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    • 专利摘要:
    A method of modifying polysaccharides, wherein: (a) reacting a polysaccharide with a modified polyetheramine (XRC (O) NH) bR '(where R' is a polyether and b = 1, 2 or 3 and X is a halogen, preferably Cl or Br, R represents an alkyl residue, possibly substituted, or an aromatic residue, possibly substituted), in the presence of a base, preferably in the presence of water and isopropanol, (b) purifying the product obtained in the presence of NaCl, at least in part, by a membrane separation method, said purification being carried out at a pH of between 9 and 13 (and preferably between 10 and 12); (c) the product resulting from step (b) is purified, at least in part, by a membrane separation method, said purification being carried out after neutralization at a pH of between 6 and 8 (preferably between 6.5 and 7.5), optionally after lyophilization and washing of the lyophilized product (preferably with ethanol).
    公开号:FR3023485A1
    申请号:FR1401564
    申请日:2014-07-11
    公开日:2016-01-15
    发明作者:Zied Souguir;Elise Demange
    申请人:Celenys;
    IPC主号:
    专利说明:

    [0001] The invention relates to organic chemistry, more particularly to polysaccharide chemistry. It relates more specifically to the modification of natural or synthetic polysaccharides by grafting polyetheramines. It also relates to the use of these modified polysaccharides in the form of a hydrogel as a cell culture medium. These hydrogel preparations may have thermosensitive rheological properties, which are of interest for their intracorporeal use in human and veterinary medicine, for cell culture and the transport of biological samples (cells, explants, biopsies, etc.).
    [0002] STATE OF THE ART One of the most widespread polysaccharides in the animal and human body is hyaluronic acid. It can be manufactured on an industrial scale by fermentation using microorganisms (in particular Streptococcus equi). This product of biological origin is a biocompatible and biodegradable polysaccharide, which can form hydrogels. For these reasons, intracorporeal uses have been sought for this product, particularly in orthopedics. Thus, the intracorporeal use of hydrogels of hyaluronic acid (HA) for the treatment of worn or damaged cartilage is well known; the best known method is viscosupplementation (i.e. addition of HA to synovial fluid, or total replacement of synovial fluid by HA). Intracorporeal use in dermatology has also been considered. It appeared the idea to chemically modify the HA. This makes it possible to generate hydrogels presenting new and particular properties. This is described in detail in the publication "Chemical modifications of hyaluronic acid for the synthesis of derivatives for broad spectrum of biomechanical applications" by C.E. Schanté et al., Published in the journal Carbohydrate Polymers, vol. 85, p. 469-489 (2011), in the doctoral thesis of Zied Souguir ("Functionalization of polysaccharides and study of their properties 'pH dependent'"), University of Rouen, 2006, and in the doctoral thesis of Kristoffer Bergman «Hyaluronan Derivatives and Injectable Gels for Tissue Engineering ", Upsala 2008. However, such a chemical modification must not induce toxicity, direct or indirect (ie through the products of decomposition during metabolism of the modified HA), and must not affect the biodegradability of the product. Numerous patents deal with the chemical modification of HA and the use of modified HA for the treatment of joint pathologies. By way of example, EP 1 095 064 (Fidia) describes a number of HA derivatives. EP 2 457 574 A1 (Fidia Andvanced Biopolymes) describes the preparation of biomaterials from derivatives of HA which are amides, and tests of their use in viscosupplementation. WO 2004/022603 (LG Life Sciences) discloses HA polymers crosslinked with glycol based polymers, while KR 1007 37954 B1 (Korea University) describes an acrylated derivative of HA; these two documents envisage the intracorporeal use of the products obtained. The grafting of hyaluronic acid by polyetheramines of the Jeffamine CD type and by poly (N-isopropylacrylamides) (PNIPAM) is known from the article "Single step synthesis and characterization of thermoresponsive hyaluronan hydrogels" by M. D'Este and al., published in the journal Carbohydrate Polymers 90 (2012), p. 1378-1385.
    [0003] Some of these modified (functionalized) HA hydrogels exhibit thermosensitive rheological properties. Intracorporeal applications for the controlled release of active ingredients have been considered for these products, see for example the following publications: Mee Ryang Kim and Tae Gwan Park, "Temperature-responsive and degradable hyaluronic acid / Pluronic acid hydrogels for controlled release of human growth hormone ", Journal of Controlled Release, vol. 80, p. 69-77 (2002); TR Hoare and DSKohane, "Hydrogels in drug delivery: Progress and Challenges", Polymer, vol 49 (2008), 1993-2007, CCChen et al., "Transdermal delivery of selegiline from alginate-Pluronic composite thermogels" , International J of Pharmaceutics, 415 (2010), 119-128, S. Van Vlierberghe et al., "Biopolymer-Based Hydrogels As Scaffolds for Tissue Engineering Applications: A Review," Biomacromolecules, 2011, 12, p. 1387-1408 It appears that the choice of the grafted molecules on the polysaccharide is critical for the physicochemical characteristics of the product, more particularly the patent application EP 1 659 143 (Teijin) describes thermosensitive hydrogels of hyaluronic acid and propylene oxide secondary polyetheramine (Jeffamine XTJ-507), the intended application is the regeneration of cartilage.According to the teaching of this document, the viscosity transition zone is spread over a range of temperature of a width of about at 15 ° C, which is too wide for an application in medicine. Several publications suggest that the choice of polyetheramine may have an influence on the physicochemical properties of the product. By way of example, the article by G. Mocanu et al., "Multi-responsive carboxymethyl polysaccharide crosslinked hydrogels containing Jeffamine side-chains" published in Carbohydrate Polymers, vol. 89, p. 578-585 (2012) shows, for a hydrogel containing a polysaccharide other than HA, a noticeable difference in temperature-sensitive properties between the Jeffamines ® M600 and M-2005 (two products which are distinguished by their ratio Propylene oxide / Ethylene oxide and their molar masses). The publication "Single step synthesis and characterization of thermoresponsive hyaluronan hydrogels" by M. d'Este et al. (Carbohydrate Polymers, vol 90, pp. 1378-1385 (2012)) shows for a HA-Jeffamine CD type hydrogel that Jeffamine® M2005 does not lead to a significant thermosensitivity, whereas the thermosensitivity of the hydrogel with Jeffamine ® M600 is noticeable but quite weak.
