Title of Invention

"A PEPTIDE OF FORMULA (I) AND THE PHARMACEUTICAL COMPOSITION COMPRISING SAID PEPTIDE"

Abstract A peptide of formula I: wherein a, b, c, d, p, q, x, y and z are as defined in the description that facilitate the intercellular communication medicated by gap junctions. The invention has a wide spectrum of useful applications including use in the treatment of diseases associated with impaired gap junction intracellular communication (GJIC).
Full Text FIELD OF THE INVENTION
The invention relates to orally available dipeptides capable of modulating intracellular gap junctional communication. The invention also relates to methods of using the peptides to modulate such communication, to the use of the peptides for the manufacture ofrhedicaments for the prevention and/or treatment of conditions associated with said communication and to pharmaceutical compositions comprising said dipeptides.
BACKGROUND
There is increasing recognition that intercellular communication is essential for cellular homeostasis, proliferation and differentiation. Such communication is believed to be facilitated by gap junctions. These structures are thought to be a route for coupling cells and permiting "cross-talk". See generally, Sperelakis, N., (1989) Cell Interactions and Gap Junctions by N. Sperelakis, William C. Cole (Editor).
There have been efforts to understand the structure and function of gap junctions. For instance, there have been reports that such junctions are a type of complex formed between adjacent cells. Most gap junctions are thought,to consist of aggregated channels that directly link the interiors (cytoplasms) of neighboring cells. In adult mammals, gap junctions are found in most cell types with the exception of circulating blood elements.
More specifically, there is acknowledgement that gap junctions are specialized regions of the cell membrane with clusters of hundreds to thousands of densely packed gap junction channels (comprising two hemichannels or connexins). Many are thought to directly connect the cytoplasmic compartments of two neighboring cells. The gap junction channel can switch between an open and a closed state. In the open state ions and small molecules are thought to pass through the pore. The conduction of electrical impulses and intercellular diffusion of signaling molecules take place through the gap junctions.
The "cross-talk" between gap junctions has been referred to as gap junctional intracellular communication (GJIC), which is believed to play an important role in the regulation of cell metabolism, proliferation, cell-to-cell signaling, and tissue integrity.

