efficient capture of the reducing sugar. The capture reaction may be carried out at any temperature, but preferably at tem- peratures in the range of 0 to 100°C. C. Washing Once the reducing sugar has been immobilised on the solid support through reac- tion with the capture group (step A+B->C of fig. 1) the solid supports may be washed to remove non-covalently bound material. Accordingly, if the reducing sugar is provided in a solution comprising other compounds, in particular other compounds that do not comprise -NH2 reactive groups, the reducing sugar may be purified from said solution. It is thus comprised within the present invention that the reducing sugar is provided in a non-purified form, such as in the form of a crude cellular ex- tract or the like. It is also comprised that the reducing sugar may be produced from a purified or partially purified glycoprotein, glycolipid or glycoside by the action of an enzymes such as glycosidase or an amidase or through the cleavage of a glycosidic bond by chemical reagents. The skilled person will readily be able to identify sultable washing conditions for a glven immoblised sugar (compound C, fig. 1). The washing may for example be done with any of the above-mentioned solvents optionally comprising any of the above-mentioned additives in addition to detergents and denaturing agents. The washing my be performed at any temperature, but preferably at temperatures in the range of 0-100°C. C->D. Capping The solid support coupled to the immobilised sugar (such as compound C of fig. 1) still contains unreacted free -NH2 groups and can be subjected to unique manipula- tions that increase the scope of its utility. In one preferred embodiment of the invention, subsequent to immobilisation of the reducing sugar, unreacted -NH2 groups are capped by a capping agent, such as an acylating agents (e.g. acetic anhydride) or other nitrogen-reactive agents well known in the art, under conditions where the C=N bond of C does not react. After capping the solid support will no longer comprise any free amine groups, but only capped nitrogen atoms (N(H)CAP) of very low reactivity towards electrophiles. The product of the capping of compound C has for example the general structure D (see fig. 1) containing an -R-N(H)CAP group, wherein the (H) may or may not be present de- pending on the structure of the CAP group. Thus if the C=N bond linking the sugar to the solid support is reduced to an -NH-, it will be a formally SP3-hybridized nitrogen atom in the sequence R-NH-CH2-. Specific reactions may thus be directed to this group allowing specific and stoichimetric reac- tions at the reducing sugar. Preferably the capping agent specifically reacts with the remaining -NH2 groups, without substantially reacting with the C=N functionality. Such reagents are well known in the art an include common acylating agents used for amid bond formation, e.g. acetic anhydride, other alkanoic acid anhydrides, aromatic anhydrides (e.g. benzoic anhydride), cyclic anhydrides (e.g. succinic anhydride, phthalic anhydride), other active esters such as N-hydroxysuccinimide esters, pentafluorophenyl esters and a variety of active esters in common use in amide bond formation including in the solid phase synthesis of peptide bonds. The -NH2 groups may alternatively be capped by adding the corresponding free acids and an in-situ activating agent such as DCC, in common use in peptide-bond formation thereby creating an active ester in situ. Other reagents known to be reactive towards -NH2 groups can be used, such as alkyl isothiocyanates (R-NCS), aryl isothiocyantes (Ar-NCS), alkylating agents R- L (where L is a leaving group typically from the series CI, Br, I, OS(O)2R' where R' can be alkyl or aryl), Michael acceptors such as alpha-beta unsaturated carbonyl compounds (CHR=CH-CO- where R can be H, alkyl or aryl or substituted alkyl or aryl) or alpha-beta unsaturated sulfones (CHR=CHS(O)2R' or Ar where R can be H, alkyl or aryl or substituted alkyl or aryl), sulfonating agents (such as RSO2CI) and derivatives thereof. In a similar manner, the -NH2 groups can be capped by reaction with active esters of carbonates of the general formual RO-C(O) L, where L is des- ribed as above. D->E. Reduction In a preferred embodiment of the invention, the C=N bond linking the sugar to the linker (for example compound D of fig. 1) is reduced using a reducing agent. The C=N bond may be reduced by a variety of well known reducing agents, preferably the reducing agent is capable of saturating the double bond while placing a hydro- gen atom on the N. Of special value are boranes or borohydrides comprising a BH bond, examples in- clude NaBH4, NaCNBH3, and BH3 complexes such as BH3-pyridine, BH3- dimethylsulfide or the like. Silanes with the structures R3SiH can also be used, such as silanes comprising SiH bonds, as can hydrogen transfer agents such as diimides, or homogeneous hydrogenation catalysts or hydrogenation catalysts comprising a metal-H bond. The reduction results in a reactive sugar containing the structure SugarCH-NH- preferably linked to a solid support via a linker and optionally a spacer. In general, if the reducing sugar was an aidehyde, then reduction will result in a compound of the structure SugarCH2-NH-. If the reducing sugar was a ketone, then the reduction will result in a compound of the structure SugarCH-NH-. The products of the reduction are for example of the general structure E (fig. 1) con- taining a formally SP3 hybridized N atom. C-»Cred—>E In another preferred implementation of the method, the order of the capping and reduction steps is reversed. Reduction of the C=N bond in compound C (fig. 1) can be effected by any of the reagents described in D=E above to produce a compound of the structure Cred (fig. 1). The reduction may also be performed in situ, meaning that a reducing agent (such as NaCNBH3) may be added to the solid support (e.g. compound B) simultaneously with the reducing sugar so that the C=N bond is re- duced as it forms producing also Cred. It is thus comprised within the present inven- tion that the sample comprising the reducing sugar may be incubated with the solid support and the reducing agent simultaneously. Thus, reduction of C=N bonds (step v) will be performed immediately following reaction of the reducing sugar with the NH2 group of the solid support (step iii). The free -NH2 groups in Cred may then be capped using any of the reagents described in C->D above under conditions that do not cause reaction with the SugarCH-NH-moiety. In particular, in this embodiment of the invention it is preferred that the capping agent preferentially reacts with primary amino groups over secondary amino group. It is also preferred that reaction tem- perature and time are adjusted to yleld preferential reaction with primary over sec- ondary amino groups. Virtually all compounds that react with amino groups react more qulckly with primary amino groups than with more substituted amino groups, but this is especially the case when such compounds are sterically large, such as for example active benzoyl esters, isopropanoic acid active-esters, pivaloyl active- esters, Boc anhydride or Boc-azide and the like. Useful compounds and conditions for preferential reaction with primary amino groups over secondary amino groups are described in Greene et al. 1999, Protective Groups in Organic Synthesis, 3rd. Ed., Chaper 7, pp. 503-653. Other very preferred capping agents are NHS-esters or sterically hindered pentafluorophenyl (PFP) esters or tetrafluorophenyl (TFP) es- ters. E->F. Adding TAGs Compound E, fig. 1, obtained by elther of the above routes, contains solids linked to a capped nitrogen atom (N(H)CAP) of very low reactivity towards electrophiles and a formally SP3-hybridized nitrogen atom in the sequence SugarCH2-NH-R. Reaction of E with sultable nitrogen-reactive functional groups (preferably the nitrogen-reactive functional group is a mild electrophile) therefore results in the exclusive, or near ex- clusive, addition of the electrophile to the SP3 nitrogen atom effectively adding a molecular structure, herein described as "TAG", or another derivatising agent onto the nitrogen to which the sugar is attached. The product of the addition of a TAG is shown as Fin fig. 1. Throughout the description the term "nitrogen-reactive group" is used to describe reactivity towards a formally SP3-hybridized nitrogen, such as in compounds of the structure R-NH-R', for example amines, wherein R and R' independently are alkyl, or aryl (optionally substituted) or compounds wherein R' has an heteroatom such as O or N attached to the -NH- such as in hydroxylamine derivatives (R-NH-OR') or hydrazine derivatives (R-NH-NH-R'). The identity of the derivatising agent (for example a TAG), i.e. the specific chemical structure of the derivatising agent, may be selected by the user. For addition to the SP3 nitrogen in E, the derivatising agent (for example the TAG) should itself com- prise an nitrogen-reactive functional group designated "X" in fig. 1„ Preferably the TAG should contain an electrophile, or be attached to an nitrogen-reactive functional group X. Preferably the derivatising agent is of the general structure TAG-X (see fig. 1), wherein X is a nitrogen-reactive functional group. Preferably X is any mild elec- trophile that is reactive with SP3 nitrogen atoms, but preferably mild electrophiles that react poorly with the -OH groups present on the sugar. Such mild electrophiles include isothiocyanates (TAG-NCS), active esters (TAG-C(O)-L) where L is a leav- ing group commonly used in amide bond formation such as in the synthesis of pep- tide bonds, carboxylic acids (TAG-COOH) which can be activated to active esters in situ by methods commonly used in amide bond formation such as in the synthesis of peptide bonds, alkylating agents (TAG-L) where L is a leaving group preferably but not exclusively from the series CI, Br, I, OS(O)2R where R can be alkyl or aryl, TAGs comprising Michael acceptors (typically containing the sequence -CR=CH-C(O)-) or alpha-beta unsaturated sulfones (-CR=CH-S(O)2-) and derivatives of any of the aformentionned, aidehydes or ketone that may react with the sugarCH2-NH-amino group by reductive amination, or substituted haloaromatic groups where the aro- matic ring bears electronegative groups such as nitro groups, for example as in the Sanger reagent 1-fluoro-2,4-dinitrobenzene or the 4-halo-7-nitro-2-oxa-1,3-diazole (NBD) reagents where the halogenis preferably F or CI. The TAG may for example be a fluorescent moiety, a mass spectrometry TAG, a first binding partner capable of binding to a second binding partner, a nuclelc acid wherein any of the aforementioned TAGs preferably comprises or are attached to an nitrogen-reactive functional group. In particular the TAG may be any of the TAGs described in more detall herein below, wherein any of these TAGs may be attached to any of the aforementioned nitrogen-reactive functional groups. An example of a compound which may be obiained by adding a TAG to compound E is shown as F in fig. 1. F. Washing In one embodiment the tagged sugar (e.g. compound F, fig. 1) is washed prior to any futher manipulations. Thus any amount of unbound TAG is removed. Washing may easily be accomplished because the tagged sugar is immobilised on a solid support. After washing, only covalent bound TAG will be present. Thus the amount of TAG will be correlatable to the amount of immobilised sugar. Accordingly, by determining the presence of TAG, the amount of immobilised sugar may be determined. If esset- tially all reducing sugar in a glven sample was immobilised, the methods therefore in one aspect allow determining the amount of reducing sugar present in a sample. The skilled person will readily be able to identify sultable washing conditions for a glven tagged, immoblised sugar (e.g. compound F, fig. 1). The washing may for ex- ample be done with a solvent selected from the group consisting of water, aqueous buffer, organic solvents and mixed aqueous and organic solvents. The solvent may also be any of the aforementioned comprising one or more additives such as salts, divalent metal cations, detergents, complexing agents including inclusion- conmplex-forming molecules such as cyclodextrins or calixarenes, chelating agents (for example EDTA), borates, boronates or silicates. Furthermore, the solvent may optionally comprise detergents and denaturing agents. The washing my be per- formed at any temperature, but preferably at temperatures in the range of 0 - 100°C. H. Cleavage of cleavable linker When the linker used is a cleavable linker, then methods of the invention may com- prise a step of cleaving said cleavable linker thereby releasing captured sugar. Pref- erably the cleavage is performed subsequent to addition of a derivatising agent, such as a TAG (added using TAG-X) or a tether-Y (added using X-tether-Y) to the - NH- group of the immobilised sugar. Thus a tagged sugar (compound G or com- pound J in fig. 1) may be released into solution from F or from I, respectively. G consists of a sugar portion that bears a TAG on the Nitrogen atom which is attached to the residue (if any) of the linker that remains after cleavage, and for simpliclty is denoted as sugar-TAG. J consists of a sugar portion that bears a tether on the ni- trogen atom, which is attached to the residue (if any) that remains after cleavage. The tether may optionally be linked to a TAG. However, the cleavable linker may be cleaved at any desirable time within the method. If the TAG added to compound E has beneficlal spectroscopic properties such as fluorescent properties, the amount of sugar-TAG (compound G, fig. 1) can be quan- titiated in solution. Furthermore, the sugar-TAG (compound G, fig. 1) can be sub- jected to analytical separation techniques such as HPLC or CE, and if more than one sugar is present, the individual components can be separated, thelr relative ratios determined, and they can be identified if authentic standards are available, and they can be quantitated. They can also be used as ligands that may bind to car- bohydrate-recognizing proteins, thus providing information on the structure of elther the carbohydrate or the protein. If the TAG is a structure glving the sugar-TAG properties that are beneficlal to the practice of mass-spectrometry, elther due to increased sensitivity, simplification of spectral interpretation, or permitting the performance of differential analysis using isotope encoding, then the sugar-TAG released into solution can be favourably ana- lyzed by mass-spectrometry. F. TAGs with spectroscopic properties In one preferred embodiment of the invention the TAG added to e.g. compound E or compound H has beneficlal spectroscopic properties. Preferably, the TAG with the beneficlal spectroscopic properties is added to e.g. compound E using a derivative of the structure X-TAG, wherein X is a nitrogen reactive functional group, such as any of the nitrogen reactive functional groups described herein above in the section "E->F Adding TAGs". By beneficial spectroscopic properties is meant that the TAG can easily be visualised, for example by spectrometry. Thus the TAG may for exam- ple be spectroscopically detectable. In a preferred embodiment the TAG is a fluo- rescent TAG. Examples of such tagglng include the reaction with isothiocyanates (e.g. FITC, TRITC), active esters, Michael acceptors, alpha-beta-unsaturated sul- fonyls (speclfically vinyl sulfones) and alkylating agents such as alkyl halides and tosylates, an halo-aryl compounds such as for example the Sanger reagent The product of addition of such a TAG (for example compound F of fig. 1) can ab- sorb and re-emit light that can be detected. The number of such TAGs present on F will reflect the number of sugar molecules A added to B and captured to produce C. The number of reducing sugar molecules (A) origlnally present in a sample can therefore be estimated by the fluorescence of compound F, provided that the pro- vided solid supports (compound B) comprise an excess of capture groups. TAGs other than fluorescent molecules can also be used. These can include radioactive TAGs, phosphorescent TAGs, chemiluminescent TAGs, UV-absorbing TAGs, nanoparticles, quantum dots, coloured compounds,, electrochemically-active TAGs, infrared-active TAGs, TAGs active in Raman spectroscopy or Raman scattering, TAGs detectable by atomic force microscopy or TAGs comprising metal atoms or clusters thereof. If the solid support of compound F is a sensor, such as a surface acoustic wave sensor or a surface plasmon resonance sensor, then addition of such a specles that binds speclfically to the TAG can result in the production of a signal that is propor- tional to the TAG and therefore to the number of sugar molecules. An example is when the TAG is a biotin residue, commonly introduced by reaction with an active ester of biotin. Addition of an avidin-protein to compound E, when the TAG is a bio- tin residue, can result in signal that is readily detected and reported by the sensor. Other examples of sensors that can be used to detect the binding of second binding partners to immobilized TAGs include but are not limited to piezoelectric sensors, amperometric sensors, surface plasmon fluorescence spectroscopy sensors, dual polarization interferometry (DPI) sensors, wavelength-interrogated optical sensors (WIOSs), impedence sensors, optical wavegulde grating coupler sensors, acoustic sensors and calorimetric sensors. Once the sugar has been attached to a TAG with spectroscopic properties, then said spectroscopic properties may be determined. The optical properties may be determined for sugars still immobilised on the solid support (such as for compound F or I of fig. 1) or for sugars released to solution (for example for compound G or J of fig. 1). The latter requlres that the linker is a cleavable linker. Depending on the na- ture of the TAG with spectroscopic properties, said properties may be determined using conventional methods, such as spectrometry. Thus the methods of the inven- tion may comprise the step of detecting the TAG attached to the sugar by spec- trometry. F. Mass-spectrometry TAGs In one embodiment of the invention, the TAG is a mass spectrometry TAG. Said mass spectrometry TAG is preferably added by a reagent of structure X-TAG, wherein X is a nitrogen-reactive functional group, such as any of the nitrogen- reactive functional group mentioned herein above in the section "Adding TAGs". The term "mass spectrometry TAGs" as used herein refers to molecules that improve the detection and structural characterization of the products by mass spectrometry, pref- erably after cleavage from the solid support (as described herein above in the sec- tion "Cleavage of cleavable linker"). Examples include the introduction of a bromine label which imparts a characteristic isotope pattern in the mass-spectrum. Such a bromine label may be added, for example, by addition of p-bromophenyl isothiocy- anate to compound E producing a compound of structure F where the TAG contains a bromine atom. The usefulness of bromine-containing labels in the mass- spectrometry of carbohydrates has been described for example in Li et al., 2003, Rapid. Commun. Mass Spectr., 17:1462-1466.. Another example includes introduc- tion of molecules that impart elther positive charges or negative charges for en- hanced detection in elther positive-ion mode or negative-ion mode of mass/charge separation. Another example includes the introduction of molecules that improve performance or sensitivity in electrospray, MaidI or other techniques of ionization common in the practice of mass spectrometry. Yet another example includes the introduction of stable isotope-labeled molecules that allow quantitation of the la- belled specles by mass-spectrometry. Useful methods for isotope labelling are for example reviewed in Tao et al., 2003, Current Opinion in Biotechnology, 14: 110- 118. Once the sugar has been attached to a mass spectrometry TAG, then the tagged sugar (F or G or I or J, fig. 1) may be detected by mass spectrometry. Mass spec- trometry may be performed on sugars still immobilised on the solid support (such as for compounds F and I of fig. 1), but preferably is performed on sugars released to solution, for example by cleavage of a cleavable linker (for example for compounds G or J of fig. 1). It is thus preferred that the linker is a cleavable linker. The skilled person will be able to perform a sultable mass spectrometry depending on the na- ture of the mass spectrometry TAG . Thus the methods of the invention may com- prise the step of detecting the sugar attached to the mass spectrometry TAG by mass spectrometry, F. Binding partner TAGs In another preferred embodiment of the present invention the TAG is a first binding partner, capable of speclfic interaction with a second binding partner, wherein said first binding partner is added to for example compound E (or to compound H) through the reaction with a reagent of structure X-TAG, wherein X is a nitrogen- reactive functional group (e.g. a "derivatising agent"). The second binding partner is preferably labelled with a detectable label, such as a dye, a fluorescent label, a ra- dioactive isotope, a heavy metal or an enzyme. The first binding partner may for example be a molecule that is a ligand for a protein useful in the detection of the resulting immobilized ligand, elther stochiometrically or following amplification. The first binding partner may also be a protein and the second binding partner a ligand for said protein. Examples of binding partners include (igand-protein palrs in common use in ELISA assays. For example compound E may be reacted with a biotinylation reagent, and after washing, detecting the now immobilized biotin with streptavidin (or other avid- ins) that is directly labelled with a detectable label, such as with a fluorescent TAG, a radioactive isotope or a heavy metal, or with streptavidin (or other avidins) that is conjugated to an enzyme such as horseradish peroxidase that can catalyze a chemical reaction that results in the production of a signal that can be detected by spectrometry. Other examples of binding partners are antibody-epitope palrs. Thus the one binding partner could comprise an epitope and the other binding partner could be an anti- body capable of binding said epitope with high affinity, preferably an antibody spe- clfically binding said epitope. F. Nuclelc acld TAGs In another embodiment of the invention the TAG is a nuclelc acld. Nuclelc aclds ac- cording to the invention may be any nuclelc acld, such as DNA or RNA, or ana- logues thereof such as LNA, PNA, HNA or the like. Preferably the nuclelc acld is DNA, preferably a DNA oligomer. Preferably, said DNA is derivatised with an nitro- gen-reactive functional group, such as any of the nitrogen-reactive functional groups mentioned herein above in the section "Adding TAGs". It is preferred that the se- quence of said nuclelc acld TAG is known or at least partially known, which will en- able the skilled person to readily detect said TAG using standard methods. The nuclelc acld TAG may be any desirable length, preferably at least a length which will allow speclfic detection. Thus preferably the nuclelc acld is at least 6 nu- cleotides, more prefereably at least 10 nucleotides, for example in the range of 10 to 5000 nucleotides long. After addition of a nitrogen-reactive nuclelc acld TAG to the sugar, then the nuclelc acld, such as the DNA oligomers can then be detected directly on the solid support by hydridisation to thelr complementary nuclelc aclds or essentially complementary nuclelc acld. By essentially complementary nuclelc aclds, is meant a nuclelc acld, which may hybridise to a glven nuclelc acld under stringent conditions as for exam- ple described in Sambrook et al., 1989, in "Molecular Cloning/A Laboratory Manual", Cold Spring Harbor. Preferably, said complementary nuclelc aclds may be attached to a detectable label. Said detectable label may for example be a flourescent label or a radioisotope or an enzyme, preferably a fluorescent label. Thus, the nuclelc acld TAG may for example be detected by hybridisation to thelr complementarty fluorescently-labeled DNA. Alternatively, a nuclelc acld TAG may be amplified using conventional methods known in the art, such as Polymerase Chain Reaction (PCR) or ligase chain reactin. Thus, the immobilised nuclelc acld TAG may be subjected to PCR reactions to amplify the immobilized DNA oligomer which can be measured in solution by a variety of well know techniques for quantification in PCR. This process has particular value in the indirect detection and quantification of very low amounts of SugarCH-NH-Linker-Spacer-Solid present on the solid support. Alternatively, the Sugar bound to DNA may be released to solution by cleavage of the linker and thereafter amplified in solution by for example PCR or detected in solution by virtue of speclfic hybridisation to essentially complementary nuclelc aclds. E->H Tethers The derivatising agent according to the present invention may also be a tether cou- pled to at least two functional groups. Such bifunctional reagents will in general be of the structure X-tether-Y or X-tether-Yp, wherein X is an nitrogen-reactive func- tional group and Y is a second reactive functional group and Yp is a latent reactive functional group or a protected reactive group Y. The product of the reaction of compound E with X-tether-Y (or X-tether-Yp) may for example have the general structure of compound H of fig. 1. The second reactive functional group Y may be reactive to any of the types of reagents in use in solid-phase synthesis. For exam- ple, the N in SugarCH-NH-Linker-Spacer-Solid can be reacted with bifunctional reagents (X-tether-Y) where one function reacts by making a bond to the immobi- lized nitrogen (the nitrogen reactive functional group X) and the other function can elther be, or can be converted to (by for example unmasking, deprotection or further reaction) a second reactive functional group Y. The tether may be any useful tether, for example alkyl, alkenyl or alkynyl (which may be linear, branched or cyclic), aryl or any of the aforementioned comprising amide bonds (NC(O)R) or etyleneglycol groups (-CH2CH2-O-) or substituted with heteroa- toms and thelr derivatives. The second functional reactive group Y may for example be selected from the group consisting of thiols, carboxyl groups, activated carboxyl groups, disulfides, activated disulfides, alkylating agents, alkenes, alkynes, aidehydes, ketones and azides. The alkylating agent may for example be an alkyl halide or an alpha-halo carbonyl group. Yp may for example be protected amines or protected derivatives of any of the aforementioned groups Y. Thus Yp may for example be selected from the group con- sisting of protected amines, protected thiols, protected carboxyl groups, protected aidehydes and protected ketones. Protected reactive groups are herein denoted Yp, wherein Yp may be deprotected to yleld a functional reactive group Y. Useful pro- tecting groups can be found in Greene et al., 1999, "Protective Groups in Organic Synthesis", 3rd. Ed., John Wiley and Sons, New York, speclfically for carbonyl groups (chapter 4, pp. 293 - 368 ), for carboxyl groups (chapter 5, pp. 369 453-), for thiols (chapter 6, pp. 454 - 493) and for amino groups (chapter 7, pp. 494 - 653). Examples of protected amines include, but are not limited to, those in common use in solid-phase peptide synthesis, such as Fmoc, Boc, Alloc, p- ntirobenzyloxycarbonyl, trityl and substituted trityl, o-nitrobenzyloxycarbonyl, N- sulfenyl or azido. However, the second reactive functional group may be any func- tional groups Y, or protected functional groups (Yp) that have been made to react on the solid phase, such as examples well known in the art of solid phase synthesis and the coupling of small molecules to solid supports and surfaces. These function- alized groups can then directly, or after deprotection to reactive specles, capture a second derivatising agent comprising a functional group (Z) capable of reacting with the second functional group Y. If Y in compound H contains an NH2 group, or on deprotection can be made to con- tain an NH2 group, then any of the amine reactive reagents described in E-goes-to-F (for example, isothiocyanates) can be used to add a TAG to produce compounds of the general structure I (fig. 1). The second derivatising agent made to react with any of the functional groups Y in compound H (fig. 1) may for example be spectroscopic TAGs or any of the TAGs mentioned above in section E->F, wherein said TAGs in stead of a nitrogen reactive group, comprises or are derivatised with a functional group (Z) capable of reacting with Y. They may also be small molecules like drugs, imaglng agents, peptides, pro- teins, enzymes and other molecules exhibiting biologlcal activities, nuclelc aclds such as DNA or RNA Said small molecules, imaglng agents, peptides or nuclelc aclds preferably com- prises or are attached to a functional group Z, capable of reacting with the glven second functional reactive group Y. The skilled person will readibly be able to iden- tify useful functional groups Y and Z. The second derivatising agent may also be any of the above-mentioned TAGs described above in the sections "TAGs with Spectro- scopic properties", "Mass spectrometry TAGs", "Binding partner TAGs" and "Nuclelc acld TAGs", wherein said TAGs in place of a nitrogen reactive functional group con- tains a functional group Z capable of reacting with the functional group Y. The func- tional group attached to the tether in H (fig. 1) may also be a latent or protected group (Yp) that can be converted by chemical or enzymatic reaction into Y which may then react further as described above. If this latent group can be converted to a primary or secondary amine (i.e. Y will comprise the structure -NH2 or -NH-), then any of the amine-reactive specles described in E-*F above may be added to pro- duce tagged compounds of the structure I. The methods of the invention may therefore comprise the step of vii. Reacting the -NH- group of the reactive sugar with a bifunctional reagent of the structure X-tether-Y or X-tether-Yp, wherein X is a nitro- gen-reactive functional group and Y is a second reactive functional group and Yp is a latent functional group that can be converted to or deprotected to a reactive functional group Y, thereby obtaining a sugar covalently attached to said tether-Y or said tether-Yp. This step is preferably performed using compound E of fig. 1 as starting material. Thus this step may for example generate a compound of the general structure H of fig. 1. In embodiments of the invention wherein the bifunctional reagent is of the structure X-tether-Yp, then preferably, the method furthermore comprises the step of convert- ing or deprotecting Yp to obtain a reactive functional group Y. This step may be per- formed before or after reacting X with -NH-, preferably it is performed subsequent to reacting X with -NH-. In addition the methods of the invention may furthermore comprise the steps of viii. providing a second derivatising agent comprising a functional group (Z) capable of reacting with Y ix. reacting the functional groups Z and Y, thereby covalently attaching the second derivatising agent to the sugar via a tether and the first de- rivatising agent. Alternatively, the methods of the invention may further comprise the step of: viii. providing a particle selected from the group consisting of eu- karyotic cells, prokaryotic cells, microbial organisms, micelles, phages, vira and nanoparticles, wherein the particle comprises a functional group (Z) capable of reacting with Y. ix. reacting the functional groups Z and Y, thereby covalently attaching the particle to the sugar via the tether and and the agent. Step ix. may thus generate a compound of the general structure I outlined in fig. 1 where the TAG is a particle. Provided that the linker is a cleavable linker, the meth- ods may further comprise the step of cleaving the linker thereby for example gener- ating a compound of the general structure J of fig. 1. The product of the reaction of SugarCH-NH-Linker-Spacer-Solid (e.g. compound E of fig. 1) with Afunctional reagents X-tether-Y for example has the general structure H and may contain, or can be made to contain, further reactive groups that can form covalent bonds to assemblies larger than molecules: for example bacteria, phage, yeast, micelles, viruses, nanoparticles or eukaryotic or prokaryotic cells. Cleavage of the linker then results in specles of the general formula SugarCH- N(assembly)-Linker, effectively adding the sugar to the assembly. Thus, the sugar can in princlple be transferred from a solid support to an assembly. Enzyme treatment If the solid support is biocompatible, i.e. permits contact with biologlcal macromoie- cules like enzymes without significantly altering thelr activities, then the immobilised sugar molecule can be acted on by enzymes that will alter its structure. The immobi- lised sugar molecule may for example be a compound of any of the general struc- tures C, Cred, D, E, F, H or I of fig. 1. Non-limiting examples of biocompatible solid supports includes glass, PEGA, SPOCC or polysaccharide gels. Within this embodiment it is preferred that the linker is relatively long, and thus it is preferred that the linker comprises at least 2 atoms, preferably at least 6 atoms, more preferably the linker comprises a chain of at least 6 atoms, for example the longest chain of atoms within the linker is at least 6 atoms long, such as in the range of 6 to 1000 atoms long. It is also preferred that the linker is hydrophilic. It is also possible to contact the sugars liberated into solution by cleavage of a cleavable linker, such as the compounds G or J of fig. 1 with biologlcal macromole- cules, such as enzymes. The enzymes can belong to any class that can act on carbohydrates, for example glycosidases, glycosyltransferases, and enzymes that modify the alcohol groups by acylation, phosphorylation, sulfation or oxidation. Alternatively, if the sugars are al- ready substituted on -OH groups, such as acylated, phosphorylated or sulphated, then