EP2833919A1

EP2833919A1 - Microparticles and nanoparticles made up of hydrophobized polysaccharides and an alpha-cyclodextrine

Info

Publication number: EP2833919A1
Application number: EP13719892.5A
Authority: EP
Inventors: Kawthar BOUCHEMAL
Original assignee: Centre National de la Recherche Scientifique CNRS
Current assignee: Centre National de la Recherche Scientifique CNRS; Universite Paris Saclay
Priority date: 2012-04-06
Filing date: 2013-04-05
Publication date: 2015-02-11
Also published as: WO2013150193A1; US20150151005A1; FR2989001A1; US10412960B2; FR2989001B1

Abstract

The invention relates to microparticles and nanoparticles made up of hydrophobized polysaccharides and an alpha-cyclodextrine. Said microparticles and nanoparticles are obtained by means of self-combining in an aqueous medium. Said hydrophobized polysaccharide is obtained by grafting alkyl chains of fatty acids via an acylation reaction. Said microparticles and nanoparticles make up systems used to encapsulate substances of interest, in particular in the pharmaceutical field, and to target said substances for therapeutic purposes.

Description

Microparticles and nanoparticles consisting of hydrophobized polysaccharides and alpha-cyclodextrin

The invention relates to microparticles and nanoparticles consisting of hydrophobized polysaccharides and alpha-cyclodextrin.

The invention also relates to their use as an encapsulation system.

Currently, particles capable of containing and vectoring or encapsulating an active ingredient are the subject of active research. These particles must be capable of trapping a substance of interest, transporting it in the body to the target cell or tissue, and then releasing it without altering its structure. It is important that these particles are not toxic. But there is a big disadvantage related to their preparation. Indeed, it often requires, during a step at least, the use of an organic solvent and / or the use of surfactants, non-biocompatible, sometimes under very important acid conditions. The removal of the solvent and / or surfactant molecules is often long, incomplete and adds a cost to the production of the particle. The residual traces, toxic, can also contribute to degrade the active substances immobilized in the particles. This is why it is sought to produce these particles in an aqueous medium preferably, from biocompatible and biodegradable polymers.

Polysaccharides form a class of polymers very interesting in the field of encapsulation. Among these polysaccharides are chitosan, chitin, hyaluronic acid and glycosaminoglycans (GAGs).

Chitosan is a linear heteropolymer of N-acetyl-D-glucosamine and β-linked D-glucosamine (1-4) according to the formula:

in which

M represents the number of D-glucosamine units,

■ n represents the number of N-acetyl-D-glucosamine units,

provided that the percentage of m in relation to the total number of units is greater than 50%. It has the advantage of being biocompatible and mucoadhesive. Nanoparticles of chitosan have been used as adjuvants for mucosal vaccination in animals (Annales de Médecine Vétérinaire, 2003, 147, 343-350). An adjuvant is a substance that, when administered together with an antigen, increases the immune response to that antigen. The advantage of mucosal vaccination is the introduction of an immune response to the entry gate of microbes. Vaccines administered alone by mucosal route have low bioavailability. They must be co-administered with substances that promote their penetration or with adjuvants.

Chitin is a linear heteropolymer of N-acetyl-D-glucosamine and β-linked D-glucosamine (1-4) according to the formula:

in which

M represents the number of D-glucosamine units,

■ n represents the number of N-acetyl-D-glucosamine units,

provided that the percentage of m in relation to the total number of units is less than 50%.

Chitin is a powerful moisturizing agent, an effective sensor of heavy metals, responsible for a large number of contact allergies. It is used in the treatment of burns because it has healing properties. Chitin is also used to filter wastewater: it forms ionizable chains that make it possible to fix the organic elements. It is also inserted in the industrial food (juice manufacturing), as a technological auxiliary.

One of the first steps in the colonization of biotic surfaces by microbes involves their interaction with receptors located at the level of cells such as glycosaminoglycans (GAGs) including heparin, heparan sulfate, hyaluronic acid, dermatan sulfate, keratan sulfate and chondroitin sulfate. Many viruses, bacteria, fungi and parasites are able to bind to GAGs on the surface of cells, facilitating their initial attachment and then cell entry followed by infection: Evidence from the literature indicates that inhibitory effect of heparin, heparan sulfate, dermatan sulfate and chondroitin sulfate have been demonstrated on human herpes simplex virus (HSV) (Journal ofbacteriology, 1964, 87 (5), 1060-1066, Virology. 1995, 208 (2), 531-539, Journal of Virology. 1989, 63 (1), 52-58), while the binding of particles mimicking human papillomavirus (HPV) to cells was inhibited by heparin (The Journal of Biological Chemistry. 1999, 274 (9), 5810-5822). In addition, heparan sulfate has been shown to play an important role in the prevention of HPV-16 infections (Journal of Virology. 2009, 83 (5), 2067-2074).

The heparin coating of abiotic surfaces has reduced bacterial adhesion by 90% (Journal of Urology. 1987, 138, 423-426). GAGs and sulfated polysaccharides showed antibacterial activity against: Staphylococcus aureus, Gardnerella vaginalis, Mycobacterium tuberculosis, Listeria monocytogenes, Neisseria gonorrhoeae, Helicobacter pylori, Yersinia enterocolitica, Mycoplasma pneumoniae, Streptococcus mutas, Chlamydia trachomatis, Staphylococcus aureus, Escherichia coli, Pseudomonas aeruginosa. (US 2005/0203055).

The heparin coating of abiotic surfaces has reduced Candida albicans adhesion by approximately 50% (Infection and Immunity. 1993, 61 (11), 4560-4568).

US Patent 2005/0203055 has shown that cellulose sulfate has properties:

- antiviral against human immunodeficiency virus (HIV), HSV, HPV, bovine papillomavirus (BPV)

- antiparasitic against Trichomonas vaginalis,

- antifungals against Aspergillus niger and Candida albicans.

Other sulfated polysaccharides such as cellulose sulfate, carrageenan, dextran sulfate, dextrin sulfate have shown antimicrobial activity.

Hyaluronic acid helps protect the joints by increasing the viscosity of the synovial fluid and making the cartilage more elastic. Hyaluronic acid is the only non-sulfated GAG. Hyaluronic acid is a natural constituent of the dermis that plays an important role in the hydration, tone and elasticity of the skin.

Polysaccharides grafted with hydrophobic chains are amphiphilic systems capable of self-associating spontaneously in aqueous medium in the form of heart-crown type micelles capable of accommodating an active ingredient {Drug Discovery Today, 2012, 17, 623-629). But their solubility in aqueous medium decreases because of the presence of hydrophobic grafted chains.

The use of cyclic polysaccharides, such as cyclodextrins, causes the formation of particles constituting inclusion systems, soluble in aqueous medium. These systems, Variable size and structure, ranging from the nanoparticle to the hydrogel, are able to vectorize a substance of interest.

Gref et al (US2005 / 004348A1) describe particles obtained by grafting one or more (for example two) cyclic polysaccharides, such as beta-cyclodextrin, onto a biodegradable polymer such as poly (ε -caprolaetone) and their use. as vectors of active substances. In this case, the cyclic polysaccharide is covalently bound to the biodegradable polymer. This same patent describes the formation of nanoparticles by mixing a dextran bearing lauryl chains and a beta-cyclodextrin polymer.

Bochot et al (US2006 / 0188464A1, EP1590077B1, International Journal of Pharmaceuticals, 2007, 339, 121) describe, in their publication and their applications, beads whose size varies from 1 to 3 mm, obtained by mixing an oil and a solution of water. alpha-cyclodextrin. They do not use linear polysaccharides described above and, on the other hand, the size of the particles formed is millimetric.

One of the aims of the invention is to provide inclusion complexes between a polysaccharide and a cyclodextrin.

Another object of the invention is to provide microparticles or nanoparticles formed from the aforementioned inclusion complexes.

Another aim is to provide a process for the simple preparation of said particles without necessarily using organic solvents or surfactants.

In addition, the invention relates to the use of said particles as such, without necessarily adding substance (s) of interest.

The invention relates to the use of said particles to encapsulate one or more substance (s) of interest.

The invention relates to an inclusion complex formed between:

B a polysaccharide having hydrophobic groups covalently bonded to said polysaccharide,

A cyclodextrin (CD) in the form of a monomer,

the polysaccharide and the cyclodextrin being non-covalently bound.

According to another advantageous aspect, the invention relates to an inclusion complex formed by the interaction between:

A polysaccharide comprising hydrophobic groups covalently bonded to said polysaccharide,

And a cyclodextrin (CD) in the form of a monomer,

the polysaccharide and the cyclodextrin being non-covalently bound. The term "inclusion complex" refers to a system that results from the interaction of a "host" molecule that admits within its cavity one or more other "guest" molecules without any covalent linkage. established.

The term "polysaccharide" refers to a carbohydrate macromolecule formed by the linking of a large number of elemental sugars. The majority of the polysaccharides are hydrophilic, they carry -OH and / or -NH _{2 groups} , and / or -COOH, and / or -CH ₂ -OH, and / or -SO ₃ ^" , or groups derived therefrom. The nature of these groups makes it possible to differentiate them from a structural point of view and from a point of view of the physicochemical and biological properties The term "polysaccharide" refers here to a linear or branched polysaccharide.

The expression "hydrophobic group-containing polysaccharide" means that the polysaccharide has been "hydrophobized" by grafting, on -OH and / or -NH _{2 groups} , and / or -COOH, and / or -CH 2 -OH groups, and / or or -S0 ₃ ^" of alkyl chains which, by their nature, are hydrophobic because of their apolar nature.The" polysaccharide having hydrophobic groups "is therefore an amphiphilic polysaccharide.In certain conditions, these polysaccharides are capable of self-association for form heart-crown type micelles in an aqueous medium {Drug Discovery Today, 2012, 623-629).

"Cyclodextrin" (or cycloamylose) is a cyclic oligosaccharide of β-D-glucopyranose linked by α (1-4) linkages. It is a molecule-cage of natural origin that can encapsulate various molecules, including molecules of therapeutic interest. There are different sizes, each having the shape of a "lampshade". It carries hydrophilic groups (-OH) located outside, the assembly delimiting a relatively hydrophobic cavity. This amphiphilic character allows the cyclodextrin to include in its cavity hydrophobic molecules to form water-soluble inclusion complexes. Its biodegradable nature predisposes it to important applications in the food, cosmetics and pharmaceutical fields. Encapsulation in cyclodextrins makes it possible to protect fragile molecules or to ensure their slow and controlled release.

Using alpha-cyclodextrin instead of a cyclodextrin polymer is an obvious economic and regulatory advantage because this cyclodextrin is commercially available and is recognized as a pharmaceutical excipient accepted by the majority. pharmacopoeia.

The expression "Polysaccharide and cyclodextrin being non-covalently bound" means that the interactions between these two molecules are Van der Waals bonds and / or hydrogen bonds, and / or electrostatic bonds, and / or hydrophobic bonds, and not covalent bonds. These inclusion complexes are thus exclusively formed by non-covalent bonds by simple mixture of alpha-cyclodextrin and polysaccharide grafted with hydrophobic groups. Thus, using the same procedure and varying the type of these non-covalent interactions, one can form particles of varying size and structure.

The invention thus relates to an inclusion complex formed by the interaction between at least:

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin; sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and derivatives thereof, said polysaccharide having hydrophobic groups selected from alkyl groups, linear or branched, containing from 2 to 1000 carbon atoms, or linear or branched, especially linear alkenyl groups, which may contain at least 1 double bond C = C, said hydrophobic groups being covalently bound to said polysaccharide,

And an α-cyclodextrin (CD) in the form of a monomer,

the polysaccharide and the cyclodextrin being non-covalently bound.

Advantageously, in the inclusion complex according to the invention, the polysaccharide is composed of at least 3 saccharide units, its molar mass being in particular between 100 Da to 1000000 kDa, and in particular equal to 20 kDa, 145 kDa or 250 kDa.

According to another aspect, in the inclusion complex according to the invention, the polysaccharide is composed of at least 3 saccharide units, its molar mass being in particular between 5 kDa and 100,000 kDa, and in particular equal to 20 kDa, kDa or 250 kDa.

