Title of Invention

IMMUNOSTIMULATORY PREPARATIONS ISOLATED FROM MICROALGAE

Abstract Immunostimulatory preparations isolated from microalgae comprising polysaccharides extractable by a solvent comprising water or a mixture of water and at least one lower alkyl alcohol where the alkyl portion is from 1 to 4 carbon atoms and where the active polysaccharldes have apparent molecular weights above approximately 2 million daltons.
Full Text This application claims priority from United States Provisional Application Serial No. 60/217,001, filed July 10, 2001, the contents of which are incorporated by reference iierein.
FIELD OF THE INVENTION
The present invention relates to a method for the extraction of immunostimulatory polysaccharide preparations from food-grade microalgae. It further relates to the identification of the structurally complex immunostimulatory water-soluble polysaccharide preparations isolated from food-grade microalgae containing active polysaccharides having an apparent molecular weight above 2 million daltons. It also relates to methods for the treatment and/or prevention of a variety of disease conditions using the preparations of this Invention.
BACKGROUND OF THE INVENTION
During the past three decades immunotherapy has become an important approach for treating human diseases and conditions through the use of regimens designed to modulate immune responses. This is particularly important in pathofogicaf conditions where the immune system becomes compromised. Studies conducted in disease models and clinical trials demonstrate that augmenting host defense mechanisms is useful in treatment and prophylaxis against microbial infections, immunodeficiency, cancer, and autoimmune disorders (1 - 5). Immune enhancing protocols may also have utility for promoting wound healing. In the process of wound healing, macrophages exhibit a principal role by modulating cellular proliferation and new tissue formation/regeneration. They afso function as phagocytes, debridement agents and produce growth factors that influence the angiogenesis stage of wound repair
(6).
Historically, the first Immunostimulants developed were bacterial products (lysates and crude fractions), attenuated microbes or heat-killed bacteria. These included agents such as bacille Calmette-Guerin (BCG), Corynebacterium parvum, and lip polysaccharide (1, 2). Although these agents have had limited success due to toxicities and side-effects, many have been licensed by the USDA for immunomodulation in veterinary medicine (3). Other substances have been

developed from various sources and include those of natural origin, those derived by chemical synthesis or those synthesized using recombinant technologies. Most immunostimulants of natural origin are high molecular weight polysaccharides, glycoprotein or complex peptides (1). For example, three fungal polysaccharides derived from Schizophyllum commune (schizophylian), Lentinus edodes (lentinan) and Orioles vermicular (krestin) are cun^ently in clinical use In Japan as biological response modifiers (4). Another polysaccharide, acemannan (isolated from Aloe vera), is licensed by the United States Department of Agriculture for the treatment of fibrosarcoma in dogs and cats (7). There are a few small molecular weight immunostimulants derived from natural products such as the glycosphlngolipid KRN-7000. A clinical trial using KRN-7000 as an Immunostimulant for treatment of solid tumors is currently in progress (8). Several immunostimulants of synthetic origin also have been developed that include compounds, like isoprinosine and muramyl peptides (2). Recently a number of other immunomodulators of endogenous origin have been developed using recombinant technologies that have gained FDA approval. These agents include colony-stimulating factors, interferons and recombinant proteins (5). However, these compounds often have short half-lives and it is difficult to determine optimal dosage and appropriate combinations.
Although current immunostimulants show promise, there is still a need to develop more potent agents and increase the arsenal of available drugs for immunotherapy. One source of chemically diverse compounds that can be used for drug discovery of immunostimulants is natural products. For centuries natural products have been exploited as therapeutically useful agents, many of which are in clinical use today. Interest in natural products as a means to drug discovery is based on their unparalleled molecular diversity and rich spectrum of biological activities (9).
Since ancient times, microalgae have been used as a nutrient-dense food source. Historical records indicate that microalgae such as Spirulina platen sis was consumed by tribes around Lake Chad in Africa and by the Aztecs living near Lake Texcoco in Mexico (10). During the last several decades there has been increasing interest in the commercial production of food-grade microalgae for human consumption and as feed for livestock. Among the various microalgae that have been explored for their commercial potential Spirulina species.

Chlorella species and Aphanizomenon flos-aquae (AFA) are three major types that have been successfully produced and are in widespread use.
Both anecdotal reports and recent studies on the consumption of food-grade microalgae have reported enhanced immune function in both animals and humans. Oral administration of Chlorella pyrenoidosa has been correlated with enhanced natural killer cell activity (11) and granulocyte-macrophage progenitor cells (12) In mice infected with Listeria monocytogenes. Dietary Spirulina platensis increases macrophage phagocytic activity in chickens (13) and Spirulina fusiformis exhibits chemopreventive effects in humans (14). Human consumption of AFA has been reported to produce changes in immune cell trafficking and enhanced immune surveillance (15). The active components for all these effects have not been conclusively established.
Various compounds have been isolated from the microalgae studied herein. A number of polysaccharides and glycoproteins from Chlorella and Spirulina species have been characterized for their antitumor, antiviral and immunosfimulating activity. In contrast, no such compounds showing any biological activity have been isolated from AFA.
A number of polysaccharides have been identified from Chlorella species that possess biological activity. In U.S. Pat. No. 4,533,548 an acidic polysaccharide was isolated from Chlorella pyrenoidosa that exhibits antitumor and antiviral activity (16). The glycosyl composition for this polysaccharide was mostly rhamnose, with minor amounts of galactose, arabinose, glucose and glucuronic acid. Another polysaccharide, isolated from marine Chlorella minutissima, reported in U.S. Pat. No. 4,831,020, appears to have tumor growth-Inhibiting effects. However, no molecular weight or glycosyl composition was reported (17).
In U.S. Pat. No. 4,786,496, the lipid fraction (glycolipid portion) of marine Chlorella species displayed antitumor properties (18). Several glycoproteins have also been isolated from Chlorella species. For example, U.S. Pat. No. 4,822,612 reported a 45,000 dalton glycoprotein that has anticancer effects (19). Various other glycoproteins (20-23) and glyceroglycolipids (24) that may have immunopotentiating and antitumor properties also have been reported in the scientific literature. None of these compounds are polysaccharides.

Several different types of polysaccharides that exhibit biological activity have been isolated from Spirulina species. For example, the sulfated polysaccharide calcium spirulan inhibits tumor invasion and metastasis (25). calcium splrulan (molecular weight 74,600 daltons) is composed of rhamnose (52.3%), 3-0-methylrhamnose (32.5%), 2,3-di-O-methylrhamnose (4.4%), 3-0-methylxylose (4.8%), uronic acids (16.5%) and sulfate (26).
U.S. Pat. No. 5,585,365 discloses that an antiviral polysaccharide with a molecular weight between 250,000 and 300,000 daltons was isolated from Spirulina species using hot water extraction (27). This polysaccharide is composed of rhamnose, glucose, fructose, ribose, galactose, xylose, mannose, glucuronic acid and galacturonic acid. A number of other low molecular weight polysaccharides that range between 12,600 and 60,000 daltons recently have been isolated from Spirulina species (28-30).
One way to determine immunostimulatory activity is to use a biological assay involving macrophages. Monocytes/macrophages are found in practically every tissue of the body where they are critical in coordinating immune responses and numerous biological processes (31). They play a major role in phagocytosis. Immune surveillance, wound healing, killing of microbes and tumor cells, and antigen presentation to T lymphocytes (32). In cancer, macrophages mediate tumor cytotoxicity functions through the production of cytokines and other immune factors (33). In order for macrophages to play a major role in adaptive and innate immunity they must respond effectively to environmental agents by first becoming activated (34). Macrophage activation Is mediated by proinflammatory transcription factors such as nuclear factor kappa B (NF-kappa B). Such transcription factors then control and modulate the activation/ repression of an array of genes that mediate a variety of immune responses.
In unstimulated macrophages, NF-kappa B exists as inactive heterodimers sequestered by inhibitory-kappa B (l-kappa B) proteins within the cytosol. Agents that cause l-kappa B proteins to dissociate and degrade allow for the translocation of NF-kappa B dimmers to the nucleus where they can activate transcription of downstream genes (35). Target genes regulated by NF-kappa B include proinflammatory cytokines, chemokines, inflammatory enzymes, adhesion molecules and receptors (36).

In this invention a transcription factor based assay for NF-kappa B in human monocots was used to guide extraction, isolation, characterization and development of immunpstimulatory polysaccharide preparations from food-grade microaigae. The polysaccharides of the present invention are both water soluble and soluble in aqueous ethanol solution unlike almost all other polysaccharides now available.
SUMMARY OF THE INVENTION
Novel water-soluble polysaccharide preparations having macrophage immunostimulatory activity and containing active polysaccharides having apparent molecular weights above 2 million daltons were isolated from Aphanizomenon flos-aquae (AFA), Chlorella pyrenoidosa, and Spirulina platensis. The instant polysaccharide preparations are at least a thousand times more active for monocots activation than polysaccharide preparations that are currently used clinically for immunotherapy in cancer patients.
According to one embodiment of the invention, immunostimulatory preparations are isolated from microaigae comprising polysaccharides extractable by a solvent comprising water or a mixture of water and at least one lower alkyl alcohol where the alkyl portion is from 1 to 4 carbon atoms and where the active polysaccharides have apparent molecular weights above approximately 2 million daltons. According to another embodiment, the immunostimulatory activity of the immunostimulatory preparation is manifested by monocyte/macrophage activation. According to another embodiment, the immunostimulatory preparation is extracted from the microaigae Aphanizomenon flos-aquae. According to another embodiment, the immunostimulatory preparation is extracted from the microaigae Chlorella pyrenoidosa. According to another embodiment, the immunostimulatory preparation is extracted from the microaigae Spirulina platensis. According to another embodiment, the glycosyl components of the active polysaccharides of the immunostimulatory preparation are substantially comprised of mannose, glucose, rhamnose, galactose, fucose, methylated sugars and N-acetylated amino sugars. According to another embodiment, the glycosyl components of the active polysaccharides of the immunostimulatory preparation are substantially comprised of arabinose, galactose, rhamnose, glucose and methylated sugars. According to another

