WO2012126824A1

WO2012126824A1 - Chondrogenic differentiation media and methods for inducing chondrogenic differentiation of cells

Info

Publication number: WO2012126824A1
Application number: PCT/EP2012/054654
Authority: WO
Inventors: Emilie REDERSTORFF; Corinne Sinquin; Jacqueline Ratiskol; Sylvia Colliec-Jouault; Jérome GUICHEUX; Pierre Weiss; Christophe MERCERON
Original assignee: Inserm (Institut National De La Sante Et De La Recherche Medicale); Institut Francais De Recherche Pour L'exploitation De La Mer (Ifremer); Universite De Nantes
Priority date: 2011-03-18
Filing date: 2012-03-16
Publication date: 2012-09-27
Also published as: ES2590752T3; AU2012230465A1; CA2828823C; CA2828823A1; US20130336937A1; EP2686435A1; EP2686435B1; JP2014509517A

Abstract

The invention provides chondrogenic differentiation media comprising chondrogenic growth factors and low-molecular-weight sulfated polysaccharide derivatives of marine native exopolysaccharides (EPS) excreted by mesophilic marine bacteria from deep-sea hydrothermal environments. The invention relates to methods for inducing chondrogenic differentiation in pluripotent or multipotent cells, to cartilage tissues obtained by such methods, and to the use of such cartilage tissues for therapeutic purposes.

Description

Chondrogenic Differentiation Media and

Methods for Inducing Chondrogenic Differentiation of Cells

Related Applications

The present application claims priority to European Patent Application No. EP 11 305 306.0 filed on March 18, 2011. The European patent application is incorporated herein by reference in its entirety.

Background of the Invention

Articular cartilage is a specialized tissue that surrounds the ends of long bones. It reduces friction and acts as shock-absorbing tissue during joint mobilization. Cartilage is composed of a single cell type, the chondrocyte, that is responsible for the synthesis of an abundant extracellular matrix essentially composed of type II, IX and XI collagens and proteoglycans. Chondrocytes play a major role in maintaining the integrity of cartilage through the control of anabolic and catabolic processes. Cartilage is however susceptible to damage originating from aging, trauma, and inflammatory or degenerative diseases. These impairments often result in extracellular matrix degradation and ultimately in the loss of joint function.

Many surgical approaches have been developed to improve the poor intrinsic self-repair capacity of cartilage. Unfortunately, these techniques have not proved satisfactory effectiveness. In this context, the regeneration of a functional cartilage through the transplantation of mesenchymal stem cells with bioactive synthetic matrices has been contemplated. Mesenchymal stem cells (MSC) have initially been identified in bone marrow and, since, in various other tissues such as for example adipose tissue, tendon, synovial membrane, muscle, periosteum. MSC exhibit a number of attractive features, particularly for regenerative medicine, including their self-renewal, their ability to proliferate in culture and their multipotency. In particular, bone-marrow-derived mesenchymal stem cells and adipose-derived stem cells (ASCs) show promise for use in cartilage repair. However, greater understanding is needed to develop a consistently reproducible approach to potently induce chondrogenic differentiation in these stem cell lines and to inhibit differentiated chondrocytes from further maturation into the hypertrophic lineage. Approaches to induce chondrogenic differentiation in these stem cell lines include appropriate chondrogenic differentiation media. Jennifer L. Puetzer et al. have reviewed the different chondrogenic differentiation media proposed to date by the scientific community (Tissue Engineering: Part B, Volume 16, Number 4, 2010). These authors conclude that none of these chondrogenic differentiation media is able to produce stable chondrocytes.

There is thus a need to provide new chondrogenic differentiation media having improved chondrogenic differentiation properties.

Summary of the Invention

The inventors have shown that the chondrogenic differentiation properties of chondrogenic differentiation media comprising growth factors known to induce chondrogenic differentiation can be dramatically increased by supplementing said media with particular low-molecular-weight sulfated polysaccharide derivatives of marine native exopolysaccharides (EPS).

The invention thus relates to chondrogenic differentiation media comprising: at least one chondrogenic growth factor selected from the group consisting of transforming growth factors β, bone morphogenetic proteins, and mixtures thereof, and a low-molecular-weight sulfated polysaccharide derivative of a marine native exopolysaccharide (EPS) excreted by a mesophilic marine bacterium from a deep-sea hydrothermal environment,

wherein said derivative is obtainable by a process comprising the following steps:

(a) a step consisting of free-radical depolymerization of said native EPS so as to obtain a depolymerized derivative having a molecular weight of 5,000 to 100,000 g/mol,

(b) a subsequent step consisting of sulfation of the depolymerized derivative, comprising adding to the depolymerized derivative at least one sulfation agent in an amount sufficient to obtain a sulfated polysaccharide derivative having a degree of sulfate-group substitution of between 10% and 45% by weight relative to the total weight of the sulfated polysaccharide derivative.

The invention also relates to kits comprising:

at least one chondrogenic growth factor selected from the group consisting of transforming growth factors β, bone morphogenetic proteins, and mixtures thereof, and a low-molecular-weight sulfated polysaccharide derivative according to the invention.

In addition, the invention provides a method for inducing chondrogenic differentiation in pluripotent or multipotent cells, wherein said method comprises the step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium according to the invention.

The invention also provides a method for obtaining a cartilage tissue wherein said method comprises the step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium according to the invention.

The invention further relates to cartilage tissues obtained using a method according to the invention, and to the use of these cartilage tissues as grafts in methods of treatment of the human or animal body.

Definitions

In the context of the present invention, the term "chondrogenic differentiation media" refers to liquid media capable of inducing chondrogenic differentiation in pluripotent or multipotent cells cultured in said media. A chondrogenic differentiation medium according to the invention typically contains, in addition to said chondrogenic growth factor(s) and said derivative(s), nutrients necessary to support the growth, proliferation, differentiation and survival of cells. Thus, appropriate chondrogenic differentiation media according to the invention typically comprise a minimal medium in which cells can grow, such as for example Dulbecco modified Eagle's minimal essential medium (DMEM), Ham's F-12 Medium, or mixtures thereof, supplemented with at least one of the followings: glucose, bovine serum albumine (BSA), BD™ ITS or ITS+ Universal Culture Supplements, insulin, transferrin, selenous acid, linoleic acid, hydrocortisone, inorganic phosphate, ascorbate-2-phosphate, ascorbate, sodium ascorbate, calcium chloride, thyroxine, proline, pyruvate, sodium pyruvate, pyridoxine hydrochloride, glutamax, non essential amino acids, L-glutamine, β-glycero phosphate, dexamethasone. Examples of appropriate media are disclosed by Jennifer L. Puetzer et al. in Tissue Engineering: Part B, Volume 16, Number 4, 2010.

