WO2008122098A1 - Composition for promoting the maintenance and function of muscle-specific progenitor cells - Google Patents
Composition for promoting the maintenance and function of muscle-specific progenitor cells Download PDFInfo
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- WO2008122098A1 WO2008122098A1 PCT/CA2007/000545 CA2007000545W WO2008122098A1 WO 2008122098 A1 WO2008122098 A1 WO 2008122098A1 CA 2007000545 W CA2007000545 W CA 2007000545W WO 2008122098 A1 WO2008122098 A1 WO 2008122098A1
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- muscle
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- creatine
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- mammal
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- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K31/00—Medicinal preparations containing organic active ingredients
- A61K31/70—Carbohydrates; Sugars; Derivatives thereof
- A61K31/715—Polysaccharides, i.e. having more than five saccharide radicals attached to each other by glycosidic linkages; Derivatives thereof, e.g. ethers, esters
- A61K31/737—Sulfated polysaccharides, e.g. chondroitin sulfate, dermatan sulfate
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K36/00—Medicinal preparations of undetermined constitution containing material from algae, lichens, fungi or plants, or derivatives thereof, e.g. traditional herbal medicines
- A61K36/18—Magnoliophyta (angiosperms)
- A61K36/185—Magnoliopsida (dicotyledons)
- A61K36/70—Polygonaceae (Buckwheat family), e.g. spineflower or dock
- A61K36/704—Polygonum, e.g. knotweed
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P21/00—Drugs for disorders of the muscular or neuromuscular system
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23V—INDEXING SCHEME RELATING TO FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES AND LACTIC OR PROPIONIC ACID BACTERIA USED IN FOODSTUFFS OR FOOD PREPARATION
- A23V2002/00—Food compositions, function of food ingredients or processes for food or foodstuffs
Definitions
- the present invention is directed towards a composition and method for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and for inducing a substantially simultaneous replenishment of myogenic precursor cells in response to exercise.
- Body composition including muscle, is influenced both by genetic factors and environmental stimuli.
- Important environmental factors or stimuli which effect muscle metabolism include food intake and exercise (Rennie MJ. Body maintenance and repair: how food and exercise keep the musculoskeletal system in good shape. Exp Physiol. 2005 Jul;90(4):427-36).
- Gene and protein expression patterns change in response to stimuli. This results in muscle adaptations such as muscle atrophy (loss) or muscle hypertrophy (gain).
- the determination of muscle loss or gain is the net effect of both positive and negative factors governing muscle development.
- 'True' muscle hypertrophy can be defined as "as an increase in fiber diameter without an apparent increase in the number of muscle fibers, accompanied by enhanced protein synthesis and augmented contractile force" (Sartorelli V, Fulco
- Satellite cells are a small population of quiescent muscle precursor cells that occupy a "satellite" position immediately outside of muscle fibers (Mauro i A. Satellite cell of skeletal muscle fibers. J Biophys Biochem Cytol. 1961 Feb;9:493- 5). They are normally maintained in a quiescent state and become activated to fulfill roles of routine maintenance, repair and hypertrophy. Satellite cells are thought to be muscle-specific stem cells which are capable of producing large numbers of differentiated progeny as well as being capable of self-renewal (Collins CA, Partridge TA. Self-renewal of the adult skeletal muscle satellite cell. Cell Cycle. 2005 Oct;4(10): 1338-41).
- Satellite cells In order that satellite cells can fulfill their biological role, they • must become activated, proliferate, differentiate and fuse to existing muscle cells (Anderson JE. The satellite cell as a companion in skeletal muscle plasticity: currency, conveyance, clue, connector and colander. J Exp Biol. 2006 Jun;209(Pt 12):2276-92). In this way, multinucleate muscle fibers are maintained or increased in size in response to stimuli.
- Activation of satellite cells is essential for their proper function and is defined as "an entry into Gl from quiescence and mobilization" (Anderson JE, Wozniak AC. Satellite cell activation on fibers: modeling events in vivo—an invited review. Can J Physiol Pharmacol. 2004 May;82(5):300-10).
- One of the main factors which has been associated with the activation of satellite cells is nitric oxide (NO) (Anderson JE, Wozniak AC. Satellite cell activation on fibers: modeling events in vivo ⁇ an invited review. Can J Physiol Pharmacol. 2004 May;82(5):300-10).
- NO is a small, freely diffusible signaling molecule produced in muscle by neuronal NO- synthase.
- NO release is regulated by stretching in skeletal muscle and is thought to be responsible for early satellite cell activation in response to muscle injury in proximal and distal muscle fibers (Anderson JE. A role for nitric oxide in muscle repair: nitric oxide-mediated activation of muscle satellite cells. MoI Biol Cell. 2000 May;l l(5):1859-74).
- NO activity is largely controlled by regulating the enzymes responsible for synthesizing NO - Nitric Oxide Synthases (NOSs). All major nitric oxide synthase (NOS) isoforms and splice variants, including a muscle-specific splice variant, are expressed in the skeletal muscles of all mammals (Stamler JS, Meissner G. Physiology of nitric oxide in skeletal muscle. Physiol Rev. 2001 Jan;81(l):209-237). Furthermore, the inner lining, or endothelium, of blood vessels uses NO to signal the surrounding smooth muscle to relax. This has the effect of dilating the artery thereby increasing blood flow in the affected region.
- NO has also been shown to play an important role in myoblast and satellite cell fusion (Pisconti A, Brunelli S, Di Padova M, De Palma C, Deponti D, Baesso S, Sartorelli V, Cossu G, Clementi E. Follistatin induction by nitric oxide through cyclic GMP: a tightly regulated signaling pathway that controls myoblast fusion. J Cell Biol. 2006 Jan 16;172(2):233-44) thereby contributing to muscle maintenance and growth.
- Myoblast fusion is itself a complex process involving migration, recognition and adhesion, each involving several mechanisms and factors.
- stem cells are to function properly, their pools must be maintained. Therefore, a defining feature of stem cells is their ability of self-renewal in addition to being able to produce differentiated cells (Collins CA, Partridge TA. Self-renewal of the adult skeletal muscle satellite cell. Cell Cycle. 2005 Oct;4(10):1338-41). Research has shown that the pool of satellite cells is maintained not only by self- renewal but also by contributions from the hematopoietic, i.e. blood, system (Doyonnas R, LaBarge MA, Sacco A, Charlton C, Blau HM. Hematopoietic contribution to skeletal muscle regeneration by myelomonocytic precursors. Proc Natl Acad Sci U S A. 2004 Sep 14;101(37):13507-12).
- hematopoietic stem cells contribute to muscle maintenance, the cells must migrate to the area at which they are required for repair or maintenance. This directed migration of stem/progenitor cells is termed 'mobilization'.
- a main mechanism for the mobilization of stem cells is through the release of signaling molecules at the site of the stem cell requirement wherein the stem cells express the corresponding cell surface receptors (Papayannopoulou T. Current mechanistic scenarios in hematopoietic stem/progenitor cell mobilization. Blood. 2004 Mar l;103(5):1580-5).