embodiment, the glycosyl components of the active polysaccharides of the mmunostimulatory preparation are substantially comprised of rhamnose, jiucuronic acid, fucose, galactose and methylated sugars. According to another 3mbodiment, a phamiaceutical composition comprises any one of the previous mmunostimulatory preparations and a pharmaceutically acceptable carrier or 3xcipient. According to another embodiment, a dietary supplement comprises any one of the previous immunostimulatory preparations and an acceptable earner or excipient for dietary supplements.
According to another embodiment, a method of enhancing immune function in an individual in need of such treatment, comprises administering to said individual an effective amount of the pharmaceutical composition or dietary supplement. According to another embodiment, the individual is suffering from a viral, bacterial or fungal infection. According to another embodiment, the individual is suffering from cancer. According to another embodiment, the individual is suffering from an immune deficiency. According to another embodiment, the individual is a human being. According to another embodiment, the individual is an animal.
According to another embodiment, a process to obtain a preparation from food-grade microalgae enriched for immunostimulatory polysaccharides, jcpmprises thesteps of: (a) producing an extract by extracting the microalgae with a solvent comprising water or a mixture of water and at least one lower alkyl alcohol where the all
process to obtain a preparation from food-grade microalgae. enriclied for immunostimulatory polysaccharides is isopropanol or propanol. According to another embodiment, the preferred alcohol concentration in step (a) is from 20-80%. According to another embodiment, the preferred temperature of extraction is between 40 and 80 degrees C. According to another embodiment, the process is used to obtain a preparation enriched for immunostimulatory polysaccharides from Aphanizomenon flos-aquae. According to another embodiment, the process is used to obtain a preparation enriched for immunostimulatory polysaccharides from Chlorelfa pyrenidosa. According to another embodiment, the process is used to obtain a preparation enriched for immunostimulatory polysaccharides from Spirulina platensis. According Xo another embodiment, the concentration step (b) is cam"ed out (when needed) by evaporation of the solvent, preferably under reduced pressure. According to another embodiment, the concentration step (b) is carried out (when needed) by freeze drying. According to another embodiment, the concentration step (b) is carried out (when needed) by dialysis. According to another embodiment, the polysaccharide preparation is precipitated in step (c) by the addition of ethanol to a final concentration of about 80% ethanol. According to another embodiment, the polysaccharide preparation is precipitated in step (c) by cooling the extract. According to another embodiment, the polysaccharide preparation is precipitated in step (c) by the addition of a salt. According to another embodiment, the salt is ammonium sulfate. According to another embodiment, the precipitated polysaccharide preparation is separated in step (d) by filtration. According to another embodiment, the precipitated polysaccharide preparation is separated in step (d) by centrifugation. According to another embodiment, the precipitated polysaccharide preparation is washed In step (e) by 95% ethanol. According to another embodiment, the process further comprises purifying the precipitate by dissolving the precipitate in water and removing substantially all components of less than approximately 100,000 daltons molecular mass by ultra-filtration. According to another embodiment, the process further comprises purifying the precipitate by dissolving the precipitate in water and removing substantially ail components of less than approximately 2 million daltons molecular mass by size exclusion column chromatography.
According to another embodiment, a method of treating an individual with an immunostimulatory polysaccharide preparation in order to provide to the

individual a stimulation of monocyte/macrophage activity comprises administering to the individual an effective amount of a polysaccharide preparation extracted from food-grade microalgae in combination with an acceptable canier. According to another embodiment, the immunostimulatory polysaccharide preparation is administered to enhance wound healing. According to another embodiment, the immunostimulatory polysaccharide preparation is administered to treat cancer. According to another embodiment, the immunostimulatory polysaccharide preparation is administered to treat immunodeficiency. According to another embodiment, the immunostimulatory polysaccharide preparation is administered to treat a viral, bacterial or fungal infection. According to another embodiment, the individual is a human being. According to another embodiment, the individual is an animal. According to another embodiment, a method of treating an individual with an immunostimulatory polysaccharide preparation in order to provide to the individual a stimulation of monocyte/macrophage activity comprises administering to the individual an effective amount of a polysaccharide preparation extracted from Aphanizomenon flos-aquae in combination with an acceptable carrier. According to another embodiment, a method of treating an individual with an immunostimulatory polysaccharide preparation in order to provide to the individual a stimulation of monocyte/macrophage activity comprises administering to the individual an effective amount of a polysaccharide preparation extracted from Chforella pyrenoidosa. According to another embodiment, a method of treating an individual with an immunostimulatory polysaccharide preparation in order to provide to the individual a stimulation of monocyte/macrophage activity comprises administering to the individual an effective amount of a polysaccharide preparation extracted from Spirullna platensis.
BRIEF DESCRIPTION OF THE FIGURES
Fig. 1. Size exclusion HPLC chromatogram of polysaccharide preparation
NP16847 (Example 1), 75 μ L injection at 500 μ g/mL
Fig, 2. Size exclusion HPLC chromatogram of polysaccharide preparation
NP16848 (Example 2), 200 μ L injection at 125|jg/mL.
Fig. 3. Size exclusion HPLC chromatogram of polysaccharide preparation
NP16846 (Example 3), 200IJL injection at 35pg/mL.

Fig. 4. Microalgal polysaccharide preparations NP16847, NP16848 and
• NP16846 enhance proinflammatory cytokine mRNA production. RT-PCR results for IL-1P mRNA, TNF-a mRNA and GAPDH mRNA in THP-1 cells at 2 hours: control, bacterial LPS at 10pg/mL, (1) polysaccharide preparation NP16847 at 0.5pg/mL, (2) polysaccharide preparation NP16846 at 0.5pg/mL, and (3) polysaccharide preparation NP16848 at 0.5pg/mL.
Fig. 5. Flow chart showing protocol for hot water extraction at 40°C
followed by 70% ethanol precipitation to remove phycocyanin material (Example
4).
Fig, 6. Flow chart showing protocol for hot water extraction at 40°C
followed by ammonium sulfate precipitation to remove phycocyanin material
(Example 5).
Fig. 7. Flow chart showing protocol for hot water extraction at 70 ° C
(Example 6).
Fig. 8. Flow chart showing protocol for 70% ethanol extraction at 40 °C
without butanol partition (Example 7).
Fig. 9. Flow chart showing protocol for 70% ethanol extraction at 40""C
followed by direct ethanol precipitation (Example 8).
Fig. 10. Flow chart showing protocol for 70% ethanol extraction at 40°C
followed by direct 80% ethanol precipitation (Example 9).
Fig. 11. SEC HPLC analysis of pre- and post-uJtrafiltrate NP16847
preparations using optimal extraction conditions of 50% ethanol/60°C (Example
24).
DETAILED DESCRIPTION OF THE INVENTION
The transcription factor-based bioassay for activation of .NF-I
(1pg/1x106 cells). This plasmid, a gift from Dr. Riccardo Dalla-Favera, contains two copies of NF-I Glycosyl composition and glycosyl linkage analyses were performed by The University of Georgia, Complex Carbohydrate Research Center. The glycosyl composition was determined using GC-mass spectrometry analysis of the TMS-methyl glycosides. In order to identify the O-methylated sugars detected during the TMS-methyl glycoside procedure, glycosyl composition was also determined using the alditol acetate procedure (38). Glycosyl linkage analysis was performed using the Hakomori procedure (39), In combination with carboxyl-reduction in order to detect uronic acid linkages (40).
EXAMPLE 1 — Initial isolation of a high molecular weight polysaccharide preparation from AFA (NP16847) that exhibits potent monocyte activation properties
A crude extract from AFA (Lot No. 0110FA from Cell Tech, Klamath Falls, OR), was prepared by extracting the freeze-dried material (125g) three times (4 hours each) with 70% ethanol at 40°C. This crude extract had an EC50 value of 10pg/mL. Aqueous ethanol extracts were evaporated to dryness and then solvent partitioned between water and chloroform (1:1). The activity was found exclusively in the water layer which was further partitioned against n-butanol (water:n-butanol, 63:37). The more active water layer (EC5o=0.5ijg/mL) was

subjected to alcohol precipitation (water:methanol:ethanol, 1:2:3) at -80 °C for 24 hours. This precipitated material, which is referred to as the pre-ultrafiltrate preparation, had an EC50 value of 0.2μg/mL and represents a recovery of 3% of dry AFA weight. This material was then passed through an ultrafiltration device with a 100,000 molecular weight cut-off polyethersulfone membrane (Centricon Plus-20 from Millipore, Bedford, MA). The retentate was subsequently washed several times with 3% KCI (w/v) to remove impurities that adhered (probably through ionic interaction) to the large molecular weight material. The retentate, which is referred to as post-ultrafiltrate material, had an EC50 value of 0.1pg/mL, representing a recovery of 0.6%.
The cryohydrates content of the post-ultrafiltrate NP16847 preparation was estimated to be between 90% and 100% using a colorimetric assay (41) with phenol-sulfuric acid at 450 nm and 490 nm. It is concluded from this result that this material is a preparation of polysaccharides. Elemental analysis performed by Galbraith Laboratories, Inc. (Knoxville, TN) revealed that this material contains the following elements: 49.1% carbon, 40.8% oxygen, 7.62% hydrogen, 2.46% nitrogen and trace amounts of sulfur. Glycosyl composition and linkage analysis for the post-ultrafiltrate is presented in Table 1. NP16847 is comprised predominantly of mannose, glucose, 4-methyl mannose, rhamnose and methylated sugar residues along with other simple sugars and acetylated amino sugars. This is the first report of any polysaccharide isolated from AFA exhibiting any type of biological activity.
The post-ultrafiltrate NP16847 was analyzed using size exclusion chromatography (SEC). The set-up consisted of a Model 600E system controller, UK6 injector, Model 600 solvent delivery system, Model 401 differential refractometer and a Model 3396A Hewlett-Packard integrator. Analyses were performed at a flow rate of 1 mL/minute using HPLC grade water and a Shodex Opal KB-805 SEC column (300mm length x 8mm ID) held at 30°C. This column is capable of separating molecules up to an estimated molecular weight of 4 million daltons. Analysis of post-ultrafiltrate NP16847 showed one peak that eluted in the void volume (Fig. 1) and had a retention time consistent with an apparent molecular weight of above 2 million daltons based on comparison with dextran standards.