The term "chondrogenic differentiation", as used herein, refers to the differentiation of pluripotent or multipotent cells into cells producing an extracellular matrix close to that of cartilage. The chondrogenic differentiation of pluripotent or multipotent cells is typically evaluated by the measurement of the pellet volume, cell morphology and matrix composition by hematoxylin-eosin-safran (HES) and alcian blue staining, as fully described by Merceron C. et al. in Am J Physiol Cell Pysiol, 2010, 298(2):p.355-64. HES staining allows to distinguish cell nuclei and cytoplasm in the cells constituting the pellets, thereby evidencing the presence or not of a structural organization of the cells within the pellet, a structural organization being indicative of a chondrogenic differentiation. HES staining further colors collagen fibers within the matrix, which is also indicative of chondrogenic differentiation. Alcian blue staining reveals the presence of sulfated glycosaminoglycan (GAG), which is another marker of chondrogenic differentiation. In addition, immunohistological detection of type II, IX and XI collagens as well as aggrecan could also be used as further markers of chondrogenic differentiation. The chondrogenic differentiation of pluripotent or multipotent cells is also evaluated by measuring the expression level in the cells of mRNA encoding for COL2A1 (collagen of type II), AC AN (aggrecan), SOX9 and COMP (cartilage oligomeric matrix protein), which are specific markers of chondrocytes.

The term "at least one chondrogenic growth factor", as used herein, refers to one, two, three, four or more chondrogenic growth factor(s).

The term "pluripotent cells", as used herein, refers to undifferentiated cells which can give rise to a variety of different cell lineages of the three germ layers (endoderm, mesoderm and ectoderm). Typically, pluripotent cells may express the following markers oct4, SOX2, Nanog, SSEA 3 and 4, TRA 1/81, see International Stem Cell Initiative recommendations (Nature Biotechnology 25, 803 - 816 (2007)).

The terms "multipotent cells" and "progenitor cells" are used herein interchangeably. They refer to undifferentiated cells which can give rise to a limited number of different cell lineages, including chondrocytes. Typical multipotent cells according to the invention are mesenchymal stem cells.

As used herein, the term "subject refers to a mammal, preferably a human being, that may or may not suffer from a disease associated with cartilage damage. In the context of the invention, the term "treating" or treatment' refers to a method that is aimed at delaying or preventing the onset of a disease, at reversing, alleviating, inhibiting, slowing down or stopping the progression, aggravation or deterioration of the symptoms of the disease, at bringing about ameliorations of the symptoms of the disease, and/or at curing the disease.

Detailed Description of Certained Preferred Embodiments

I - Chondrogenic differentiation media

The invention relates to chondrogenic differentiation media comprising:

at least one chondrogenic growth factor selected from the group consisting of transforming growth factors β, bone morphogenetic proteins, and mixtures thereof, and a low-molecular-weight sulfated polysaccharide derivative of a marine native exopolysaccharide (EPS) excreted by a mesophilic marine bacterium from a deep-sea hydrothermal environment,

1. Processes for obtaining low-molecular-weight sulfated polysaccharide derivatives of EPS

Processes for obtaining low-molecular-weight sulfated polysaccharide derivatives of marine native exopolysaccharides (EPS) according to the invention are fully described in the international application WO 2006/003290, and also by Colliec Jouault S. et al. in Biochim Biophys Acta 2001, 1528(2-3):p.141-151, and by Guezenec J. et al. in Carbohydrate Polymers 1998, 37(l):p.19-24.

In certain embodiments, the depolymerized derivatives obtained after step (a) are lyophilized. In other embodiments, step (b) of the process is followed by a dialysis step.

During the first depolymerization step, the native EPS can be used in a liquid form, i.e. as it is excreted by the bacteria into the culture medium. Preferably, the culture medium is centrifuged and only the supernatant containing the native EPS and that is free of bacterial debris is collected. The native EPS can be collected by any suitable technique known to those skilled in the art, such as for example membrane ultrafiltration, and can then optionally be lyophilized as is or in the form of an addition salt.

The step consisting of free-radical depolymerization of the native EPS is preferably carried out by addition of a solution of an oxidizing agent to a reaction mixture comprising the native EPS, preferably in the presence of a metal catalyst. The oxidizing agent is preferably chosen from peroxides, in particular hydrogen peroxide, and peracids, in particular peracetic acid and 3-chloroperbenzoic acid. The addition is preferably carried out continuously and with stirring for a period of between 30 minutes and 10 hours. Reaction mixture is preferably maintained at a pH of between 6 and 8, for example by addition of a basifying agent such as sodium hydroxide, and at a temperature of between approximately 30 and 70°C throughout the duration of the free-radical depolymerization reaction.

According to a specific embodiment of the present invention, in this step, the native EPS is present in the reaction mixture at a concentration of between approximately 2 and 10 mg/ml of reaction mixture.

In preferred embodiments, the oxidizing agent is a solution of hydrogen peroxide (H₂O₂) preferably having a concentration of between approximately 0.1% and 0.5% by weight, preferably of the order of 0.1% to 0.2% by weight, and is added at a flow rate of Vl/1000 to V 1/10 ml/minute, preferably Vl/50 and Vl/500 ml/minute, and more preferably of the order of Vl/100 ml/minute, VI being the volume of the reaction medium containing a marine exopolysaccharide (EPS) to which a solution of hydrogen peroxide is added.

The metal catalysts that can be used during the depolymerization step are preferably chosen from Cu⁺⁺, Fe⁺⁺ and Cr⁺⁺⁺ ions and the Cr₂0₇ ^2" anion, as described in particular in patent application EP 0 221 977. According to a specific embodiment, the metal catalyst is present in the reaction mixture at a concentration of between approximately 10^"3 M and 10^"1 M, and preferably at a concentration of between approximately 0.001 and 0.05 M.

The free-radical depolymerization process in accordance with the invention and as described above makes it possible to obtain, in a single step and with a good yield, homogeneous, low-molecular-weight polysaccharide derivatives. In the context of the present invention, the term "homogeneous derivatives" is intended to mean derivatives which, when assessed using high performance size exclusion chromatography, exhibit a single main peak representing a predominant population of polysaccharide chains that are homogeneous with respect to size, characterized by a polydispersity index I (Mw/Mn) < 5, where Mw = weight-average molecular weight and Mn = number- average molecular weight.

In certain embodiments, when the depolymerization reaction is over, the polysaccharide derivatives obtained are reduced using a reducing agent, so as to stabilize the chains, the reducing ends of which are very reactive, and in particular to avoid chain hydrolysis by the "peeling" reaction. The nature of the reducing agents that can be used to this effect is not essential. The reducing may be, in particular, sodium borohydride.

The metal catalyst used in the depolymerization step can be eliminated at the end of the depolymerization reaction, (or at the end of the reduction reaction if a reduction step is carried out) using any suitable method, for example by ion exchange chromatography, preferably a weak cation exchange resin passivated beforehand, or by treatment with EDTA (ethylenediaminetetraacetic acid).

In certain embodiments, prior to the sulfation step, a step consisting of N- deacetylation of the polysaccharide derivatives comprising N-acetylated hexosamines which are obtained at the end of the free-radical depolymerization step and/or at the end of the reduction step is carried out. This N-deacetylation step is carried out according to a protocol adapted from Zou et al. (Carbohyd. Res., 1998, 309: 297-301). Advantageously, the N-deacetylation step is carried out by addition, to the reaction mixture comprising the polysaccharide derivatives, of a solution of sodium borohydride, under stirring conditions. When the temperature of the reaction mixture reaches approximately 80°C, a basifying agent, preferably sodium hydroxide, is added to the reaction medium. After reaction for one hour, the reaction medium is neutralized by continuous addition of acetic acid until a pH of 5 is obtained. The polysaccharide derivatives obtained can be recovered by membrane ultrafiltration and then can optionally be lyophilized.