deacylases, phosphatases and sulfatases can alter thelr structures. Thus the methods of the invention may furthermore comprise the step of contacting the sugar (for example any of the compounds C, Cred, D, E, F, G, H, I or J of fig. 1) with one or more enzymes selected from the classes of glycosyltransferases, sulfatases, pho- phorylases, sulfotransferases, phosphotransferases, glycosynthases and transgly- cosidases, thereby converting said sugar into a new structure. In a preferred em- bodiment the methods furthermore comprise the step of contacting the sugar (for example any of the compounds C, Cred, D, E, F, G, H, I or J of fig. 1) with one or more glycosidases, thereby generating a new reducing sugar, provided that the first sugar is a substrate for said glycosidase(s). An example would include the incubation of uncapped Sugar-C=N-Linker-Spacer- Solid (for example, compounds C of fig. 1), which still contains free -NH2 groups, with an exoglycosidase causing the decrease in the length of the sugar by one monosaccharide residue. The cleavage of this monosaccharide residue leaves an oligosaccharide attached to the solid support that is one sugar unit shorter, and pro- duces a reducing sugar which can be captured by the same or a different solid sup- port, such as a solid support of the general structure B in fig 1, which can subse- quently be submitted to any of the manipulations described above in B to J. Thus the methods of the invention may furthermore comprise the steps of a) providing one or more enzymes that can act on carbohydrates b) contacting the sugar with said one or more enzymes These steps may be performed at any glven time during the method. The enzymes may be any of the enzymes described in the present section. In a particular embodiment the enzyme is a glycosidase and the method described herein above in the summary section comprises the further steps of: iii.a) providing one or more glycosidases that can act on carbohydrates iii.b) contacting the sugar with said one or more glycosidases, thereby generating a new reducing sugar, provided that the first sugar is a substrate for said glycosi- dase(s). iii.c) immobilising newly generated reducing sugar(s) on a solid support. The steps iii.a-iii.c may be carried out following step iii. of the method outlined in the section "Summary of the invention" herein above. However, the steps iii.a to iii.c may also be carried out following any of steps iv, v, vi or vii of said method. Accord- ingly, steps iii.a-iii.c may be carried out on any of the immobilized sugars exemplified by structures C, Cred- D, E, F, H or I of fig. 1. In particular, said newly generated reducing sugars may be immobilised to free - NH2 groups of the same solid support or on another solid support. Said other solid support may for example elther be unsubstituted or carry an immobilised reference standard. It is preferred that said other solid support is a solid support as described herein above, and that the solid support is attached to a linker (optionally via a spacer), wherein said linker comprises a capture group (see detalled description of linkers, capture groups and spacers herein above). Of particular value is the reduction and fluorescence labeling of the glycosidase product and the released monosaccharide on the same or a different solid support, for purposes of obtaining structural information. A speclfic example includes the cap- ture of Gal-GlcNAc-Gal-glc (lacto-N-tetraose, LNT) on NH2-Linker-Spacer-Solid of structure B (fig 1), incubation of the captured and immobilized LNT (an example of a compound of structure C of fig. 1) with beta-galactosidase followed by capture of the released galactose on the same solid support (C) to yleld a mixture of unreacted Gal-GlcNAc~Gal-GlcC=N-Linker-Spacer-Solid, and the products of the reaction which are GlcNAc-Gal-GlcC=N-Linker-Spacer-Solid and Gal- C=N-Linker-Spacer- Solid. Capping, reduction, fluorescence tagglng with TRITC and cleavage form the solid as described in step F—>G above then allows confirmation that the immobilized LNT had a terminal beta-galactose residue, by co-migration of the trisaccharide and monosaccharide products with known standards. Many useful glycosidases are described in the art, for example any of the glycosi- dases described in US5,100,778 or W092/19974 may be employed with the present invention. If the solid support is biocompatible, then the unreacted -NH2 groups in Sugar-C=N- Linker-Spacer-Solid (e.g. compound C, fig 1) can be capped (for example with ace- tic anhydride as described in C->D above) and then exposed to carbohydrate-active enzymes, or further reduced to SugarCH-NH-Linker-Spacer-Solid (as described in section D—>E above) and then exposed to carbohydrate-active enzymes. Alterna- tively, compound C of fig. 1 can be reduced to Cred and then exposed to carbohy- drate active enzymes. The SugarCH-NH-Linker-Spacer-Solid (e.g. compound E, fig 1) can be further tagged (as described in sections E-»F herein above) to yleld Sug- arCH-N(TAG)-Linker-Spacer-Solid (e.g. compound F, fig 1), and then exposed to carbohydrate-active enzymes. In any of these processes, the product of the enzyme reaction that remains attached to the solid support can be further manipulated ac- cording to the methods of the invention or cleaved by reaction at the linker, for fur- ther analysis. Any product of the enzyme reaction that results in cleavage of frag- ments of the immobilized sugar will appear in solution, where it may be further in- vestigated using established techniques of analytical chemistry or, in the case where it is itself a reducing sugar, may be subjected to the manipulations described for the generic sugar A in Fig 1. The individual sugars may be detected by capillary gas chromatography (GC), mi- crocolumn supercritical fluld chromatography (SFC), microcolumn liquld chromatog- raphy (LC), high performance liquld chromatography (HPLC), high performance cap- illary electrophoresis (HPCE), ion-exchange chromatography or mass-spectrometry. Detection of individual sugars may be done before or after labelling with a derivatis- ing agent, and elther in solution or on the solid phase. Detection agents In one embodiment of the invention, the method comprises the steps of viii. contacting the sugar with a detection agent capable of assoclating with said sugar ix. detecting the detection agent Preferably, said sugar is immobilised on a solid support as described herein above, and thus for example a compound of the general structure C, Cred, D, E, F, H or I of fig. 1 may be contacted with said detection agent. It is also possible that said sugar has been released from the solid support by cleavage of a cleavable linker, as thus a compound of the general structure G or J may also be contacted with said detec- tion agent. The detection agent may be any agent capable of assoclating with said sugar. Pre- ferred detection agents are compounds capable of assoclating with sugars with much higher affinity than with any other compounds, such as compounds having at least a 2-fold, such as at least a 5-fold higher affinity for sugars, than for any other compound. In addition it is preferred that said detection agent is directly or indirectly detectable by a method known to the skilled person. For example the detection agent may itself be for example a fluorescent or coloured compound, The detection agent may also be a compound for which easy detection methods are avallable. In one embodiment of the invention the detection agent comprises an aryl boronate or heteroaryl boronate where the aryl moiety is substituted with a spectroscopically active group such as a fluorescent TAG or any of the other detectable TAGs de- scribed herein above in the section "F. TAGs with spectroscopic properties". In another embodiment the detection agent is a polypeptide, preferably a polypep- tide selected from the group consisting of lectins, selectins and other carbohydrate binding proteins, toxins, receptors, antibodies and enzymes. When the detection agent is a polypeptide, said polypeptide may be coupled to a detectable label, such as an enzyme or a fluorescent compound. The polypeptide may also be detected by the aid of antibodies or similar high affinity compounds. Examples The following are illustrative examples of the methods of the invention and should not be considered as limiting for the invention. Unless otherwise clear from the con- text, capital letters A, B, C, Cred, D, E, F, G, H, I and J refers to the general struc- tures outlined in fig. 1. Experimental 1. Examples of A: Reducing sugars used in the present work The structures of the reducing sugars captured by solid supports B are shown in Fig. 2. These included the monosaccharides D-glc (1) and D-Gal (2), the disaccha- ride N-acetyllactosamine (LacNAc, 3), the trisaccharide maltotriose (maltotriose G3, 4) and the tetrasaccharide lacto-N-tetraose (LNT, 5). Samples 6 and 7 contained mixtures of the monosaccharides Fuc:Man:GainAc in ratios of 2:3:1 and 1:3:2, re- spectively. Sample 8 contained a 1:1 mixture of Gal (2) and LNT (5). Sample 9 con- tained an approximately equlmolar mixture of maltobiose (G2), maltotriose (G3), maltotetraose (G4), maltopentaose (G5), maltohexaose (G6) and maltoheptaose (G7). Sample 10 consisted of the N-linked oligosaccharide chains released from ribonuclease B (Sigma) by the action of PNGase F (product number 1365177, Boe- hringer Mannhelm GmbH, Germany). 2. Linkers, spacers and tagged-sugar reference standards 2.1 Linker and spacer The synthesis of the cleavable linker and the structure of the spacer are shown in Fig. 3 and described below. 12: N-Fmoc-4-aminooxymethyl-benzoic acld To a solution of 4-aminooxymethyl-benzoic acld, hydrochloride 111 (2.0 g, 0.010 mol) in dioxane (20 mL) and half saturated Na2CO3 solution (20 mL) was added Fmoc-cl (2.8 g, 0.011 mol) and the mixture was stirred for 2 h. Ethyl acetate (100 mL) was added and the pH of the aqueous phase was adjusted to 1-3 by careful addition of Hcl(oonc.). The mixture was poured in to a separating funnel and the or- ganic phase was isolated, washed once with water (100 mL), dried over Na2SO4 and the solvent was removed on a rotavap to glve an oil that solidified upon standing. The crude product was purified by flash column chromatography (petroleum ether, ethyl acetate, AcOH 60:40:1). yleld: 3.5 g (92%) 1H-NMR (250 MHz, DMSO-d6) 5 = 4.05 (1H, t, J= 6.3 Hz), 4.27 (2H, d, J = 6.3 Hz), 4.51 (2H, s), 7.08-7.22 (6H, m), 7.46 (2H, d, J = 7.4 Hz), 7.66 (2H, d, J = 7.1 Hz), 7.72 (2H, d, J = 8.4 Hz), 10.29 (1H, br. s), 12.78 (1H, br. s). 13C-NMR (63 MHz, DMSO-d6) δ = 47.04, 66.03, 76.91, 120.51, 125.41, 127.45, 128.03, 128.89, 129.33, 129.63, 130.82, 141.19, 144.01, 157.12, 167.48. MS (ES) m/z = 389 (MH+). 13: Reaction of N-Fmoc-4-aminooxymethyl-benzoic acld (12) with t-butyl bro- moacetate N-Fmoc-4-aminooxymehtyl-benzoic acld (12) (1.0 g, 2.57 mmol) was dissolved in DMF (15 mL) and Cs2CO3 (0.42 g, 1.28 mmol, aidrich) was added followed by stir- ring for 5 min at rt. tert-Butyl bromoacetate (0.55 g, 2.28 mmol, Fluka) was added and the mixture was heated to 50°C for 30 min and then cooled to rt again. CH2Cl2 (70 mL) was added and the mixture as poured in to a separating funnel and washed with half saturated NaHCO3 solution (3 x 50 mL) and then water (2 x 50 mL), dried over MgSO4.The solvent was removed under reduced pressure to glve the crude product as an oil. After flash column chromatography (20-40% ethyl acetate in petro- leum ether) a white solid was obtained in a yleld of 1.15 g (89%). 1H-NMR (250 MHz, CDcl3) 5= 1.37 (9H, s), 4.06 (1H, t, J = 6.7 Hz), 4.37 (2H, d, J = 6.7 Hz), 4.61 1The material was prepared as previously described: Deles,J. et al.; PJCHDQ; Pol. J. Chem.; EN; 53; 1979; 1025-1032 (2H, s), 4.67 (2H, S), 7.11-7.18 (2H, m), 7.22-7.27 (4H, m), 7.43 (2H, d, J= 7.5 Hz), 7.60 (2H, d, J = 7.3 Hz), 7.75 (1H, s), 7.93 (2H, dd, J = 1.7 Hz, 6.6 Hz). 13C-NMR (63 MHz, CDcl3) δ = 26.31, 45.28, 59.95, 65.52, 75.99, 80.84, 118.30, 123.27, 125.41, 126,10, 126.93, 127.23, 128.30, 139.29, 139.58, 141.73, 155.70, 163.94, 165.15. MS (ES) m/z = 542 (MK+). 14: Preparation of linker The white solid 13 (1.15 g) obtained in the previous experiment was stirred in a 50% solution of CF3CO2H in CH2Cl2 (30 ml) for 3 h and evaporated to dryness. The oily residue was taken up in a small amount of ethyl acetate and the product was pre- clpitated as a fine white powder by slow addition of hexanes to the solution. The product was filtered and washed a couple of times with hexanes and dried under vacuum to glve the desired product in an almost quantitative yleld (1.0 g, 98%). 1H- NMR (250 MHz, DMSO-d6) 5 = 4.07 (1H, t, J = 6,3 Hz), 4.28 (2H, d, J = 6,3 Hz), 4.53 (2H, s), 4.62 (2H, S), 7.07-7.14 (2H, m), 7.17-7.26 (4H, m), 7.46 (2H, d, J = 7.4 Hz), 7.66 (2H, d, J = 7.2 Hz), 7.77 (2H, d, J= 8.3 Hz), 10.30 (1H, br. s). 13C-NMR (63 MHz, DMSO-d6) δ = 47.04, 61.62, 66.04, 76.79, 120.50, 125.41, 127.46, 128.03, 129.05, 129.69, 141.19, 142.20, 144.00, 157.12, 165.50, 169.47. MS (ES) m/z = 446 (M-H+). HRMS (ES) calculated (C25H21NO7Na+): 470.1210 found: 470.1224. 2.2 Synthesis of tetramethylrhodamine (TMR)-tagged monosaccharide stan- dards of the general structure G. The 8 monosaccharides D-glc, D-Gal, D-Man, D-Xyl, D-GlcNAc, D-GainAc, L-Fuc and D-glcA were used. The general synthetic scheme is shown in Fig. 4 for D-Gal (2), and the structure of the product 21 is shown in Fig. 4 and is abbreviated GalCH2-N(R)-TMR as shown. The structures of all elght SugarCH2-N(R)-TMR monosaccharide derivatives prepared are shown in Fig. 5. 16: Reaction of N-Fmoc-4-aminooxymethyl-benzoic acld (12) with benzylbromide N-Fmoc-4-aminooxymethyl-benzoic acld (12, 2.0 g, 5.14 mmol) was dissolved in DMF (30 mL) and Cs2CO3 (0.84 g, 2.57 mmol) was added followed by stirring for 5 min at rt. Benzyl bromide (1.05 g, 6.17 mmol) was added and the mixture was al- lowed to stir for another 30 min at rt. Water (200 mL) was added and the mixture was extracted with CH2Cl2 (2 x 100 mL). The combined organic phases were washed with water (3 x 50 mL), dried over MgSO4, evaporated to dryness to yleld an oil which was used without further characterization in the next experiment. 17: Removal of Fmoc-group from benzyl-(N-Fmoc-4-aminooxymethyl)- benzoate The crude product (16) obtained in the previous experiment was stirred with 20% piperidine in DMF (20 mL) for 1 min and passed through a bed of silica gel to re- move the majority of DMF and piperidine by suction. The product was eluted from the bed of silica gel with a mixture of ethyl acetate and pet. ether (1:1) and concen- trated on a rotavap. Further purification was achieved by flash column chromatogra- phy (ethyl acetate, petroleum ether 1:1) to glve a clear oil in a yleld of 1.16 g (88%, two steps). 1H-NMR (250 MHz, CDcl3) 6 = 4.66 (2H, s), 5.29 (2H, s), 7.25-7.39 (7H, m), 7.99 (2H, dd, J =1.7 Hz, 6.5 Hz). 13C-NMR (63 MHz, CDcl3) δ = 67.11, 77.59, 128.32, 128.57, 128.66, 129.02, 129.19, 130.32, 136.48, 143.47, 166.64. MS (MaidI-TOF) m/z = 258 (MH+). General procedure for preparation of TMR labelled monosaccharide standards ex- emplified by the preparation of galactose standard. 18: Oxime formation between galactose and benzyl-(4-aminooxymethyl)- benzoate Galactose (90 mg, 0.50 mmol) was dissolved in a mixture of DMSO and AcOH (7:3, 3 mL) and (17,128 mg, 0.50 mmol) was added. The mixture was heated for 3 h at 55°C and poured into water (30 mL) and cooled on an ice bath which caused the product to crystallize as fine white crystals. The product was isolated by filtration, washed with water (2x10 mL) and dried under vacuum to yleld the 170 mg (83%) of product as a single isomer. 1H-NMR (250 MHz, DMSO-d6) 5 = 3.38-3.55 (4H, m), 3.67-3.75 (1H, m), 4.27-4.33 (1H, m), 5.12 (2H, s), 5.37 (2H, s), 7.36-7.52 (7H, m), 7.56 (1H, d, J= 7.6 Hz), 8.00 (2H, d, J= 8.1 Hz). 13C-NMR (63 MHz, DMSO-d6) δ = 63.40, 66.52, 68.37, 69.21, 70.04, 72.63, 74.27, 128.25, 128.33, 128.49, 128.91, 129.13, 129.67, 136.52, 144.22, 154.00, 165.78. MS (MaidI-TOF) m/z = 442 (MNa+) 19: Reduction of "galaclose-oxime" (18) with BH3-pyridine The oxime (18, 150 mg, 0.36 mmol) obtained in the previous experiment was dis- solved in methanol (10 mL). BH3-pyridine (225 µL, 8 M solution in pyridine, 1.80 mmol, Fluka) and CCl3CO2H (0.50 mL, 50% aqueous solution) were added and the mixture was stirred for 1 h at rt. The reaction mixture was carefully poured into a half-saturated solution of Na2CO3 (20 mL) and extracted with a 1:1 mixture of ether and hexanes (2x10 ml) to remove excess borane reagent. The pH was now ad- justed to 2-3 by careful addition of Hcl(COnc.) and the volume was reduced to half of the origlnal on a ratovap. During the evaporation the product separated out as nice white crystalline solid, which was filtered of, washed with water (2x10 mL), ether (2 x 10 mL) and finally the product was dried under vacuum to glve 112 mg (75%) of pure product. 1H-NMR (250 MHz, DMSO-d6) δ = 3.31-3.33 (2H, m), 3.40-3.55 (5H, m), 3.74 (1H, t, J= 6.3 Hz), 5.24 (2H, s), 5.37 (2H, s), 7.36-7.50 (5H, m), 7.60 (2H, d, J = 8.2 Hz), 8.04 (2H, d, J = 8.2 Hz). 13C-NMR (63 MHz, DMSO-d6) S = 53.34, 63.40, 64.73, 66.68, 69.37, 70.19, 70.89, 74.20, 128.36, 128.53, 128.92, 129.47, 129.87, 130.27, 136.41, 139.73, 165.62. MS (MaidI-TOF) m/z = 422 (MH+). 20: Labelling of reduced product (19) using TRITC A small amount of the product (19,4.2 mg, 10 µmol) prepared in previous experi- ment was dissolved in DMF (1 mL) and TRITC (4.4 mg, 10 µmol) was added. After stirring for 1 h water (10 mL) was added and the preclpitated product was re- dissolved by addition of Hcl(Conc.) and the clear red solution was applied to a small C- 18 Sep-Pak column to bind the product. The column was flushed several times with water (total volume 30 mL) followed by release of the product with methanol (5 mL). The volume was reduced to approximately 0.5 mL and the material was purified by flash column chromatography on silica gel with a mixture of CH2Cl2, methanol, wa- ter, AcOH (70:20:9:1). The identity of the compound was confirmed by MS and used directly in the next experiment. MS (MaidI-TOF) m/z = 865 (MH+). 21: Hydrolysis of ester protecting group to glve final standard All the material (2O) obtained in the previous experiment was dissolved in 1 M LiOH (1 mL) and stirred for 30 min followed by addition of water (10 mL) and acldification with Hcl(conc.) to glve a clear red solution. The product was desalted on a small C-18 Sep-Pak column by repeated washings with water (total volume 30 mL) followed by release of the product with methanol (5 mL). The volume was reduced to approxi- mately 0.5 mL and the product was purified by flash column chromatography on silica gel with a mixture of chloroform, methanol, water (120:85:2O). The identity of the compound was confirmed by high resolution MS and its purity was analysed using CE. HRMS (ES) calculated (C39H43N4O11S): 775,2649 found: 775.2700 Standards of the remaining monosaccharides (glucose, mannose, N- acetylglucosamine, N-acetylgalactosamine, xylose, fucose and glucuronic acld) were prepared using the same protocol as described for galactose in similar ylelds and purity. The compounds' identities were likewise confirmed by high resolution mass spectroscopy (see table below). Each compound gave a single peak in CE, and all 8 compounds (21-28) could be resolved in CE (Fig. 10). 3. Examples of B: Preparation and nomenclature of solid supports Solid supports of general structure B (Fig. 1) were prepared using both PEGA resin (PEGA 1900, Versamatrix A/S) and controlled-pore glass (CPG). Bp indicates a PEGA resin where the linker is attached directly to the amino groups on the com- merclal resin without a spacer. B°, B1 and B2 indicate CPG where the linker has been attached through 0,1 and 2 spacers respectively to aminopropylated glass (AMP-CPG, CPG-Biotech). The structures of the four solid supports are shown in Fig. 6. 3.1 Bp (PEGA resin of general structure B) 1 g of commerclal PEGA 1900 resin (loading of amino groups: 0.23 mmol/g) swelled in methanol was washed repeated time with DMF to ensure complete removal of the methanol. The linker (14) (308 mg, 0.69 mmol), TBTU (207 mg, 644 mmol) and DIPEA (119 mg, 0.92 mmol) were mixed in DMF (10 mL) and left to pre-activate for 5 min before adding the mixture to the resin. After 3 h the reagents were removed by suction and the resin was washed with CH2Cl2 (5 x 20 mL). A small portion of the resin was taken out for Kalser test which confirmed a success- ful coupling of the linker to the resin. Likewise, the loading of linker on the resin was determined as described in example 3.3 and found to be approximately 0.20 mmol/g by comparison with a standard curve. The hydroxylamine protecting group (Fmoc) was now removed from the remaining resin by treatment with 20% piperidine in DMF (15 mL for 2 min and 15 mL fori 8 min) followed by extensive washings with DMF (5 x 20 mL) and CH2Cl2 (7 x 20 mL). The resin was dried under high vacuum for 24 h to glve the final PEGA resin (Bp) which was used for all subsequent experi- ments. 3.2 B°, B1 and B2 (Controlled pore glass, CPG) B°: Coupling of linker 14 with CPG-NH2 AMP CPG (250 mg, loading = 50.1 µmol/g, 0.0125 mmol. Millipore, product no. AMP1400B) was washed with DMF (3 x 2 mL), 50% DIPEA in DMF (3 x 2 mL), and DMF (3x2 mL). The beads were treated with a mixture of 14 (17 mg, 0.038 mmol), TBTU (12 mg, 0.037 mmol), and DIPEA (8.6 µL, 0.05 mmol) in DMF at rt over night. The beads were washed with DMF (3x2 mL), CH2Cl2 (3x2 mL), and treated with 50% of AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3^2 mL), DMF (3x2 mL), CH2Cl2 (3x2 mL), and dried. The loading was determent to 14.2 µmol/g as described for B1. The Fmoc group was removed using 20% piperidine in DMF for 2 x 10 min at rt and washed with, DMF (3x2 mL), CH2Cl2 (3x2 mL), and ethanol (3 x 2 mL), and CH2Cl2 (3x2 mL). The resin was dried in vacuum. B1: Coupling of one spacer 15 and linker 14 with CPG-NH2 AMP CPG (2.26 g, loading = 50.1 pmol/g, 0.11 mmoi. Millipore, product no. AMP1400B) was washed with DMF (3> DMF (3x2 mL). The beads were treated with a mixture of 15 (168 mg, 0.34 mmol), TBTU (105 mg, 0.33 mmol), and DIPEA (78 µL, 0.45 mmol) in DMF for 3 h at rt. The resin was washed with DMF (3x5 mL), CH2Cl2 (3x5 mL), and treated with 50% AC20 in pyridine for 15 min at rt. The beads were washed with CH2Cl2 (3x5 mL), DMF (3x5 mL), CH2Cl2 (3x5 mL), and treated with 50% TFA in CH2Cl2 for 2 h at rt. Washed with CH2Cl2 (3x5 mL), DMF (3x5 mL), and CH2Cl2 (3x5 mL). 1/3 of the beads (2.5 mL, -0.70 g, -35 µmol) were washed with DMF (3x5 mL). Treated with 14 (47 mg, 0.11 mmol), TBTU (33 mg, 0.10 mmol), and DIPEA (34 µL, 0.20 mmol) in DMF over night at rt. The beads were washed with DMF (3x5 mL), CHaCl2 (3x5 mL), and treated with 50% AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3x5 mL), DMF (3x5 mL), CH2Cl2 (3x5 mL), and dried. The loading was determined (29 pmol/g) and the beads were treated with 20% piperidine in DMF at rt for 2 x 10 min. The beads were washed with, DMF (3x2 mL), CH2Cl2 (3x2 mL), and ethanol (3x2 mL), CH2Cl2 (3x2 mL), and dried. B2: Coupling of two spacers 15 and linker 14 with CPG-NH2 2/3 of the resin with one spacer from B1 (5.5 mL, ~1.54 g, -77 µmol) was washed with DMF (3x5 mL). The beads were treated with a mixture of 15 (114 mg, 0.23 mmol), TBTU (72 mg, 0.22 mmol), and DIPEA (53 µL, 0.31 mmol) in DMF over night at rt. The beads were washed with DMF (3x5 mL), CH2Cl2 (3x5 mL), and treated with 50% AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3x5 mL), DMF (3 x 5 mL), CH2Cl2 (3x5 mL), and treated with 50% CF3CO2H in CH2Cl2 for 2 h at rt, washed with CH2Cl2 (3 × 5 mL), DMF (3 x 5 mL), and CH2Cl2 (3 x 5 mL). Half the amount of the beads (~ 42 µmol) were washed with DMF (3x5 mL) and treated with 14 (56 mg, 0.13 mmoi), TBTU (39 mg, 0.12 mmol), and DIPEA (29 µL, 0.17 mmol) at rt over night. The beads were washed with DMF (3x5 mL), CH2Cl2 (3x5 mL) and treated with 50% AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3 x 5 mL), DMF (3x5 mL), CH2Cl2 (3x5 mL) and dried. The loading was determent as described for B1 to 36 umo!/g. The resin was covered with 20% piperidine in DMF at rt for 2 x 10 min, washed with, DMF (3x5 mL), CH2Cl2 (3x5 mL), ethanol (3x5 mL) 3 x CH2Cl2 (3x5 mL), and dried in vacuum. 3.3 Example of the estimation of the loading of capture groups on solid sup- ports of general structure B (Fig. 1) Seven concentrations of Fmoc-Gly-OH in 20% piperidine in DMF (0.0 mM, 0.1 mM, 0.25 mM, 0.5 mM, 1.0 mM, 1.5 mM, 2,0 mM) were prepared. The UV absorbance of released fulvene were measured at 290 nm using nonodrop technology (Saveen Werner Nanodrop, Model: ND-1000, Serial No: 0911). The absorbance was plotted against the concentration glving a linear curve with slope 0.581 mM"1. Fmoc protected B1 beads (4.8 mg) were treated with 20% piperidine in DMF (200 pL) for 10 min. The UV absorbance at 290 nm was measured to 0.410 and the lib- erated fulvene concentration was calculated 4. Examples of A+B->C, and processing of C. 4.1 Variation of capture conditions using glucose as the reducing sugar and B2 as the solid support. Various solvents, temperatures and additives were examined in order to find prefer- able conditions for the capture of reducing sugars on solid supports of general struc- ture B, to produce C. D-glc was used as the model compound, as the amount of uncaptured Glc in solution could be readily estimated with high sensitivity using the Ampiex Red assay from Molecular Probes. The amount of Glc captured was thus calculated to be the amount added minus the amount remaining in solution after incubation. 15-20 mg of beads (B2) were treated with a solution of glucose under different con- ditions. After end reaction time the supernatant was removed and the amount of un- reacted glucose was estimated using the Amplex Red Glucose/Glucose Oxidase Assay Kit (A-22189, Molecular Probes). Capture of glucose using different solvents, concentrations, temperatures and reaction times 4.2 Capture, processing and analysis of representative reducing sugars on Bp. The following designations are used below to describe compounds of the general structures C, Cred, D, E, F,G, H, I and J (Fig. 1). The particular letter describing the particular structure under discussion is glven first, e.g. C or E. The next superscript number refers to which of the four solid supports shown in Fig. 6 was used. Thus, by way of example if Bp (Fig. 6) is used to capture a sugar, then the product will have the general structure C which is further designated as Cp. The next number refers to which of the ten samples of reducing sugars shown in Fig. 2 was captured. Thus, Cp2 refers to the product of the PEGA resin Bp that has captured galactose (com- pound 2 of Fig. 2). In the same way, D25 would refer to the product obtained when the solid support B2 has captured the tetrasaccharide LNT (5, Fig. 2) to glve Cz5, and then been further capped to D25. 4.2.1 Capture and processing of reducing sugar 3 Cp3: Capture of LacNAc (3) on Bp A stock solution was made by first dissolving LacNAc (3) (38 mg, 0.10 mmol) in wa- ter (1.0 mL) and then diluting the sample 10 times with a mixture of DMSO and AcOH (7:3, 9 mL) to glve a 10 mM stock solution of LacNAc (3). 40 µL (0.40 pmol) was then taken from the stock solution and diluted further with the mixture of DMSO and AcOH (7:3,150 µL) and the whole was added to Bp (10 mg, 2 Mmol) and left to incubate at 60°C over night. The resin was washed several times: DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiments. Dp3: Capping of Cp3 with acetic anhydride All the resin obtained in experiment Cp3 was treated with a mixture of AC20 and methanol 1:1 (0.4 mL) for 1 h followed by washing with DMF (5 x 0.5 mL), water (2 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiment. Ep3: Reduction of Dp3 with BH3-pyridine The resin obtained in experiment Dp3 was covered with methanol (0.1 mL) and BH3- pyridine (20 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H acld in water (40 pL). The reaction was left to proceed for 2 h at rt followed by wash- ing with DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and CH2Cl2 (5 x 0.5 mL). The resin was used directly in the next step. Fp3: Tagglng of Ep3 using TRITC TRITC (0.89 mg, 2 pmol) was dissolved in DMF (0.2 mL) and the solution was added to the resin (Ep3) and left for 2 h at rt followed by extensive washing DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL), and finally water (5 x 0.5 mL) to remove excess dye. The resin was used directly in the next step. Gp3: Cleavage of TMR tagged LacNAc from support The resin obtained in the previous experiment Fp3 was covered with a 1 M solution of LiOH (0.2 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 0.5 mL). The collected liquld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The dark red solution was adsorbed on a Sep-Pak coiumn (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The identity of the product was confirmed by MS (ES) rn/z = 978 (MH+) and the profile was recorded by CE (Fig. 11). 4.2.2 Capture and processing of reducing sugar 5 Cp5: Capture of Lacto-N-tetraose (5) on Bp A solution was made by dissolving 5 (5.0 mg, 7.1 µmol) in a mixture of DMSO and AcOH 7:3 (3 mL). This mixture was added to PEGA resin Bp (175 mg, 35 µmol) and incubated at 60°C over night. The resin was washed several times: DMF (5x5 mL), methanol (5x5 mL) and used directly in the next experiments. Dp5: Capping of Cp5 with acetic anhydride All the resin obtained in experiment Cp5 was treated with a mixture of AC20 and methanol 1:1 (5 mL) for 1 h followed be washing with DMF (5x5 mL), water (2x5 mL), methanol (5 x 5 mL) and used directly in the next experiment. Ep5: Reduction of Dp5 with BH3-pyridine The resin obtained in experiment Dp5 was swelled in methanol (2 mL) and BH3- pyridine (200 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H acld in water (400 µL). The reaction was left to proceed for 2 h at rt followed by washing with DMF (5x5 mL), methanol (5x5 mL) and CH2Cl2 (5x5 mL). Finally the resin was dried down under vacuum over night and stored at room temperature for further use. Fp5: Tagglng of Ep5 with bromine containing MS-tag A small amount of the dried resin Ep5 (10 mg, 0.4 µmol) was washed with CH2Cl2 (3 x 0.5 mL) in order to swell the resin. A solution was made by dissolving 4- bromophenyl isothiocyante (0.85 mg, 4 µmol) in DMF (0.2 mL) and the mixture was added to the resin and left to react for 2 h at rt followed by washing of the resin DMF (5 x 0.5 mL), CH2clZ (5 x 0.5 mL), methanol (5 x 0.5 mL), and finally water (5 x 0.5 mL). The resin was used directly in the next step. Gp5: Cleavage of bromine tagged Lacto-N-tetraose from support The resin obtained in the previous experiment Fp5 was covered with a 1 M solution of LiOH (0.2 mL) and left for 2 h. The iiquld was collected from the beads by suction followed by washing of the beads with water (3 × 0.5 mL). The collected liquld and washings were pooled and pH was adjusted to slightly acldic (pH 3-4) with 10% AcOH. The solution containing the desired product was adsorbed on a Sep-Pak column (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The identity of the product was confirmed by MS (ES) m/z = 1072 (98%, MH+), 1074 (100%, MH+), m/z = 1070 (98%, M-H+), 1072 (100%, M-H+). Fig. 12 shows the mass-spectrum with an inset expansion where the two isotopes of bromine can clearly be distingulshed. 4.2.3 Capture and processing of reducing sugar mixture 6 Cp6: Capture of monosaccharide mixture 6 (Fuc:Man:GainAc, 2:3:1) on Bp A series of 3 stock solutions were made by dissolving the 3 individual monosaccha- rides (Fuc: 16 mg, 0.10 mmol, Man: 18 mg, 0.10 mol, GainAc: 22 mg, 0.10 mmol) in water (3 x 1.0 mL) and then diluting the samples 10 times with a mixture of DMSO and AcOH (7:3, 3x9 mL) to glve 10 mM stock solutions of the 3 monosaccharides. A mixture was now prepared by taking the following amounts from the 3 stock solu- tions: Fuc (20 pi, 0.2 pmol), Man (30 µL, 0.3 µmol) and GainAc(10 µL, 0.1 µmol). This monosaccharide solution was diluted further by addition of the mixture of DMSO and AcOH (7:3,150 µL) and the whole was added to PEGA resin Bp (10 mg, 2 pmol) and left to incubate at 60°C over night. The resin was washed several times: DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiments. Dp6: Capping of Cp6 with acetic anhydride All the resin obtained in experiment Cp6 was treated with a 1:1 mixture of AC2O and methanol (0.4 mL) for 1 h followed be washing with DMF (5 x 0.5 mL), water (2 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiment. Ep6: Reduction of Dp6 with BH3-pyridine The resin obtained in experiment Dp6 was covered with methanol (0.1 mL) and BH3- pyridine (20 µL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H in water (40 pL). The reaction was left to proceed for 2 h at rt followed by washing with DMF (5 x 0,5 mL), methanol (5 x 0.5 mL) and CH2Cl2 (5 x 0.5 mL). The resin was split into 2 separate containers (Ep6a and Ep6b, app. 5 mg each) and used di- rectly in the next steps. Fp6a: Tagglng of Ep6a using TRITC TRITC (0.5 mg, 1.2 jjmol) was dissolved in DMF (0.2 mL) and the solution was added to the resin (Ep6a) and left for 2 h at rt followed by extensive washing DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL) to remove excess dye. The resin was used directly in the next step. Gp6a: Cleavage of TMR tagged monosaccharide mixture from support The resin obtained in the previous experiment (Fp6a) was covered with a 1 M solu- tion of LiOH (0.1 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq- uld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The dark red solution was adsorbed on a Sep-Pak column (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The identity of the 3 tagged products was confirmed by MS (ES) m/z = 759 (Fuc, Mt-T), 775 (Man, MH+) δ16 (GainAc, MH+) and thelr profile was recorded by CE (Fig. 13). Fp6b: Tagglng of Ep6b with acetic anhydride A 1:1 mixture of AC20 and methanol (0.2 mL) was added to the resin (Ep6b) and left for 16 h at rt followed by extensive washing DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL). The resin was used directly in the next step. Gp6b: Cleavage of acetic acld tagged monosaccharide mixture from support The resin obtained in the previous experiment (Fp6b) was covered with a 10% solu- tion of NH4OH (0.1 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq- uld and washings were pooled and evaporate to dryness on a rotavap, re-dissolved in water (1 mL) and freeze dried. The identity of the 3 tagged products was con- firmed by MS (ES) m/z = 356 (Fuc, M-H+), 372 (Man, M-H+), 413 (GainAc, M-H+). The ratio of the intensities of the 3 signals was approximately 1.3:2:1. 