The isolation procedure described in Example 1 for the purification of AFA poiysaccharides is novel since tlie initial extraction uses 70% ethanol as compared with prior art procedures which employ hot water. To determine if this procedure could be used as a general method for the extraction of immunostimulatory polysaccharides from other food-grade microalgae, the procedure described in Example I was applied to two other microalgae commonly consumed as food supplements namely Chlorella pyrenoidosa and Spirullna platensis.
EXAMPLE 2 — initial isolation of a high molecular weight polysaccharide preparation from Chlorella pyrenoidosa (NP16848) that exhibits potent monocyte activation properties
A crude extract from Chlorella (Lot No. VP0978 from Sun Chlorella, Torrance, CA), was prepared by extracting the freeze-drled material (35g) three times (4 hours each) with 70% ethanol at 40°C. This crude extract had an EC50 value of 25ijg/mL. Aqueous ethanol extracts were evaporated to dryness and then solvent partitioned between water and chloroform (1:1). The activity was found exclusively in the water layer which was further partitioned against n-butanol (water:n-butanol, 63:37). The more active water layer was subjected to alcohol precipitation (water:methanol:ethanoI, 1:2:3) at -80°C for 24 hours. The precipitate material was then passed through an ultrafiltration device with a 100,000 molecular weight cut-off polyethersulfone membrane (Centricon Plus-20 from Millipore, Bedford, MA). The retentate was subsequently washed several times with 3% KCI (w/v) to remove impurities that adhered (probably through ionic interaction) to the large molecular weight material. The post-ultrafiltrate material had an EC50 value of 0.3μg/mL, and represented a recovery of 0.2%.
The carbohydrate content of the post-ultrafiltrate NP16848 preparation was estimated to be between 90% and 100% using a colorimetric assay (41) with phenol-sulfuric acid at 450 nm and 490 nm. It is concluded from this result that this material is a preparation of polysaccharides. Glycosyl composition and Iinl
preparations from Chlorella species have been reported in the literature, NP16848 is a novel composition.
The post-ultrafiitrate NP16848 analyzed using the HPLC size exclusion chromatography procedure described in Example 1 was found to contain one peak that eluted in the void volume (Fig. 2) and had a retention time consistent with an apparent molecular weight of above 2 million daltons based on comparison with dextran standards.
EXAMPLE 3 — Initial isolation of a high molecular weight polysaccharide preparation from Spirufina platensis ^NP16846) that exhibits potent monocyte activation properties
A crude extract from Spinilina (Lot No. B16933 from Triarco Industries, Wayne, NJ) was prepared by extracting the freeze-dried material (35g) three times (4 hours each) with 70% ethanol at 40""C. This crude extract had an EC50 value of 50μg/mL. Aqueous ethanol extracts were evaporated to dryness and then solvent partitioned between water and chloroform (1:1). The activity was found exclusively in the water layer which was further partitioned against n-butanol (watern-butanol, 63:37). The water layer was the more active and was subjected to alcohol precipitation (water:methanoi:ethanol, 1:2:3) at -80°C for 24 hours. The precipitate material was then passed through an ultrafiltration device with a 100,000 molecular weight cut-off polyethersulfone membrane (Centricon Plus-20 from Millipore, Bedford, MA). The retentate was subsequently washed several times with 3% KCl (w/v) to remove impurities that adhered (probably through ionic interaction) to the large molecular weight material. The post-ultrafiltrate material had an EC50 value of 0.3μg/mL, representing a recovery of 0.1%.
The carbohydrate content of the post-ultrafiltrate Spirulina preparation was estimated to be between 90% and 100% using a colorimetric assay (41) with phenol-sulfuric acid at 450 nm and 490 nm. It is concluded from this result that this material is a preparation of polysaccharides. Glycosyl composition and linkage analysis for the post-ultrafiltrate is presented in Table 3. NP16846 Is comprised predominantly of rhamnose, glucuronic acid, fucose, galactose and methylated sugar residues along with other simple sugars, uronic acids and acetylated amino sugars. Other polysaccharides with similar glycosyl

compositions from Spirulina species have been reported in the literature but are mucli smaller in size than NP16846.
The post-ultrafiltrate NP16846 analyzed using the HPLC size exclusion chromatography procedure described in Example 1 was found to contain one peak that eluted in the void volume (Fig. 3) and had a retention time consistent with an apparent molecular weight of above 2 million daltons based on comparison with dextran standards.
Monocyte/macrophage activation
Messenger RNA (MRNA) levels of proinflammatory cytokines IL-1p and TNF-a were measured to confirm THP-1 monocyte/macrophage activation by microalgal polysaccharide preparations. The mRNA levels of GAPDH were also assayed as a control to detaining the specificity of changes in IL-1p and TNF-a mRNA levels. Since GAPDH is a housekeeping gene, mRNA levels would be expected to remain constant unless changes were induced artifactually.
RT-PCR primers for IL-ip, TNF-a and GAPDH were purchased from Integrated DNA technologies, Inc. (Coralville, lA). Sequences for the primers were described in Su et al. (42). IL-lp poniard (5"-ATG-GCA-GAA-GTA-CCT-AAG-CTC-GC-3"); IL-lp reverse (5"-ACA-CAA-ATT-GCA-TGG-TGA-AGT-CAG-TT-3"); TNF-a fonward (5"-GAG-TGA-CAA-GCC-TGT-AGC-CCA-TGT-TGT-AGC-3"); TNF-a reverse (5"-GCA-ATG-ATC-CCA-AAG-TAG-ACC-TGC-CCA-GAC-T-3"); GAPDH fonfl/ard (5"-TGA-AGG-TCG-GAG-TCA-ACG-GAT-TTG-GT-3"); GAPDH reverse (5"-CAT-GTG-GGC-CAT-GAG-GTC-CAC-CAC-3").
Actively growing THP-1 cells (3 mLs, 1x10® cells/mL) were incubated for 2 hours in the presence of test material. Total RNA was isolated using the TRI Reagent® kit (Molecular Research Center, Inc., Cincinnati, OH) in which cells are lysed using a combination of phenol and guanidine thiocyanate. After the addition of bromochloropropane, RNA is separated into the aqueous phase and subsequently precipitated with isopropanol. Total RNA recovered using this method was about 30pg. Electrophoresis of isolated RNA using 0.8% vagaries gel showed no signs of contaminating DNA.
RT-PCR reactions were run using kit reagents from Promega (Madison, Wl). Each reaction used the following components (total volume of 30pL): 6pL AMV/Tfl 5x reaction buffer, 0.6pL dNTP mix (lOmM), 1.2pL MgSd4 (25mM),

0.6pL AMV reverse transcriptase (5units/|jL), 0.6pL Tfl DNA polymerase (5units/pL), 1.2ML of each primer (15pmoi/ML), and 2ng total RNA (IL-1p, TNF-a) or 5ng total RNA (GAPDH). The RT-PCR protocol used a Techne Unit Progene automatic thermal cycler. First cycle consisted of 45 minutes at 48°C, followed by 2 minutes at 94""C. Amplification was achieved using 35 cycles: denature at 94°C for 45 seconds, anneal at 60°C for 1 minute, and extend at Sa"C for 2 minutes. The final cycle held samples at 68°C for 7 minutes. Electrophoresis of RT-PCR products (mRNA IL-ip, TNF-a and GAPDH) was accomplished using 12|jL of reaction mix on 5% polyacrylamide gels with ethidium bromide used as the staining agent.
Treatment of THP-1 cells with either LPS or microalgal polysaccharide preparations resulted in a dramatic increase in both IL-ip mRNA (810bp) and TNF-a mRNA (444bp), as compared with the control. The mRNA levels of the housekeeping gene glyceraidehyde phosphate dehydrogenase (GAPDH, lOOObp) was the same for all samples (Fig. 4).
The observed NF-kappa B activation by NP16847, NP16848, and NP16846 was not due to endotoxin contamination of the preparations. This was confirmed by the results of the following two experiments which were conducted to address this possibility. First, polymyxin B (10pg/mL, Sigma Chemical Co., St. Louis, MO) was added in combination with each polysaccharide preparation (0.1 to 1pg/mL) to observe whether there was any abrogation in NF-kappa B activation. Polymyxin B is a polycationic antibiotic known to block many of the biological effects of LPS by binding to the lipid A portion of the molecule. All three microalgal polysaccharide preparations were insensitive to polymyxin B addition (data not shown). Addition of polymyxin B to LPS (10pg/mL) suppressed NF-kappa B activation by 75%. The second experiment used to examine possible endotoxin-mediated effects was to look for the presence of p-hydroxymyristate in the glycosyl composition analysis. There was no detectable levels of p-hydroxymyristate in sample preparations of NP16848 and NP16846 . Thus, it is unlikely that the observed macrophage activation by NP16848 and NP16846 is due to endotoxins.
However, in two different sample preparations of NP16847 small amounts of p-hydroxymyristate (0.6% of total peak area) were detected. In order to

determine how much "endotoxin-like" material was present, six samples of AFA were analyzed using the Limulus amebocyte lysate (LAL) assay (analysis performed by BioWhittaker, Walkersville, MD). The amount of LAL positive material detected using this assay represented 0.002% of microalgal dry weight. By comparison, the percent recovery of NP16847 is about 300 times greater (0.6% of microalgal dry weight). This means that at the concentration required to produce half-maximal NF-kappa B activation by NP16847 (100ng/mL), the total amount of potential LAL positive material present would be 300pg/mL. This concentration of endotoxin would not be detectable using the macrophage assay system. Therefore, possible endotoxin contamination cannot account for the stimulatory effect of NP16847 on macrophage activation.
Examples 1 through 3 demonstrate that polysaccharide preparations with potent immunostimulatory activity are extractable from food-grade microalgae using 70% ethanol at 40°C. Subsequent steps in the isolation of these polysaccharide preparations involved a complex protocol and the use of organic solvents. Polysaccharides are traditionally extracted from natural sources using hot water due to their high water solubility. This hot water isolation procedure therefore would be expected to yield a higher percent recovery of these polysaccharides as compared to the initial extraction using 70% ethanol. In addition, since a hot water extract would be less likely to contain non-polar material, it would not be necessary to use organic solvent partitioning if this method proved successful. However, contrary to the predicted behavior, water extraction (Examples 4 through 6) gave preparations substantially less active than the procedure using the initial extraction with aqueous ethanol (Example 1) and also posed additional problems.
Both the HPLC size exclusion chromatographic analysis and immunostimulatory activity (macrophage activation) were measured as described in the earlier Examples. The microalgae used in each Example was freeze-dried AFA (Lot. 041900 Merc) obtained from Klamath Algae Products Inc., Klamath Falls, OR. Ultrafiltration (when used) was carried out using a device with a 100,000 molecular weight cut-off polyethersulfone membrane (Centricon Plus-20 from Millipore, Bedford, MA). For each experiment, the retentate material from ultrafiltration was washed several times with 3% KCI (w/v) to remove impurities