The polysaccharide derivatives resulting from the depolymerization and/or from the reduction and/or from the N-deacetylation can, if necessary, be recovered by any suitable technique well known to those skilled in the art, such as, for example, by membrane ultrafiltration or dialysis. Then, they are lyophilized and fractionated by size exclusion chromatography to increase their purity required to improve the subsequent sulfation step. Finally, the purified polysaccharide derivatives are conditioned in salt form by addition of a weak or strong base, that may be chosen, for example, from pyridine, triethylamine, tributylamine, tetrabutylammonium hydroxide and sodium hydroxide. This lyophilized salt may be prepared, for example, by elution of an aqueous solution of the polysaccharide derivatives at a concentration of between 1 and 8 mg/ml on an ion exchange resin column such as, for example, those sold under the name Dowex^® by the company Dow Chemical. The eluate is collected as long as the pH remains acid, for example less than 5, then the pH is subsequently adjusted to approximately 6.5 with the desired base as defined above. The polysaccharide derivatives in the form of a salt are then ultrafiltered and lyophilized.

The lyophilized polysaccharide derivatives, possibly in the form of an addition salt, are preferably dissolved in an anhydrous solvent at the beginning of the sulfation step; this solvent is preferably chosen from dimethylformamide (DMF), dimethyl sulfoxide (DMSO) formamide, and mixtures thereof. The amount of polysaccharide derivatives present in the anhydrous solvent may be between approximately 1 and 10 mg/ml, preferably between approximately 1 and 5 mg/ml, and even more preferably this amount is approximately 2.5 mg/ml. The dissolution of the EPS in the anhydrous solvent is preferably carried out, with stirring, at ambient temperature for approximately 1 to 2 hours and then at a temperature of between 40 and 50°C, preferably at a temperature of approximately 45°C for approximately 2 hours under argon or azote with molecular sieve. The one or more chemical sulfation agents used during the sulfation step can be added to the depolymerized and/or reduced and/or N-deacetylated EPSs that are in lyophilized form or in the form of a solution.

The sulfation agents are preferably chosen from complexes of pyridine sulfate (free or coupled to a polymer), of dimethylformamide sulfate, triethylamine sulfate and of trimethylamine sulfate. The one or more chemical sulfation agents are added to the solution of polysaccharide derivatives in a weight amount preferably representing from approximately 4 to 6 times, and even more preferably approximately 5 times, the mass of polysaccharide derivatives in solution. The chemical sulfation reaction is then preferably carried out with stirring for a period of between approximately 2 and 24 hours depending on the desired degree of sulfation. When the desired degree of sulfation is reached, the sulfation reaction is stopped after cooling of the reaction medium:

either by precipitation in the presence of sodium-chloride- saturated acetone or of methanol, and then dissolution of the precipitate in water;

or, preferably, by addition of water in a proportion preferably equal to 1/10 of the reaction volume and adjustment of the pH of the reaction medium to 9 with a basifying agent such as, for example, sodium hydroxide (3 M).

According to certain embodiments, the solution of sulfated polysaccharide derivatives is preferably dialyzed in order to remove the various salts, and then lyophilized. The final product, typically with an accurate molecular weight and a low polydispersity index of less than 2, is obtained by fractionation performed by size exclusion chromatography.

The low-molecular-weight sulfated polysaccharide derivatives in accordance with the invention have a molecular weight of 5,000 to 100,000 g/mol, 5,000 to 60,000 g/mol, 5,000 to 50,000 g/mol, 5,000 to 40,000 g/mol, preferably of 5,000 to 30,000 g/mol, more preferably of 10,000 to 25,000 g/mol.

The low-molecular-weight sulfated polysaccharide derivatives in accordance with the invention have a polydispersity index of less than 5, preferably of 1.5 to 4, more preferably of less than 2. The polydispersity index (PDI) according to the invention is a measure of the distribution of molecular mass of the derivatives. The PDI calculated is the weight average molecular weight divided by the number average molecular weight. PDI is typically measured by size-exclusion chromatography.

The sulfated polysaccharide derivatives according to the invention have a degree of sulfate-group substitution of between 10% and 45% by weight relative to the total weight of the sulfated polysaccharide derivative. In certain embodiments, the degree of sulfate-group substitution is of between 10% and 40%, of between 20% and 45% or of between 20% and 40%.

In certain embodiments, the sulfated polysaccharide derivatives according to the invention have a molecular weight of 5,000 to 50,000 g/mol, a polydispersity index of less than 5, particularly of 1.5 to 4, more particularly of less than 2, and a degree of sulfate-group substitution of between 20% and 40% by weight relative to the total weight of the sulfated polysaccharide derivative.

2. Mesophilic marine bacteria

In certain embodiments, the derivatives according to the invention are derived from marine native exopolysaccharides (EPS) excreted by a mesophilic marine bacterium selected from the group consisting of bacteria of the Alteromonas genus, Pseudoalteromonas genus and Vibrio genus. In a particular embodiment, the bacterium of t e Alteromonas genus is selected from the group consisting of the strains GY785, HYD 657, HYD 708, HYD 721, HYD 1545, HYD 1644, ST 716 and MS 907. In another particular embodiment, the mesophilic marine bacterium is the strain HE 800 of the Vibrio genus.

In certain preferred embodiments, the derivative according to the invention is derived from the strain GY785 of the Alteromonas genus {Alteromonas infernus). Such a derivative is called "GY 785 DRS" (see figure 1 for molecular structure). 3. Chemical characteristics of the native EPSs and derivatives

In certain embodiments, the low-molecular-weight sulfated polysaccharide derivatives obtained from native EPSs excreted by bacteria of the Alteromonas genus.

The native EPSs typically have a neutral monosaccharide content of from 20% to 70%, preferably from 30% to 60%, and more preferably from 38% to 57% by weight. In addition, the native EPSs typically have an acidic monosaccharide content of from 5% to 60%), preferably of between 6% and 50%, and more preferably of between 8% and 42% by weight. The native EPSs also typically have an amino sugar content of from 0%> to 1%) by weight in their oside composition.

In a particular embodiment, the native EPSs excreted by bacteria of the Alteromonas genus have an oside composition comprising:

- from 20% to 70%, preferably from 30% to 60%, and more preferably from 38% to 57%) by weight of neutral monosaccharides,

from 5% to 60%, preferably from 6% to 50%, and more preferably from 8% to 42%) by weight of acidic monosaccharides,

from 0%> to 1%) by weight of amino sugars.

According to another embodiment, the low- molecular- weight sulfated polysaccharide derivatives of the invention are obtained from native EPSs excreted by bacteria of the Vibrio genus, preferably by the bacterial strain HE 800. The native EPSs excreted by bacteria of the Vibrio genus are not sulfated. The native EPSs typically have a neutral monosaccharide content of from 0% to 5%, preferably from 0%> to 1%) by weight. The native EPSs also typically have an acidic monosaccharide content of from 20% to 50%, preferably from 25% to 40%, and more preferably from 30%) to 32%) by weight. The native EPSs still typically have an amino sugar content of from 20% to 50%, preferably from 25% to 40%, and more preferably from 30% to 35%) by weight. Lastly, the native EPSs typically have an N-acetylated group content of from 0% to 15%, preferably from 4% to 8%, and more preferably from 5% to 6% by weight.