Advantageously, the ratio between the concentration of the cyclodextrin and the concentration of the polysaccharide is from 10 ^-6 to 90,000, in particular from 4 to 15, and in particular equal to 10.

According to another aspect, the ratio between the concentration of the cyclodextrin and the polysaccharide concentration is from 0.01 to 1500, in particular from 4 to 15, and especially equal to 10.

This parameter is very important because it makes it possible to modulate the size of the particles obtained from the aforementioned inclusion complexes by modifying the concentration ratio between the cyclodextrin and the polysaccharide. The average particle size may increase as the ratio of cyclodextrin concentration to polysaccharide concentration decreases.

If the ratio is less than 0.01, no particles are formed. If the ratio is greater than 20, particles are formed. Beyond a concentration ratio of 1500, and especially for a concentration greater than 50 g / L, alpha-cyclodextrin is no longer soluble in water.

The solubility of the polysaccharide is not a limiting factor in the formation of the particles, because they form even if the polysaccharide is used as a suspension in water. The fact that a suspension polysaccharide can be used to formulate the nanoparticles and the microparticles has the advantage of obtaining more concentrated particles. Thanks to this new technology, polysaccharides that were difficult to formulate in the form of nanoparticles or microparticles because of their solubility problems in water (especially chitin) thus find a new use.

Advantageously this process is simple, reduces environmental pollution because solvents, surfactants or reagents are not necessarily used. It also decreases energy consumption. It does not necessarily use a heating step if a purification step after their preparation.

Advantageously, the polysaccharides retain their antimicrobial properties even after their formulation in the form of nanoparticles and microparticles

The invention particularly relates to an inclusion complex in which the polysaccharide is selected from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, cellulose, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlane, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and their derivatives, and is especially chitosan.

They can be neutral (dextran for example), or globally positively charged (chitosan for example) or negatively (heparin, hyaluronic acid, pectin).

In a particular aspect of the invention, the polysaccharides have intrinsic properties even without adding active molecules. Chitosan has the advantage of being biocompatible, mucoadhesive and can be used as an adjunct for mucosal vaccination. Chitin has moisturizing and healing properties and has the ability to capture heavy metals and purify wastewater. GAGs and sulfated polysaccharides have activity to prevent, inhibit and / or treat fungal infections, bacterial, viral and / or parasitic on biotic or abiotic surfaces. Hyaluronic acid is known to promote hydration, tone and elasticity of the skin and to protect the joints by increasing the viscosity of the synovial fluid and making the cartilage more elastic.

These polysaccharides have the ability to prevent and inhibit biofilm formation. A biofilm is defined as an organized community of cells attached to a biotic or abiotic surface, inserted into an extracellular material. Biofilms are the predominant form of life of microorganisms and constitute a mode of resistance of these to antimicrobial agents. They can colonize biotic surfaces such as the surface of cells, tissues or organs (such as the skin and mucous membranes of the mouth, nose, eye, ear, vagina, rectum and / or the digestive tract) or abiotic surfaces such as plastic, glass, metal or any other material on which microorganisms can develop.

According to another particular embodiment, in the inclusion complex of the invention, the degree of substitution of the polysaccharide by the hydrophobic groups is from 0.001 to 100%, in particular from 0.05 to 50%.

According to another particular embodiment, in the inclusion complex of the invention, the degree of substitution of the polysaccharide by the hydrophobic groups is between 0.1% and 70%, in particular equal to 2%, 13% or 17%. .

The degree of substitution reflects the number of hydrophobic groups bound to 100 saccharide units of the polysaccharide chain. It is determined by the experimental conditions of the grafting and can be measured by nuclear magnetic resonance (RM) or by elemental analysis for example.

It is also a parameter for modulating the average size of particles formed from inclusion complexes. As the degree of substitution increases, their average size is likely to decrease or increase depending on the polysaccharide used.

According to a particular embodiment, in the inclusion complex of the invention, the hydrophobic groups are alkyl groups, linear or branched, in particular linear, containing from 2 to 1000 carbon atoms, or linear or branched alkenyl groups, in particular linear, which may contain at least one C = C double bond.

According to another particular embodiment, in the inclusion complex of the invention, the hydrophobic groups are alkyl groups, linear or branched, in particular linear, containing from 2 to 20 carbon atoms, or linear alkenyl groups or branched, especially linear, containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise. According to a particular embodiment, the hydrophobic groups are not aromatic groups.

The fatty acids used for the grafting of the hydrophobic chains on the polysaccharide are in particular lauric acid, palmitic acid, oleic acid, stearic acid, linoleic acid, this list being by no means exhaustive and limiting.

According to a particular embodiment, in the inclusion complex of the invention, the hydrophobic groups are covalently attached to the polysaccharide by a nitrogen atom of said polysaccharide.

This relates to polysaccharides having amino groups, especially chitosan and heparin.

These amino groups may undergo an N-acylation reaction by reaction with a fatty acid or a fatty acid derivative such as a fatty acid chloride or a fatty acid anhydride.

According to another particular embodiment, in the inclusion complex of the invention, the hydrophobic groups are covalently attached to the polysaccharide by one or more oxygen atoms of said polysaccharide.

According to another particular particular embodiment, in the Inclusion complex of the invention, the hydrophobic groups are covalently attached to the polysaccharide by one or more oxygen atoms of said polysaccharide, and in particular at the level of the carboxylic function COOH and / or a CH ₂ -OH group and / or -SO 3 ^"of said polysaccharide.-OH groups are numerous on polysaccharides.They react with fatty acids or fatty acid derivatives such as chlorides. acid, the acid anhydrides, to give esters. The hydrophobic group of the fatty acid or its derivative is thus grafted to the polysaccharide by one of its oxygen atoms, in the form of an acyl group: it is an "O-acylation" reaction.

The O-acylation reaction leads to the formation of easily ester-degradable ester bonds after in vivo administration.

According to another embodiment of the invention, in the inclusion complex of the invention, the hydrophobic groups are covalently attached to the polysaccharide by a nitrogen, phosphorus or sulfur atom and by atoms of oxygen of said polysaccharide in the proportions of 0.001 to 100%.

According to another embodiment of the invention, in the inclusion complex of the invention, the hydrophobic groups are covalently attached to the polysaccharide by a nitrogen, phosphorus or sulfur atom and by atoms of oxygen of said polysaccharide in the proportions of 0.5 to 20%.

When the polysaccharide contains amino groups and hydroxyl groups, by reaction with fatty acids or fatty acid derivatives such as acid chlorides, acid anhydrides, it can undergo both N-acylation and O-acylation. However, the amino groups are more reactive than the hydroxyl groups.

When methanesulphonate is used, O-acylation of chitosan is predominant.

According to another embodiment, in the inclusion complex of the invention, the cyclodextrin CD has the formula:

in which

• p is an integer equal to 6,

1 2 3

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino groups, groups; ammonium -NH ₃ , or -S0 ₄ ^" -sulphate groups, and are in particular hydrogen atoms or methyl groups, said CD being talpha-cyclodextrin (α-CD) in monomer form." Cyclodextrins "(CD ) are cyclic oligomers of β-D-glucopyranoses linked by α (1-4) linkages Three families are mainly used: α-, β- and γ-cyclodextrins respectively 6, 7 or 8 glucopyranose subunits. p = 6 corresponds to α-cyclodextrin; p = 7 corresponds to β-cyclodextrin and p = 8 corresponds to γ-cyclodextrin. They are schematized below:

Their geometry is comparable to a truncated cone delimiting a cavity at its center. It is described in Figure 15.

They are therefore caged molecules capable of accommodating molecules by inclusion, in particular species of hydrophobic nature. The size of the cavity depends on the nature of the cyclodextrin. The inner part of the cavity is hydrophobic, the outer part is hydrophilic. The -OH groups may be substituted, in particular with methyl, hydroxypropyl or sulphobutyl groups. Substitutions can increase the solubility of the cyclodextrin.

The cyclodextrin only used in the invention is Ι'α-cyclodextrin. The advantage of this cyclodextrin is related to its small size which allows it to interact with the hydrophobic chains linked to the polysaccharide.

According to a particular embodiment in the inclusion complex of the invention, the cyclodextrin is functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins, biotin or its derivatives.

The term "ligand" refers to a molecule capable of covalently binding to CD.

The ligand is chosen from protein compounds involved in particular in the recognition and / or neutralization of pathogens (anti-bodies or fragments, receptors, lectins), involved in the metabolism of fatty acids (biotin and derivatives).

According to another particular aspect, in the inclusion complex of the invention, the cyclodextrin is charged or uncharged. In yet another aspect, in the inclusion complex of the invention, the cyclodextrin is substituted or unsubstituted.

By "substituted cyclodextrin" is meant, for example, an alkyl-substituted cyclodextrin, for example a methylated cyclodextrin, a hydroxyalkyl group, a maltosyl group, a galactosyl group, or any other molecule,

According to another particular embodiment of the invention, in the inclusion complex:

The polysaccharide is a chitosan bearing hydrophobic groups,

■ the cyclodextrin is Γ a-CD.

Chitosan, a linear polysaccharide of natural origin, randomly composed of β- (1-4) linked D-glucosamine deacylated units to acetylated N-acetyl-D-glucosamine units, is produced by chemical or enzymatic deacetylation of chitin. . Chitosan is biocompatible, biodegradable. It is non-toxic, bio-adhesive because of the interaction between the positive charges in acidic medium (pH <6.0-6.5) carried by the amine functions and the negative charges carried by the biological membranes. It also has antibacterial and anti viral activity.

Chitosan is soluble in an aqueous solution of acetic acid in low concentration by protonation of the amino groups present. The glucoside chain of chitosan is essentially hydrophilic. But it is possible to graft groups, in particular hydrophobic groups, on the amino and hydroxyl groups. The polysaccharide then becomes amphiphilic and can form micelles, nanoparticles but also hydrogels at higher concentration by self-association in an aqueous medium. It is therefore possible to encapsulate active ingredients in the objects it forms. It can be used to encapsulate active ingredients (paclitaxel, ibuprofen, ...).

According to another embodiment, in the inclusion complex of the invention, the chitosan carries hydrophobic groups grafted at certain nitrogen atoms and has the formula:

in which

"M represents the number of units of desacetylated units, N represents the number of units of acetylated units,

provided that the degree of deacetylation (DDA) representing the percentage of m in relation to the total number of units is greater than 50%,

R ⁴ represents the hydrophobic group and is chosen from:

an alkyl group, linear or branched, containing from 1 to 20 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH 3 or - (CH ₂ ) ₁₆ -C] ¾,

A linear or branched alkenyl group containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₂ ) ₇ -CH3 or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ .

According to another embodiment, in the inclusion complex of the invention, the chitosan carries hydrophobic groups grafted at certain nitrogen atoms and has the formula

in which

M represents the number of units of D-glucosamine units,

N represents the number of units of N-acetyl-D-glucosamine units,

R ⁴ represents the hydrophobic group and is chosen from:

A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH ₃ or - (CH ₂ ) ₁₆ -CH ₃ ,

n a linear or branched alkenyl group containing 2 to 1000 carbon atoms and containing at least one C doubleC double bond, especially the groups - (C¾) ₇ - CH =CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ .

The 50% DDA is the limit between chitin and chitosan: when the DDA is less than 50%, it is called chitin, otherwise it is called chitosan.

The - (CH ₂ ) ₁₄ -CH _{3 group} comes from palmitic acid, - (CH) ₁₆ -CH ₃ comes from stearic acid, - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ₇ -CH _{3 is} derived from linoleic acid, - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH _{3 is} derived from oleic acid. The N-acylated chitosan is obtained from an N-acylation reaction in the presence of a coupling agent, EDCI (1-ethyl-3- (3-dimethylaminopropyl) carbodiimide), which reacts with the groups carboxylic acids of the fatty acid (oleic or palmitic for example) to form an intermediate ester capable of binding to the free amino functions of chitosan (Lee, KY, et al., Structural Determination and Interior Polarity of Self-Aggregate Prepared from Deoxycholic Acid-Modified Chitosan in Water., Macromolecules, 1998, 31, 2, 378-383). The following diagram shows the sequence of reactions carried out to obtain an N-acylated chitosan, grafted with chains derived from oleic acid. We proceed in the same way with other fatty acids such as palmitic acid for example.