that adhered (probably through ionic interaction) to the large molecular weight material.
EXA!\/IPLE 4 — 40°C water extraction and phvcocvanin removal with alcohol precipitation
Water extraction of AFA at 40°C was problematic because this crude extract contained a large amount of phycocyanin (a blue proteinaceous pigment). Attempts to remove phycocyanin by ultrafiltration were unsuccessful since this material was retained along with the NP16847 polysaccharide preparation in the 100,000-daIton molecular weight cut-off filter. Complete precipitation of the phycocyanin material by alcohol requires a solution of 70% ethanol or greater (data not shown). In order to evaluate this method, 10g of freeze-dried AFA was extracted three times with water (62.5mLs each time) at 40°C, between 4 and 8 hours each time. Crude water extract was lyophilized and ridiculed in 40mLs of water. Ethanol was added (92mLs) at room temperature to achieve a final concentration of 70% ethanol. Perceivable materials (containing phycocyanin) were removed and the supernatant passed through an ultrafiltration device. The material at each step in the isolation procedure was evaluated for macrophage activation (Fig. 5). Clearly, the majority of the immunostimulatory activity was lost in the precipitate (also containing phycocyanin) during the 70% ethanol precipitation. The percent recovery of post-ultrafiltrate material (above 100,000 daltons) using this method was 1.0%. Although this percent recovery is higher than the 0.6% recovery of the post-ultrafiltrate obtained using the 70% ethanol extraction procedure of Example 1, this material contains other substances besides NP16847 since it had an EC50 value of 1000ng/mL. By comparison, the material from Example 1 has an EC50 value of lOOng/mL.
EXAMPLE 5 — 40°C water extraction and phvcocvanin removal with ammonium sulfate
Methods for the isolation of phycocyanin (43, 44) typically use an ammonium sulfate precipitation (40 - 65% saturation). • This protocol was investigated to evaluate whether ammonium sulfate precipitation could selectively remove phycocyanin from the crude extract. Freeze-dried AFA (lOg) was extracted three times with water (62.5mLs each time) at 40°C, between 4 and 8 hours each time. Crude water extract was lyophilized and redissolved in 40 mLs

of water containing 48g of ammonium sulfate (50% saturation). Perceivable materials (containing phycocyanin) were removed and the supematant passed through an ultrafiltration device. The percent recovery of post-ultrafiltrate material was 1.32%, but probably contained little NP16847 since its specific activity was quite low (EC50 > 1000ng/mL). Figure 6 summarizes the immunostimulatory activity of the material at each step in the isolation procedure. Similar to the previous approach, the majority of NP16847 was precipitated along with the phycocyanin by the addition of ammonium sulfate.
Clearly, the attempts to separate phycocyanin from NP16847 in the crude water extract were not successful. In addition, re-extraction of the marc material (leftover from the 40°C water extraction) using aqueous ethanol at higher temperatures (e.g. 50% ethanol/60°C) resulted in the isolation of a substantial amount of NP16847 (see Example 43). Thus, extracting with water at 40°C did not provide a complete recovery of NP16847.
EXAMPLE 6 — 70°C hot water extraction
Water extraction at higher temperatures such as 70°C would cause phycocyanin to denature and precipitate, leaving NP16847 and other polar molecules in solution. To evaluate this approach, 20g of freeze-dried AFA was extracted three times with water (125mLs each time) at 70°C, between 4 and 8 hours each time. This crude extract did not appear to contain any phycocyanin material as evidenced by the lack of blue color. The crude water extract was lyophilized and redissolved in 80mLs of water. NP16847 was precipitated using alcohol (watenmethanokethanol, 1:2:3) at -20°C for 24 hours. Precipitable materials were passed through an ultrafiltration device. Figure 7 summarizes the immunostimulatory activity of the material at each step in the isolation procedure. The EC50 value for macrophage activation of the post-ultrafiltrate material (200ng/mL) was slightly higher than the material obtained in Example 1 (100ng/mL). The percent recovery of post-ultrafiltrate material obtained using this method was 1.74%, substantially higher than the 0.6% NP16847 recovery obtained from the 70% ethanol procedure of Example 1. Therefore extraction with 70°C water recovers about 3 times as much NP16847 as indicated by the comparable EC50 values of the post-ultrafiltrate materials.

Isolation of NP16847 using hot water extraction (at 70°C) offers several advantages over the isolation procedure in Example 1. No organic solvents are used, only a few steps are required to obtain the final material, and about 3 times more NP16847 is extracted. However, there are several disadvantages. First, the crude water extract needs to be lyophilized in order to concentrate it to avoid excessively high volumes of alcohol in the precipitation. Second, the pre-ultrafiltrate contains a substantial amount of inactive material (as evidenced by a low ECso value of about 500ng/mL and the HPLC chromatogram in Fig. 7) which results in a very slow purification using the ultrafiltration devices.
Several additional methods were evaluated based on modifications to the 70% ethanol extraction procedure described in Example 1. The following Examples describe isolation procedures where the use of organic solvents was not required and the isolation is accomplished in a limited number of steps. A simple, economic and efficient process was developed which overcame all problems associated with hot water extraction.
EXAI\/IPLE 7 — 70% ethanol extraction at 40°C with chloroform partitioning
For the extraction of NP16847 in Example 1, the second solvent partitioning step between n-butanol and water resulted in a substantial loss of immunostimulatory activity into the butanol layer. Therefore, the protocol in Example 1 was modified to remove the n-butanol solvent partition step. This new method is Identical to the procedure in Example 1 except that there is only one solvent partition between chloroform and water (1:1). Figure 8 summarizes the isolation scheme and immunostimulatory activity at each step in the isolation process. The EC50 value for the post-ultrafiltrate material obtained using this method (200ng/mL) was slightly higher than the material obtained in Example 1 (100ng/mL). The percent recovery of post-ultrafiltrate NP16847 obtained using this procedure was 1.97%. Therefore, the removal of the butanol solvent partition step from the 70% ethanol extraction procedure (Example 1) enhanced recovery of post-ultrafiltrate NP16847 by over 3 fimes. However, the major disadvantage of this procedure is the use of chloroform in the organic solvent partition.
EXAMPLE 8 — 70% ethanol extraction at 4Q°C and direct alcohol precipitation
In order to evaluate an approach that skips both the butanol and chloroform partition, lOg of freeze-dried AFA was extracted two times with 70%

ethanol (125mLs each time) at 40°C. The first extraction was for 3 hours and the second extraction was for 12 hours. Crude 70% ethanol extract was stored at -20°C for several hours and precipitable material removed by centrifugation. Precipitate was washed with cold 95% ethanol (to remove remaining non-polar material), redissolved in water and then passed through an ultrafiltration device. Figure 9 summarizes the immunostimulatory activity of the material at each step in the isolation procedure. EC50 value of the post-ultrafiltrate material was slightly higher (200ng/mL) as compared to the material obtained in Example 1 (lOOng/mL). The percent recovery of post-ultrafiltrate NP16847 was 1.2%. Although this yield Is 2 times higher than that obtained using the extraction procedure described in Example 1, It Is about 30% less than the recovery obtained using the protocol in Example 7. This lower yield is probably due to incomplete precipitation in 70% ethanol.
EXAMPLE 9 — 70% ethanol extraction at 4Q°C and direct 80% alcohol precipitation
The previous method (Example 8) was slightly modified to obtain a greater recovery of NP16847. The cmde extract from the 70% ethanol extraction was adjusted to 80% ethanol by addition of cold 100% ethanol and stored at -20°C for several hours. Precipitable material was processed the same as above. Figure 10 summarizes the Isolation scheme and immunostimulatory activity at each step in the isolation process. This modified method resulted In 5.7% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 200ng/mL in the monocyte activation assay. The percent recovery of post-ultrafiltrate material was 1.8%. EC50 value for the post-ultrafiltrate material {200ng/mL) was slightly higher than that observed for the material obtained in Example 1 (lOOng/mL), but identical to post-ultrafiltrate values obtained from Examples 6 and 7.
The procedure of direct precipitation of the NP16847 polysaccharide preparation from the crude 70% ethanol extract (Example 9) successfully achieves the original aims. No organic solvents (or methanol) are used, there is no lyophilization/solvent evaporation step, and only a few steps are required to obtain a relatively pure preparation of NP16847. A semi-pure preparation of NP16847 (70% of which is less frian 100,000 daltons) can be obtained with elimination of the ultrafiltration purification step (refer to pre- and post-ultrafiltrate

HPLC chromatograms in Fig. 10). This pre-ultraflltrate NP16847 preparation would be sufficient for a dietary supplement (botanical) extract. Isolation of this material would simply require a direct alcohol precipitation from a crude 70% ethane extract.
Tlie following points summarize why this isolation procedure (Example 9) was superior to the others tested.
1. Water extraction at 40°C.
a. Contains high levels of phycocyanin which cannot be separated
from NP16847 by ultrafiltration or by ethanoi or ammonium sulfate
precipitation.
b. NP16847 obtained following ultrafiltration was of a low specific
activity, EC50 -lOOOng/mL vs. 200ng/mL (Example 9).
c. The marc material contained a substantial amount of NP16847
that could not be recovered using water extraction at this
temperature (see Example 43).
2. Water extraction at 70""C.
a. Water extraction at this temperature contains excessive amounts
of inactive polar material in the pre-ultrafiltrate. This is undesirable
for two reasons. First, development of a pre-ultrafiltrate preparation
would contain low levels of NP16847. Second, ultrafiltration is
extremely slow to obtain a post-ultrafiltrate NP16847 preparation.
b. Although the procedure does not use toxic organic solvents it
does require a lyophilization step of the crude extract.
3. 70% ethanoi extraction followed by organic solvent partitioning.
a. Clearly the major disadvantage of this step is the use of an
organic solvent (i.e. chloroform) to remove non-polar material.
From the examples described above, the optimum general procedure
(Example 9) involves two initial extractions of freeze-dried AFA with 70% ethanoi
at 40°C. Crude extract is adjusted to 80% ethanoi and cooled to -20°C.
Precipitate is collected and washed with cold 95% ethanoi to remove residual
lipophilic material. The high molecular weight material (over 100,000 daltons),
comprising -30% of the pre-ultrafiltrate polysaccharide preparation, can be
isolated using ultrafiltration. The following provides a comparison between the

NP16847 preparation obtained in Example 9 and NP16847 prepared by extraction with 70% ettianolMCC (Example 1):
NP16847 (Example 9) NP16847 (Example 1)
Pre-ultrafiltrate Recovery 5.7% 3.0%
Pre-ultrafiltrate EC50 value 200ng/mL 200ng/mL
Post-ultrafiltrate Recovery 1.8% 0.6%
Post-ultraflltrate EC50 value 200ng/mL lOOng/mL
These data demonstrate that extracting AFA using the procedure in Example 9 results in 2 times more pre-ultrafiltrate and 3 times more post-ultrafiltrate NP16847. However, the EC50 value of the post-ultrafiltrate preparation obtained by this procedure is slightly higher than that obtained from Example 1, indicating that some of the enhanced recovery is due to inactive material. Therefore, the conditions used in Example 9 were selected as a starting point for further optimization to improve the specific activity of the NP16847 preparation because of the following advantages that are offered by this new isolation method:
1. Optimal yield and good specific activity of both the pre- and post-ultrafiltration NP 16847 polysaccharide preparations.
2. No toxic organic solvents are used.
3. No rotary evaporation or lyophilization of large volumes of water or solvent is involved.
Examples 10-38 provide a detailed analysis of changing both extraction temperature and ethanol concentration in order to optimize conditions used in Example 9.
EXAMPLE 10 — 70% ethanol extraction at 50°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at SCC with 70% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined {11.2mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL.