- CXCR-4 receptor An important receptor-ligand system for the relationship between the hematopoietic and muscle systems is the CXCR-4 receptor and the secreted chemokine, SDF-I (Ratajczak MZ, Majka M, Kucia M, Drukala J, Pietrzkowski Z, Peiper S, Janowska-Wieczorek
- SDF-I Rosatajczak MZ, Majka M, Kucia M, Drukala J, Pietrzkowski Z, Peiper S, Janowska-Wieczorek
- the present invention comprises, in accordance with an embodiment thereof, the administration, to a mammal, of a composition comprising at least creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine and a source of fucoidan, to induce muscle hypertrophy via satellite cell fusion to muscle fibres and to provide substantially coincident support for the replenishment of myogenic precursor cells in response to exercise.
- a composition comprising at least creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine and a source of fucoidan, to induce muscle hypertrophy via satellite cell fusion to muscle fibres and to provide substantially coincident support for the replenishment of myogenic precursor cells in response to exercise.
- the present invention is directed towards inducing muscle hypertrophy via satellite cell fusion to muscle fibres and provide substantially coincident support for the replenishment of myogenic precursor cells in response to exercise.
- the composition and method of the present invention accomplishes said support by encouraging multiple distinct aspects of muscle-specific progenitor cell biology.
- the term "muscle-specific progenitor cell” refers to any undifferentiated cell that is, or will be, at any time, capable of differentiating into any cell type which contributes to mature, functional adult skeletal muscle. This, for the purposes of the present disclosure, includes satellite cells and any other multi-potent cells such as hematopoietic stem cells which have the potential to contribute to skeletal muscle hypertrophy and growth, development or maintenance. It is herein understood that, despite a lack of consensus regarding nomenclature, there exists a continuum of cell types that lie between a classical pluripotent 'embryonic stem cell' capable of giving rise to all cell types on one extreme and a terminally-differentiated cell on the other extreme.
- undifferentiated cell types having increasingly limited developmental potential progressing from an embryonic stem cell toward a terminally-differentiated cell exist between said extremes. Furthermore, it is herein understood that such undifferentiated cells with limited, yet still multiple, developmental possibilities are generally termed 'tissue- specific stem cells'. However, undifferentiated cells with only one developmental possibility are generally termed 'progenitor cells'.
- Ingredients of the present composition may also be fine-milled in order to improve the immediacy of absorption, and thus the rate of bioavailability upon consumption by an individual.
- the fine-milling techniques and the immediacy of absorption employed in the present invention are disclosed in U.S. Patent Application No. 11/709,526, entitled “Method For Increasing The Rate And Consistency Of Bioavailability Of Supplemental Dietary Ingredients” and U.S. Patent Application No. 11/709,525, entitled “Method for a Supplemental Dietary Composition Having a Multi-Phase Dissolution Profile,” both herein incorporated fully by reference.
- rate of bioavailability is increased via a narrowing of particle size range and a concomitant reduction in the average particle size, improving the immediacy of absorption of said supplemental dietary ingredient. Furthermore, the consistency of dissolution, and thus the absorption of orally administered supplemental dietary ingredients, is improved by the fine-milled process.
- fine-milled and/or fine-milling refers to the process of micronization.
- Micronization is a mechanical process that involves the application of force to a particle, thereby resulting in a reduction in the size of the particle.
- the force in the case of micronization may be applied in any manner such as, e.g., the collision of particles at high rates of speed, grinding, or by an air-jet micronizer.
- fine-milled particles are obtained by jet- milling with nitrogen and compressed air.
- particle size refers to the diameter of the particle.
- average particle size means that at least 50% of the particles in a sample will have the specified particle size.
- at least 80% of the particles in a sample will have the specified particle size, and more preferably, at least 90% of the particles in a given sample will have the specified particle size.
- the preferred particle size range for fine-milled particles is between 2 and 50 microns.
- Methods for particle size determination which may be employed are, for example, sieves, sedimentation, electrozone sensing (Coulter counter), microscopy, and/or Low Angle Laser Light Scattering.
- the preferred methods for the particle size determination of the present invention are the methods which are most commonly used in the pharmaceutical industry, such as laser diffraction, e.g., via light scattering Coulter Delsa 440SX.
- the fine-milling process may be employed in the processing of one or more of the ingredients of the present invention in the dosage forms of tablets, e.g., immediate-release film coated, modified-release and fast-dissolving; capsules, e.g., immediate-release and modified-release; liquid dispersions; powders; drink mixes, etc. Creatine
- Creatine use has been thoroughly studied and is well-established as a beneficial dietary supplement for replenishing energy stores in working muscle cells (Greenhaff PL, Bodin K, Soderlund K, Hultman E. Effect of oral creatine supplementation on skeletal muscle phosphocreatine resynthesis. Am J Physiol. 1994 May;266(5 Pt l):E725-30).
- the resultant increase in muscular energy stores from creatine supplementation in an individual, combined with physical exercise leads to increased strength, and a reduction in fatigue resulting from high-intensity exercise (Greenhaff PL, Casey A, Short AH, Harris R, Soderlund K, Hultman E.
- the supplemental composition comprises creatine or derivatives thereof.
- a serving of the supplemental composition comprises from about 1.00 g to about 10.00 g of creatine or derivatives thereof.
- the preferred dosage of a serving of the supplemental composition of the present invention comprises about 3.50 g of creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine.
- the creatine may be present in various embodiments of the present invention as creatine salts of malate, maleate, fumarate, tartrate, citrate, succinate, pyruvate, pyroglutamate, glutamate or any other pharmaceutically acceptable salt as known in the art.
- the creatine may be present in various embodiments of the present invention as creatine esters of phosphate, sulphate or any other pharmaceutically acceptable esters as known in the art.
- the present invention may further comprise creatine pyroglutamate as a pharmaceutically acceptable derivative of creatine.
- a serving of the supplemental composition may comprise from about 0.005 g to about 0.10 g of creatine pryoglutamate.
- the preferred dosage of a serving of the supplemental composition comprises about 0.01 g of creatine pyroglutamate.
- the present invention may further comprise at least a portion of the creatine or pharmaceutically acceptable salts or esters thereof in a fine-milled format.
- the supplemental composition comprises fine-milled creatine or pharmaceutically acceptable salts or esters of said creatine.
- a serving of the supplemental composition comprises from about 0.005 g to about 0.05 g of fine-milled creatine or pharmaceutically acceptable salts or esters of said creatine.
- the preferred dosage of a serving of the supplemental composition comprises about 0.02 g of fine-milled creatine or pharmaceutically acceptable salts or esters of said creatine.