Scheme: N-acylation of chitosan by oleic acid in the presence of EDCI.

The IR and NMR spectra of the grafted chitosan make it possible to demonstrate the secondary amino function obtained after N-acylation and the presence of the grafted alkyl chains.

According to another embodiment of the invention, in the inclusion complex, the chitosan carries hydrophobic groups grafted at oxygen atoms from -OH groups and / or -CH ₂ OH groups attached to the ring. chitosan, and having the formula:

wherein n, m and R have the meanings given above.

in which

■ R represents

a hydrogen atom, or

a group of formula

in which n, m and R have the meanings given above, and provided that R

represents at least one group of formula

In "Biomacromolecules 2002, 5, 1126-1128", Sashiwa et al. describe the one-pot reaction of O-acylation of chitosan. Methylsulfonate, MeSO ₃ H, makes it possible to protect the N¾ of the N-acylation to give predominantly compounds grafted at the oxygen atoms of chitosan, and more particularly at the level of the primary -OH function of chitosan (-CH ₂ OH).

The infrared (IR) spectra of the products obtained show a characteristic band of an ester bond at 1700 cm ^-1 , while the proton MR spectra compared to that of the native chitosan make it possible to establish the presence of the alkyl chains.

According to another particular embodiment, in the inclusion complex of the invention, the chitosan carries hydrophobic groups grafted at certain oxygen atoms and certain nitrogen atoms, and has the formula:

in which

wherein n, m and R ⁴ have the meanings given above.

in which

■ R represents

a hydrogen atom, or • a group of formula

in which n, m and R ⁴ have the meanings defined above, and subject to

represents at least one group of formula

According to yet another embodiment, in the inclusion complex

The polysaccharide is a dextran bearing hydrophobic groups, attached by oxygen atoms of said dextran and containing groups of formula

in which

p R ⁴ has the meanings indicated above,

α * represents dextran,

■ the cyclodextrin is Γ a-CD.

Dextran is a dextrose polymer.

The IR spectrum of O-palmitoyl-dextran shows an absorption band corresponding to the carbonyl ester group.

According to another embodiment, in the inclusion complex

The polysaccharide is hyaluronic acid bearing hydrophobic groups, attached by oxygen atoms of said hyaluronic acid and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents hyaluronic acid,

Cyclodextrin is a-CD.

According to yet another embodiment, in the inclusion complex of the invention

The polysaccharide is an amylopectin bearing hydrophobic groups attached by oxygen atoms of said amylopectin and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents hyaluronic acid,

■ the cyclodextrin is Γ a-CD.

By comparison of the IR spectra of O-palmitoyl amylopectin and native amylopectin, the presence of the ester group carbonyl in the product obtained is established.

According to another embodiment, in the inclusion complex of the invention

The polysaccharide is a pullulan bearing hydrophobic groups attached to the oxygen atoms of said pullulan and resenting groups of formula

in which

n R ⁴ has the meanings given above,

α * represents pullulan,

Cyclodextrin is a-CD.

Pullulan consists of maltotriose units. The three units of glucose that make up maltotriose are linked by a saccharide bond of the α-1,4 type, while the maltotrioses are connected to each other by osidic bonds of the α-1,6 type. It is grafted, in particular by palmitic acid.

By comparison of the IR spectra of O-palmitoyl-pullulan and native pullulan, the presence of the ester carbonyl in the product obtained is established.

According to another embodiment, in the inclusion complex of the invention

The polysaccharide is a heparin carrying hydrophobic groups fixed by nitrogen atoms of said heparin and containing groups of formula

in which

° R ⁴ has the meanings given above,

0 * represents heparin, Or the polysaccharide is a heparin bearing hydrophobic groups attached by oxygen atoms of said heparin, these oxygens possibly originating from the hydroxyl or carboxyl groups of heparin, and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents heparin,

■ and the cyclodextrin is the ct-CD.

According to another advantageous aspect, in the inclusion complex of the invention, the polysaccharide is a carrageenan carrying hydrophobic groups fixed by nitrogen atoms of said sulfate carrageenan and containing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents carrageenan,

Or the polysaccharide is a carrageenan bearing hydrophobic groups attached by oxygen atoms of said carrageenan, these oxygens possibly originating from hydroxyl or carboxyl groups of carrageenan, and representing groups of formula

in which

° R ⁴ has the meanings given above,

D * represents carrageenan,

■ and the cyclodextrin is Γ a-CD.

According to another advantageous aspect, in the inclusion complex of the invention

The polysaccharide is a hyaluronic acid bearing hydrophobic groups attached by nitrogen atoms of said hyaluronic acid and representing groups of formula in which

° R ⁴ has the meanings given above,

* * Represents hyaluronic acid,

Or the polysaccharide is a hyaluronic acid bearing hydrophobic groups attached by oxygen atoms of said hyaluronic acid, these oxygens possibly originating from the hydroxyl or carboxyl groups of hyaluronic acid, and representing groups of formula

in which

° R ⁴ has the meanings given above,

α * represents hyaluronic acid,

■ and the cyclodextrin is Γ a-CD.

The polysaccharide is a glycosaminoglycan bearing hydrophobic groups attached by nitrogen atoms of said glycosaminoglycan and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents glycosaminoglycan,

Or the polysaccharide is a glycosaminoglycan bearing hydrophobic groups attached by oxygen atoms of said glycosaminoglycan, these oxygens possibly originating from hydroxyl or carboxyl groups of glycosaminoglycan, and representing groups of formula

in which

n R ⁴ has the meanings given above,

0 * represents glycosaminoglycan,

■ and the cyclodextrin is Γ a-CD.

According to another advantageous aspect, in the inclusion complex of the invention The polysaccharide is a carrageenan sulfate bearing hydrophobic groups attached by nitrogen atoms of said carrageenan sulfate and representing groups of formula

in which

^D R ⁴ has the meanings given above,

a * represents carrageenan sulfate,

Or the polysaccharide is a carrageenan sulfate bearing hydrophobic groups attached by oxygen atoms of said carrageenan sulfate, these oxygens possibly originating from hydroxyl or carboxyl groups of carrageenan sulfate, and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents carrageenan sulfate,

■ and the cyclodextrin is Γ a-CD.

The polysaccharide is a dextran sulphate carrying hydrophobic groups attached by nitrogen atoms of said dextran sulphate and containing groups of formula

in which

α R ⁴ has the meanings indicated above,

n * represents the. dextran sulfate,

Or the polysaccharide is a dextran sulfate bearing hydrophobic groups attached by oxygen atoms of said dextran sulfate, these oxygens possibly coming from hydroxyl or carboxyl groups of dextran sulfate, and representing groups of formula in which

° R ⁴ has the meanings given above,

* * Represents dextran sulfate,

■ and the cyclodextrin is Γ a-CD.

The polysaccharide is a sulfate cellulose carrying hydrophobic groups attached by nitrogen atoms of said cellulose sulphate and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents cellulose sulfate,

Or the polysaccharide is a cellulose sulfate carrying hydrophobic groups attached by oxygen atoms of said cellulose sulfate, these oxygens possibly originating from hydroxyl or carboxyl groups of cellulose sulfate, and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents cellulose sulfate,

■ and the cyclodextrin is Γ a-CD.

The polysaccharide is a heparan sulphate carrying hydrophobic groups attached by nitrogens of nitrate representing groups of formula

in which

α R ⁴ has the meanings indicated above,

* * Represents heparan sulfate,

Or the polysaccharide is a heparan sulfate bearing hydrophobic groups attached by oxygen atoms of said heparan sulfate, these oxygens being able to from the hydroxyl or carboxyl groups of heparan sulfate, and representing groups of formula

in which

^D R ⁴ has the meanings given above,

* * Represents heparan sulfate,

■ and the cyclodextrin is Γ a-CD.

The polysaccharide is a keratan sulfate bearing hydrophobic groups fixed by nitrogen atoms of said keratan ulfate and representing groups of formula

in which

° R ⁴ has the meanings given above,

* * Represents keratan sulfate,

Or the polysaccharide is a keratan sulfate bearing hydrophobic groups attached by oxygen atoms of said keratan sulfate, these oxygens possibly coming from hydroxyl or carboxyl groups of keratan sulfate, and representing groups of formula

in which

^D R ⁴ has the meanings given above,

n * represents keratan sulfate,

■ and the cyclodextrin is the a-CD.

The polysaccharide is a chondroitin sulfate bearing hydrophobic groups attached by nitrogen atoms of said chondroitin sulfate and representing groups of formula in which

^D R ⁴ has the meanings given above,

* * Represents chondroitin sulfate,

Or the polysaccharide is a chondroitin sulfate bearing hydrophobic groups attached by oxygen atoms of said chondroitin sulfate, these oxygens possibly originating from hydroxyl or carboxyl groups of chondroitin sulfate, and representing groups of formula

in which

n R ⁴ has the meanings given above,

n * represents chondroitin sulfate,

■ and the cyclodextrin is Γ -CD.

The polysaccharide is a sulfate dextrin carrying hydrophobic groups attached by nitrogen atoms of said sulfate dextrin and containing groups of the formula

in which

° R ⁴ has the meanings given above,

* * Represents dextrin sulfate,

Or the polysaccharide is a sulfate dextrin carrying hydrophobic groups attached by oxygen atoms of said sulfate dextrin, these oxygens possibly originating from hydroxyl or carboxyl groups of dextrin sulfate, and representing groups of formula

in which

° R ⁴ has the meanings given above,

0 * represents dextrin sulfate,

■ and the cyclodextrin is Γ a-CD. According to an advantageous embodiment, the invention also relates to a particle of size ranging from 10 nm to 100,000 nm containing inclusion complexes formed by the interaction between at least

A polysaccharide comprising hydrophobic groups covalently bonded to said polysaccharide, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives,

A cyclodextrin in the form of a monomer, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives.

The invention also relates to a particle of size ranging from 50 nm to 10,000 nm containing inclusion complexes between:

And a cyclodextrin in the form of a monomer, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives.

According to an advantageous embodiment, the invention relates to nanometric particles, ranging in size from 10 nm to 1000 nm and micrometric particles of size ranging from

1000 nm to 100000 nm.

The invention relates to nanoscale particles having a size of from 50 nm to 1000 nm and micrometric particles ranging in size from 1000 nm to 10000 nm.

According to one advantageous aspect, the invention relates to a particle of

10 nm to 100000 nm containing inclusion complexes according to the invention formed by interaction between at least:

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, puUulane, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinane, polymannuronic acid, and derivatives thereof, comprising hydrophobic groups selected from linear or branched alkyl groups or linear or branched alkenyl groups and carrying from 1 to 4 double bonds C = C, conjugated or otherwise, said groups hydrophobic agents being covalently bonded to said polysaccharide, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives,

And a monomeric α-cyclodextrin, optionally functionalized with a ligand selected from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives.

The sizes of the particles formed were evaluated by quasi-elastic light scattering (DQEL) on the one hand and by transmission electron microscopy (TEM) on the other hand.

Size plays a very important role regarding the amount of encapsulated active ingredient, the applications envisaged, and the route of administration of the active ingredient.

The invention also relates to a particle of size ranging from 10 nm to 100000 nm containing inclusion complexes formed by the interaction between at least:

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinane, polymannuronic acid, and derivatives thereof, comprising hydrophobic groups selected from alkyl groups, linear or branched, containing from 2 to 1000 carbon atoms, or linear or branched, especially linear alkenyl groups, which may contain at least least 1 C = C double bond, said hydrophobic groups being covalently bonded to said polysaccharide, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins and u biotin or its derivatives,

And an α-cyclodextrin in the form of a monomer, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives.