    [0004] Heat-sensitive hydrogels of chitosan modified by acetylation or deacetylation are also known, see US 2009/0004276 (Mor Research Applications Ltd). It is also known that the modification of certain polysaccharides makes it possible to prepare hydrogels whose properties depend on the pH, see the thesis quoted by Zied Souguir and the publication of G. Mocanu et al., "New anionic crosslinked multi-responsive pullulan hydrogels" , published in Carbohydrate Polymers, vol. 87, p. 14401446 (2012). However, in all these cases, the variation of the properties of the hydrogel as a function of the biological environment in which it is found in the case of an intrabody use, and in particular the variation of its properties as a function of the temperature , is quite weak and quite difficult to control during the synthesis of the product. There is clearly a need for a new approach for preparing a wider range of modified, biocompatible, non-toxic polysaccharides, which can be used intracorporeally, and in particular useful for the transport and / or controlled release of principles. active and / or cell, which have thermosensitive properties showing a wider variation and which are easier to control during their synthesis.
    [0005] OBJECTS OF THE INVENTION According to the invention, the problem is solved by a novel route of synthesis of polysaccharides modified by grafting polyetheramines. The Applicant has realized that the available polyetheramines did not solve the problem, and that it was first necessary to develop new molecules of polyetheramines capable of being grafted onto a polysaccharide. This allowed him then to prepare new polysaccharides modified by grafting said polyetheramines, as well as new preparations based on polysaccharides thus modified, which have particularly advantageous thermosensitive rheological properties. Thus a first object of the invention is a method for modifying polysaccharides, wherein: (a) a polysaccharide is reacted with a modified polyetheramine of the type (X-RC (O) NH) bR '(where R' represents a polyether and b = 1, 2 or 3 and X represents a halogen, preferably Cl or Br, R represents an alkyl residue, possibly substituted, or an aromatic residue, possibly substituted), in the presence of a base, preferably in the presence of water and isopropanol, (b) the product obtained in the presence of NaCl is purified, at least in part, by a membrane separation method, said purification being carried out at a pH of between 9 and 13 (and preferably between 10 and 12); (c) the product resulting from step (b) is purified, at least in part, by a membrane separation method, said purification being carried out after neutralization at a pH of between 6 and 8 (preferably between 6.5 and 7.5), optionally after lyophilization and washing of the lyophilized product (preferably with ethanol). R is advantageously an alkyl radical, which may be substituted (for example a C1, C2, C3, C4, C5, C6, C7, C8, C9 or C10 C11 or C12 radical), or an aromatic radical (for example a phenyl radical), possibly substituted.
    [0006] In one embodiment, said modified polyetheramine is a polyethermonoamine in which the radical R 'has the following structure: H3C "(where Z is a hydrogen atom (in the case of ethylene oxide) or a methyl (in the case of propylene oxide), and wherein, preferably, x = 1 to 3, Z = CH 3 and y = 7 to 11 (with x = 1 and y = 9 preferred) x = 17 to 21, Z = CH 3 and y = 2 to 5 (with x = 19 and y = 3 preferred), x = 5 to 8, Z = CH 3 and y = 25 to 32 (with x = 6 and y = 29 preferred). polyetheramine R 'has a molar mass of between about 300 and about 3,000, and even more preferably between about 500 and about 2,500, and / or said polyetheramine having a molar ratio of [ropylene oxide] / [ethylene oxide] of between 10/1 and 1/10 In an advantageous embodiment of the process according to the invention, at least one carboxylic functional group FS-COOH of the polysaccharide ps is activated first with the aid of a quaternary amine, and then said modified polyetheramine is added.
    [0007] To allow the use of the modified polysaccharide in pharmaceutical or intracorporeal uses, the process according to the invention may comprise at least one purification step, and preferably all purification steps after neutralization, is carried out at a temperature below 20 °. C, preferably between 0 ° C and 15 ° C, and even more preferably between 2 ° C and 8 ° C. In the process for modifying the polysaccharides according to the invention, the product resulting from stage (c) may be lyophilized, washed with ethanol and dried. Advantageously, for use in a hydrogel, said polysaccharide is selected from the group formed by neutral polysaccharides (and especially by pullulan and dextran), natural anionic polysaccharides (and in particular: alginate, hyaluronic acid, xanthan gum, agar agar gum, pectins, heparin), synthetic anionic polysaccharides (and in particular: carboxymethylcellulose, carboxymethylpullunane), natural cationic polysaccharides (and in particular chitosan), cationic synthetic polysaccharides (and especially: diethylaminoethylcellulose, diethylamonithyldextran), amphiphilic polysaccharides, zwitterionic polysaccharides natural or obtained by chemical modification (and in particular carboxymethylchitosan), or mixtures of these polysaccharides. Pullulan, xanthan, alginate and hyaluronic acid are particularly preferred.
    [0008] Another subject of the invention is a modified polysaccharide obtainable by the process according to the invention. Yet another subject of the invention is a hydrogel formed by at least one modified polysaccharide according to the invention and an aqueous liquid. Said aqueous liquid may comprise serum and / or cell culture medium. In one embodiment, the hydrogel according to the invention advantageously has thermosensitive rheological properties with a transition temperature of between 33 and 39 ° C. In another embodiment, it has thermosensitive rheological properties with a transition temperature of between 4 and 20 ° C. Yet another object of the invention is the use of a hydrogel according to the invention in a medium for cell culture or in a medium for the transport of cells. A final subject of the invention is the use of a hydrogel according to the invention for the preparation of a composition intended to be used as a skin dressing, an embolization agent, a viscosupplementation agent, a filler, an agent limiting post surgical adhesion, or tissue regenerative agent. DESCRIPTION OF THE FIGURES FIGS. 1 to 6, 8 and 9 illustrate various aspects of the invention, FIG. 7 relates to the state of the art. Figures 1 and 2 relate to an attempt to modify a Jeffamine® M2005 type polyetheramine by reaction with a halogenated acyl halide. The vertical axis represents the normalized intensity. Figure 1 shows the 1H NMR Spectrum (in CDCl3) of the modified polyetheramine. FIG. 2 shows infrared (FT-IR) spectra: curve (a) corresponds to the starting polyetheramine, curve (b) to modified polyetheramine. FIGS. 3 to 5 relate to a grafting test of a polysaccharide (in this case hyaluronic acid) with a Jeffamine M2005 polyetheramine which has been previously modified by reaction with a halogenated acyl halide (and which is the same as that of Figures 1 and 2). Figure 3 shows the 1H NMR spectrum (in D20) of a hyaluronic acid (HA) grafted by the modified polyetheramine.