- Fucoidans are naturally-occurring sulfated sugar polymers. They are constituents of edible seaweed and have been consumed by humans for centuries. The specific type of fucoidan differs dependent upon the source. Brown seaweed, in particular, is a source of branched-chain Fucoidans and several species have been used experimentally as a source of Fucoidans including Fucus vesiculosus, Undaria pinnatifida and Laminaria japonica. One of the main and earliest mechanisms elucidated for the activity of Fucoidans has been the binding with L- and P-selectin, members of a family of cell surface receptors involved in the inflammatory response.
- selectins mediate the binding and adhesion of cells expressing the selectins to other cells such as those on the endothelium upon cytokine activation (Bevilacqua MP, Nelson RM. Selectins. J Clin Invest. 1993 Feb;91(2):379-87).
- Fucoidan (Berteau O, Mulloy B. Sulfated fucans, fresh perspectives: structures, functions, and biological properties of sulfated fucans and an overview of enzymes active toward this class of polysaccharide. Glycobiology. 2003 Jun;13(6):29R-40R). Fucoidan has been shown to have immunomodulating effects by stimulating lymphocytes and macrophages (Choi EM, Kim AJ, Kim YO, Hwang JK. Immunomodulating activity of arabinogalactan and fucoidan in vitro. J Med Food. 2005 Winter;8(4):446-53).
- fucoidan can induce the mobilization of these stem cells to muscles (Sweeney EA, Priestley GV, Nakamoto B, Collins RG, Beaudet AL, Papayannopoulou T. Mobilization of stem/progenitor cells by sulfated polysaccharides does not require selectin presence. Proc Natl Acad Sci U S A. 2000 Jun 6;97(12):6544-9). This effect is most likely due to the observed effect of increasing SDF-I plasma levels (Sweeney EA, Lortat- Jacob H, Priestley GV, Nakamoto B, Papayannopoulou T.
- the supplemental composition comprises fucoidan.
- a serving of the supplemental composition comprises from about 0.01 g to about 0.1 g of fucoidan.
- the preferred dosage of a serving of the supplemental composition of the present invention comprises about 0.024 g of fucoidan.
- the supplemental composition comprises Laminaria japonica extract as a source of fucoidan.
- Sphinoglipids are important constituents of eukaryotic organisms.
- sphingolipids and their metabolic products are highly bioactive molecules which are involved in the regulation of many important biological functions including cell growth, differentiation and apoptosis (Vesper H, Schmelz EM, Nikolova- Karakashian MN, Dillehay DL, Lynch DV, Merrill AH Jr. Sphingolipids in food and the emerging importance of sphingolipids to nutrition. J Nutr. 1999 Jul;129(7):1239- 50). Sphingolipid metabolism and biological function can be modulated by dietary intake of sphingolipids. Supplying supplemental sphingolipids promotes the synthesis of sphingosine 1 -phosphate.
- Sphingosine 1 -phosphate is a bioactive sphingolipid metabolite that has been shown to regulate a number of important biological functions including satellite cell activation (Nagata Y, Partridge TA, Matsuda R, Zammit PS. Entry of muscle satellite cells into the cell cycle requires sphingolipid signaling. J Cell Biol.
- the supplemental composition comprises a source of sphingolipids.
- a serving of the supplemental composition of the present invention comprises from about 0.005 g to about 0.05 g of a source of sphingolipids.
- the preferred dosage of a serving of the supplemental composition of the present invention comprises about 0.014 g of a source of sphingolipids.
- Resveratrol is a polyphenol found in many plant sources, most notably in grape skins, grape juice and red wine. One of the most abundant sources is from the roots of Polygonum cuspidatum. In plants, the biological function of resveratrol is as an antibiotic to fight infection. However, as a component of the diet, either as a constituent of plant-based foods or as a nutritional supplement, resveratrol has been reported to confer many health benefits. The main beneficial function of polyphenols from plant sources is generally attributed to antioxidant activity. However, resveratrol has been shown to increase NO production by tissue-specific induction of NOSs (Das S, Alagappan VK, Bagchi D, Sharma HS, Maulik N, Das DK.
- the supplemental composition of the present invention comprises Polygonum cuspidatum as a source of resveratrol.
- a serving of the supplemental composition of the present invention comprises from about 0.001 g to about 0.01 g of Polygonum cuspidatum as a source of resveratrol.
- the preferred dosage of a serving of the supplemental composition of the present invention comprises about 0.004 g of Polygonum cuspidatum as a source of resveratrol.
- the composition of the present invention comprises at least creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine and a source of fucoidan.
- the composition of the present invention comprises creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine, a source of fucoidan and a source of sphingolipids.
- the composition of the present invention comprises creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine, a source of fucoidan, a source of sphinoglipids and a source of resveratrol.
- the compositions of the present invention may also comprise, in addition to the aforementioned constituents, any number of amino acids in sufficient quantities to be effective in inducing muscle hypertrophy, or salts or esters of said amino acids.
- proteins such as whey protein, casein protein, milk proteins, or soy protein, may further be included in the compositions of the present invention in quantities effective to induce muscle hypertrophy. Amino acids and proteins are well known in the art to aid in the generation and repair of muscle protein.
- composition of the present invention when used in conjunction with the method provided herein, induces muscle hypertrophy via satellite cells fusion to muscle fibres and induces the substantially simultaneous replenishment of myogenic precursor cell in response to exercise.
- a method for enhancing the effectiveness of the immune system in an individual comprises at least the step of administering to an individual a therapeutically effective and acceptable amount of the composition of the present invention.
- compositions of the present invention may be administered to a mammal via any therapeutically acceptable format.
- the compositions of the present invention may be administered to a mammal intravenously, intramuscularly, or interperitoneally as routes of administration distinct from the aforementioned oral method.
- routes of administration may also be combined with an oral administration of the composition of the present invention as an additional method of administration to a mammal.
- the nutritional supplement may be consumed in any form.
- the dosage form of the nutritional supplement may be provided as, e.g., a powder beverage mix, a liquid beverage, a ready-to-eat bar or drink product, a capsule, a liquid capsule, a tablet, a caplet, or as a dietary gel.
- the preferred dosage forms of the present invention are as a caplet or as a liquid capsule.
- the present composition may also be provided in various time-release formats, e.g. a slow-release format, a quick-release format, or a phase-release format, as are known in the art as well.
- the dosage form of the nutritional supplement may be provided in accordance with customary processing techniques for herbal and nutritional supplements in any of the forms mentioned above.
- the nutritional supplement set forth in the example embodiments herein may contain any appropriate number and type of excipients, as is well known in the art.
- the present nutritional composition or those similarly envisioned by one of skill in the art may be utilized in methods to support the biological function of muscle-specific progenitor cells required for skeletal muscle recovery and growth in response to exercise.
- the present compositions and method disclosed herein are provided to induce muscle hypertrophy via satellite cell fusion to muscle fibres and induce a substantially coincident replenishment of myogenic precursor cell in response to exercise.
- a nutritional supplement for inducing muscle hypertrophy via satellite cell fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided.
- the nutritional supplement is in the form of caplets.