In a particular embodiment, the native EPSs excreted by bacteria of the Vibrio genus have an oside composition comprising:

from 0%> to 5%), preferably from 0% to 1%> by weight of neutral monosaccharides, - from 20% to 50%, preferably from 25% to 40%, and more preferably from 30% to 32%) by weight of acidic monosaccharides,

from 20% to 50%, preferably from 25% to 40%, and more preferably from 30% to 35%) by weight of amino sugars,

from 0%> to 15%), preferably from 4% to 8%, and more preferably from 5% to 6% by weight of N-acetylated groups. Still typically, the native EPSs excreted by a mesophilic marine bacterium according to the invention have a protein content of from 0% to 15%, preferably from 0% to 5%), and more preferably from 0% to 1% by weight.

4. Amount of derivatives in the chondrogenic differentiation media

In certain embodiments, chondrogenic differentiation media according to the invention comprise 5μg/mL to 20C^g/mL, particularly 25μg/mL to 10C^g/mL, more particularly 25μg/mL to 75μg/mL, most particularly about 5C^g/mL of said derivative.

5. Chondrogenic growth factors

The chondrogenic growth factors are fully described in the prior art and well known by the skilled person. The review of Jennifer L. Puetzer (Tissue Engineering: Part B, Volume 16, Number 4, 2010) for instance discloses different chondrogenic growth factors, used alone or in combination to induce chondrogenic differentiation of pluripotent or multipotent cells.

Major chondrogenic growth factors families are transforming growth factors β and bone morphogenetic proteins. The transforming growth factors β are typically selected from TGF-βΙ, TGF-P2 and TGF-P3. The bone morphogenetic proteins are typically selected from BMP-2, BMP-4, BMP-6, BMP-7 and BMP-9.

Other chondrogenic growth factors include fibroblast growth factors, in particular FGF-2, and insulin-like growth factors, in particular IGF-1.

Examples of particular chondrogenic growth factor or mixtures of chondrogenic growth factors that may be included in chondrogenic differentiation media according to the invention are: TGF-βΙ; TGF- 2; TGF-p3; TGF-βΙ + TGF- 2 + TGF-p3; TGF- βΐ + FGF-2; TGF-βΙ + IGF-1; TGF-βΙ + BMP-2; TGF-βΙ + BMP-6; TGF- 2 + IGF- 1; TGF- 3 + FGF-2; BMP-2; BMP-4; BMP-6; BMP-7; BMP-9; BMP-2 + BMP-9; TGF- 3 + BMP-6; TGF- 3 + BMP-2; TGF- 3 + BMP-6 + IGF-1; TGF-βΙ + TGF- 3 + BMP-6 + IGF-1; BMP-2 + BMP-7; TGF- 3 + BMP-2 + BMP-4 + BMP-6 + BMP-7 + IGF-1; TGF- 2 + BMP-2 + BMP-6 + BMP-7.

In certain embodiments, the media according to the invention typically also comprise insulin, transferrin, selenous acid or ITS or ITS+ Universal Culture Supplements (BD™). II - Kits for chondrogenic differentiation

The invention also relates to kits comprising at least one chondrogenic growth factor selected from the group consisting of transforming growth factors β, bone morphogenetic proteins, and mixtures thereof, and a low-molecular-weight sulfated polysaccharide derivative of a marine native exopolysaccharide (EPS) excreted by a mesophilic marine bacterium from a deep hydrothermal environment, as described above.

In certain embodiments, the kits according to the invention further comprise a cell culture medium. Examples of cell culture media typically comprise a minimal medium in which cells can grow, such as for example Dulbecco modified Eagle's minimal essential medium (DMEM), Ham's F-12 Medium, or mixtures thereof, supplemented with at least one of: glucose, bovine serum albumine (BSA), BD™ ITS or ITS+ Universal Culture Supplements, insulin, transferrin, selenous acid, linoleic acid, hydrocortisone, inorganic phosphate, ascorbate-2-phosphate, ascorbate, sodium ascorbate, calcium chloride, thyroxine, proline, pyruvate, sodium pyruvate, pyridoxine hydrochloride, glutamax, non essential amino acids, L-glutamine, β-glycero phosphate, dexamethasone. Particular examples of suitable cell culture media are fully described in the review of Jennifer L. Puetzer (Tissue Engineering: Part B, Volume 16, Number 4, 2010). III - Chondrogenic differentiation methods

Another aspect of the invention relates to ex vivo methods for inducing chondrogenic differentiation in pluripotent or multipotent cells, the methods comprising a step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium according to the invention.

The invention also provides ex vivo methods for obtaining a cartilage tissue, wherein the methods comprise a step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium according to the invention.

The invention also relates to the cartilage tissue obtained using a method according to the invention. The invention further relates to the cartilage tissue obtainable by a method according to the invention, for use in methods of treatment of the human or animal body.

The invention still relates to the cartilage tissue obtainable by a method according to the invention, for use in methods of treatment of a disease associated with cartilage damage in the human or animal body.

The invention also relates to methods for treatment of a disease associated with cartilage damage in a subject in need thereof, the method comprising a step of placing in said subject a cartilage tissue obtained by a method according to the invention. The step of placing of such a cartilage tissue in a subject may be carried out by grafting.

Examples of diseases associated with cartilage damage including, but are not limited to, osteoarthritis, traumatic rupture or detachment of cartilage, osteochondritis, degenerative disc disease (degeneration of the intervertebral disc), relapsing polychondritis.

The step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium of the invention must be carried out for a time duration allowing chondrogenic differentiation. Typically, the culture of pluripotent or multipotent cells with the medium of the invention is carried out for at least 15 days, preferably at least 20 days, even more preferably at least 25 days, most preferably during 28 days.

If necessary, the chondrogenic differentiation medium of the invention can be renewed, partly or totally, at regular intervals. Typically, the chondrogenic differentiation medium of the invention can be replaced with fresh chondrogenic differentiation medium of the invention every 2-3 days, for 28 days.

In certain embodiments, the culture of human stem cells in the chondrogenic differentiation medium is performed by using a three-dimensional culture system. Three-dimensional culture systems are particularly preferred for obtaining cartilage tissues. Examples of three-dimensional culture systems are pellets, micromass, high density cell cultures, and tridimensional cultures in biomaterials, fully described by Vinatier C. et al. in Trends Biotechnol, 2009, 27(5): p.307-14. In certain embodiments, the pluripotent or multipotent cells are human pluripotent or multipotent cells.

In other embodiments, the pluripotent or multipotent cells are non-human mammalian pluripotent or multipotent cells.

In certain embodiments, the pluripotent or multipotent cells are stem cells.

In a particular embodiment, the pluripotent or multipotent cells are multipotent stem cells, particularly human mesenchymal stem cells. The human mesenchymal stem cells are typically isolated from bone marrow, adipose tissue, synovial membrane, umbilical cord blood, muscle, periosteum or placenta. In a particular embodiment, the human mesenchymal stem cells are human adipose tissue-derived stem cells (hATSC).