This extraction procedure resulted in 6.5% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 100ng/mL in tiie monocyte activation assay (Table 4).
EXAMPLE 11 — 70% etiianol extraction at 60°C and direct 80% alcohol precipitation
One g of freeze-drled AFA was extracted at BCC with 70% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.2mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This execration procedure resulted in 7.1% recovery of pre-ultrafiltrate NP 16847 preparation and an EC50 value of lOOng/mL in the monocyte activation assay (Table 4).
EXAMPLE 12 — 70% ethanol extraction at 70°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 70°C with 70% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted In 7.1% recovery of pre-ultrafiltrate NP 16847 preparation and an EC50 value of 75ng/mL in the monocyte activation assay (Table 4). Removal of low molecular weight material ( EXAMPLE 13 — 70% ethanol extraction at 80°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 80° C with 70% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from

both extractions were combined (11.2mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 7.6% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 50ng/mL in the monocyte activation assay (Table 4).
EXAIVIPLE 14 — 70% ethanol extraction at ZZ"C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 23°C with 70% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for T2 hours. Supernatants from both extractions were combined (11.5mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 4.5% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of >250ng/mL in the monocyte activation assay (Table 4).
EXAIVIPLE 15 — 60% ethanol extraction at 23°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 23""C with 60% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.3mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 7.0% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of >250ng/mL in the monocyte activation assay (Table 4).

EXAMPLE 16 — 60% ethanol extraction at 40°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 40°C with 60% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.2mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 8.4% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 200ng/mL in the monocyte activation assay (Table 4).
EXAIVIPLE 17 — 60% ethanol extraction at 50°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 50°C with 60% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (II.OmLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 9.4% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 100ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 18 — 60% ethanol extraction at 60°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 60°C with 60% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL.

This extraction procedure resulted in 9.5% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 100ng/mL in the monocyte activation assay (Table 4). Removal of low molecular weight material ( EXAMPLE 19 — 60% ethanol extraction at 70°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 70""C with 60% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supematants from both extractions were combined (11.2mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 10.0% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 50ng/mL in the monocyte activation assay {Table 4).
EXAMPLE 20 — 60% ethanol extraction at 80°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 80°C with 60% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supematants from both extractions were combined (11.2mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20""C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 11.2% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 25ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 21 — 50% ethanol extraction at 23°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 23°C with 50% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supematants from

both extractions were combined (11.3mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanoi. Following incubation at -20""C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanoi. The isolated material was dried.under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 9.1% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 200ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 22 — 50% ethanoi extraction at 40°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at AO"C with 50% ethanoi, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (II.SmLs) following centrifugation. The ethanoi concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanoi. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanoi. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 8.9% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of lOOng/mL in the monocyte activation assay (Table 4).
EXAMPLE 23 — 50% ethanoi extraction at 50°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 50""C with 50% ethanoi, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.1mLs) following centrifugation. The ethanoi concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanoi. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanoi. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 9.4% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 75ng/mL in the monocyte activation assay (Table 4).

EXAMPLE 24 — 50% ethanol extraction at 60°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 60°C with 50% ethanol, first with T.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20""C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 10.8% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 25ng/mL in the monocyte activation assay (Table 4). Removal of low molecular weight material ( EXAMPLE 25 — 50% ethanol extraction at 70°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 70°C with 50% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 10.2% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 25ng/mL in the monocyte activation assay (Table 4). Removal of low molecular weight material ( EXAMPLE 26 — 50% ethanol extraction at 80°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 80° C with 50% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.2mLs) following centrifugation. The ethanol

concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20""C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 11.7% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 25ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 27 — 40% ethanol extraction at 23°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 23°C with 40% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supematants from both extractions were combined (11.3mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 11.4% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of >250ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 28 — 40% ethanol extraction at 40°C and direct 80% alcohol precipitation
One 9 of freeze-dried AFA was extracted at 40°C with 40% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supematants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 10.7% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of lOOng/mL in the monocyte activation assay (Table 4).

EXAMPLE 29 — 40% ethanol extraction at 50°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 50°C with 40% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11 .OmLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20""C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted In 10.3% recovery of pre-ultrafiltrate NP16847 preparation and an ECso value of lOOng/mL in the monocyte activation assay (Table 4).
EXAMPLE 30 — 40% ethanol extraction at 60°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 60°C with 40% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 10.8% recovery of pre-ultrafiltrate NP 16847 preparation and an EC50 value of 50ng/mL in the monocyte activation assay (Table 4). Removal of low molecular weight material ( EXAMPLE 31 — 40% ethanol extraction at 70°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 70°C with 40% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.4mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were

collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 11.1% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 50ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 32 — 40% ethanol extraction at 80°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at SO"C with 40% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.3mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20""C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 12.6% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 50ng/mL in the monocyte activation assay (Table 4). Removal of low molecular weight material ( EXAMPLE 33 —• 30% ethanol extraction at 23°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 23°C with 30% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.2mLs) following centrifugation. The ethanol concentration of the supernatant was. adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 13.7% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 200ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 34 — 30% ethanol extraction at 40°C and direct 80% alcohol precipitation

One g of freeze-dried AFA was extracted at 40°C with 30% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.3mLs) following centrifugations. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20""C for several hours, precipitates were collected by centrifugations and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 13.8% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of lOOng/mL in the monocyte activation assay (Table 4).
EXAMPLE 35 — 30% ethanol extraction at SO"C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 50°C with 30% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.lmLs) following centrifugatlon. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugatlon and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 10.9% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of lOOng/mL in the monocyte activation assay (Table 4).
EXAMPLE 36 — 30% ethanol extraction at 60°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at BO-C with 30% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.2mLs) following centrifugatlon. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugatlon and subsequently washed with cold 95% ethanol. The Isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 10.5% recovery of pre-ultrafiltrate NP16847

preparation and an EC50 value of lOOng/mL in the monocyte activation assay (Table 4).
EXAMPLE 37 — 30% etiiano! extraction at 70°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 70°C with 30% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11.1mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 11.0% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 75ng/mL in the monocyte activation assay (Table 4).
EXAMPLE 38 — 30% ethanol extraction at 80°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 80° C with 30% ethanol, first with 7.5mLs for 3 hours and then with 6.25mLs for 12 hours. Supernatants from both extractions were combined (11 .OmLs) following centrifugation. The ethanol concentration of the supematant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 11.9% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 75ng/mL in the.monocyte activation assay (Table 4).
Table 4 summarizes the influence of both temperature and the ethanol concentration used during the initial extraction on the end-points described above. The endpoints used to evaluate the effectiveness of each extraction condition were percent recovery of the pre-ultrafiftrate in addition to its EC50 value. The pre-ultrafiitrate material was selected for these analyses because of its potential use as either a dietary, supplement or pharmaceutical preparation.

Elimination of the ultrafiltration step would represent a substantial simplification of the isolation procedure.
The conditions used in Example 9 (70% ethanol/40°C) resulted in 5.7% recovery of pre-ultrafiltrate NP16847 with an EC50 value of 200ng/mL. Increasing extraction temperatures above 40°C coupled with the presence of 70% ethanol during the initial extraction improved recovery and specific activity of the NP16847 polysaccharide preparation. However, decreasing the extraction temperature from 40°C to 23°C with 70% ethanol, or any other concentration of ethanol, did not result in lower EC50 values. At this temperature {23°C), recoveries were enhanced at lower ethanol concentrations. Part of this increased recovery was probably due to a more efficient extraction of phycocyanin as evidenced by the enhanced blue color of the material. Extraction at higher temperatures using 70% ethanol slightly enhanced recovery and substantially increased specific activity (e.g. 70% ethanol/80°C). Extraction with 50% ethanol at any temperature above 40°C resulted in lower EC50 values as compared with other ethanol concentrations. At ethanol concentrations above and below 50% ethanol, specific activities generally decreased at each temperature condition. Ethanol concentrations above and below 50% had opposite effects on recovery: recoveries decreased with higher ethanol concentration but slightly increased with lower concentrations (at temperatures of 50°C and below). The lower recoveries coupled with decreased specific activity at ethanol concentrations higher than 50% suggest that less NP 16847 is being extracted under these conditions. For ethanol concentrations below 50%, the higher recoveries coupled with decreased specific activity suggest that more inactive material is extracted along with NP16847. At temperatures below 60°C with 30% and 40% ethanol, part of this inactive material is most likely due to more effective extraction of phycocyanin, again evidenced by the enhanced blue color of the precipitate.
The region of Table 4 from 60° C - 80° -C at 50% ethanol represented conditions for both optimal recovery and specific activity. The preferred temperature range is between 60°C and 70°C (Examples 24 and 25) because further analysis of both the pre- and post-ultrafiltrate material derived from the 80°C, 40% to 60% ethanol extraction conditions showed substantial amounts of water insoluble material. These optimal conditions yield post-ultrafiltrate

recoveries between 4.5% and 5.6% (7.5 to 9.3 times more than the eariier 70% ethanol/40°C condition from Example 1) and an EC50 value of about 20ng/mL (5 times less than the 70% ethanolMO"C condition).
EXAMPLE 39 — Shorter extraction times
The data in Table 4 were collected on material extracted twice, first for 3 hours and second for 12 hours, under each condition. To optimize for large scale extraction of NP16847, shorter extractions times of 1 hour each were tested and found to be equivalent in terms of both recovery and specific activity.
EXAMPLE 40 — Single hot water extraction at 95°C for 30 minutes
Prior art procedures for the isolation of immunostlmulatory polysaccharides from other types of microalgae (17, 27) typically involve a single hot water extraction at Gd^C for 30 minutes. To evaluate this method, 1g of freeze-dried AFA was extracted once with 20mLs of water at gS"C for 30 minutes. The water extract was adjusted to 80% ethanol and Incubated at -20°C for several hours. The precipitate collected represented a recovery of 12.1% but contained very little NP16847 since the EC50 of this material was about 500ng/mL. Ultrafiltration resulted in a recovery of 5.1% and no change in specific activity. Clearly these conditions are not suitable for extraction of NP16847 from AFA.
EXAMPLE 41 — Water extraction at 4°C followed by re-extraction with 50% ethanol/60°C
It is possible that contaminating polar material can be selectively removed by an initial water extraction without substantial loss of NP16847. A two stage extraction procedure was tested to evaluate this approach. The first stage involved an initial water extraction of AFA at 4°C followed by a second stage re-extraction of AFA at optimal conditions (50% ethanol/60°C). Although the specific activity of NP 16847 using this method was comparable to the optimal conditions alone, the recovery was about 70% less for both pre- and post-ultrafiltrate.