For instance, GJIC is thought to permit rapid equilibration of nutrients, ions, and fluids between cells. Gap junctions are also thought to serve as electrical synapses in electrically excitable cells. In many tissues, electrical coupling is thought to permit more rapid cell-to-cell transmission of action potentials than chemical synapses. In cardiomyocytes and smooth muscle cells, for instance, this is thought to assist synchronous contraction.
There have been reports of other functions mediated by GJIC. For example, GJIC is thought to enhance the responsiveness of tissues to external stimuli. Second messengers are generally believed to be small enough to pass from hormonally activated cells to quiescent cells through junctional channels and activate the latter.
Additionally, there have been reports that gap junctions may provide intercellular pathways for chemical and/or electrical developmental signals and assist in defining the boundaries of developmental compartments. It has been disclosed that GJIC occurs in specific patterns in embryonic cells and the impairment of GJIC has been related to developmental anomalies and the teratogenic effects of many chemicals. Further, GJIC is thought to assist co­ordination of cell activities.
Some reports have established a link between abnormalities in GJIC and a range of disease states has been established both in vitro and in vivo. For example, there is thought to be a link between abnormalities in connexins and heart disease. Several studies of the expression and distribution of Cx43 in hearts describe a reduced degree of Cx43 expression and a changed pattern of distribution for this gap junction protein. See Kaprielian, R. R., et al. (1998) Circulation 97: 651-660; and Saffitz, J. E., et a!., (1999) Cardiovasc Res. 42: 309-317.
Accordingly, there is recognition in the field of a relationship between a malfunction or absence of gap junctions and an increased risk of arrhythmias. There is thought to be a further relationship between altered connexin expression/distribution and chronic heart disease.
Attempts to analyze peptides that influence GJIC have been made. For instance, a group of peptides (the antiarrhythmic peptides) have been disclosed with capacity to increase gap junction conductance in the heart. In particular, a hexapeptide with a molecular weight of 470D was reported to have been isolated from bovine atria. In neonatal rat cardiomyocytes,
it was reported that the peptide could convert fibrillation induced by ouabain, calcium, or potassium, to normal rhythm. In addition, the peptide has been reported to convert arrhythmic movement of isolated rat atria induced by the combination of potassium and acetylcholine to normal rhythm. This peptide is often referred to as antiarrhytmic peptide (AAP). See eg., Aonuma, S., et al. (1980) Chem Pharm Bull (Tokyo) 28: 3332-3339
There is increasing understanding that AAP is an important peptide with capacity to modulate GJIC in the heart.
For example, in cell culture, AAP has been shown to increase the number of beating centers, the relative content of spreading cells, and protein synthesis. See Aonuma, S., et al. (1980) Chem Pharm Bull (Tokyo) 28: 3340-3346. In other studies, the antiarrhythmic effect of AAP observed in vitro has been confirmed. It has been reported that AAP is effective against CaCI2-, oubain- and acotinine-induced arrhythmia in mice. See Ronsberg, M.A., et al. (1986) Mod. Sci. 14: 350-351.
The AAP sequence has been disclosed. See eg., Aonuma, S., et al. (1982) JPharmacobiodyn. 5: 40-48.
There have been efforts to prepare a variety of AAP derivatives. See eg., Dikshit, M., et al. (1988) Indian J. Exp. Biol. 26: 874-876; Kohama, Y., et al. (1987) Chem. Pharm. Bull. (Tokyo) 35: 3928-3930; and Kohama, Y., et al. (1988) Chem. Pharm. Bull. (Tokyo) 36: 4597-4599).
For instance, one such derivative, AAP10, is believed to impact GJIC. See Dhein, S., et al. (1994) Naunyn Schmiedebergs Arch Pharmacol. 350: 174-184; and Muller, A., et al. (1997) Eur. J. Pharmacol. 327: 65-72. It has been reported that AAP improves GJIC, reduces action potential dispersion and improves conductance.
There is increasing understanding that many of the antiarrhythmic peptides positively impact GJIC, often without affecting action potential duration or shape. Further, many of such peptides are thought to lack undesirable proarrhythmic side-effects. Such effects are thought to limit the use of many currently available antiarrhythmic drugs. Moreover, AAP, as well as certain AAP derivatives, are thought to have some undesired features, e.g., low stability and a need for high doses before therapeutic efficacy is achieved.
Many potentially important peptides suffer from a lack of acceptable oral availability. That is, the peptides are degraded in the gastrointestinal tract, enterocytes, or both. In such cases, the peptides are often administered to subjects by more painful and less convenient intravenous routes.
There have been attempts to improve the oral availability of certain compounds by
enhancing contact with an intestinal peptide transporter protein called PepTL Much is
known about the PepT1 transporter system. See Bailey, P.O., et al. (2000) Angew. Chem.
Int. Ed. 39: 506; and references cited therein. ti-
lt would be desirable to have more effective peptide modulators of GJIC. It would be especially desirable to have peptide modulators that are orally available.
SUMMARY OF THE INVENTION
The invention generally relates to peptides that modulate gap junction intercellular communication (GJIC). Preferred peptides are orally available. The invention has a wide spectrum of useful applications including use in the treatment or prevention of pathologies associated with impaired GJIC.
TEXT ENDS HERE INTENTIONALLY.
A preferred peptide in accord with the present invention is represented by the following general formula I:
where, if a = 1 then b = 0;
if p = 1 then x and q = 0 and y = 1; and further, wherein,
if r! = H then d = 0-8;
if r! ?t H then d = 0;
wherein ri = side chain of any amino acid: e.g., alanine, arginine, asparagine, aspartic acid, cysteine, glutamic acid, glutamine, glycine, histidine, isoleucine, leucine, lysine, methionine, phenylalanine, proline, serine, threonine, tryptophan, tyrosine, and valine;
R2 = NH2, NHR, NR2, NR3+H, OH, SH, RO, RS, RSO, RSO2, COR, GSR, COOH, COOR, CONH2, CONHR, CONR2, OCOR, SCOR, (R = alkyl, alkenyl, aryl, aralkyl, cycloalkyl, etc.); R3 = H, CH3;and
wherein Rx is a hydrophobic group, and preferably, comprises an aromatic carbon ring, more preferably, comprising a 6- or 12 -membered aromatic carbon ring. In one aspect, the aromatic ring is substituted with at least one of: a lower alkyl, alkoxy, hydroxyl, carb.bxy, amine, thiol, hydrazide, amide, halide, hydroxyl, ether, amine, nitrile, imine, nitro, sulfide, sulfoxide, sulfone, thiol, aldehyde, keto, carboxy, ester, an amide group; including seleno and thio derivatives thereof. Optionally substituted rings also include sulfide, sulfoxide, sulfone, and thiol derivates with, or without, a seleno group. In embodiments in which the aromatic carbon ring is substituted, such substitutions will typically number less than about 10 substitutions, more preferably, substitutions will number about 1 to 5, or 1 to 2 substitutions.
Further, the invention concerns A peptide represented by the general formula II:
0; if a is 0 then b is 1; z is 1-7;
if x is 1 then y and q is 1 and p is 0; if p is 1 then x and q is 0 and y is1; and further, wherein, . if r! is H then d is 0-8; if R1 is not H then d is 0;
wherein R-i is the side chain of an amino acid selected from the group consisting of alanine, arginine, asparagine, aspartic acid, cysteine, glutamic acid, glutamine, glycine, histidine, isoleucine, leucine, lysine, methionine, phenylalanine, proline, serine, threonine, tryptophan, tyrosine, and valine;
wherein R2 is selected from the group consisting of NH2, NHR, NR2, NR^H, OH, SH, RO, RS, RSO, RSO2, COR, GSR, COOH, COOR, CONH2, CONHR, CONR2, OCOR, and SCOR, wherein R = alkyl, alkenyl, aryl, aralkyl, or cycloalkyl;
wherein R3 = H or CH3;
wherein R4 and R5 are independently selected from the group consisting of H, alkyl, alkenyl, aryl, aralkyl, halogen, CN, NO2, alkoxy, aryloxy, aralkyloxy, thioalkoxy, thioaryloxy, thioaralkyloxy, +S(CH3)2, SO3H, SO2R, NH2, NHR, NR2, +NR3, OH, SH, COOH, COOR, CONH2> CONHR, CONR2, CH2OH,. NCO, NCOR, NHOH, NHNH2, NHNRH, CH2OCOR, CH2OCSR, COR, CSR, CSOR, CF3, and CCI3, and wherein R is alkyi, alkenyl, aryl, aralkyl, or cycloalkyl.
Such peptides may also comprise a peptide bond that is alkylated or otherwise modified to stabilize the peptide against enzymatic degradation and/or may comprise D-amino acids.
More preferred peptides as represented by Formula I and II are orally available to a mammal, and particularly, to a human subject. Various assays to establish oral availability are known in the field and include, but are not limited to, the following specific tests.
Oral availability assays
One assay ("the Bailey assay") is a predictive assay and is generally followed in accordance with the invention by other empirical assays, described further below. In the Bailey assay, candidate peptides are virtually aligned with a substrate template that is modeled to represent a compound, which binds to PepT1, to identify peptides likely to bind to PepT1 in vitro and in vivo. The Bailey assay can be used to facilitate detection of orally available peptides of the invention.
In one embodiment, the peptides according to Formula I and II are in substantial agreement with this substrate template model (e.g., the peptides show substantially the same three-dimensional conformation as previously identified substrates which bind to hPepTI with high affinity) and therefore are good candidates for peptides, which are orally available. Thus, such peptides are typically dipeptides.
More preferred dipeptides are those which exhibit at least the following four properties ascribed to high affinity substrates for PepT1; i.e., from the N- to the C-terminus of the peptide, the peptide comprises: 1) a strong binding site for an N-terminal NH3+ group; 2) a hydrogen bond to the carbonyl group of the first peptide bond; 3) a hydrophobic pocket preferably featuring a strong directional vector and 4) a carboxylate binding site. Preferably,
the first carboxylate binding site is followed by a second carboxylate binding site according to the model. See, e.g., Bailey, P.O., et ai, (2000) supra.
One empirical assay to validate the predictive Bailey assay described above, is a "standard in vivo oral availability assay". In this assay, a peptide is orally administered to a mammal and blood samples are taken over time. The concentration of the peptide is determined at different time intervals using standard quantitation assays such as LC/MS/MS to calculate an area under the curve (AUC) from a plot of plasma protein concentration vs. time, using routine methods known in the art. Preferably, different doses of peptides are administered to a plurality of animals in parallel to identify those peptides that show a dose-proportional increase in maximum plasma concentration and AUC values. As a control, the same concentrations of peptide may be administered intravenously and the area under AUC obtained for oral administration can be compared to the AUC obtained for intravenous administration. See, e.g., Milo Gibal (1991) Biopharmaceutics and Pharmacology, 4th edition (Lea and Sediger). In a preferred embodiment peptides with good oral availability are those, in which the dose normalised AUC after oral administration represents at least 20% of the dose normalised AUC after intravenously administration.
Peptides which show good oral availability according to the standard in vivo oral availability assay described above, may or may not be in substantial agreement with the Bailey assay.
It will often be useful to perform a second empirical assay to further validate orally available peptides as represented by Formula I or II. In one such assay, the ability of the peptide to bind to the hPepTI transporter or a functionally active fragment thereof is determined. Preferably, peptides according to the invention have good affinity for an hPepTI transporter or a biologically active fragment thereof. Preferably, the Kj of such peptides is less than about 20 mM, more preferably, is less than about 10 mM, and still more preferably, is less than about 5 mM, or less than about 1 mM.
An hPepTI binding assay may be performed as an initial screen for peptides which are then screened for in a standard in vivo oral availability assay and/or may be performed to confirm the results of a standard in vivo oral availability assay; however, the standard in vivo oral availability assay provides the most meaningful test of the peptide oral availability.
Additionally preferred peptides as represented by Formula I above, exhibit a good half-life according to what is referred to herein as an "in vitro plasma stability assay" or related phrase. Such peptides may be in substantial agreement with the foregoing PepT1 substrate template model (Bailey assay). However, for some peptides there may be little or no agreement with the model. Peptides that show a good stability in the assay have in one embodiment a half-life of more than about 48 hours, such as more than 24 hours, for example more than 12 hours, such as more than 6 hours, for example more than 3 hours, such as more than 1 hour, for example more than 30 minutes. In this embodiment, the peptides of the invention show enhanced stability in the bloodstream.
Peptides within the scope of the present invention are in one embodiment represented herein with free N-terminal and/or C-terminal group. These groups may remain free for some invention uses. However, in another embodiment, the peptides can feature blocked C-terminal groups and free N-groups. Alternatively, such peptides may have blocked N-groups and free C-terminal groups, or blocked N- and C-terminal groups. The nature of the terminal groups at either side of the molecule is not critical so long as the peptides are able to bind with satisfactory affinity to hPepTI such that the peptides and/or are orally available. As discussed, "satisfactory affinity" for the hPepTI transporter can be predicted, in advance, by determining if a subject peptide is in substantial agreement with the substrate template model for binding to the hPepTI carrier. See Bailey, P.O., et al. (2000), supra.
Additionally, amino acids residues within the dipeptides may be D- or L-amino acids. In certain aspects, to enhance stability of the compounds, D- amino acids are preferred.
The peptides according to the invention have a wide variety of important uses and advantages.
For instance, such peptides may be used for preventing and/or treating conditions associated with impaired gap junction function resulting in reduced intercellular communication or overcoupling of intercellular communication or misregulated cellular communication and be used for the manufacture of a medicament for preventing an/or treating conditions associated with impaired gap junction function. In one aspect, the invention provides a method of administering to a patient having, or at risk of developing
such a condition, a therapeutically effective amount of any of the peptides described above. Preferably, administration is oral. In one preferred aspect, a patient is a human being.
Examples of conditions which can be treated include, but are not limited to, cardiovascular disease, inflammation of airway epithelium, disorders of alveolar tissue, bladder incontinence, impaired hearing due to diseases of the cochlea, endothelial lesions, diabetic retinopathy and diabetic neuropathy, ischemia of the central nervous system and spinal cord, dental tissue disorders including periodontal disease, kidney diseases, failures of bone marrow transplantation, wounds, erectile dysfunction, urinary bladder incontinence, neuropathic pain, subchronic and chronic inflammation, cancer and failures of bone marrow and stem cell transplantation, conditions which arise during transplantation of cells and tissues or during medical procedures such as surgery; as well as conditions caused by an excess of reactive oxygen species and/or free radicals and/or nitric oxide.
The invention additionally provides pharmaceutical compositions suitable for use in the methods described above, comprising any of the peptides described above and a pharmaceutically acceptable carrier. Preferably, the carrier is sterile, pyrogen-free and virus-free. Still more preferably, the composition is orally adminstrable.
BRIEF DESCRIPTION OF THE DRAWINGS
Figures 1A and 1B show exemplary synthesis schemes for generating peptides according to certain aspects of the invention.
Figure 2 shows the effect of Compound 4, Compound 22, Compound 23 and Compound 95 on ALP (Alkaline Phosphatase) in human osteoblasts.
DETAILED DESCRIPTION OF THE INVENTION
As discussed, the invention relates to orally available peptides that modulate gap junction intercellular communication (GJIC). The invention has a wide spectrum of useful applications including use in the treatment or prevention of pathologies associated with impaired GJIC. Particular invention peptides are represented by Formula I above.
More specific peptides according to the invention are represented by the following general formula II:
where, if a = 1 then b = 0; if a = 0 then b= 1; z=1-7;
if x = 1 then y and q = 1 and p = 0; if p = 1 then x and q = 0 and y = 1; and further, wherein, if Ri = H then d = 0-8; if r! * H then d = 0;
where Rt = side chain of any amino acid: e.g., aianine, arginine, asparagine, aspartic acid, cysteine, glutamic acid, glutamine, glycine, histidine, isoleucine, leucine, lysine, methionine, phenylalanine, praline, serine, threonine, tryptophan, tyrosine, and valine;
R2 = NH2, NHR, NR2, NR3+H, OH, SH, RO, RS, RSO, RSO2, COR, CSR, COOH, COOR, CONH2, CONHR, CONR2, OCOR, SCOR, (R = alkyl, alkenyl, aryl, aralkyl, cycloalkyl, etc.);
R3 = H, CH3;
R4 and R5 are independently selected from the group consisting of H, alky], alkenyl, aryl, aralkyl, halogen, CN, NO2, alkoxy, aryloxy, aralkyloxy, thioalkoxy, thioaryloxy, thioaralkyloxy, +S(CH3)2, SO3H, SO2R, NH2, NHR, NR2, +NR3, OH, SH, COOH, COOR, CONH2l CONHR, CONR2, CH2OH,. NCO, NCOR, NHOH, NHNH2, NHNRH, CH2OCOR, CH2OCSR, COR, CSR, CSOR, CF3, and CCI3, (R=alkyl, alkenyl, aryl, aralkyl, cycloalkyl, etc.).
As discussed, the peptide can include a free N-terminal, or a free C-terminal, or both.
Preferably, the peptide comprises at least one hydrophobic group and at least one hydrogen bond group. In one aspect of the invention the three dimensional structure of the peptide the distance between the at least one hydrophobic group and the at least one hydrogen bonding group is from about 4 Angstroms to about 12 Angstr0ms, preferably 5 to about 10 Angstr0ms. More preferably, the hydrophobic group is an aromatic group, including, but not limited to, a benzoyl or benzyl group, or substituted, or modified forms thereof. Substituted benzoyl or benzyl groups preferably comprise substituents at the 4- position. More preferably, the substitutents have a radius of 3-11 Angstr0ms in the sphere taken up by the substitutent. Suitable substituents include, but are not limited to: methyl, ethyl, t-butyl, c-hexyl, phenyl, n-butyl, n-hexyl, n-octyl, ethoxy, t-butoxy, phenoxy, butoxy, benzyloxy, n-hexyloxy, n-octyloxy.
More specific peptides within the scope of the invention and having this general formula are shown in Table 1.
Table 1
Compound
No Compound Name
H-Gly-Lys(4-nitrobenzoyl)-OH
H-Gly-Lys(4-fluorobenzoyl)-OH
H-Gly-Lys(4-cyanobenzoyl)-OH
4 H-Gly-Lys(4-methoxybenzoyl)-OH
' 5 H-Gly-Lys(4-chlorobenzoyl)-OH
H-Gly-Lys(benzoyl)-OH
H-Lys(4-nitrobenzoyl)-GIy-OH
H-Lys(4-nitrobenzoyl)-Sar-OH
9 H-Lys(benzoyl)-Sar-OH
10 H-Lys(benzoyl)-Gly-OH
11 H-Lys(4-methoxybenzoyl)-Gly-OH
12 H-Gly-D-Lys(4-methoxybenzoyl)-OH
H-GIy-D-Lys(4-nitrobenzoyl)-OH
H-Gly-D-Lys(4-fluorobenzoyl)-OH
H-Gly-D-Lys(4-cyanobenzoyl)-OH
16 H-Gly-D-Lys(4-nitrobenzoyl)-OH
H-Gly-D-Lys(benzoyl)-OH
H-Lys(4-fluorobenzoyl)-Gly-OH
H-Lys(4-cyanobenzoyl)-Gly-OH
H-Lys(4-chlorobenzoyl)-Gly-OH
H-D-Lys(4-methoxybenzoyl)-Gly-OH
H-D-Lys(4-nitrobenzoyl)-G ly-OH
H-D-Lys(benzoyO-Gly-OH
H-D-Lys(4-fuorobenzoyl)-Gly-OH
H-D-Lys(4-cyanobenzoyl)-GIy-OH
H-D-Lys(4-chlorobenzoyl)-G ly-OH
H-Lys(4-cyanobenzoyl)-Sar-OH
H-Lys(4-methoxybenzoyl)-Sar-OH
H-Lys(4-fuorobenzoyl)-Sar-OH
H-Lys(4-chlorobenzoyl)-Sar-OH
H-D-Lys(4-cyanobenzoyl)-Sar-OH
H-D-Lys(4-methoxybenzoyl)-Sar-OH
H-D-Lys(4-fuorobenzoyl)-Sar-OH
H-D-Lys(4-chlorobenzoyl)-Sar-OH
H-D-Lys(4-nitrobenzoyl)-Sar-OH
H-D-Lys(benzoyl)-Sar-OH
H-A!a-D-Lys(4-methoxybenzoyl)-OH
H-Val-D-Lys(4-methoxybenzoyl)-OH
H-lle-D~Lys(4-methoxybenzoyl)-OH
H-Leu-D-Lys(4-rnethoxybenzoyl)-OH
H-Phe-D-Lys(4-methoxybenzoyl)-OH
H-Trp-D-Lys(4-methoxybenzoyl)-OH
H-His-D-Lys(4-methoxybenzoyl)-OH
H-Tyr-D-Lys(4-methoxybenzoyl)-OH
H-D-Lys(4-methoxybenzoyl)-A!a-OH
H-D-Lys(4-methoxybenzoyl)-Phe-OH
H-D-Lys(4-methoxybenzoyl)-lle-OH
H-D-Lys(4-methoxybenzoyl)-Leu-OH
H-D-Lys(4-methoxybenzoyl)-Va!-OH
H-D-Lys(4-methoxybenzoyl)-His-OH
H-D-Lys(4-methoxybenzoyl)-Trp-OH
H-D-Lys(4-methoxybenzoyl)-Tyr-OH
H-D-Lys(4-phenoxybenzoyl)-Gly-OH
H-D-Lys(4-t-butylbenzoyl)-Gly-OH
H-D-Lys(4-n-butoxybenzoyI)-G ly-OH
H-D-Lys(4-methylbenzoyl)-Gly-OH
H-D-Lys(4-ethy!benzoyl)-Gly-OH
H-D-Lys(4-n-butylbenzoyl)-G!y-OH
H-D-Lys(4-n-hexylbenzoyl)-Gly-OH
H-D-Lys(4-n-octylbenzoyl)-Gly-OH
H-D-Lys(4-pheylbenzoyl)-Gly-OH
H-D-Lys(4-benzyloxybenzoyl)-Gly-OH
H-D-Lys(4-ethoxybenzoyl)-Gly-OH
H-Asn(NH(4-trifluoromethylbenzyl))-Ala-OH
H-Asn(NH(4-methoxybenzy!))-Ala-OH
H-Asn(NH(4-nitrobenzyl))-Ala-OH
H-Asn(NH(benzyl))-Ala-OH
H-Asn(NH(4-fluorobenzyl))-Ala-OH
H-Asn(NH(4-chlorobenzyl))-Ala-OH
H-Asn(NH(4-cyanobenzyl))-A!a-OH
H-Asn(NH(4-methylbenzyl))-Ala-OH
H-Asn(NH(4-n-butylbenzyl))-Ala-OH
H-Asn(NH(4-t-butylbenzyl))-Ala-OH
H-Asn(NH(4-n-hexylbenzyl))-Ala-OH
H-Asn(NH(4-n-octylbenzyl))-Ala-OH
H-Asn(NH(4-phenylbenzyl))-Ala-OH
H-Asn(NH(4-phenoxybenzyl))-Ala-OH
H-Asn(NH(4-n-butoxybenzyl))-Ala-OH
H-Asn(NH(4-trifluoromethylbenzyl))-D-Ala-OH
H-Asn(NH(4-methoxybenzyl))-D-Ala-OH
H-Asn(NH(4-nitrobenzyl))-D-Ala-OH
H-Asn(NH(benzyl))-D-Ala-OH
H-Asn(NH(4-fluorobenzyl))-D-Ala-OH
H-Asn(NH(4-chlorobenzyl))-D-Ala-OH
H-Asn(NH(4-cyanobenzyl))-D-Ala-OH
H-Asn(NH(4-methylbenzyl))-D-Ala-OH
H-Asn(NH(4-n-butylbenzyl))-D-Ala-OH
H-Asn(NH(4-t-butylbenzyl))-D-A!a-OH
H-Asn(NH(4-n-hexylbenzyl))-D-Ala-OH
H-Asn(NH(4-n-octylbenzy())-D-Ala-OH
H-Asn(NH(4-phenylbenzyl))-D-A!a-OH
H-Asn(NH(4-phenoxybenzy!))-D-Ala-OH
H-Asn(NH(4-n-butoxybenzyl))-D-Ala-OH
94 • H-D-Asn(NH(4-trifluoromethylbenzyl))-Ala-OH
H-D-Asn(NH(4-methoxybenzyl))-Ala-OH
H-D-Asn(NH(4-nitrobenzy!))-Ala-OH
H-Asn(NH(4-methoxybenzyl))-Sar-OH
H-Asn(NH(4-methoxybenzyl))-Leu-OH
H-Asn(NH(4-rnethoxybenzyl))-Phe-OH