In another embodiment, said pluripotent or multipotent cells are pluripotent cells, in particular embryonic stem cells.

In a particular embodiment, the pluripotent cells are human embryonic stem cells (hES cells). Typically, hES cell lines such as the ones described in the table below may be employed in the practice of a method of the invention:

In one embodiment, the pluripotent cells are non-human embryonic stem cells a mouse stem cells.

In one embodiment, the pluripotent cells are induced pluripotent stem cells (iPS). Induced pluripotent stem cells (iPS cells) are a type of pluripotent stem cells artificially derived from a non-pluripotent, typically an adult somatic cell, by inducing a "forced" expression of certain genes. iPS cells were first produced in 2006 from mouse cells (Takahashi et al. Cell 2006 126 :663-76) and in 2007 from human cells (Takahashi et al. Cell 2007 131-861-72, Yu et al. Science 2007 318 : 1917).

Further aspects and advantages of this invention will be disclosed in the following figures and examples, which should be regarded as illustrative and not limiting the scope of this application.

Brief Description of the Figures

Figure 1: Structure of the nonasaccharidic repeating unit of GY785 DR. GY785 DR is naturally sulfated at position C2 of the galacturonic acid residue in blue. GY785 DRS is a chemically over-sulfated form of GY785 DR. Putative positions for additional sulfate groups (S0₃Na) are indicated by arrows.

Figure 2: Human ATSC viability and proliferation. Human ATSC were cultured in the presence of either GY785 DR (A and C), GY785 DRS (B and D) at the indicated concentrations or actinomycin D ^g/mL) for 72 hours. Viability (A and B) was evaluated by MTS activity measurement and expressed as the relative MTS activity compared to the untreated control. Proliferation (C and D) was estimated by viable cell counting after trypan blue exclusion dye. * <0.05 compared to the control condition (^g/mL of polysaccharide).

Figure 3: Histological characterization of hATSC pellets. Human ATSC were cultured in pellets in the presence of control (CT) or chondrogenic (CH) medium supplemented or not with 50μg/mL of GY785 DR or GY785 DRS during 28 days. The pellet volumes were calculated by equating these entities to ellipsoids. * <0.05 compared to the control condition ( ^g/mL of polysaccharide). GAG production was evaluated at a gross level after alcian blue staining of the whole pellets. Bar: 500μπι.

Figure 4: Analysis of the expression levels of chondrogenic markers. Human ATSC pellets were cultured in the presence of control (CT) or chondrogenic (CH) medium supplemented or not with 50μg/mL of GY785 DR or GY785 DRS for 28 days. Expression of the chondrogenic markers COL2A1, ACAN, SOX9 and COMP was investigated by real-time PCR. Results are expressed as relative expression level compared to the chondrogenic medium in the absence of polysaccharide. * p <0.05 compared to chondrogenic medium (CH). # p <0.05 compared to chondrogenic medium supplemented with GY785 DR. Examples

Materials and Methods

Materials

Cell culture plasticwares were purchased from Corning-Costar BV Life Sciences (Schipol-Rijk, The Netherlands). Hank's Balanced Sodium Salt (HBSS), Dulbecco's Modified Eagle Medium high glucose (4.5g/L) (DMEM), alpha minimum essential medium (ocMEM), phosphate buffered salt (PBS), penicillin/streptomycin, trypsin/EDTA (0.05%/0.53mM), L-glutamine, superscript III kit, NuPAGE™ 4%- 12% Bis-Tris gel, PVDF (polyvinylidene difluoride). Invitrolon membranes were obtained from Invitrogen Corporation (Paisley, UK). MTS reagents were from Promega (Charbonnieres, France). Collagenase crude type I A, red blood cell lysis buffer, trypan blue, sodium L-ascorbate, ITS media supplement, dexamethasone, alcian blue and anisomycin were purchased from Sigma-Aldrich (St. Louis, MO). Brilliant^® SYBR^® Green Master Mix was obtained from Stratagene Europe (Amsterdam Zuidoost, The Netherlands). PCR primers were synthesized by MWG Biotech (Ebersberg, Germany). Fetal calf serum (FCS) was purchased from Dominique Dutscher (Brumath, France). TGF-βΙ was obtained from PeproTech Inc. (London, UK). RNeasy micro kit was purchased from Qiagen and turbo DNase from Ambion Inc. both distributed by Applied Biosystem (Courtaboeuf, France). Protein content was determined using the Pierce Coomassie Plus assay (Pierce, Rockford, IL). The rabbit anti phospho-SMAD 2 (3101), phospho-ERKl/2 (9101), phospho-JNK 1/2 (9251), phospho-p38 (9211), SMAD 2 (3102), ERKl/2 (9102) and goat anti-rabbit IgG HRP-linked (7074) antibodies were purchased from Cell Signaling Inc. (Beverly, MA). The Western blot detection system was obtained from GE Healthcare (Buckin- ghamshire, UK). All the other chemicals were obtained from standard laboratory suppliers and were of the highest purity available.

Production, purification and characterization of GY785 DR and GY785 DRS polysaccharides

The two low molecular weight polysaccharides GY785 DR and GY785 DRS were derived from GY785, a high molecular weight exopolysaccharide (1.5xl0⁶ Da) produced by a bacterium: Alteromonas infernus, isolated from a sample of fluid collected in the vicinity of an active hydrothermal vent. The isolation procedure and characterization of the strain Alteromonas infernus have previously been described by Raguenes et al. (Raguenes GH et al. J Appl Microbiol. 1997;82:422-430). The native polysaccharide can undergo a radical depolymerization to obtain GY785 DR. Then, the GY785 DR can be chemically over-sulfated to obtain the GY785 DRS as described elsewhere (Guezennec J et al. Carbohydrate Polymers. 1998;37: 19-24). GY785 DR and GY785 DRS are homogenous fractions with average molecular mass of 15 kDa and 20 kDa and 10% and 45% sulfate groups, as determined by analytical high performance size-exclusion chromatography and elemental analysis, respectively (Figure 1) (Colliec Jouault S et al. Biochim Biophys Acta. 2001; 1528: 141-151). Cell culture

Human adipose tissue stromal cells (hATSC) were isolated by collagenase digestion of lipoaspirates obtained from 3 different patients undergoing liposuction and who had given their informed consent. All protocols were approved by the French national ethical committee. Briefly and as previously described (Estes BT et al. Nat Protoc. 2010;5: 1294-1311; Merceron C et al. Am J Physiol Cell Physiol. 2010;298:355-364), lipoaspirates were washed extensively with FIBSS to remove debris. Washed lipoaspirates were treated with collagenase (0.025%) in FIBSS for 1 hour at 37°C with gentle agitation. The collagenase treatment was inactivated by adding an equal volume of DMEM high glucose containing 1% penicillin/streptomycin, 1% L-glutamine and 10% FCS (control medium). The digested product was then centrifuged at 250 x g for 5 min to separate adipocytes from stromal cells. The supernatant was removed and cells were re-suspended in the control medium and filtered through a 70μπι nylon mesh filter. The filtrate was centrifuged and cells re-suspended in red blood cell lysis buffer. The lysis reaction was stopped by adding control medium. The suspension was centrifuged and cells were finally re- suspended in control medium and plated at 5xl0⁴ cells/cm² in 75cm² culture flasks. Cells were incubated at 37°C in a humidified atmosphere containing 5% C0₂ and 95% air and the control medium was replaced 24 hours after seeding to remove non adherent cells. Thereafter, the control medium was renewed every 2-3 days. To prevent spontaneous differentiation, hATSC primary cultures were grown to 90% confluence and then detached from the cell culture flask using trypsin/EDTA and plated at 10⁴ cells/cm². For all subsequent experiments hATSC were used at passage 2. Human ATSC isolated using the above described protocol have been extensively characterized in our laboratory (for details see Merceron C et al. Am J Physiol Cell Physiol. 2010;298:355-364, and Merceron C et al. The effect of two and three dimensional cell culture on the chondrogenic potential of human adipose-derived mesenchymal stem cells after subcutaneous transplantation with an injectable hydrogel, Cell Transplant. 2011 Feb 3., Epub ahead of print).