According to a particular embodiment, the invention also relates to particles of size ranging from 10 nm to 100000 nm containing inclusion complexes formed by the interaction between:

A mixture of at least two polysaccharides chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlane, xylan, acid polyguluronic acid, xanthan, arabinan, polymannuronic acid, and derivatives thereof, comprising hydrophobic groups chosen from linear or branched alkyl groups containing from 2 to 1000 carbon atoms, or linear or branched alkenyl groups, in particular linear, which may contain at least one C = C double bond, said hydrophobic groups being covalently bonded to said polysaccharide, optionally functionalized with a ligand selected from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives,

And at least one α-cyclodextrin in the form of a monomer, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives.

The invention also relates to an encapsulation system containing one or more previously defined particles, and a substance used for its properties in the pharmaceutical, paramedical, medical device, animal feed, agrochemical, medical, cosmetic and veterinary fields. agri-foodstuffs, pesticides, cosmetic textiles, perfumery, the environment (eg water pollution control) or in the paint, building and / or automobile industry.

A medical device is an instrument, apparatus, equipment or software for use in humans or animals for the purposes of: diagnosis, prevention, control, treatment or mitigation of disease , diagnosis, control, treatment, mitigation or compensation of injury or disability, study or replacement or modification of anatomy or physiological process, mastery of conception .

According to an advantageous aspect, the substance has pharmaceutical properties and is chosen from inorganic compounds and organic, synthetic or natural compounds.

The encapsulation system previously defined according to the invention can be used to prepare appropriate compositions in the pharmaceutical, medical, paramedical, medical device, animal feed, cosmetic, veterinary, food, pesticide, cosmeto-textile, perfumery, environmental (eg water pollution control) or in the paint, packaging, building and / or automobile industry.

The encapsulated substance may possess pharmaceutical properties and be an active ingredient for therapeutic use. It may belong to the following list, the latter being in no way limiting, to the group of compounds with vitamin properties, in particular vitamin A, vitamin E, vitamin C, vitamin K, vitamin B, vitamin D , antitumor agents, in particular paclitaxel, docetaxel, tamoxifen, doxorubicin, painkillers, in particular paracetamol, anti-inflammatories, in particular diclofenac, ibuprofen, ketoprofen, antibiotics, in particular penicillins, tetracyclines and antifungals, in particular ketoconazole, clotrimazole, nystatin, chlorhexidine and its derivatives, antiparasitic agents, in particular albendazole, metronidazole, enzymatic agents, in particular alkaline phosphatase, acetylcholinesterase, alcohol dehydrogenase, hormonal agents, in particular testosterone, levonorgestrel, anxiolytics, especially benzodiazepines, antidiabetic drugs, especially glicabide, antihypertensives, especially nifedipine, or vaccines, antivirals, in particular ΑΖΤ, analgesics or combinations of analgesics, especially paracetamol antiepileptics including barbiturates and derivatives, local and general anesthetics including Atropine, but also s hypnotics, sedatives, antipsychotics, neuroleptics, antidepressants, anxiolytics, especially antagonists, neuronal blocking agents, anticholinergics, cholinomimetics, antimuscarinics, muscarinics, especially, antiadrenergic, antiarrhythmic, antiarthritic, antiasthmatic, anticonvulsant, antihistamine, anti-nausea, antineoplastic, antipyretic, antipruriginals, antispasmsdiuretics, vasodilators, central nervous system stimulants, including cough and cold preparations, decongestants, bone growth stimulants, bone resorption inhibitors, immunosuppressants, muscle relaxants, psychostimulants, sedatives, tranquillizers, proteins, peptides or their fragments, said proteins, peptides or fragments being natural, recombinant or produced by chemical means, nucleic acids (ribonucleotides or deoxyribonucleotides), in particular single and double-stranded molecules, gene constructs, expression vectors, antisense molecules and the like.

This substance for therapeutic use can be used in humans and animals.

The encapsulated substance may also have cosmetic properties and belong to the group of compounds with anti-inflammatory, anti-aging, anti-ultraviolet (anti-UV), depigmenting, healing, moisturizing, fragrancing, deodorizing, antibacterial, antiperspirant, cleansing, coloring, conservative.

In a particular encapsulation system, the substance has food properties and belongs to the group of compounds with vitamin, enzymatic and sweetening properties. It can also be an essential oil, a dye, a preservative, an antioxidant, a probiotic.

Some molecules or families of molecules that can be encapsulated are: molsidomine, ketoconazole, gliclazide, diclofenac, levonorgestrel, paclitaxel, docetaxel, tamoxifen, hydrocortisone, pancratistatin, ketoprofen, diazepam, ibuprofen, nifedipine, testosterone, tamoxifen, furosemide, tolbutamide, chloramphenicol, benzodiazepines, naproxen, dexamethasone, diflunisal, anadamide, pilocarpine, daunorubicin, doxorubicin, essential oils, terpenes, terpenoids.

To improve the solubility of the molecules of interest, it is possible to use a solvent or a mixture of solvents, especially: alkyl acetate (ethyl acetate, butyl acetate, methyl acetate), acetone, acetonitrile, acetic acid, methanoic acid, ammonia, acetic anhydride, aniline, anisole, benzene, butanol, butanone, chlorobenzene, chloroform, cyclohexane, cyclopentane, dichloroethane, dichloromethane, diisopropyl ether, dimethylformamide, dimethylsulfoxide, dioxane, water, ethanol, glycol ether, diethyl ether, ethylene glycol, heptane, hexamethylphosphoramide, hexane, methanol, methyl ethyl ketone, nitrobenzene, pentane, percgloroethylene, propanol, propoxypropane, pyridine, carbon disulfide, tetrachloroethane, tetrahydrofuran, toluene, trichloroethane, trichlorethylene, tremethylpentane, xylene.

The fields of use of the compositions containing the encapsulation system with the active ingredient are therefore the medical, veterinary, cosmetic, cosmeto-textile, the environmental field particularly related to the depollution of water, the field of paints, building or the automobile, perfumery.

The invention also relates to the use of previously defined particles. The invention thus relates to the use of said particles as medicaments, especially as adjuvants for vaccination, treatment of burns, and / or for cicatrization. The invention also relates to the use of said particles in the preparation of medicaments having at least one activity for preventing, inhibiting and / or treating fungal, bacterial, viral and / or parasitic infections on biotic or abiotic surfaces. The invention also relates to the use of said particles as veterinary medicaments, especially as adjuvants for vaccination.

The invention also relates to the use of particles as a cosmetic agent, especially as an anti-aging agent, depigmenting, healing, moisturizing, perfuming, deodorant, antiperspirant, cleanser, dye, preservative.

The invention also relates to the use of particles for the implementation of a method for preparing devices, in particular healing dressings, said devices comprising said particles, and being capable of releasing said particles or one or more substance (s) active (s) of interest contained in said particles.

The invention also relates to a pharmaceutical composition containing as active substance the substance encapsulated in the particles, in solid form, or in the form of solution or suspension in a physiological medium, optionally enriched with an excipient such as glucose, sucrose or any other pharmaceutically acceptable excipient, usable for the routes:

parenteral, oral, cutaneous, subcutaneous, nasal, pulmonary or ocular and, for any mucosal administration, or at a specific site (tumor, light of certain blood vessels),

in the form of pills (tablets), soft capsules, hard capsules (capsules), powders, granules, soluble or dispersible tablets, patch, implant, suppositories, solutions, suspension, syrup, pastes, creams, gels, emulsions, sprays, lotions, ointments, shampoos.

The invention also relates to a pharmaceutical composition containing as active substance a substance encapsulated in inclusion complexes or in particles defined above, in association with a pharmaceutically acceptable vehicle, in solid form, or in the form of a solution or suspension. in a physiological medium, usable by the ways:

parenteral, oral, dermal, subcutaneous, nasal, pulmonary or ocular and, for any mucosal administration, especially in the form of pills (tablets), soft capsules, hard capsules (capsules), powders, granules, tablets soluble or dispersible, patch, implant, suppositories, solutions, suspension, syrup, pastes, creams, gels, emulsions, sprays, lotions, or ointments.

Advantageous forms in the pharmaceutical field are tablets, soft capsules, hard capsules (capsules), powders, granules, patches, implants, suppositories, solutions, suspensions, syrups, pastes, creams, gels, emulsions, sprays, lotions and ointments.

Advantageous forms in the paramedical field are dressings, catheters, compress, gauze, hydrophilic cotton, physiological saline, spray, etc.

Advantageous forms in the field of medical devices are implants, prostheses, instrument washer-disinfectors, compresses, dressings (especially healing), sprays, gauzes, hydrophilic cotton, etc.

Advantageous forms in the veterinary field are the oral forms (tablets, powders, soft capsules, hard capsules (capsules), granules, pastes, solutions, suspensions), injectables (solutions, suspensions) and topical agents, the action of which may be local or systemic (spray, necklaces, ear loops, powders, lotions, ointments, shampoos, patch, emulsions, milk, gel, cream).

Advantageous forms in the food field are solutions, emulsions, pastes, gels, powders used alone or included in food preparations; in the field of food supplements: mainly oral forms (powders, tablets, capsules, granules, soft capsules or hard capsules (capsules), pastes, solutions, suspensions, infusions).

The invention also relates to a cosmetic composition containing as active substance the substance encapsulated in the particles, and containing cosmetically acceptable excipients, usable in the form of gels, pastes, ointments, lotions, creams, milks, sticks, shampoos, powders, aerosols, patches.

The invention also relates to a process for preparing an inclusion complex comprising a mixing step:

A polysaccharide comprising hydrophobic groups covalently bound by a nitrogen atom or by one or more oxygen atoms to said polysaccharide,

And a cyclodextrin (CD) in monomeric form,

to obtain an inclusion complex in which said polysaccharide and cyclodextrin are non-covalently bound.

According to a particular embodiment, the process for preparing the invention of an inclusion complex comprises a mixing step:

A polysaccharide comprising hydrophobic groups covalently bound to the polysaccharide by a nitrogen atom of said polysaccharide,

And a cyclodextrin (CD) in monomeric form,

According to one particular embodiment, the method for preparing the invention of an inclusion complex comprises a step of mixing at least:

A polysaccharide comprising hydrophobic groups covalently bound to the polysaccharide by a nitrogen atom of said polysaccharide, and

A cyclodextrin (CD) in the form of a monomer,

The invention also relates to a method for preparing an inclusion complex as defined above, comprising a mixing step of at least

A polysaccharide in the form of a suspension in a solvent, especially water comprising hydrophobic groups covalently bound to the polysaccharide by oxygen atoms of said polysaccharide, and

An α-cyclodextrin (CD) in the form of a monomer, to obtain an inclusion complex in which said polysaccharide and cyclodextrin are non-covalently bound,

and in particular comprising a mixing step:

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and their derivatives,

said polysaccharide having hydrophobic groups of formula:

in which

* represents the polysaccharide,

R ⁴ represents

A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₄ -CH ₃ or - (CH ₂ ) ₁₆ -CH ₃ ,

• a linear or branched alkenyl group containing from 2 to 1000 carbon atoms and having at least one double bond C = C, such as - (CH ₂₎ ₇ - CH = CH-CH ₂ - (CH ₂₎ ₇ -CH ₃ or - (CH ₂ ) 7-CH = CH- (CH ₂ ) ₇ -CH ₃ ,

And an α-cyclodextrin (CD) having the formula:

in which

P is equal to 6,

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - NH ₃ , or sulfate groups --SO4 and are especially hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form, to obtain an inclusion complex in which said polysaccharide and cyclodextrin are non-covalently bound.