    [0009] FIGS. 4 and 5 show the variation of the storage modules (elastic modulus) G '(s) and of the loss (viscous modulus) G "(-) of the grafted HA as a function of the temperature: the concentration of grafted HA is 40 g In the RPMI culture medium (FIG. 4) or 20 g / I (FIG. 5) The reversible sol-gel transition is noted for a temperature below 37 ° C. (approximately 29 ° C. for FIG. 34 ° C for Figure 5) Figures 6 to 9 refer to the tests described in detail in the "Examples" section Figure 6 shows the UV absorbance as a function of temperature for a polysaccharide (in FIG. occurrence HA) grafted with a Jeffamine® M2005 type polyetheramine which had been previously modified by the action of 2-Bromo-2-methylpropionylbromide (Williamson reaction) The figure represents a measurement made on the reaction mixture.
    [0010] FIGS. 7 and 8 compare the variation of conservation modulus (elastic modulus) G '(curve A) and loss (viscous modulus) G "(curve B) as a function of temperature for ungrafted hyaluronic acid (FIG. ) and for the grafted hyaluronic acid (grafting rate: 2 mol%) with a Jeffamine 0 M2005 polyetheramine which had been previously modified by the action of 2-Bromo-2-methylpropionylbromide (esterification reaction) (FIG. In both cases, the concentration of HA (grafted or ungrafted) was 40 g / l in the RPMI culture medium, and Figure 9 shows DSC (differential scanning calorimetry) curves. ) for a sample of HA hydrogel grafted with a Jeffamine® M2005 type polyetheramine which had been previously modified by the action of 2-Bromo-2-methylpropionylbromide (esterification reaction), these hydrogels were formed with a medium of culture Cell RPMI type Curve A: Hydrogel of HA grafted by a modified Jeffamine ®. Curve B: Modified Jeffamine ® (for comparison).
    [0011] Curve C: Jeffamine ® M2005 (for comparison). DETAILED DESCRIPTION OF THE INVENTION The modified polysaccharides according to the invention which give the best resultants being modified by grafting of polyetheramine derivatives which are not commercially available, here a general method is first described (section A) in order to obtain modified polyetheramines which are capable of being grafted onto polysaccharides, and then two methods (sections B and C) of grafting by esterification of the polysaccharide are described, making it possible to obtain polysaccharides with thermosensitive rheological properties. These two methods give substantially the same products. Finally, we describe (section D) the use of these products. A) Modification of Polyetheramine by Reaction with Halogenated Acyl Halide This reaction proceeds according to the following scheme: XRC (O) X + (H2N) bR '---> (XRC (O) NH) bR' where b is 1, 2 or 3, where X is halogen (preferably Cl or Br); R represents an alkyl radical, possibly substituted (for example a C1, C2, C3, C4, C5, C6, C7, C8, C9 or C10 C11 or C12 radical), or an aromatic radical (for example a phenyl radical), possibly substituted (but the functionalization of the aromatic residue is not preferred); and R 'represents a polyether, preferably of the PPO or (PEO) xco- (PPO) y type. The polyetheramine may be a polyethermonoamine (with b = 1), or a polyetherdiamine (with b = 2), or a polyethertriamine (with b = 3). Primary amines are preferably used. The reaction proceeds in the presence of a base, preferably Et3N and / or NaOH, which captures the HX resulting from the reaction. The temperature is below 35 ° C, preferably below 25 ° C, and even more preferably below 20 ° C, and optimally between 0 ° C and 10 ° C; a temperature of about 4 ° C is suitable.
    [0012] Preferably, the reaction of the polyetheramine H2N-R 'with the halide of a halogenated acyl X-R-C (O) X is carried out without a solvent. After the reaction, the mixture is purified by simply washing with acidic water: this wash removes the unreacted amine and the HX acid (or its salt) which results from the reaction.
    [0013] The following scheme shows an advantageous embodiment of this reaction using a polyethermonoamine: Et3N or NaOH / OXR + H2N-R '→ XR 4 ° C NR' HX: Halogen (Cl, Br, ...) R Alkyl, aromatic, ... R ': PPO or (PEO) x-co- (PPO) Polyetherdiamine may also be used: XR Et3N or NaOH + H2N-R "-NH2 .- XRH4 ° C NR "-NH-RX X: Halogen (Cl, Br, ...) 0 R: alkyl, aromatic, ... R": PPO or (PEO) x-co- (PPO) Polyethertriamine may also be used : $ 0, NH RX i 2 and N 3 or NaOH 0 7 + H2N-R "-NH 2 a. XR / NH 4 ° C NR "HH (R) OXR X: Halogen (Cl, Br, ...) R: alkyl, aromatic, ... R": PPO or (PEO) x-co- ( PPO) here PPO means polypropylene oxide and PEO means polyethylene oxide, and (PEO) xco- (PPO) y is a copolymer between PO (propylene oxide) and EO (ethylene oxide). The abbreviation Et3N means triethylamine.
    [0014] As polyetheramine H2N-R 'or R "(NH2) 2 or R" (NH2) 3 may be used in particular products available under the trademark Jeffamine ®, and in particular products Jeffamine ® M600, Jeffamine M2005, Jeffamine ® M2070, Jeffamine D2000 ...). All these products are liquids, and the reaction can proceed without solvent; as a rule, the product X-R-C (O) NHR 'obtained has a viscosity greater than the starting polyetheramine H2N-R'. The same applies to polyetherdiamines and polyethertriamines. The absence of solvent (such as: DMF, THF) for the reaction has several advantages: these solvents are expensive, and they are toxic and must then be removed from the product because it is necessary to avoid contaminating the product with molecules that are likely to embarrassing for its end use (which may be used in cell culture or even intracorporeal use). The product can be stored in isopropanol (in the form of solution), this solvent being chosen according to the subsequent use of the product. The product can be characterized by NMR and Infrared spectroscopy to demonstrate its identity and purity. B) Modification of polysaccharides by the Williamson reaction This method aims to graft the modified polyetheramine, obtained for example according to step 1 described above, on a polysaccharide to obtain in particular polysaccharides with thermosensitive rheological properties. An alternative method is presented below (method C).