4.2.4 Capture and processing of reducing sugar mixture 7 Cp7: Capture of monosaccharide mixture 7 (Fuc:Man:GainAc, 1:3:2) on Bp The same 3 stock solutions of monosaccharides (10 mM each) that were used in experiment Cp6 was used in the following experiment. A mixture was prepared by taking the following amounts from the 3 stock solutions: Fuc (10 µL, 0.1 µmol), Man (30 µL, 0.3 µmol) and GainAc (20 µL, 0.2 µmol). This monosaccharide solution was diluted further by addition of the mixture of DMSO and AcOH (7:3,150 µL) and the whole was added to PEGA resin Bp (10 mg, 2 µmol) and left to incubate at 60°C over night. The resin was washed several times: DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiments. Dp7: Capping of Cp7 with acetic anhydride All the resin obtained in experiment Cp7 was treated with a 1:1 mixture of AC20 and methanol (0.4 mL) for 1 h followed by washing with DMF (5 x 0.5 mL), water (2 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiment. Ep7: Reduction of Dp7 with BH3-pyridine The resin obtained in experiment Dp7 was covered with methanol (0.1 mL) and BH3- pyridine (20 µL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H in water (40 µL). The reaction was left to proceed for 2 h at rt followed by washing with DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and CH2Cl2 (5 x 0.5 mL). The resin was split into 2 separate containers (Ep7a and Ep7b, app. 5 mg each) and used di- rectly in the next step. Fp7a: Tagglng of Ep7a using TRITC TRITC (0.5 mg, 1.2 µmol) was dissolved in DMF (0.2 mL) and the solution was added to the resin (Ep7a) and left for 2 h at rt followed by extensive washing DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL) to remove excess dye. The resin was used directly in the next step. Gp7a: Cleavage of TMR tagged monosaccharide mixture from support The resin obtained in the previous experiment (Fp7a) was covered with a 1 M solu- tion of LiOH (0.1 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq- uld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The dark red solution was adsorbed on a Sep-Pak column (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The identity of the 3 tagged products was confirmed by MS (ES) m/z = 759 (Fuc, MH+), 775 (Man, MH+) δ16 (GaSNAc, MH+) and thelr profile was recorded by CE (Fig. 14). Fp7b: Tagglng of Ep7b with deuteroacetic anhydride A 1:1 mixture of deuteroacetic anhydride and methanol (0.2 mL) was added to the resin (Ep7b) and left for 16 h at rt followed by extensive washing DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL). The resin was used directly in the next step. Gp7b: Cleavage of deuterium tagged monosaccharide mixture from support The resin obtained in the previous experiment (Fp7b) was covered with a 10% solu- tion of NH4OH (0.1 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq- uld and washings were pooled and evaporate to dryness on a rotavap, re-dissolved in water (1 mL) and freeze dried. The identity of the 3 deuterium tagged products was confirmed by MS (ES) m/z = 359 (Fuc, M-H+), 375 (Man, M-H+), 416 (GainAc, M-H+). The ratio of the intensities of the 3 signals was approximately 1:4:4. 4.2.5 Capture and processing of reducing oligosaccharide mixture 9 Cp9: Capture of oligosaccharide mixture 9 (G2-G7) on Bp A solution was made by dissolving an equlmolar amount (10 µmol each) of the pure oligosaccharides G2-G7 in water (1 mL). 100 µL of the oligosaccharide containing solution was added to a mixture of DMSO and AcOH (7:3, 0.9 mL) and the whole was added to PEGA resin Bp (60 mg, 12 µmol) and left to incubate at 50°C over night. The resin was washed several times: DMF (5x2 mL), methanol (5x2 mL) and used directly in the next experiments. Dp9: Capping of Cp9 with acetic anhydride All the resin obtained in experiment Cp9 was treated with a 1:1 mixture of AC20 and methanol (2 mL) for 1 h followed be washing with DMF (5 x 2 mL), water (2x2 mL), methanol (5x2 mL) and used directly in the next experiment. Ep9: Reduction of Dp9 with BH3-pyridine The resin obtained in experiment Dp9 was covered with methanol (1 mL) and BH3- pyridine (150 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H in water (300 µL). The reaction was left to proceed for 2 h at rt followed by washing with DMF (5x2 mL), methanol (5x2 mL) and CH2C!2 (5x2 mL). The resin was used directly in the next step. Fp9: Tagglng of Ep9 using FITC FITC (12 mg, 30 pmol) was dissolved in a 1:1 mixture of DMF and methanol (1 mL) and the solution was added to the resin (Ep9) and left for 2 h at rt followed by exten- sive washing DMF (5x2 mL), CH2Cl2 (5x2 mL), methanol (5x2 mL) and finally water (5x2 mL) to remove excess dye. The resin was used directly in the next step. Gp9: Cleavage of oligosaccharide mixture tagged using FITC from support The resin obtained in the previous experiment (Fp9) was covered with a 1 M solution of LiOH (1 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 3 mL). The collected liquld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The strong yellow solution was adsorbed on a Sep-Pak column (350 mg), washed with water (10 mL) and eluted with methanol (3 mL). The presence of all 6 tagged oligosaccha- rides was confirmed by MS (ES) m/z = 881 (G2, MH+), 1043 (G3, MH+), 1205 (G4, MH+), 1367 (GS, MH+), 1529 (G6, MIT), 1691 (G7, MH+) and the profile of the mix- ture was recorded by CE (Fig. 15). 4.2.6 Capture and processing of oligosaccharides released from ribonuclease B. Cp10: Capture and processing of oligosaccharides from RNAse B (10) on Bp Crude oligosaccharides from PNGase F digestion of RNAse B (Sigma, R-7884) were used after protein removal on a Centricon-10 concentrator (Millipore) followed by carbohydrate purification on a Carbograph SPE column (150 mg bed welght; Scantec Lab). A solution was made by dissolving crude oligosaccharides from RNAse B (10)2 (300 ug, app. 0.2 µmol) in a mixture of DMSO containing 0.9 M cltric acld and THF 2:1 (100 µL). This mixture was added to PEGA resin Bp (5 mg, 1.0 µmol) and incubated at 60°C over night. The resin was washed several times: DMF (5 x 0.3 mL), methanoi (5 x 0.3 mL) and used directly in the next experiments. Dp10: Capping of Cp10 with acetic anhydride All the resin obtained in experiment Cp10 was treated with a 1:1 mixture of AC20 and methanol (0.2 mL) for 1 h followed be washing with DMF (5 x 0.3 mL), water (2 x 0.3 mL), methanol (5 x 0.3 mL) and used directly in the next experiment. Ep10: Reduction of Dp10 with BH3-pyridine The resin obtained in experiment Dp10 was covered with methanol (0.2 mL) and BH3-pyridine (10 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H in water (20 pL). The reaction was left to proceed for 2 h at rt followed by washing with DMF (5 x 0.3 mL), methanol (5 x 0.3 mL) and CH2Cl2 (5 x 0.3 mL). The resin was used directly in the next step. Fp10: Tagglng of Ep10 using FITC FITC (1.9 mg, 5 pmol) was dissolved in a mixture of DMF and methanol (1:1, 0.2 mL) and the solution was added to the resin (Ep10) and left for 2 h at 60° followed by extensive washing DMF (5 x 0.3 mL), CH2Cl2 (5 x 0.3 mL), methanol (5 x 0.3 mL) and finally water (5 x 0.3 mL) to remove excess dye. The resin was used directly in the next step. Gp10: Cleavage of oligosaccharides from RNAse tagged using FITC from sup- port The resin obtained in the previous experiment (Fp10) was covered with a 1 M solu- tion of LiOH (0.2 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq- uld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The yellow solution containing the desired product was adsorbed on a Sep-Pak column (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The profile of the labelled oligosaccharides was analysed by CE. The CE (Fig. 16) indicates the presence of several oligosaccharides and some unidentified contaminants. The identity of at least one of the known components was confirmed by MS (ES) m/z = 1775 (Man5GlcNAcGlcNAcCHz-N-(R)-TAG, MH+). 4.3 Capture and processing of representative reducing sugars on CPG sup- ports. 4.3.1 Capture and processing of 2 on B1 C12: Capture of galactose (2) on B1 B1 (20 mg, 0.6 µmol) was treated with 2 (6.6 µL, 1 mg/mL water, 0.03 µmol) in clt- rate-phosphate buffer (113 µL) and left over night at 55°C. The beads were trans- ferred to a syringe and washed with water (3 x 0.5 mL) and ethanol (3 × 0.5 mL) glving C12. D12: Capping of C12 with acetic anhydride C12 (0.6 µmol) were capped with 50% AC20 in ethanol for 15 min at rt and washed with ethanol (3 x 0.5 mL) glving D12. E12: Reduction of D12 with BH3-pyridine D12 (0.6 µmol) was treated with 100 µL of a solution of BH3-pyridine (25 µL), 50% CCl3CO2H (50 pL) in ethanol (500 µL). The mixture was left for 2 h at rt. The beads were washed with ethanol (3 × 0.5 mL) glving E12. F12: Labelling of E12 with TRITC E12 (0.6 pmol) was treated with TRITC (100 µL of 1.0 mg in 300 µL NMP and 300 uL CH2Cl2) and left for 2 h at rt. The beads were washed with CH2Cl2 (3 × 0.5 mL), ethanol (3 × 0.5 mL), and water (3 × 0.5 mL) glving F12 (red beads). G12: Base treatment of F12 F12' (0.6 µmol) was treated with 1 M solution of LiOH (100 µL) for 1 h at rt and the red solution was isolated and neutralised with 50% AcOH in water glving G12 (red solution) which were passed through a Sep-Pak column (30% CH3CN in water) and analysed by MS (775.3, MH+) and CE (Fig. 17). 4.3.2 Capture and processing of 5 on B1 C15: Capture of LNT (5) on B1 B1 (20 mg, 0.6 µmol) was treated with 5 (25 µL, 2 mg/mL water, 0.03 umo!) in clt- rate-phosphate buffer (113 µL) and left over night at 55°C, The beads were trans- ferred to a syringe and washed with water (3 × 0.5 mL) and ethanol (3 × 0.5 mL) glving C15. D15: Capping of C15 with acetic anhydride C15 (0.6 µmol) was treated with 50% AC20 in ethanol for 15 min at rt and washed with (3 × 0.5 mL) glving D15. E15: Reduction of D15 with BH3-pyridine D15 (0.6 µmol) was treated with 100 µL of a solution of BH3-pyridine (25 µL), 50% CCl3CO2H (50 µL) in ethanol (500 µL). The mixture was left for 2 h at rt. The beads were washed with ethanol (3 x 0.5 mL) glving E15. F15: Labelling of E15 with TRITC E15 (0.6 µmol) was treated with TRITC (100 µL of 1.0 mg in 300 µL NMP and 300 µL CH2Cl2) and left for 2 h at rt. The beads were washed with CH2Cl2 (3 x 0.5 mL), ethanol (3 x 0.5 mL), and water (3 x 0.5 mL) glving F'5 (red beads). G15: Base treatment of F15 The resin was treated with a 1 M solution of LiOH (100 µL) for 1 h at rt and the red solution was isolated by filtration and the beads were washed with water (3 x 75 µL) and neutralised with 50% AcOH in water glving G15 (red solution) which were passed through a Sep-Pak column (30% CH3CN in water) and analysed by MS (ES) m/z = 1300.6 (M-H+), 1302.4 (MH+) and by CE (Fig. 18). Alternatively, E15 could be labelled with 1- fluoro-2,4-dinitrobenzene (Sanger's re- agent, (Fig. 8) as follows. The resin was treated with Sanger's reagent (20 eq, 0.4 µL, Sigma) and TEA (10 eq, 0.2 µL) in ethanol (70 µL) for 2 h at 55°C. The beads were washed with ethanol (3 x 0.5 mL), CH2Cl2 (3 x 0.5 mL), ethanol (3 x 0.5 mL), and water (3 x 0.5 mL) (yellow beads), then treated with 1 M solution of LiOH (70 µL) for 1 h at rt (brown solution). The solution was collected by filtration and the beads were washed with water (3 x 50 µL). The mixture was neutralised with 50% AcOH (yellow solution). The mixture was passed through a Sep-Pak column with 30% CH3CN in water. MS (ES) m/z = 1023.1 (M-H+). 4.3.3 Capture and and processing of mixture 8 on B1 C18: Capture of Galactose (2) and LNT (5) on B1 B1 (20 mg, 0.6 µmol) was treated with 2 (6.6 pL, 1 mg/mL water, 0.03 pmol), 5 (25 pL, 2 mg/mL water, 0.03 µmol), cltrate-phosphate buffer (100 pL), and left over night at 55°C. The beads were washed with water (3 × 0.5 mL) and ethanol (3 × 0.5 mL) glving C18. D18: Capping of C18 with acetic anhydride The remaining hydroxylamines in C18 (0.6 µmol) were capped with 50% AC20 in ethanol for 15 min at rt and washed with ethanol (3 × 0.5 mL) glving D18. E18: Reduction of D18 with BH3-pyridine D18 (0.6 µmol) was treated with 100 pL of a solution of BH3-pyridine (Fluka, 25 pL), 50% CCl3CO2H (50 pL) in ethanol (500 pL). The mixture was left for 2 h at rt. The beads were washed with ethanol (3 × 0.5 mL) glving E18. F18: Labelling of E18 using TRITC E18 (0.6 µmol) was treated with TRITC (100 pL of 1.0 mg in 300 pL NMP and 300 pL CH2Cl2) and left for 2 h at rt glving F18. The beads were washed with CH2Cl2 (3 × 0.5 mL), ethanol (3 x 0.5 mL), and water (3 x 0.5 mL) (red beads). G18: Base treatment of F18 F18 was treated with 1 M solution of LiOH (100 µi) for 1 h at rt and the red solution was isolated and neutralised with 50% AcOH in water glving G18 (red solution) which were passed through a Sep-Pak column (30% CH3CN in water) and analysed by CE (Fig. 19). 5. Reaction of immobilized oligosaccharides with enzymes 5.1 Reaction of an immobilized tagged oligosaccharide with a glycosidase 5.1.1 Reaction of immobilized lacto-N-tetraose (LNT, 5) of structure F (cap = acetyl, TAG = TMR) with beta-galactosidase (bovine testes, SIGMA product G-4142, 1U/mL) on CPG supports with none (F°5), one (F15) and two (F25)spacers. All 3 immobilized oligosaccharides were prepared essentially as described for F15 (sec- tion 4.3.2). The solid supports (5 mg) were incubated with beta-galactosidase (100 ul_ of 0.2 U/mL solution in 0.1 M cltrate/phosphate buffer pH 5.0 containing 0.2% BSA for 23 h at 37°C, and the resin was then washed with 3 x water, 3 × ethanol, 3 × CH2Cl2, 3 x Et ethanol OH, and 3 x water. The beads were treated with 1 M solution of LiOH (60 3 µL) for 1 h at rt glving products of the general structures G°5, G15, and G25 in solu- tion. Each red solution was collected by filtration. The filtrate was neutralised with 50% AcOH and analysed using CE. Fig. 20 shows that there was no detectable cleavage of galactose from LNT for F°5, 39% conversion for F15 (i.e. 39% of the tetrasaccharide had lost the terminal Gal residue and been converted to the trisaccharide) and 83% conversion for F25. The nature of the spacer was therefore found to be important to the course of the en- zyme reaction. 5.1.2 Reaction of immobilized maltotriose F24 (cap = acetyl, TAG = TMR) with glu- coamylase 2 from Asperglllus niger (kindly provided by Dr. Birte Svensson, Carls- berg Laboratories) on CPG support with two spacers. F24 was prepared essentially as described for F15 (section 4.3.2) but using maltotriose (G3, Fig. 2) as the reduc- ing sugar and B2 as the solid support. F24 (ca 5 mg) was incubated for 23 h at 37°C with 50 µL of 0.1 mg/mL of enzyme in 0.1 M sodium acetate buffer pH 5.5 contain- ing 0.2% BSA. After washing and cleavage as described above, the product was analyzed by CE (Fig. 21), which showed complete conversion of immobilized la- belled maltotriose to a new peak eluting between labelled maltotriose and glucose, therefore assigned as the maltobiose (G2) TMR adduct. 5.2 Reaction of an immobilized untagged oligosaccharide with a glycosidase and capture of the released reducing monosaccharide on the same support. Reaction of immobilized LNT of structure C25 (non-reduced, non-capped, non- tagged) with beta-galactosidase (bovine testes) was carried out on CPG solid sup- port with two spacers. C25 was prepared essentially as described for C15 (section 4.3.2). Prior to use, the enzyme solution was freed from small-molecule contami- nants by repeated centrifugation using a Microcon YM-3 centrifugal filter device (Mil- lipore). C25 (5 mg) was incubated for 23 h at 37°C with 55 µL of 0.9 U/mL of enzyme in 0.1 M cltrate/phosphate, pH 5.0, containing 0.2% BSA, and then a further 20 h at 55CC to permit capture of released galactose. The solid was washed, reduced, capped with acetic anhydride, tagged using TRITC and cleaved with LiOH as de- scribed above for the conversion of C15 to G15. The CE of cleaved product is shown in Fig. 22 which shows the presence of unreacted LNT (32%) and similar amounts of both the TMR-labelled product trisaccharide and cleaved galactose. This experi- ments confirms the capture of cleaved sugar on the same uncapped support from which it was cleaved. 6. Variation of capping agents 6.1. Capping of C to produce D A selection of capping agents was used to effect the conversions C goes to D (Fig. 1). C22 was used as the substrate (where the solid was CPG with 2 spacers and the captured sugar was galactose). The amino groups on C were then capped with, among others, acetic anhydride, benzoic anhydride, tricholoracetic anhydride and dibromoxylene (Fig. 6). The capping was carried with 50% solutions of the capping agent in ethanol, for 15-120 min at it The samples were then processed as de- scribed for the conversion of C12 to G12 (section 4.3.1), i.e., reduction, labelling us- ing TRITC, base-cleavage and analysis by CE. The results are shown in Fig. 23 which shows that all conditions provided the target TMR-labelled galactose (com- pound 21, Fig. 5) with varylng amounts of other impurities appearing before com- pound 21 in the electropherogram. 6.2 ExampJe of capping of Cred to produce E C22 from section 6.1 above was reduced with BH3-pyridine as described for the con- version of D12 to E12 above (section 4.3.1). The product CreCl22 differs from E12 in that it contains uncapped NH2 groups. Cred22 (5 mg) was reacted with benzoic acld NHS-ester (0.4 mg, 1.75 µmol) and TEA (1.0 µL) in DMF (50 pL) over night at 60°C. The product of the reaction having the general structure E22 (with the cap being a benzoate) was then washed and processed as usual, by tagglng using TRITC, cleavage and analysis by CE. Fig. 24 shows the product to be substantially the same as that formed by the sequence C goes to D goes to E and on to G. The iden- tity of the product was confirmed by its MS (ES) m/z = 775.0 (Mt-f). 7. Example of the use of a tether: E goes to H goes to I goes to J (Fig. 1) Synthesis of 29 as example of X-tether-YP 29: 4-lsothiocyanato-benzyl)-carbamic acld 9W-fluoren-9-ylmethyl ester To a solution of 4-aminobenzylamine (0.93 mL, 8.20 mmol) in anhydrous CH2Cl2 (20 mL) was added TEA (1.15 mL, 8.27 mmol) followed by a solution of Fmoc-N- hydroxysuccinimide ester (2.48 g, 7.35 mmol) in dry CH2Cl2 (10 mL). After 30 min of stirring, CH2Cl2 (100 mL) was added and the mixture was washed successively with sat. aq. NaHCO3 (2 x 50 mL) and brine (50 mL), and dried (Na2SO4). The solvent was removed under reduced pressure and the residue purified by dry column vac- uum chromatography (0-60% EtOAc in n-heptane) to yleld the Fmoc-protected ma- terial (4-Amino-benzyl)-carbamic acld 9/-/-fluoren-9-ylmethyl ester (2.30 g, 91%). 1H- NMR (250 MHz, DMSO-d6) 5 = 4.03 (2H, d, J = 5,3 Hz), 4.22 (1H, t, J = 6,8 Hz), 4.33 (2H, d, J = 6,8 Hz), 4.95 (2H, s), 6.53 (2H, d, J = 8.3 Hz), 6.92 (2H, d, J = 8.2 Hz), 7.29-7.44 (4H, m), 7.64-7.72 (3H, m), 7.88 (2H, d, J = 7.3 Hz). 13C-NMR (63 MHz, DMSO-d6) 5 = 43.97, 47.19, 65.65,114.09, 120.46, 121.75, 125.58,127.11, 127.42,127.96, 128.47,129.30, 141.13, 144.32,147.89, 156.63. MS(ES)m/z = 345 (MH+). A solution of (4-Amino-benzyl)-carbamic acld 9H-fluoren-9-ylmethyl ester (718 mg, 2.09 mmol) in CH2Cl2 (30 mL) was added dropwise to a solution of thiophosgene (199 \il, 2.61 mmol) in a CH2Cl2-water mixture (40 mL, 1:1, v/v). After the mixture was stirred over night, the organic phase was isolated and dried (Na2SC>4). The sol- vent was removed under reduced pressure and the residue purified by dry column vacuum chromatography (0-100% CH2Cl2 in n-heptane) to yleld 29 (643 mg, 80%). 1H-NMR (250 MHz, DMSO-d6) S = 4.18-4.25 (3H, m), 4.38 (2H, d, J = 6.7 Hz), 7.25- 7.45 (8H, m), 7.69 (2H, d, J= 7.3 Hz), 7.87-7.90 (3H, m). ,3C-NMR (63 MHz, DMSO-d6) δ = 43.64, 47.19, 65.70, 115.55, 120.48, 125.15,125.49, 126.20, 127.42, 127.98, 128.72, 128.83, 133.55, 136.29, 140.26, 141.16, 144.23, 156.74. MS (ES) m/z = 387 (MH+). Hp5: Attachment of Fmoc-protected amino tether to Ep5 using 29 (Fig. 9) 5 mg of the dried resin (Ep5) (0.2 nmol) was washed a couple of times with CH2Cl2 to ensure proper swelling of the resin. The Fmoc-protected tether (29) (0.8 mg, 2 pmol) was dissolved in DMF (0.2 mL) and added to the resin and left to react for 2 h. The resin was washed with DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL) and the Fmoc protecting group was removed under standard conditions (20 % piperidine in DMF, 0.5 ml 2 x 10 min). The resin was used directly in the next experiment after washing with DMF (5 x 0.5 mL) lp5: Tagglng of Hp5 using TR1TC The resin obtained in experiment Hp5, now containing a free primary amino group, was incubated with TRITC (0.9 mg, 2 µmol) in DMF (0.2 mL) at rt for 2 h followed by extensive washing with DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL) to remove excess dye. The resin was used di- rectly in the next step. Jp5: Cleavage of Lacto-N-tetraose tagged using TRITC via an amino tether The resin obtained in the previous experiment (lp5) was covered with a 1 M solution of LiOH (0.2 mL) and left for 2 h. The liquld was collected from the beads by suction followed by washing of the beads with water (3 × 0.5 mL). The collected liquld and washings were pooled and pH was adjusted to slightly acldic (pH 3-4) with 10% AcOH. The dark red solution containing the desired product was adsorbed on a Sep-Pak column (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The identity of the product was confirmed by MS (ES) m/z = 1465 (MH+). Capillary electrophoresis analysis of labeled carbohydrates Capillary electrophoresis (CE) was performed using an automated PrinCE 2-lift, model 560 CE system (Prince Technologles, The Netherlands). Separations were carried out in an uncoated fused-silica capillary of 75 µm ID with an effective length in the range 50 -75 cm (plus 30 cm of extra length from the detection window to the outlet), thermostatically controlled at 25°C. The CE background electrolyte (BGE) was elther (A) 50 mM borate buffer pH 9.3 containing 150 mM SDS or (B) 0.2 M borate buffer pH 9.3 containing 0.8% (w/v) γ-CD (Sigma, C-4892). Conditions A were used for the analyses shown in Figs. 11 and 15-22. Conditions B were used for the analyses shown in Figs. 10, 13, 14, 23 and 24. The capillary was conditioned at room temperature by rinsing at 2000 mbar for 30 min with 1 M NaOH, 10 min with water, and 10 min with BGE before use. Between runs the capillary was washed at 2000 mbar for 3 min with 1 M NaOH, 3 min with water, and 3 min with BGE. Samples were injected hydrodynamically for 6 sec at 50 mbar and electrophoresed across a potential difference of 25 kV. All experiments were carried out at a normal polarity, i.e. inlet anodic. Detection was carried out us- ing a fluorescence detector (Argos 250B, Flux Instruments, Switzerland) equlpped with the appropriate filters. For samples labeled using TRITC, the excltation and emission filters were respectively 546.1/10 and 570 nm. For samples labeled using FITC, the excltation and emission filters were respectively UG11 (200-400 nm) and 495 nm. Abbreviations The following abbreviations have been used throughout the present application: AMP CPG Aminopropyl controlled pore glass BGE Background electrolyte BSA Bovine serum albumin CE Capillary electrophoresis CPG Controlled pore glass DIPEA N,N-Diisopropylethylamine DMF N,N-Dimethylformamide ES Electrospray FITC Fluorescein isothiocyanate Fmoc 9-Fluorenylmethyloxycarbonyl HRMS High resolution mass spectroscopy LNT Lacto-N-tetraose MS Mass spectroscopy NHS N-Hydroxysuccinimide NMP 1 -methyl-2-pyrrolidone PEGA Polyethylenglycol acrylamide polymer RNAse B Ribonuclease B rt Room temperature TBTU N,N,N',N'-tetramethyl-O-{1 H-benzotriazol-1 - yl)uroniumtetrafluorborate TEA Triethylamine TMR Tetramethylrhodamine TRITC Tetramethylrhodamine isothiocyanate WE CLAlM 1. A method of preparing a reactive sugar, said method comprising the steps of i. Providing a sample comprising a reducing sugar ii. Providing a solid support covalently attached to a linker comprising a capture group comprising an -NH2 group, wherein said linker optionally is attached to said solid support via a spacer iii. Reacting said reducing sugar with said -NH2 group, thereby obtaining an immobilised sugar, iv. Reacting free -NH2 groups with a capping agent, wherein the capping agent comprises a reactive group capable of reacting with an -NH2 group; v. Reducing C=N bonds with a reducing agent; vi. thereby obtaining an reactive sugar of the structure SugarCHn-NH-linked to a solid support via a linker and optionally a spacer, wherein n is 1 or 2. wherein step iv is performed prior to step v. 2. The method as clalmed in clalm 1, wherein the method further comprises the step of vii. Reacting the -NH- group of the reactive sugar with a derivatising agent comprising an nitrogen-reactive functional group (X), thereby obtaining a sugar covalently attached to said agent. 3. The method as clalmed in clalm 2, wherein said nitrogen-reactive functional group is selected from the group consisting of isothiocyanates, active esters, carboxylic aclds, Michael acceptors, alpha-beta unsaturated sulfones, alkylating agents, aidehydes, ketones and substituted haloaromatic groups bearing electronegative groups. 4. The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a spectroscopically detectable compound derivatised with a nitrogen-reactive functional group. 5. The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a fluorescent compound derivatised with a nitrogen-reactive functional group. 6. The method as clalmed in any of clalms 4 and 5, wherein said method comprises the step of viii.detecting said agent attached to the sugar by spectrometry. 7. The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a mass spectrometry TAG derivatised with a nitrogen-reactive functional group, wherein the mass spectrometry TAG is capable of improving the detection and/or structural charaterisation of a sugar. 8. The method as clalmed in clalm 7, wherein the mass spectrometry TAG is a molecule comprising bromine. 9. The method as clalmed in clalm 7, wherein the mass spectrometry TAG is a charged molecule. 10.The method as clalmed in clalm 7, wherein the mass spectrometry TAG is an isotope labelled molecule. 11.The method as clalmed in any of clalms 7 to 10, wherein the method comprises the step of ix. detecting said mass spectrometry TAG attached to said sugar by mass spectrometry 12.The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a first binding partner capable of speclfic interaction with a second binding partner, and wherein said first binding partner is derivatised with a nitrogen- reactive functional group. 13.The method as clalmed in clalm 12, wherein one binding partner is a protein and the other binding partner is a ligand of said protein. 14.The method as clalmed in clalm 12, wherein one binding partner comprises an epitope and the other binding partner is an antibody speclfically recognising said epitope. 15.The method as clalmed in clalm 12, wherein one binding partner is biotin and the other binding partner is an avidin. 16.The method as clalmed in any of clalms 12 to 15, wherein the second binding partner is conjugated to a detectable label. 17.The method as clalmed in any of clalms 2 and 3, wherein the derivatising agent is a nuclelc acld derivatised with a nitrogen-reactive functional group or a protected nitrogen reactive functional group. 18.The method as clalmed in clalm 17, wherein said nuclelc acld is a DNA. 19.The method as clalmed in any of clalms 17 to 18, wherein the method comprises the step of x. detecting said nuclelc acld attached to said sugar 20.The method as clalmed in clalm 19, wherein said nuclelc acld is detected by an essentially complementary nuclelc acld conjugated to a detectable label. 21.The method as clalmed in clalm 19, wherein detection of said nuclelc acld involves amplification of the nuclelc acld. 22.The method as clalmed in any of clalms 2 and 3, wherein said agent is a bifunctional reagent of the structure X- tether-Y or X-tether-Yp, wherein X is a nitrogen-reactive functional group and Y is a second reactive functional group and Yp is a protected reactive group Y. 23.The method as clalmed in clalm 22, wherein said second reactive functional group Y is selected from the group consisting of, thiols, carboxyl groups, activated carboxyl groups, disulfides, activated disulfides, alkylating agents, alkenes, alkynes, aidehydes, ketones and azides or Yp is selected from the group consisting of protected derivatives of aforementioned groups Y and protected amines. 24.The method as clalmed in any of clalms 22 and 23, wherein the method further comprises the steps of: xi) providing a second derivatising agent comprising a functional group (Z) capable of reacting with Y xii) reacting the functional groups Z and Y, thereby covalently attaching the second derivatising agent to the sugar via a tether and the first derivatising agent. 25.The method as clalmed in clalm 24, wherein the second derivatising agent is selected from the group consisting of drugs, imaglng agents, peptides, polypeptides, proteins, enzymes, nuclelc aclds, spectroscopically detectable compounds, mass spectrometry TAGs and first binding partners capable of speclfic interaction with a second binding partner. 26.The method as clalmed in any of clalms 22 and 23, wherein the method further comprises the steps of: xiii) providing a particle selected from the group consisting of microbial organism, micelles, phages, vira and nanoparticles, wherein the particle comprises a functional group (Z) capable of reacting with Y. xiv) reacting the functional groups Z and Y, thereby covalently attaching the particle to the sugar via the tether and the agent. 27.The method according to clalm 1, wherein the method comprises the steps of xv) contacting the sugar with a detection agent capable of assoclating with said sugar xvi) detecting the detection agent 28.The method as clalmed in clalm 27, wherein said detection agent comprises aryl boronate or heteroarylboronate. 29.The method as clalmed in clalm 27, wherein the detection agent is a polypeptide. 30.The method as clalmed in clalm 29, wherein said polypeptide is selected from the group consisting of lectins, selectins, toxins, receptors, antibodies and enzymes. 31.The method as clalmed in any of the preceding clalms, wherein the capture group comprises or consists of the structure M-NH2 wherein M is a heteroatom. 32.The method as clalmed in any of the preceding clalms, wherein the linker is a non-cleavable linker selected from the group consisting of alkyls, aryls, ethers and amides, wherein any of the aforementioned may optionally be substituted. 33.The method as clalmed in any of clalms 1 to 31, wherein the linker is a cleavable linker. 34.The method as clalmed in clalm 33, wherein the linker is cleavable by reaction with acld, base, nucleophiles, electrophiles, oxidation, reduction, free radicals, light, heat or enzymes. 35.The method as clalmed in any of clalms 33 and 34, wherein the method comprises the step of cleaving said cleavable linker thereby releasing the sugar, wherein this step may be performed subsequent to step v, vi, vii, viii or ix. 36.The method as clalmed in any of the preceding clalms, wherein the linker is attached to said solid support via a spacer. 37.The method as clalmed in clalm 36, wherein the spacer is in the range of 0 to 1000 atoms long and optionally branched. 38.The method as clalmed in any of the preceding clalms, wherein the solid support is selected from the group consisting of polymers, solids, insoluble particles and surfaces. 39.The method as clalmed in any of the preceding clalms 1 to 37, wherein the solid support is a sensor. 40.The method as clalmed in any of the preceding clalms, wherein the method comprises the step of contacting the sugar with one or more glycosidases, thereby generating a new reducing sugar, provided that the first sugar is a substrate for said glycosidase(s). 41.The method as clalmed in clalm 40, wherein the method comprises the step of immobilising newly generated reducing sugars on a solid support. 42.The method as clalmed in any of the preceding clalms, wherein the method comprises the step of contacting the sugar with one or more enzymes selected from the classes of glycosyltransferases, sulfatases, phophorylases, sulfotransferases, phosphotransferases, glycosynthases and transglycosidases, thereby converting said sugar into a new structure. 43.The method as clalmed in any of the clalms 40 to 42, comprising detecting newly generated sugars or structures. 44.The method as clalmed in any of the preceding clalms, wherein the reducing agent is a borane or borohydride comprising a BH bond or a silane comprising a SiH bond. ABSTRACT Title : SOLID-PHASE OLIGOSACCHARIDE TAGGlNG: A TECHNIQUE FOR MANIPULATION OF IMMOBILIZED CARBOHYDRATES The invention relates to methods of manipulating immobilized carbohydrates by derivatisation. Depending on the nature of the derivatisation, the carbohydrate may thereby be more easily detected and/or identified or handled. In particular, the ivention relates to methods of preparing a reactive sugar comprising the steps of: i) providing a sample comprising a reducing sugar; (ii) providing a solid support covalently attached to a linker comprising a capture group comprising an - NH2 group, wherein said linker optionally is attached to said solid support via a spacer; iii) reacting said reducing sugar with said -NH2 group, thereby obtaining an immobilized sugar; iv) reacting free -NH2 groups with a capping agent, wherein the capping agent com-prises a reactive group capable of reacting with an -NH2 group; and v) reducing C=N bonds with a reducing agent, thereby obtaining an reactive sugar of the struc-ture SugarCHn- NH-linked to a solid support via linker and optionally a spacer, wherein n is 1 or 2.