EXAMPLE 42 — Water extraction at 23°C followed bv re-extraction with 50% etlianol/60°C
The procedure used in Example 41 was slightly modified by increasing the extraction temperature from 4°C to 23°C. Thus, the first extraction involved an initial water extraction of AFA at 23°C followed by a second stage re-extraction of AFA at optimal conditions (50% ethanol/eO-C). The results were similar to those in Example 41 (i.e. the specific activity was comparable to optimal conditions, yet the recovery was about 70% less for both pre- and post-ultrafiltrate).
EXAMPLE 43 — Water extraction at 40°C followed bv re-extraction with 50% ethanol/60°C
The procedure used in Example 41 was slightly modified by increasing the extraction temperature from 4""C to 40°C. Thus, the first extraction involved an initial water extraction of AFA at 40°C followed by a second stage re-extraction of AFA at optimal conditions (50% ethanol/60°C). The results were similar to those in Example 41 (i.e. the specific activity was comparable to optimal conditions, yet > the recovery was about 70% less for both pre- and post-ultrafiltrate).
EXAMPLE 44 — Extraction with 70% ethanol/40°C followed bv re-extraction with 50% ethanol/eO"C
It is possible that contaminating non-polar material can be selectively removed by an initial ethanol extraction without substantial loss of NP16847. To evaluate this approach a two stage extraction procedure was tested. The first stage involved an initial extraction of AFA with 70% ethanol at 40°C followed by a second stage re-extraction of AFA at optimal conditions (50% ethanol/60°C). Although this procedure gave a slightly better EC50 value (lOng/mL) than did Examples 24 and 25 for the post-ultrafiltrate NP16847, the recovery was only 1.0%. The pre-ultrafillrate had a recovery of 2.2% with an EC50 value of 20ng/mL.
One property of purified NP16847 was that it appeared to adhere to polypropylene pipette tips. To avoid exaggerated EC50 yalues caused by carryover of the material during serial dilutions, pipette tips were changed between each dilution.
Chromatographic analysis of NP16847 before and after ultrafiltration is displayed in Figs. 5-11. NP16847 preparation isolated using the procedure

outlined in Example 1 generally eluted as a broad single peak (Fig. 1). However, using the modified procedures (Examples 4-9), post-ultrafiltrate NP16847 eluted as a broad region containing what appears to be three peal Carbohydrate composition of different NP16847 preparations was . evaluated using GC-mass spectrometry analysis of TMS-methyl glycosides (Table 5). NP16847 material from Example 1 (NP1) was re-analyzed and found to have an identical carbohydrate composition profile as previously detemnined. Since a different batch of AFA (purchased from another company) was used in Examples 4-44 a preparation of NP 16847 was isolated from this new material using the extraction procedure of Example 1 (NP2). Both this NP 16847 preparation and NP1 have a comparable glycosyl composition, indicating consistency between different batches of AFA. The NP2 preparation however, was five times less active than NP1 JTable 5) due to partial loss of active

polysaccharides into the n-butanol phase during the n-butanol/water partitioning. In general, similar carbohydrate compositions were also found in pre- and post-ultrafiltrate NP16847 preparations (NP3 - NP6) obtained using optimal extraction conditions (50% ethanol at 60°C and yCC). Pre-ultrafiltrate NP16847 was, however, consistently higher in glucose composition and lower in N-acetylated sugar units than post-ultrafiltrate preparations. Based on the consistency of carbohydrate composition between these different NP16847 preparations (NP1 -NP7), it is clear that the major glycosyl residues present in this material are mannose, rhamnose, arabinose and glucose. In order to identify the O-methylated sugars detected during the TMS-methyl glycoside procedure, glycosyl composition was also determined using alditol acetate analysis. Methylated sugar residues contained in these preparations include 2-methyl rhamnose, 3-methyl rhamnose, 4-methyl rhamnose, 2-methyl fucose, 3-methyl arabinose and 3-methyl mannose. Interestingly, these NP 16847 preparations contain 5.1 -12.5% methylated carbohydrate residues and a high percent of deoxyhexoses (e.g. rhamnose and fucose). Both these characteristics may explain the unusual extractability of NP16847 polysaccharide material using relatively high concentrations of aqueous ethanol.
Because the samples tested (NP1 - NP7) represent up to a 50-fold difference in EC50 values, one would expect to see some difference in carbohydrate composition among them. Since this is not the case, It is obvious that the purity or activity of NP16847 preparations cannot be determined using this parameter. Therefore, NP16847 preparations would more appropriately be characterized by biological activity, size and extractability in aqueous ethanol. It may be that a unique structural feature is responsible for NP16847"s ability to activate monocytes/macrophages rather than a specific carbohydrate composition. It is also possible that the carbohydrate composition of NP1 - NP7 . reflects polysaccharides extractable with aqueous ethanol solutions and immunostimulatory ones would be present as a structural class within this group. This interpretation is supported by the observation that material obtained with hot water extraction (NP8 and NP9) has a very different carbohydrate profile than NP16847 preparations isolated using aqueous ethanol extraction (NP1 - NP7). The predominant glycosyl residue from both pre- and post-ultrafiltrate material obtained from hot water extraction of AFA was glucose (Table 5). Another

distinguishing characteristic of NP8 and NP9 is the lower percent composition of rhamnose as compared wjth NP16847 material isolated using aqueous ethanol extraction.
EXAMPLE 45 — Extraction with 60% methanol at 65° C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 65° C with 60% methanol, first with 7.5mLs for 1 hour and then with 6.25mLs for 1 hour. Superpatants from both extractions were combined (11.5mLs) following centrifugation. The methanol concentration of the supematant was adjusted to 80% by the addition of cold 100% methanol. Following Incubation at -20° C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved In water at 10mg/mL. This extraction procedure resulted in 1.8% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of 75ng/mL in the monocyte activation assay.
EXAMPLE 46 — Extraction with 40% isopropanol at 65°C and direct 80% alcohol precipitation
One g of freeze-dried AFA was extracted at 65° C with 40% isopropanol, first with 7.5mLs for 1 hour and then with 6.25mLs for 1 hour. Supematants from both extractions were combined (11.5mLs) following centrifugation. The isopropanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% isopropanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at lOmg/mL. This extraction procedure resulted in 12.0% recovery of pre-ultrafiltrate NP 16847 preparation and an EC50 value of lOOng/mL in the monocyte activation assay.
EXAMPLE 47 — Extraction with 100% ethanol bv reflux and precipitation by cooling to -20°C
One g of freeze-dried AFA was extracted by reflux using 100% ethanol, first with S.OmLs for 1 hour and then with 6.50mLs for 1 hour. Supernatants from both extractions were combined (II.OmLs) following centrifugation. Combined supernatant was then stored at -20°C for several hours and precipitable material

removed by centrifugation. Precipitate was subsequently washed with washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL. This extraction procedure resulted in 0.68% recovery of pre-ultrafiltrate NP16847 preparation and an EC50 value of about 750ng/mL in the monocyte activation assay,
EXAMPLE 48 — Extraction of immunostimulatorv oolvsaccharide material using aqueous alcohol from other food-grade microalqae iChlorella and SplrulJna)
The process of obtaining NP16847 from AFA using an initial extraction with aqueous alcohol, under optimal conditions, results in a preparation that is 20 times more active than material obtained using a hot water extraction (EC50 values for monocyte activation of 25ng/mL verses 500ng/mL, respectively).
The same aqueous alcohol extraction procedure can also be applied to other food-grade microalgae to obtain preparations that are enriched for immunostimulatory polysaccharides. For example, previous patents (16,17,27) have reported that Chlorella species and Spirulina species contain immunostimulatory polysaccharides that are extracted using hot water. However, extraction with aqueous alcohol (instead of hot water) results in selective enrichment for polysaccharides that are immunostimulatory and thereby results in preparations from these organisms that exhibit superior biological activity as well as a higher percent recovery of active material (see experiments below).
The following food-grade microalgae were used in these experiments: Chlorella pyrenoidosa (Sun Chlorella, Lot. No. WS 1422) and Spirulina platensis (Nature"s Way, Lot. No. 912091). All polysaccharide preparations represent pre-ultrafiltrate material. For preparation of hot water extracts, 1g of freeze-dried microalgae was extracted once with 20mLs of water at 95°C for 30 minutes. Hot water extracts were adjusted to 80% ethanol and incubated at -20""C overnight. The precipitate collected from Cf)lorella represented a recovery of 13.2% and an EC50 value of 1,000ng/mL. The precipitate collected from Spirulina represented a recovery of 16.5% and an EC50 value of 10,000ngymL for monocyte/macrophage activation.
Aqueous ethanol extracts were prepared by systematically changing both temperature and solvent concentration (percent ethanol in water) used during the initial extraction. The endpoints of percent recovery and EC50 value for

macrophage activation were used to determine optimal conditions for preparation of immunostimuiatory polysaccharide material. Chlorella and Spirulina extracts were prepared using the following procedure. One g of freeze-dried microalgae was extracted at the appropriate temperature, first with 7.5mLs of aqueous ethanol solvent for 2 hours and then with 6.25mLs of aqueous ethanol solvent for 2 hours. Supernatants from both extractions were combined (11.3mLs) following centrifugation. The ethanol concentration of the supernatant was adjusted to 80% by the addition of cold 100% ethanol. Following incubation at -20°C for several hours, precipitates were collected by centrifugation and subsequently washed with cold 95% ethanol. The isolated material was dried under vacuum and dissolved in water at 10mg/mL.
The extraction conditions for both optimal recovery and specific activity of immunostimuiatory polysaccharide preparations from Chlorella and Spirulina were similar to the optimal conditions (BO"C - 70°C at 50% ethanol) for extraction of NP16847 from AFA. For Chlorella, optimal conditions for preparation of immunostimuiatory polysaccharide material involve an initial extraction with 50% ethanol at 70° C. This condition yields a pre-ultrafiltrate recovery of 6.5% with an ECso value of 25ng/mL. For Spirulina, optimal conditions for preparation of immunostimuiatory polysaccharide material involve an initial extraction with 40% -50% ethanol at temperatures between 50°C and 70° C. These conditions yield pre-ultrafiltrate recoveries of about 9.0% with EC50 values of 500ng/mL. By comparison, although hot water extracts result in recoveries of about 2 times more material, they are 20 to 40 times less active than the preparations obtained using optimal extraction conditions with aqueous ethanol.
In summary, a simple and effective isolation procedure for optimal recovery of NP16847 from AFA was developed. The optimal extraction method for the pre-ultrafiltrate NP16847 preparation is a direct alcohol precipitation (80% at -20""C) from two pooled extracts of 1 hour each using 50% ethanol at 60°C-70""C. This pre-ultrafiltrate NP16847 preparation represents 11% recovery of AFA dry weight. Using one additional step involving ultrafiltration to exclude all material below 100,000 daltons, a relatively pure preparation of NP16847 polysaccharides can be obtained with recoveries between 4.5% and 5.6%. Both pre- and post-ultrafiltrate preparations have approximately the same EC50 value (25ng/mL for pre-ultrafiltrate and 20na/mL for Dost-ultrafiltrate). In comparison