    [0015] The reaction comprises the grafting of a modified polyetheramine of the type (XR-C (O) NH) bR '(for example an XRC (0) NHR' type modified polyetheramino, or a modified polyetherdiamine of the type (XRC (O) NH 2R ', or alternatively a modified polyethertriamine of the type (XRC (O) NH) 3R') on a -OH group of a polysaccharide (PS -OH), which leads to a modified polysaccharide of the type (PS -0- RC (O) NH) bR '(in the case of a modified polysaccharide-modified polyether-amylamino may be of the type Ps-O-RC (O) NHR', in the case of a modified polyether-amine the modified polysaccharide may be type (PS-O-RC (O) NH) 2R ', and in the case of a modified polyethertriamine the modified polysaccharide may be of the type (PS - O - RC (O) NH) 3R'), in which the The oxygen atom which constitutes the grafting point between the polysaccharide and the graft is derived from the OH group of the polysaccharide. In this reaction scheme, the symbols X, R and R 'have the same meaning as that described in relation to method A above.
    [0016] The reaction is preferably carried out in a mixture of water and isopropanol, employing directly the product of method A described above. The following scheme shows an advantageous embodiment of this reaction: NR 'H H 2 O / isopropanol NaOH 70 ° CX: Halogen (Cl, Br, ...) R: alkyl, aromatic, ... R': PPO or (PEO ) x-co- (PPO) y Physicochemical analyzes carried out in a cell culture medium (RPMI) by rheological measurements, conservation modules (G ') and loss modules (G ") as a function of temperature for two concentrations (40 and 20 g / l) show the reversible sol gel transition for temperatures below 37 ° C. C) Modification of polysaccharides by esterification This method is intended to graft the modified polyetheramine, obtained for example according to step 1 described above. above, on a polysaccharide to obtain in particular polysaccharides with thermosensitive rheological properties.This is an alternative to the method B presented above.
    [0017] The reaction comprises activating the PS-COOH carboxylic function of a PS polysaccharide with a quaternary amine, and preferably tetrabutylamine (TBA), resulting in ps-co- function, followed by graft grafting. a modified polyetheramine (XRC (O) NH) bR 'on said -000- group of the polysaccharide, which leads to a modified polysaccharide of the type (S-000-RC (O) NH) b R', in which the oxygen atom which constitutes the grafting point between the polysaccharide and the graft comes from the COOH group of the polysaccharide. In this reaction scheme, the symbols X, R and R 'have the same meaning as that described in relation to method A above. The reaction is preferably carried out in a mixture of water and isopropanol, employing directly the product of method A described above. A temperature above 25 ° C, preferably between 40 ° C and 95 ° C, and even more preferably between 55 ° C and 90 ° C, a temperature of about 70 ° C is preferred. The following scheme shows an advantageous embodiment of this reaction: X: Halogen (Cl, Br, ...) R: alkyl, aromatic, ... O H 2 O / isopropanol XR NR 'H R': PEO, PPO or ( PEO) x-co- (PPO) y 70 ° C OR .4 NR 'H Common remarks for methods B and C: a) Purification Polysaccharide The reaction product from method B or C must be purified if it is intended for intracorporeal use. This purification is advantageously in the presence of NaCl and in at least two stages which are distinguished by their pH.
    [0018] A first purification step is carried out at a pH of between 9 and 13 (preferably between 10 and 12, and even more preferentially about 11), preferably at least partly (and possibly all) by a membrane separation method. such as diafiltration. It is at this pH that the unreacted polyetheramine molecules (ie which have not been grafted onto the polysaccharide) are removed, probably by neutralization of the quaternary ammonium functions of the polyetheramine and elimination of the ionic bonds between the ammonium of the polyetheramine. polyetheramine and the carboxylate of the polysaccharide; the unreacted polyetheramine generally exhibits cellular toxicity which hinders the subsequent use of the hydrogel in cell culture, and which would in any case be unacceptable for the intracorporeal use of the hydrogel. A second purification step is performed after neutralization, preferably at a pH of about 7, which is generally the pH at which the hydrogel will be used later, whether in cell culture or for intracorporeal applications. This second purification step may also be made, partially or totally, by a membrane separation method such as diafiltration, or by another suitable technique. This second step at neutral pH can be done after lyophilization (the powder is then washed with ethanol to remove residues of free polyetheramines and other by-products).
    [0019] The membrane separation can be carried out in a known manner, for example with membranes having a MWCO value ("molecular weight cut-off") of about 10 kDa to 30 kDa, for example between 12 kDa to 14 kDa in coil mode. Dialysis can be done against water and / or against a mixture of water and ethanol (for example with the volume ratio: water 2/3, ethanol 1/3). There is a decrease in pH during dialysis. According to a very advantageous aspect of the invention, at least one purification step (and preferably at least all the purification steps before neutralization, and even more preferably also at least one (and preferably all) purification steps after neutralization) is (are) carried out at a temperature below 20 ° C, preferably between 0 ° C and 15 ° C, and even more preferably between 2 ° C and 8 ° C, especially at a temperature of about 4 ° C.
    [0020] Indeed, the applicant has observed that at room temperature the reaction mixture is cloudy and tends to form aggregates at room temperature which hinder the purification; however, obtaining a pure product is necessary for any intracorporeal use of the hydrogel. In contrast, the product according to the invention, purified at low temperature as indicated above, is translucent after gelation, unlike many polysaccharide hydrogels of the state of the art. The Applicant tends to think (without being bound by this theory) that the unmodified (free) polyetheramine participates in the formation of said aggregates in which it could be trapped, since the aggregates disappear after a sufficient purification of the hydrogel.
    [0021] The Applicant has found that apart from the toxicity of the residual polyetheramine (unreacted, free), there is another reason for optimally purifying the polysaccharide modified by grafting a polyetheramine: the presence of free polyetheramine in hydrogels which show a change in viscosity as a function of temperature leads to a lower viscosity gradient and spread over a wider temperature range compared to a purified hydrogel. The purified product is frozen (for example at -20 ° C.) and lyophilized, then washed with ethanol (for example twice) and dried (preferably at 40 ° C. under vacuum).
    [0022] The final product is in the form of a dry powder. It can be converted into a hydrogel by dispersing it in a desired amount of an aqueous medium. Said aqueous medium may be a cell culture medium. By way of example, the culture media known under the name RPMI (Roswell Park Memorial Institute) can be used. The aqueous medium may include additives, such as growth factors and / or pharmaceutically active ingredients (such as antibiotics), and serum. b) Useful Polysaccharides In the context of the present invention, different types of polysaccharides may be used to be modified by grafting according to method B or according to method C.