Full Text

Solid-Phase Oligosaccharide Tagging: A technique for manipulation of immo-
bilized carbohydrates.
All patent and non-patent references cited herein are hereby incorporated by refer-
ence.
Field of invention
The present invention relates to the field of carbohydrate manipulation. In particular,
the invention relates to methods of manipulating immobilised carbohydrates by deri-
vatisation. Depending on the nature of the derivatisation, the carbohydrate may
thereby be more easily detected and/or identified or handled. Thus, in one aspect
the invention relates to the field of carbohydrate detection and identification.
Background of the invention
Carbohydrates exist in many forms in nature. In animals including man, examples
include free reducing sugars in solution (such as the monosaccharide glucose in
serum), free oligosaccharides in solution (such as the disaccharide lactose in milk),
they can be attached to peptides or proteins through covalent linkages to a variety of
amino acids (such as asparagine, serine, threonine and others), covalently attached
to lipids such as ceramide (as in gangliosides) or attached to membrane anchors via
phosphatidylinositols. Sugars are also found attached to many small molecules in-
cluding some involved in metabolism, such as glucuronides. In the above examples,
the length of the sugar chains can vary from one to over 100 sugar residues.
In lower organisms, including bacteria and plants, an even wider array of structures
exists. The surface of bacterial cells can be covered by sugar polymers that are
thousands of residues long, which can act as antigens in the detection of bacteria
and as vaccines. Sugars are an integral part of bacterial cell walls. The sugars can
themselves be antibiotics (such as the aminoglycoside antibiotics, for example
streptomycin), or can be found as essential components of antibiotics (such as

erythromycin and vancomycin), as enzyme inhibitors (as in Acarbose) or as anti-
cancer agents (such as for example calicheamycin).
One area of particular interest is the structure of the carbohydrate chains (glycans)
found attached to glycoproteins and glycoiipids. The glycosylation pattern of glyco-
proteins has been shown to be important for their biologlcal functions, including their
bioavailablity, their targeting, and have even been directly correlated with the metas-
tatic potential of tumor cells. The glycosylation pattern of human serum transferrin,
for example, is being used as a diagnostic test for a series of genetic diseases
termed Carbohydrate-Deficient Glycosylation Syndromes. Specific glycolipid se-
quences have been shown to be involved in neuronal development and cell surface
signalling, in diabetes, and are accumulated in certain specific metabolic diseases
such as Tay-Sachs, for which they are diagnostic.
The linkages between the sugar residues in the oligosaccharides and polysaccha-
rides described above can have either the alpha or beta configurations, and the gly-
cans can be multiply branched. The diversity of structures possible for glycan chains
is therefore enormous and their structural characterization is therefore inherently
complex. There is therefore a strong interest in methods for the detection, structural
characterization, identification, quantitation, and chemical/enzymatic manipulation of
carbohydrate and glycan structures, in research, in diagnostics, in monitoring the
glycosylation of recombinant glycoproteins and in the development of new pharma-
ceutical agents.
Several methods are in current use for the analysis for carbohydrate structures, and
these have recently been reviewed. Underivatized oligosaccharides and glycoiipids
can be analyzed by NMR-spectroscopy, by mass-spectrometry, and by chromatog-
raphy. For the much larger glycoproteins, mass spectrometry provides more limited
information but analysis of their proteolytic digests, i.e. glycopeptides, has been ex-
tensively used. Indirect structural information about underivatized oligosaccharides
can also be deduced from their abilities to interact with carbohydrate-binding pro-
teins such as lectins, antibodies or enzymes.
Carbohydrates themselves have no characteristic chromophores, only N-acetyl
groups, so monitoring their separation by optical or spectroscopic detection is not

commonly used. Pulsed amperometric detection of the polyols has however been an
important technique for detection in chromatography.
The most widely used method for high-sensitivity detection of carbohydrates has
been the labeling of the reducing ends (lactols, tautomers of hydroxyaidehydes and
hydroxyketones) with either radioactive or fluorescent TAGs. Both chemical and
enzymatic methods have been described that cleave carbohydrates from glycopro-
teins and glycolipids, permitting the generation of the required reducing sugars from
glycoproteins, glycolipds and other glycoconjugates. Most commonly, such reducing
sugars are reacted with amino-containing derivatives of fluorescent molecules under
conditions of reductive amination: i.e., where the initially formed imines (C=N) are
reduced to amines (CH-NH) to produce a stable linkage. In most cases, the labeling
reactions have been performed in solution using a large excess of labeling agent.
This requires separation of the excess labeling agent and its by-products prior to or
during analysis. Other TAGs of utility in mass-spectrometry have been added in the
same manner, by either amination or reductive amination, the detection then being
performed by the mass-spectrometer.
Once the label has been added to permit specific detection, the carbohydrates de-
scribed above can subsequently be subjected to separation and detec-
tion/quantification. Additional structural information can be obtained by exposing the
tagged carbohydrates to enzymes such as glycosidases. If specific glycosidases act
on the tagged carbohydrates, they can cleave one or more sugar residues resulting
in a change in chromatographic or electrophoretic mobility, as detected by, for ex-
ample, a fluorescence detector in HPLC, CE or by a change in their mobility in SDS-
PAGE, or a change in their mass as detected by a change in m/z value in a mass-
spectrometer. Arrays of enzymes have been used to provide a higher throughput
analysis.
Below a short overview of prior art is glven:
Gao et al. 2003 reviews suitable techniques for derivatisation of carbohydrates in
solution. In solution carbohydrates may be derivatised by reductive amination. In
general, -NH2 groups of amines may react with aidehyde or ketone group of reduc-
ing sugars, thereby producing compounds of -C=N structure. Such compounds may

further be reduced for example by NaCNBH3. Gao et al., 2003 does not disclose
manipulation of immobilised carbohydrates.
US5,100,778 describes a method for oligosaccharide sequencing comprising plac-
ing an identifylng label on the reducing terminal residue of an oligosaccharide, divid-
ing into a plurality of separate portions, treating each portion with for example spe-
cific glycosidases, pooling product and analysing the pools obtained. The document
does not describe immobilised oligosaccharides.
US4,419,444 describes methods for chemically binding organic compounds contain-
ing carbohydrate residues to a support bearing reactive -NH2 groups. The methods
involve either the periodate oxidation of carbohydrate diols to produce reactive aide-
hydes by cleaving of C-C bonds in the carbohydrate or oxidation of -CH2OH groups
to -CHO groups enzymatically. Both oxidations will result in alteration of the struc-
ture of the carbohydrate. The reactive aidehydes can be immobilised by reaction
with the -NH2 groups. After immobilisation of the carbohydrate containing com-
pound a reduction step (for example using NaBH4) may be performed to increase
stability. The document describes neither the immobilization of a reducing sugar
through its reducing end nor manipulation of immobilised altered carbohydrate con-
taining compounds via the reduced amine bond. Furthermore, the chemical nature
of the carbohydrate has been altered and this alteration may impair further modula-
tions, such as specific enzymatic cleavage by glycosidases. The document also
does not describe the addition of any chemical reagents to the immobilised oligo-
saccharide that result in the addition of molecular structures to it.
W092/719974 describes a method of sequencing oligosaccharides. The method
involves immobilising oligosaccharides on a solid support and subsequent treatment
with a variety of glycosidases. Prior to immoblisation, the oligosaccharide may be
linked to a conjugate. The document does not describe modulation of immobilised
oligosaccharides other than glycosidase treatment.
The above describes the biologlcal importance and complexity of glycans, and
summarizes some benefits of attaching TAGs to reducing sugars, such as mono-
saccharides, as well as to the reducing sugar end of oligosaccharides. To date, such
attachment has been performed in solution using large excesses of tagglng agent

(and often additional chemical agents such as reducing agents), and thus require
time consuming and frequently difficult separation techniques to be applied before
either detection or further manipulation. Such separation techniques invariably result
in losses of material, and dilution, thus considerably complicating and biasing the
analysis. There is therefore a great need for simple methods that can install a TAG
onto a carbohydrate structure and further manipulate the structure, without the need
for complex and biased methods for separating reaction starting materials, reagents,
by-products and sought after products. We describe herein such simple methods.
Summary of the invention
The present invention relates to methods of covalent attachment of reducing sugars,
(which may be any of the reducing sugars mentioned herein below in the section
"Reducing sugar") to a solid-support (which may be any of the solid supports de-
scribed herein below in the section "Solid support") through reaction with an immobi-
lized molecule consisting of an optional spacer (i.e. with or without spacer) and a
linker (which can be cleavable) that incorporates a capture group containing an -NH2
functionality. The resulting immobilized sugar has an acyclic form with a C=N bond,
which may be in equilibrium with it's cyclic glycosylamine tautomer.
Free -NH2 groups on the solid support after immobilisation may be capped and the
C=N bond can be reduced. This method is outlined in fig. 1 A+B^E. The figure
shows an underivatised pyranose, which however is meant to represent any reduc-
ing sugar.
In a variation, the methods of the invention may comprise reduction of the immobi-
lized sugar containing a C=N bond (exemplified by structure C, fig. 1) to CH-NH prior
to capping free -NH2 groups, producing a compound of structure Cred (fig. 1). The -
NH2 groups in Cred may then be capped at this stage to produce a compound of the
same structure E as that produced by the sequence C to D to E described above
and shown in fig. 1.
Compounds of the structure E may thus be produced by either the sequence A+B
goes to C goes to D goes to E, or A+B goes to C goes to Cred goes to E.

It is therefore an object of the present invention to provide methods of preparing a
reactive sugar, said method comprising the steps of
i. Providing a sample comprising a reducing sugar (such as A in fig. 1)
ii. Providing a solid support (e.g. solid in fig. 1) covalently attached to a
linker comprising a capture group comprising an -NH2 group, wherein
said linker optionally is attached to said solid support via a spacer (such
as B in fig. 1)
iii. Reacting said reducing sugar with said -NH2 group, thereby obtaining
an immobilised sugar (such as C in fig. 1),
iv. Reacting free -NH2 groups with a capping agent, wherein the capping
agent comprises a reactive group capable of reacting with a -NH2 group
v. Reducing C=N bonds with a reducing agent
vi. thereby obtaining a reactive sugar containing the structure SugarCHn-
NH- linked to a solid support via a linker and optionally a spacer, wherein
n is 1 or 2 (such as compound E of fig. 1),
wherein steps iv and v may be performed in any order.
In embodiments of the invention wherein step iv is performed prior to step v, capping
-NH2 groups in step iv will for example result in compound D of fig. 1, whereas the
reduction performed in step v will for example result in compound E of fig. 1;
In embodiments of the invention wherein step v is performed prior to step iv, then
the reduction of the C=N bond (for example of compound C of fig. 1) will for example
result in compound Cred of fig. 1. The capping of the -NH2 groups in step iv will for
example produce the compounds of structure E, fig.1. It is comprised within the pre-
sent invention that the sample comprising the reducing sugar may be incubated with
the solid support and the reducing agent simultaneously. Thus, reduction of C=N
bonds (step v) will be performed immediately following reaction of the reducing
sugar with the -NH2 group of the solid support (step iii).

In step iii), preferably, the reducing end of said reducing sugar is reacted with said -
NH2 group. Thus preferably the aidehyde group or the hemiacetal of the reducing
sugar is reacted with the -NH2 group.
it is preferred that the methods further comprise the step of
vii. Reacting the -NH- group of the reactive sugar (for example com-
pound E of fig. 1) with a derivatising agent comprising a nitrogen-
reactive functional group (X), thereby obtaining a sugar covalently at-
tached to said agent. Said sugar covalently attached to said agent may
for example be compound F of fig. 1 (when the derivatising agent is a
TAG) or compound H of fig.1, when the derivatising agent is a tether
linked to functional group.
The term "TAG" in the present context, and in fig. 1 (vide infra) is meant to indicate
any atom, molecule or entity that can become covalently attached to another mole-
cule thereby labelling said another molecule as having undergone the covalent at-
tachment.
Brief Description of the drawings
Fig. 1 illustrates an example of the method according to the invention. Fig. 1: A-E
illustrates capture and manipulation of a reducing sugar on a solid support to glve a
reactive sugar E. Fig. 1: E-G and J illustrates manipulation of a reactive sugar E on
a solid support, and cleavage of a tagged sugar. The methods of the invention may
comprise one or more of the steps illustrated in the fig. 1. In the fig. 1 the reducing
sugar is exemplified with a pyranose, however any reducing sugar may be used with
the method. The figure shows an example where the linker is linked to the solid sup-
port via a spacer, however, the linker may also be directly linked to the solid support.
The solid support is designated "Solid" in the figure, however it may be any of the
solid supports mentioned herein below.

Fig. 2. Structures 1 -10 of the reducing sugars, and mixtures thereof, used in the
examples of the present invention.
Fig. 3. Synthesis of a linker (14) and structure of a spacer (15).
Fig. 4. Solution-phase synthesis of the TMR-tagged D-galactose derivative, GalCH2-
N(R)-TMR (21), and description of nomenclature used for monosaccharide stan-
dards.
Fig. 5. Structures 21 - 28 of synthetic tagged derivatives of the eight common
mammalian monosoaccharides of general structure SugarCH2-N(R)-TMR.
Fig. 6. Structures of the four solid supports Bp, B°, B1 and B2.
Fig. 7. Structures of some capping agents.
Fig. 8. Structures of some nitrogen-reactive tagglng agents used, of general struc-
ture TAG-X
Fig. 9. Example of E goes to J (30) using the protected nitrogen-reactive agent 29 of
general structure X-tether-YP.
Fig. 10. Separation by CE of the eight TMR-labelled monosaccharide standards
shown in Fig. 5. The order of elution is GainAc (27), Xyl (24), Man (23), Glc (22),
GlcNAc (26), Fuc (25), Gal (21), and glcA (28). The top trace is an expansion.
Fig. 11. CE of Gp3 (with LacNAc as the reducing sugar tagged using TRITC, section
4.2.1).

Fig. 12. Eiectrospray mass-spectrum in the negative ion mode of Gp5 (with lacto-N-
tetraose as the reducing sugar tagged using 4-bromophenylisothiocyanate, section
4.2.2). The inset is an expansion showing the two peaks corresponding to the major
isotopes of Br.
Fig. 13. CE of Gp6a (with monosaccharide mixture 6 tagged using TRITC, section
4.2.3). X denotes unidentified peaks. The order of elution is GainAc (27), Man (23)
and Fuc (25). The lower trace is an expansion.
Fig. 14. CE of Gp7a (with monosaccharide mixture 7 tagged using TRITC, section
4.2.4). X denotes unidentified peaks. The order of elution is GainAc (27), Man (23)
and Fuc (25). The lower trace is an expansion.
Fig. 15. CE of Gp9 (with the oligosaccharide mixture 9 tagged using FITC, section
4.2.5). The order of elution is G7 to G2 (Fig. 2).
Fig. 16. CE of Gp10 (ribonuclease B oligosaccharides 10 tagged using FITC, section
4.2.6).
Fig. 17. CE of G12 (with Gal 2 as the reducing sugar tagged using TRITC, section
4.3.1).
Fig. 18. CE of G15 (with LNT 5 as the reducing sugar tagged using TRITC, section
4.3.2).
Fig. 19. CE of G18 (with 8 as the reducing sugar mixture tagged using TRITC, sec-
tion 4.3.3). The order of elution is LNT followed by Gal.
Fig. 20. CE of the cleaved products G°5 (A), G15 (B) and G25 (C) after beta-

galactosidase digestion of immobilized LNT (5), section 5.1.1). The TRITC-labelled
LNT tetrasaccharide elutes first near 36 minutes. Loss of galactose ylelds the trisac-
charide product eluting after 38 minutes.
Fig. 21. CE of the cleaved product before (trace A) and after (trace B) incubation of
F24 (maltotriose (G3) as the reducing sugar tagged using TRITC) with glucoamy-
lase, section 5.1.2). A reference sample of tagged Glc (22, Fig. 5) was added to the
sample prior to recording trace A.
Fig. 22. CE of the cleaved products obtained after beta-galactosidase treatment of
C25 (bearing LNT and free NH2 groups), followed by capture of the released galac-
tose, reduction and tagglng using TRITC, section 5.2. The order of elution is LNT,
the trisaccharide resulting from loss of galactose and galactose (21).
Fig. 23. CE analysis of the cleaved products derived from C22 (immobilized galac-
tose) after capping with various agents, reduction and labelling using TRITC, section
6.1). The capping agents were A (acetic anhydride), B (benzoic anhydride), C (tri-
chloroacetic anhydride) and D (dibromoxylene). Tagged galactose (21) elutes near
17 minutes in all traces.
Fig. 24. CE of the cleaved product obtained from processing galactose through the
sequence C->Cred->G, section 6.2). The galactose 21 elutes at 17 minutes.
Detalled description of the invention
Methods of manipulating a reducing sugar.
The present invention relates to methods of manipulating a reducing sugar. An ex-
ample of the methods of the invention is outlined in fig. 1. It should be noted that the
methods of the invention do not necessarily involve all of the steps illustrated in fig.
1. Thus the methods may comprise only some of the steps outlined in fig. 1. Pref-

erably, the methods will comprise at least the steps A+B—>C, C->D and D->E, or the
steps A+B->C, C—>Cred and Cred->E In fig, 1 the reducing sugar is exemplified by a
pyranose, however any reducing sugar may be used with the invention, in particular
any of the reducing sugars described herein below in the section "Reducing sugar".
The -OH group dissecting the pyranose ring in fig. 1 is meant to indicate that the
reducing sugar may bear one or more hydroxyl groups attached to it.
Each of the steps of the methods of the invention are described herein below in
more detall, wherein capital letters A to J and Cred refer to fig. 1
The identity of each of the compounds or intermediates of the present invention, for
example of compounds A, B, C, Cred D, E, F, G, H, I or J may be verified by stan-
dard techniques known to the skilled person, such as by NMR.
A. Reducing sugar
The term "reducing sugar" as used herein covers the classical definition of sugars
that are capable of reducing Cu2+ to Cu+. Whether a sugar is reducing may for ex-
ample be tested using Fehlings reagent. In more modem terminology, reducing
sugars are sugars that comprise an aidehyde group or a hemiacetal of the formula
R2C(OH)OR', wherein R' is not H. Preferably, a reducing sugar is a carbohydrate
structure containing an aidehyde, which is in equilibrium with the cyclized form
called a hemiacetal. D-glucose is a non-iimiting example of such a reducing sugar.
The most abundant cyclic forms contain 5-membered rings, termed furanoses, and
6-membered rings termed pyranoses. (See rules of nomenclature).
The term "sugar" as used herein covers monosaccharides, oligosaccharides, poly-
saccharides, as well as compounds comprising monosaccharide, oligosaccharide,
or polysaccharide. The terms "carbohydrate" and "sugar" are herein used inter-
changeably.

Oligosaccharides and polysaccharides are compounds consisting of monosaccha-
rides linked glycosidically. in general polysaccharides comprise at least 10 mono-
saccharide residues, whereas oligosaccharides in general comprise in the range of
2 to 10 monosaccharides. Oligosaccharides and polysaccharides may be linear or
branched. A monosaccharide is defined as a polyhydroxy aidehyde H-(CHOH)n-
CHO or polyhydroxyketone H-(CHOH)n-CO-(CHOH)m-H, wherein m and n are inte-
gers. Preferred monosaccharides comprises in the range of 4 to 9 carbons, thus
preferably for polyhydroxy aidehydes n is an integer in the range of 3 to 8 and for
polyhydroxyketones n+m is an integer in the range of 3 to 8. Monosaccharides are
compounds such as aidoses and ketoses and a wide variety of derivatives thereof.
Derivation includes those obtained by oxidation, deoxygenation, replacement of one
or more hydroxyl groups by preferably a hydrogen atom, an amino group or thiol
group, as well as alkylation, acylation, sulfation or phosphorylation of hydroxy
groups or amino groups. According to IUPAC nomenclature, carbohydrates are
compounds of the stoichiometric formula Cn(H2O)n, such as aidoses and ketoses as
well as substances derived from monosaccharides by reduction of the carbonyl
group (aiditols), by oxidation of one or more terminal groups to carboxylic acids, or
by replacement of one or more hydroxyl group(s) by a hydrogen atom, an amino
group, thiol group or similar groups or derivatives of these compounds.
In a preferred embodiment, the reducing sugar is a naturally occurring reducing
sugar or a reducing sugar, which has been liberated from a naturally occurring or
recombinantly produced compound comprising a carbohydrate, preferably without
having been subject to furthermore modifications after liberation. In particular it is
preferred that the reducing sugar, is a naturally occurring reducing sugar or a reduc-
ing sugar liberated from a naturally occurring or recombinantly produced compound,
wherein none of the alcohol groups of said naturally occurring sugar or said liber-
ated sugar have been enzymatically transformed to an aidehyde or ketone by oxida-
tion at the level of the oligosaccharide. It is also preferred that the reducing sugar, is
a naturally occurring reducing sugar or a reducing sugar liberated from a naturally
occurring or recombinantly produced compound, wherein said naturally occurring
sugar or said liberated sugar have not been subjected to periodate treatment. It is
thus generally preferred that no alcohol group of said naturally occurring sugar or
said liberated sugar have been transformed to an aidehyde or ketone. In this context

recombinantly produced compounds are compounds produced by a living organism
with the aid of recombinant technologles, for example heterologous glycoproteins.
Reducing sugars may be derived from a variety of sources. For example the reduc-
ing sugar may be obtained from a living organism or part of a living organism, such
as animals or plants or from one or more specific animal or plant tissues, from or-
ganisms such as prokaryotic or eukaryotic cells, from viruses, from in vitro culti-
vated mammalian cells, insect cells, plant cells, fungl, bacterial cells, yeast, or
phages. For example the reducing sugar may be isolated from extracts of any of the
aforementioned cells, microbial organisms or living organisms. Such extracts may
comprise reducing sugars, such as free carbohydrates. Extracts may also comprise
compounds comprising monosaccharide, oligosaccharide, polysaccharide or carbo-
hydrate moieties, notably glycoproteins or glycolipids or small organic molecules to
which carbohydrates are attached, which are generally referred to as glycosides.
Glycoproteins are compounds in which a carbohydrate component is linked to a
peptide, polypeptide or protein component. Thus as used herein the term glycopro-
tein also cover proteoglycans and glycosaminoglycans. Glycolipids are compounds
containing one or more monosaccharide, oligosaccharide, polysaccharide or carbo-
hydrate moieties bound by a glycosidic linkage to a hydrophobic moiety such as an
acylglycerol, a sphingoid, a ceramide (W-acylsphingoid) or a prenyl phosphate. Gly-
cosides are meant to describe small (MWt 100 - 5000) organic molecule glycosidi-
cally linked to one or more sugars via elther O, N or S.
Reducing sugars may also be the products of chemical synthesis, or chemi-
cal/enzymatic synthesis, such as oligosaccharides prepared in vitro by chemical
synthesis in solution or on the solid phase. These same synthetic oligosaccharides
may be further modified by enzymatic reaction, such as for example by the sulfation,
phosphorylation or glycosylation. Thus the methods described herein may also be
used for manipulation of synthetic or semi-synthetic oligosaccharides or oligosac-
charide libraries.