- One serving of the nutritional supplement is 7 caplets and each serving comprises:
- a nutritional supplement for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided.
- the nutritional supplement is in the form of caplets.
- One serving of the nutritional supplement is 7 caplets and each serving comprises:
- Laminaria japonica extract (standardized to 85% fucoidan), and about 0.0145 g of soy/milk sphingolipids.
- Example 3 A nutritional supplement for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided.
- the nutritional supplement is in the form of caplets.
- One serving of the nutritional supplement is 7 caplets and each serving comprises: [0052] about 3.5 g of creatine monohydrate (fine-milled), about 0.024 g of
- Laminaria japonica extract (standardized to 85% fucoidan), about 0.0145 g of soy/milk sphingolipids, and about 0.004 g of Polygonum cuspidatum,.
- a nutritional supplement for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided.
- the nutritional supplement is in the form of caplets.
- One serving of the nutritional supplement is 7 caplets and each serving comprises:
Abstract
The biological function of skeletal muscle precursor cells in the repair and growth of skeletal muscle in response to exercise is promoted by providing a supplemental composition comprising at least creatine and fucoidin to reinforce biochemical pathways involved in the maintenance of skeletal muscle satellite cells and other myogenic precursors. The composition and method of the present invention induce muscle hypertrophy via satellite cells fusion to muscle fibres and induce a substantially simultaneous replenishment of myogenic precursor cells in response to exercise in a mammal.
Description
Composition for Promoting the Maintenance and Function of Muscle-Specific Progenitor Cells
Field of the Invention [001] The present invention is directed towards a composition and method for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and for inducing a substantially simultaneous replenishment of myogenic precursor cells in response to exercise.
Background of the Invention [002] Body composition, including muscle, is influenced both by genetic factors and environmental stimuli. Important environmental factors or stimuli which effect muscle metabolism include food intake and exercise (Rennie MJ. Body maintenance and repair: how food and exercise keep the musculoskeletal system in good shape. Exp Physiol. 2005 Jul;90(4):427-36). Gene and protein expression patterns change in response to stimuli. This results in muscle adaptations such as muscle atrophy (loss) or muscle hypertrophy (gain). The determination of muscle loss or gain is the net effect of both positive and negative factors governing muscle development.
[003] 'True' muscle hypertrophy can be defined as "as an increase in fiber diameter without an apparent increase in the number of muscle fibers, accompanied by enhanced protein synthesis and augmented contractile force" (Sartorelli V, Fulco
M. Molecular and cellular determinants of skeletal muscle atrophy and hypertrophy.
Sci STKE. 2004 JuI 27;2004(244):rel 1). However, postnatal muscle growth is known to involve both myofiber hypertrophy and increased numbers of myonuclei - the source of which are satellite cells (Olsen S, Aagaard P, Kadi F, Tufekovic G, Verney
J, Olesen JL, Suetta C, Kjaer M. Creatine supplementation augments the increase in satellite cell and myonuclei number in human skeletal muscle induced by strength training. J Physiol. 2006 Jun l;573(Pt 2):525-34). The growth in the size of muscles after birth is, in reality, a combination of an increase in the actual diameter of a given muscle fiber and an increase in the number of mononuclei.
[004] Satellite cells are a small population of quiescent muscle precursor cells that occupy a "satellite" position immediately outside of muscle fibers (Mauro i
A. Satellite cell of skeletal muscle fibers. J Biophys Biochem Cytol. 1961 Feb;9:493- 5). They are normally maintained in a quiescent state and become activated to fulfill roles of routine maintenance, repair and hypertrophy. Satellite cells are thought to be muscle-specific stem cells which are capable of producing large numbers of differentiated progeny as well as being capable of self-renewal (Collins CA, Partridge TA. Self-renewal of the adult skeletal muscle satellite cell. Cell Cycle. 2005 Oct;4(10): 1338-41). In order that satellite cells can fulfill their biological role, they • must become activated, proliferate, differentiate and fuse to existing muscle cells (Anderson JE. The satellite cell as a companion in skeletal muscle plasticity: currency, conveyance, clue, connector and colander. J Exp Biol. 2006 Jun;209(Pt 12):2276-92). In this way, multinucleate muscle fibers are maintained or increased in size in response to stimuli.
[005] Activation of satellite cells is essential for their proper function and is defined as "an entry into Gl from quiescence and mobilization" (Anderson JE, Wozniak AC. Satellite cell activation on fibers: modeling events in vivo—an invited review. Can J Physiol Pharmacol. 2004 May;82(5):300-10). One of the main factors which has been associated with the activation of satellite cells is nitric oxide (NO) (Anderson JE, Wozniak AC. Satellite cell activation on fibers: modeling events in vivo~an invited review. Can J Physiol Pharmacol. 2004 May;82(5):300-10). NO is a small, freely diffusible signaling molecule produced in muscle by neuronal NO- synthase. NO release is regulated by stretching in skeletal muscle and is thought to be responsible for early satellite cell activation in response to muscle injury in proximal and distal muscle fibers (Anderson JE. A role for nitric oxide in muscle repair: nitric oxide-mediated activation of muscle satellite cells. MoI Biol Cell. 2000 May;l l(5):1859-74).
[006] NO activity is largely controlled by regulating the enzymes responsible for synthesizing NO - Nitric Oxide Synthases (NOSs). All major nitric oxide synthase (NOS) isoforms and splice variants, including a muscle-specific splice variant, are expressed in the skeletal muscles of all mammals (Stamler JS, Meissner G. Physiology of nitric oxide in skeletal muscle. Physiol Rev. 2001 Jan;81(l):209-237). Furthermore, the inner lining, or endothelium, of blood vessels uses NO to signal the surrounding smooth muscle to relax. This has the effect of dilating the artery thereby increasing blood flow in the affected region.
[007] NO has also been shown to play an important role in myoblast and satellite cell fusion (Pisconti A, Brunelli S, Di Padova M, De Palma C, Deponti D, Baesso S, Sartorelli V, Cossu G, Clementi E. Follistatin induction by nitric oxide through cyclic GMP: a tightly regulated signaling pathway that controls myoblast fusion. J Cell Biol. 2006 Jan 16;172(2):233-44) thereby contributing to muscle maintenance and growth. Myoblast fusion is itself a complex process involving migration, recognition and adhesion, each involving several mechanisms and factors.
[008] If stem cells are to function properly, their pools must be maintained. Therefore, a defining feature of stem cells is their ability of self-renewal in addition to being able to produce differentiated cells (Collins CA, Partridge TA. Self-renewal of the adult skeletal muscle satellite cell. Cell Cycle. 2005 Oct;4(10):1338-41). Research has shown that the pool of satellite cells is maintained not only by self- renewal but also by contributions from the hematopoietic, i.e. blood, system (Doyonnas R, LaBarge MA, Sacco A, Charlton C, Blau HM. Hematopoietic contribution to skeletal muscle regeneration by myelomonocytic precursors. Proc Natl Acad Sci U S A. 2004 Sep 14;101(37):13507-12).