    [0023] These polysaccharides may belong to the groups of neutral polysaccharides (for example pullulan, dextran), natural anionic polysaccharides (for example: alginate, hyaluronic acid, xanthan gum, agar agar gum, pectins, heparin), synthetic anionic polysaccharides ( for example carboxymethylcellulose, carboxymethylpullunane), natural cationic polysaccharides (especially chitosan), synthetic cationic polysaccharides (for example diethylaminoethylcellulose, diethylamonithyldextran), amphiphilic polysaccharides, natural zwitterionic polysaccharides or obtained by chemical modification (for example carboxymethylchitosan).
    [0024] The polysaccharides of the pullulan, xanthan, alginate and hyaluronic acid type (the latter being abbreviated to HA) are the polysaccharides which are particularly preferred for preparing grafted polysaccharides with thermosensitive rheological properties. Cell culture tests at different concentrations show the non-toxicity of these products as well as the proliferation of cells in these systems. Moreover, these polysaccharides are biocompatible and biodegradable. By way of example, hyaluronic acid (HA), which has a well-known biocompatibility, can be used. It is possible to use a bacterial origin HA (Streptococcus equi) which is commercially available with a number-average molar mass which varies typically from 103 to more than 106 g / mol (determined by steric exclusion chromatography, mufti light diffusion). -angle and refractometry). c) Preffa rate The method according to the invention makes it possible to obtain high levels of grafting, which can reach 20 mol%. The Applicant knows no known method which allows to obtain so high grafting rates. For the use of the products as polysaccharides with thermosensitive rheological properties, a degree of grafting of between 5% and 20% by mole, preferably between 5% and 15%, and even more preferentially between 10% and 15%, is preferred. Indeed, in some grafted systems, beyond 15 to 20% the effect of thermosensitivity of the rheological properties tends to decrease. d) Choice of Polyetheramines The polyetheramines preferred in the context of the present invention (and this section "Choice of polyetheramines" relates to methods A, B and C) are polyether type copolymers composed of propylene oxide (PO) and of ethylene oxide (EO). The presence of these propylene oxides renders the macromolecule hydrophobic and thermosensitive, resulting in an aqueous solution precipitation depending on the temperature. The temperature of this transition depends inter alia on the relative amount P0 / E0. The polyetheramines used in the present invention are preferably primary amines. In general (and in particular for methods B and C) polyethermonoamines, and in particular those having the following structure: where Z1 is a hydrogen atom (in the case of ethylene oxide) are preferred or methyl (in the case of propylene oxide) and x and y indicate the length of the chains, knowing that for a given molecule, x and y are integers, but on a given product as it will be used (which may have molecules whose length may not be the same) x and y represent mean values.
    [0025] The molar mass of the polyetheramines that can be used can vary from about 300 to about 3000, and a range of between 500 and 2500 is preferred. The molar ratio of PO / EO can vary within fairly wide limits, for example between 10/1 and 1/1. 10.
    [0026] By way of example, the following polyetheramines may be used: x = 1 to 3, Z1 = CH3 and y = 7 to 11 (with x = 1 and y = 9 preferred); x = 17 to 21, Z1 = CH3 and y = 2 to 5 (with x = 19 and y = 3 preferred); x = 5 to 8, Z1 = CH3 and y = 25 to 32 (with x = 6 and y = 29 preferred).
    [0027] But it is also possible to use polyetherdiamines, and in particular those which have the following structure: or the following structure: where Z1, x and y have the meaning indicated above, and z represents, as x and y, and thus is explained above, the length of the chain. It is also possible to use polyethertriamines, and in particular those which have the following structure: where Z1, x and y have the meaning indicated above, and z represents, as x and y, and as explained above. , the length of the chain. Z2 is hydrogen or C1-C4 alkyl, preferably methyl or ethyl. The number n can range from 0 to 12, and is preferably 0, 1 or 2.
    [0028] It is possible to use, for example, the polyethermonoamines sold under the trade name Jeffamine 0 (M series), or the polyetherdiamines sold under the trade name Jeffamine 0 (D series, ED), or the polyethertriamines sold under the trade name Jeffamine 0 (T series), for example Huntsman society.
    [0029] D) Use of graft-modified polysaccharide hydrogels according to the invention The graft-modified polysaccharide hydrogels according to the invention can be used in biology and medicine, extracorporeally or intracorporeally. These hydrogels can be prepared with water or with aqueous liquids, such as: buffered aqueous solutions, physiological saline, usual or specific cell culture media.
    [0030] These uses in biology and medicine are made possible thanks to the possibility of purifying the modified polysaccharides according to the invention in a very effective manner, in order to eliminate any toxic residue. Certain uses, in particular intracorporeal, are also made possible thanks to the rheology of the modified polysaccharides according to the invention (orthopedics, cosmetology (for example, wrinkle-filling, dermatology) Extracorporeal uses include the use as a cell culture medium , in particular animals or humans, or the use in a culture medium composition of cells, in particular animal and human cells, which hydrogels can also be used in microfluidic systems, and also include use as a medium (or in a composition medium) for storing and / or transporting cells, biopsies or explants, in particular animal or human cells The hydrogels according to the invention have a three-dimensional network that accommodates the cells to be grown under conditions conducive to their growth. and multiplication Intracorporeal uses include the use of as a skin dressing, an embolizing agent, a viscosupplementation agent, a filler, a post-surgical adhesion limiting agent, a tissue regenerating agent, or in the composition of such agents. These applications make it possible in particular to take advantage of the thermosensitive properties of the hydrogel according to the invention.
    [0031] Here we describe a typical use of a modified polysaccharide hydrogel with thermosensitive rheological properties according to the invention. For use as a three-dimensional cell culture medium, the hydrogel is solubilized in the cell culture medium, and the cells are deposited in the heat-sensitive gel at room temperature. During the increase in temperature (passage to 37 ° C, temperature of the incubator) of the system, the cells will be sequestered inside the hydrogel. One of the important characteristics of the thermosensitive is its optical transparency when the system is in gel form, allowing a microscopic analysis. The cells can then develop in suspension inside the system and proliferate in this system. During a new transition at room temperature the cells can be recovered and analyzed. The thermosensitive rheological hydrogel can also be used to transport cells (strains, primers and lines) or specimens (such as biopsies) at a temperature of about 37 ° C. Indeed, these precious samples undergo shocks during the transport due to shaking and often arrive altered. The hydrogel with thermosensitive rheological properties then makes it possible to limit the impact of these shakes due to the handling of the items by sequestering the cells or samples (such as biopsies) inside the hydrogel. Once the sample has been received by the recipient, a transition at room temperature will suffice to liquefy the medium and thus easily recover the cells or samples it contains. The hydrogel with thermosensitive rheological properties can also be used in regenerative medicine, for example during the regeneration of a cartilage.