Preferably, the monosaccharide, oligosaccharide, polysaccharide or carbohydrate
moiety is liberated from the glycoprotein, prior to performing the methods of the in-
vention. This may be done by standard methods known to the skilled person, N-
linked monosaccharides, oligosaccharides, polysaccharides or carbohydrates may
be cleaved from glycoproteins by chemical or enzymatic methods. Enzymatic
methods may for example involve use of glycosidases such as endoglycosidases H
and F or N-glycanases such as PNGase-F.O-linked monosaccharides, oligosac-
charides, polysaccharides or carbohydrates may be cleaved from glycoproteins by
chemical methods, including hydrazinolysis or alkaline β-elimination or enzymatically
using enzymes such as an O-glycosidase. Chemical methods useful for release of
both N-linked and O-linked includes reactions with strong nucleophiles and/or strong
bases such as hydrazine. Carbohydrates may be cleaved from small organic mole-
cules using elther acidic or basic reactions, or by the action of glycosidases.
In one embodiment of the invention a predetermined amount of a reference stan-
dard is added to the sample comprising the reducing sugar. This may facilitate
quantification of said reducing sugar after immobilisation or after immobilisation and
release in embodiments of the invention wherein the linker is cleavable.
The reference standard may be any compound capable of reacting with -NH2, for
example any compound comprising one of the nitrogen reactive functional groups
described herein below in the section "E->F. Adding TAGs". Preferably the refer-
ence standard is an aidehyde or a ketone, more preferably a sugar. In another em-
bodiment of the invention, the same or different reference standard is added to the
solid support prior to contact with the solution containing the reducing sugar with or
without the added reference standard included in the solution (see herein below in
section "B. Solid support"). Thus two or more reference standards may be used, one
(or more) added to the solid support prior to contact of the solid support with the
solution comprising a reducing sugar, and one or more added to the solution con-
taining the reducing sugar.
One or more reference standards may also be added to to the solid support after
contact with the reducing sugar, but preferably prior to capping. Thus for example
the reference standard may be added to compound C or Cred of fig. 1, preferably
after a washing step.

In embodiments of the invention wherein the solid support is coupled to a reference
standard (see herein below in section "B. Solid support") it is preferred that different
reference standards are used.
In one embodiment of the invention the methods comprises a step of pre-treatment
of the sample to be used with the method. In particular, a sample comprising glyco-
sidically-linked sugars such as a glycoproteins, glycolipids or glycosides may be
pretreated with a scavenger resin prior to reaction with the solid support. The scav-
enger resin is preferably a resin comprising a nucleophilic group capable of reacting
with aidehydes and ketones, including reducing sugars, preferably the scavenger
resin comprises an amino group or a hydrazine. Incubation of the sample with the
scavenger resin will thus remove additional aidehydes, ketones and reducing sug-
ars. After pre-treatment, such methods will in general further comprise the step of
liberating reducing sugars from said glycosidically-linked sugars thereby obtaining a
sample comprising reducing sugars. The vast majority of aidehydes and ketone
within said sample will thus be reducing sugars released from glycosidically-linked
sugars. Said reducing sugars may be liberated by a number of methods, including
chemical or enzymatic methods, such as any of the methods described herein
above in this section. Treatment of the pretreated sample with for example
PNGaseF can cause the release of reducing oligosaccharides into solution for cap-
ture and manipulation according to the methods of the invention. The oligosaccha-
rides thus released will be essentially free of contaminating carbonyl compounds.
Release of reducing carbohydrates may also be effected by other enzymes, such as
glycosidases, or using chemical reactions, after scavenglng of contaminating car-
bonyl compounds as described above.
B. Solid support
The methods according to the present invention involve immobilisation of a reducing
sugar to a solid support. Solid phase chemistry offers a number of advantages, such
as easy handling, purification and concentration of immobiiised compounds. How-
ever, not all reactions doable in solution can be performed on solid phases. The
attachment to a solid support practically confer infinite size to each molecular entity.

This has the effect that the molecule reacts much more slowly in a bimolecular reac-
tion than the same molecule would do in solution. Some reactions that may be car-
ried out in solution with an acceptable yleld simply will not perform on solid support.
The term "solid support" as used herein covers physical solids as well as insoluble
polymers, insoluble particles, surfaces, membranes and resins, preferably the solid
support is an insoluble polymer, an insoluble particle, a surface or a resin.
Thus the "solid support" may be an insoluble inorganic matrix (such as glass), an
insoluble polymer (such as a plastic, for example polystyrene), an insoluble matrix
consisting of parts of both organic and inorganic components (e.g. some hybrid
silicates, such as compounds of the structure R-Si-O-), organic polymers in common
use in solid-phase synthesis (polystyrenes, PEGA resins, PEG resins, SPOCC res-
ins and hybrids thereof), polyethylene glycol chains (which can be soluble in certain
organic solvents and made insoluble by the addition of other solvents). The solid
may also be a metal (such as gold), an alloy, or a composite such as for example
indium-tin oxide or mica.
Any of the above listed solid supports may additionally be coated with agents that
have an affinity for carbohydrates, such as but not limited to aryl boronates or poly-
mers thereof. Such coatings can increase the concentration of carbohydrate at the
surface of the solid support, enhancing the rate and yleld of capture.
Organic polymers used in solid-phase synthesis for example includes
TentaGel (commercially available from Rapp polymere, Tubingen, Germany), Ar-
goGel (commercially available from Argonaut Technologles Inc., San Carlos, CA),
PEGA (commercially available from Polymer Laboratories, Amherst, MA), POEPOP
(Renil et al., 1996, Tetrahedron Lett., 37; 6185-88; available from Versamatrix, Co-
penhagen, Denmark) and SPOCC (Rademann et al, 1999, J. Am, Chem. Soc., 121:
5459-66; available from Versamatrix, Copenhagen, Denmark).
In one embodiment of the invention the solid support is a sensor, such as a surface
acoustic wave sensor (such as any of the sensors described in Samoyolov et al.
2002, J. Molec. Recognit. 15:197-203) or a surface plasmon resonance sensor
(such as any of the sensors reviewed by Homola et at., 1999, Sensors and Actua-

tors B, 54: 3-15). Such solid supports may be inorganic materials such as glass,
metals such as gold, organic polymeric materials or hybrids thereof and may be
covered various coatings such as proteins or polysaccharides, oligomers such as as
dendrimers or polymers such as polyacrylamide or polyethylene glycol.
In a preferred embodiment the solid support is glass or PEGA resins.
In one embodiment of the present invention the solid support is coupled to a refer-
ence standard, which may facilitate quantification of immobilised reducing sugar. In
particular, it is preferred that said reference standard is attached to the solid support
(elther directly or indirectly) by a cleavable linker, which could facilitate quantification
of immobilised and released reducing sugar. In embodiments of the invention
wherein the reducing sugar is immobilised to the solid support via a cleavable linker,
it is preferred that the reference standard is immobilised to the solid support via an
identical or similar cleavable linker.
The reference standard may be any detectable compound, for example the refer-
ence standard may or may not be a sugar, preferably however it is carbohydrate.
The amount of reference standard may vary, in general the solid support may com-
prise in the range of 20 to 500, preferably in the range of 50 to 200, such as in the
range of 90 to 110 -NH2 groups per reference standard.
B. Spacer
According to the present invention the solid support is optionally coupled to a linker
via a spacer. However, it is also comprised within the present invention that the solid
support is directly coupled to the linker.
A spacer is a chemical entity in the range of 1 to 1000 atoms long. Preferably, said
spacer is a linear or branched chain and/or a ring structure. The nature of the spacer
may be hydrophobic or hydrophilic or have a mixture of these two properties. The
group of spacers comprises molecules in common use in solid phase synthesis and
on-bead, in-well or on-slide assays involving the detection of molecules attached via
spacers to solid-supports. The skilled person will readily be able to identify a useful
spacer for a glven solid support.

The spacer is preferably an alkyl chain (more preferably a C1 to C1000 alkyl chain),
which optionally may be branched, wherein said alkyl chain optionally is substituted
at one or more positions by groups containing one or more of B, O, N, S, P, Si, F,
CI, Br or I. The spacer may also comprise one or more aryl residues which optionally
may be branched or substituted in the same manner. In one preferred embodiment,
the spacer is selected from the group consisting of amides and ethers. Thus the
spacer may essentially consist of a chain containing one or more amide bonds (-
CONH-), one more ethylene glycol units (-CH2-CH2-O-), or combinations of these
units with the alkyl or aryl chains.
In one embodiment of the invention, the spacer preferably does not comprise elther
a primary or a secondary amine. In another embodiment of the invention any amines
comprised within the spacer are capped.
B. Linker
The present invention relates to capture of reducing sugars onto solid supports co-
valently attached to a linker comprising a capture group. The linker serves to link the
capture group, terminating in -NH2, to the solid support optionally through a spacer.
The linker may be any of a large variety of linkers such as those in common use in
solid-phase organic synthesis.
The linker may elther be a non-cleavable linker or a cleavable linker.
Non-cleavable linkers may for example be alkyl, aryl, ethers or amides, wherein any
of the aforementioned may optionally be substituted. For example any of the afore-
mentioned may be substituted with heteroatoms or they may contain, 0-alkyl,alkyl,
aryl or heteroatoms as branches. In one example the linker comprises or essentially
consists of PEG and/or polyamide.
The linker may comprise a site where a reaction can be made to occur to sever the
part containing the capture group (including the molecules it has captured and which
have been optionally further modified) from the spacer and the solid support. Such
linkers are referred to as cleavable linkers, and are in wide use in solid phase or-

ganic synthesis. Examples of cieavable linkers are known where the cleavage can
be effected by electrophiles, nucleophiles, oxidizing agents, reducing agents, free
radicals, acid, base, light, heat or enzymes.
Cieavable linkers may for example be acid labile (for example, the Rink amide as
described in Rink, 1987, Tetrahedron) Lett., 28: 387 and traceless silyl linkers as
described in Plunkett et at., 1995, J. Org. Chew., 60: 6006-7), base labile (for exam-
ple, HMBA as described in Atherton et al. 1981, J. Chem. Soc. Perkin Trans, 1:
538), or photolabile (for example, 2-nitrobenzyl type as described in Homles et al.,
1995, J. Org. Chem., 60: 2318-2319). The linkers may be more specific and restric-
tive of the type of chemistry performed, such as silyl linkers (for example, those
cleaved with fluoride as described in Boehm et al., 1996, J. Org. Chem., 62: 6498-
99), allyl linkers (for example, Kunz et al., 1988, Angew. Chem. Int. Ed. Engl., 27:
711-713), and the safety catch sulfonamide linker (for example, as described in
Kenner et al., 1971, Chem. Commun., 12: 636-7). Enzyme cieavable linkers may for
example be any of the enzyme cieavable linkers described in Reents et al., 2002,
Drug Discov. Today, 7: 71-76, or any functionalised derivatives of the enzyme-labile
protecting groups described in the review by Waidmann et al., 2001, Chem. Rev.
101: 3367-3396. Heat labile linkers may for example be of the type described in
Meng et al., 2004, Angew. Chem. Int. Ed., 43: 1255-1260.
B. Capture group
According to the present invention the linker comprises a capture group, wherein the
capture group comprises at least one -NH2 group. In a favourable format, the cap-
ture group terminates in an -NH2 group that is attached to the linker through an op-
tional group R. Thus the capture group preferably is of the structure R-NH2. R may
be a simple alkyl, aryl or substituted alkyl or aryl group. Preferably, R should contain
a heteroatom directly attached to the -NH2 group, to produce structures of the type
linker-M-NH2, wherein M is a heteroatom (i.e. not carbon), preferably M is selected
from the group consisting of N, O and S. Especially favourable are compounds
where M is a heteroatom, such as in the structures linker-O-NH2 linker-NH-NH2,
linker-CO-NH-NH2, linker-NH-CO-NH-NH2, linker-S(O)2NH-NH2 and Iinker-S-NH2.

A+B—>C, Methods of capture
The capture of the reducing sugar is done by reacting the -NH2 group of the capture
group with the reducing end of said reducing sugar, i.e. with the aidehyde or he-
miacetal group. The reaction can occur at any pH values but is most favored in the
range of pH 2 - 9. The methods may involve the addition of one or more additives,
such as additives which may elther facilitate or favourably alter the equllibrium be-
tween the open chain aidehyde form of the reducing sugar and the hemiacetal form
of the reducing sugar (e.g. compound A, fig. 1), wherein the open chain aidehyde
form is preferred. The additive may for example be metal ions, boronates or sili-
cates. The capture produces a species attached to the solid support through a cova-
lent double bond (shown as C=N) where the C is derived from the sugar moiety and
N from the capture group. This immobilized sugar may also be in equllibrium with its
cyclic ring form, in particular if the reducing sugar was a pyranose, then the immobi-
lised sugar may be in equllibrium with its cyclic 6-membered ring form (see for ex-
ample compounds C and C of fig. 1), but it may also be in equllibrium with its 5-
membered ring form if the appropriate OH group on the sugar is unsubstituted.
The capture reaction may be performed in any useful solvent. A person of ordinary
skill in the art will readily be able to identify a useful solvent for any glven com-
pounds A and B. The solvent may for example be selected from the group consist-
ing of water, aqueous buffer, organic solvents and mixed aqueous and organic sol-
vents. The solvent may also be any of the aforementioned comprising one or more
additives such as acids, bases, salts, divalent metal cations, detergents, complex-
ing agents including inclusion-complex-forming molecules such as cyclodextrins or
calixarenes, chelating agents (for example EDTA), borates, boronates or silicates.
In a preferred embodiment the amount of solid support (compound B of fig. 1) added
to the reaction is adjusted so that a molar excess of capture groups are present in
relation to the reducing sugar, preferably said excess is large, such as at least 2
times, preferably at least 5 times, more preferably at least 10 times, such as at least
50 times, for example at least 100 times or more. This excess will ensure a more
efficient capture of the reducing sugar.

The capture reaction may be carried out at any temperature, but preferably at tem-
peratures in the range of 0 to 100°C.
C. Washing
Once the reducing sugar has been immobilised on the solid support through reac-
tion with the capture group (step A+B->C of fig. 1) the solid supports may be
washed to remove non-covalently bound material. Accordingly, if the reducing sugar
is provided in a solution comprising other compounds, in particular other compounds
that do not comprise -NH2 reactive groups, the reducing sugar may be purified from
said solution. It is thus comprised within the present invention that the reducing
sugar is provided in a non-purified form, such as in the form of a crude cellular ex-
tract or the like. It is also comprised that the reducing sugar may be produced from a
purified or partially purified glycoprotein, glycolipid or glycoside by the action of an
enzymes such as glycosidase or an amidase or through the cleavage of a glycosidic
bond by chemical reagents.
The skilled person will readily be able to identify sultable washing conditions for a
glven immoblised sugar (compound C, fig. 1). The washing may for example be
done with any of the above-mentioned solvents optionally comprising any of the
above-mentioned additives in addition to detergents and denaturing agents. The
washing my be performed at any temperature, but preferably at temperatures in the
range of 0-100°C.
C->D. Capping
The solid support coupled to the immobilised sugar (such as compound C of fig. 1)
still contains unreacted free -NH2 groups and can be subjected to unique manipula-
tions that increase the scope of its utility.
In one preferred embodiment of the invention, subsequent to immobilisation of the
reducing sugar, unreacted -NH2 groups are capped by a capping agent, such as an
acylating agents (e.g. acetic anhydride) or other nitrogen-reactive agents well known

in the art, under conditions where the C=N bond of C does not react. After capping
the solid support will no longer comprise any free amine groups, but only capped
nitrogen atoms (N(H)CAP) of very low reactivity towards electrophiles. The product
of the capping of compound C has for example the general structure D (see fig. 1)
containing an -R-N(H)CAP group, wherein the (H) may or may not be present de-
pending on the structure of the CAP group.
Thus if the C=N bond linking the sugar to the solid support is reduced to an -NH-, it
will be a formally SP3-hybridized nitrogen atom in the sequence R-NH-CH2-. Specific
reactions may thus be directed to this group allowing specific and stoichimetric reac-
tions at the reducing sugar.
Preferably the capping agent specifically reacts with the remaining -NH2 groups,
without substantially reacting with the C=N functionality. Such reagents are well
known in the art an include common acylating agents used for amid bond formation,
e.g. acetic anhydride, other alkanoic acid anhydrides, aromatic anhydrides (e.g.
benzoic anhydride), cyclic anhydrides (e.g. succinic anhydride, phthalic anhydride),
other active esters such as N-hydroxysuccinimide esters, pentafluorophenyl esters
and a variety of active esters in common use in amide bond formation including in
the solid phase synthesis of peptide bonds. The -NH2 groups may alternatively be
capped by adding the corresponding free acids and an in-situ activating agent such
as DCC, in common use in peptide-bond formation thereby creating an active ester
in situ. Other reagents known to be reactive towards -NH2 groups can be used, such
as alkyl isothiocyanates (R-NCS), aryl isothiocyantes (Ar-NCS), alkylating agents R-
L (where L is a leaving group typically from the series CI, Br, I, OS(O)2R' where R'
can be alkyl or aryl), Michael acceptors such as alpha-beta unsaturated carbonyl
compounds (CHR=CH-CO- where R can be H, alkyl or aryl or substituted alkyl or
aryl) or alpha-beta unsaturated sulfones (CHR=CHS(O)2R' or Ar where R can be H,
alkyl or aryl or substituted alkyl or aryl), sulfonating agents (such as RSO2CI) and
derivatives thereof. In a similar manner, the -NH2 groups can be capped by reaction
with active esters of carbonates of the general formual RO-C(O) L, where L is des-
ribed as above.

D->E. Reduction
In a preferred embodiment of the invention, the C=N bond linking the sugar to the
linker (for example compound D of fig. 1) is reduced using a reducing agent. The
C=N bond may be reduced by a variety of well known reducing agents, preferably
the reducing agent is capable of saturating the double bond while placing a hydro-
gen atom on the N.
Of special value are boranes or borohydrides comprising a BH bond, examples in-
clude NaBH4, NaCNBH3, and BH3 complexes such as BH3-pyridine, BH3-
dimethylsulfide or the like. Silanes with the structures R3SiH can also be used, such
as silanes comprising SiH bonds, as can hydrogen transfer agents such as diimides,
or homogeneous hydrogenation catalysts or hydrogenation catalysts comprising a
metal-H bond.
The reduction results in a reactive sugar containing the structure SugarCH-NH-
preferably linked to a solid support via a linker and optionally a spacer. In general, if
the reducing sugar was an aidehyde, then reduction will result in a compound of the
structure SugarCH2-NH-. If the reducing sugar was a ketone, then the reduction will
result in a compound of the structure SugarCH-NH-.
The products of the reduction are for example of the general structure E (fig. 1) con-
taining a formally SP3 hybridized N atom.
C-»Cred—>E
In another preferred implementation of the method, the order of the capping and
reduction steps is reversed. Reduction of the C=N bond in compound C (fig. 1) can
be effected by any of the reagents described in D=E above to produce a compound
of the structure Cred (fig. 1). The reduction may also be performed in situ, meaning
that a reducing agent (such as NaCNBH3) may be added to the solid support (e.g.
compound B) simultaneously with the reducing sugar so that the C=N bond is re-
duced as it forms producing also Cred. It is thus comprised within the present inven-
tion that the sample comprising the reducing sugar may be incubated with the solid

support and the reducing agent simultaneously. Thus, reduction of C=N bonds (step
v) will be performed immediately following reaction of the reducing sugar with the NH2 group of the solid support (step iii). The free -NH2 groups in Cred may then be
capped using any of the reagents described in C->D above under conditions that do
not cause reaction with the SugarCH-NH-moiety. In particular, in this embodiment of
the invention it is preferred that the capping agent preferentially reacts with primary
amino groups over secondary amino group. It is also preferred that reaction tem-
perature and time are adjusted to yleld preferential reaction with primary over sec-
ondary amino groups. Virtually all compounds that react with amino groups react
more qulckly with primary amino groups than with more substituted amino groups,
but this is especially the case when such compounds are sterically large, such as for
example active benzoyl esters, isopropanoic acid active-esters, pivaloyl active-
esters, Boc anhydride or Boc-azide and the like. Useful compounds and conditions
for preferential reaction with primary amino groups over secondary amino groups
are described in Greene et al. 1999, Protective Groups in Organic Synthesis, 3rd.
Ed., Chaper 7, pp. 503-653. Other very preferred capping agents are NHS-esters or
sterically hindered pentafluorophenyl (PFP) esters or tetrafluorophenyl (TFP) es-
ters.
E->F. Adding TAGs
Compound E, fig. 1, obtained by elther of the above routes, contains solids linked to
a capped nitrogen atom (N(H)CAP) of very low reactivity towards electrophiles and a
formally SP3-hybridized nitrogen atom in the sequence SugarCH2-NH-R. Reaction of
E with sultable nitrogen-reactive functional groups (preferably the nitrogen-reactive
functional group is a mild electrophile) therefore results in the exclusive, or near ex-
clusive, addition of the electrophile to the SP3 nitrogen atom effectively adding a
molecular structure, herein described as "TAG", or another derivatising agent onto
the nitrogen to which the sugar is attached. The product of the addition of a TAG is
shown as Fin fig. 1.
Throughout the description the term "nitrogen-reactive group" is used to describe
reactivity towards a formally SP3-hybridized nitrogen, such as in compounds of the
structure R-NH-R', for example amines, wherein R and R' independently are alkyl,

or aryl (optionally substituted) or compounds wherein R' has an heteroatom such as
O or N attached to the -NH- such as in hydroxylamine derivatives (R-NH-OR') or
hydrazine derivatives (R-NH-NH-R').
The identity of the derivatising agent (for example a TAG), i.e. the specific chemical
structure of the derivatising agent, may be selected by the user. For addition to the
SP3 nitrogen in E, the derivatising agent (for example the TAG) should itself com-
prise an nitrogen-reactive functional group designated "X" in fig. 1„ Preferably the
TAG should contain an electrophile, or be attached to an nitrogen-reactive functional
group X. Preferably the derivatising agent is of the general structure TAG-X (see fig.
1), wherein X is a nitrogen-reactive functional group. Preferably X is any mild elec-
trophile that is reactive with SP3 nitrogen atoms, but preferably mild electrophiles
that react poorly with the -OH groups present on the sugar. Such mild electrophiles
include isothiocyanates (TAG-NCS), active esters (TAG-C(O)-L) where L is a leav-
ing group commonly used in amide bond formation such as in the synthesis of pep-
tide bonds, carboxylic acids (TAG-COOH) which can be activated to active esters in
situ by methods commonly used in amide bond formation such as in the synthesis of
peptide bonds, alkylating agents (TAG-L) where L is a leaving group preferably but
not exclusively from the series CI, Br, I, OS(O)2R where R can be alkyl or aryl, TAGs
comprising Michael acceptors (typically containing the sequence -CR=CH-C(O)-) or
alpha-beta unsaturated sulfones (-CR=CH-S(O)2-) and derivatives of any of the
aformentionned, aidehydes or ketone that may react with the sugarCH2-NH-amino
group by reductive amination, or substituted haloaromatic groups where the aro-
matic ring bears electronegative groups such as nitro groups, for example as in the
Sanger reagent 1-fluoro-2,4-dinitrobenzene or the 4-halo-7-nitro-2-oxa-1,3-diazole
(NBD) reagents where the halogenis preferably F or CI.
The TAG may for example be a fluorescent moiety, a mass spectrometry TAG, a
first binding partner capable of binding to a second binding partner, a nuclelc acid
wherein any of the aforementioned TAGs preferably comprises or are attached to an
nitrogen-reactive functional group. In particular the TAG may be any of the TAGs
described in more detall herein below, wherein any of these TAGs may be attached
to any of the aforementioned nitrogen-reactive functional groups.

An example of a compound which may be obiained by adding a TAG to compound
E is shown as F in fig. 1.
F. Washing
In one embodiment the tagged sugar (e.g. compound F, fig. 1) is washed prior to
any futher manipulations. Thus any amount of unbound TAG is removed. Washing
may easily be accomplished because the tagged sugar is immobilised on a solid
support.
After washing, only covalent bound TAG will be present. Thus the amount of TAG
will be correlatable to the amount of immobilised sugar. Accordingly, by determining
the presence of TAG, the amount of immobilised sugar may be determined. If esset-
tially all reducing sugar in a glven sample was immobilised, the methods therefore in
one aspect allow determining the amount of reducing sugar present in a sample.
The skilled person will readily be able to identify sultable washing conditions for a
glven tagged, immoblised sugar (e.g. compound F, fig. 1). The washing may for ex-
ample be done with a solvent selected from the group consisting of water, aqueous
buffer, organic solvents and mixed aqueous and organic solvents. The solvent may
also be any of the aforementioned comprising one or more additives such as salts,
divalent metal cations, detergents, complexing agents including inclusion-
conmplex-forming molecules such as cyclodextrins or calixarenes, chelating agents
(for example EDTA), borates, boronates or silicates. Furthermore, the solvent may
optionally comprise detergents and denaturing agents. The washing my be per-
formed at any temperature, but preferably at temperatures in the range of 0 -
100°C.
H. Cleavage of cleavable linker
When the linker used is a cleavable linker, then methods of the invention may com-
prise a step of cleaving said cleavable linker thereby releasing captured sugar. Pref-
erably the cleavage is performed subsequent to addition of a derivatising agent,
such as a TAG (added using TAG-X) or a tether-Y (added using X-tether-Y) to the -
NH- group of the immobilised sugar. Thus a tagged sugar (compound G or com-

pound J in fig. 1) may be released into solution from F or from I, respectively. G
consists of a sugar portion that bears a TAG on the Nitrogen atom which is attached
to the residue (if any) of the linker that remains after cleavage, and for simpliclty is
denoted as sugar-TAG. J consists of a sugar portion that bears a tether on the ni-
trogen atom, which is attached to the residue (if any) that remains after cleavage.
The tether may optionally be linked to a TAG.
However, the cleavable linker may be cleaved at any desirable time within the
method.
If the TAG added to compound E has beneficlal spectroscopic properties such as
fluorescent properties, the amount of sugar-TAG (compound G, fig. 1) can be quan-
titiated in solution. Furthermore, the sugar-TAG (compound G, fig. 1) can be sub-
jected to analytical separation techniques such as HPLC or CE, and if more than
one sugar is present, the individual components can be separated, thelr relative
ratios determined, and they can be identified if authentic standards are available,
and they can be quantitated. They can also be used as ligands that may bind to car-
bohydrate-recognizing proteins, thus providing information on the structure of elther
the carbohydrate or the protein.
If the TAG is a structure glving the sugar-TAG properties that are beneficlal to the
practice of mass-spectrometry, elther due to increased sensitivity, simplification of
spectral interpretation, or permitting the performance of differential analysis using
isotope encoding, then the sugar-TAG released into solution can be favourably ana-
lyzed by mass-spectrometry.
F. TAGs with spectroscopic properties
In one preferred embodiment of the invention the TAG added to e.g. compound E or
compound H has beneficlal spectroscopic properties. Preferably, the TAG with the
beneficlal spectroscopic properties is added to e.g. compound E using a derivative
of the structure X-TAG, wherein X is a nitrogen reactive functional group, such as
any of the nitrogen reactive functional groups described herein above in the section
"E->F Adding TAGs". By beneficial spectroscopic properties is meant that the TAG

can easily be visualised, for example by spectrometry. Thus the TAG may for exam-
ple be spectroscopically detectable. In a preferred embodiment the TAG is a fluo-
rescent TAG. Examples of such tagglng include the reaction with isothiocyanates
(e.g. FITC, TRITC), active esters, Michael acceptors, alpha-beta-unsaturated sul-
fonyls (speclfically vinyl sulfones) and alkylating agents such as alkyl halides and
tosylates, an halo-aryl compounds such as for example the Sanger reagent
The product of addition of such a TAG (for example compound F of fig. 1) can ab-
sorb and re-emit light that can be detected. The number of such TAGs present on F
will reflect the number of sugar molecules A added to B and captured to produce C.
The number of reducing sugar molecules (A) origlnally present in a sample can
therefore be estimated by the fluorescence of compound F, provided that the pro-
vided solid supports (compound B) comprise an excess of capture groups. TAGs
other than fluorescent molecules can also be used. These can include radioactive
TAGs, phosphorescent TAGs, chemiluminescent TAGs, UV-absorbing TAGs,
nanoparticles, quantum dots, coloured compounds,, electrochemically-active TAGs,
infrared-active TAGs, TAGs active in Raman spectroscopy or Raman scattering,
TAGs detectable by atomic force microscopy or TAGs comprising metal atoms or
clusters thereof.
If the solid support of compound F is a sensor, such as a surface acoustic wave
sensor or a surface plasmon resonance sensor, then addition of such a specles that
binds speclfically to the TAG can result in the production of a signal that is propor-
tional to the TAG and therefore to the number of sugar molecules. An example is
when the TAG is a biotin residue, commonly introduced by reaction with an active
ester of biotin. Addition of an avidin-protein to compound E, when the TAG is a bio-
tin residue, can result in signal that is readily detected and reported by the sensor.
Other examples of sensors that can be used to detect the binding of second binding
partners to immobilized TAGs include but are not limited to piezoelectric sensors,
amperometric sensors, surface plasmon fluorescence spectroscopy sensors, dual
polarization interferometry (DPI) sensors, wavelength-interrogated optical sensors
(WIOSs), impedence sensors, optical wavegulde grating coupler sensors, acoustic
sensors and calorimetric sensors.
Once the sugar has been attached to a TAG with spectroscopic properties, then
said spectroscopic properties may be determined. The optical properties may be

determined for sugars still immobilised on the solid support (such as for compound F
or I of fig. 1) or for sugars released to solution (for example for compound G or J of
fig. 1). The latter requlres that the linker is a cleavable linker. Depending on the na-
ture of the TAG with spectroscopic properties, said properties may be determined
using conventional methods, such as spectrometry. Thus the methods of the inven-
tion may comprise the step of detecting the TAG attached to the sugar by spec-
trometry.
F. Mass-spectrometry TAGs
In one embodiment of the invention, the TAG is a mass spectrometry TAG. Said
mass spectrometry TAG is preferably added by a reagent of structure X-TAG,
wherein X is a nitrogen-reactive functional group, such as any of the nitrogen-
reactive functional group mentioned herein above in the section "Adding TAGs". The
term "mass spectrometry TAGs" as used herein refers to molecules that improve the
detection and structural characterization of the products by mass spectrometry, pref-
erably after cleavage from the solid support (as described herein above in the sec-
tion "Cleavage of cleavable linker"). Examples include the introduction of a bromine
label which imparts a characteristic isotope pattern in the mass-spectrum. Such a
bromine label may be added, for example, by addition of p-bromophenyl isothiocy-
anate to compound E producing a compound of structure F where the TAG contains
a bromine atom. The usefulness of bromine-containing labels in the mass-
spectrometry of carbohydrates has been described for example in Li et al., 2003,
Rapid. Commun. Mass Spectr., 17:1462-1466.. Another example includes introduc-
tion of molecules that impart elther positive charges or negative charges for en-
hanced detection in elther positive-ion mode or negative-ion mode of mass/charge
separation. Another example includes the introduction of molecules that improve
performance or sensitivity in electrospray, MaidI or other techniques of ionization
common in the practice of mass spectrometry. Yet another example includes the
introduction of stable isotope-labeled molecules that allow quantitation of the la-
belled specles by mass-spectrometry. Useful methods for isotope labelling are for
example reviewed in Tao et al., 2003, Current Opinion in Biotechnology, 14: 110-
118.