In another aspect, the invention also relates to a process for preparing an inclusion complex as defined above, comprising a step of mixing at least:

A polysaccharide comprising hydrophobic groups covalently bound to the polysaccharide by oxygen atoms of said polysaccharide, and

An α-cyclodextrin (CD) in the form of a monomer suspended in a solvent, in particular water,

to obtain an inclusion complex in which said polysaccharide and cyclodextrin are non-covalently bound,

and in particular comprising a mixing step:

said polysaccharide having hydrophobic groups of formula:

in which

- * represents the polysaccharide,

- R ⁴ represents

"A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least 1 C = C double bond, in particular the groups - (CH ₂ ) ₇ - CH = CH-CH ₂ - (CH ₂ ) ₇ -CH" ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ , and

An α-cyclodextrin (CD) having the formula:

in which

P is equal to 6,

1 2 3 * *

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - NH ₃ ⁺ , or sulphate -SO ^{2 -} groups, and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

In yet another particular embodiment, the invention also relates to a process for preparing an inclusion complex as defined above, comprising a step of mixing at least:

A polysaccharide in the form of a suspension in a solvent, in particular water comprising hydrophobic groups covalently bound to the polysaccharide by oxygen atoms of said polysaccharide,

H and an α-cyclodextrin (CD) in monomeric form, preferably in suspension in a solvent, in particular water,

and in particular comprising a mixing step:

said polysaccharide having hydrophobic roups of formula:

in which

- ^· * represents the polysaccharide,

- R ⁴ represents A linear or branched alkyl group containing from 1 to 1000 carbon atoms, especially the groups - (CH ₂ ) 14 -CH ₃ or - (CH ₂ ) ₁₆ -CH ₃ ,

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least one C = C double bond, in particular the groups - (CH ₂ ) --CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ , and

An α-cyclodextrin (CD) having the formula:

in which

P is equal to 6,

1 2 3

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, chosen from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - NH ₃ ⁺ , or sulfate groups -SO ₄ ^2- , and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

According to another embodiment, the process for preparing an inclusion complex comprises a mixing step

A polysaccharide comprising hydrophobic groups covalently bound to the polysaccharide by oxygen atoms of said polysaccharide,

And a cyclodextrin (CD) in monomeric form,

According to another advantageous aspect of the invention, the process for preparing an inclusion complex comprises a step of mixing at least:

And a cyclodextrin (CD) in the form of a monomer,

to obtain an inclusion complex in which said polysaccharide and cyclodextrin are non-covalently bound. The invention also relates to a method for preparing an inclusion complex comprising a mixing step:

A chitosan comprising hydrophobic groups covalently attached to chitosan by one or more oxygen atoms of said chitosan,

■ and an α-cyclodextrin (CD),

and in particular comprising a step of mixing a chitosan of formula I:

or a chitosan of formu

in which

M represents the number of units of D-glucosamine units,

N represents the number of units of N-acetyl-D-glucosamine units,

provided that the degree of deacetylation representing the percentage of m in relation to the total number of units is greater than 50%,

R ⁴ represents a hydrophobic group and is chosen from:

a linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₄ -CH ₃ or - (CH ₂ ) ₁₆ -CH _3;

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₂ ) 7-CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

► and an α-cyclodextrin (CD) of formula:

in which

P is equal to 6,

R ¹ , R ² and R ³ , identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino groups -NH ₂ , ammonium groups - NH ₃ ⁺ , or sulfate groups -SO ₄ ^" , and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

at a concentration of from 0.01 to 9000 g / l of aqueous medium, in particular of from 1 to 300 g / l of aqueous medium, and in particular of approximately 200 g / l of aqueous medium, to obtain a complex of inclusion in which the chitosan of formula I and the cyclodextrin are non-covalently bound.

According to one particular embodiment, the process for preparing an inclusion complex comprises a mixing step:

A plurality of polysaccharides comprising hydrophobic groups covalently attached to said polysaccharides by a nitrogen atom and / or by one or more oxygen atoms of said polysaccharides, the polysaccharides being chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and their derivatives,

■ a cyclodextrin (CD),

to obtain an inclusion complex in which the polysaccharides and the cyclodextrin are non-covalently bound. The use of several polysaccharides may have the advantage of modulating the properties of the particles by modifying the ratio between the polysaccharides. Thus, it is expected that the size, overall charge and target applications of these particles may be modulated.

According to a particular embodiment, the process for preparing an inclusion complex comprises a mixing step: A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, puUulane, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlane, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and their derivatives, and is especially chitosan, said polysaccharide comprising hydrophobic groups of formula:

in which

■ * represents the polysaccharide,

■ R ⁴ represents:

An alkyl group, linear or branched, containing from 1 to 20 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH ₃ or - (CH ₂ ) ₆ -CH ₃ ,

A linear or branched alkenyl group containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ , and

A cyclodextrin (CD) having the formula:

in which

· P is an integer equal to 6,

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - NH ₃ , or sulfate groups -SO ₄ and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

to obtain an inclusion complex in which said polysaccharide and cyclodextrin are non-covalently bound. According to a particular embodiment, the process for preparing an inclusion complex comprises a mixing step of at least

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, puUulane, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinane, polymannuronic acid, and their derivatives, and is especially chitosan, said polysaccharide comprising hydrophobic groups of formula:

in which

■ * represents the polysaccharide,

■ R ⁴ represents:

A linear or branched alkyl group containing from 1 to 20 carbon atoms, in particular the groups - (CH ₂ ) ₄ -CH ₃ or - (CH ₂ ) ₁₆ -CH 3,

A linear or branched alkenyl group containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

a cyclodextrin (CD) having the formula:

in which

• p is an integer equal to 6,

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - N¾, or sulfate groups -SO ₄ ^' , and are in particular hydrogen atoms or methyl groups,

According to one particular aspect, the process for preparing an inclusion complex comprises a step of mixing the polysaccharide:

In aqueous solution at a concentration of from 0.01 to 9000 g / l, in particular of from 1 to 600 g / l, and in particular approximately equal to 10 g / l, the aqueous solvent being chosen from pure water, an aqueous solution of pH ranging from 1 to 7 or 7 to 14, in particular from 5 to 7, or a physiological saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, medical, paramedical, medical devices, food animal, cosmetic, veterinary, agri-food, pesticides, cosmeto-textiles, perfumery, environmental (eg water pollution control) or in the paint, packaging, building and / or automotive industry .

Or in dispersion in an aqueous medium chosen from pure water, an aqueous solution of pH of from 1 to 7 or 7 to 14, in particular of from 5 to 7, or a saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, medical, paramedical, medical devices, animal nutrition, cosmetics, veterinary, agri-food, pesticides, cosmeto-textiles, perfumery, environmental (eg water depollution) or in the industry paintings, packaging, building and / or automobile,

with a cyclodextrin, Γα-CD.

The process for preparing an inclusion complex comprises a step of mixing the polysaccharide

In aqueous solution at a concentration of from 1 to 150 g / l, in particular of from 5 to 50 g / l, and in particular approximately equal to 10 g / l, the aqueous solvent being chosen from pure water, a solution of aqueous pH ranging from 1 to 7 or 7 to 12, in particular from 5 to 7, or a physiological saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, cosmetic, agri-food or veterinary use,

Or in dispersion in an aqueous medium chosen from pure water, an aqueous solution of pH ranging from 1 to 7 or from 7 to 12, in particular from 5 to 7, or a saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, cosmetic, agri-food or veterinary use,

with a cyclodextrin, Γα-CD. In the process for preparing an inclusion complex, the step of mixing the polysaccharide in aqueous solution or dispersion is carried out at a concentration of from 0.01 to 9000 g / l, in particular from 1 to 600 g / l. L, and in particular approximately equal to 10 g / l, with a cyclodextrin, especially Ι'α-CD, at a concentration of from 0.01 to 9000 g / l, in particular of from 1 to 300 g / l, and in particular about 200 g / L.

In the process for preparing an inclusion complex, the step of mixing the polysaccharide in aqueous solution or dispersion is carried out at a concentration of from 1 to 150 g / l, in particular from 5 to 50 g / l, and in particular approximately equal to 10 g / l, with a cyclodextrin, Ι'α-CD, at the concentration of 1 to 150 g / l, in particular of 5 to 50 g / l, and in particular approximately equal to 10 g / L.

According to another embodiment, the process for preparing an inclusion complex comprises a step of mixing the polysaccharide in dispersion in an aqueous medium,

the concentration of said polysaccharide being from 0.01 to 9000 g / l of aqueous medium, in particular ranging from 1 to 600 g / l of aqueous medium, and in particular being approximately equal to 1 g / l or approximately equal to 10 g / L of aqueous medium,

with a cyclodextrin, Ι'α-CD, at a concentration of from 0.01 to 9000 g / l of aqueous medium, in particular of from 0.01 to 300 g / l of aqueous medium, and in particular of approximately 10 g / L aqueous medium.

the mass of said polysaccharide being from 1 to 150 g / l of aqueous medium, in particular being from 1 to 10 g / l of aqueous medium, and in particular being approximately equal to 1 g / l or approximately equal to 10 g / l of aqueous medium,

with a cyclodextrin, Γα-CD, at a concentration of from 1 to 150 g / l of aqueous medium, in particular of from 1 to 50 g / l of aqueous medium, and in particular of approximately 10 g / l of aqueous medium.

The complexes are also formed when the polysaccharide is used in the form of a suspension.

The process for preparing an inclusion complex comprises a step of mixing the polysaccharide with a cyclodextrin, Γα-CD,

The mass percentage of said polysaccharide being from 0.01% to 90%, and especially from 0.5% to 50%, The weight percentage of the cyclodextrin being from 0.01% to 90%, and especially from 0.5% to 50%,

The mass percentage of the water or of the aqueous medium being comprised from 10% to 99.99%, and especially from 50% to 99.5%.

The mass percentage of said polysaccharide being from 0.1% to 15%, and in particular from 0.5% to 5%,

The weight percentage of the cyclodextrin being from 0.1% to 15%, and especially from 0.5% to 5%,

The mass percentage of water or of the aqueous medium being comprised from 70% to 99.9%, and in particular from 90% to 99%.

According to a particular embodiment of the process for preparing an inclusion complex, the step of mixing the polysaccharide with a cyclodextrin, α-CD,

is carried out with stirring, in particular magnetic, at a stirring speed of between 10 and 1000 rpm, in particular at a stirring speed of from 100 to 500 rpm, and in particular at a stirring speed of approximately equal at 200 rpm, at a temperature of 1 to 100 ° C, in particular at a temperature of 10 to 35 ° C, and in particular at a temperature of about 20 ° C,

the duration of the stirring being from 6 hours to 15 days, in particular from 24 hours to 96 hours, and in particular approximately equal to 72 hours.

is carried out with stirring, in particular magnetic stirring at a speed of between 50 and 1000 revolutions / minute, in particular at a stirring speed of 100 to 500 revolutions / minute, and in particular at a stirring speed of about equal to at 200 rpm, at a temperature of 4 to 60 ° C, in particular at a temperature of 10 to 35 ° C, and especially at a temperature of about 20 ° C,

the duration of stirring being from 24 hours to 15 days, in particular from 24 hours to 48 hours, and in particular approximately equal to 36 hours.

The process for preparing an inclusion complex also comprises a step for preparing a polysaccharide bearing hydrophobic groups, by reaction of N-acylation

Between the polysaccharide and an acid chloride of formula R ⁴ -C (O) C1,

in which

R ⁴ represents: A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH ₃ or - (CH ₂ ) ₁₆ -CH ₃ ,

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least one C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

Or between the polysaccharide and a fatty acid of formula R ⁴ -C0 ₂ H, in which R ⁴ has the meanings indicated above,

in the presence of a coupling agent such as N- (3-dimethylaminopropyl) -N-ethylcarbodiimide chloride (EDCI) at room temperature for 24 hours,

"Or between the polysaccharide and an acidic cyclic anhydride of the formula R ⁴ -CO-O-CO-R ⁴ , wherein R ⁴ has the meanings indicated above,

to give a polysaccharide carrying hydrophobic groups covalently attached to the polysaccharide by a nitrogen atom of said polysaccharide.

Between the polysaccharide and an acid chloride of formula R -C (O) C1,

in which

R ⁴ represents:

A linear or branched alkyl group containing from 1 to 20 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH ₃ or - (CH ₂ ) ₁₆ -CH ₃ ,

A linear or branched alkenyl group containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₂ ) ₇ -CH ₃ or - (C¾) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

Or between the polysaccharide and an acidic cyclic anhydride of formula R ⁴ -CO-O-CO-R ⁴ , in which R ⁴ has the meanings indicated above,

The N-acylation reaction relates in particular to chitosan. It is carried out by the action of an acid chloride (Li, Y.-Y. et al., 2006, J Appl Polym Sci 102, 1968-1973), a carboxylic acid, less reactive than the chloride of acid, in the presence of the coupling agent EDCI, or by the action of acid anhydrides (Lee, KY et al., 1995, Biomaterials 16, 1211-1216, Lee, MY et al, 2005, Int J Biol Macromol, 36, 152-158; Mourya, VK and Inamdar, NN (2008) Fact Sheet Polymer 68 (6), 1013-1051).