with the NP16847 material obtained in Example 1 (70% ethanol extraction at 40""C), this optimized post-ultrafiltrate preparation contains between 7.5 and 9.3 times more NP16847 with 5 times greater activity. This procedure is well suited for both a preparation of a dietary supplement (botanical) extract as well as a bulk pharmaceutical product.
The same process described for obtaining immunostimulatory polysaccharide compositions (NP16847) from AFA microalgae can be used to obtain preparations from other microalgae (which include Chlorella species and Spirulina species) that are enriched for immunostimulatory polysaccharides (for example that activate monocytes/macrophages). The unique carbohydrate composition of ail three microalgae polysaccharide preparations allows the use of a procedure that selectively enriches for those that are immunostimulatory. These polysaccharides are extracted very poorly using the traditional hot water extraction procedure. Hot water preparations are 20 to 40 times less active than those using the optimized procedure.
Pharmaceutical Formulations
The present invention further includes low cost bulk polysaccharide preparations. The microalgae from which these polysaccharide preparations are isolated can be grown in tanks similar to current commercial methods that cultivate these microalgae for human consumption. This means that there would not be a supply problem, which is often a major issue for drug development of compounds isolated from natural products. The instant polysaccharide preparations exist in high concentrations (between 6.5% and 11 % of microalgae dry weight) and can be isolated using the simple, fast and low-cost techniques of the present invention.
Since the present polysaccharide preparations are useful as agents for immunotherapy in the treatment of immunodeficiency disorders, cancer, wound healing and infectious diseases, the present invention includes pharmaceutical compositions containing the instant polysaccharide preparations optionally in combination with acceptable phamnaceuticai earners or recipients.
Pharmaceutical compositions suitable for use in the present invention include compositions wherein the active ingredients are contained in an effective amount to achieve its intended purpose. More specifically, a therapeutically

effective amount means an amount effective to prevent development of or to alleviate the existing symptoms of the subject being treated. Determination of ttie effective amounts is well within the capability of those skilled in the art, especially in light of the detailed disclosure provided herein.
The amount of composition administered will be dependent upon the condition being treated, the subject being treated, on the subject"s weight, the severity of"the affliction, the manner of administration and the judgment of the personalizing physician.
The pharmaceutical compositions of the present invention may be manufactured in a manner that Is itself known, e.g., by means of conventional mixing, dissolving, granulating, dragger-making, levitating, emulsifying, encapsulating, entrapping or lyophilizing processes.
Pharmaceutical compositions for use in accordance with the present invention thus may be fomnulated in conventional manner using one or more physiologically acceptable carriers comprising recipients and auxiliaries which facilitate processing of the compositions compounds into preparation which can be used pharmaceutically. Proper formulation is dependent upon the route of administration chosen.
For injection, the agents of the invention may be formulated in aqueous solutions, preferably in physiologically compatible buffers such as Hanks solution, Ringer"s solution, or physiological saline buffer. For Tran mucosal administration, penetrants appropriate to the barrier to be permeated are used in the formulation. Such penetrants are generally known in the art.
For oral administration, the compositions can be formulated readily by combining the active compositions with phannaceutically acceptable carriers well known in the art. Such carriers enable the compounds of the invention to be formulated as tablets, pills, drapes, capsules, liquids, gels, syrups, slurries, suspensions and the like, for oral ingestion by a patient to be treated. Pharmaceutical preparations for oral use can be obtained solid excipient, optionally grinding a resulting mixture, and processing the mixture of granules, after adding suitable auxiliaries, if desired, to obtain tablets or dragee cores. Suitable excipients are, in particular, fillers such as sugars, including lactose, sucrose, Manito, or sorbitol; cellulose preparations such as, for example, maize starch, wheat starch, rice starch, potato starch, gelatin, gum tragacanth, methyl

cellulose, hydroxypropylmethyl-cellulose, sodium carboxymethylcellulose, and/or polyvinylpyrrolidone (PVP).
If desired, disintegrating agents may be added, such as the cross-linked polyvinyl pyrrolidone, agar, or alginic acid or a salt thereof such as sodium alginate.
Dragee cores are provided with suitable coatings. For this purpose, concentrated sugar solutions may be used, which may optionally contain gum arable, talc, polyvinyl pyn-olidone, carbopol gel, polyethylene glycol, and/or titanium dioxide, lacquer solutions, and suitable organic solvents or solvent mixtures. Dyestuffs or pigments may be added to the tablets or dragger coatings for identification or to characterize different combinations of active compound doses.
Pharmaceutical preparations which can be used orally include push-fit capsules made of gelatin, as well as fit, sealed capsules made of gelatin and a plasticizer, such as glycerol or sorbitol. The push-fit capsules can contain the active ingredients in admixture with filler such as lactose, binders such as starches, and/or lubricants such as talc or magnesium stearate and, optionally, stabilizers. In soft capsules, the active compounds may be dissolved or suspended in suitable liquids, such as fatty oils, liquid paraffin, or liquid polyethylene glycols. In addition, stabilizers may be added. All formulations for oral administration should be in dosages suitable for such administration.
For buccal administration, the compositions may take the form of tablets or lozenges formulated in conventional manner.
For administration by inhalation, the compositions for use according to the
present invention are conveniently delivered in the form of an aerosol spray
presentation from pressurized packs or a nebulizer, with the use of a suitable
propellant, e.g., dichlorodifluoromethane, trichlorofluoromethane,
dichlorotetrafluoroethane, carbon dioxide or other suitable gas. In the case of a pressurized aerosol the dosage unit may be determined by providing a valve to deliver a metered amount. Capsules and cartridges of e.g., gelatin for use in an inhaler or insufflator may be formulated containing a power mix of the compound and a suitable powder base such as lactose or starch.
The compositions may be formulated for parenteral administration by injection, e.g., by bolus injection or continuous infusion. Formulations for

injection may be presented in unit dosage form, e.g., in ampoules or in multitude containers, with an added preservative. The compositions may take such forms as suspensions, solutions or emulsions in oily or aqueous vehicles, and may contain formulator agents such as suspending, stabilizing and/or dispersing agents.
Pharmaceutical formulations for parenteral administration include aqueous solutions of the active compounds in water-soluble form. Additionally, suspensions of the active composition may be prepared as appropriate oily injection suspensions. Suitable lipophilic solvents or vehicles include fatty oils such as sesame oil, or synthetic fatty acid esters, such as ethyl oleate or triglycerides, or liposome. Aqueous injection suspensions may contain substances which increase the viscosity of the suspension, such as sodium carboxymethyl cellulose, sorbitol, or dextran. Optionally, the suspension may also contain suitable stabilizers or agents which increase the solubility of the compounds to allow for the preparation of highly concentrated solutions.
Alternatively, the active ingredient may be in powder fomi for constitution with a suitable vehicle, e.g., sterile pyrogen-free water, before use.
The compositions may also be formulated in rectal compositions such as suppositories or retention enemas, e.g., containing conventional suppository bases such as cocoa butter or other glycerides.
In addition to the formulations described previously, the compositions may also be fomnulated as a depot preparation. Such long acting formulations may be administered by implantation (for example subcutaneously or intramuscularly) or by intramuscular injection. Thus, for example, the compositions may be formulated with suitable polymeric or hydrophobic materials (for example as an emulsion in an acceptable oil) or ion exchange resins, or as sparingly soluble derivatives, for example, as a sparingly soluble salt.
The pharmaceutical compositions also may comprise suitable solid or gel phase carriers or excipients. Examples of such carriers or excipients include but are not limited to calcium carbonate, calcium phosphate, various sugars, starches, cellulose derivatives, gelatin, and polymers such as polyethylene glycols.
Suitable routes of administration may, for example, include oral, rectal, Tran mucosal, transferal, or intestinal administration, parenteral delivery.

including intramuscular, subcutaneous, intramedullary injections, as well as intrathecal, direct intraventricular, intravenous, intraperitoneal, intranasal, or intraocular injections.
Alternatively, one may administer the composition in a local rather than systemic manner, for example, via injection of the compound directly into an affected area, often in a depot or sustained release formulation.
Furthermore, one may administer the drug in a targeted drug delivery system, for example, in a liposome coated with an antibody specific for affected cells. The liposomes will be targeted to and taken up selectively by the cells.
The compositions may, if desired, be presented in a pack or dispenser device which may contain one or more unit dosage forms containing the active ingredient. The pack may for example comprise metal or plastic foil, such as a blister pack. The pack or dispenser device may be accompanied by instructions for administration. Compositions comprising a composition of the invention formulated in a compatible pharmaceutical carrier may also be prepared, placed in an appropriate container, and labeled for treatment of an indicated condition. Suitable conditions indicated on the label may include treatment of a disease. Dietary Supplements
Dietary supplements suitable for use in the present invention include compositions wherein the active ingredients are contained in an effective amount to achieve its intended purpose. More specifically, an effective amount means an amount effective to prevent development of or to alleviate the existing symptoms of the subject being treated. Determination of the effective amounts is well within the capability of those skilled in the art, especially in light of the detailed disclosure provided herein. The amount of composition administered will be dependent upon the condition being treated, the subject being treated, on the subjects weight, the severity of the affliction, the manner of administration and the judgment of the personalizing physician.
The ingredients of the dietary supplement of this invention are contained in acceptable excipients and/or carriers for oral consumption. The actual form of the cam"er, and thus, the dietary supplement itself, may not be critical. The carrier may be a liquid, gel, gelcap, capsule, powder, solid tablet (coated or non-coated), tea or the like; Suitable excipient and/or carriers include maltodextrin, calcium carbonate, declaims phosphate, tricalcium phosphate, microcrystalline

cellulose, dextrose, rice flour, magnesium steerage, stair acid, croscarmellose sodium, sodium starch glycolate, crospovidone, sucrose, vegetable gums, agar, lactose, methylcellulose, poisoned, carboxymethylcellulose, corn starch, and the like (including mixtures thereof). The various ingredients and the excipient and/or carrier are mixed and formed into the desired form using conventional techniques. Dose levels/unit can be adjusted to provide the recommended levels of ingredients per day in a reasonable number of units.:
The dietary supplement may also contain optional ingredients including, for example, herbs, vitamins, minerals, enhancers, colorants, sweeteners, flavorings, inert ingredients, and the like. Such optional ingredients may be either naturally occurring or concentrated forms. Selection of one or several of these ingredients is a matter of formulation, design, consumer preference and end-user. The amounts of these ingredients added to the dietary supplements of this invention are readily known to the skilled artisan. Guidance to such amounts can be provided by the U.S." RDA doses for divider and adults.