Once the sugar has been attached to a mass spectrometry TAG, then the tagged
sugar (F or G or I or J, fig. 1) may be detected by mass spectrometry. Mass spec-
trometry may be performed on sugars still immobilised on the solid support (such as
for compounds F and I of fig. 1), but preferably is performed on sugars released to
solution, for example by cleavage of a cleavable linker (for example for compounds
G or J of fig. 1). It is thus preferred that the linker is a cleavable linker. The skilled
person will be able to perform a sultable mass spectrometry depending on the na-
ture of the mass spectrometry TAG . Thus the methods of the invention may com-
prise the step of detecting the sugar attached to the mass spectrometry TAG by
mass spectrometry,
F. Binding partner TAGs
In another preferred embodiment of the present invention the TAG is a first binding
partner, capable of speclfic interaction with a second binding partner, wherein said
first binding partner is added to for example compound E (or to compound H)
through the reaction with a reagent of structure X-TAG, wherein X is a nitrogen-
reactive functional group (e.g. a "derivatising agent"). The second binding partner is
preferably labelled with a detectable label, such as a dye, a fluorescent label, a ra-
dioactive isotope, a heavy metal or an enzyme. The first binding partner may for
example be a molecule that is a ligand for a protein useful in the detection of the
resulting immobilized ligand, elther stochiometrically or following amplification. The
first binding partner may also be a protein and the second binding partner a ligand
for said protein.
Examples of binding partners include (igand-protein palrs in common use in ELISA
assays. For example compound E may be reacted with a biotinylation reagent, and
after washing, detecting the now immobilized biotin with streptavidin (or other avid-
ins) that is directly labelled with a detectable label, such as with a fluorescent TAG,
a radioactive isotope or a heavy metal, or with streptavidin (or other avidins) that is
conjugated to an enzyme such as horseradish peroxidase that can catalyze a
chemical reaction that results in the production of a signal that can be detected by
spectrometry.

Other examples of binding partners are antibody-epitope palrs. Thus the one binding
partner could comprise an epitope and the other binding partner could be an anti-
body capable of binding said epitope with high affinity, preferably an antibody spe-
clfically binding said epitope.
F. Nuclelc acld TAGs
In another embodiment of the invention the TAG is a nuclelc acld. Nuclelc aclds ac-
cording to the invention may be any nuclelc acld, such as DNA or RNA, or ana-
logues thereof such as LNA, PNA, HNA or the like. Preferably the nuclelc acld is
DNA, preferably a DNA oligomer. Preferably, said DNA is derivatised with an nitro-
gen-reactive functional group, such as any of the nitrogen-reactive functional groups
mentioned herein above in the section "Adding TAGs". It is preferred that the se-
quence of said nuclelc acld TAG is known or at least partially known, which will en-
able the skilled person to readily detect said TAG using standard methods.
The nuclelc acld TAG may be any desirable length, preferably at least a length
which will allow speclfic detection. Thus preferably the nuclelc acld is at least 6 nu-
cleotides, more prefereably at least 10 nucleotides, for example in the range of 10 to
5000 nucleotides long.
After addition of a nitrogen-reactive nuclelc acld TAG to the sugar, then the nuclelc
acld, such as the DNA oligomers can then be detected directly on the solid support
by hydridisation to thelr complementary nuclelc aclds or essentially complementary
nuclelc acld. By essentially complementary nuclelc aclds, is meant a nuclelc acld,
which may hybridise to a glven nuclelc acld under stringent conditions as for exam-
ple described in Sambrook et al., 1989, in "Molecular Cloning/A Laboratory Manual",
Cold Spring Harbor. Preferably, said complementary nuclelc aclds may be attached
to a detectable label. Said detectable label may for example be a flourescent label
or a radioisotope or an enzyme, preferably a fluorescent label. Thus, the nuclelc
acld TAG may for example be detected by hybridisation to thelr complementarty
fluorescently-labeled DNA. Alternatively, a nuclelc acld TAG may be amplified using
conventional methods known in the art, such as Polymerase Chain Reaction (PCR)
or ligase chain reactin. Thus, the immobilised nuclelc acld TAG may be subjected to

PCR reactions to amplify the immobilized DNA oligomer which can be measured in
solution by a variety of well know techniques for quantification in PCR. This process
has particular value in the indirect detection and quantification of very low amounts
of SugarCH-NH-Linker-Spacer-Solid present on the solid support. Alternatively, the
Sugar bound to DNA may be released to solution by cleavage of the linker and
thereafter amplified in solution by for example PCR or detected in solution by virtue
of speclfic hybridisation to essentially complementary nuclelc aclds.
E->H Tethers
The derivatising agent according to the present invention may also be a tether cou-
pled to at least two functional groups. Such bifunctional reagents will in general be
of the structure X-tether-Y or X-tether-Yp, wherein X is an nitrogen-reactive func-
tional group and Y is a second reactive functional group and Yp is a latent reactive
functional group or a protected reactive group Y. The product of the reaction of
compound E with X-tether-Y (or X-tether-Yp) may for example have the general
structure of compound H of fig. 1. The second reactive functional group Y may be
reactive to any of the types of reagents in use in solid-phase synthesis. For exam-
ple, the N in SugarCH-NH-Linker-Spacer-Solid can be reacted with bifunctional
reagents (X-tether-Y) where one function reacts by making a bond to the immobi-
lized nitrogen (the nitrogen reactive functional group X) and the other function can
elther be, or can be converted to (by for example unmasking, deprotection or further
reaction) a second reactive functional group Y.
The tether may be any useful tether, for example alkyl, alkenyl or alkynyl (which may
be linear, branched or cyclic), aryl or any of the aforementioned comprising amide
bonds (NC(O)R) or etyleneglycol groups (-CH2CH2-O-) or substituted with heteroa-
toms and thelr derivatives.
The second functional reactive group Y may for example be selected from the group
consisting of thiols, carboxyl groups, activated carboxyl groups, disulfides, activated
disulfides, alkylating agents, alkenes, alkynes, aidehydes, ketones and azides. The
alkylating agent may for example be an alkyl halide or an alpha-halo carbonyl group.
Yp may for example be protected amines or protected derivatives of any of the

aforementioned groups Y. Thus Yp may for example be selected from the group con-
sisting of protected amines, protected thiols, protected carboxyl groups, protected
aidehydes and protected ketones. Protected reactive groups are herein denoted Yp,
wherein Yp may be deprotected to yleld a functional reactive group Y. Useful pro-
tecting groups can be found in Greene et al., 1999, "Protective Groups in Organic
Synthesis", 3rd. Ed., John Wiley and Sons, New York, speclfically for carbonyl
groups (chapter 4, pp. 293 - 368 ), for carboxyl groups (chapter 5, pp. 369 453-),
for thiols (chapter 6, pp. 454 - 493) and for amino groups (chapter 7, pp. 494 - 653).
Examples of protected amines include, but are not limited to, those in common use
in solid-phase peptide synthesis, such as Fmoc, Boc, Alloc, p-
ntirobenzyloxycarbonyl, trityl and substituted trityl, o-nitrobenzyloxycarbonyl, N-
sulfenyl or azido. However, the second reactive functional group may be any func-
tional groups Y, or protected functional groups (Yp) that have been made to react on
the solid phase, such as examples well known in the art of solid phase synthesis
and the coupling of small molecules to solid supports and surfaces. These function-
alized groups can then directly, or after deprotection to reactive specles, capture a
second derivatising agent comprising a functional group (Z) capable of reacting with
the second functional group Y.
If Y in compound H contains an NH2 group, or on deprotection can be made to con-
tain an NH2 group, then any of the amine reactive reagents described in E-goes-to-F
(for example, isothiocyanates) can be used to add a TAG to produce compounds of
the general structure I (fig. 1).
The second derivatising agent made to react with any of the functional groups Y in
compound H (fig. 1) may for example be spectroscopic TAGs or any of the TAGs
mentioned above in section E->F, wherein said TAGs in stead of a nitrogen reactive
group, comprises or are derivatised with a functional group (Z) capable of reacting
with Y. They may also be small molecules like drugs, imaglng agents, peptides, pro-
teins, enzymes and other molecules exhibiting biologlcal activities, nuclelc aclds
such as DNA or RNA
Said small molecules, imaglng agents, peptides or nuclelc aclds preferably com-
prises or are attached to a functional group Z, capable of reacting with the glven
second functional reactive group Y. The skilled person will readibly be able to iden-

tify useful functional groups Y and Z. The second derivatising agent may also be any
of the above-mentioned TAGs described above in the sections "TAGs with Spectro-
scopic properties", "Mass spectrometry TAGs", "Binding partner TAGs" and "Nuclelc
acld TAGs", wherein said TAGs in place of a nitrogen reactive functional group con-
tains a functional group Z capable of reacting with the functional group Y. The func-
tional group attached to the tether in H (fig. 1) may also be a latent or protected
group (Yp) that can be converted by chemical or enzymatic reaction into Y which
may then react further as described above. If this latent group can be converted to a
primary or secondary amine (i.e. Y will comprise the structure -NH2 or -NH-), then
any of the amine-reactive specles described in E-*F above may be added to pro-
duce tagged compounds of the structure I.
The methods of the invention may therefore comprise the step of
vii. Reacting the -NH- group of the reactive sugar with a bifunctional
reagent of the structure X-tether-Y or X-tether-Yp, wherein X is a nitro-
gen-reactive functional group and Y is a second reactive functional
group and Yp is a latent functional group that can be converted to or
deprotected to a reactive functional group Y, thereby obtaining a sugar
covalently attached to said tether-Y or said tether-Yp.
This step is preferably performed using compound E of fig. 1 as starting material.
Thus this step may for example generate a compound of the general structure H of
fig. 1.
In embodiments of the invention wherein the bifunctional reagent is of the structure
X-tether-Yp, then preferably, the method furthermore comprises the step of convert-
ing or deprotecting Yp to obtain a reactive functional group Y. This step may be per-
formed before or after reacting X with -NH-, preferably it is performed subsequent to
reacting X with -NH-.
In addition the methods of the invention may furthermore comprise the steps of
viii. providing a second derivatising agent comprising a functional
group (Z) capable of reacting with Y

ix. reacting the functional groups Z and Y, thereby covalently attaching
the second derivatising agent to the sugar via a tether and the first de-
rivatising agent.
Alternatively, the methods of the invention may further comprise the step of:
viii. providing a particle selected from the group consisting of eu-
karyotic cells, prokaryotic cells, microbial organisms, micelles, phages,
vira and nanoparticles, wherein the particle comprises a functional
group (Z) capable of reacting with Y.
ix. reacting the functional groups Z and Y, thereby covalently attaching
the particle to the sugar via the tether and and the agent.
Step ix. may thus generate a compound of the general structure I outlined in fig. 1
where the TAG is a particle. Provided that the linker is a cleavable linker, the meth-
ods may further comprise the step of cleaving the linker thereby for example gener-
ating a compound of the general structure J of fig. 1.
The product of the reaction of SugarCH-NH-Linker-Spacer-Solid (e.g. compound E
of fig. 1) with Afunctional reagents X-tether-Y for example has the general structure
H and may contain, or can be made to contain, further reactive groups that can
form covalent bonds to assemblies larger than molecules: for example bacteria,
phage, yeast, micelles, viruses, nanoparticles or eukaryotic or prokaryotic cells.
Cleavage of the linker then results in specles of the general formula SugarCH-
N(assembly)-Linker, effectively adding the sugar to the assembly. Thus, the sugar
can in princlple be transferred from a solid support to an assembly.
Enzyme treatment
If the solid support is biocompatible, i.e. permits contact with biologlcal macromoie-
cules like enzymes without significantly altering thelr activities, then the immobilised
sugar molecule can be acted on by enzymes that will alter its structure. The immobi-
lised sugar molecule may for example be a compound of any of the general struc-
tures C, Cred, D, E, F, H or I of fig. 1.

Non-limiting examples of biocompatible solid supports includes glass, PEGA,
SPOCC or polysaccharide gels. Within this embodiment it is preferred that the linker
is relatively long, and thus it is preferred that the linker comprises at least 2 atoms,
preferably at least 6 atoms, more preferably the linker comprises a chain of at least
6 atoms, for example the longest chain of atoms within the linker is at least 6 atoms
long, such as in the range of 6 to 1000 atoms long. It is also preferred that the linker
is hydrophilic.
It is also possible to contact the sugars liberated into solution by cleavage of a
cleavable linker, such as the compounds G or J of fig. 1 with biologlcal macromole-
cules, such as enzymes.
The enzymes can belong to any class that can act on carbohydrates, for example
glycosidases, glycosyltransferases, and enzymes that modify the alcohol groups by
acylation, phosphorylation, sulfation or oxidation. Alternatively, if the sugars are al-
ready substituted on -OH groups, such as acylated, phosphorylated or sulphated,
then deacylases, phosphatases and sulfatases can alter thelr structures. Thus the
methods of the invention may furthermore comprise the step of contacting the sugar
(for example any of the compounds C, Cred, D, E, F, G, H, I or J of fig. 1) with one or
more enzymes selected from the classes of glycosyltransferases, sulfatases, pho-
phorylases, sulfotransferases, phosphotransferases, glycosynthases and transgly-
cosidases, thereby converting said sugar into a new structure. In a preferred em-
bodiment the methods furthermore comprise the step of contacting the sugar (for
example any of the compounds C, Cred, D, E, F, G, H, I or J of fig. 1) with one or
more glycosidases, thereby generating a new reducing sugar, provided that the first
sugar is a substrate for said glycosidase(s).
An example would include the incubation of uncapped Sugar-C=N-Linker-Spacer-
Solid (for example, compounds C of fig. 1), which still contains free -NH2 groups,
with an exoglycosidase causing the decrease in the length of the sugar by one
monosaccharide residue. The cleavage of this monosaccharide residue leaves an
oligosaccharide attached to the solid support that is one sugar unit shorter, and pro-
duces a reducing sugar which can be captured by the same or a different solid sup-
port, such as a solid support of the general structure B in fig 1, which can subse-
quently be submitted to any of the manipulations described above in B to J.

Thus the methods of the invention may furthermore comprise the steps of
a) providing one or more enzymes that can act on carbohydrates
b) contacting the sugar with said one or more enzymes
These steps may be performed at any glven time during the method. The enzymes
may be any of the enzymes described in the present section.
In a particular embodiment the enzyme is a glycosidase and the method described
herein above in the summary section comprises the further steps of:
iii.a) providing one or more glycosidases that can act on carbohydrates
iii.b) contacting the sugar with said one or more glycosidases, thereby generating a
new reducing sugar, provided that the first sugar is a substrate for said glycosi-
dase(s).
iii.c) immobilising newly generated reducing sugar(s) on a solid support.
The steps iii.a-iii.c may be carried out following step iii. of the method outlined in the
section "Summary of the invention" herein above. However, the steps iii.a to iii.c
may also be carried out following any of steps iv, v, vi or vii of said method. Accord-
ingly, steps iii.a-iii.c may be carried out on any of the immobilized sugars exemplified
by structures C, Cred- D, E, F, H or I of fig. 1.
In particular, said newly generated reducing sugars may be immobilised to free -
NH2 groups of the same solid support or on another solid support. Said other solid
support may for example elther be unsubstituted or carry an immobilised reference
standard. It is preferred that said other solid support is a solid support as described
herein above, and that the solid support is attached to a linker (optionally via a
spacer), wherein said linker comprises a capture group (see detalled description of
linkers, capture groups and spacers herein above).
Of particular value is the reduction and fluorescence labeling of the glycosidase
product and the released monosaccharide on the same or a different solid support,
for purposes of obtaining structural information. A speclfic example includes the cap-
ture of Gal-GlcNAc-Gal-glc (lacto-N-tetraose, LNT) on NH2-Linker-Spacer-Solid of

structure B (fig 1), incubation of the captured and immobilized LNT (an example of a
compound of structure C of fig. 1) with beta-galactosidase followed by capture of the
released galactose on the same solid support (C) to yleld a mixture of unreacted
Gal-GlcNAc~Gal-GlcC=N-Linker-Spacer-Solid, and the products of the reaction
which are GlcNAc-Gal-GlcC=N-Linker-Spacer-Solid and Gal- C=N-Linker-Spacer-
Solid. Capping, reduction, fluorescence tagglng with TRITC and cleavage form the
solid as described in step F—>G above then allows confirmation that the immobilized
LNT had a terminal beta-galactose residue, by co-migration of the trisaccharide and
monosaccharide products with known standards.
Many useful glycosidases are described in the art, for example any of the glycosi-
dases described in US5,100,778 or W092/19974 may be employed with the present
invention.
If the solid support is biocompatible, then the unreacted -NH2 groups in Sugar-C=N-
Linker-Spacer-Solid (e.g. compound C, fig 1) can be capped (for example with ace-
tic anhydride as described in C->D above) and then exposed to carbohydrate-active
enzymes, or further reduced to SugarCH-NH-Linker-Spacer-Solid (as described in
section D—>E above) and then exposed to carbohydrate-active enzymes. Alterna-
tively, compound C of fig. 1 can be reduced to Cred and then exposed to carbohy-
drate active enzymes. The SugarCH-NH-Linker-Spacer-Solid (e.g. compound E, fig
1) can be further tagged (as described in sections E-»F herein above) to yleld Sug-
arCH-N(TAG)-Linker-Spacer-Solid (e.g. compound F, fig 1), and then exposed to
carbohydrate-active enzymes. In any of these processes, the product of the enzyme
reaction that remains attached to the solid support can be further manipulated ac-
cording to the methods of the invention or cleaved by reaction at the linker, for fur-
ther analysis. Any product of the enzyme reaction that results in cleavage of frag-
ments of the immobilized sugar will appear in solution, where it may be further in-
vestigated using established techniques of analytical chemistry or, in the case where
it is itself a reducing sugar, may be subjected to the manipulations described for the
generic sugar A in Fig 1.
The individual sugars may be detected by capillary gas chromatography (GC), mi-
crocolumn supercritical fluld chromatography (SFC), microcolumn liquld chromatog-
raphy (LC), high performance liquld chromatography (HPLC), high performance cap-

illary electrophoresis (HPCE), ion-exchange chromatography or mass-spectrometry.
Detection of individual sugars may be done before or after labelling with a derivatis-
ing agent, and elther in solution or on the solid phase.
Detection agents
In one embodiment of the invention, the method comprises the steps of
viii. contacting the sugar with a detection agent capable of assoclating
with said sugar
ix. detecting the detection agent
Preferably, said sugar is immobilised on a solid support as described herein above,
and thus for example a compound of the general structure C, Cred, D, E, F, H or I of
fig. 1 may be contacted with said detection agent. It is also possible that said sugar
has been released from the solid support by cleavage of a cleavable linker, as thus
a compound of the general structure G or J may also be contacted with said detec-
tion agent.
The detection agent may be any agent capable of assoclating with said sugar. Pre-
ferred detection agents are compounds capable of assoclating with sugars with
much higher affinity than with any other compounds, such as compounds having at
least a 2-fold, such as at least a 5-fold higher affinity for sugars, than for any other
compound.
In addition it is preferred that said detection agent is directly or indirectly detectable
by a method known to the skilled person. For example the detection agent may itself
be for example a fluorescent or coloured compound, The detection agent may also
be a compound for which easy detection methods are avallable.
In one embodiment of the invention the detection agent comprises an aryl boronate
or heteroaryl boronate where the aryl moiety is substituted with a spectroscopically
active group such as a fluorescent TAG or any of the other detectable TAGs de-
scribed herein above in the section "F. TAGs with spectroscopic properties".

In another embodiment the detection agent is a polypeptide, preferably a polypep-
tide selected from the group consisting of lectins, selectins and other carbohydrate
binding proteins, toxins, receptors, antibodies and enzymes. When the detection
agent is a polypeptide, said polypeptide may be coupled to a detectable label, such
as an enzyme or a fluorescent compound. The polypeptide may also be detected by
the aid of antibodies or similar high affinity compounds.
Examples
The following are illustrative examples of the methods of the invention and should
not be considered as limiting for the invention. Unless otherwise clear from the con-
text, capital letters A, B, C, Cred, D, E, F, G, H, I and J refers to the general struc-
tures outlined in fig. 1.
Experimental
1. Examples of A: Reducing sugars used in the present work
The structures of the reducing sugars captured by solid supports B are shown in
Fig. 2. These included the monosaccharides D-glc (1) and D-Gal (2), the disaccha-
ride N-acetyllactosamine (LacNAc, 3), the trisaccharide maltotriose (maltotriose G3,
4) and the tetrasaccharide lacto-N-tetraose (LNT, 5). Samples 6 and 7 contained
mixtures of the monosaccharides Fuc:Man:GainAc in ratios of 2:3:1 and 1:3:2, re-
spectively. Sample 8 contained a 1:1 mixture of Gal (2) and LNT (5). Sample 9 con-
tained an approximately equlmolar mixture of maltobiose (G2), maltotriose (G3),
maltotetraose (G4), maltopentaose (G5), maltohexaose (G6) and maltoheptaose
(G7). Sample 10 consisted of the N-linked oligosaccharide chains released from
ribonuclease B (Sigma) by the action of PNGase F (product number 1365177, Boe-
hringer Mannhelm GmbH, Germany).

2. Linkers, spacers and tagged-sugar reference standards
2.1 Linker and spacer
The synthesis of the cleavable linker and the structure of the spacer are shown in
Fig. 3 and described below.
12: N-Fmoc-4-aminooxymethyl-benzoic acld
To a solution of 4-aminooxymethyl-benzoic acld, hydrochloride 111 (2.0 g, 0.010
mol) in dioxane (20 mL) and half saturated Na2CO3 solution (20 mL) was added
Fmoc-cl (2.8 g, 0.011 mol) and the mixture was stirred for 2 h. Ethyl acetate (100
mL) was added and the pH of the aqueous phase was adjusted to 1-3 by careful
addition of Hcl(oonc.). The mixture was poured in to a separating funnel and the or-
ganic phase was isolated, washed once with water (100 mL), dried over Na2SO4 and
the solvent was removed on a rotavap to glve an oil that solidified upon standing.
The crude product was purified by flash column chromatography (petroleum ether,
ethyl acetate, AcOH 60:40:1). yleld: 3.5 g (92%) 1H-NMR (250 MHz, DMSO-d6) 5 =
4.05 (1H, t, J= 6.3 Hz), 4.27 (2H, d, J = 6.3 Hz), 4.51 (2H, s), 7.08-7.22 (6H, m),
7.46 (2H, d, J = 7.4 Hz), 7.66 (2H, d, J = 7.1 Hz), 7.72 (2H, d, J = 8.4 Hz), 10.29
(1H, br. s), 12.78 (1H, br. s). 13C-NMR (63 MHz, DMSO-d6) δ = 47.04, 66.03, 76.91,
120.51, 125.41, 127.45, 128.03, 128.89, 129.33, 129.63, 130.82, 141.19, 144.01,
157.12, 167.48. MS (ES) m/z = 389 (MH+).
13: Reaction of N-Fmoc-4-aminooxymethyl-benzoic acld (12) with t-butyl bro-
moacetate
N-Fmoc-4-aminooxymehtyl-benzoic acld (12) (1.0 g, 2.57 mmol) was dissolved in
DMF (15 mL) and Cs2CO3 (0.42 g, 1.28 mmol, aidrich) was added followed by stir-
ring for 5 min at rt. tert-Butyl bromoacetate (0.55 g, 2.28 mmol, Fluka) was added
and the mixture was heated to 50°C for 30 min and then cooled to rt again. CH2Cl2
(70 mL) was added and the mixture as poured in to a separating funnel and washed
with half saturated NaHCO3 solution (3 x 50 mL) and then water (2 x 50 mL), dried
over MgSO4.The solvent was removed under reduced pressure to glve the crude
product as an oil. After flash column chromatography (20-40% ethyl acetate in petro-
leum ether) a white solid was obtained in a yleld of 1.15 g (89%). 1H-NMR (250
MHz, CDcl3) 5= 1.37 (9H, s), 4.06 (1H, t, J = 6.7 Hz), 4.37 (2H, d, J = 6.7 Hz), 4.61
1The material was prepared as previously described: Deles,J. et al.; PJCHDQ; Pol. J. Chem.;
EN; 53; 1979; 1025-1032

(2H, s), 4.67 (2H, S), 7.11-7.18 (2H, m), 7.22-7.27 (4H, m), 7.43 (2H, d, J= 7.5 Hz),
7.60 (2H, d, J = 7.3 Hz), 7.75 (1H, s), 7.93 (2H, dd, J = 1.7 Hz, 6.6 Hz). 13C-NMR
(63 MHz, CDcl3) δ = 26.31, 45.28, 59.95, 65.52, 75.99, 80.84, 118.30, 123.27,
125.41, 126,10, 126.93, 127.23, 128.30, 139.29, 139.58, 141.73, 155.70, 163.94,
165.15. MS (ES) m/z = 542 (MK+).
14: Preparation of linker
The white solid 13 (1.15 g) obtained in the previous experiment was stirred in a 50%
solution of CF3CO2H in CH2Cl2 (30 ml) for 3 h and evaporated to dryness. The oily
residue was taken up in a small amount of ethyl acetate and the product was pre-
clpitated as a fine white powder by slow addition of hexanes to the solution. The
product was filtered and washed a couple of times with hexanes and dried under
vacuum to glve the desired product in an almost quantitative yleld (1.0 g, 98%). 1H-
NMR (250 MHz, DMSO-d6) 5 = 4.07 (1H, t, J = 6,3 Hz), 4.28 (2H, d, J = 6,3 Hz),
4.53 (2H, s), 4.62 (2H, S), 7.07-7.14 (2H, m), 7.17-7.26 (4H, m), 7.46 (2H, d, J = 7.4
Hz), 7.66 (2H, d, J = 7.2 Hz), 7.77 (2H, d, J= 8.3 Hz), 10.30 (1H, br. s). 13C-NMR
(63 MHz, DMSO-d6) δ = 47.04, 61.62, 66.04, 76.79, 120.50, 125.41, 127.46,
128.03, 129.05, 129.69, 141.19, 142.20, 144.00, 157.12, 165.50, 169.47. MS (ES)
m/z = 446 (M-H+). HRMS (ES) calculated (C25H21NO7Na+): 470.1210 found:
470.1224.
2.2 Synthesis of tetramethylrhodamine (TMR)-tagged monosaccharide stan-
dards of the general structure G.
The 8 monosaccharides D-glc, D-Gal, D-Man, D-Xyl, D-GlcNAc, D-GainAc, L-Fuc
and D-glcA were used. The general synthetic scheme is shown in Fig. 4 for D-Gal
(2), and the structure of the product 21 is shown in Fig. 4 and is abbreviated
GalCH2-N(R)-TMR as shown. The structures of all elght SugarCH2-N(R)-TMR
monosaccharide derivatives prepared are shown in Fig. 5.
16: Reaction of N-Fmoc-4-aminooxymethyl-benzoic acld (12) with
benzylbromide
N-Fmoc-4-aminooxymethyl-benzoic acld (12, 2.0 g, 5.14 mmol) was dissolved in
DMF (30 mL) and Cs2CO3 (0.84 g, 2.57 mmol) was added followed by stirring for 5
min at rt. Benzyl bromide (1.05 g, 6.17 mmol) was added and the mixture was al-
lowed to stir for another 30 min at rt. Water (200 mL) was added and the mixture

was extracted with CH2Cl2 (2 x 100 mL). The combined organic phases were
washed with water (3 x 50 mL), dried over MgSO4, evaporated to dryness to yleld an
oil which was used without further characterization in the next experiment.
17: Removal of Fmoc-group from benzyl-(N-Fmoc-4-aminooxymethyl)-
benzoate
The crude product (16) obtained in the previous experiment was stirred with 20%
piperidine in DMF (20 mL) for 1 min and passed through a bed of silica gel to re-
move the majority of DMF and piperidine by suction. The product was eluted from
the bed of silica gel with a mixture of ethyl acetate and pet. ether (1:1) and concen-
trated on a rotavap. Further purification was achieved by flash column chromatogra-
phy (ethyl acetate, petroleum ether 1:1) to glve a clear oil in a yleld of 1.16 g (88%,
two steps). 1H-NMR (250 MHz, CDcl3) 6 = 4.66 (2H, s), 5.29 (2H, s), 7.25-7.39 (7H,
m), 7.99 (2H, dd, J =1.7 Hz, 6.5 Hz). 13C-NMR (63 MHz, CDcl3) δ = 67.11, 77.59,
128.32, 128.57, 128.66, 129.02, 129.19, 130.32, 136.48, 143.47, 166.64. MS
(MaidI-TOF) m/z = 258 (MH+).
General procedure for preparation of TMR labelled monosaccharide standards ex-
emplified by the preparation of galactose standard.
18: Oxime formation between galactose and benzyl-(4-aminooxymethyl)-
benzoate
Galactose (90 mg, 0.50 mmol) was dissolved in a mixture of DMSO and AcOH (7:3,
3 mL) and (17,128 mg, 0.50 mmol) was added. The mixture was heated for 3 h at
55°C and poured into water (30 mL) and cooled on an ice bath which caused the
product to crystallize as fine white crystals. The product was isolated by filtration,
washed with water (2x10 mL) and dried under vacuum to yleld the 170 mg (83%)
of product as a single isomer. 1H-NMR (250 MHz, DMSO-d6) 5 = 3.38-3.55 (4H, m),
3.67-3.75 (1H, m), 4.27-4.33 (1H, m), 5.12 (2H, s), 5.37 (2H, s), 7.36-7.52 (7H, m),
7.56 (1H, d, J= 7.6 Hz), 8.00 (2H, d, J= 8.1 Hz). 13C-NMR (63 MHz, DMSO-d6) δ
= 63.40, 66.52, 68.37, 69.21, 70.04, 72.63, 74.27, 128.25, 128.33, 128.49, 128.91,
129.13, 129.67, 136.52, 144.22, 154.00, 165.78. MS (MaidI-TOF) m/z = 442
(MNa+)

19: Reduction of "galaclose-oxime" (18) with BH3-pyridine
The oxime (18, 150 mg, 0.36 mmol) obtained in the previous experiment was dis-
solved in methanol (10 mL). BH3-pyridine (225 µL, 8 M solution in pyridine, 1.80
mmol, Fluka) and CCl3CO2H (0.50 mL, 50% aqueous solution) were added and the
mixture was stirred for 1 h at rt. The reaction mixture was carefully poured into a
half-saturated solution of Na2CO3 (20 mL) and extracted with a 1:1 mixture of ether
and hexanes (2x10 ml) to remove excess borane reagent. The pH was now ad-
justed to 2-3 by careful addition of Hcl(COnc.) and the volume was reduced to half of
the origlnal on a ratovap. During the evaporation the product separated out as nice
white crystalline solid, which was filtered of, washed with water (2x10 mL), ether (2
x 10 mL) and finally the product was dried under vacuum to glve 112 mg (75%) of
pure product. 1H-NMR (250 MHz, DMSO-d6) δ = 3.31-3.33 (2H, m), 3.40-3.55 (5H,
m), 3.74 (1H, t, J= 6.3 Hz), 5.24 (2H, s), 5.37 (2H, s), 7.36-7.50 (5H, m), 7.60 (2H,
d, J = 8.2 Hz), 8.04 (2H, d, J = 8.2 Hz). 13C-NMR (63 MHz, DMSO-d6) S = 53.34,
63.40, 64.73, 66.68, 69.37, 70.19, 70.89, 74.20, 128.36, 128.53, 128.92, 129.47,
129.87, 130.27, 136.41, 139.73, 165.62. MS (MaidI-TOF) m/z = 422 (MH+).
20: Labelling of reduced product (19) using TRITC
A small amount of the product (19,4.2 mg, 10 µmol) prepared in previous experi-
ment was dissolved in DMF (1 mL) and TRITC (4.4 mg, 10 µmol) was added. After
stirring for 1 h water (10 mL) was added and the preclpitated product was re-
dissolved by addition of Hcl(Conc.) and the clear red solution was applied to a small C-
18 Sep-Pak column to bind the product. The column was flushed several times with
water (total volume 30 mL) followed by release of the product with methanol (5 mL).
The volume was reduced to approximately 0.5 mL and the material was purified by
flash column chromatography on silica gel with a mixture of CH2Cl2, methanol, wa-
ter, AcOH (70:20:9:1). The identity of the compound was confirmed by MS and used
directly in the next experiment. MS (MaidI-TOF) m/z = 865 (MH+).
21: Hydrolysis of ester protecting group to glve final standard
All the material (2O) obtained in the previous experiment was dissolved in 1 M LiOH
(1 mL) and stirred for 30 min followed by addition of water (10 mL) and acldification
with Hcl(conc.) to glve a clear red solution. The product was desalted on a small C-18
Sep-Pak column by repeated washings with water (total volume 30 mL) followed by

release of the product with methanol (5 mL). The volume was reduced to approxi-
mately 0.5 mL and the product was purified by flash column chromatography on
silica gel with a mixture of chloroform, methanol, water (120:85:2O). The identity of
the compound was confirmed by high resolution MS and its purity was analysed
using CE. HRMS (ES) calculated (C39H43N4O11S): 775,2649 found: 775.2700
Standards of the remaining monosaccharides (glucose, mannose, N-
acetylglucosamine, N-acetylgalactosamine, xylose, fucose and glucuronic acld)
were prepared using the same protocol as described for galactose in similar ylelds
and purity. The compounds' identities were likewise confirmed by high resolution
mass spectroscopy (see table below). Each compound gave a single peak in CE,
and all 8 compounds (21-28) could be resolved in CE (Fig. 10).