[009] In the case where hematopoietic stem cells contribute to muscle maintenance, the cells must migrate to the area at which they are required for repair or maintenance. This directed migration of stem/progenitor cells is termed 'mobilization'. A main mechanism for the mobilization of stem cells is through the release of signaling molecules at the site of the stem cell requirement wherein the stem cells express the corresponding cell surface receptors (Papayannopoulou T. Current mechanistic scenarios in hematopoietic stem/progenitor cell mobilization. Blood. 2004 Mar l;103(5):1580-5). An important receptor-ligand system for the relationship between the hematopoietic and muscle systems is the CXCR-4 receptor and the secreted chemokine, SDF-I (Ratajczak MZ, Majka M, Kucia M, Drukala J, Pietrzkowski Z, Peiper S, Janowska-Wieczorek A Expression of functional CXCR4 by muscle satellite cells and secretion of SDF-I by muscle-derived fibroblasts is associated with the presence of both muscle progenitors in bone marrow and hematopoietic stem/progenitor cells in muscles. Stem Cells. 2003;21(3):363-71).
[0010] The foregoing disclosure describes a composition and method for stimulating the aforementioned for purposes of muscle hypertrophy in a mammal.
Summary of the Invention
[0011] The present invention comprises, in accordance with an embodiment thereof, the administration, to a mammal, of a composition comprising at least creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine and a source of fucoidan, to induce muscle hypertrophy via satellite cell fusion to muscle fibres and to provide substantially coincident support for the replenishment of myogenic precursor cells in response to exercise.
Detailed Description of the Invention
[0012] In the following description, for the purposes of explanations, numerous specific details are set forth in order to provide a thorough understanding of the present invention. It will be apparent, however, to one of ordinary skill in the art that the present invention may be practiced without these specific details.
[0013] The present invention is directed towards inducing muscle hypertrophy via satellite cell fusion to muscle fibres and provide substantially coincident support for the replenishment of myogenic precursor cells in response to exercise. The composition and method of the present invention accomplishes said support by encouraging multiple distinct aspects of muscle-specific progenitor cell biology.
[0014] As used herein, the term "muscle-specific progenitor cell" refers to any undifferentiated cell that is, or will be, at any time, capable of differentiating into any cell type which contributes to mature, functional adult skeletal muscle. This, for the purposes of the present disclosure, includes satellite cells and any other multi-potent cells such as hematopoietic stem cells which have the potential to contribute to skeletal muscle hypertrophy and growth, development or maintenance. It is herein understood that, despite a lack of consensus regarding nomenclature, there exists a continuum of cell types that lie between a classical pluripotent 'embryonic stem cell' capable of giving rise to all cell types on one extreme and a terminally-differentiated cell on the other extreme. It is herein understood that a number of undifferentiated cell types having increasingly limited developmental potential progressing from an embryonic stem cell toward a terminally-differentiated cell exist between said extremes. Furthermore, it is herein understood that such undifferentiated cells with limited, yet still multiple, developmental possibilities are generally termed 'tissue-
specific stem cells'. However, undifferentiated cells with only one developmental possibility are generally termed 'progenitor cells'.
[0015] Ingredients of the present composition may also be fine-milled in order to improve the immediacy of absorption, and thus the rate of bioavailability upon consumption by an individual. The fine-milling techniques and the immediacy of absorption employed in the present invention are disclosed in U.S. Patent Application No. 11/709,526, entitled "Method For Increasing The Rate And Consistency Of Bioavailability Of Supplemental Dietary Ingredients" and U.S. Patent Application No. 11/709,525, entitled "Method for a Supplemental Dietary Composition Having a Multi-Phase Dissolution Profile," both herein incorporated fully by reference. Briefly, rate of bioavailability is increased via a narrowing of particle size range and a concomitant reduction in the average particle size, improving the immediacy of absorption of said supplemental dietary ingredient. Furthermore, the consistency of dissolution, and thus the absorption of orally administered supplemental dietary ingredients, is improved by the fine-milled process.
[0016] As used herein, the term "fine-milled" and/or "fine-milling" refers to the process of micronization. Micronization is a mechanical process that involves the application of force to a particle, thereby resulting in a reduction in the size of the particle. The force, in the case of micronization may be applied in any manner such as, e.g., the collision of particles at high rates of speed, grinding, or by an air-jet micronizer. In a preferred embodiment, fine-milled particles are obtained by jet- milling with nitrogen and compressed air.
[0017] As used herein, the term "particle size" refers to the diameter of the particle. The term "average particle size" means that at least 50% of the particles in a sample will have the specified particle size. Preferably, at least 80% of the particles in a sample will have the specified particle size, and more preferably, at least 90% of the particles in a given sample will have the specified particle size. For the purposes of the present invention, the preferred particle size range for fine-milled particles is between 2 and 50 microns. [0018] The size of a particle can be determined by any of the methods known within the art. Methods for particle size determination which may be employed are, for example, sieves, sedimentation, electrozone sensing (Coulter counter),
microscopy, and/or Low Angle Laser Light Scattering. The preferred methods for the particle size determination of the present invention are the methods which are most commonly used in the pharmaceutical industry, such as laser diffraction, e.g., via light scattering Coulter Delsa 440SX. [0019] The fine-milling process may be employed in the processing of one or more of the ingredients of the present invention in the dosage forms of tablets, e.g., immediate-release film coated, modified-release and fast-dissolving; capsules, e.g., immediate-release and modified-release; liquid dispersions; powders; drink mixes, etc. Creatine
[0020] Creatine use has been thoroughly studied and is well-established as a beneficial dietary supplement for replenishing energy stores in working muscle cells (Greenhaff PL, Bodin K, Soderlund K, Hultman E. Effect of oral creatine supplementation on skeletal muscle phosphocreatine resynthesis. Am J Physiol. 1994 May;266(5 Pt l):E725-30). The resultant increase in muscular energy stores from creatine supplementation in an individual, combined with physical exercise leads to increased strength, and a reduction in fatigue resulting from high-intensity exercise (Greenhaff PL, Casey A, Short AH, Harris R, Soderlund K, Hultman E. Influence of oral creatine supplementation of muscle torque during repeated bouts of maximal voluntary exercise in man. Clin Sci (Lond). 1993 May;84(5):565-71) as well as increasing muscle growth (Volek JS, Duncan ND, Mazzetti SA, Staron RS, Putukian M, Gomez AL, Pearson DR, Fink WJ, Kraemer WJ. Performance and muscle fiber adaptations to creatine supplementation and heavy resistance training. Med Sci Sports Exerc. 1999 Aug;31(8):l 147-56). [0021] More recently however, creatine supplementation has been shown to augment the increase in satellite cell numbers in response to exercise (Olsen S, Aagaard P, Kadi F, Tufekovic G, Verney J, Olesen JL, Suetta C, Kjaer M. Creatine supplementation augments the increase in satellite cell and myonuclei number in human skeletal muscle induced by strength training. J Physiol. 2006 Jun l;573(Pt 2):525-34). Furthermore, it was suggested by the results of Olsen et al., that the rate of fusion of satellite cells was also increased in response to creatine supplementation and exercise, adding to an observed increase in the size of muscle fibers.