Viability and proliferation

Cell viability was evaluated using a MTS assay as previously described (Vinatier C et al. Biomaterials. 2005;26:6643-6651). hATSC were plated in 24-well plates at a density of lxlO⁴ cells/cm² and cultured in control medium in the absence or presence of 25, 50, 75 and 100 μg/mL of GY785 DR or GY785 DRS for 72 hours. As a negative control, cells were cultured in the presence of actinomycin D ^g/mL) a well known cell death inducer (Vinatier C et al. Biomaterials. 2005;26:6643-6651). Briefly, culture medium was removed and replaced by fresh medium containing MTS reagents according to the manufacturer's instructions. Results were expressed as relative MTS activity compared to the control condition (cells cultured in the absence of polysaccharide).

To correlate MTS activity with cell proliferation, the number of viable cells was also estimated. As previously described, cells were treated with trypsin/EDTA after 72h of culture and counted using trypan blue exclusion dye (Merceron C et al. Am J Physiol Cell Physiol. 2010;298:355-364; Vinatier C et al. Biomaterials. 2005;26:6643- 6651). Results were expressed as the total number of viable cells/cm² compared with the control condition (cells cultured in the absence of polysaccharide).

Chondrogenic differentiation

For the in vitro chondrogenic differentiation of hATSC, 5x10⁵ cells were placed into a 15 mL polypropylene tube containing lmL of control medium, as previously described (Merceron C et al. Am J Physiol Cell Physiol. 2010;298:355-364). They were then centrifuged for 5 min at 250 x g. The tubes were fitted with vented caps to permit gas exchange, and the cell pellets were maintained at 37°C in a humidified atmosphere containing 5% C0₂ and 95% air. After 24 hours, pellets of hATSC were divided into 6 experimental groups and cultured either in the presence of control (CT) or chondrogenic (CH) medium alone or supplemented with GY785 DR or GY785 DRS. The chondrogenic medium was composed of serum- free control medium supplemented with 6.25μg/mL insulin, 6.25μg/mL transferin, 6.25ng/mL sodium selenite (ITS), 50nM sodium L-ascorbate, 10^"8M dexamethasone and lOng/mL TGF-βΙ (Merceron C et al. Am J Physiol Cell Physiol. 2010;298:355-364; Merceron C et al. The effect of two and three dimensional cell culture on the chondrogenic potential of human adipose-derived mesenchymal stem cells after subcutaneous transplantation with an injectable hydrogel, Cell Transplant. 2011 Feb 3., Epub ahead of print). Culture media were changed every 2-3 days for 28 days. Pellets were maintained at 37°C in a humidified atmosphere (5% C0₂ and 95% air). Human ATSC pellet characterization

For the measurement of the pellet volume, pellets were considered as scalene ellipsoid entities. Their volumes were estimated using the following formula:

Scalene ellipsoid volume = 4/3 π a b c

where a, b and c represent the radius of long axis in each spatial plane.

For pellet gross appearance, the production of sulfated GAGs was investigated on whole 28-day old pellets by alcian blue staining. Pellets were washed with ice-cold PBS and fixed for 20 minutes in 100%> ethanol. Pellets were then stained at room temperature with 0.1%> alcian blue solution in 0.1 M HCl. After overnight incubation, the solution was discarded and the pellets were rinsed with 0.1 M HCl to eliminate nonspecific staining. Photographs were obtained with a stereo-microscope (Leica MZ6, Wetzlar, Germany).

For histological analysis, 28 day-old pellets of hATSC were fixed in 10%> formalin and embedded in paraffin. Paraffin sections (5 μηι thick) were de- paraffinized using toluene, rehydrated through a graded series of ethanol, and rinsed in distilled water. Tissue sections were stained with hematoxylin-eosin-safran (HES) and alcian blue as previously described (Merceron C et al. Am J Physiol Cell Physiol. 2010;298:355-364). Sections were then visualized using a light microscope (Zeiss Axioplan 2, Gottingen, Germany). Alcian blue reveals the presence of a GAG containing cartilaginous matrix and HES stains nucleus in purple, cytoplasm in pink and collagen fibres in yellow. Transcript analysis

Total RNA from 28 day-old pellets of hATSC was extracted using the RNeasy micro kit in accordance with the manufacturer's instructions. After DNase digestion, RNA was quantified using a UV-spectrophotometer (Nanodrop ND-1000, Labtech, Palaiseau, France) and quality was determined with the Agilent Bioanalyser 2100 system (Waldbronn, Germany). 500ng of RNA per sample were reverse transcribed using the superscript III kit in a total volume of 30μ Complementary DNA (cDNA) was amplified in a total volume of 25 μΙ_, PCR reaction mix containing 12.5 μΙ_, of Brilliant^® SYBR^® Green Master Mix (IX) and 30nM of SYBR green reference dye. The sequence and concentration of each primer set are provided in Table 1.

Table 1 : Sequences of primer pairs, gene bank accession numbers used for real time RT-PCR analysis and size of PCR products.

The real-time polymerase chain reaction was carried out in a MX3000P realtime PCR system (Stratagene) under the following conditions: lOmin at 95°C followed by 40 cycles of 30 s at 95°C, 1 min at 60°C and 30 s at 72°C. The efficiency and specificity of each primer set was confirmed with standard curves of cycle threshold (Ct) values versus serial dilution of total RNA and melting profile evaluation. Cycle Thresholds were normalized to β-actin to control for cDNA quantification differences. Results were reported as relative expression levels compared to the cells cultured in the presence of chondrogenic medium. Surface plasmon resonance

Experiments were carried out on a Biacore 3000 instrument (Biacore, Uppsala, Sweden). TGF-βΙ and insulin were covalently immobilized to the dextran matrix of a CM5 sensor chip (Biacore) as recommended by the manufacturer at flow rate of 5nL/min. Binding assay of GY785 DR (1.5, 3.125, 6.25, 12.5, 25, 50 and 100 μg/mL) and GY785 DRS (0.0312, 0.0625, 0.125, 0.25, 0.50 and ^g/mL) were performed in lOmM HEPES buffer, pH 7.4, containing 0.15M NaCl and 0.005% P20 surfactant (HBS-P buffer,Biacore) and dissociation was monitored for 15 minutes. Regeneration was achieved with NaOH (4.5 mmol/L) after each cycle. The resulting sensorgrams were fitted using BiaEval 4.1 software (Biacore). For K_d calculations, the following molecular weights were used: GY785 DR: 15,000 g/mol and GY785 DRS: 20,000 g/mol.