3. Examples of B: Preparation and nomenclature of solid supports
Solid supports of general structure B (Fig. 1) were prepared using both PEGA resin
(PEGA 1900, Versamatrix A/S) and controlled-pore glass (CPG). Bp indicates a
PEGA resin where the linker is attached directly to the amino groups on the com-
merclal resin without a spacer. B°, B1 and B2 indicate CPG where the linker has
been attached through 0,1 and 2 spacers respectively to aminopropylated glass

(AMP-CPG, CPG-Biotech). The structures of the four solid supports are shown in
Fig. 6.
3.1 Bp (PEGA resin of general structure B)
1 g of commerclal PEGA 1900 resin (loading of amino groups: 0.23 mmol/g) swelled
in methanol was washed repeated time with DMF to ensure complete removal of the
methanol. The linker (14) (308 mg, 0.69 mmol), TBTU (207 mg, 644 mmol) and
DIPEA (119 mg, 0.92 mmol) were mixed in DMF (10 mL) and left to pre-activate for
5 min before adding the mixture to the resin. After 3 h the reagents were removed
by suction and the resin was washed with CH2Cl2 (5 x 20 mL).
A small portion of the resin was taken out for Kalser test which confirmed a success-
ful coupling of the linker to the resin. Likewise, the loading of linker on the resin was
determined as described in example 3.3 and found to be approximately 0.20 mmol/g
by comparison with a standard curve. The hydroxylamine protecting group (Fmoc)
was now removed from the remaining resin by treatment with 20% piperidine in
DMF (15 mL for 2 min and 15 mL fori 8 min) followed by extensive washings with
DMF (5 x 20 mL) and CH2Cl2 (7 x 20 mL). The resin was dried under high vacuum
for 24 h to glve the final PEGA resin (Bp) which was used for all subsequent experi-
ments.
3.2 B°, B1 and B2 (Controlled pore glass, CPG)
B°: Coupling of linker 14 with CPG-NH2
AMP CPG (250 mg, loading = 50.1 µmol/g, 0.0125 mmol. Millipore, product no.
AMP1400B) was washed with DMF (3 x 2 mL), 50% DIPEA in DMF (3 x 2 mL), and
DMF (3x2 mL). The beads were treated with a mixture of 14 (17 mg, 0.038 mmol),
TBTU (12 mg, 0.037 mmol), and DIPEA (8.6 µL, 0.05 mmol) in DMF at rt over night.
The beads were washed with DMF (3x2 mL), CH2Cl2 (3x2 mL), and treated with
50% of AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3^2 mL), DMF (3x2
mL), CH2Cl2 (3x2 mL), and dried. The loading was determent to 14.2 µmol/g as
described for B1. The Fmoc group was removed using 20% piperidine in DMF for 2
x 10 min at rt and washed with, DMF (3x2 mL), CH2Cl2 (3x2 mL), and ethanol (3
x 2 mL), and CH2Cl2 (3x2 mL). The resin was dried in vacuum.

B1: Coupling of one spacer 15 and linker 14 with CPG-NH2
AMP CPG (2.26 g, loading = 50.1 pmol/g, 0.11 mmoi. Millipore, product no.
AMP1400B) was washed with DMF (3> DMF (3x2 mL). The beads were treated with a mixture of 15 (168 mg, 0.34 mmol),
TBTU (105 mg, 0.33 mmol), and DIPEA (78 µL, 0.45 mmol) in DMF for 3 h at rt. The
resin was washed with DMF (3x5 mL), CH2Cl2 (3x5 mL), and treated with 50%
AC20 in pyridine for 15 min at rt. The beads were washed with CH2Cl2 (3x5 mL),
DMF (3x5 mL), CH2Cl2 (3x5 mL), and treated with 50% TFA in CH2Cl2 for 2 h at
rt. Washed with CH2Cl2 (3x5 mL), DMF (3x5 mL), and CH2Cl2 (3x5 mL). 1/3 of
the beads (2.5 mL, -0.70 g, -35 µmol) were washed with DMF (3x5 mL). Treated
with 14 (47 mg, 0.11 mmol), TBTU (33 mg, 0.10 mmol), and DIPEA (34 µL, 0.20
mmol) in DMF over night at rt. The beads were washed with DMF (3x5 mL),
CHaCl2 (3x5 mL), and treated with 50% AC20 in pyridine for 15 min at rt, washed
with CH2Cl2 (3x5 mL), DMF (3x5 mL), CH2Cl2 (3x5 mL), and dried. The loading
was determined (29 pmol/g) and the beads were treated with 20% piperidine in DMF
at rt for 2 x 10 min. The beads were washed with, DMF (3x2 mL), CH2Cl2 (3x2
mL), and ethanol (3x2 mL), CH2Cl2 (3x2 mL), and dried.
B2: Coupling of two spacers 15 and linker 14 with CPG-NH2
2/3 of the resin with one spacer from B1 (5.5 mL, ~1.54 g, -77 µmol) was washed
with DMF (3x5 mL). The beads were treated with a mixture of 15 (114 mg, 0.23
mmol), TBTU (72 mg, 0.22 mmol), and DIPEA (53 µL, 0.31 mmol) in DMF over night
at rt. The beads were washed with DMF (3x5 mL), CH2Cl2 (3x5 mL), and treated
with 50% AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3x5 mL), DMF (3 x
5 mL), CH2Cl2 (3x5 mL), and treated with 50% CF3CO2H in CH2Cl2 for 2 h at rt,
washed with CH2Cl2 (3 × 5 mL), DMF (3 x 5 mL), and CH2Cl2 (3 x 5 mL). Half the
amount of the beads (~ 42 µmol) were washed with DMF (3x5 mL) and treated
with 14 (56 mg, 0.13 mmoi), TBTU (39 mg, 0.12 mmol), and DIPEA (29 µL, 0.17
mmol) at rt over night. The beads were washed with DMF (3x5 mL), CH2Cl2 (3x5
mL) and treated with 50% AC20 in pyridine for 15 min at rt, washed with CH2Cl2 (3 x
5 mL), DMF (3x5 mL), CH2Cl2 (3x5 mL) and dried. The loading was determent as
described for B1 to 36 umo!/g. The resin was covered with 20% piperidine in DMF at
rt for 2 x 10 min, washed with, DMF (3x5 mL), CH2Cl2 (3x5 mL), ethanol (3x5
mL) 3 x CH2Cl2 (3x5 mL), and dried in vacuum.

3.3 Example of the estimation of the loading of capture groups on solid sup-
ports of general structure B (Fig. 1)
Seven concentrations of Fmoc-Gly-OH in 20% piperidine in DMF (0.0 mM, 0.1 mM,
0.25 mM, 0.5 mM, 1.0 mM, 1.5 mM, 2,0 mM) were prepared. The UV absorbance of
released fulvene were measured at 290 nm using nonodrop technology (Saveen
Werner Nanodrop, Model: ND-1000, Serial No: 0911). The absorbance was plotted
against the concentration glving a linear curve with slope 0.581 mM"1.
Fmoc protected B1 beads (4.8 mg) were treated with 20% piperidine in DMF (200
pL) for 10 min. The UV absorbance at 290 nm was measured to 0.410 and the lib-
erated fulvene concentration was calculated

4. Examples of A+B->C, and processing of C.
4.1 Variation of capture conditions using glucose as the reducing sugar and
B2 as the solid support.
Various solvents, temperatures and additives were examined in order to find prefer-
able conditions for the capture of reducing sugars on solid supports of general struc-
ture B, to produce C. D-glc was used as the model compound, as the amount of
uncaptured Glc in solution could be readily estimated with high sensitivity using the

Ampiex Red assay from Molecular Probes. The amount of Glc captured was thus
calculated to be the amount added minus the amount remaining in solution after
incubation.
15-20 mg of beads (B2) were treated with a solution of glucose under different con-
ditions. After end reaction time the supernatant was removed and the amount of un-
reacted glucose was estimated using the Amplex Red Glucose/Glucose Oxidase
Assay Kit (A-22189, Molecular Probes).
Capture of glucose using different solvents, concentrations, temperatures and
reaction times

4.2 Capture, processing and analysis of representative reducing sugars on Bp.
The following designations are used below to describe compounds of the general
structures C, Cred, D, E, F,G, H, I and J (Fig. 1). The particular letter describing the
particular structure under discussion is glven first, e.g. C or E. The next superscript
number refers to which of the four solid supports shown in Fig. 6 was used. Thus, by
way of example if Bp (Fig. 6) is used to capture a sugar, then the product will have
the general structure C which is further designated as Cp. The next number refers to
which of the ten samples of reducing sugars shown in Fig. 2 was captured. Thus,
Cp2 refers to the product of the PEGA resin Bp that has captured galactose (com-
pound 2 of Fig. 2). In the same way, D25 would refer to the product obtained when

the solid support B2 has captured the tetrasaccharide LNT (5, Fig. 2) to glve Cz5,
and then been further capped to D25.
4.2.1 Capture and processing of reducing sugar 3
Cp3: Capture of LacNAc (3) on Bp
A stock solution was made by first dissolving LacNAc (3) (38 mg, 0.10 mmol) in wa-
ter (1.0 mL) and then diluting the sample 10 times with a mixture of DMSO and
AcOH (7:3, 9 mL) to glve a 10 mM stock solution of LacNAc (3). 40 µL (0.40 pmol)
was then taken from the stock solution and diluted further with the mixture of DMSO
and AcOH (7:3,150 µL) and the whole was added to Bp (10 mg, 2 Mmol) and left to
incubate at 60°C over night. The resin was washed several times: DMF (5 x 0.5
mL), methanol (5 x 0.5 mL) and used directly in the next experiments.
Dp3: Capping of Cp3 with acetic anhydride
All the resin obtained in experiment Cp3 was treated with a mixture of AC20 and
methanol 1:1 (0.4 mL) for 1 h followed by washing with DMF (5 x 0.5 mL), water (2 x
0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiment.
Ep3: Reduction of Dp3 with BH3-pyridine
The resin obtained in experiment Dp3 was covered with methanol (0.1 mL) and BH3-
pyridine (20 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H
acld in water (40 pL). The reaction was left to proceed for 2 h at rt followed by wash-
ing with DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and CH2Cl2 (5 x 0.5 mL). The
resin was used directly in the next step.
Fp3: Tagglng of Ep3 using TRITC
TRITC (0.89 mg, 2 pmol) was dissolved in DMF (0.2 mL) and the solution was
added to the resin (Ep3) and left for 2 h at rt followed by extensive washing DMF (5
x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL), and finally water (5 x 0.5 mL)
to remove excess dye. The resin was used directly in the next step.
Gp3: Cleavage of TMR tagged LacNAc from support
The resin obtained in the previous experiment Fp3 was covered with a 1 M solution
of LiOH (0.2 mL) and left for 2 h. The liquld was collected from the beads by suction
followed by washing of the beads with water (3 x 0.5 mL). The collected liquld and

washings were pooled and pH was adjusted to neutral with 10% AcOH. The dark
red solution was adsorbed on a Sep-Pak coiumn (50 mg), washed with water (2 mL)
and eluted with methanol (0.5 mL). The identity of the product was confirmed by MS
(ES) rn/z = 978 (MH+) and the profile was recorded by CE (Fig. 11).
4.2.2 Capture and processing of reducing sugar 5
Cp5: Capture of Lacto-N-tetraose (5) on Bp
A solution was made by dissolving 5 (5.0 mg, 7.1 µmol) in a mixture of DMSO and
AcOH 7:3 (3 mL). This mixture was added to PEGA resin Bp (175 mg, 35 µmol) and
incubated at 60°C over night. The resin was washed several times: DMF (5x5 mL),
methanol (5x5 mL) and used directly in the next experiments.
Dp5: Capping of Cp5 with acetic anhydride
All the resin obtained in experiment Cp5 was treated with a mixture of AC20 and
methanol 1:1 (5 mL) for 1 h followed be washing with DMF (5x5 mL), water (2x5
mL), methanol (5 x 5 mL) and used directly in the next experiment.
Ep5: Reduction of Dp5 with BH3-pyridine
The resin obtained in experiment Dp5 was swelled in methanol (2 mL) and BH3-
pyridine (200 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H
acld in water (400 µL). The reaction was left to proceed for 2 h at rt followed by
washing with DMF (5x5 mL), methanol (5x5 mL) and CH2Cl2 (5x5 mL). Finally
the resin was dried down under vacuum over night and stored at room temperature
for further use.
Fp5: Tagglng of Ep5 with bromine containing MS-tag
A small amount of the dried resin Ep5 (10 mg, 0.4 µmol) was washed with CH2Cl2 (3
x 0.5 mL) in order to swell the resin. A solution was made by dissolving 4-
bromophenyl isothiocyante (0.85 mg, 4 µmol) in DMF (0.2 mL) and the mixture was
added to the resin and left to react for 2 h at rt followed by washing of the resin DMF
(5 x 0.5 mL), CH2clZ (5 x 0.5 mL), methanol (5 x 0.5 mL), and finally water (5 x 0.5
mL). The resin was used directly in the next step.

Gp5: Cleavage of bromine tagged Lacto-N-tetraose from support
The resin obtained in the previous experiment Fp5 was covered with a 1 M solution
of LiOH (0.2 mL) and left for 2 h. The iiquld was collected from the beads by suction
followed by washing of the beads with water (3 × 0.5 mL). The collected liquld and
washings were pooled and pH was adjusted to slightly acldic (pH 3-4) with 10%
AcOH. The solution containing the desired product was adsorbed on a Sep-Pak
column (50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The
identity of the product was confirmed by MS (ES) m/z = 1072 (98%, MH+), 1074
(100%, MH+), m/z = 1070 (98%, M-H+), 1072 (100%, M-H+). Fig. 12 shows the
mass-spectrum with an inset expansion where the two isotopes of bromine can
clearly be distingulshed.
4.2.3 Capture and processing of reducing sugar mixture 6
Cp6: Capture of monosaccharide mixture 6 (Fuc:Man:GainAc, 2:3:1) on Bp
A series of 3 stock solutions were made by dissolving the 3 individual monosaccha-
rides (Fuc: 16 mg, 0.10 mmol, Man: 18 mg, 0.10 mol, GainAc: 22 mg, 0.10 mmol) in
water (3 x 1.0 mL) and then diluting the samples 10 times with a mixture of DMSO
and AcOH (7:3, 3x9 mL) to glve 10 mM stock solutions of the 3 monosaccharides.
A mixture was now prepared by taking the following amounts from the 3 stock solu-
tions: Fuc (20 pi, 0.2 pmol), Man (30 µL, 0.3 µmol) and GainAc(10 µL, 0.1 µmol).
This monosaccharide solution was diluted further by addition of the mixture of
DMSO and AcOH (7:3,150 µL) and the whole was added to PEGA resin Bp (10 mg,
2 pmol) and left to incubate at 60°C over night. The resin was washed several times:
DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and used directly in the next experiments.
Dp6: Capping of Cp6 with acetic anhydride
All the resin obtained in experiment Cp6 was treated with a 1:1 mixture of AC2O and
methanol (0.4 mL) for 1 h followed be washing with DMF (5 x 0.5 mL), water (2 x 0.5
mL), methanol (5 x 0.5 mL) and used directly in the next experiment.
Ep6: Reduction of Dp6 with BH3-pyridine
The resin obtained in experiment Dp6 was covered with methanol (0.1 mL) and BH3-
pyridine (20 µL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H
in water (40 pL). The reaction was left to proceed for 2 h at rt followed by washing

with DMF (5 x 0,5 mL), methanol (5 x 0.5 mL) and CH2Cl2 (5 x 0.5 mL). The resin
was split into 2 separate containers (Ep6a and Ep6b, app. 5 mg each) and used di-
rectly in the next steps.
Fp6a: Tagglng of Ep6a using TRITC
TRITC (0.5 mg, 1.2 jjmol) was dissolved in DMF (0.2 mL) and the solution was
added to the resin (Ep6a) and left for 2 h at rt followed by extensive washing DMF (5
x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL)
to remove excess dye. The resin was used directly in the next step.
Gp6a: Cleavage of TMR tagged monosaccharide mixture from support
The resin obtained in the previous experiment (Fp6a) was covered with a 1 M solu-
tion of LiOH (0.1 mL) and left for 2 h. The liquld was collected from the beads by
suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq-
uld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The
dark red solution was adsorbed on a Sep-Pak column (50 mg), washed with water
(2 mL) and eluted with methanol (0.5 mL). The identity of the 3 tagged products was
confirmed by MS (ES) m/z = 759 (Fuc, Mt-T), 775 (Man, MH+) δ16 (GainAc, MH+)
and thelr profile was recorded by CE (Fig. 13).
Fp6b: Tagglng of Ep6b with acetic anhydride
A 1:1 mixture of AC20 and methanol (0.2 mL) was added to the resin (Ep6b) and left
for 16 h at rt followed by extensive washing DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL),
methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL). The resin was used directly in
the next step.
Gp6b: Cleavage of acetic acld tagged monosaccharide mixture from support
The resin obtained in the previous experiment (Fp6b) was covered with a 10% solu-
tion of NH4OH (0.1 mL) and left for 2 h. The liquld was collected from the beads by
suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq-
uld and washings were pooled and evaporate to dryness on a rotavap, re-dissolved
in water (1 mL) and freeze dried. The identity of the 3 tagged products was con-
firmed by MS (ES) m/z = 356 (Fuc, M-H+), 372 (Man, M-H+), 413 (GainAc, M-H+).
The ratio of the intensities of the 3 signals was approximately 1.3:2:1.

4.2.4 Capture and processing of reducing sugar mixture 7
Cp7: Capture of monosaccharide mixture 7 (Fuc:Man:GainAc, 1:3:2) on Bp
The same 3 stock solutions of monosaccharides (10 mM each) that were used in
experiment Cp6 was used in the following experiment. A mixture was prepared by
taking the following amounts from the 3 stock solutions: Fuc (10 µL, 0.1 µmol), Man
(30 µL, 0.3 µmol) and GainAc (20 µL, 0.2 µmol). This monosaccharide solution was
diluted further by addition of the mixture of DMSO and AcOH (7:3,150 µL) and the
whole was added to PEGA resin Bp (10 mg, 2 µmol) and left to incubate at 60°C
over night. The resin was washed several times: DMF (5 x 0.5 mL), methanol (5 x
0.5 mL) and used directly in the next experiments.
Dp7: Capping of Cp7 with acetic anhydride
All the resin obtained in experiment Cp7 was treated with a 1:1 mixture of AC20 and
methanol (0.4 mL) for 1 h followed by washing with DMF (5 x 0.5 mL), water (2 x 0.5
mL), methanol (5 x 0.5 mL) and used directly in the next experiment.
Ep7: Reduction of Dp7 with BH3-pyridine
The resin obtained in experiment Dp7 was covered with methanol (0.1 mL) and BH3-
pyridine (20 µL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H
in water (40 µL). The reaction was left to proceed for 2 h at rt followed by washing
with DMF (5 x 0.5 mL), methanol (5 x 0.5 mL) and CH2Cl2 (5 x 0.5 mL). The resin
was split into 2 separate containers (Ep7a and Ep7b, app. 5 mg each) and used di-
rectly in the next step.
Fp7a: Tagglng of Ep7a using TRITC
TRITC (0.5 mg, 1.2 µmol) was dissolved in DMF (0.2 mL) and the solution was
added to the resin (Ep7a) and left for 2 h at rt followed by extensive washing DMF (5
x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL)
to remove excess dye. The resin was used directly in the next step.
Gp7a: Cleavage of TMR tagged monosaccharide mixture from support
The resin obtained in the previous experiment (Fp7a) was covered with a 1 M solu-
tion of LiOH (0.1 mL) and left for 2 h. The liquld was collected from the beads by
suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq-
uld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The

dark red solution was adsorbed on a Sep-Pak column (50 mg), washed with water
(2 mL) and eluted with methanol (0.5 mL). The identity of the 3 tagged products was
confirmed by MS (ES) m/z = 759 (Fuc, MH+), 775 (Man, MH+) δ16 (GaSNAc, MH+)
and thelr profile was recorded by CE (Fig. 14).
Fp7b: Tagglng of Ep7b with deuteroacetic anhydride
A 1:1 mixture of deuteroacetic anhydride and methanol (0.2 mL) was added to the
resin (Ep7b) and left for 16 h at rt followed by extensive washing DMF (5 x 0.5 mL),
CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5 mL) and finally water (5 x 0.5 mL). The resin
was used directly in the next step.
Gp7b: Cleavage of deuterium tagged monosaccharide mixture from support
The resin obtained in the previous experiment (Fp7b) was covered with a 10% solu-
tion of NH4OH (0.1 mL) and left for 2 h. The liquld was collected from the beads by
suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq-
uld and washings were pooled and evaporate to dryness on a rotavap, re-dissolved
in water (1 mL) and freeze dried. The identity of the 3 deuterium tagged products
was confirmed by MS (ES) m/z = 359 (Fuc, M-H+), 375 (Man, M-H+), 416 (GainAc,
M-H+). The ratio of the intensities of the 3 signals was approximately 1:4:4.
4.2.5 Capture and processing of reducing oligosaccharide mixture 9
Cp9: Capture of oligosaccharide mixture 9 (G2-G7) on Bp
A solution was made by dissolving an equlmolar amount (10 µmol each) of the pure
oligosaccharides G2-G7 in water (1 mL). 100 µL of the oligosaccharide containing
solution was added to a mixture of DMSO and AcOH (7:3, 0.9 mL) and the whole
was added to PEGA resin Bp (60 mg, 12 µmol) and left to incubate at 50°C over
night. The resin was washed several times: DMF (5x2 mL), methanol (5x2 mL)
and used directly in the next experiments.
Dp9: Capping of Cp9 with acetic anhydride
All the resin obtained in experiment Cp9 was treated with a 1:1 mixture of AC20 and
methanol (2 mL) for 1 h followed be washing with DMF (5 x 2 mL), water (2x2 mL),
methanol (5x2 mL) and used directly in the next experiment.

Ep9: Reduction of Dp9 with BH3-pyridine
The resin obtained in experiment Dp9 was covered with methanol (1 mL) and BH3-
pyridine (150 pL, 8 M in pyridine) was added followed by addition of 50% CCl3CO2H
in water (300 µL). The reaction was left to proceed for 2 h at rt followed by washing
with DMF (5x2 mL), methanol (5x2 mL) and CH2C!2 (5x2 mL). The resin was
used directly in the next step.
Fp9: Tagglng of Ep9 using FITC
FITC (12 mg, 30 pmol) was dissolved in a 1:1 mixture of DMF and methanol (1 mL)
and the solution was added to the resin (Ep9) and left for 2 h at rt followed by exten-
sive washing DMF (5x2 mL), CH2Cl2 (5x2 mL), methanol (5x2 mL) and finally
water (5x2 mL) to remove excess dye. The resin was used directly in the next step.
Gp9: Cleavage of oligosaccharide mixture tagged using FITC from support
The resin obtained in the previous experiment (Fp9) was covered with a 1 M solution
of LiOH (1 mL) and left for 2 h. The liquld was collected from the beads by suction
followed by washing of the beads with water (3 x 3 mL). The collected liquld and
washings were pooled and pH was adjusted to neutral with 10% AcOH. The strong
yellow solution was adsorbed on a Sep-Pak column (350 mg), washed with water
(10 mL) and eluted with methanol (3 mL). The presence of all 6 tagged oligosaccha-
rides was confirmed by MS (ES) m/z = 881 (G2, MH+), 1043 (G3, MH+), 1205 (G4,
MH+), 1367 (GS, MH+), 1529 (G6, MIT), 1691 (G7, MH+) and the profile of the mix-
ture was recorded by CE (Fig. 15).
4.2.6 Capture and processing of oligosaccharides released from ribonuclease
B.
Cp10: Capture and processing of oligosaccharides from RNAse B (10) on Bp
Crude oligosaccharides from PNGase F digestion of RNAse B (Sigma, R-7884)
were used after protein removal on a Centricon-10 concentrator (Millipore) followed
by carbohydrate purification on a Carbograph SPE column (150 mg bed welght;
Scantec Lab). A solution was made by dissolving crude oligosaccharides from

RNAse B (10)2 (300 ug, app. 0.2 µmol) in a mixture of DMSO containing 0.9 M cltric
acld and THF 2:1 (100 µL). This mixture was added to PEGA resin Bp (5 mg, 1.0
µmol) and incubated at 60°C over night. The resin was washed several times: DMF
(5 x 0.3 mL), methanoi (5 x 0.3 mL) and used directly in the next experiments.
Dp10: Capping of Cp10 with acetic anhydride
All the resin obtained in experiment Cp10 was treated with a 1:1 mixture of AC20 and
methanol (0.2 mL) for 1 h followed be washing with DMF (5 x 0.3 mL), water (2 x 0.3
mL), methanol (5 x 0.3 mL) and used directly in the next experiment.
Ep10: Reduction of Dp10 with BH3-pyridine
The resin obtained in experiment Dp10 was covered with methanol (0.2 mL) and
BH3-pyridine (10 pL, 8 M in pyridine) was added followed by addition of 50%
CCl3CO2H in water (20 pL). The reaction was left to proceed for 2 h at rt followed by
washing with DMF (5 x 0.3 mL), methanol (5 x 0.3 mL) and CH2Cl2 (5 x 0.3 mL).
The resin was used directly in the next step.
Fp10: Tagglng of Ep10 using FITC
FITC (1.9 mg, 5 pmol) was dissolved in a mixture of DMF and methanol (1:1, 0.2
mL) and the solution was added to the resin (Ep10) and left for 2 h at 60° followed
by extensive washing DMF (5 x 0.3 mL), CH2Cl2 (5 x 0.3 mL), methanol (5 x 0.3 mL)
and finally water (5 x 0.3 mL) to remove excess dye. The resin was used directly in
the next step.
Gp10: Cleavage of oligosaccharides from RNAse tagged using FITC from sup-
port
The resin obtained in the previous experiment (Fp10) was covered with a 1 M solu-
tion of LiOH (0.2 mL) and left for 2 h. The liquld was collected from the beads by
suction followed by washing of the beads with water (3 x 0.5 mL). The collected liq-
uld and washings were pooled and pH was adjusted to neutral with 10% AcOH. The
yellow solution containing the desired product was adsorbed on a Sep-Pak column
(50 mg), washed with water (2 mL) and eluted with methanol (0.5 mL). The profile of
the labelled oligosaccharides was analysed by CE. The CE (Fig. 16) indicates the
presence of several oligosaccharides and some unidentified contaminants. The

identity of at least one of the known components was confirmed by MS (ES) m/z =
1775 (Man5GlcNAcGlcNAcCHz-N-(R)-TAG, MH+).
4.3 Capture and processing of representative reducing sugars on CPG sup-
ports.
4.3.1 Capture and processing of 2 on B1
C12: Capture of galactose (2) on B1
B1 (20 mg, 0.6 µmol) was treated with 2 (6.6 µL, 1 mg/mL water, 0.03 µmol) in clt-
rate-phosphate buffer (113 µL) and left over night at 55°C. The beads were trans-
ferred to a syringe and washed with water (3 x 0.5 mL) and ethanol (3 × 0.5 mL)
glving C12.
D12: Capping of C12 with acetic anhydride
C12 (0.6 µmol) were capped with 50% AC20 in ethanol for 15 min at rt and washed
with ethanol (3 x 0.5 mL) glving D12.
E12: Reduction of D12 with BH3-pyridine
D12 (0.6 µmol) was treated with 100 µL of a solution of BH3-pyridine (25 µL), 50%
CCl3CO2H (50 pL) in ethanol (500 µL). The mixture was left for 2 h at rt. The beads
were washed with ethanol (3 × 0.5 mL) glving E12.
F12: Labelling of E12 with TRITC
E12 (0.6 pmol) was treated with TRITC (100 µL of 1.0 mg in 300 µL NMP and 300
uL CH2Cl2) and left for 2 h at rt. The beads were washed with CH2Cl2 (3 × 0.5 mL),
ethanol (3 × 0.5 mL), and water (3 × 0.5 mL) glving F12 (red beads).
G12: Base treatment of F12
F12' (0.6 µmol) was treated with 1 M solution of LiOH (100 µL) for 1 h at rt and the
red solution was isolated and neutralised with 50% AcOH in water glving G12 (red
solution) which were passed through a Sep-Pak column (30% CH3CN in water) and
analysed by MS (775.3, MH+) and CE (Fig. 17).
4.3.2 Capture and processing of 5 on B1