[0022] In various embodiments of the present invention, which are set forth in greater detail in Examples 1 to 4 below, the supplemental composition comprises creatine or derivatives thereof. A serving of the supplemental composition comprises from about 1.00 g to about 10.00 g of creatine or derivatives thereof. The preferred dosage of a serving of the supplemental composition of the present invention comprises about 3.50 g of creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine.
[0023] For example, the creatine may be present in various embodiments of the present invention as creatine salts of malate, maleate, fumarate, tartrate, citrate, succinate, pyruvate, pyroglutamate, glutamate or any other pharmaceutically acceptable salt as known in the art.
[0024] Additionally or alternatively, the creatine may be present in various embodiments of the present invention as creatine esters of phosphate, sulphate or any other pharmaceutically acceptable esters as known in the art. [0025] The present invention, as set forth in greater detail in Example 4 below, may further comprise creatine pyroglutamate as a pharmaceutically acceptable derivative of creatine. A serving of the supplemental composition may comprise from about 0.005 g to about 0.10 g of creatine pryoglutamate. The preferred dosage of a serving of the supplemental composition comprises about 0.01 g of creatine pyroglutamate.
[0026] The present invention may further comprise at least a portion of the creatine or pharmaceutically acceptable salts or esters thereof in a fine-milled format. In various embodiments of the present invention, the supplemental composition comprises fine-milled creatine or pharmaceutically acceptable salts or esters of said creatine. A serving of the supplemental composition comprises from about 0.005 g to about 0.05 g of fine-milled creatine or pharmaceutically acceptable salts or esters of said creatine. The preferred dosage of a serving of the supplemental composition comprises about 0.02 g of fine-milled creatine or pharmaceutically acceptable salts or esters of said creatine. Fucoidan
[0027] Fucoidans are naturally-occurring sulfated sugar polymers. They are constituents of edible seaweed and have been consumed by humans for centuries.
The specific type of fucoidan differs dependent upon the source. Brown seaweed, in particular, is a source of branched-chain Fucoidans and several species have been used experimentally as a source of Fucoidans including Fucus vesiculosus, Undaria pinnatifida and Laminaria japonica. One of the main and earliest mechanisms elucidated for the activity of Fucoidans has been the binding with L- and P-selectin, members of a family of cell surface receptors involved in the inflammatory response. The selectins mediate the binding and adhesion of cells expressing the selectins to other cells such as those on the endothelium upon cytokine activation (Bevilacqua MP, Nelson RM. Selectins. J Clin Invest. 1993 Feb;91(2):379-87). [0028] A number of potential beneficial uses have been suggested for
Fucoidan (Berteau O, Mulloy B. Sulfated fucans, fresh perspectives: structures, functions, and biological properties of sulfated fucans and an overview of enzymes active toward this class of polysaccharide. Glycobiology. 2003 Jun;13(6):29R-40R). Fucoidan has been shown to have immunomodulating effects by stimulating lymphocytes and macrophages (Choi EM, Kim AJ, Kim YO, Hwang JK. Immunomodulating activity of arabinogalactan and fucoidan in vitro. J Med Food. 2005 Winter;8(4):446-53). As well, Herpes virus reactivation can be inhibited by treatment with Fucoidan (Cooper R, Dragar C, Elliot K, Fitton JH, Godwin J, Thompson K. GFS, a preparation of Tasmanian Undaria pinnatifida is associated with healing and inhibition of reactivation of Herpes. BMC Complement Altern Med. 2002 Nov 20;2:l 1). Importantly, orally administered Fucoidan in humans has been shown to increase the number of CXCR-4-expressing stem cells which can replenish the pool of satellite cells (Irhimeh MR et al. Fucoidan and CXCR4+ hemopoietic progenitor stem cell population, 2004, The Sydney Convention Centre North, Darling Harbour, Australian StemCell Centre). Furthermore, fucoidan can induce the mobilization of these stem cells to muscles (Sweeney EA, Priestley GV, Nakamoto B, Collins RG, Beaudet AL, Papayannopoulou T. Mobilization of stem/progenitor cells by sulfated polysaccharides does not require selectin presence. Proc Natl Acad Sci U S A. 2000 Jun 6;97(12):6544-9). This effect is most likely due to the observed effect of increasing SDF-I plasma levels (Sweeney EA, Lortat- Jacob H, Priestley GV, Nakamoto B, Papayannopoulou T. Sulfated polysaccharides increase plasma levels of SDF-I in monkeys and mice: involvement in mobilization of stem/progenitor cells. Blood. 2002 Jan 1;99(1):44-51).
[0029] In a preferred embodiment of the present invention, the supplemental composition comprises fucoidan. A serving of the supplemental composition comprises from about 0.01 g to about 0.1 g of fucoidan. The preferred dosage of a serving of the supplemental composition of the present invention comprises about 0.024 g of fucoidan.
[0030] In various embodiments of the present invention, which are set forth in greater detail in Examples 1 to 4 below, the supplemental composition comprises Laminaria japonica extract as a source of fucoidan.
Sphinoglipids [0031] Sphingolipids are important constituents of eukaryotic organisms.
Complex sphingolipids and their metabolic products are highly bioactive molecules which are involved in the regulation of many important biological functions including cell growth, differentiation and apoptosis (Vesper H, Schmelz EM, Nikolova- Karakashian MN, Dillehay DL, Lynch DV, Merrill AH Jr. Sphingolipids in food and the emerging importance of sphingolipids to nutrition. J Nutr. 1999 Jul;129(7):1239- 50). Sphingolipid metabolism and biological function can be modulated by dietary intake of sphingolipids. Supplying supplemental sphingolipids promotes the synthesis of sphingosine 1 -phosphate.
[0032] Sphingosine 1 -phosphate is a bioactive sphingolipid metabolite that has been shown to regulate a number of important biological functions including satellite cell activation (Nagata Y, Partridge TA, Matsuda R, Zammit PS. Entry of muscle satellite cells into the cell cycle requires sphingolipid signaling. J Cell Biol.
2006 JuI 17;174(2):245-53) and myogenic differentiation (Donati C, Meacci E, Nuti
F, Becciolini L, Farnararo M, Bruni P. Sphingosine 1 -phosphate regulates myogenic differentiation: a major role for S1P2 receptor. FASEB J. 2005 Mar;19(3):449-51), both of which are processes important for increasing muscle hypertrophy.
[0033] In embodiments of the present invention, which are set forth in greater detail in Examples 2 to 4 below, the supplemental composition comprises a source of sphingolipids. A serving of the supplemental composition of the present invention comprises from about 0.005 g to about 0.05 g of a source of sphingolipids. The preferred dosage of a serving of the supplemental composition of the present invention comprises about 0.014 g of a source of sphingolipids.