H-Gln(NH(4-methoxybenzyl))-Ala-OH
H-Orn(4-methoxybenzoyl)-Gly-OH
H-Gly-Asn(NH(4-methoxybenzyl))-OH
H-D-Lys(2,4-dinitrobenzoyl)-Gly-OH
H-D-Lys(2,4-dimethylbenzoy!)-Gly-OH
H-D-Lys(2,5-dimethy!benzoyl)-G[y-OH
H-D-Lys(3,5-dimethylbenzoyl)-G!y-OH
H-D-Lys(2,4-dichlorobenzoyl)-Gly-OH
H-D-Lys(2,5-dichlorobenzoyl)-Gly-OH
H-D-Lys(4-fluoro-3-nitrobenzoyl)-Gly-OH
H-D-Lys(3-fluoro-4-methylbenzoyl)-Gly-OH
More particular peptides according to the invention in one aspect facilitate and/or maintain or inhibit the intercellular communication mediated by gap junctions. In one embodiment the peptides may be antiarrhythmic peptides which target the same cells targeted by AAP, AAP10, HP5, and/or functional analogs thereof, i.e., the peptides are able to modulate the function of these cells by agonizing or antagonizing the function of AAP, AAP10, HP5, and/or functional analogs thereof. The invention also relates to the preparation and use of pharmaceutical compositions for the treatment of pathologies associated with impaired intercellular gap junctional communication and methods for using these compositions.
Further preferred peptides in accord with the invention show good activity in one or more of the following assays. Although not necessary to identify orally available peptides as represented by Formulae I and II, above, they can be used to further confirm and optionally quantify activity of one or a pool of peptides.
In one embodiment of the invention the peptide is selected from the group consisting of H-Gly-Lys(4-nitrobenzoyl)-OH (Compound 1); H-Gly-l_ys(4-methoxybenzoyl)-OH (Compound 4); H-D-Lys(4-methoxybenzoyl)-Gly-OH (Compound 21); H-D-Lys(4-nitrobenzoyl)Gly-OH (Compound 22); H-D-Lys(4-t-butylbenzoyl)-Gly-OH (Compound 54); and H-D-Asn(NH(4-nitrobenzyl)Ala-OH (Compound 96).
In another embodiment the present peptide is selected from the group consisting of H-D-Lys(benzoyl)Gly-OH (Compound 23) and H-D-Asn(NH(4-methoxybenzyl)Ala-OH (Compound 95).
In yet another embodiment of the invention the peptide is H-Gly-Lys(4-nitrobenzoyl)-OH (Compound 1).
According to the invention in one aspect the peptide is H-Gly-Lys(4-methoxybenzoyl)-OH (Compound 4).
Further, in yet another embodiment the peptide is H-D-Lys(4-methoxybenzoyl)-Gly-OH (Compound 21).
In yet another aspect the peptide is H-D-Lys(4-nitrobenzoyl)Gly-OH (Compound 22). In a further aspect the peptide is H-D-Lys(4-t-butylbenzoyl)-Gly-OH (Compound 54). In still another aspect the peptide is H-D-Asn(NH(4-nitrobenzyl)Ala-OH (Compound 96).
Further, in yet another embodiment the peptide peptide is H-D-l_ys(benzoy!)Gly-OH (Compound 23).
In still another embodiment the peptide is H-D-Asn(NH(4-methoxybenzyl)Ala-OH (Compound 95).
Preferred peptides according to Formulae I and II above show good function as a modulator of gap junctional communication (e.g., as agonists or antagonists). In one aspect the peptides have the function as an antiarrhythmic drug.
In one embodiment the preferred agonist peptides of the invention provide an intracellular conductance (Gj) that is substantially the same as, or is greater than, the Gj of AAP in what is referred to herein as a "standard cardiomyocyte assay".
In another embodiment the preferred antagonist peptides provide a Gj that is less than the Gj of AAP and/or block the ability of AAP to normalize the Gj of an ischemic cell, i.e., to return the Gj to substantially the same values found in non-ischemic cells. In one aspect of the invention the present antagonists provide a Gj that is at least about 40% less than the Gj of AAP, such as at least about 50% less, for example at least about 60% less, such as at least about 70% less, for example at least about 80% less, such as at least 90% less, for example at least 100% less.
The inhibitory properties of the present antagonists are not limited to the relative Gj as described above. In further embodiments and assay types the antagonists may display a different relative Gj. This may further depend on the comparative peptide/compound.
Heart
Additionally preferred peptides according to the invention increase the time to an AV block in a mouse after infusion of CaCI2l in what is referred to herein as a "standard calcium-induced arrhythimia assay". Preferably, the peptides provide at least about 40% of the activity of AAP, for example at least about 50% of the activity of AAP, such as about 60% of the activity of AAP, for example at least about 70% of the activity of AAP, such as at least about 80% of the activity of AAP, for example at least about 90% of the activity of AAP, for example at least about substantially the same activity of AAP, such as about 110% of^the activity of AAP, for example at least about 120% of the activity of AAP, such as at least about 130% of the activity of AAP, for example at least about 140% of the activity of AAP, such as about 150% of the activity of AAP, for example at least about 160% of the activity of AAP, such as at least about 170% of the activity of AAP, for example at least about 180% of the activity of AAP, preferably at least about 190% of the activity of AAP, more preferably at least about 200 or greater % of the activity of AAP (i.e., show time lags of approximately the same duration).
Peptides may additionally show decreases in the incidence of reentry arrhythmias or in the size of an infarct zone observed in what is referred to herein as a "standard ventricular reentry assay". Preferably, the peptides provide at least about 40% of the activity of AAP, for example at least about 50% of the activity of AAP, such as about 60% of the activity of AAP, for example at least about 70% of the activity of AAP, such as at least about 80% of the activity of AAP, for example at least about 90% of the activity of AAP, for example at least about substantially the same activity of AAP, such as about 110% of the activity of AAP, for example at least about 120% of the activity of AAP, such as at least about 130% of the activity of AAP, for example at least about 140% of the activity of AAP, such as about 150% of the activity of AAP, for example at least about 160% of the activity of AAP, such as at least about 170% of the activity of AAP, for example at least about 180% of the activity of AAP, preferably at least about 190% of the activity of AAP, more preferably at least about 200 or greater % of the activity of AAP (i.e., providing similar decreases in incidence or infarct zones of similar or smaller size).
Osteoporosis
There is understanding that GJIC is important in bone formation. Additionally preferred peptides additionally, or alternatively, increase osteoblast activity in what is referred to herein as a "standard osteoblast activity assay" which measures either calcium wave formation and/or alkaline phosphatase activity of osteoblast cells in the presence of peptides. Preferably, such peptides increased calcium wave activity, manifested as an increase in the number of cells involved in a wave (as determined by measuring levels of intracellular Ca2* using a calcium sensitive fluorescent dye, such as fura-2 and counting the number of cells which fluoresce). Alkaline phosphatase activity also can be used to provide a measure of osteoblast activity using standard colorimetric assays. Agonist peptides according to the invention provide at least about 10% of the activity of AAP in such an assay, such as at least about 20% activity, for example at least about 30% activity, such as at least about 40% activity, for example at least about 50% of the activity of AAP, preferably, at least about 70% activity, and still more preferably, 100% or greater activity of the activity of AAP.
Cancer
Preferred peptides according to the invention, alternatively, or additionally, decrease GJIC inhibition mediated by tumor promoters such as DTT, in what is referred to herein as a "standard tumor promoter assay." Preferably, the peptides show decreases in GJIC inhibition, which are at least 50%, preferably 70%, and more preferably 100% or greater, than decreases observed for AAP.
As discussed, it is an object of the invention to provide peptides that modulate gap junction intercellular communication (GJIC). Thus, many peptides in accord with the invention may include one or more of the following features: the ability to decrease cellular uncoupling, to normalize dispersion of action potential duration, and to normalize conduction velocity, the ability to control of the cellular quantity of gap junctions normalizing (up-regulating or down-regulating as needed) the expression of connexins; to normalize degradation of gap junctions (inhibit or enhance), to normalize cellular trafficking of connexins to the plasma membrane (increase or decrease); to facilitate assembly of connexins into functional gap junctions; to normalize opening of existing gap junctions, e.g., inducing or enhancing opening when they have been closed or gated by inhibitors (e.g., such as by mediating or enhancing hyperphosphorylation of the cytoplasmic carboxy terminal domain of one or more
connexins (e.g., such as Cx43)) or closing these when they are aberrantly opened (e.g., as in Charcot-Marie-Tooth disease); and the like.
Particular assays useful for identifying and optionally quantifying the activity of preferred invention peptides are described below. The assays are non-limiting and are merely serving the purpose of illustrating a variety of assays in which the present peptides may be tested for their gap junction modulating abilities. It is to be understood that the assays are not mutually exclusive, i.e. a peptide according to the invention may show activity in one particular assay, but show a different, or no, activity in another particular assay. This may be a reflection of the diversity of the individual peptides and types of assays for testing said peptides.
A. Standard Oral Availability Assay
It is a preferred aspect of the invention to provide peptides with enhanced availability in vivo. Absorption of peptides after oral administration is often limited because they are degraded by either enzymes in the gastrointestinal (Gl) tract or by enzymes in the intracellular lumen of the enterocytes. Further, the physico-chemical properties of peptides, especially their large hydrogen-bonding potential, makes it difficult for these molecules to permeate the enterocytes by transcellular passive diffusion. However, di- and tri-peptides, which have survived the gastrointestinal fluid enzymes can enter the intracellular lumen by means of the peptide transporter hPepTI, which is a membrane protein localized in the apical membrane of the enterocytes of the upper small intestine.
Preferred peptides according to the invention are therefore peptides that have affinity for an hPepTI transporter or an analog thereof. The three-dimensional conformation and key binding sites of peptide compounds which bind the PepT1 transporter are described by Bailey, P.D., et al., 2000, supra, and desired peptides can be modeled in silico to optimally fit within this binding site, as described above (see, e.g., Bailey, P.O., et al., (2000), supra; Vinter, J.G., (1996) J. Comput. Aided Des. 10:417).
The oral availability of a peptide comprising a structure as shown in Formula I, Formula II, Table 1, or more generally identified using the Bailey assay, may be evaluated for its ability to bind to a PepT1 transporter, preferably an hPepTI transporter. For example, a PepT1 cDNA, preferably, an hPepTI cDNA (see, e.g., Covitz, K. M., et al., (1996) Pharm. Res.
13(11): 1631-34) may be expressed in a Xenopus oocyte expression system and the uptake of labeled peptide into the oocyte can be monitored to approximate Ki values as described in Temple, C.S., et al. (1996) J. Physiol. (London) 494: 795; Meredith, D., et al., (1998) J. Physiol. (London) 512: 629.
In one aspect of the invention, a standard in vivo oral availability assay is performed to determine the oral availability of a peptide which has been modeled to optimally conform to the Bailey substrate template, as discussed above, in this assay, a peptide is orally administered to a mammal, such as a rat, in anorally administrable form (e.g., as part of a food pellet or in water), while at the same time, the same concentration of peptide is administered i.v. (e.g., through a catheter inserted into the femoral vein and artery). Peptides may be administered as bolus injections at concentrations ranging from 10"5-10"10 in volumes of 1 ml/kg for both oral and i.v. dosing. The animals are given 500 I.U. of heparin i.v. 5 minutes before the first blood sample is taken. A control blood sample, "before dose" or B.D. sample, is collected approximately 5 minutes before administration of the peptides. A sample of the dosing solution (e.g., 100 //I of water comprising 10"5-10"10 M of peptide) is retained for concentration determination. Blood samples are collected at t=B.D. 5, 15, 30, 60, 90,120, 180, and 240 minutes.
Blood is collected in labeled ice-chilled EDTA stabilized blood sample vials and stored on ice until quickly centrifuged at 4°C for 5 minutes (10,000 x g). Plasma (100 //I) is harvested, transferred to a labeled polypropylene microcentrifuge vial (e.g., 0.5 ml eppendorf), frozen on ice and stored at -20°C until further analysis. Approximately 40 fA of the filtrate is injected onto an HPLC column (XterraMS C18, 3 x 50 mm, 3.5 //m particles) and eluted using a linear gradient from 0 to 100% B in 4.0 minutes. The column is washed for 2.9 minutes in buffer B (0.1% formic acid in acetonitrile or another suitable buffer) and equilibrated for 5 minutes in Buffer A (0.1% formic acid in water or another suitable buffer) prior to the next injection of sample. Mass spectrometry is performed using methods routine in the art and as described further below in Examples 1 and 2.
The concentrations of compounds in the plasma samples are calculated from an external standard curve covering the range from 1.00 to 1000 nM. The plasma concentrations versus time data are used for pharmacokinetic modeling in WinNonLin 3.5 (Pharsight, Mountain view, CA) using non-compartmental analysis and ADC values are determined as is known in
the art. Preferably, orally available peptides according to the invention are observed in significant levels in plasma within about 30 minutes or less. ADC values observed in animals receiving i.v. administrations of peptide are used to evaluate such effects as clearance and half-life which should be the same in the two systems.
B. Standard Plasma Stability Assays
The invention also provides peptides that have enhanced stability in vitro or in vivo. In one aspect the peptide comprises a peptide bond that is alkylated or otherwise modified to stabilize the peptide against enzymatic degradation. In another aspect, the peptide comprises one or more D-amino acids. In a further aspect, the peptide has enhanced stability in a standard stability assay.
In one aspect, an in vitro plasma stability assay is performed as described in PCT/US02/05773, filed February 22, 2002.
As disclosed in the PCT/US02/05773 application, peptides can be incubated in plasma or serum and samples taken at regular intervals for analysis by HPLC or LC/MS/MS, to quantitate the amount of undegraded peptide. Appropriate conditions (column, solvent, gradient, and temperature) for such analyses are estimated to ensure that the peptide peak and the plasma peaks do not have the same retention time. This is done by subsequent injections of a peptide, plasma, and a co-injection with the peptide and the plasma, followed by optimization of LC method parameters until a satisfactory separation is obtained. A control plasma sample without the peptide, treated in the same manner, also can be taken and evaluated. The samples may include, but are not limited to, a blank, the peptide at a suitable concentration (e.g., 0.1 mg/mL), plasma without peptide, one or more samples for t = 0, and one or more samples at each regular interval. Preferably, multiple samples are taken in parallel. The sample concentrations (peak height in mAU or ion counts) can be plotted vs. time and fitted to a function describing a mono exponential decay (e.g., using a standard Excel package). Preferably, a peptide according to the invention has a half-life of more than about 48 hours, such as more than 24 hours, for example more than 12 hours, such as more than 6 hours, for example more than 3 hours, such as more than 1 hour, for example more than 30 minutes as determined using this assay.
Plasma stability can be examined in vivo using standard assays. For example, peptides may be administered to a mammal, such as a rat, by bolus injections in volumes of about 1 ml/kg for both i.v. and p.o. dosing. Preferably, peptides are tested in parallel with control samples such as buffer or an antiarrythmic peptide with a known stability. Blood samples are collected at different time periods (e.g., at B.D. 5, 15, 30, 60, 90,120, 180, and 240 minutes, where B.D. refers to before dose). Amounts of peptides in samples can be quantitated using methods routine in the art, such as LC/MS/MS. For example, the concentrations of peptides in plasma samples may be calculated from an external standard curve covering ranges of peptide from 1.00 to 1000 nM. The plasma concentrations versus time data can be used for pharmacokinetic modeling in WinNonLin 3.5 (Pharsight, Mountain view, CA) using non-compartmental analysis and the resulting parameters of AUC, Fpo, Clb, t1/2, Cmax and trnax can be determined as is known in the art.
C. Standard Cardiomyocyte Assays
In one aspect, a peptide according to the invention is administered to a cardiac cell and gap junction function is evaluated. Optimal peptides for such procedures can be identified in standard cardiomycte assays. In one aspect, cardiac cells are isolated from a mammal, such as a guinea pig hearts by perfusion with collagenase according to the Langendorf method. The cells are exposed to peptide and evaluated for GJIC by patch clamp using methods known in the art. Intercellular conductance (Gj) using the formula:
Where Ip.pulse and Ip.rest represent the current in the passive cell during the pulse and before the pulse respectively, and Up and Ua represent the voltage of the passive and active cell. The change in Gj value upon peptide administration is analyzed by comparing the relative changes in Gj. For example, the relative Gj as a function of time before, and during, stimulation with peptide (e.g., at about 10"8 M) can be determined.
In one embodiment the peptide provides a Gj, which is substantially the same as the Gj (by + 10%) of an antiarrhythmic peptide such as AAP, AAP10, HP5, and functional analogs thereof. In one aspect, the cell is an ischemic cell, and the peptide provides a Gj, which is substantially the same as that of a non-ischemic cell (±20%, preferably, + 10%).
In another embodiment the present peptides provides a Gj, which is different from the Gj (by + 40%) of an antiarrhytmic peptide such as AAP, AAP10, HP5, and functional analogs thereof.
Additional details concerning performing cardiomyocyte assays are provided in PCT/US02/05773, filed February 22, 2002.
D. Standard Calcium-Induced Arrhythmia Assay
Peptides suitable for administration to cardiac cells can be identified in an in vivo model of calcium-induced arrhythmias according to the model of Lynch et al. (1981).J Cardiovasc.Pharmacol. 3: 49-60. Mice (25-30 g) are anaesthetized with a neurolept anaesthetic combination and an i.v. cannula is inserted into the tail vein. A lead II EGG signal is recorded continuously by positioning a stainless steel EGG electrodes on the right forelimb and on the left hind limb. The ground electrode is placed on the right hind limb. The signal is amplified (x 5.000-10.000) and filtered (0.1-150 Hz) via a Hugo Sachs Electronic model 689 EGG module. The analog signal is digitized via a 12 bit data acquisition board (Data Translation model DT321) and sampled at 1000 Hz using the Notocord HEM 3.1 software for Windows NT. After a 10-minute equilibration period, the test sample of peptide is injected into the tail vein. Mice pre-treated with buffer are tested as a measure of the control level in untreated animals. The injection volume is 100 fil in all experiments.
Infusion of CaCI2 (30 mg/ml, 0.1 ml/min » 100 mg/kg/min (calcium chloride-2-hydrate, Riedel-de Haen, Germany)) is started 3 min after i.v. administration of drug or vehicle. The time lag to onset of 2nd degree AV-block is determined as the time from the start of CaCI2 infusion until the first arrhythmic event occurs. An event of 2nd degree AV-block is defined as intermittent failure of the AV conduction characterised by a P-wave without the concomitant QRS complex.
Responses are expressed relative to the time until 2nd degree AV-block occurred in vehicle treated mice. The maximal effect of compounds (e.g., peptides, AAP, AAP10 or controls) is determined. Preferably, peptides according to the invention have antiarrhythmic activity comparable to the compounds AAP, AAP10, HP5, or a functional analog thereof, i.e., the peptides increase the time to an AV block in a mouse after infusion of CaCI2. Preferably, Preferably, the peptides provide at least about 40% of the activity of AAP, for example at
least about 50% of the activity of AAP, such as about 60% of the activity of AAP, for example at least about 70% of the activity of AAP, such as at least about 80% of the activity of AAP, for example at least about 90% of the activity of AAP, for example at least about substantially the same activity of AAP, such as about 110% of the activity of AAP, for example at least about 120% of the activity of AAP, such as at least about 130% of the activity of AAP, for example at least about 140% of the activity of AAP, such as about 150% of the activity of AAP, for example at least about 160% of the activity of AAP, such as at least .about 170% of the activity of AAP, for example at least about 180% of the, activity of AAP, preferably at least about 190% of the activity of AAP, more preferably at least about 200 or greater % of the activity of AAP (i.e., the peptides show time lags of approximately the same duration as induced by AAP).
E. Standard Osteoblast Activity Assay
Modulation of intercellular communication represents a mechanism by which osteotropic factors regulate the activity of bone forming cells. Therefore, in one aspect, peptides according to the invention are used to increase osteoblast activity by increasing gap junctional communication between bone cells, thereby enhancing bone formation in vivo.
The efficacy of a peptide according to the invention may be assayed in preliminarily in human osteblast cells (hOB), for example by measuring calcium wave activity and/or alkaline phosphatase activity.
In one aspect, cells are isolated from human bone marrow obtained by puncture of the posterior iliac spine of healthy volunteers (aged 20-36): 10-15 ml marrow material was collected in 15 ml PBS+Ca,Mg (Life Technologies, Cat. No. 14040) with 100 U/ml Heparin (Sigma, Cat. No. H-3149). The mononuclear fraction of the marrow is isolated on a Lymphoprep gradient (Nycomed Pharma, Cat.No. 1001967), by centrifugation at 2200 rpm Tor 30 min. After harvesting, the mononuclear fraction is washed once with culture medium and centrifuged at 1800 rpm for 10 min. Subsequently cells are counted and plated in culture medium at 5x106 cells/100 mm dish. hOB medium (all reagents obtained from Life Technologies): MEM w/o Phenol Red w/ Glutamax (Cat.No. 041-93013) supplemented with 10% heat inactivated fetal calf serum (Cat.No. 10106) and 0.1% Penicillin/Streptomycin XDat.No. 15140). Medium is changed the following day and the cells are cultured at 37°C in
5%CO2 with medium change every 7 days. After 4-6 weeks of culture, the cells will reach 70% confluence. The medium is then supplemented with 100 nM Dexamethasone (Sigma, Cat.No. D-4902) for 7 days. Cells are then plated for video imaging experiments: a 25 mm #1 glass coverslip is placed in a 35 mm dish (or each well of a 6-well multidish), cells are plated at 2.5x10s cells/coverslip and cultured for 2-3 days before use.
ROS 17/2.8 cells are cultured in 100 mm dishes at 37°C with 5% CO2 and medium changed every 2-3 days. ROS medium (all reagents obtained from Life Technologies): MEM (Cat.No. 31095) is supplemented with 10% heat-inactivated calf serum (Cat.No. 16170), 1% NEAA (CatNo. 11140), 1% Sodium Pyruvate (Cat.No. 11360), 1% L-Glutamine (Cat.No. 25030) and 0.1% Penicillin/Streptomycin (Cat.No. 15140). For video imaging experiments, cells are plated on coverslips at 2-3x10s cells/coverslip and cultured for 2-3 days before use.
The cells cultured on coverslips are loaded with 5 uM fura-2-AM (Molecular Probes, CatNo. F-1221), for 30 minutes at 37°C, and incubated in fresh medium for 20 minutes. Coverslips are then affixed to a PDMI-2 culture chamber (Medical Systems Corp.), maintained at 37°C with superfused CO2, on a Zeiss Axiovert microscope. Intercellular calcium waves are induced by mechanical stimulation of a single cell using a borosilicate glass micro pipette affixed to an Eppendorf 5171 micromanipulator.
Imaging is performed using a MetaMorph imaging system (Universal Imaging). The excitation light (340 and 380 nm) is provided by a monochromator (T.I.L.L. Photonics GmbH). Images are acquired with an intensified CCD camera (Dage MTI) and digitized with a Matrox MVP image processing board. The number of cells involved in a calcium wave in the presence and absence of peptide can be used to provide a measure of increase in GJIC.
In one aspect, administration of a peptide increases the number of cells involved in a wave at least about two-fold compared to cells which have been exposed to a control, such as buffer. In another aspect, administration of a peptide decreases the number of cells involved in a wave by at least about two-fold. Agonist peptides according to the invention provide at least about 10% of the activity of AAP in such an assay, such as at least about 20% activity, for example at least about 30% activity, such as at least about 40% activity, for example at
least about 50% of the activity of AAP, preferably, at least about 70% activity, and still more preferably, 100% or greater activity of the activity of AAP.
Cells also can be measured for the presence of alkaline phosphatase activity to provide a general measure of osteoblast activity. In one aspect, cells are plated in 96-well plates at a concentration of 8000 cells/well (hOB) or 3000 cells/well (ROS) in 200ul normal culture medium. On day 4 (or day 3 for ROS cells), cells are washed with 200 pi MEM, 0.1% BSA (Sigma, Cat.No. A-9418). Samples comprising a suitable medium (e.g., 200 ul MEM, 0.1% BSA) containing various concentrations of peptides,'control, AAP or AAP10 are added to the cells, and culture is continued for about 4 days (2 days for ROS cells).
On about day 8 (preferably day 5 for ROS cells), cells are assayed for alkaline phosphatase using an Alkaline Phosphatase (ALP) assay such as is known in the art. ALP assays are generally colorimetric endpoint methods for measuring enzyme activity, and can be performed using an Alkaline Phosphatase Kit (Sigma, Cat.No. 104-LL). Preferably, cells are washed once with 200 ul PBS+Ca, Mg, 100ul Alkaline Buffer Solution is added to each well and the cells are incubated at 37°C for 10 minutes. 100 ul Substrate Solution is subsequently added to each well and the plate is incubated at 37°C for 30 min. 100 ul 2.0 N NaOH is added to each well to stop the reaction. Absorbance is measured using a plate reader at 405 nm.
Agonist peptides according to the invention provide at least about a 5% increase in alkaline phosphatase production relative to isotonic saline, preferably, at least about 10% increase in alkaline phosphatase production relative to isotonic saline, and still more preferably a 15% or greater increase in alkaline phosphatase production relative to isotonic saline. The increase in production of alkaline phosphatase is a measure for increased activity of osteoblasts and accordingly a measure for an increase in bone formation.
F. Standard Tumor Promotor Assay
The compound 1,1-bis(p-chlorophenyl)-2,2,2-trichlorethane, also known as the insecticide DDT, is an inhibitor of gap junctional communication, and has tumor promoting abilities. It inhibits cell-to-cell communication by reducing the gap junction number and size, and exposure to DDT is associated with decreased cellular levels of phosphorylated (active) forms of the gap junction protein Cx43. These actions are considered pivotal for the
compound's oncogenic properties (X. Guan, et al. (1996) Carcinogenesis, 17 1791-1798; R. J. Ruch, et al. (1994) Carcinogenesis, 15 301-306); B. V. Madhukar, et al. (1996) Cancer Lett. 106 117-123). As a means of monitoring the therapeutic efficacy of the peptides, the effects of the peptides on DDT-induced uncoupling in human osteoblast cells can be determined. Thus, in one aspect, peptides according to the invention are used to inhibit or prevent tumor-promoter induced decreases of GJIC (W. K. Hong, et al. (1997) Science, 278 1073-1077).
In one exemplary assay, Human osteoblast cells are isolated from human bone marrow obtained by puncture of the posterior iliac spine of healthy volunteers (aged 20-36). Approximately 10-15 ml of bone marrow material are collected in 15 ml PBS + Ca, Mg (Life Technologies, Cat.No. 14040) with 100 U/ml Heparin (Sigma, CatNo. H-3149). The mononuclear fraction of the marrow is isolated on a Lymphoprep gradient (Nycomed Pharma, CatNo. 1001967), by centrifugation at 2200 rpm for 30 minutes.
After harvesting, the mononuclear fraction iswashed once with culture medium and centrifuged at 1800 rpm for 10 minutes. Subsequently cells are counted and plated in culture medium at 8x10s cells/100 mm dish. Medium is changed the following day and the cells are cultured at 37°C in 5%CO2 with medium changes every 7 days. After 3-4 weeks of culture, the cells typically reach 70% confluence. The medium is then supplemented with 100 nM Dexamethasone (Sigma, Cat.No. D-4902) for 7 days. Cells are then plated for video imaging experiments. Generally, cells are plated at 2.5x105 cells/coverslip and are cultured for 2-3 days before imaging.
After culturing, cells are affixed to a PDMI-2 culture chamber (Medical Systems Corp.), maintained at 37°C with superfused CO2, on a Zeiss Axiovert microscope. Microinjections are performed using a micropipette is loaded with a 10 mM Lucifer Yellow solution (Sigma, Cat.No. L-0259). A cell in the monolayer is carefully injected with LY for 30 seconds; the micropipette is removed from the cell and after 30 seconds the number of cells that show dye transfer is counted. For a subset of cell cultures, DDT is added to the medium in a final concentration of 13 uM, and is left on for 60 minutes. Images of cells are acquired with an intensified CCD camera (Dage MTI) and digitized with a Matrox MVP image processing board, using the MetaMorph imaging software (Universal Imaging).
Under control conditions (no DDT treatment), the dye generally spreads to a median of 14.5 cells (n=12). DDT-exposed cells typically show decreased cellular coupling with a median of 7(n=13).
Peptides are added to the bathing solution in a final concentration of 10"8 mol/l, and after 10 minutes, another microinjection is performed. Preferably, agonist peptides according to the invention show an increase in cell-to-cell dye transfer. More preferably, this increase is significantly different from control samples (without peptides) as determined using routine statistical tests, such as the Wilcoxon non-pararaetric statistical test (with p This assay can be used to identify candidate peptides with the highest therapeutic efficacy in reversing the decreased intercellular coupling related to tumor promotion and in one aspect, such peptides are administered to patients at risk for developing or having cancer. A peptide may be used alone or in combination with other peptides and/or in a combination therapy with other anti-cancer agents.
Still other assays may be performed to identify peptides which elicit substantially the same physiological responses as the antiarrhythmic peptides AAP, AAP10, HP, and their functional analogs (e.g., to identify agonists) or which inhibit or suppress these physiological responses (e.g., to identify antagonists). Suitable assays include, but are not limited to: assays to measure cAMP formation in cells (e.g., CHO cells); cAMP efficacy assays (e.g., measuring inhibition of forskoline-stimulated cAMP formation of APP-like compounds in CHO cells); phosphoinositol turnover in cardiomyocytes (Meier et al.) (E. Meier, et al. (1997) Drug Development Research, 40:1-16); and responses to glucose and oxygen deprivation.
A number of standard assays are detailed above. Additional assays are described in PCT/US02/05773, filed February 22, 2002, the entirety of which is incorporated herein by reference. These assays are exemplary only and other suitable assays that may be developed and become standardized are encompassed within the scope of the invention.
Pharmaceutical Compositions
The invention also concerns a pharmaceutical composition comprising one or more of any of the peptides described above, in combination with a pharmaceutically acceptable carrier and/or diluent. Such compositions are preferably in a form adapted for oral administration.
Formulations for oral administration may be prepared in a manner well-known to the person skilled in the art, e.g., as generally described in "Remington's Pharmaceutical Sciences", 17. Ed. Alfonso R. Gennaro (Ed.), Mark Publishing Company, Easton, PA, U.S.A., 1985 and more recent editions and in the monographs in the "Drugs and the Pharmaceutical Sciences" series, Marcel Dekker. In one preferred aspect, the compositions are in the form of tablets, capsules, granules, pellets, troches, lozenges, and the like. Suitable enteric formulations are described, e.g., in U.S. Patent No. 5,350,741.
The pharmaceutical carrier or diluent employed may be a conventional solid or liquid carrier. Examples of solid carriers are lactose, terra alba, sucrose, cyclodextrin, talc, gelatin, agar, pectin, acacia, magnesium stearate, stearic acid or lower alkyl ethers of cellulose. Examples of liquid carriers are syrup, peanut oil, olive oil, phospholipids, fatty acids, fatty acid amines, polyoxyethylene and water.
Similarly, the carrier or diluent may include any sustained release material known in the art, such as glyceryl monostearate or glyceryl distearate, alone or mixed with a wax.
If a solid carrier is used for oral administration, the preparation may be tabletted, placed in a hard gelatin capsule in powder or pellet form, or it can be in the form of a troche or lozenge. The amount of solid carrier will vary widely but will usually be from about 25 mg to about 1 g.