C15: Capture of LNT (5) on B1
B1 (20 mg, 0.6 µmol) was treated with 5 (25 µL, 2 mg/mL water, 0.03 umo!) in clt-
rate-phosphate buffer (113 µL) and left over night at 55°C, The beads were trans-
ferred to a syringe and washed with water (3 × 0.5 mL) and ethanol (3 × 0.5 mL)
glving C15.
D15: Capping of C15 with acetic anhydride
C15 (0.6 µmol) was treated with 50% AC20 in ethanol for 15 min at rt and washed
with (3 × 0.5 mL) glving D15.
E15: Reduction of D15 with BH3-pyridine
D15 (0.6 µmol) was treated with 100 µL of a solution of BH3-pyridine (25 µL), 50%
CCl3CO2H (50 µL) in ethanol (500 µL). The mixture was left for 2 h at rt. The beads
were washed with ethanol (3 x 0.5 mL) glving E15.
F15: Labelling of E15 with TRITC
E15 (0.6 µmol) was treated with TRITC (100 µL of 1.0 mg in 300 µL NMP and 300
µL CH2Cl2) and left for 2 h at rt. The beads were washed with CH2Cl2 (3 x 0.5 mL),
ethanol (3 x 0.5 mL), and water (3 x 0.5 mL) glving F'5 (red beads).
G15: Base treatment of F15
The resin was treated with a 1 M solution of LiOH (100 µL) for 1 h at rt and the red
solution was isolated by filtration and the beads were washed with water (3 x 75 µL)
and neutralised with 50% AcOH in water glving G15 (red solution) which were
passed through a Sep-Pak column (30% CH3CN in water) and analysed by MS (ES)
m/z = 1300.6 (M-H+), 1302.4 (MH+) and by CE (Fig. 18).
Alternatively, E15 could be labelled with 1- fluoro-2,4-dinitrobenzene (Sanger's re-
agent, (Fig. 8) as follows. The resin was treated with Sanger's reagent (20 eq, 0.4
µL, Sigma) and TEA (10 eq, 0.2 µL) in ethanol (70 µL) for 2 h at 55°C. The beads
were washed with ethanol (3 x 0.5 mL), CH2Cl2 (3 x 0.5 mL), ethanol (3 x 0.5 mL),
and water (3 x 0.5 mL) (yellow beads), then treated with 1 M solution of LiOH (70
µL) for 1 h at rt (brown solution). The solution was collected by filtration and the
beads were washed with water (3 x 50 µL). The mixture was neutralised with 50%

AcOH (yellow solution). The mixture was passed through a Sep-Pak column with
30% CH3CN in water. MS (ES) m/z = 1023.1 (M-H+).
4.3.3 Capture and and processing of mixture 8 on B1
C18: Capture of Galactose (2) and LNT (5) on B1
B1 (20 mg, 0.6 µmol) was treated with 2 (6.6 pL, 1 mg/mL water, 0.03 pmol), 5 (25
pL, 2 mg/mL water, 0.03 µmol), cltrate-phosphate buffer (100 pL), and left over night
at 55°C. The beads were washed with water (3 × 0.5 mL) and ethanol (3 × 0.5 mL)
glving C18.
D18: Capping of C18 with acetic anhydride
The remaining hydroxylamines in C18 (0.6 µmol) were capped with 50% AC20 in
ethanol for 15 min at rt and washed with ethanol (3 × 0.5 mL) glving D18.
E18: Reduction of D18 with BH3-pyridine
D18 (0.6 µmol) was treated with 100 pL of a solution of BH3-pyridine (Fluka, 25 pL),
50% CCl3CO2H (50 pL) in ethanol (500 pL). The mixture was left for 2 h at rt. The
beads were washed with ethanol (3 × 0.5 mL) glving E18.
F18: Labelling of E18 using TRITC
E18 (0.6 µmol) was treated with TRITC (100 pL of 1.0 mg in 300 pL NMP and 300
pL CH2Cl2) and left for 2 h at rt glving F18. The beads were washed with CH2Cl2 (3 ×
0.5 mL), ethanol (3 x 0.5 mL), and water (3 x 0.5 mL) (red beads).
G18: Base treatment of F18
F18 was treated with 1 M solution of LiOH (100 µi) for 1 h at rt and the red solution
was isolated and neutralised with 50% AcOH in water glving G18 (red solution)
which were passed through a Sep-Pak column (30% CH3CN in water) and analysed
by CE (Fig. 19).

5. Reaction of immobilized oligosaccharides with enzymes
5.1 Reaction of an immobilized tagged oligosaccharide with a glycosidase
5.1.1 Reaction of immobilized lacto-N-tetraose (LNT, 5) of structure F (cap = acetyl,
TAG = TMR) with beta-galactosidase (bovine testes, SIGMA product G-4142,
1U/mL) on CPG supports with none (F°5), one (F15) and two (F25)spacers. All 3
immobilized oligosaccharides were prepared essentially as described for F15 (sec-
tion 4.3.2).
The solid supports (5 mg) were incubated with beta-galactosidase (100 ul_ of 0.2
U/mL solution in 0.1 M cltrate/phosphate buffer pH 5.0 containing 0.2% BSA for 23 h
at 37°C, and the resin was then washed with 3 x water, 3 × ethanol, 3 × CH2Cl2, 3 x
Et ethanol OH, and 3 x water. The beads were treated with 1 M solution of LiOH (60 3
µL) for 1 h at rt glving products of the general structures G°5, G15, and G25 in solu-
tion. Each red solution was collected by filtration. The filtrate was neutralised with
50% AcOH and analysed using CE.
Fig. 20 shows that there was no detectable cleavage of galactose from LNT for F°5,
39% conversion for F15 (i.e. 39% of the tetrasaccharide had lost the terminal Gal
residue and been converted to the trisaccharide) and 83% conversion for F25. The
nature of the spacer was therefore found to be important to the course of the en-
zyme reaction.
5.1.2 Reaction of immobilized maltotriose F24 (cap = acetyl, TAG = TMR) with glu-
coamylase 2 from Asperglllus niger (kindly provided by Dr. Birte Svensson, Carls-
berg Laboratories) on CPG support with two spacers. F24 was prepared essentially
as described for F15 (section 4.3.2) but using maltotriose (G3, Fig. 2) as the reduc-
ing sugar and B2 as the solid support. F24 (ca 5 mg) was incubated for 23 h at 37°C
with 50 µL of 0.1 mg/mL of enzyme in 0.1 M sodium acetate buffer pH 5.5 contain-
ing 0.2% BSA. After washing and cleavage as described above, the product was
analyzed by CE (Fig. 21), which showed complete conversion of immobilized la-
belled maltotriose to a new peak eluting between labelled maltotriose and glucose,
therefore assigned as the maltobiose (G2) TMR adduct.

5.2 Reaction of an immobilized untagged oligosaccharide with a glycosidase and
capture of the released reducing monosaccharide on the same support.
Reaction of immobilized LNT of structure C25 (non-reduced, non-capped, non-
tagged) with beta-galactosidase (bovine testes) was carried out on CPG solid sup-
port with two spacers. C25 was prepared essentially as described for C15 (section
4.3.2). Prior to use, the enzyme solution was freed from small-molecule contami-
nants by repeated centrifugation using a Microcon YM-3 centrifugal filter device (Mil-
lipore). C25 (5 mg) was incubated for 23 h at 37°C with 55 µL of 0.9 U/mL of enzyme
in 0.1 M cltrate/phosphate, pH 5.0, containing 0.2% BSA, and then a further 20 h at
55CC to permit capture of released galactose. The solid was washed, reduced,
capped with acetic anhydride, tagged using TRITC and cleaved with LiOH as de-
scribed above for the conversion of C15 to G15. The CE of cleaved product is shown
in Fig. 22 which shows the presence of unreacted LNT (32%) and similar amounts
of both the TMR-labelled product trisaccharide and cleaved galactose. This experi-
ments confirms the capture of cleaved sugar on the same uncapped support from
which it was cleaved.
6. Variation of capping agents
6.1. Capping of C to produce D
A selection of capping agents was used to effect the conversions C goes to D (Fig.
1). C22 was used as the substrate (where the solid was CPG with 2 spacers and the
captured sugar was galactose). The amino groups on C were then capped with,
among others, acetic anhydride, benzoic anhydride, tricholoracetic anhydride and
dibromoxylene (Fig. 6). The capping was carried with 50% solutions of the capping
agent in ethanol, for 15-120 min at it The samples were then processed as de-
scribed for the conversion of C12 to G12 (section 4.3.1), i.e., reduction, labelling us-
ing TRITC, base-cleavage and analysis by CE. The results are shown in Fig. 23
which shows that all conditions provided the target TMR-labelled galactose (com-
pound 21, Fig. 5) with varylng amounts of other impurities appearing before com-
pound 21 in the electropherogram.

6.2 ExampJe of capping of Cred to produce E
C22 from section 6.1 above was reduced with BH3-pyridine as described for the con-
version of D12 to E12 above (section 4.3.1). The product CreCl22 differs from E12 in
that it contains uncapped NH2 groups. Cred22 (5 mg) was reacted with benzoic acld
NHS-ester (0.4 mg, 1.75 µmol) and TEA (1.0 µL) in DMF (50 pL) over night at 60°C.
The product of the reaction having the general structure E22 (with the cap being a
benzoate) was then washed and processed as usual, by tagglng using TRITC,
cleavage and analysis by CE. Fig. 24 shows the product to be substantially the
same as that formed by the sequence C goes to D goes to E and on to G. The iden-
tity of the product was confirmed by its MS (ES) m/z = 775.0 (Mt-f).
7. Example of the use of a tether: E goes to H goes to I goes to J (Fig. 1)
Synthesis of 29 as example of X-tether-YP
29: 4-lsothiocyanato-benzyl)-carbamic acld 9W-fluoren-9-ylmethyl ester
To a solution of 4-aminobenzylamine (0.93 mL, 8.20 mmol) in anhydrous CH2Cl2 (20
mL) was added TEA (1.15 mL, 8.27 mmol) followed by a solution of Fmoc-N-
hydroxysuccinimide ester (2.48 g, 7.35 mmol) in dry CH2Cl2 (10 mL). After 30 min of
stirring, CH2Cl2 (100 mL) was added and the mixture was washed successively with
sat. aq. NaHCO3 (2 x 50 mL) and brine (50 mL), and dried (Na2SO4). The solvent
was removed under reduced pressure and the residue purified by dry column vac-
uum chromatography (0-60% EtOAc in n-heptane) to yleld the Fmoc-protected ma-
terial (4-Amino-benzyl)-carbamic acld 9/-/-fluoren-9-ylmethyl ester (2.30 g, 91%). 1H-
NMR (250 MHz, DMSO-d6) 5 = 4.03 (2H, d, J = 5,3 Hz), 4.22 (1H, t, J = 6,8 Hz),
4.33 (2H, d, J = 6,8 Hz), 4.95 (2H, s), 6.53 (2H, d, J = 8.3 Hz), 6.92 (2H, d, J = 8.2
Hz), 7.29-7.44 (4H, m), 7.64-7.72 (3H, m), 7.88 (2H, d, J = 7.3 Hz). 13C-NMR (63
MHz, DMSO-d6) 5 = 43.97, 47.19, 65.65,114.09, 120.46, 121.75, 125.58,127.11,
127.42,127.96, 128.47,129.30, 141.13, 144.32,147.89, 156.63. MS(ES)m/z =
345 (MH+).
A solution of (4-Amino-benzyl)-carbamic acld 9H-fluoren-9-ylmethyl ester (718 mg,
2.09 mmol) in CH2Cl2 (30 mL) was added dropwise to a solution of thiophosgene
(199 \il, 2.61 mmol) in a CH2Cl2-water mixture (40 mL, 1:1, v/v). After the mixture
was stirred over night, the organic phase was isolated and dried (Na2SC>4). The sol-

vent was removed under reduced pressure and the residue purified by dry column
vacuum chromatography (0-100% CH2Cl2 in n-heptane) to yleld 29 (643 mg, 80%).
1H-NMR (250 MHz, DMSO-d6) S = 4.18-4.25 (3H, m), 4.38 (2H, d, J = 6.7 Hz), 7.25-
7.45 (8H, m), 7.69 (2H, d, J= 7.3 Hz), 7.87-7.90 (3H, m). ,3C-NMR (63 MHz,
DMSO-d6) δ = 43.64, 47.19, 65.70, 115.55, 120.48, 125.15,125.49, 126.20, 127.42,
127.98, 128.72, 128.83, 133.55, 136.29, 140.26, 141.16, 144.23, 156.74. MS (ES)
m/z = 387 (MH+).
Hp5: Attachment of Fmoc-protected amino tether to Ep5 using 29 (Fig. 9)
5 mg of the dried resin (Ep5) (0.2 nmol) was washed a couple of times with CH2Cl2
to ensure proper swelling of the resin. The Fmoc-protected tether (29) (0.8 mg, 2
pmol) was dissolved in DMF (0.2 mL) and added to the resin and left to react for 2 h.
The resin was washed with DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL) and the Fmoc
protecting group was removed under standard conditions (20 % piperidine in DMF,
0.5 ml 2 x 10 min). The resin was used directly in the next experiment after washing
with DMF (5 x 0.5 mL)
lp5: Tagglng of Hp5 using TR1TC
The resin obtained in experiment Hp5, now containing a free primary amino group,
was incubated with TRITC (0.9 mg, 2 µmol) in DMF (0.2 mL) at rt for 2 h followed by
extensive washing with DMF (5 x 0.5 mL), CH2Cl2 (5 x 0.5 mL), methanol (5 x 0.5
mL) and finally water (5 x 0.5 mL) to remove excess dye. The resin was used di-
rectly in the next step.
Jp5: Cleavage of Lacto-N-tetraose tagged using TRITC via an amino tether
The resin obtained in the previous experiment (lp5) was covered with a 1 M solution
of LiOH (0.2 mL) and left for 2 h. The liquld was collected from the beads by suction
followed by washing of the beads with water (3 × 0.5 mL). The collected liquld and
washings were pooled and pH was adjusted to slightly acldic (pH 3-4) with 10%
AcOH. The dark red solution containing the desired product was adsorbed on a
Sep-Pak column (50 mg), washed with water (2 mL) and eluted with methanol (0.5
mL). The identity of the product was confirmed by MS (ES) m/z = 1465 (MH+).
Capillary electrophoresis analysis of labeled carbohydrates

Capillary electrophoresis (CE) was performed using an automated PrinCE 2-lift,
model 560 CE system (Prince Technologles, The Netherlands). Separations were
carried out in an uncoated fused-silica capillary of 75 µm ID with an effective length
in the range 50 -75 cm (plus 30 cm of extra length from the detection window to the
outlet), thermostatically controlled at 25°C. The CE background electrolyte (BGE)
was elther (A) 50 mM borate buffer pH 9.3 containing 150 mM SDS or (B) 0.2 M
borate buffer pH 9.3 containing 0.8% (w/v) γ-CD (Sigma, C-4892). Conditions A
were used for the analyses shown in Figs. 11 and 15-22. Conditions B were used
for the analyses shown in Figs. 10, 13, 14, 23 and 24.
The capillary was conditioned at room temperature by rinsing at 2000 mbar for 30
min with 1 M NaOH, 10 min with water, and 10 min with BGE before use. Between
runs the capillary was washed at 2000 mbar for 3 min with 1 M NaOH, 3 min with
water, and 3 min with BGE. Samples were injected hydrodynamically for 6 sec at 50
mbar and electrophoresed across a potential difference of 25 kV. All experiments
were carried out at a normal polarity, i.e. inlet anodic. Detection was carried out us-
ing a fluorescence detector (Argos 250B, Flux Instruments, Switzerland) equlpped
with the appropriate filters. For samples labeled using TRITC, the excltation and
emission filters were respectively 546.1/10 and 570 nm. For samples labeled using
FITC, the excltation and emission filters were respectively UG11 (200-400 nm) and
495 nm.

Abbreviations
The following abbreviations have been used throughout the present application:
AMP CPG Aminopropyl controlled pore glass
BGE Background electrolyte
BSA Bovine serum albumin
CE Capillary electrophoresis
CPG Controlled pore glass
DIPEA N,N-Diisopropylethylamine
DMF N,N-Dimethylformamide
ES Electrospray
FITC Fluorescein isothiocyanate
Fmoc 9-Fluorenylmethyloxycarbonyl
HRMS High resolution mass spectroscopy
LNT Lacto-N-tetraose
MS Mass spectroscopy
NHS N-Hydroxysuccinimide
NMP 1 -methyl-2-pyrrolidone
PEGA Polyethylenglycol acrylamide polymer
RNAse B Ribonuclease B
rt Room temperature
TBTU N,N,N',N'-tetramethyl-O-{1 H-benzotriazol-1 -
yl)uroniumtetrafluorborate
TEA Triethylamine
TMR Tetramethylrhodamine
TRITC Tetramethylrhodamine isothiocyanate

WE CLAlM
1. A method of preparing a reactive sugar, said method comprising the steps of
i. Providing a sample comprising a reducing sugar
ii. Providing a solid support covalently attached to a linker comprising a capture group
comprising an -NH2 group, wherein said linker optionally is attached to said solid support
via a spacer
iii. Reacting said reducing sugar with said -NH2 group, thereby obtaining an immobilised
sugar,
iv. Reacting free -NH2 groups with a capping agent, wherein the capping agent comprises a
reactive group capable of reacting with an -NH2 group;
v. Reducing C=N bonds with a reducing agent;
vi. thereby obtaining an reactive sugar of the structure SugarCHn-NH-linked to a solid
support via a linker and optionally a spacer, wherein n is 1 or 2.
wherein step iv is performed prior to step v.
2. The method as clalmed in clalm 1, wherein the method further comprises the step of
vii. Reacting the -NH- group of the reactive sugar with a derivatising agent comprising an
nitrogen-reactive functional group (X), thereby obtaining a sugar covalently attached to
said agent.
3. The method as clalmed in clalm 2, wherein said nitrogen-reactive functional group is selected
from the group consisting of isothiocyanates, active esters, carboxylic aclds, Michael
acceptors, alpha-beta unsaturated sulfones, alkylating agents, aidehydes, ketones and
substituted haloaromatic groups bearing electronegative groups.
4. The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a
spectroscopically detectable compound derivatised with a nitrogen-reactive functional group.

5. The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a
fluorescent compound derivatised with a nitrogen-reactive functional group.
6. The method as clalmed in any of clalms 4 and 5, wherein said method comprises the step of
viii.detecting said agent attached to the sugar by spectrometry.
7. The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a mass
spectrometry TAG derivatised with a nitrogen-reactive functional group, wherein the mass
spectrometry TAG is capable of improving the detection and/or structural charaterisation of a
sugar.
8. The method as clalmed in clalm 7, wherein the mass spectrometry TAG is a molecule
comprising bromine.
9. The method as clalmed in clalm 7, wherein the mass spectrometry TAG is a charged
molecule.
10.The method as clalmed in clalm 7, wherein the mass spectrometry TAG is an isotope labelled
molecule.
11.The method as clalmed in any of clalms 7 to 10, wherein the method comprises the step of
ix. detecting said mass spectrometry TAG attached to said sugar by mass spectrometry
12.The method as clalmed in any of clalms 2 and 3, wherein said derivatising agent is a first
binding partner capable of speclfic interaction with a second binding partner, and wherein
said first binding partner is derivatised with a nitrogen- reactive functional group.

13.The method as clalmed in clalm 12, wherein one binding partner is a protein and the other
binding partner is a ligand of said protein.
14.The method as clalmed in clalm 12, wherein one binding partner comprises an epitope and
the other binding partner is an antibody speclfically recognising said epitope.
15.The method as clalmed in clalm 12, wherein one binding partner is biotin and the other
binding partner is an avidin.
16.The method as clalmed in any of clalms 12 to 15, wherein the second binding partner is
conjugated to a detectable label.
17.The method as clalmed in any of clalms 2 and 3, wherein the derivatising agent is a nuclelc
acld derivatised with a nitrogen-reactive functional group or a protected nitrogen reactive
functional group.
18.The method as clalmed in clalm 17, wherein said nuclelc acld is a DNA.
19.The method as clalmed in any of clalms 17 to 18, wherein the method comprises the step of
x. detecting said nuclelc acld attached to said sugar
20.The method as clalmed in clalm 19, wherein said nuclelc acld is detected by an essentially
complementary nuclelc acld conjugated to a detectable label.
21.The method as clalmed in clalm 19, wherein detection of said nuclelc acld involves
amplification of the nuclelc acld.

22.The method as clalmed in any of clalms 2 and 3, wherein said agent is a bifunctional reagent
of the structure X- tether-Y or X-tether-Yp, wherein X is a nitrogen-reactive functional group
and Y is a second reactive functional group and Yp is a protected reactive group Y.
23.The method as clalmed in clalm 22, wherein said second reactive functional group Y is
selected from the group consisting of, thiols, carboxyl groups, activated carboxyl groups,
disulfides, activated disulfides, alkylating agents, alkenes, alkynes, aidehydes, ketones and
azides or Yp is selected from the group consisting of protected derivatives of aforementioned
groups Y and protected amines.
24.The method as clalmed in any of clalms 22 and 23, wherein the method further comprises
the steps of:
xi) providing a second derivatising agent comprising a functional group (Z) capable of
reacting with Y
xii) reacting the functional groups Z and Y, thereby covalently attaching the second
derivatising agent to the sugar via a tether and the first derivatising agent.
25.The method as clalmed in clalm 24, wherein the second derivatising agent is selected from
the group consisting of drugs, imaglng agents, peptides, polypeptides, proteins, enzymes,
nuclelc aclds, spectroscopically detectable compounds, mass spectrometry TAGs and first
binding partners capable of speclfic interaction with a second binding partner.
26.The method as clalmed in any of clalms 22 and 23, wherein the method further comprises
the steps of:
xiii) providing a particle selected from the group consisting of microbial organism, micelles,
phages, vira and nanoparticles, wherein the particle comprises a functional group (Z)
capable of reacting with Y.
xiv) reacting the functional groups Z and Y, thereby covalently attaching the particle to the
sugar via the tether and the agent.

27.The method according to clalm 1, wherein the method comprises the steps of
xv) contacting the sugar with a detection agent capable of assoclating with said sugar
xvi) detecting the detection agent
28.The method as clalmed in clalm 27, wherein said detection agent comprises aryl boronate or
heteroarylboronate.
29.The method as clalmed in clalm 27, wherein the detection agent is a polypeptide.
30.The method as clalmed in clalm 29, wherein said polypeptide is selected from the group
consisting of lectins, selectins, toxins, receptors, antibodies and enzymes.
31.The method as clalmed in any of the preceding clalms, wherein the capture group comprises
or consists of the structure M-NH2 wherein M is a heteroatom.
32.The method as clalmed in any of the preceding clalms, wherein the linker is a non-cleavable
linker selected from the group consisting of alkyls, aryls, ethers and amides, wherein any of
the aforementioned may optionally be substituted.
33.The method as clalmed in any of clalms 1 to 31, wherein the linker is a cleavable linker.
34.The method as clalmed in clalm 33, wherein the linker is cleavable by reaction with acld,
base, nucleophiles, electrophiles, oxidation, reduction, free radicals, light, heat or enzymes.
35.The method as clalmed in any of clalms 33 and 34, wherein the method comprises the step
of cleaving said cleavable linker thereby releasing the sugar, wherein this step may be
performed subsequent to step v, vi, vii, viii or ix.
36.The method as clalmed in any of the preceding clalms, wherein the linker is attached to said
solid support via a spacer.

37.The method as clalmed in clalm 36, wherein the spacer is in the range of 0 to 1000 atoms
long and optionally branched.
38.The method as clalmed in any of the preceding clalms, wherein the solid support is selected
from the group consisting of polymers, solids, insoluble particles and surfaces.
39.The method as clalmed in any of the preceding clalms 1 to 37, wherein the solid support is a
sensor.
40.The method as clalmed in any of the preceding clalms, wherein the method comprises the
step of contacting the sugar with one or more glycosidases, thereby generating a new
reducing sugar, provided that the first sugar is a substrate for said glycosidase(s).
41.The method as clalmed in clalm 40, wherein the method comprises the step of immobilising
newly generated reducing sugars on a solid support.
42.The method as clalmed in any of the preceding clalms, wherein the method comprises the
step of contacting the sugar with one or more enzymes selected from the classes of
glycosyltransferases, sulfatases, phophorylases, sulfotransferases, phosphotransferases,
glycosynthases and transglycosidases, thereby converting said sugar into a new structure.
43.The method as clalmed in any of the clalms 40 to 42, comprising detecting newly generated
sugars or structures.
44.The method as clalmed in any of the preceding clalms, wherein the reducing agent is a
borane or borohydride comprising a BH bond or a silane comprising a SiH bond.

ABSTRACT

Title : SOLID-PHASE OLIGOSACCHARIDE TAGGlNG: A TECHNIQUE
FOR MANIPULATION OF IMMOBILIZED CARBOHYDRATES

The invention relates to methods of manipulating immobilized carbohydrates by derivatisation. Depending on the nature of the derivatisation, the carbohydrate may
thereby be more easily detected and/or identified or handled. In particular, the ivention relates to methods of preparing a reactive sugar comprising the steps of: i) providing a sample comprising a reducing sugar; (ii) providing a solid support covalently
attached to a linker comprising a capture group comprising an - NH2 group, wherein
said linker optionally is attached to said solid support via a spacer; iii) reacting said
reducing sugar with said -NH2 group, thereby obtaining an immobilized sugar; iv)
reacting free -NH2 groups with a capping agent, wherein the capping agent com-prises
a reactive group capable of reacting with an -NH2 group; and v) reducing C=N bonds
with a reducing agent, thereby obtaining an reactive sugar of the struc-ture SugarCHn-
NH-linked to a solid support via linker and optionally a spacer, wherein n is 1 or 2.

Documents:

03342-kolnp-2007-abstract.pdf

03342-kolnp-2007-claims.pdf

03342-kolnp-2007-correspondence others.pdf

03342-kolnp-2007-description complete.pdf

03342-kolnp-2007-drawings.pdf

03342-kolnp-2007-form 1.pdf

03342-kolnp-2007-form 2.pdf

03342-kolnp-2007-form 3.pdf

03342-kolnp-2007-form 5.pdf

03342-kolnp-2007-gpa.pdf

03342-kolnp-2007-international publication.pdf

03342-kolnp-2007-international search report.pdf

03342-kolnp-2007-pct priority document notification.pdf

03342-kolnp-2007-pct request form.pdf

03342-kolnp-2007-translated copy of priority document.pdf

3342-KOLNP-2007-(15-03-2013)-ABSTRACT.pdf

3342-KOLNP-2007-(15-03-2013)-CLAIMS.pdf

3342-KOLNP-2007-(15-03-2013)-CORRESPONDENCE.pdf

3342-KOLNP-2007-(15-03-2013)-DESCRIPTION (COMPLETE).pdf

3342-KOLNP-2007-(15-03-2013)-DRAWINGS.pdf

3342-KOLNP-2007-(15-03-2013)-FORM 1.pdf

3342-KOLNP-2007-(15-03-2013)-FORM 2.pdf

3342-KOLNP-2007-(15-03-2013)-FORM 3.pdf

3342-KOLNP-2007-(15-03-2013)-OTHERS.pdf

3342-KOLNP-2007-(15-03-2013)-PETITION UNDER RULE 137.pdf

3342-KOLNP-2007-CANCELLED PAGES.pdf

3342-KOLNP-2007-CORRESPONDENCE.pdf

3342-KOLNP-2007-EXAMINATION REPORT.pdf

3342-kolnp-2007-form 18.pdf

3342-KOLNP-2007-GPA.pdf

3342-KOLNP-2007-GRANTED-ABSTRACT.pdf

3342-KOLNP-2007-GRANTED-CLAIMS.pdf

3342-KOLNP-2007-GRANTED-DESCRIPTION (COMPLETE).pdf

3342-KOLNP-2007-GRANTED-DRAWINGS.pdf

3342-KOLNP-2007-GRANTED-FORM 1.pdf

3342-KOLNP-2007-GRANTED-FORM 2.pdf

3342-KOLNP-2007-GRANTED-FORM 3.pdf

3342-KOLNP-2007-GRANTED-FORM 5.pdf

3342-KOLNP-2007-GRANTED-SPECIFICATION-COMPLETE.pdf

3342-KOLNP-2007-INTERNATIONAL PUBLICATION.pdf

3342-KOLNP-2007-INTERNATIONAL SEARCH REPORT & OTHERS.pdf

3342-KOLNP-2007-OTHERS.pdf

3342-KOLNP-2007-PETITION UNDER RULE 137.pdf

3342-KOLNP-2007-REPLY TO EXAMINATION REPORT.pdf

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Patent Number

256776

Indian Patent Application Number

3342/KOLNP/2007

PG Journal Number

31/2013

Publication Date

02-Aug-2013

Grant Date

29-Jul-2013

Date of Filing

10-Sep-2007

Name of Patentee

MERCK PATENT GMBH

Applicant Address

FRANKFURTER STRASSE 250, 64293 DARMSTADT

Inventors:

#	Inventor's Name	Inventor's Address
1	LOHSE, ANDERS	ØSTERBROGADE 87, 3.TV. 2100 COPENHAGEN Ø
2	MARTINS, RITA	VILDGASVAGEN 25A, LGH. 8 227 35 LUND
3	HINDSGAUL OLE	GAMLE CARLSBERG VEJ 15 2500 VALBY
4	JØRGENSEN, MALENE RYBORG	SNORRESGADE 4,5. TH. 2300 COPENHAGEN

PCT International Classification Number

G01N 33/543

PCT International Application Number

PCT/DK2006/000066

PCT International Filing date

2006-02-08

PCT Conventions:

#	PCT Application Number	Date of Convention	Priority Country
1	PA 2005 00209	2005-02-11	Denmark
2	60/652,247	2005-02-11	Denmark