Western blotting

Confluent hATSC were cultured in the presence of TGF-βΙ (lOng/mL) alone or in combination with GY785 DR or GY785 DRS (50μg/mL) in control medium containing low serum levels (0.5%) for 1, 4, 8 and 24 hour-periods. For each time point, cells were rapidly frozen in liquid nitrogen and conserved at -80°C until use. For western blotting, cells were thawed on ice and lysed by addition of a RIPA buffer (20mM Tris HC1, pH 7.5, lOOmM potassium chloride, ImM EDTA, ImM EGTA, ImM dithiothreitol, 20mM β-glycerophosphate, 2mM Na₃V0₄, ImM PMSF and ImM NaF). The protein concentration of cell lysates was determined with a Pierce Coomassie-Plus-protein assay. 30μg of total protein were resolved by sodium dodecyl sulfate-polyacrylamide gels, and proteins were transferred to a PVDF membrane following the manufacturer' s protocol. Membranes were blocked and probed in 5% non-fat dry milk in PBS/Tween20. Primary antibodies were diluted 1/1000 and were detected using goat anti-rabbit (FIRP)-conjugated secondary antibodies diluted 1/2000 in 5% non-fat dry milk in PBS/Tween20. The blots were visualized by Enhanced ChemiLuminescence (ECL) development using a Western blotting detection system.

As a positive control for SMAD and MAP Kinase activation, confluent osteoblastic MC3T3-E1 cells were serum starved overnight and treated for 15 minutes with anisomycin ^g/mL), TGF-βΙ (lOng/mL) or inorganic phosphate (Pi; lOmM) as previously described ( ien M et al. J Bone Miner Res. 2009;24: 1856-1868). Statistical analysis

Each experiment was repeated at least 3 times with similar results. Results are expressed as mean ± SEM of triplicate determinations. Comparative studies of means were performed by using one-way ANOVA followed by a post hoc test (Fisher's projected least significant difference) with a statistical significance at / 0.05.

Results

Viability and proliferation of hATSC cultured in the presence of polysaccharides

To examine the viability and proliferation of hATSC cultured in the presence of 0, 25, 50, 75 and 100 μg/mL of GY785 DR or GY785 DRS, MTS activity was measured and cells were enumerated using trypan blue exclusion dye after 72 hours. As a negative control, cells were cultured in the presence of actinomycin D ^g/mL). When treated with actinomycin D, the MTS activity and the proliferation of hATSC were significantly reduced by nearly 90%. At the concentration of 50μg/mL, GY785 DR induced a slight but significant increase in MTS activity (Figure 2A). GY785 DRS was found to trigger a dose-dependent increase in MTS activity, with a maximum at 50 μg/mL (Figure 2B). Regarding hATSC proliferation, GY785 DR did not elicit any beneficial effect (Figure 2C), whereas, the sulfated form of the molecule (GY785 DRS) at 50 and 75 μg/mL significantly increased hATSC proliferation in comparison to the control condition (Figure 2D).

These results indicate that GY785 DR and GY785 DRS have only a slight but significant effect on the viability and proliferation of hATSC. In all subsequent experiments, GY785 DR and GY785 DRS were used at the dose of 50μg/mL.

Chondrogenic differentiation of hATSC cultured in the presence of polysaccharides hATSC were cultured in three-dimensional pellet in the presence of control (CT) or chondrogenic (CH) medium supplemented with 50μg/mL of GY785 DR or GY785 DRS during 28 days. Chondrogenic differentiation was evaluated by a measurement of pellet volume and by the production of a GAG-containing cartilaginous matrix using alcian blue staining (Figure 3).

Surprisingly, volume estimation revealed that pellets exposed to GY785 DRS in combination with the chondrogenic medium undergo a massive increase by nearly 8- fold (Figure 3 upper panel). In addition to highlight differences in terms of GAG production between the different conditions, the gross appearance of pellets was observed after alcian blue staining. Alcian blue staining revealed that in the presence of chondrogenic medium, and regardless of polysaccharides supplementation, GAG production was up-regulated as evidenced by the intense dark blue color (Figure 3 lower panel).

To further characterize hATSC chondrogenic differentiation, cell morphology and matrix composition were then histologically examined by HES and alcian blue staining on pellets sections. In the presence of control medium (CT), HES staining allows distinguishing cell nuclei (purple) and cytoplasm (pink) but does not evidence a particular organization of the cells. On the contrary, in the presence of chondrogenic medium (CH), supplemented or not with polysaccharide, HES staining evidenced a particular structural organization of the cells within the pellet. In the external zone, cells are tangentially oriented to the surface of the pellet and in the innermost part, cells seem to be arranged radially. Moreover, in the presence of chondrogenic medium, a yellow-orange ring is visible, indicative of the synthesis of collagen fibers within the matrix. Alcian blue staining failed to reveal the presence of sulfated GAG within the matrix of pellets cultured in control medium. Interestingly, in the presence of chondrogenic medium pellet sections were strongly positive for sulfated GAG detection, especially in the presence of chondrogenic medium supplemented with GY785 DRS polysaccharide, where a denser deep blue staining can be observed.

To confirm the cartilage-like appearance of hATSC pellets evidenced by the histological observations of the present inventors, the relative expression of COL2A1, ACAN, SOX9 and COMP transcripts was determined by real-time PCR (Figure 4). The data obtained indicate that in the presence of control medium (CT) supplemented or not with polysaccharide, transcripts coding for the various chondrocyte markers could not be detected ( D) or remained at barely detectable levels. For each transcript analyzed, the expression level was significantly increased in the presence of chondrogenic medium compared to the control medium. Of interest, GY785 DRS used in combination with chondrogenic medium induced a marked increase in the expression levels of the 4 chondrogenic markers when compared to GY785 DR. GY785 DR failed to induce any additive or synergistic effect with the chondrogenic medium. Taken together, these results show that GY785 DRS potentiates the chondrogenic differentiation of hATSC when used concomitantly with chondrogenic medium.

Interactions between GY785 DR or GY785 DRS polysaccharides with TGF- βΐ/insulin of chondrogenic medium.

To further address whether GY785 DRS may stimulate hATSC chondrogenic differentiation, several surface plasmon resonance experiments were performed. The chondrogenic medium used contained 2 major constituents: TGF- βΐ (Awad HA et al. Tissue Eng. 2003;9: 1301-1312; Puetzer JL et al. Tissue Eng Part B Rev. 2010; 16:435- 444) and insulin (Malafaya PB et al. Tissue Eng Part A. 2010; 16:735-747; Wang CY et al. Apoptosis. 2010; 15:439-449), which are known to drive the chondrogenic differentiation of MSC. To investigate whether TGF- βΐ and insulin can specifically interact with GY785 DR or GY785 DRS, quantitative measurements of their potential physical interaction were performed by Biacore analysis. TGF-β and insulin were immobilized on the chip and increasing concentrations of GY785 DR and GY785 DRS polysaccharides were injected over the chip surface. The results expressed in response units were recorded for each analyte concentration in the form of sensorgram and dissociation constant (KJ) was calculated. GY785 DR and GY785 DRS polysaccharides were both able to bind immobilized TGF-β. Binding affinity of GY785 DR for TGF-β is about one-hundred-fold lower than that of GY785 DRS polysaccharide with respective Kd of 3,45.10^"8 and 5,5.10^"10 M. No modification of the kinetic parameters of the interaction between GY785 DR or GY785 DRS in the binding of immobilized insulin was observed (data exhibiting a flat sensorgram are not shown). These results indicate that GY785 DRS can bind TGF-βΙ with higher affinity than GY785 DR and none of them interacts with insulin.