Resveratrol
[0034] Resveratrol is a polyphenol found in many plant sources, most notably in grape skins, grape juice and red wine. One of the most abundant sources is from the roots of Polygonum cuspidatum. In plants, the biological function of resveratrol is as an antibiotic to fight infection. However, as a component of the diet, either as a constituent of plant-based foods or as a nutritional supplement, resveratrol has been reported to confer many health benefits. The main beneficial function of polyphenols from plant sources is generally attributed to antioxidant activity. However, resveratrol has been shown to increase NO production by tissue-specific induction of NOSs (Das S, Alagappan VK, Bagchi D, Sharma HS, Maulik N, Das DK. Coordinated induction of iNOS-VEGF-KDR-eNOS after resveratrol consumption: a potential mechanism for resveratrol preconditioning of the heart. Vascul Pharmacol. 2005 Apr-May;42(5-6):281-9 Abstract).
[0035] In various embodiments of the present invention, which are set forth in greater detail in Examples 3 and 4 below, the supplemental composition of the present invention comprises Polygonum cuspidatum as a source of resveratrol. A serving of the supplemental composition of the present invention comprises from about 0.001 g to about 0.01 g of Polygonum cuspidatum as a source of resveratrol. The preferred dosage of a serving of the supplemental composition of the present invention comprises about 0.004 g of Polygonum cuspidatum as a source of resveratrol.
[0036] In a preferred embodiment of the present invention, the composition of the present invention comprises at least creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine and a source of fucoidan.
[0037] In another embodiment of the present invention, the composition of the present invention comprises creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine, a source of fucoidan and a source of sphingolipids.
[0038] In yet another embodiment of the present invention, the composition of the present invention comprises creatine or pharmaceutically acceptable derivatives of creatine such as salts and esters of creatine, a source of fucoidan, a source of sphinoglipids and a source of resveratrol.
[0039] The compositions of the present invention may also comprise, in addition to the aforementioned constituents, any number of amino acids in sufficient quantities to be effective in inducing muscle hypertrophy, or salts or esters of said amino acids. For example, proteins, such as whey protein, casein protein, milk proteins, or soy protein, may further be included in the compositions of the present invention in quantities effective to induce muscle hypertrophy. Amino acids and proteins are well known in the art to aid in the generation and repair of muscle protein.
[0040] Not wishing to be bound by theory, it is believed that the various components of the present invention will act via multiple, distinct biological pathways to aid in the maintenance and function of myogenic precursor cells in repair and growth of skeletal muscle. The composition of the present invention, when used in conjunction with the method provided herein, induces muscle hypertrophy via satellite cells fusion to muscle fibres and induces the substantially simultaneous replenishment of myogenic precursor cell in response to exercise.
[0041] Additionally, by way of ingestion of the composition of the present invention, a method for enhancing the effectiveness of the immune system in an individual is provided. The method of the present invention comprises at least the step of administering to an individual a therapeutically effective and acceptable amount of the composition of the present invention.
[0042] According to additional methods, the compositions of the present invention may be administered to a mammal via any therapeutically acceptable format. For example, the compositions of the present invention may be administered to a mammal intravenously, intramuscularly, or interperitoneally as routes of administration distinct from the aforementioned oral method. These instantly disclosed routes of administration may also be combined with an oral administration of the composition of the present invention as an additional method of administration to a mammal.
[0043] According to various embodiments of the present invention, the nutritional supplement may be consumed in any form. For instance, the dosage form of the nutritional supplement may be provided as, e.g., a powder beverage mix, a liquid beverage, a ready-to-eat bar or drink product, a capsule, a liquid capsule, a
tablet, a caplet, or as a dietary gel. The preferred dosage forms of the present invention are as a caplet or as a liquid capsule. The present composition may also be provided in various time-release formats, e.g. a slow-release format, a quick-release format, or a phase-release format, as are known in the art as well. [0044] Furthermore, the dosage form of the nutritional supplement may be provided in accordance with customary processing techniques for herbal and nutritional supplements in any of the forms mentioned above. Additionally, the nutritional supplement set forth in the example embodiments herein may contain any appropriate number and type of excipients, as is well known in the art. [0045] The present nutritional composition or those similarly envisioned by one of skill in the art, may be utilized in methods to support the biological function of muscle-specific progenitor cells required for skeletal muscle recovery and growth in response to exercise. Specifically, the present compositions and method disclosed herein are provided to induce muscle hypertrophy via satellite cell fusion to muscle fibres and induce a substantially coincident replenishment of myogenic precursor cell in response to exercise.
[0046] Although the following examples illustrates the practice of the present invention in several of its embodiments, the examples should not be construed as limiting the scope of the invention. Other embodiments will be apparent to one of skill in the art from consideration of the specifications and examples.
Examples Example 1
[0047] A nutritional supplement for inducing muscle hypertrophy via satellite cell fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided. The nutritional supplement is in the form of caplets. One serving of the nutritional supplement is 7 caplets and each serving comprises:
[0048] about 3.5 g of creatine monohydrate (fine-milled), and about 0.024 g of Laminaria japonica extract (standardized to 85% fucoidan). Example 2
[0049] A nutritional supplement for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided. The nutritional supplement is in the form of caplets. One serving of the nutritional supplement is 7 caplets and each serving comprises:
[0050] about 3.5 g of creatine monohydrate (fine-milled), about 0.024 g of
Laminaria japonica extract (standardized to 85% fucoidan), and about 0.0145 g of soy/milk sphingolipids.
Example 3 [0051] A nutritional supplement for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and inducing a substantially simultaneous replenishment of myogenic precursor cell in response to exercise is provided. The nutritional supplement is in the form of caplets. One serving of the nutritional supplement is 7 caplets and each serving comprises: [0052] about 3.5 g of creatine monohydrate (fine-milled), about 0.024 g of
Laminaria japonica extract (standardized to 85% fucoidan), about 0.0145 g of soy/milk sphingolipids, and about 0.004 g of Polygonum cuspidatum,.
Example 4
[0053] A nutritional supplement for inducing muscle hypertrophy via satellite cells fusion to muscle fibres and inducing a substantially simultaneous replenishment
of myogenic precursor cell in response to exercise is provided. The nutritional supplement is in the form of caplets. One serving of the nutritional supplement is 7 caplets and each serving comprises:
[0054] about 2.00 g of creatine monohydrate (fine-milled), about 0.02 g of creatine monohydrate (nanodiffuse), about 0.01 g of creatine pyroglutamate, about
1.30 g of creatine citrate, about 0.001 g of creatine malate, about 0.02 g of creatine pyruvate, about 0.024 g of Laminaria japonica extract (standardized to 85% fucoidan), about 0.0145 g of soy/milk sphingolipids, about 0.004 g of Polygonum cuspidatum, about 0.05 g of L-glycine ethyl ester, about 2.9 g of L-tyrosine, about 0.001 g of L-tyrosine methyl ester, and about 0.002 g of Yohimbe.