Another embodiment of the process for preparing an inclusion complex comprises a step for preparing a polysaccharide bearing hydrophobic groups, by reacting O-acylation between said polysaccharide dissolved in methanesulphonate and 1 to 20 equivalents per polysaccharide unit. of fatty acid chloride, the reaction being carried out at ambient temperature,

said polysaccharide and acid chloride being previously designated,

to give a polysaccharide bearing hydrophobic groups covalently attached to the polysaccharide by one or more oxygen atoms of said polysaccharide.

Another embodiment of the process for preparing an inclusion complex comprises a step of mixing at least:

A chitosan comprising hydrophobic groups covalently attached to chitosan by a nitrogen atom and / or by one or more oxygen atoms of said chitosan,

■ and a cyclodextrin (CD),

to obtain an inclusion complex in which chitosan and cyclodextrin are non-covalently bound.

■ and a cyclodextrin (CD),

According to a particular embodiment, the process for preparing an inclusion complex comprises a mixing step between

► a chitosan of formula:

or a chitosan of formula:

in which

M represents the number of units of desacetylated units,

N represents the number of units of acetylated units,

R ⁴ represents a hydrophobic group and is chosen from:

An alkyl group, linear or branched, containing from 1 to 20 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH 3 or - (CH ₂ ) ₆ -CH _3j

^D a linear or branched alkenyl group containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

► and a cyclodextrin (CD) of formula:

in which

• p is an integer equal to 6,

1 2 3

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - N¾, or sulfate groups -SO ₄ ^" , and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form, at a concentration of from 1 to 150 g / l of aqueous medium, in particular of from 1 to 50 g of aqueous medium, and in particular of approximately 10 g / l of aqueous medium,

said chitosan of formula I or II being

In aqueous solution at the concentration of from 1 to 150 g / l, in particular being from 1 to 10 g / l, and in particular being approximately equal to 1 or approximately equal to 10 g / l,

the aqueous solvent being chosen from pure water, an aqueous solution of pH ranging from 1 to 7 or from 7 to 12, in particular from 5 to 7, or a physiological saline solution optionally enriched with glucose or containing any other excipient to pharmaceutical, cosmetic, agri-food or veterinary use,

Or in dispersion in an aqueous medium chosen from pure water, an aqueous solution of pH ranging from 1 to 7 or 7 to 12, in particular from 5 to 7, or a saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, cosmetic, agri-food or veterinary use, the mass of said polysaccharide being from 1 to 150 g / l of aqueous medium, in particular being from 1 to 10 g / l of aqueous medium, and in particular being equal to 1 g / L or 10 g / L of aqueous medium,

· The weight percentage of the cyclodextrin being from 0.1% to 15%, and especially from 0.5% to 5%,

The mass percentage of the water or of the aqueous medium being from 70% to 99.9%, and especially from 90% to 99%,

said mixture being carried out with stirring, in particular magnetic stirring at a speed of between 50 and 1000 revolutions / minute, in particular at a stirring speed of 100 to 500 revolutions / minute, and in particular at a stirring speed approximately equal to 200 rpm, at a temperature of 4 to 60 ° C, in particular at a temperature of 10 to 35 ° C, and especially at a temperature of about 20 ° C,

the duration of the stirring being between 24 hours and 15 days, in particular between 24 hours and 48 hours, and in particular approximately equal to 36 hours,

to obtain an inclusion complex in which the chitosan of formula I or II and the cyclodextrin are non-covalently bound.

►a chitosan of formula:

in which

■ R represents

• a hydrogen atom, or

• a group of formula in which

R ⁴ represents a hydrophobic group and is chosen from:

α is a linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₄ -CH 3 or - (CH ₂ ) ₁₆ -CH _3;

α is a linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least 1 C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

provided that R represents at least one group of formula

M represents the number of units of D-glucosamine units,

N represents the number of units of N-acetyl-D-glucosamine units,

provided that the percentage of m in relation to the total number of units is greater than 50%, ► and a cyclodextrin (CD) of formula:

in which

• p is an integer equal to 6,

R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, chosen from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups - NH ₃ ⁺ , or sulphate groups -S0 ₄ ^{2 ~} , and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

at a concentration of from 0.01 to 9000 g / l of aqueous medium, in particular of from 1 to 300 g / l of aqueous medium, and in particular equal to about 200 g / l of aqueous medium, said chitosan of formula I or II being

In aqueous solution at a concentration of from 0.01 to 9000 g / l, in particular ranging from 1 to 300 g / l, and in particular being approximately equal to 200 g / l, the aqueous solvent being chosen from water pure, an aqueous solution of pH of 1 to 7 or 7 to 14, in particular of 5 to 7, or a saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, medical, paramedical, medical devices animal feed, cosmetics, veterinary, agri-food, pesticides, cosmeto-textiles, perfumery, environmental (eg water pollution control) or in the paint, packaging, building and / or building industry automobile,

Or in dispersion in an aqueous medium chosen from pure water, an aqueous solution of pH of from 0 to 7 or 7 to 14, in particular of from 5 to 7, or a physiological saline solution optionally enriched with glucose or containing any other excipient for pharmaceutical, medical, paramedical, medical devices, animal nutrition, cosmetics, veterinary, food, pesticides, cosmetic textiles, perfumery, environmental (eg water depollution) or in the industry paintings, packaging, building and / or automobile. the mass of said polysaccharide being from 0.01 to 9000 g / L of aqueous medium, in particular ranging from 1 to 60 g / L of aqueous medium, and in particular being equal to 1 g / L or 10 g / L of medium aqueous,

The mass percentage of said polysaccharide being from 0.01% to 90%, and especially from 0.5% to 5%,

The weight percentage of the cyclodextrin being from 0.01% to 90%, and especially from 0.5% to 5%,

The mass percentage of water or of the aqueous medium being from 10% to 99.99%, and especially from 50% to 99.5%,

said mixture being carried out with stirring, in particular magnetic stirring at a stirring speed of between 10 and 1000 rpm, in particular at a stirring speed of 100 to 500 rpm, and especially at a stirring speed about 200 rpm, at a temperature of 1 to 100 ° C, in particular at a temperature of 10 to 35 ° C, and especially at a temperature of about 20 ° C,

the duration of the stirring being between 12 hours and 15 days, in particular between 24 hours and 96 hours, and in particular approximately equal to 72 hours,

In another aspect, the invention also relates to particles obtained according to the methods described above.

The invention also relates to a chitosan bearing hydrophobic groups having for formula II:

in which

■ R ⁴ represents

A linear or branched alkenyl group containing 2 to 20 carbon atoms and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

M represents the number of units of desacetylated units,

N represents the number of units of acetylated units,

provided that the degree of deacetylation representing the percentage of m relative to the total number of units is greater than 50%.

in which

■ R represents

a hydrogen atom, or

a group of formula

in which

■ R ⁴ represents

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least one C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH-CH ₂ ) ₇ -CH ₃ ,

provided that R represents at least one group of formula

M represents the number of units of D-glucosamine units,

N represents the number of units of N-acetyl-D-glucosamine units, provided that the degree of deacetylation (DDA) representing the percentage of m relative to the total number of units is greater than 50%.

The invention also relates to a carrageenan bearing hydrophobic groups having the formula I and / u II:

II

R represents

a hydrogen atom, or

a group of formula

*

in which

■ R ⁴ represents

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least one C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ - = CH- (CH ₂ ) ₇ -CH ₃ ,

provided that R represents at least one group of formula

The invention also relates to a heparin carrying hydrophobic groups having the formula:

in which

■ R represents

• a hydrogen atom, or

• a group of formula

R represents

A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH 2) ₄ --CH ₃ or - (CH ₂ ) ₆ --CH ₃ ,

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and carrying at least one C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH-CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -C = CH- (CH ₂ ) ₇ -CH ₃ ,

provided that R represents at least one group of formula

The invention also relates to an amylopectin bearing hydrophobic groups having the formula:

R represents a hydrogen atom, or

a group of formula

in which

■ R ⁴ represents

An alkyl group, linear or branched, containing from 1 to 1000 carbon atoms, in particular the - (CH 2) ₁₄ -CH 3 or - (CH ₂ ) ₆ -CH _{3 groups} ,

provided that R represents at least one group of formula

The invention also relates to a pullulan carrying hydrophobic groups having the formula:

R represents

a hydrogen atom,

a group of formula

in which

■ R ⁴ represents

An alkyl group, linear or branched, containing from 1 to 1000 carbon atoms, in particular the groups - (C¾) ₁₄ -CH3 or - (CH ₂ ) ₁₆ -CH ₃ , A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least one C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -C = CH- (CH ₂ ) ₇ -CH ₃ ,

provided that R represents at least one group of formula

The invention also relates to a dextran bearing hydrophobic groups having the formula:

in which

■ R represents

a hydrogen atom, or

a group of formula

in which

■ R ⁴ represents

An alkyl group, linear or branched, containing from 1 to 20 carbon atoms, in particular the groups - (CH 2) ₁₄ -CH ₃ or - (CH ₂ ) ₁ -CH ₃ ,

provided that R represents at least one group of formula

The invention also relates to a pectin bearing hydrophobic groups having the formula:

in which

■ R represents

a hydrogen atom,

a group of formula

R represents

A linear or branched alkenyl group containing 2 to 20 carbon atoms and bearing from 1 to 4 C = C double bonds, conjugated or otherwise, the - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH _{2 groups} ) ₇ -CH ₃ or - (CH ₂₎ ₇ -CH = CH- (CH ₂₎ ₇ -CH _3.

provided that R represents at least one group of formula

The invention also relates to hyaluronic acid bearing hydrophobic groups having the formula:

in which

■ R represents

a hydrogen atom, or

a group of formula

R represents

A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH ₃ or _T (CH ₂ ) ₁₆ -CH ₃ ,

provided that R represents at least one group of formula

The invention also relates to a chitin bearing hydrophobic groups having the formula:

R represents

a hydrogen atom, or

a group of formula

in which

■ R ⁴ represents

A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₄ -CH ₃ or - (CH 2) ₁₆ -CH ₃ ,

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and bearing at least one C = C double bond, in particular the groups - (CH ₂ ) ₇ -CH = CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ , provided that R represents at least one group of formula O

M represents the number of N-glucosamine units,

■ n represents the number of N-acetyl-glucosamine units,

provided that the percentage of units n in relation to the total number of units is greater than 50%.

In a preferred embodiment, the linear or branched alkyl group containing from 1 to 20 carbon atoms and the linear or branched alkenyl group containing 2 to 20 carbon atoms and having from 1 to 4 C = C double bonds, conjugated or not, are selected from fatty acids.

The invention also relates to a method for preparing an encapsulation system comprising a step of mixing particles containing inclusion complexes according to the invention,

with a substance used for its properties in the pharmaceutical, medical, paramedical, medical devices, animal feed, cosmetics, veterinary, agro-food, pesticides, cosmeto-textiles, perfumery, environmental (water depollution for example) or in the paint, packaging, building and / or automobile industry.

said substance being previously dissolved in an aqueous medium such as water, physiological saline, said medium optionally being enriched with glucose or containing any other excipient for pharmaceutical, medical, paramedical, medical devices, animal feed, cosmetic, veterinary, agro food, pesticides, cosmeto-textiles, perfumery, environmental (water pollution for example) or in the industry of paints, packaging, building and / or automobile.

said medium optionally containing a cosolvent selected from ethanol or acetone, or a surfactant selected from polysorbate derivatives, in particular Tween 80 or Tween 40, to obtain particles containing inclusion complexes containing said substance.