Effects of GY785 DRS on TGF- 1 signalling pathway.

TGF-βΙ is known to activate several signalling pathways including SMAD 2 (Massague J. et al. Genes Dev. 2000; 14:627-644). Therefore, to address whether GY785 DRS/ TGF-βΙ interaction evidenced by surface plasmon resonance may lead to specific activation of cellular events in hATSC, the potential up-regulation of TGF-β dependent activation of SMAD 2 was determined in hATSC. To this end hATSC were exposed to lOng/mL of TGF-βΙ and 50μg/mL of GY785 DRS alone or concomitantly for 1, 4, 8 and 24 hours. MC3T3-E1 cells were used as positive controls. Cells were rapidly frozen in liquid nitrogen before lysis at 4°C. The resulting samples were analyzed by Western blot using specific antibodies against P-SMAD 2, P-ERK1/2, P- J K1/2 and P-p38, and/or antibodies against SMAD 2 and ERK1/2. Immunoblots of cell lysates indicated that TGF-βΙ alone or in association with GY785 DRS polysaccharide induced the phosphorylation of SMAD 2 in as early as 1 hour and until 24 hours. The presence of the sulfated polysaccharide alone is not sufficient to promote SMAD 2 activation and no additive or synergistic effect of GY785 DRS and TGF-βΙ could be detected on the phosphorylation of SMAD 2. Since MAP kinase signalling pathways, including ERK, INK and p38, have been largely involved in TGF-β dependent chondrogenic differentiation (Derynck R et al. Nature. 2003;425:577-584; Arita NA et al. Biochem Biophys Res Commun. 2011), the present inventors sought to decipher whether MAPK could be activated in response to treatment with TGF-βΙ and GY785 DRS. Of particular interest, whereas ERK 1/2 phosphorylation was barely stimulated by TGF-βΙ or GY785 DRS alone, the concomitant treatment of cells with TGF-βΙ and GY785 DRS induced a marked up-regulation of the phosphorylation of ERK 1/2 as early as 4 hours. This stimulation was maintained up to 24 hours. Analysis of the phosphorylation of the other MAPK showed no detectable phosphorylation of either INK or p38 in response to TGF-βΙ and GY785 DRS treatment alone or combined.

To ensure the reliability of our detection method for the phosphorylation of SMAD 2, ERK1/2, INK and p38, MC3T3-E1 cells were treated with anisomycin, Pi and TGF-βΙ and used as a positive control. As expected, in these conditions, phosphorylation of p38 and JNKl/2 were observed after anisomycin treatment (Julien M et al. J Bone Miner Res. 2009;24: 1856-1868), phosphorylation of ERK 1/2 was observed after Pi stimulation (Julien M et al. J Bone Miner Res. 2009;24: 1856-1868) and phosphorylation of SMAD 2 was observed in the presence of TGF-βΙ (Lai CF et al. J Biol Chem. 2000;275:36400-36406). The phosphorylation of the various SMAD and MAPK was not associated with changes in their basal levels, suggesting that their phosphorylation resulted from the stimulation of regulatory upstream kinases. These data suggest that TGF-βΙ and GY785 DRS may act concomitantly in a synergic manner to stimulate the MAP Kinase ERK 1/2 activation in hATSC.

Throughout this application, various references describe the state of the art to which this invention pertains. The disclosures of these references are hereby incorporated by reference into the present disclosure.

Claims

A chondrogenic differentiation medium comprising:

- at least one chondrogenic growth factor selected from the group consisting of transforming growth factors β, bone morphogenetic proteins, and mixtures thereof, and

- a low-molecular-weight sulfated polysaccharide derivative of a marine native exopolysaccharide (EPS) excreted by a mesophilic marine bacterium from a deep-sea hydrothermal environment,

The chondrogenic differentiation medium according to claim 1, wherein said derivative:

- has a molecular weight of 5,000 to 60,000 g/mol, 5,000 to 50,000 g/mol, 5,000 to 40,000 g/mol, 5,000 to 30,000 g/mol, or of 10,000 to 25,000 g/mol, and

- has a polydispersity index of less than 5, particularly of 1.5 to 4, more particularly of less than 2.

The chondrogenic differentiation medium according to claim 1 or 2, wherein said mesophilic marine bacterium is selected from the group consisting of bacteria of the Alteromonas genus, Pseudoalteromonas genus and Vibrio genus.

4. The chondrogenic differentiation medium according to any one of claims 1-3, wherein said mesophilic marine bacterium is the strain GY785 of the Alteromonas genus.

5. The chondrogenic differentiation medium according to any one of claims 1-4, wherein said medium comprises 5μg/mL to 20C^g/mL, particularly 25μg/mL to 10C^g/mL, more particularly 25μg/mL to 75μg/mL, most particularly about 5C^g/mL of said derivative.

6. The chondrogenic differentiation medium according to any one of claims 1-5, wherein said at least one chondrogenic growth factor is selected from the group consisting of TGF-βΙ, TGF- 2, TGF- 3, BMP-2, BMP-4, BMP-6, BMP-7 and BMP-9, and mixtures thereof.

7. The chondrogenic differentiation medium according to any one of claims 1-6, wherein said medium further comprises a fibroblast growth factor and/or an insulin-like growth factor, in particular IGF-1.

8. A kit comprising:

wherein said derivative is as defined in any one of claims 1-4.

9. The kit according to claim 8, wherein said kit further comprises a cell culture medium.

10. A method for inducing chondrogenic differentiation in pluripotent or multipotent cells, wherein said method comprises the step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium according to any one of claims 1-7.

11. A method for obtaining a cartilage tissue, wherein said method comprises the step of culturing pluripotent or multipotent cells with a chondrogenic differentiation medium according to any one of claims 1-7.

12. The method according to claim 10 or 11, wherein said cells are human mesenchymal stem cells, in particular human adipose tissue-derived stem cells (hATSC).

13. A cartilage tissue obtainable by the method according to claim 11 or 12.

14. Use of the cartilage tissue according to claim 13 as a graft in a method of treatment of a disease associated with cartilage damage in a human or animal body.

15. Use of the cartilage tissue according to claim 13 as a graft in a method of treatment of a disease associated with cartilage damage in a human or animal body.

16. A method for treating a disease associated with cartilage damage in a subject in need thereof, wherein said method comprises a step of placing a cartilage tissue according to claim 13 in said subject.

17. The method according to claim 16, wherein the subject has a disease associated with cartilage damage.

18. The use according to 15 or the method according to claim 17, wherein the disease associated with cartilage damage is osteoarthritis, traumatic rupture, detachment of cartilage, osteochondritis, degenerative disc disease, or relapsing polychondritis.