    [0032] Currently, one of the main techniques used for the regeneration of cartilage is micro fracture. The practitioner performs on a patient suffering from a grade III or IV lesion a punching of the underlying bone of the cartilage. These punctures result in a blood effusion containing stem cells. These stem cells have the ability to regenerate cartilage. However, a problem with this technique is that the cells do not always stay on the injured site and disperse. The injection of a thermosensitive rheological hydrogel loaded with blood containing stem cells (or another biological medium, enriched in stem cells or containing stem cells) during the microfracture would locate the cells on the site of lesion and promote the regeneration of cartilage.
    [0033] E) Advantages of the invention The use of modified polyetheramines according to the invention as a graft makes it possible to obtain grafted polysaccharides with new physicochemical characteristics, and in particular with a viscosity which depends on the temperature. Indeed, the use of polyetheramines according to the invention makes it possible to obtain higher grafting rates. The purification of the hydrogels at low temperature makes it possible to obtain more pure, non-toxic hydrogels without free polyetheramine. The absence of free polyetheramine also enhances the variation of viscosity as a function of temperature and narrows the temperature range in which the viscosity transition occurs. The hydrogels according to the invention may have thermosensitive rheological properties, passing from a liquid state to a state with a higher viscosity in which they constitute a three-dimensional nanostructure; in this state they can accommodate cells. They are optically transparent and thus allow the optical observation of said cells.
    [0034] Examples The following examples are given by way of illustration only, to enable those skilled in the art to carry out the invention. They do not limit the scope of the invention.
    [0035] I. Examples relating to the Synthesis of Polyetheramine Derivatives EXAMPLE 1 Modification of a Polyethermonoamine with X = 6, Z = CH 3 and Y = 29 by Chloroacetyl Chloride in the Presence of Triethylamine (TEA) a volume of 250 ml 100 g (50 mmol) of polyethermonoamine (x = 6, Z = CH3 and y = 29, product available under the trademark Jeffamine® M2005, molecular weight about 2000 g / mol) and 6.7 ml ( 50 mmol) of triethylamine (TEA). The mixture was placed in an ice bath at 4 ° C, and chloroacetyl chloride (3.96 ml, 50 mmol) was added dropwise with vigorous stirring. The reaction mixture was kept for 2 hours. After 2 hours, 100 ml of 2-propanol was added. Then the mixture was transferred to a separatory funnel, and 200 ml of water at acidic pH (pH = 3) was added. After the phase separation, the organic phase containing the modified Jeffamine® M2005 was recovered. EXAMPLE 2 Modification of a Polyethermonoamine with X = 6, Z = CH 3 and Y = 29 by Chloroacetyl Chloride in the Presence of NaOH (NaOH 250 g (50 mmol) of polyethermonoamine (x = 6, Z = CH 3 and y = 29, a product available under the trade name Jeffamine M2005) and 2 ml of a solution were introduced into a 250-ml reactor. of sodium hydroxide at 50 mmol of NaOH. The mixture was placed in an ice bath at 4 ° C, and chloroacetyl chloride (3.96 ml, 50 mmol) was added dropwise with vigorous stirring. The reaction mixture was kept for 2 hours. After 2 hours, 100 ml of 2-propanol was added. Then the mixture was transferred to a separatory funnel, and 200 ml of water at acidic pH (pH = 3) was added. After the phase separation, the organic phase containing the modified Jeffamine ® M2005 was recovered. EXAMPLE 3 Modification of a polyethermonoamine with x = 1, Z = CH 3 and y = 9 by 2-Bromo-2-methylpropionyl bromide (BIBB) in the presence of triethylamine (TEA) It was introduced into a reactor of a volume 250 ml 100 g (166 mmol) of polyethermonoamine (x = 1, Z = CH3 and y = 9, product available under the tradename Jeffamine ® M600 or XTJ-505, molecular weight about 600 g / mol) and 22.5 ml (166 mmol) triethylamine (TEA). The mixture was placed in an ice bath at 4 ° C, and 20.5 ml (166 mmol) of chloroethyl chloride was added dropwise with vigorous magnetic stirring. The mixture was kept for 2 hours. After 2 hours, 100 ml of 2-propanol was added to the reaction mixture. Then the mixture was transferred to a separatory funnel, and 200 ml of water at acidic pH (pH = 3) was added. After the phase separation, the organic phase containing the modified Jeffamine M600 was recovered. Complementary Example: According to one of the procedures described above, the following modified polyether monoamines were produced: Base polyethermonoamine: (a) Z = CH 3, x = 6, y = 29 (commercially under the trade name Jeffamine 0 M2005 ) (B) Z = CH3, x = 1, y = 9 (commercially under the trademark Jeffamine® M600) (c) Z = H (for EO) or CH3 (for PO), x = 6, y = (Jeffamine® M2070) Each of these three polyethermonoamines was modified by the reaction with: (a1, b1, cl): chlorylacetyl chloride (a2, b2, c2): α-bromoisobutyryl bromide (cl, c2, c3): 6-bromohexanoyl chloride. It has moreover been verified that these syntheses can be carried out with polyetherdiamines and polyethertriamines.
    [0036] Examples relating to the modification of polysaccharides by polyetheramine derivatives Example 4: Grafting of Jeffamine CD M2005 modified with 2-Bromo-2-methylpropionyl bromide on hyaluronic acid (HA) by the Williamson reaction. In a reactor 1 g (2.5 mmol) of HA was solubilized in 100 ml of water with mechanical stirring. The solution was heated to 70 ° C. Then 0.8 g of NaOH (0.2 mol) was dissolved in 5 ml of water, and this sodium hydroxide solution was added to the medium with 0.5 g of sodium iodide. After 15 minutes, 11 ml of the modified Jeffamine ® M2005 solution in isopropanol was added. The reaction mixture was heated at 70 ° C for 4 h, then 2 g of NaCl was added and the pH was adjusted to 11 by addition of HCl (1M). The mixture was kept at 4 ° C for 12 h. Purification was obtained by diafiltration at 4 ° C. Measurements of the UV absorbance as a function of temperature of the reaction mixture (FIG. 6) show an increase in absorbance, indicating the presence of a cloudy phase due to the formation of aggregates. This observation implies that it is not possible to purify the mixture at room temperature. To purify the reaction mixtures effectively the diafiltration system was placed at 4 ° C. The purification was carried out in 3 steps. The diafiltration was started at pH = 11 by passing 3 times the volume of the initial solution. Then the solution was neutralized to pH = 7 and the volume of the solution was 4 times. After controlling the conductivity, the diafiltration was stopped. The sample was frozen and then lyophilized. The lyophilizate was washed with absolute ethanol and finally dried under vacuum. Example 5: Grafting of Jeffamine M2005 modified with 2-Bromo-2-methylpropionyl bromide on hyaluronic acid (HA) by the esterification reaction.