If a liquid carrier is used, the preparation may be in the form of a syrup or liquid suitable for oral ingestion.
It will be appreciated that the actual preferred amounts of active compounds used in a given therapy will vary according to e.g. the specific compound being utilized, the particular composition formulated, the mode of administration and characteristics of the subject, e.g. the species, sex, weight, general health and age of the subject. Optimal administration rates for a given protocol of administration can be readily ascertained by those skilled in the art using conventional dosage determination tests conducted with regard to the foregoing
guidelines. Suitable dose ranges may include from about 1mg/kg to about 100mg/kg of body weight per day.
Therapeutic compounds of the invention are suitably administered in a protonated and water-soluble form, e.g., as a pharmaceutically acceptable salt, typically an acid addition salt such as an inorganic acid addition salt, e.g., a hydrochloride, sulfate, or phosphate salt, or as an organic acid addition salt such as an acetate, maleate, fumarate, tartrate, or citrate salt. Pharmaceutically acceptable salts of therapeutic compounds of the invention also can include metal salts, particularly alkali metal salts such as a sodium salt or potassium salt; alkaline earth metal salts such as a magnesium or calcium salt; ammonium salts such an ammonium or tetramethyl ammonium salt; or an amino acid addition salts such as a lysine, glycine, or phenylalanine salt.
The compounds of the invention may also be administered topically to treat peripheral vascular diseases and as such may be formulated as a cream or ointment.
The present peptides may also be formulated in compositions such as sterile solutions or suspensions for non-oral administration. Peptides of the invention may be administered parenterally, that is by intravenous, intramuscular, subcutaneous, intranasal, intrarectal, intravaginal or intrapritoneal administration.
The present invention will now be further described by the following working examples, which illustrate preferred embodiments of the invention.
Treatment Methods
In one aspect, the invention provides a method of administering to a patient having, or at risk of developing, a condition associated with impaired GJIC, a therapeutically effective amount of any of the peptides described above. Preferably, administration is oral. Patients who may be treated using peptides according to the invention include, but are not limited to, animals, preferably mammals, e.g., rodents (including mice, rats, hamsters, and lagomorphs, such as rabbits), dogs, pigs, goats (generally any domestic animal), and primates. In one preferred aspect, a patient is a human being.
In another aspect the invention concerns the use of a peptide according to the invention for the manufacture of a medicament for the treatment of a pathological condition involving impaired gap junctional communication comprising administering to a patient a therapeutically effective amount of said peptide.
Examples of conditions which can be treated include, but are not limited to, cardiovascular disease, inflammation of airway epithelium, disorders of alveolar tissue, bladder incontinence, impaired hearing due to diseases of the cochlea, endothelial lesions, diabetic retinopathy and diabetic neuropathy, ischemia of the central nervous system and spinal cord, dental tissue disorders including periodontal disease, kidney diseases, failures of bone marrow transplantation, wounds, erectile dysfunction, urinary bladder incontinence, neuropathic pain, subchronic and chronic inflammation, cancer and failures of bone marrow and stem cell transplantation, conditions which arise during transplantation of cells and tissues or during medical procedures such as surgery; as well as conditions caused by an excess of reactive oxygen species and/or free radicals and/or nitric oxide.
Arrhvtmia
In one preferred aspect, the invention provides a pharmacologically active antiarrhythmic peptide, and the use thereof, for treatment of arrhythmias and thrombptic complications arising during cardiovascular disorders, such as acute ischemic heart disease (e.g., stable angina pectoris, unstable angina pectoris, acute myocardial infarction), congestive heart failure (e.g., systolic, diastolic, high-output, low-output, right or left sided heart failure), congenital heart diseases, cor pulmonale, cardiomyopathies, myocarditis, hypertensive heart disease, during coronary revascularization, and the like.
In specific embodiments, an antiarrhythmic peptide according to the present invention is used to treat and/or prevent bradyarrhythmias (e.g., due to disease in sinus node, AV node, bundle of His, right or left bundle branch), and tachyarrhythmias associated with reentry (e.g., atrial premature complexes, AV junctional complexes, ventricular premature complexes, atrial fibrillation, atrial flutter, paroxymal supraventricular tachycardia, sinus node reentrant tachycardia, AV nodal reentrant tachycardia, and non-sustained ventricular tachycardia) either alone or in combination with other antiarrhythmic compounds, such as
class I agents (e.g., lidocaine), class II agents (e.g., metoprolol or propranolol), class III agents (e.g., amiodarone or sotalol) or class IV agents (e.g., verapamil).
Additionally, or alternatively, peptides according to the invention are used to treat one or more of: a reentry arrhythmia; ventricular reentry (e.g., such as arises during acute myocardial infarction, chronic myocardial infarction, stable angina pectoris and unstable angina pectoris); infectious or autonomic cardiomyopathy; atrial fibrillation;repolarization alternans; monomorphic ventricular tachycardia; T-wave alternans; bradyarrhythmias; and generally, reduced contractility of cardiac tissue, thrombosis and the like.
Osteoporosis
In a further aspect, peptides according to the invention are used to prevent and/or treat osteoporosis or other pathologies affecting bone formation, growth or maintenance. Peptides which are able to normalize the attenuated GJIC between human osteoblast during hypoxia are particularly suitable for the treatment of bone diseases with impaired bone formation relative to bone resorption. Optimal peptides for use in such methods can be selected in assays for increased alkaline phosphatase (ALP) activity in osteoblasts, which provides a means to monitor cell viability and growth as a consequence of proper maintenance of GJIC. In one aspect, human osteoblasts are stimulated with different concentrations of peptides from 1 x 10"13 to 1 x.10"6, and compared to untreated controls. Under normal culture conditions, peptides preferably increase ALP activity. Even more preferably, the peptides stimulate ALP activity during hypoxic conditions at concentrations ranging from 10~11 to 10"8 mol/l. The assay can thus be used to optimize peptide compositions for the treatment and/or prevention of bone diseases associated with poor vascularization, hypoxia and ischemia in bone tissue.
In another aspect, peptides according to the invention are used for the prevention and/or treatment of joint diseases that involves impaired cell-to-cell coupling. For example, the peptides can be used for the prevention and/or treatment of joint diseases that involve metabolic stress. These would include any form of arthritis associated with decreased vascularization or healing of fractured cartilage tissue.
Cancer
In still another aspect, peptides according to the invention are used to treat cancer. Carcinogenesis is characterized by the progressive impairment of growth control mechanisms in which growth factors, oncogenes and tumor suppressor genes are involved. A general theme in carcinogenesis and tumorigenesis is the down regulation of the GJIC. Permeability of gap junctions in tumor cells using the dye-transfer assay is typically lower than GJIC in surrounding tissue. Further, the gating of gap junctions is known to be effected by tumor promoters, which decrease GJIC. Therefore, in one aspect, peptides according to the invention are used as medicaments for the treatment of cancer, alone, or in conjunction with traditional anti-cancer therapies.
Wounds
In a further aspect, peptides according to the invention are used to treat wounds and, in particular, to accelerate wound healing. Wound healing involves the interactions of many cell types, and intercellular communication mediated by gap junctions is considered to play an important role in the coordination of cellular metabolism during the growth and development of cells involved in tissue repair and regeneration (K. M. Abdullah, et a!. (1999) Endocrine, 7035-41; M. Saitoh, etal. (1997) Carcinogenesis, 18:1319-1328; J. A. Goliger, et al. (1995) Moi.Biol.Cell, 6 1491-1501). Peptides may be administered to the site of a wound by topical administration using carriers well known in the art (e.g., ointments, creams, etc.) or may administered systemically, e.g., for treating wounds of internal tissues, such as in the treatment of chronic gastric ulcer lesions.
Additional functions in which endothelial gap-junctional intercellular communication has been implicated are the migratory behavior of endothelial cells after injury, angiogenesis, endothelial growth and senescence, and the coordination of vasomotor responses (G. J. Christ, et al. (2000) Braz. J Med Biol.Res., 33: 423-429). Therefore, in one aspect, a peptide according to the invention is used to enhance conducted vascular responses and to improve blood supply during conditions with increased metabolic demand (e.g., physical exercise, tachycardia), and during ischemia.
Gap junctions are also believed to provide the molecular link for co-ordinated long-range signaling among individual members of the glial compartment. Likewise, astrocytes are
ideally suited for metabolic support of neurons since they are functionally polarized with one extremity touching the vascular bed and the other pole approximates neuronal parenchyma (R. Dermietzel (1998) Brain Res. Brain Res. Rev., 26: 176-183). Therefore, in one preferred embodiment, peptides according to the invention are administered to a patient in need to prevent ischemic damage in the brain by increasing the metabolic support between glia cells and neurons. Such patients may include patients with organic psychoses, which may present with signs such as depression, anxiety, learning and memory deficit, phobias, and hallucinations or patients who have suffered a traumatic brain injury. Preferably, such peptides are selected or formulated so as to be available to the central nervous system (i.e., provided with or conjugated with carriers which facilitate transport across the blood-brain barrier).
Peptides according to the invention may also be used to accelerate repair after nerve injury or during grafting of immature cells (progenitor cells) into brain tissue, e.g., such as in patients with neurotrauma, brain ischemia and chronic neurodegenerative diseases, such as Parkinson's disease or Huntington's disease (H. Aldskogius, et al. (1998) Prog. Neurobiol, 55:1-26).
In specific embodiments, a peptide according to the present invention may, due to the effect on the intercellular gap junction channels, be used to treat and/or prevent cataract (D. Mackay, et al. (1999) Am J Hum.Genet, 64 1357-1364) treat and/or prevent vascularization of the cornea in disease states with poor nutrition of the cornea and increase the healing of corneal lesions (S. G. Spanakis, et al. (1998) Invest Ophthalmol.Vis.Sci.,39: 1320-1328) and/or prevent hypertension.
It should be obvious to those of skill in the art, that the peptides and pharmaceutical compositions according to the invention can be used to treat any condition or pathology associated with impaired (abnormal decreases or increases in) gap junctional communication. Preferably, one or more of the peptides or pharmaceutical compositions comprising the one or more peptides are administered to a patient in need thereof in a therapeutically effective amount. As used herein, "a therapeutically effective amounf is one which reduces symptoms of a given condition or pathology, and preferably which normalizes physiological responses in a patient with the condition or pathology. Reduction of symptoms or normalization of physiological responses can be determined using methods routine in the
art and may vary with a given condition or pathology. In one aspect, a therapeutically effective amount of one or more peptides or pharmaceutical composition comprising the one or more peptides is an amount which restores a measurable physiological parameter to substantially the same value (preferably to within ± 30%, more preferably to within + 20%, and still more preferably, to within 10% of the value) of the parameter in a patient without the DMF.
EXAMPLES
The invention will now be further illustrated with reference to the following examples. It will be appreciated that what follows is by way of example only and that modifications to detail may be made while still falling within the scope of the invention.
Example 1. Peptide Synthesis
A preferred general procedure is described below. However, more detailed descriptions of solid phase peptide syntheses are found in WO98/11125 hereby incorporated in its entirety.
a. General Peptide Synthesis
Apparatus and synthetic strategy
Peptides were synthesized batchwise in a polyethylene vessel equipped with a polypropylene filter for filtration using 9-fluorenylmethyloxycarbonyl (Fmoc) as N-cc-amino protecting group and suitable common protection groups for side-chain functionalities.
Solvents
Solvent DMF (/V,A/-dirnethylformamide, Riedel de-Haen, Germany) was purified by passing through a column packed with a strong cation exchange resin (Lewatit S 100 MB/H strong acid, Bayer AG Leverkusen, Germany) and analyzed for free amines prior to use by addition of 3,4-dihydro-3-hydroxy-4-oxo-1,2,3-benzotriazine (Dhbt-OH) giving rise to a yellow color
(Dhbt-O~ anion) if free amines are present. Solvent DCM (dichloromethane, analytical grade, Riedel de-Haen, Germany) was used directly without purification. Acetonitril ( HPLC-grade, Lab-Scan, Dublin Ireland) was used directly without purification.
Ami no Acids
Fmoc-protected amino acids were purchased from Advanced ChemTech (ACT) in suitabel side-chain protected forms. Otherwise protected amino acids (Boc-Asp(OFm)-OH, Boc-D-Asp(OFm)-OH, Fmoc-Lys(Aloc)-OH, Fmoc-D-Lys(Aloc)-OH, Boc-Lys(Frnoc)-OH Boc-D-Lys(Fmoc)-OH, Boc-Orn(Fmoc)-OH from Bachem (Switzerland); Fmoc-Lys(ivDde)-OH, Fmoc-Sar-OH from NovaBiochem (Switzerland).
Benzole acid and Benzyl Amine Derivatives
Benzoic acid and Benzyl amine derivatives were purchased from Aldrich and used without further purification.
Coupling Reagents
Coupling reagent diisopropylcarbodiimide (DIG) was purchased from (Riedel de-Haen, Germany), PyBop from Advanced ChemTech.
Linkers
(4-hydroxymethylphenoxy)acetic acid (HMPA), was purchased from Novabiochem, Switzerland; and was coupled to the resin as a preformed 1-hydroxybenzotriazole (HOBt) ester generated by means of DIG.
Solid Supports
Peptides synthesized according to the Fmoc-strategy on TentaGel S resins 0,22-0,31 mmol/g (TentaGel-S-NH2; TentaGel S-Ram, Rapp polymere, Germany).
Catalysts and Other Reagents
Diisopropylethylamine (DIEA) was purchased from Aldrich, Germany, and ethylenediamine from Fluka, piperidine and pyridine from Riedel-de Haen, Frankfurt, Germany. 4-(N,N-dimethylamino)pyridine (DMAP) was purchased from Fluka, Switzerland and used as a catalyst in coupling reactions involving symmetrical anhydrides. Ethandithiol was purchased from Riedel-de Haen, Frankfurt, Germany. S-dihydro-S-hydroxy-oxo-I.S-benzotriazine (Dhbt-OH), 1-hydroxybenzotriazole (HOBt) (HOAt) were obtained from Fluka, Switzerland.
Coupling Procedures
The first amino acid can be coupled as a symmetrical anhydride in DMF generated from the appropriate n-a-protected amino acid and the subsequent amino acids can be coupled as in situ generated HOBt or HOAt esters made from appropriate n-a-protected amino acids and HOBt or HOAt by means of DIG in DMF. The acylations were checked by the ninhydrin test performed at 80 oc in order to prevent Fmoc deprotection during the test (B, D. Larsen, A. Holm, IntJ Pept.Protein Res. 1994, 43 1-9).
Deprotection of the N-a-amino Protecting Group (Fmoc)
Deprotection of the Fmoc group was performed by treatment with 20% piperidine in DMF (1x5 and 1x10 min.), followed by wash with DMF (5 x 15 ml, 5 min. each) until no yellow color could be detected after addition of Dhbt-OH to the drained DMF.
Deprotection ofAllyl/Aloc
A solution of 3 eq. Pd(PPh3)4 dissolved in 15-20 ml CHCI3l AcOH, NMM (37:2:1) was added to the peptid resin. The treatment was continued for three hours at room temperature accompanied by bubbling a stream of N2 through the mixture.
Coupling Of Hobt-Esters
3 eq. N-a-amino protected amino acid was dissolved in DMF together with 3 eq. HOBt and 3 eq. DIG and then added to the resin.
Preformed Symmetrical Anhydride
Six eq. N-a-amino protected amino acid was dissolved in DCM and cooled to 0°C. DIG (3 eq.) was added and the reaction continued for 10 minutes. The solvent was removed in vacuo and the remanence dissolved in DMF. The solution was immediately added to the resin followed by 0.1 eq. of DMAP.
Cleavage OfPeptide From Resin With Acid
Peptides were cleaved from the resins by treatment with 95% triflouroacetic acid (TFA, Riedel-de Haen, Frankfurt, Germany)-water v/v or with 95% TFA and 5% ethandithiol v/v at
r.t. for 2 hours. The filtered resins were washed with 95% TFA-water and filtrates and washings evaporated under reduced pressure. The residue was washed with ether and freeze-dried from acetic acid-water. The crude freeze-dried product was analyzed by high-performance liquid chromatography (HPLC) and identified by electrospray ionisation mass spectrometry (ESMS).
Batchwise Peptide Synthesis on TentaGel Resin (PEG-PS)
TentaGel resin (1g, 0.22-0.31 mmol/g) was placed in a polyethylene vessel equipped with a polypropylene filter for filtration. The resin was swelled in DMF (15ml), and treated with 20% piperidine in DMF to secure the presence of non-protonated amino groups on the resin. The resin was drained and washed with DMF until no yellow color could be detected after addition of Dhbt-OH to the drained DMF. HMPA (3 eq.) was coupled as a preformed HOBt-ester as described above and the coupling was continued for 24 h. The resin was drained and washed with DMF (5x5 ml, 5 min each) and the acylation checked by the ninhydrin test. The first amino acid was coupled as a preformed symmetrical anhydride as described above. The following amino acids according to the sequence were coupled as preformed Fmoc-protected HOBt esters (3 eq.) as described above. The couplings were continued for 2 h, unless otherwise specified. The resin was drained and washed with DMF (5 x 15 ml, 5 min each) in order to remove excess reagent. All acylations were checked by the ninhydrin
test performed at 80 °C. After completed synthesis the peptide-resin was washed with DMF (3x15 ml, 5 min each), DCM (3x15 ml, 1 min each) and finally diethyl ether (3x15 ml, 1 min each) and dried in vacuo.
Preparative HPLC conditions.
Preparative chromatography was carried out using a VISION Workstation (PerSeptive Biosystem) equipped with AFC2000 automatic fraction collector/autosampler. VlSION-3 software was used for instrument control and data acquisition.
Column
Kromasil (EKA Chemicals) KR100-10-C8 100A, C-8, 10 D; CER 2230, 250 x 50,8 mm or a VYDAC 218TP101550, 300A, C-18, 10-15 D, 250 x 50 mm. The buffer system used included A: 0,1% TFA in MQV; B: 0,085% TFA, 10% MQV, 90% MeCN. Flow rates were
35-40 ml/min and the column temperature was 25°C. UV detection was performed at 215 nm and 280 nm. Suitable gradients were optimized for individual peptides.
Analytical HPLC Conditions
Gradient HPLC analysis was done using a Hewlett Packard HP 1100 HPLC system consisting of a HP 1100 Quaternary Pump, a HP 1100 Autosampler a HP 1100 Column Thermostat and HP 1100 Multiple Wavelength Detector. Hewlett Packard Chemstation for LC software (rev. A.06.01) was used fqr.instrument control and data acquisition.
For analytical HPLC, different columns were used as appropriate, such as VYDAC 238TP5415, C-18, 5^.m, 300A, or a Jupiter, Phenomenex OOF-4053-EO; 5 Dm C-18, 300A 150 x 4,6 mm and others. The buffer system included A: 0,1% TFA in MQV; B: 0,085% TFA, 10% MQV, 90% MeCN. Flow rates were 1 ml/min. The preferred column temperature was 40°C. UV detection was performed at 215 nm. As above, suitable gradients were optimized for the individual peptides. Mass Spectroscopy
\ The peptides were dissolved in super gradient methanol (Labscan, Dublin, Ireland), Milli-Q
water (Millipore, Bedford, MA) and formic acid (Merck, Damstadt, Germany) (50:50:0.1 v/v/v) to give concentrations between 1 and 10 ^ig/ml. The peptide solutions (20 |il) were analysed in positive polarity mode by ESI-TOF-MS using a LCT mass spectrometer (Micromass, Manchester, UK) accuracy of +/- 0.1 m/z.
General synthetic procedure
In all syntheses, dry TentaGel-S-NH2 (0.23 mmol/g, 1g) was placed in a polyethylene vessel equipped with a polypropylene filter for filtration and treated as described under "batchwise peptide synthesis on TentaGel resin". Lysine and analogs thereof (e.g. Ornithin, 2,4-Diaminobutanoic acid, 1,3-diaminopropanoic acid etc.) when situated C-terminally were coupled as the N-oc Fmoc protected derivatives with either ivDde or Aloe protection of the side chain functionality (e.g. Fmoc-Lys(Aloc)-OH). Lysine and analogs thereof when situated N-terminally were coupled as the N-a Boc protected derivatives with Fmoc protection of the side chain functionality (e.g. Boc-Lys(Fmoc)-OH). Aspartic acid, Glutamic acid and analogs thereof when situated C-terminally were coupled as N-a Fmoc protected derivatives with
Allylic protection of the side chain functionality (e.g. Fmoc-Asp(Oallyl)-OH). Aspartic acid, Glutamic acid and analogs thereof when situated N-terminally were coupled as N-a Boc protected derivatives with Fm protection of the side chain functionality (e.g. Boc-Asp(OFm)-OH). Other amino acids than the above mentioned when situated C-terminally were coupled as N-a Fmoc protected derivatives with suitable protection of the side chain functionalities or when situated N-terminally as N-a Boc protected derivatives with suitable protection of the side chain functionalities.
In all cases the dipeptide was assembled followed by deprotection of the side chain protecting group of the Lysine, Aspartic- or Glutamic acid or analogs thereof.
In case of Lysine or analogs thereof, the hydrophobic group functionalised as a carboxylic acid was coupled as an in situ generated HOBt ester by means of DIG in THF.
In case of Aspartic- and Glutamic acid or analogs thereof, the hydrophobic group functionalised as an amine was coupled to the pre generated HOBt ester of the side chain carboxylic acid by means of DIG in DMF catalyzed by triethylamine.
All couplings were continued for at least 2 hours. The acylations were checked by the
ninhydrin test performed at 80 °C as earlier described. After completed synthesis the peptide-resin was washed with DMF (3x 15 ml, 1 min each), DCM (3x 15 ml, 1 min each), diethyl ether (3x 15 ml, 1 min each) and dried in vacua. The peptide was then cleaved from the resin as described above and freeze-dried.
After purification using preparative HPLC as described above, the peptide product was collected and the identity of the peptide was confirmed by ES-MS .
The above procedure was used for the synthesis of all peptides exemplified further below and the peptides shown in Table 1 of the specification. Exemplary synthesis schemes are shown in Figures 1A and 1B.
b. synthesis of Individual Peptides
Synthesis ofH-Gly-Lys (4-nitrobenzoyl)-OH (Compound 1)
Lysine was coupled as Fmoc-Lys(ivDde)-OH and the N-terminal Glycine as the Boc derivative. The ivDde protecting group was removed as described above. The Lysine and Giycine were first assembled on the solid support. The ivDdde group was then removed and subsequently 4-nitrobenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in THF. After purification using preparative HPLC as described above, 35 mg peptide product was collected with a purity greater than 99 %. The identity of the peptide was confirmed by ES-MS (found MH+ 352.28, calculated MH+ 352.21).
Synthesis of H-Gly-Lys(4-cyanobenzoyl)-OH (Compound 3)
Lysine was coupled as Fmoc-Lys(ivDde)-OH and the N-terminal Glycine as the Boc derivative. The ivDde protecting group was removed as described above. The Lysine and the Glycine were first assembled on the solid support. The ivDdde group was then removed and subsequently 4-cyanobenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in DMF. After purification using preparative HPLC as described above, 6 mg peptide product was collected with a purity greater than 90 %. The identity of the peptide was confirmed by ES-MS (found MH+ 332.25, calculated MH+ 332.21).
Synthesis ofH-Gly-Lys(4-methoxybenzoyl)-OH (Compound 4)
Lysine was coupled as Fmoc-Lys(ivDde)-OH and the N-terminal Glycine as the Boc derivative. The ivDde protecting group was removed as described above. The Lysine and the Glycine were first assembled on the solid support. The ivDdde group was then removed and subsequently 4-methoxybenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in DMF. After purification using preparative HPLC as described above, 7 mg peptide product was collected with a purity greater than 95 %. The identity of the peptide was confirmed by ES-MS (found MH+ 337.28, calculated MH* 337.21).
Synthesis of H-Lys(4-nitrobenzoyl)-Gly-OH (Compound 7)
Glycine was coupled as Fmoc-Glycine and the N-terminal Lysine was coupled as Boc-Lys(Fmoc)-OH. The Glycine and the Lysine were first assembled on the solid support. The
Fmoc in the side chain of Lysine was then removed and subsequently 4-nitrobenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in THF. After purification using preparative HPLC as described above, 64 mg peptide product was collected with a purity greater than 98 %. The identity of the peptide was confirmed by ES-MS (found MH+ 352.19, calculated MH+ 352.24).
Synthesis ofH-D-Lys(4-methoxybenzoyl)-Gly-OH (Compound 21)
Glycine was coupled as Fmoc-Glycine and the N-terminal Lysine was coupled as Boc-D-Lys(Fmoc)-OH. The Glycine and the Lysine were first assembled on the solid support. The Fmoc in the side chain of Lysine was then removed and subsequently 4-methoxybenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in DMF. After purification using preparative HPLC as described above, 31 mg peptide product was collected with a purity greater than 97 %. The identity of the peptide was confirmed by ES-MS (found MH+ 337.24, calculated MH* 337.21).
Synthesis ofH-D-Lys(4-nitrobenzoyl)-Gly-OH (Compound 22)
Glycine was coupled as Fmoc-Glycine and the N-terminal Lysine was coupled as Boc-D-Lys(Fmoc)-OH. The Glycine and the Lysine were first assembled on the solid support. The Fmoc in the side chain of Lysine was then removed and subsequently 4-nitrobenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in THF. After purification using preparative HPLC as described above, 65 mg peptide product was collected with a purity greater than 98 %. The identity of the peptide was confirmed by ES-MS (found MH+ 352.27, calculated MH+352.24).
Synthesis of H-D-Lys(benzoyl)-Gly-OH (Compound 23)
Glycine was coupled as Fmoc-Glycine and the N-terminal Lysine was coupled as Boc-D-Lys(Fmoc)-OH. The Glycine and the Lysine were first assembled on the solid support. The Fmoc in the side chain of Lysine was then removed and subsequently Benzoic acid was coupled as an in situ generated HOBt ester by means of DIG in DMF. After purification using preparative HPLC as described above, 31 mg peptide product was collected with a purity greater than 96 %. The identity of the peptide was confirmed by ES-MS (found MH+ 307.22, calculated MH+ 307.24).
Synthesis ofH-D-Lys(4-t-Butylbenzoyl)-Gly-OH (Compound 54)
Glycine was coupled as Fmoc-Glycine and the N-terminal Lysine was coupled as Boc-D-Lys(Fmoc)-OH. The Glycine and the Lysine were first assembled on the solid support. The Fmoc in the side chain of Lysine was then removed and subsequently 4-t-Butylbenzoic acid was coupled as an in situ generated HOBt ester by means of DIG in DMF. After purification using preparative HPLC as described above, 34 mg peptide product was collected with a purity greater than 97 %. The identity of the peptide was confirmed by ES-MS (found MH+ 363.27, calculated MH+ 363.22).
Synthesis of H-Asn(NH(4-methoxybenzyl))- D-Alanine-OH (Compound 80)
Alanine was coupled as Fmoc-D-Alanine and the N-terminal Asparagine was coupled as Boc-Asp(OFm)-OH. The Alanine and the Aspartic acid were first assembled on the solid support. The Fm in the side chain of Aspartic acid was then removed and subsequently 4-methoxybenzylamine was coupled catalyzed by triethylamine to the pre generated HOBt ester of the side chain carboxylic acid by means of DIG in DMF. After purification using preparative HPLC as described above, 17 mg peptide product was collected with a purity greater than 98 %. The identity of the peptide was confirmed by ES-MS (found MH+ 323.17, calculated MH+323.15).
Synthesis ofH-D-Asn(NH(4-methoxybenzyl))-Alanine-OH (Compound 95)
Alanine was coupled as Fmoc-Alanine and the N-terminal Asparagine was coupled as Boc-D-Asp(OFm)-OH. The Alanine and the Aspartic acid were first assembled on the solid support. The Fm in the side chain of Aspartic acid was then removed and subsequently 4-methoxybenzylamine was coupled catalyzed by triethylamine to the pre generated HOBt ester of the side chain carboxylic acid by means of DIG in DMF. After purification using preparative HPLC as described above, 25 mg peptide product was collected with a purity greater than 98 %. The identity of the peptide was confirmed by ES-MS (found MH+ 323.12, calculated MH+323.15).
Synthesis ofH-D-Asn(NH(4~nitrobenzyl))-AIanine-OH (Compound 96)
Alanine was coupled as Fmoc-Alanine and the N-terminal Asparagine was coupled as Boc-D-Asp(OFm)-OH. The Alanine and the Aspartic acid were first assembled on the solid
support. The Fm in the side chain of Aspartic acid was then removed and subsequently 4-nitrobenzylamine was coupled catalyzed by triethylamine to the pre generated HOBt ester of the side chain carboxylic acid by means of DIG in DMF. After purification using preparative HPLC as described above, 102 mg peptide product was collected with a purity greater than 99 %. The identity of the peptide was confirmed by ES-MS (found MH+ 338.14, calculated MH+338.12).
Example 2 Bioavailability
MATERIALS AND METHODS
Pharmacokinetic screening and food interaction studies
Chemicals & Materials
The water used for these experiments was of highest quality obtained from a reversed osmosis primary system in combination with a Milli-Q water secondary treatment system (Millipore, Bedford, MA, USA). Methanol was super gradient quality obtained from Labscan Ltd. (Dublin, Ireland). Formic acid p.a. (98-100%) was obtained from Merck (Darmstadt, Germany). Heptafluorobuturicacid, HPLC grade wAs obtained from Pierce (Rockford, III, USA). EDTA stabilised plasma from rat (Sprague-Dawley) was obtained from Harlan Sera Lab Ltd. (Loughborough, UK). Blood samples were collected in potassium EDTA coated microtainers from BD Vacutainer Systems (Plymouth, UK). Sample preparation by ultra filtration was performed using Microcon centrifugal filter devices with a molecular weight cut off of 3000 obtained from Millipore (Bedford, MA, USA).
Instrumentation
The LC/MS/MS analysis was performed on a Waters Alliance 2790 HPLC instrument in combination with a Quattro Ultima mass spectrometer from Micromass (Manchester, UK). Both the LC and MS were controlled by MassLynx 3.5 software. The LC separations prior to MS/MS detection were performed on an XTerra MS Ci8 (2.0 x 50 mm), 3.5 pm particles, (Waters, Milford, MA, USA). Animals
Twelve male Sprague-Dawley rats (approx 350 g) were obtained from M&B (Denmark) and catheters were inserted into the femoral vein and artery during Hypnorm®-Dormicum® anaesthesia. After surgery, the rats were allowed to recover for five days before drug administration was initiated.
Drugs and Dose Levels
The dipeptides (Compound 22, Compound 21, Compound 23, Compound 96, Compound 95
and Compound 54) were obtained as the TFA salts and dissolved in PBS (2.6 mM KCI, 137
mM NaCI, 1.5 mM KH2PO4 and 8.2 mM Na2HPO4 adjusted to pH=7.4) to give concentrations
of 500 jaM. The dosing volumes were 1 ml_/kg corresponding to doses of 500 nmol/kg,
respectively. After each experiment the dosing solutions were diluted in 0.5% formic acid in
water and analysed by LC/MS/MS for their content of drug substance. The concentrations of
drug substance in the dosing solutions were calculated from the responses of standards in
the range from 1 to 1000 nM. &.
Study Design
The drug substances were administered to two animals as i.v. and p.o. bolus in a cross-over study design. The p.o. dose was administered to rats fasted for a 17 hours period prior to drug administration. The animals were allowed to rest for 48 hours in between drug administrations. After the first experiment the rats received a blood transfusion with heparin treated blood.
Prior to drug administration (5 min) the rats received 500 IU heparin as an i.v. bolus and a control blood sample was collected. After drug administration blood samples of approx. 250 jj.l were collected from the femoral artery at the following time points; before dose (B.D.), 5, 15, 30, 60, 120, 180 and 240 min after i.v. administration and at B.D., 10, 30, 50, 80, 120, 180, 240, and 300 min after p.o. administration. The blood samples were stored on ice until centrifugation for 5 min at 10.000 x g (4°C) and the plasma (100 jj.L) were transferred to 1.5 ml polypropylene tubes and stored at -20°C until sample preparation and LC/MS/MS analysis.
Sample Preparation and LC/MS/MS Analysis
The plasma samples were thawed on ice, and 100 pi plasma was mixed with 100 uL 1% (v/v) formic acid and transferred to microcon YM-3 filter units. The samples were then centrifuged for 1 hr at 8.300 x g at room temperature. The filtrates were collected in 300 fiL autosampler vials and stored at 4°C until injection (40 (iL) onto the LC column. The chromatography was performed at 50°C using a linear gradient from 100 % buffer A (0.1% formic acid in water) to 100% buffer B (0.1% formic acid in acetonitrile) in 4 min, followed by 3 min wash using buffer B and finally a reequiiibration period for 7 min using buffer A. The detection of the drug substances were performed by MS/MS using argon as collision gas
(1.3 x 10"3 mbar). The specific MS/MS settings for each of the tested compounds are given in Table 2.