Extensions and Alternatives
[0055] In the foregoing specification, the invention has been described with specific embodiments thereof. However, it will be evident that various modifications and changes may be made thereto without departing from the broader spirit and scope of the invention.
Claims
1. A composition comprising creatine or derivatives thereof and a source of fucoidan in amounts effective to induce muscle hypertrophy and to induce a substantially simultaneous replenishment of myogenic precursor cells in a mammal.
2. The composition of claim 1, wherein muscle hypertrophy is induced via satellite cells fusion to muscle fibres in a mammal.
3. The composition of claim 1, further comprising a source of sphingo lipids.
4. The composition of claim 3, wherein the source of sphingolipids is provided in an amount effective to promote the synthesis of sphingosine 1 -phosphate in a mammal.
5. The composition of claim 3, further comprising a source of resveratrol.
6. The composition of claim 5, wherein the source of resveratrol is provided in an amount effective to increase the production of nitric oxide in a mammal.
7. A method comprising at least the step of administering to a mammal a composition comprising creatine or derivative thereof and a source of fucoidan wherein said composition induces muscle hypertrophy and substantially simultaneously induces a replenishment of myogenic precursor cells in said mammal in response to physical exercise.
8. The method of claim 7, wherein the composition further comprises a source of sphingolipids.
9. The method of claim 8, wherein the source of sphingolipids promote the synthesis of sphingosine 1 -phosphate in the mammal.
10. The method of claim 7, wherein the composition further comprises a source of resveratrol.
11. The method of claim 10, wherein the source of resveratrol increases the production of nitric oxide in the mammal.
Priority Applications (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CA002682589A CA2682589A1 (en) | 2007-04-04 | 2007-04-04 | Composition for promoting the maintenance and function of muscle-specific progenitor cells |
| EP07719475A EP2142195A4 (en) | 2007-04-04 | 2007-04-04 | Composition for promoting the maintenance and function of muscle-specific progenitor cells |
| PCT/CA2007/000545 WO2008122098A1 (en) | 2007-04-04 | 2007-04-04 | Composition for promoting the maintenance and function of muscle-specific progenitor cells |
| AU2007350793A AU2007350793A1 (en) | 2007-04-04 | 2007-04-04 | Composition for promoting the maintenance and function of muscle-specific progenitor cells |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
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| PCT/CA2007/000545 WO2008122098A1 (en) | 2007-04-04 | 2007-04-04 | Composition for promoting the maintenance and function of muscle-specific progenitor cells |
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| WO2008122098A1 true WO2008122098A1 (en) | 2008-10-16 |
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| PCT/CA2007/000545 WO2008122098A1 (en) | 2007-04-04 | 2007-04-04 | Composition for promoting the maintenance and function of muscle-specific progenitor cells |
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| Country | Link |
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| EP (1) | EP2142195A4 (en) |
| AU (1) | AU2007350793A1 (en) |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2010086746A3 (en) * | 2009-01-28 | 2010-09-30 | Life Science Nutrition As | Compositions and methods of treating viral infections |
Citations (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2005110448A2 (en) * | 2004-05-07 | 2005-11-24 | Thermo Formulations Ltd. | Nutritional composition for increasing creatine uptake in skeletal muscle |
| US20070020358A1 (en) * | 2005-03-18 | 2007-01-25 | Mower Thomas E | Sports drink concentrate |
-
2007
- 2007-04-04 CA CA002682589A patent/CA2682589A1/en not_active Abandoned
- 2007-04-04 WO PCT/CA2007/000545 patent/WO2008122098A1/en active Application Filing
- 2007-04-04 AU AU2007350793A patent/AU2007350793A1/en not_active Abandoned
- 2007-04-04 EP EP07719475A patent/EP2142195A4/en not_active Withdrawn
Patent Citations (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2005110448A2 (en) * | 2004-05-07 | 2005-11-24 | Thermo Formulations Ltd. | Nutritional composition for increasing creatine uptake in skeletal muscle |
| US20070020358A1 (en) * | 2005-03-18 | 2007-01-25 | Mower Thomas E | Sports drink concentrate |
Non-Patent Citations (8)
| Title |
|---|
| DAS S. ET AL.: "Coordinated induction of iNOS-VEGF-KDR-eNOS after resvatrol consumption: a potential mechanism for resvatrol preconditioning of the heart", VASCULAR PHARMACOLOGY, vol. 42, no. 5-6, 2005, pages 281 - 289, XP004910836 * |
| DONATI C. ET AL.: "Sphingosine 1-phosphate regulates myogenic differentiation: A major role for SIP2 receptor", THE FASEB JOURNAL, vol. 19, no. 3, 2005, pages 449 - 451, XP008119605 * |
| DOYONNAS ET AL.: "Hematopoietic contribution to skeletal muscle regeneration by myelomonocytic precursors", PROC. NATL. ACAD. SCI., vol. 101, no. 37, 2004, pages 13507 - 13512, XP008119557 * |
| LUYT ET AL.: "Low-molecular-weight fucoidan promotes therapeutic revasularization in a rat model of critical hindlimb ischemia", JOURNAL OF PHARMACOLOGY AND EXPERIMENTAL THERAPEUTICS, vol. 305, no. 1, 2003, pages 24 - 30, XP008039129 * |
| NAGATA Y. ET AL.: "Entry of muscle satellite cells into the cell cycle requires sphingolipid signaling", THE JOURNAL OF CELL BIOLOGY, vol. 174, no. 2, 2006, pages 245 - 253, XP008119604 * |
| See also references of EP2142195A4 * |
| SWEENEY ET AL.: "Mobilization of stem/progenitor cells by sulfated polysaccharides does not require selectin presence", PROC. NATL. ACAD. SCI., vol. 97, no. 12, 2000, pages 6544 - 6549, XP008119556 * |
| SWEENEY ET AL.: "Sulfated polysaccharides increase plasma levels of SDF-1 in monkeys and mice: involvement in mobilization of stem/progenitor cells", BLOOD, vol. 99, no. 1, 2002, pages 44 - 51, XP008119555 * |
Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2010086746A3 (en) * | 2009-01-28 | 2010-09-30 | Life Science Nutrition As | Compositions and methods of treating viral infections |
| US8697670B2 (en) | 2009-01-28 | 2014-04-15 | Life Science Nutrition As | Compositions and methods of treating viral infections |
| US9789142B2 (en) | 2009-01-28 | 2017-10-17 | Life Science Nutrition As | Method of increasing lean body mass |
Also Published As
| Publication number | Publication date |
|---|---|
| EP2142195A4 (en) | 2011-10-12 |
| CA2682589A1 (en) | 2008-10-16 |
| EP2142195A1 (en) | 2010-01-13 |
| AU2007350793A1 (en) | 2008-10-16 |
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