    [0037] In a reactor, 1 g (2.5 mmol) of HA is solubilized in 100 ml of water with mechanical stirring. Then the pH of the solution is adjusted to 2 by addition of HCl (1M). The mixture is dialyzed against pure water for 24 hours. After dialysis the solution is neutralized to pH = 7 by the addition of tetrabutylammonium hydroxide (TBAOH). For the grafting reaction, the neutralized HA solution was heated to 70 ° C. Then, 11 ml of the modified Jeffamine 0 M2005 solution in isopropanol was added. The reaction mixture was heated at 70 ° C for 12 h. Then 2 g of NaCl was added, and the mixture was kept at 4 ° C for 12 h. The same purification method as that described for Example 4 was used. Example 6: Rheological properties of polysaccharide hydrogels as a function of temperature The elastic modulus G 'and the viscous modulus G "of different polysaccharide hydrogels as a function of temperature were measured at a concentration of 40 g / l in RPMI culture medium: Results are shown in FIGS. 7 and 8. For the unmodified HA (FIG. 7), these measurements show that the system has no thermosensitive transition (no gelation) and there is simply a decrease moduli as a function of temperature, a classic phenomenon for polymers For the HA modified using the process according to the invention (BIBB-Jeffamine M-2005 with a grafting rate of 2%) these measurements show (FIG. the system has no thermosensitive transition (no gelation), and there is simply a decrease of the modules as a function of temperature Example 7: Reversible sol-gel transition in Cell Culture Hydrogel A modified Jeffamine® type polyetheramine-modified HA hydrogel was prepared with a culture medium known as RMPI (Roswell Park Memorial Institute Medium). A clear, translucent liquid is obtained at 20 ° C., which is solid at 37 ° C., but remains clear and translucent. The solidification of the liquid is reversible.
    [0038] EXAMPLE 8 Reversible sol-gel transition of a hydrogel for cell culture A HA hydrogel grafted with a modified Jeffamine 2005 polyetheramine according to the invention was prepared by a halide acid (BIBB-Jeffamine® M-2005 with a 10% grafting) in a medium of the DMEM type ("Dulbecco / Vogt Modified Eagle's Minimal Essential Medium") buffered with 4- (2-hydroxyethyl) -1-piperazine ethanesulfonic acid (HEPES); this cell culture medium is known as HDMEM or hDMEM. A Differential Scanning Calorimetry (DSC) differential scanning thermogram was recorded at a rate of 2 ° C. min-1. This technique measures changes in enthalpy as a function of temperature. The recorded thermogram is shown in Figure 9, curve A. For comparison, the same thermogram is recorded for halide-modified Jeffamine IO (curve B) and for Jeffamine (-.) M2005 (curve C).
    [0039] An endothermic phenomenon is observed during a rise in temperature between 10 ° C and 40 ° C; it is probably the formation of hydrophobic associations. It is noted that the peaks are not at the same temperature. The comparison of the peak temperatures shows that the modification of the polyetheramine by a halide acid decreases its transition temperature (formation of hydrophobic associations) from about 29 ° C to about 18 ° C. It also shows that after grafting this modified polyetheramine on a HA type polysaccharide the system transition temperature is closer to that of the modified polyetheramine than that of the unmodified polyetheramine.
    [0040] The behavior is reversible with an exothermic phenomenon during the cooling phase of 40 ° C to 10 ° C (not shown in the graph). EXAMPLE 9 Grafting of Modified Polyethermonoamines on Various Polysaccharides Following the approaches described in the preceding examples, the following modified polysaccharides were prepared: (i) with the basic polyethermonoamine corresponding to Z = CH 3, x = 6, y = 29 (commercially under the brand name Jeffamine ® M2005) modified by the reaction with α-bromoisobutyryl bromide: - Polysaccharide = hyaluronic acid (HA) with a degree of grafting of between 2% and 21% (molar). Polysaccharide = alginate with a degree of grafting of 1% - polysaccharide = pullulan with a degree of grafting of 4% - polysaccharide = xanthan with a degree of grafting of 2% (ii) with the basic polyethermonoamine corresponding to Z = CH 3, x = 6, y = 29 (commercially under the trademark Jeffamine ® M2005) modified by the reaction with 6-bromohexanoyl chloride: - Polysaccharide = hyaluronic acid (HA) with a degree of grafting of between 2% and 10% (molar) - Polysaccharide = alginate with a degree of grafting of 5% - polysaccharide = diethylaminoethylpullulane (DEAE-pullulan) with a degree of grafting of 10% (iii) with the basic polyethermonoamine corresponding to Z = CH3, x = 1, y = 9 (commercially under the trademark Jeffamine O M600) modified by the reaction with 6-bromohexanoyl chloride: - Polysaccharide = hyaluronic acid (HA) with a grafting rate of 1% (molar) (iv) with the base polyethermonoamine corresponding to Z = H (for EO) or CH3 (for PO), x = 6, y = 35 (commercially under the trade name Jeffamine ® M2070) modified by the reaction with α-bromoisobutyryl bromide: - Polysaccharide = hyaluronic acid (HA) with a grafting rate of 18 % (molar).
    [0041] The best results for use as a hydrogel having thermosensitive rheological properties with a transition around normal body temperature (about 370) were achieved with HA grafted at 3-10 mol% with the corresponding base polyethermonoamine. at Z = H (for EO) or CH3 (for PO), x = 6, y = 35 (commercially under the trademark Jeffamine CD M2070) modified by the reaction with 6-bromohexanoyl chloride.