Table 2: MS/MS settings used for the detection of compounds x-y in the bioavailability study.
Data Analysis
The plasma concentrations of the drug substance were calculated from the area related to an external calibration curve obtained from spiked plasma samples treated as described above. The calibration curve was obtained by linear regression of the log(peak area) vs. log(concentration). The calibration curve covered the concentration range from 0.1 to 100 nM.
The plasma concentrations versus time data from each animal was used for pharmacokinetic modelling in WinNonLin 3.5 (Pharsight, Mountain View, CA, USA) using non-compartmental analysis and the value of the area under the plasma concentrartion curve (AUC) were reported. The oral bioavailability Fpo was calculated as the ratio in % between the dose (D) normalised AUC's after iv and po administration:
The oral bioavailability of 6 compounds was tested and all compounds were detected after oral administration. The calculated bioavailabilities are summarised in Table 3. The bioavailability of Compounds 22, 23, 96, and 95 were moderate (within 10 - 31%) and the bioavailability of Compounds 54 and 21 were low (within 2 - 8%).
Table 3: The mean bioavailability ± standard error on mean (SEM) of the 6 tested
compounds.
CONCLUSION
The peptides of the invention showed oral availability having a range of availability in Sprague-Dawley rats between 2 an 31%.
Example 3 Osteoblast Activity (ALP assay)
MATERIALS AND METHODS
Human primary osteoblasts were obtained from bone marrow biopsies of the posterior iliac spine from voluntary donors. Cells were used at 6 weeks of culturing. Cells were cultured in 24-well plates in an 8 days process and stimulated with the test compounds in concentrations from 1x10~13 to 1x10~6 for the last 4 days of the experiment. Cell lysate was collected for determination of ALP activity. hOB cells from 10-15 donors were used for the experiments. For ALP measurements a commercially available kit (Alkaline Phosphatase Kit, Sigma-Aldrich Denmark A/S) was used. All determinations were performed according to the manufacturer's recommendations.
Analyses
ALP was determined on cell lysate collected at termination of the experiment.
Measurements were compared with and to vehicle treated control cultures.
Data analysis
Data are presented as means and standard deviations or medians and percentiles as appropriate. Two-way ANOVA is performed using Fisher's LSD test for post-hoc comparisons, using a 0.05 level of significance.
RESULTS
Table 4
The activity of Compounds 1, 22, 23, and 95 are illustrated in Figure 2 and summarized in the above Table 4.
CONCLUSION
The peptides of the invention increased the activity of human osteoblasts in primary culture
as measured by an increase in production of alkaline phosphatase.
Example 4 Standard Calcium-Induced Arrhythmia Assay
The anti-arrhythmic effect of the dipeptides was determined in a model of calcium-induced arrhythmias according to the model of Lynch et al. [6]. Male NMRI mice (25-30 g; Bomholdtgaard, LI. Skendsved, Denmark) were anaesthetised with a neurolept anaesthetic combination (Hypnorm® (fentanyl citrate 0.315 mg/ml and fuanisone 10 mg/ml) + midazolam (5 mg/ml)). Commercial solutions of Hypnorm® and midazolam were diluted 1:1 in distilled water, and one part diluted Hypnorm® was mixed with one part diluted midazolam. Anaesthesia was induced by s.c. administration of this solution in a dose of 50 - 75 u.l/10 gram mouse.
An i.v. cannula was inserted into the tail vein. The lead II EGG signal was recorded continuously by positioning of stainless steel ECG electrodes on the right forelimb and on the left hind limb. The ground electrode was placed on the right hind limb. The signal was amplified (x 5.000-10.000) and filtered (0.1-150 Hz) via a Hugo Sachs Electronic model 689 ECG module. The analogue signal was digitised via a 12-bit data acquisition board (Data Translation model DT321) and sampled at 1000 Hz using the Notocord HEM 3.1 software for Windows NT. After a 10-min equilibration period, the test sample of drug was injected into the tail vein and three minutes later i.v. infusion of CaCI2 (30 mg/ml, 0.1 ml/min « 100 mg/kg/min), (calciumchlorid-2-hydrat, Riedel-de Hae'n, Germany) was started.
Mice pre-treated with vehicle (phosphate buffered saline with 0.1% bovine albumin) were tested on all days as a measure for the control level in untreated animals. Injection volume was 100 fil in all experiments. The time lag to onset of arrhythmias (tan.) was determined as the time from the start of CaCI2 infusion until the first event of 2nd degree AV block (defined as intermittent failure of the AV conduction characterised by a P-wave without the concomitant QRS complex).
RESULTS
The % response of the tested compounds are given in Table 5. The given response is estimated according to (tarr (testcompound) - tarr (vehicle)) x 100/ tarr (vehicle).