References
All references or citations made or referred to In this Application are expressly incorporated into the specification by reference thereto.
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We claim
1. Immunostimulatory preparations isolated from microalgae comprising polysaccharides extractable by a solvent comprising water or a mixture of water and at least one lower aikyi alcohol where the alkyl portion is from I to 4 carbon atoms and where the active polysaccharides have apparent molecular weights above approximately 2 miiiion daitons.
2. The Immunostimulatory preparation of claim 1 whereln the immunostimulatory activity is manifested by monocyte/macrophage activation.
3. The immunostimulatory preparation of claim 1 wherein the microalgae are those of Aphanizomenan flos-aquae.
4. The immunostimulatory preparation of claim 2 wherein the microalgae are those of Aphanizomenon flos-aquae.
5. The tmrnunostimuiatory preparation of claim 1 wherein the microalgae are those of Chlorella pyroidosa.
6. The immunostimulatory preparation of daim 2 wherein the microalgae are those of Chlorella pyrenoidosa.
7. The immunostimulatory preparation of claim 1 wherein the microalgae are those of SpiruUna platensfs
8. The immunostimulatory preparation of claim 2 wherein the microalgae are those of Spirulina platensis.
9. The Immunostimulatory preparation of claim 3 or 4, wherein the glyoosyl components of the active polysaccharides are substantially comprised of mannose, glucose, rhamnose, galactose, fucose, methylated sugars and N-acetytated amino sugars.

10. The immunostlmulatory preparation of claim 5 or 6, wherein the glycosyl components of the active polysaccharides are substantially comprised of arabinose, galactose, rhamnose, glucose and methylated sugars.
11. The immunostlmulatory preparation of claim 7 or 8, wherein the 5 glycosyl componens of the active polysaccharides are substantially comprised of rhamnose, glucuronic acid, fucose, galactose and methylated sugars.
12. A pharmaceutical composition comprising the immunostimulatory preparations of any one of daims 1-11 and a phamiaceufically aoceptebJe carrier or exclplent.
13. A dietary supplement comprising the immunostlmulatory preparations of any one of claims 1-11 and an acceptable carrier or exdpient for dietary supplements.
14. A process to obtain a preparation from food-grade mlcroalgae enriched for immunostiTiulatory polysaccharides, comprising the steps of:

(a) produdng an extract by extracting the microalgae with a solvent comprising water or a mixture of water and at least one lower alkyl alcohol where the alkyl portion is from to 4 carbon atoms at an extraction temperature of between about 4 degrees C to 100 degrees C;
(b) optionally concentrating the extract to a small volume where a large volume makes a concentration step desirable;
(c) precipitating the polysaccharide preparation out of the extract by precipitation means;
(d) separating the precipitated polysaccharide preparation by separation means; and
(e) washing the precipitate of (d) with 95% alcohol.

15. The process of claim 14 wherein the alcohol used in the extraction is ethanol.
16. The process of dalm 14 wherein the alcohol used in the extraction is methanol,
17. The process of claim 14 wherein the alcohol used in the extraction Is isopropanol or propanol.

18. The process of anyone of claims 14-17 wherein the preferred alcohol concentraton in (a) is from 20-80%.
19. The process of any one of claims 14-17 wherein the preferred temperature of extraction is between 40 and 80 degrees C.
20. The process of any one of claims 14-17 wherein the microalgae are those of Aphanizomenon flos-aquae, Chlorella pyrenldosa or Spinilina platansis.
21. The process of any one of claims 14-17 wherein the concentration step (b). is canrled out (when needed) by evaporation of the solvent, preferably under reduced pressure.
22. The process of any one of claims 14-17 wherein the concentration step (b) is canied out (when needed) by freeze drying or by dialysis
23. The process of any one of claims 14-17 wherein the polysaccharide preparation is precipitated in step (c) by the addition of ethanol to a final concentration of about 80% ethanoi.
24. The process of any one of claims 14-17 wherein the polysaccharide preparation is precipitated in step (c) by cooling the extract.
25. The process of any one of claims 14-17 wherein the polysaccharide preparation is precipitated in step (c) by &\e addition of a salt.
26. The process of claim 25 wherein the salt is ammonium sulfate.
27. The process of any one of claims 14-17 wherein the precipitated polysaccharide preparation is separated in step (d) by filtration.
28. The process of any one of claims 14-17 wherein the precipitated polysaccharide preparatlo.- is separated in step (d) by centrifugation.
29. The process of any one of claims 14-17 wherein the predpitated polysaccharide preparation is washed in step (e) by 95% ethanol.

30. The process of any one of claims 14-17 further comprising purifying the precipitate by dissolving the precipitate in water and removing substantially all components of less than approximately 100,000 daltons molecular mass by ultrafiltration.
31. The process of any one of claims 14-17 further comprising purifying the precipitate by dissolving the precipitate in water and removing substantially alt components of less than approximately 2 miinon daltons molecular mass by size exclusion column chromatogiaphy.
32. The process of claim 18 wherein the microalgae are those of Aphanfzomenon flos-aquae, Chlorella pyrenoidosa or Spirulfna platensfs
33. The process of claim 18 wherein the preferred temperature of extraction is between 40 and 80 degrees C.
34. The process of claim 18 wherein the concentration step (b) Is carried out (when needed) by evaporation of the solvent, preferably under reduced pressure.
■i
36. The process of claim 18 wherein the concentration step (b) is carried out (when needed) by freeze drying or by dialysis.
36. The process of claim 18 wherein the polysaccharide preparation is precipitated in step (c) by the addition of ethanol to a final concentration of about 80% ethanol,
37. The process of claim 18 wherein the polysaccharide preparation is precipitated in step (c) by the addition of a salt.
38. The process of claim 37 wherein the salt Is ammonium sulfate.
39. The process of claim 18 wherein the polysaccharide preparation is precipitated in step (c) by cooling the extract.
40. The process of claim 18 wherein the predpltated polysaccharide preparation Is separated in step (d) by filtration or by centrifugation.
41. The process of claim 18 wherein the precipitated polysaccharide preparation is washed in step (e) by 95% ethanol.

42. The process of claim 18 further comprising puri^ng the precipitate by dissolving the preciplate In water and removing substantially all components of less than approximately 100,000 daltons molecular mass by ultrafittratton.
43. The process of claim 18 further comprising purlfying the precipitate by dissolving the precipitate in water and removing substantially all componente of less than approximately 2 million daltons molecular mass by size exclusion column chromatography.
44. The process of claim 19 wherein the microalgae are those of Aphanlzomenon flos-aquae, CNorella pyrenoldosa or Spirultna platensls.
45. The process of claim 19 wherein the concentration step (b) is carried out (when needed) by evaporation of the solvent, preferably under reduced pressure or by freeze drying,
46. The process of claim 19 wherein the concentration step (b) is canled out (when needed) by dialysis.
47. The process of claim 19 wherein the polysaccharide preparation is precipitated in step (c) by the addition of ethanol to a final concentration of about 80% ethanol.
ft
48. The process of claim 19 wherein the polysaccharide preparation is precipitated in step (c) by the addition of a salt.
49. The process of claim 48 wherein the salt is ammonium sulfate.
50. The process of claim 19 wherein the polysaccharide preparation is precipitated in step (c) by cooling the extract,
51. The process of claim 19 wherein the precipitated polysaccharide preparation is separated in step (d) by filtration or by centrifugation..
52. The process of claim 19 wherein the precipitated polysaccharide preparation is washed in step (e) by 95% ethanol.

53. The process of claim 19 further comprising purifying the precipitate by dissolving
the precipitate in water and removing substantially all components of less than
approxinriateiy 100,000 daltons molecular mass by ultrafiltration.
54. The process of claim 19 further comprising purifying the precipitate by dissolving
the predpltate in water and removing substantially all components of less than
approximately 2 million daltons molecular mass by size exclusion column
chromatography.
55. Immunostlmulatory preparations Isolated from microalgae substantially as herein
described with reference to the accompanying drawings.

Documents:

0181-chenp-2005 abstract-duplicate.pdf

0181-chenp-2005 abstract.pdf

0181-chenp-2005 claims-duplicate.pdf

0181-chenp-2005 claims.pdf

0181-chenp-2005 correspondences-others.pdf

0181-chenp-2005 correspondences-po.pdf

0181-chenp-2005 description (complete)-duplicate.pdf

0181-chenp-2005 description (complete).pdf

0181-chenp-2005 drawings-duplicate.pdf

0181-chenp-2005 drawings.pdf

0181-chenp-2005 form-1.pdf

0181-chenp-2005 form-18.pdf

0181-chenp-2005 form-26.pdf

0181-chenp-2005 form-3.pdf

0181-chenp-2005 form-5.pdf

0181-chenp-2005 others.pdf

0181-chenp-2005 pct.pdf

0181-chenp-2005 petition.pdf


Patent Number 214154
Indian Patent Application Number 181/CHENP/2003
PG Journal Number 13/2008
Publication Date 31-Mar-2008
Grant Date 05-Feb-2008
Date of Filing 29-Jan-2003
Name of Patentee THE UNIVERSITY OF MISSISSIPPI
Applicant Address National Center for Natural Products Research Thad Cochran Research Center University, MI 38677,
Inventors:
# Inventor's Name Inventor's Address
1 PASCO, David, Stanley The University of Mississippi University, MI 38677,
2 Elsohly, Mahmoud The University of Mississippi University, MI 38677,
3 PUGH, Nirmal The University of Mississippi University, MI 38677,
4 ROSS, Samir The University of Mississippi University, MI 38677,
PCT International Classification Number A61K 31/715
PCT International Application Number PCT/US2001/021770
PCT International Filing date 2001-07-10
PCT Conventions:
# PCT Application Number Date of Convention Priority Country
1 60/217,001 2000-07-10 France