    权利要求:
    Claims (10)
    [0001]
    REVENDICATIONS1. A method of modifying polysaccharides, wherein: (a) reacting a polysaccharide with a modified polyetheramine of the type (X-RC (O) NH) bR '(where R' is a polyether and b = 1, 2 or 3 and X represents a halogen, preferably Cl or Br, R represents an alkyl residue, possibly substituted, or an aromatic residue, possibly substituted), in the presence of a base, preferably in the presence of water and isopropanol, (b ) the product obtained is purified in the presence of NaCl, at least in part, by a membrane separation method, said purification being carried out at a pH of between 9 and 13 (and preferably between 10 and 12); (c) the product resulting from step (b) is purified, at least in part, by a membrane separation method, said purification being carried out after neutralization at a pH of between 6 and 8 (preferably between 6.5 and 7.5), optionally after lyophilization and washing of the lyophilized product (preferably with ethanol).
    [0002]
    The process according to claim 1, wherein said polyether R 'has the following structure: (0 x Z where Z is a hydrogen atom (in the case of ethylene oxide) or a methyl (in the case of propylene oxide), and where, preferably, x = 1 to 3, Z = CH 3 and y = 7 to 11 (with x = 1 and y = 9 preferred) x = 17 to 21, Z = CH 3 and y = 2 to 5 (with x = 19 and y = 3 preferred), x = 5 to 8, Z = CH 3 and y = 25 to 32 (with x = 6 and y = 29 preferred), said polyetheramine having preferably a molar mass of between about 300 and about 3000, and even more preferably between about 500 and about 2500, and / or - said polyetheramine having a molar ratio of [propylene oxide] / [ethylene oxide] of between 10 / 1 and 1 / 10.30
    [0003]
    3. Process according to claim 2, in which at least one PS-COOH carboxylic function of the polysaccharide P.sub.S 'is activated with the aid of a quaternary amine, and then said modified polyetheramine is added.
    [0004]
    4. Method according to any one of claims 1 to 3, wherein at least one purification step, and preferably all purification steps after neutralization, is carried out at a temperature below 20 ° C, preferably between 0 ° C and 15 ° C, and even more preferably between 2 ° C and 8 ° C.
    [0005]
    5. Process according to any one of claims 1 to 4, wherein the product from step (c) is lyophilized, washed with ethanol and dried.
    [0006]
    6. Method according to any one of claims 1 to 5, wherein said polysaccharide is selected from the group consisting of neutral polysaccharides (and in particular by pullulan and dextran), natural anionic polysaccharides (and in particular: alginate, acid hyaluronic acid, xanthan gum, agar agar gum, pectins, heparin), synthetic anionic polysaccharides (and in particular: carboxymethylcellulose, carboxymethylpullunane), natural cationic polysaccharides (and especially chitosan), cationic synthetic polysaccharides (and in particular: diethylaminoethylcellulose, diethylamonithyldextran), amphiphilic polysaccharides, natural or chemically modified zwitterionic polysaccharides (and in particular carboxymethylchitosan), or mixtures of these polysaccharides, and is preferably selected from the group formed by pullulan, xanthan, alginate and hyaluronic acid.
    [0007]
    7. Modified polysaccharide obtainable by the method according to any one of claims 1 to 6.
    [0008]
    8. Hydrogel formed by at least one polysaccharide according to claim 7 and an aqueous liquid, said aqueous liquid possibly comprising serum and / or cell culture medium.
    [0009]
    9. Hydrogel according to claim 8, characterized in that it has temperature-sensitive rheological properties with a transition temperature between 33 and 39 ° C or with a transition temperature between 4 and 20 ° C.
    [0010]
    10. Use of a hydrogel according to claim 8 or 9 in a medium for cell culture or in a medium for the transport of cells.
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    同族专利:
    公开号 | 公开日
    US20170204364A1|2017-07-20|
    CA2954455A1|2016-01-14|
    AU2015287484A1|2017-02-02|
    JP2017520674A|2017-07-27|
    FR3023485B1|2016-07-01|
    WO2016005700A1|2016-01-14|
    引用文献:
    公开号 | 申请日 | 公开日 | 申请人 | 专利标题
    EP1659143A1|2003-07-28|2006-05-24|Teijin Limited|Temperature-responsive hydrogel|
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    CN105963756A|2016-06-27|2016-09-28|林春梅|Medicinal dressing and preparation method thereof|
    PL235628B1|2017-10-13|2020-09-21|Politechnika Lodzka|Method for producing low-molecular initiators for creation of star-shaped polymers|
    CN109464702B|2019-01-14|2021-02-26|浙江瑞谷生物科技有限公司|Alveolar bone repair material containing BMP-2 and preparation method and application thereof|
    CN111481734A|2020-04-28|2020-08-04|北京诺康达医药科技股份有限公司|Modified sodium alginate self-developing embolism microsphere and preparation method and application thereof|
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    FR1401564A|FR3023485B1|2014-07-11|2014-07-11|METHOD OF MODIFYING POLYSACCHARIDES BY GRAFTING POLYETHERAMINES, POLYSACCHARIDES SO MODIFIED, AND PREPARATIONS COMPRISING THEM AND HAVING RHEOLOGICAL PROPERTIES THERMOSENSITIVE|FR1401564A| FR3023485B1|2014-07-11|2014-07-11|METHOD OF MODIFYING POLYSACCHARIDES BY GRAFTING POLYETHERAMINES, POLYSACCHARIDES SO MODIFIED, AND PREPARATIONS COMPRISING THEM AND HAVING RHEOLOGICAL PROPERTIES THERMOSENSITIVE|
    PCT/FR2015/051883| WO2016005700A1|2014-07-11|2015-07-08|Method for modifying polysaccharides by grafting polyetheramines, polysaccharides thus modified and preparations comprising same and having heat-sensitive rheological properties|
    CA2954455A| CA2954455A1|2014-07-11|2015-07-08|Method for modifying polysaccharides by grafting polyetheramines, polysaccharides thus modified and preparations comprising same and having heat-sensitive rheological properties|
    AU2015287484A| AU2015287484A1|2014-07-11|2015-07-08|Method for modifying polysaccharides by grafting polyetheramines, polysaccharides thus modified and preparations comprising same and having heat-sensitive rheological properties|
    JP2017521618A| JP2017520674A|2014-07-11|2015-07-08|Method for modifying polysaccharides by grafting polyetheramine, polysaccharides modified by the method, and preparations comprising the polysaccharides and having temperature-sensitive rheological properties|
    US15/324,934| US20170204364A1|2014-07-11|2015-07-08|Method for modifying polysaccharides by grafting polyetheramines, polysaccharides thus modified and preparations comprising same and having heat-sensitive rheological properties|
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