CONCLUSION
The peptides of the invention showed both an antiarrhytmic effect and a non-antiarrhytmic
effect.
DEFINITIONS
Unless specified otherwise, the following definitions are provided for specific terms which are used in the following written description.
Throughout the description and claims the three-letter code for natural amino acids is used as well as generally accepted three letter codes for other oc-amino acids, such as Sarcosin
(Sar). Where the L or D form has not been specified, it is to be understood that the amino acid in question can be either the L or D form.
The term "halogen" refers to F, Cl, Br, and I, where F and I are preferred.
The term "alky!" refers to univalent groups derived from alkanes by removal of a hydrogen atom from any carbon atom: CnH2n+i-. The groups derived by removal of a hydrogen atom from a terminal carbon atom of unbranched alkanes form a subclass of normal alkyl (n-alkyl) groups: HtCHJn-. The groups RCH2-, R2CH- (R not equal to H), and R3C- (R not equal to H) are primary, secondary and tertiary alkyl groups respectively. C(1-22)alkyl refers to any alkyl group having from 1 to 22 carbon atoms and includes C(1-6)alkyl, such as methyl, ethyl, propyl, iso-propyl, butyl, pentyl and hexyl and all possible isomers thereof.
By the phrase "lower alkyl" is meant a linear or branched alkyl having less than about 6 carbon atoms, preferably methyl, ethyl, propyl, or butyl.
The term "alkenyl" refers to a straight or branched or cyclic hydrocarbon group containing one or more carbon-carbon double bonds. C(2-22)alkenyl refers to any alkenyl group having from 1 to 22 carbon atoms and includes C(2-6)alkenyl, vinyl, allyl, 1-butenyl, etc.
The term "aralkyl" refers to aryl C(1-22)alkyl, and the term "aryl" throughout this specification means phenyl or naphthyl.
By the phrase "hydrophobic group" is meant an optionally substituted aromatic carbon ring, preferably a 6 or 12 -membered aromatic carbon ring. By the phrase "optionally substituted" is meant substitution of the 6 or 12-membered aromatic carbon ring with at least one of a lower alkyl, alkoxy, hydroxyl, carboxy, amine, thiol, hydrazide, amide, halide, hydroxyl, ether, amine, nitrile, imine, nitro, sulfide, sulfoxide, sulfone, thiol, aldehyde, keto, carboxy, ester, an amide group; including seleno and thio derivatives thereof. Also included in the definition of "optionally substituted" are are sulfide, sulfoxide, sulfone, and thiol derivates with or without a seleno group. In embodiments in which the aromatic carbon ring is substituted such substitutions will typically number less than about 10 substitutions, more preferably about 1 to to 5 of same with about 1 or 2 substitutions being preferred for many invention applications. Preferred alkoxy groups include methoxy, ethoxy, and propoxy. Illustrative hydrophobic groups include unsubstituted benzyl, phenyl, and napthyl.
By the phrase "hydrogen bond group" is meant a donor or acceptor of a (non-covalent) hydrogen bond. In embodiments in which the hydrogen bond group is the donor, it will typically include at least one electronegative atom bound to a hydrogen atom. Examples of such electronegative atoms include, but are not limited to, nitrogen, oxygen, halide (eg., Cl, F, Br, etc), and sulfur. Illustrative hydrogen bond donors include hydroxyl, amine, thiol, hydrazide and amide. In embodiments in which the first hydrogen bond group is an acceptor, it will preferably include at least one electronegative atom such as those mentioned above in which the atom includes a non-bonded electron pair. Such pairs are often referred to as "lone pairs". Examples of preferred hydrogen bond acceptors include, but are not limited to, halide, hydroxyl, ether, amine, nitrile, imine, nitro, aldehyde, keto, carboxy, ester, amide group; and seleno derivatives thereof. Also envisioned are suitable sulfide, sulfoxide, sulfone, and thiol hydrogen bond acceptors including seleno derivatives thereof.
The terms "intercellular communication modulator", "gap junction facilitator", "compound that facilitates gap junction communication" and "gap junction opener", etc., all refer to a compound that facilitates, or maintains, or normalizes (e.g. either by inhibiting of enhancing), GJIC, irrespective of the particular mechanism behind this action. More specifically, the term "gap junction opener" may refer to a substance which normalizes (i.e., increases) the exchange of molecules that are able to pass through gap junctions between extracellular . and intracellular spaces and/or which can normalize increase GJIC.
The term "agonist" refers to a peptide that can interact with a tissue, cell or cell fraction which is the target of for example, but not limited to, an AAP, AAP10, HP5 peptide, or functional analog thereof, to cause substantially, or at least substantially the same physiological responses in the tissue, cell or cell fractionas the AAP, AAP10, HP5 peptide, or functional analog thereof. In one aspect, the physiological response is one or more of: contraction, relaxation, secretion, and enzyme activation. Preferably, the peptide binds to the tissue, cell or cell fraction, in one aspect, the peptide binds to a receptor on the tissue, cell, or cell fraction, which binds to AAP, AAP10, HP5, or a functional analog thereof. However, the present "agonist" may interact with a tissue, cell or cell fraction, which is the target of any given peptide, causing the same, or at least substantially the same physiological response.
An "antiarrhythmic peptide agonist" as used herein is a peptide, which comprises an antiarrhythmic activity, which is substantially the same, or greater than, the antiarrhythmic activity of an AAP, AAP10, HP5 peptide or functional analog thereof. "Greater than" refers to an antiarrhythmic activity, which is observed at lower concentrations of peptide or in shorter periods of time compared to the antiarrhythmic activity of an AAP, AAP10, HP5 peptide or functional analog thereof.
The term "antagonist" refers to a peptide which inhibits or antagonizes one or more
. •_",
physiological responses observed in a tissue, cell or cell fraction after contacting the tissue, cell, or cell fraction with any given peptide, such as AAP, AAP10, HP5 peptide, or a functional analog thereof. In one aspect, the physiological response is one or more of: contraction, relaxation, secretion, and enzyme activation. Preferably, the peptide binds to the tissue, cell or cell fraction. In one aspect, the peptide binds to a receptor on the tissue, cell, or cell fraction which binds to AAP, AAP10, HP5, or a functional analog thereof and/or which inhibits binding of one or more of AAP, AAP 10, HP5, a functional analog thereof to the receptor.
As used herein, "normalize" refers to a change in a physiological response such that the response becomes insignificantly different from one observed in a normal patient. Thus, normalization may involve an increase or decrease in the response depending on the pathology involved.
EC50 of less than about 10"6M, and preferably, less than about, 1CT8 M.
As used herein "oral availability" refers to the rate and extent of absorption of an orally administered drug into the blood stream.
Abbreviations used in the instant application are defined further below.
Methyl (Me) — CH3 Methoxy (MeO) — OCH3
Ethyl (Et) — CH2CH3 Ethoxy (EtO) — OCH2CH3
n-Butyl (n-Bu) — CH2CH2CH2CH3 n-Butoxy (n-BuO) — OCH2CH2CH2CH3
n-Hexyl (n-Hex) — CH2CH2CH2CH2CH2CH3 n-Hexyloxy (n-HexO) — OCH2CH2CH2CH2CH2CH3
n-Octyl (n-Oct) — CH2CH2CH2CH2CH2CH2CH2CH3 n-Octyloxy (n-OctO) — OCH2CH2CH2CH2CH2CH2CH2CH3
All references cited herein are incorporated by reference in their entireties herein.
Variations, modifications, and other implementations of what is described herein will occur to those of ordinary skill in the art without departing from the spirit and scope of the invention and the claims herein.