According to a particular embodiment, the process for preparing an encapsulation system according to the invention comprises a mixing step:

A polysaccharide comprising hydrophobic groups covalently attached to the polysaccharide by a nitrogen atom and by oxygen atoms of said polysaccharide,

said polysaccharide being selected from chitosan, dextran, acid, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlane, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and derivatives thereof, and is especially chitosan,

• a cyclodextrin referred to above,

• a substance used for its properties in the pharmaceutical, medical, paramedical, medical devices, animal feed, cosmetics, veterinary, agro-food, pesticides, cosmeto-textiles, perfumery, environmental (water depollution by example) or in the paint, packaging, building and / or automotive industry.

The mass percentage of said solvent being from 0 to 50% and in particular approximately equal to 25%,

The percentage by weight of the water or of the aqueous medium being from 30% to 99.9%, and especially from 90% to 99%,

to obtain an inclusion complex containing said substance.

The step of mixing the process for preparing an encapsulation system comprises a step of dissolving the active ingredient in an aqueous medium, followed by the addition in the medium of the amphiphilic polysaccharide and α-cyclodextrin. The mixture is placed under magnetic stirring for 3 days. But in a practical way, it is possible to mix all the components at the same time.

The particles can then be isolated

either by sedimentation or by centrifugation if it is microparticles (hydrodynamic diameter greater than one micrometer),

either by ultracentrifugation or by membrane separation methods such as ultrafiltration and microfiltration, in the case of nanoparticles (hydrodynamic diameter less than a micrometer).

DESCRIPTION OF THE FIGURES;

Figure 1

FIG. 1 represents the characteristic IR spectrum of N-acylated chitosan by oleic acid (1) in comparison with that of native chitosan (2). Figure 2

Figure 2 shows the formula of unmodified chitosan and its 1 H-NMR spectrum (300 MHz) in DCl at 1% v / v in D ₂ 0. The hydrogen atoms are numbered on the formula of the compound, these numbers appearing on the peaks of the NMR spectrum.

Figure 3

Figure 3 shows the 1H-NMR spectrum (300 MHz) of chitosan after N-acylation with oleic acid solubilized in DCl at 1% v / v in D ₂ 0.

Figure 4

Figure 4 shows the IR spectrum of O-palmitoyl-cbitosan (1) in comparison with native chitosan (2).

Figure 5

Figure 5 shows the proton NMR spectrum in DMSO-d ₆ , O-palmitoyl-chitosan.

Figure 6

Figure 6 shows the IR spectrum of O-palmitoyl-pullulan (1) compared to that of native pullulan (2).

Figure 7

Figure 7 shows the IR spectrum of O-palmitoyl amylopectin (1) compared to that of native amylopectin (2).

Figure 8

Figure 8 shows the IR spectrum of O-palmitoyl dextran (1) compared to that of native dextran (2).

Figure 8bis

Figure 8bis shows the IR spectrum of O-palmitoyl-dextran Figure 9 shows the IR spectrum of chitin esterified with palmitic acid (1) in comparison with that of native chitin (2).

Figure 9-bis

Figure 9-bis shows the IR spectrum of O-palmitoyl-chitin

Figure 10

Figure 10 shows the solid ¹³ C-NMR spectrum of O-oleoyl-chitin.

Figure 11

Figure 11 shows the characteristic IR spectrum of O-palmitoyl heparin (1) compared to native heparin (2). Figure 12

Figure 12 shows the characteristic IR spectrum of Ο-parmitoyl-carrageenan (1) in comparison with native carrageenan (2).

Figure 13

Figure 13 shows the characteristic IR spectrum of O-palmitoyl hyaluronic acid (1) in comparison with native hyaluronic acid (2).

Figure 14

Figure 14 shows the images obtained by transmission electron microscopy of different particle preparations.

Figure 15

FIG. 15 represents the α, β and γ cyclodextrins. In the figure, the dimensions are given in Angstroms.

Figure 16

FIG. 16 represents the effect of the concentration of O-palmitoyl heparin DS 1% on the D _h of the nanoparticles.

Figure 17

FIG. 17 represents the effect of the concentration of Γα-CD on the D _h of the microparticles composed of O-palmitoyl heparin DS2.

Figure 18

FIG. 18 represents the observation in MET of particles composed of O-palmitoyl heparin DS2

Figure 19

FIG. 19 represents the effect of the concentration of α-CD on the D _h of the microparticles composed of O-palmitoyl-carrageenan DS I.

Figure 20

Figure 20 shows the effect of the concentration of O-palmitoyl-carrageenan DSI on the D _h of the microparticles.

Figure 21

Figure 21 shows the effect of the Γα-CD concentration on the D _h of O-pallitoyloyl-carrageenan DS2 particles.

Figure 22

Figure 22 shows the effect of the concentration of Ο-palmitoyl-carrageenan DS3 on the D _h of the microparticles formed. Figure 23

FIG. 23 (1) represents an image obtained by transmission electron microscopy of the preparation α-cyclodextrin / native chitosan / water (10/1/89)% indicating the absence of formation of nanoparticles or microparticles.

Figure 23 (2) shows nanoparticles composed of α-cyclodextrin / CM6 / water (10/1/89)%.

Figure 24

FIG. 24 (1) represents an image obtained by transmission electron microscopy of the nanoparticles at the laboratory scale.

FIG. 24 (2) shows an image obtained by transmission electron microscopy of the nanoparticles at the pilot scale.

EXAMPLES

Meaning of the abbreviations used:

CD: cyclodextrin

CDC1 ₃ : deuterated chloroform

CM: modified chitosan

D ₂ 0: deuterated water

Da: unit of molar mass in dalton, which corresponds to g L

DC1: deuterated hydrochloric acid

DDA: degree of deacetylation

D _h : hydrodynamic diameter

DMF: dimethylformamide

DMSO-d6: deuterated dimethyl sulfoxide

DS: degree of substitution

EDCI: 1-ethyl-3- (3-dimethylaminopropyl) carbodiimide

HSV: the human herpes simplex virus

HPV: the human papillomavirus

IR: infrared

kDa: kilodalton

kHz: kilohertz

MET: transmission electron microscopy

M _m : molar mass

MHz: Megahertz NaN0 ₂ : Sodium nitrite

QSP: sufficient quantity for

NMR: nuclear magnetic resonance

RPM: rotation per minute

RSV: Respiratory syncytial virus

δ: displacement of the proton, expressed in ppm

M _m : molar mass

AP: palmitic acid

AO: Oleic acid

Characteristics / types of analytical devices used:

1H-NMR (Bruker ARX, 300 MHz or 500 MHz): All the N- or O-acylated chitosan compounds obtained were analyzed by proton NMR. Depending on the solubility of the acylated polysaccharides, several solvents can be used such as deuterated water (D ₂ 0) with 1% v / v of DC1, deuterated chloroform (CDCl ₃ ), deuterated dimethyl sulfoxide (DMSO-d 6). The spectra are made at room temperature. If the acylated polysaccharide is poorly soluble or if the viscosity is high, the samples are heated up to 85 ° C. and an electromagnetic field of 500 MHz is used.

Characterization by ¹³ C-NMR of the solid: The spectra were carried out on an AVANCE II BRUKER spectrometer, and specialized NMR techniques of the solid were used, in particular the Magic Angle Rotation (MAS) and the polarization transfer of 1H to ^13C (CP) to avoid the inconveniences associated with sometimes very long relaxation times in the solid state.

It was operated at G> L = 500 MHz ( ^! H) and 125.77 MHz ( ¹³ C); the contact time was set at 1.5 ms. These samples were turned at the magic angle at a frequency of 10 kHz, we used a 4 mm rotor.

IR spectra (ATR-FTIR, FT spectrometer TR-4100, JASCO): the principle consists in putting a crystal (diamond) in contact with the sample to be analyzed, before being crossed by the infrared beam.

Particle size measurements: The particle sizes were evaluated by the hydrodynamic diameter. Measurements of the average hydrodynamic diameters of the nanoparticles and microparticles were carried out with a Nano-ZS90 nanoseries Zetasizer from Malvern Instruments SA (Orsay, France) by quasi-elastic light scattering. The samples were previously diluted by taking 30 μΕ of suspension of nanoparticles or microparticles and diluting them in 1 ml of MilliQ ^® water. Diameters The hydrodynamics of the microparticles were remeasured by a laser granulometer (MasterSizer 2000) from Malvern Instruments SA (Orsay, France).

Transmission electron microscopy (TEM) was used to observe microparticles and nanoparticles using a Jeol 1400 60 kV microscope and a camera. Lyophilization of the Grafted Polysaccharides by Hydrophobic Groups: Some synthesized polysaccharide derivatives were lyophilized using an Alpha 1-2 lyophilizer (vaulted, France) for 48 hours after the solutions were frozen for at least 12 hours.

Details on the products used: The active ingredients, vitamin B6, paracetamol, ketoprophene, indomethacin, caffeine were obtained from INRESA, Bartenheim, France. Parsol 1789 is from DSM Nutritional Products, Germany.

All the solvents: anhydrous dimethylformamide, dichloromethane, diethyl ether, ethanol, methanol, ammonia, glacial acetic acid (98% (m / m)) come from VWR, France.

Chitosan (medium viscosity, molar mass M _m = 250 kDa), pullulan, amylopectin, dextran-carrageenan, heparin, hyaluronic acid, N- (3-dimethylaminopropyl) chloride N-ethylcarbodiimide (EDCI), palmitic acid (99% (w / w)), oleic acid (> 98% (mm)), sodium bicarbonate, sodium hydroxide, sodium chloride, sodium nitrite (NaNO ₂ ), methanesulfonic acid, palmitoyl chloride, oleoyl chloride, deuterated water, deuterated hydrochloric acid (DCl), deuterated chloroform (CDCl ₃ ) _; deuterated dimethyl sulphoxide (DMSO-d ₆ ), anhydrous pyridine, triethylamine, Sudan III, hydroxypropyl-cyclodextrin (ΗΡ-β-CD) were supplied by Sigma-Aldrich Chemical Co., Saint Quentin Fallavier, France. Castor oil comes from the company Croda, France. Α-Cyclodextrin (α-CD), methyl-β-cyclodextrin (Με-β-CD) Rameb ^® , degree of substitution -1.8, M _m = 1320 g / mol, was purchased from Cyclolab (Budapest, Hungary). ).

The other chitosans (20 and 145 kDa) were obtained after depolymerization of the commercial chitosan M _m = 250 kDa according to the technique developed by Huang et al (Pharmaceutical Research, 2004, 21 (2), 344): 2 g of commercial chitosan are solubilized overnight in 100 mL of acetic acid (6% v / v), this chitosan solution is then depolymerized by chemical reaction for 1 h with 10 mL of NaN0 ₂ (85 mg / mL). The depolymerized chitosan is then precipitated by increasing the pH to 9 with sodium hydroxide solution (4 mol / L) and recovered by filtration (sintered glass filter No. 4, under vacuum). It is then solubilized in 20 mL of acetic acid (0.1 mol / L) and dialyzed (membrane dialysis Spectra / Por, MWCO 3500, lot 3228543, Spectrum Laboratories Inc. ^®) against 1 L of distilled water twice for lh30 then overnight then lyophilized.

The molar mass of the depolymerized chitosan is determined by capillary viscometry. The flow time (f) in μ-Ubbelohde microrube (type 53710 1, no. 1016187, R = 0.01022 mm ² / s ² , Schott Gerâte) of chitosan solutions in a 0.1 mol acetic acid mixture / L and NaCl 0.2 mol / L at different concentrations (c = 0.25 / 0.50 / 1.00 / 1.50 / 2.00 g L) is measured at 20 ° C (bath CT1450 Schott Gerâte and cooling system CK100 Schott Gerâte) using an AVS400 viscometer (Schott Gerâte). For each concentration, the equilibration time is 5 min and five successive measurements are made. From the results obtained, the intrinsic viscosity [η] is deduced by taking the ordinate at the origin of the straight line = f (C) with t ₀ the flow time of the 0.1 mol / acetic acid mixture. L and 0.2 mol / L NaCl. The molar mass is then calculated using the Mark-Houwink-Sakurada equation η = ΚΜ ^, with K = 1.81 × 10 ^-6 and α = 0.93.