WE CLAIM:
1. A dipeptide of formula I capable of modulating intracellular gap junctional communication
(Formula Removed)
wherein:
a Is 0 or 1;
b is 0 or 1;
d is 0-8;
and
Z is 1-7; wherein ff a is 1 then b is 0;
wherein if a is 0 then b is 1;
wherein x is 1, y and q are 1, and p is 0; or p is 1, x and q are 0, and y Is 1;
and further, wherein,
wherein if R-, is H then d is 0-8;
wherein if Ri is not H then d is 0;
wherein R1 is the side chain of an amino acid selected from the group consisting of alanine, arginine, asparagine, aspartic acid, cysteine, glutamic acid, glutamine, glycine, histidine, isoleucine, leucine, lysine, methionine, phenylalanine, proline, serine,

threonine, tryptophan, tyrosine, and valine;
wherein R2 is selected 1mm the group consisting of NH2, NHR, NR2, NR3 H, OH, SH, RO, RS, RSO, RSO2, COR, CSR, COOH, COOR, CONH2, CONHR,
CONR2, OCOR, and SCOR, wherein R = alkyl, alkenyl, aryl, aralkyl, or cycloalkyl; wherein R3 = H or CH3 and
wherein Rx is a 6-membered aromatic carbon ring comprising a substituent at the 4-position;
or a pharmaceutical^ acceptable salt thereof.
2. The peptide as claimed in claim 1, wherein said peptide is of having formula II:

(Formula Removed)

wherein: a is 0 or 1; b is 0 or 1;

d is 0-8; and
z is 1-7,
wherein if a is 1 then b Is 0;
wherein if a is 0 then b Is 1;
wherein x is 1, y and q are 1, and p is 0; or
p is 1, x and q are 0, and y is 1;
wherein if R, is H then d is 0-8; wherein if R1 is not H then d is 0;
wherein R1 is the side chain of an amino acid selected from the group consisting of alanine, arginine, asparagine, aspartlc acid, cysteine, glutamic acid, glutamine, glycine, histidine, isoleucine, leucine, lysine, methionine, phenylalanine, proline, serine, threonine, tryptophan, tyrosine, and valine;
wherein R2 is selected from the group consisting of NH2> NHR, NR2, NRs*H, OH, SH, RO, RS, RSO, RSO2, COR, CSR, COOK COOR, CONH2, CONHR. C0NR2l OCOR, and SCOR, wherein R = alkyl, alkenyl, aryl, aralkyl, or cycloalkyl;
wherein R3 = H or CH3;
wherein R* and Rg are independently selected from the group consisting of H, alkyl, alkenyl, aryl, aralkyl, halogen, CN, N02, alkoxy, aryloxy, aralkyloxy, thioalkoxy, thioaryloxy, thioaralkyloxy, +S(CH3)2, SO3H, SO2R, NH2, NHR. NR2l +NR3, OH, SH. COOH, COOR, CONHz, CONHR, CONR2, CH2OH,. NCO, NCOR, NHOH, NHNH2( NHNRH, CH2OCOR, CH2OCSR, COR, CSR, CSOR, CF„ and CCI3, and wherein R is alkyl, alkenyl, aryl, aralkyl, or cycloalkyl; and
wherein R4 or R5 is a substitueht on the 4-position of the 6-membered aromatic carbon ring; or a pharmaceutically acceptable salt thereof,
3 The peptide as claimed in claim 1 or claim 2, wherein d is 0 and Ri is the side
chain of an amino acid selected from the group consisting of alanine, arginine, asparagine, aspartic acid, cysteine, glutamic acid, glutamine, glycine, histidine, isoleucine, leucine, lysine methionine, phenylalanine, proline, serine, threonine, tryptophan, tyrosine, and valine.

4. The peptide as claimed in claim 1 or claim 2, wherein said peptide contains at least one D amino acid.
5. The peptide as claimed in claim 1 or claim 2, wherein z is 1, 2, 4, 5, 6 or 7.
6. The peptide as claimed in claim 1, wherein the aromatic carbon ring is substituted with at least one of: a lower alkyl, alkoxy, hydroxyl, carboxy, amine, thiol, hydrazide, amide, halide, hydroxyl, ether, amine, nitrile, irnine, nitro, sulfide, sulfoxide, sulfone, thiol, aldehyde, keto, carboxy, ester, an amide group; a seleno group, a thio group and derivatives thereof.
7. The peptide as claimed in any one of the preceding claims, wherein the peptide comprises a tree N-terminal, a free C-terminal, or both a free N- and C-terminal.
8. The peptide as claimed in any one of the preceding claims, wherein the pharmaceutically acceptable salt is an acid addition salt a metal salt, an amrncnium salt or an amino acid addition salt.
9. The peptide as claimed in claim 4, wherein the pharmaceutically acceptable salt is
a hydrochloride salt, a sulfate salt, a phosphate salt, an acetate salt, a maleate salt, a
fumarate salt, a tartrate salt, a citrate salt, a sodium salt, a potassium salt, a magnesium
salt, a calcium salt an ammonium or tetramethyl ammonium salt,
a lysine salt, a glycine salt or a phenylalanine salt.
10. The peptide as claimed in any one of the preceding claims, wherein the peptide
optionally comprises a hydrogen bond group and the distance between the mass center of
the hydrogen bond group and the hydrophobic group comprises from about 4 Angstroms
to about 12 Angstroms.
11. The peptide as claimed in any one of the preceding claims, wherein the peptide further comprises a hydrogen bond group and the distance between the mass center of the hydrogen bond group and the hydrophobic group comprises from about 5 Angstroms to about 10 Angstroms.
12. The peptide as claimed in claim 1, wherein the substituent has a radius of from about 3 to about 11 Angstroms.

13. The peptide as claimed in claim 12, wherein the substituent is selected from the group consisting of a methyl, ethyl, t-butyl, c-hexyl, phenyl, n-butyl, n-hexyl, n-octyl, ethoxy, t-butoxy, phenoxy, butoxy, benzyloxy, n-hexyloxy, and n-octyloxy group,
14. The peptide as claimed in any one of the preceding claims, wherein the peptide is an orally available peptide.
15. The peptide as claimed in any one of the preceding claims, wherein the peptide has a half-life in an in vitro plasma stability assay of more than about 30 minutes.
16. The peptide as claimed in any one of the preceding claims, wherein the peptide has a half-life in an in vitro plasma stability assay of more than about 48 hours.

17. The peptide as claimed in any one of the preceding claims, wherein the peptide binds to a tissue, cell, or cell fraction that is a site of action for an antiarrhythmic peptide.
18. The peptide as claimed in claim 17, wherein the antiarrhythmic peptide is selected from the group consisting of AAP, AAP10, HP5, or a functional analog thereof.
19. The peptide as claimed in claim 18, wherein the peptide antagonizes the function of the antiarrhythmic peptide.
20. The peptide as claimed in claim 19, wherein the peptide agonizes the function of the antiarrhythmic.
21. The peptide as claimed in claim 20, wherein the peptide is a modulator of a receptor of the antiarrhythmic peptide.
22. The peptide as claimed in any one of the preceding claims, wherein the peptide is selected from the group consisting of the peptides shown in Table 1.
23. The peptide as claimed in any one of the preceding claims, wherein the peptide is;

H-Gly-Lys(4-nitrobenzoyl)-OH (Compound 1);
H-Gly-Lys(4-metboxybenzoyl)-OH (Compound 4);
H-D-Lys(4-methoxybenzoyl)-Gly-OH (Compound 21}; H-0-Lys(4-nitroben20yl)G/y-OH (Compound 22); H-D-Lys(4-t-burylbenzoyl)-Gly-OH (Compound 54); H-D-Asn(NH(4-nitrobenzyl)Ala-OH (Compound 96); H-D-Lys(benzoyl)Gly-OH (Compound 23) or H-D-Asn(NH(4-methoxybenzyl)AIa-OH (Compound 95).
24. The peptide as claimed in any of the preceding claims wherein used in preparing orally administrable pharmaceutical composition.



Documents:

1974-DELNP-2005-Abstract-14-05-2008.pdf

1974-delnp-2005-abstract.pdf

1974-DELNP-2005-Claims-(04-06-2009).pdf

1974-DELNP-2005-Claims-(16-07-2008).pdf

1974-DELNP-2005-Claims-14-05-2008.pdf

1974-delnp-2005-claims.pdf

1974-delnp-2005-complete specification (granted).pdf

1974-DELNP-2005-Correspondence-Others-(16-07-2008).pdf

1974-DELNP-2005-Correspondence-Others-14-05-2008.pdf

1974-delnp-2005-correspondence-others.pdf

1974-delnp-2005-description (complete)-14-05-2008.pdf

1974-delnp-2005-description (complete)-16-07-2008.pdf

1974-delnp-2005-description (complete).pdf

1974-DELNP-2005-Drawings-14-05-2008.pdf

1974-delnp-2005-drawings.pdf

1974-DELNP-2005-Form-1-14-05-2008.pdf

1974-delnp-2005-form-1.pdf

1974-delnp-2005-form-18.pdf

1974-DELNP-2005-Form-2-(16-07-2008).pdf

1974-DELNP-2005-Form-2-14-05-2008.pdf

1974-delnp-2005-form-2.pdf

1974-DELNP-2005-Form-3-14-05-2008.pdf

1974-delnp-2005-form-3.pdf

1974-delnp-2005-form-5.pdf

1974-DELNP-2005-GPA-14-05-2008.pdf

1974-delnp-2005-gpa.pdf

1974-delnp-2005-pct-220.pdf

1974-delnp-2005-pct-306.pdf

1974-delnp-2005-pct-308.pdf

1974-delnp-2005-pct-409.pdf

1974-delnp-2005-pct-416.pdf

1974-delnp-2005-pct-notification.pdf

1974-delnp-2005-pct-request form.pdf

1974-delnp-2005-pct-search report.pdf

1974-DELNP-2005-Petition-137-14-05-2008.pdf

1974-DELNP-2005-Petition-138-14-05-2008.pdf


Patent Number 234561
Indian Patent Application Number 1974/DELNP/2005
PG Journal Number 26/2009
Publication Date 26-Jun-2009
Grant Date 08-Jun-2009
Date of Filing 10-May-2005
Name of Patentee ZEALAND PHARMA A/S,
Applicant Address SMEDELAND 26B, DK-2600 GLOSTRUP, DENMARK
Inventors:
# Inventor's Name Inventor's Address
1 BJARNE DUE LARSEN JYLLINGEVEJ 16, 1, DK-2720 VANLOSE, DENMARK
2 CARSTEN BOYE KNUDSEN MAGNOLIAVEJ 10, DK-2670 GREVE, DENMARK
3 JORGEN SOBERG PETERSEN HELLEBAKKEN 1, DK-3150 HELLEBAEK, DENMARK
PCT International Classification Number C07K 5/06
PCT International Application Number PCT/DK2003/000805
PCT International Filing date 2003-11-25
PCT Conventions:
# PCT Application Number Date of Convention Priority Country
1 60/428,973 2002-11-25 U.S.A.