Synthesis of polysaccharides bearing hydrophobic groups

Example 1 Synthesis and Characterization of N-Acylated Chitosan

The protocol consists in dissolving 1 g of chitosan (M _m = 20, 145, 250 kDa), whose degree of deacetylation (DDA) is equal to 85%, in an aqueous solution of acetic acid at 1% v / v ( 100 mL) diluted with methanol (75 mL). Oleic or palmitic acid is dissolved in 10 mL of methanol and added to the chitosan solution. A number of moles of EDCI equal to that of the fatty acid is added dropwise to the mixture of fatty acid and chitosan with continuous magnetic stirring. After 24 hours of reaction, the product is precipitated in a 7/3 v / v methanol / ammonia mixture. The precipitate is filtered on a sintered glass filter and washed successively with water, methanol and then diethyl ether. Finally, the product is dried under vacuum for 48 hours.

During this reaction, several parameters have been modified. Thus, it is possible to obtain several types of N-acyl chitosan according to the type of fatty acid grafted, the degree of grafting (degree of substitution) and the molar mass of chitosan.

The IR spectra of the grafted chitosan obtained were recorded. The two curves of FIG. 1 show a very wide band between 3430 cm ^-1 and 3440 cm ^-1 corresponding to the OH groups (FIG. 1). The native chitosan has a low absorption at the level of the vibration of the NH groups around 1578 cm- ^1, after N-acylation, it is necessary to note the weak absorption of its derivatives in the bands 3000 cm ^-1 and 3600 cm ^-1 and the appearance of two bands 1636 cm ^-1 and 1657 cm ^-1 , characteristics of the carbonyl groups and secondary amides respectively and which confirm well the formation of the amide bond . For strips to 2922 cm ^", 2853 ^cm" \ 1457 cm ^"1 and 1198 ^cm", they correspond to alkyl chains of the fatty acid.

The comparison of the proton RM spectra (FIGS. 2 and 3) shows an additional signal with respect to the spectrum of unmodified chitosan at δ = 1.017 ppm. It corresponds to the signal of the methyl group of the end of the fatty acid chain. Example 2 Characteristics of Modified Chitosan CM1-CM9

The characteristics of the modified chitosan CM1-CM9 are summarized in Table 1 below. The degree of substitution was calculated from the results of the elemental analysis of α-acylated chitosan and native chitosan.

Table 1: Characteristics of N-acylated chitosan

Example 3 Preparation of Modified Chitosan Samples, CM1-CM9 Characterization by proton NMR

For the characterization of N-acyl chitosan by proton NMR, a solution of polymer at a concentration of 5 g / L is prepared in deuterated water (D ₂ 0) in the presence of deuterated hydrochloric acid (DCl). This step allows the exchange of labile protons of the hydroxyl groups by deuterium atoms. The labile protons of the hydroxyl groups all resonant at the same frequency, their exchange by deuterium atoms makes it possible to eliminate the residual signal of the light water. In order to reduce the viscosity, the experiments were recorded at a temperature of 85 ° C with an acquisition number and a relaxation time of 5 and 1 seconds respectively.

¹ H-NMR (300 MHz) unmodified chitosan: the correspondence of each proton displacement is shown in FIG.

1 H-NMR (300 MHz) modified chitosan: an additional peak with respect to the spectrum of unmodified chitosan appears for a chemical shift equal to δ ₈ = 1.017 ppm (FIG. 3). It corresponds to the signal of the fatty acid chain.

Example 4 Synthesis and Characterization of O-Acylated Chitosan

The chitosan (250 kDa, 2 g) is dissolved in 20 mL of methanesulfonic acid at room temperature with continuous magnetic stirring for one hour. The acid chloride (oleic or palmitic) is then introduced into the reaction medium. After 5 hours, the mixture is cooled in an ice bath to stop the reaction, a precipitate is formed. The precipitate is dialyzed for 12 hours and then neutralized with sodium bicarbonate. It is then dialyzed for 48 hours and lyophilized.

The IR spectrum (FIG. 4) of O-palmitoyl-chitosan shows a characteristic band of carbonyls of an ester group at 1700 cm ^-1 and bands at 2916 cm ^-1 , 2849 cm ^-1 correspond to the alkyl chains of the acid. The proton NMR spectrum (Figure 5) compared to the native chitosan spectrum (Figure 2), shows the appearance of new peaks including those characteristic of the CH ₃ group at the end of the 0.88 ppm chain and the proton methylene CH ₂ groups near the CO function at 2.8 ppm.

Example 5: Table 2, characteristics of modified chitosan CM10-CM12

The characteristics of the modified chitosan CM10-CM12 are summarized in Table 2 below. The degree of substitution was calculated from the results of the elemental analysis of O-acylated chitosan and native chitosan.

Table 2: Characteristics of O-acylated chitosan Example 6 Synthesis and Characterization of Pullulan Grafted with Palmitic Acid

O-palmitoyl-pullulan was prepared according to the reference of Sunamoto et al (Sunamoto J, Sato T, Taguchi T, Hamazaki H, Naturally occuring polysaccharid derivatives which is an artificial cell wall on an artificial liposome, Macromolecules, 1992, 25, 5665-5670). Pullulan (5 g) is dissolved in anhydrous dimethylformamide (55 mL) at 60 ° C. 5 ml of anhydrous pyridine and palmitoyl chloride (5 equivalents per unit of glucose triholoside) are added to the resulting solution. The reaction mixture is stirred at 60 ° C for 2 h and then for 1 h at room temperature. The mixture is poured into ethanol (350 mL). The precipitate obtained is extracted and washed with ethanol and then with diethyl ether. The white solid obtained is dried under vacuum.

IR spectrum ΓΟ-palmitoyl-pullulan: band at 1739 cm ^"1 corresponding ester group to the carbonyl of (Figure 6) and the bands 2916 ^cm", 2849 cm ^"", 1467 cm ^"1 and 1197 cm correspond to the channels fatty acid alkyls. Example 7 Synthesis and Characterization of Amylopectin Derivatives Grafted with Palmitic Acid

Amylopectin (5 g) is mixed with anhydrous dimethylformamide. The mixture is stirred at 70 ° C. until the polysaccharide is completely dissolved. Then, anhydrous triethylamine and palmitoyl chloride are added and then heated under stirring for 2 hours. The solution is then diluted in methanol which is responsible for precipitation of O-palmitoyl amylopectin. The white solid obtained is filtered and then dried under vacuum.

IR spectrum of O-palmitoyl amylopectin: 1739 cm ^{-1 band} corresponding to the carbonyl of the ester group (FIG. 7), and in particular 2916 cm- ¹ , 2849 cm ^-1 and 1462 cm- ¹ bands corresponding to the alkyl chains fatty acid.

Example 7bis: Synthesis and Characterization of Amylopectin Derivatives Grafted with Palmitic Acid

The (-palnitoyl amylopectin was prepared according to the reference of Sunamoto et al (Sunamoto J, Sato T, Taguchi T, Hamazaki H, Naturally occuring polysaccharid derivatives which is an artificial cell wall on an artificial liposome, Macromolecules, 1992, 25, 5665-5670) The amylopectin (5 g) is mixed with 55 ml of anhydrous dimethylformamide at 60 ° C. with continuous magnetic stirring To the solution obtained are added 5 ml of anhydrous pyridine, 1.2 ml of anhydrous DMF. The amount of palmitoyl chloride was varied depending on the degree of substitution desired. The reaction mixture is stirred at 60 ° C for 2 h and then for 1 h at room temperature. The mixture is poured into 350 mL of ethanol. The white solid obtained is dried under vacuum. Example 8 Synthesis and Characterization of Dextran Derivatives Grafted with Palmitic Acid

Dextran is suspended in anhydrous dimethylformamide. The mixture is stirred at 70 ° C until complete dissolution of the polysaccharide. Then, the anhydrous triethylamine and palmitoyl chloride are added and then heated with stirring for 2 hours. The solution is then diluted in methanol which causes precipitation of O-palmitoyl dextran. The white solid obtained is filtered and then dried under vacuum. IR spectrum of O-palmitoyl-dextran: 1739 cm ^{-1 band} corresponding to the carbonyl of the ester group (FIG. 8), and in particular bands at 2914 cm ^-1 , 2853 cm ^-1, correspond to the alkyl chains of the fatty acid.

Example 8bis: Synthesis and Characterization of Dextran Derivatives Grafted with Palmitic Acid

O-palmitoyl-dextran was prepared according to the protocol described by Sunamoto et al (Sunamoto J, Sato T, Taguchi T, Hamazaki H, Naturally occuring polysaccharid derivatives which is an artificial cell wall on an artificial liposome, Macromolecules, 1992 , 25, 5665-5670). Dextran (5 g) is mixed with 55 mL of anhydrous dimethylformamide at 60 ° C. 5 ml of anhydrous pyridine and palmitoyl chloride are added to the solution obtained. The reaction mixture is stirred at 60 ° C for 2 hours and then for 1 hour at room temperature. The mixture is poured into 350 mL of ethanol. The precipitate obtained is extracted and washed with ethanol and then with diethyl ether. The white solid obtained is dried under vacuum.

IR spectrum of O-palmitoyl dextran (FIG. 8bis): bands at 2914 cm ^-1 and 2848 cm ^-1 corresponding to the alkyl chains of the fatty acid. Example 9 Synthesis and Characterization of O-Oleoyl-Chitin and O-Palmitoyl-Chitin

Synthesis: Chitin was esterified with oleic acid according to the method described in reference (Yang B.Y., Ding Q, Montgomery R., Preparation and physical properties of chitin fatty acid esters, Carbohydrate Research, 2009, 344 (3) , 336-342). Chitin (7.5 g), previously dried under vacuum at 60 ° C. for 16 hours, is introduced into a mixture of trifluoroacetic acid (75 ml) and palmitic acid or oleic acid (28 g). The mixture is then heated to 70 ° C with continuous stirring for 30 min, then cooled to room temperature. Subsequently, 300 mL of cold absolute ethanol (-20 ° C) is added, and the mixture is concentrated in a rotary evaporator at a temperature of 20 ° C under vacuum. The product obtained is dispersed in absolute ethanol and heated to 80 ° C. After decantation and removal of the supernatant, the final product is dried and dissolved in 30 ml of DMF and then centrifuged at 3600 g. The esterification of chitin with palmitic acid or oleic acid is carried out in the presence of trilfluoroacetic acid, known to be an esterification promoter for other polysaccharides, in particular the starch mentioned in the reference ( Yang B. Y, Montgomery R, Acylation of Starch using Trifluoroacetic Anhydride Promoter, Starch-Stark, 2006, 58 (10), 520-526). Indeed trifluoroacetic acid causes the formation of the acid anhydride which is much more reactive than the carboxylic acid itself. Being strongly electronegative and having a strong acid power, trifluoroacetic acid causes the protonation of the amine functions, thus allowing a preferential esterification on the alcohol functions.

Characterization of O-oleoyl-chitin and O-palmitoyl-chitin: Infrared spectroscopy analysis is a fast and efficient method for identifying the chemical groups of esterified chitin compared to the native chitin spectrum. The spectrum shown in FIG. 9 is typical of chitin, the frequency of the carbonyl (CO) regions of the amides between 1600 cm ^-1 and 1500 cm ^-1 is of great intensity. The band corresponding to amide I is divided into two peaks at 1654 cm ^"1 and 1619 ^cm". The band corresponding to amide II is unique and is 1556 cm ^-1 .

With regard to the spectrum obtained from O-palmitoyl-chitin (FIG. 9bis), we observe a greater absorption for the bands at 1649 cm ^-1 and 1554 cm ^-1 , which explains the presence of the CO and amide II carbonyl groups. thus demonstrating N-acylation of the free amino functions of chitin. Figure 9bis (1) also shows bands at 2916 cm- ¹ and 2849 cm- ¹ corresponding to the alkyl chains of the fatty acid.

Characterization by ^I3 C-NMR of the oleic acid-esterified chitin solid is particularly suitable for the characterization of this derivative which is insoluble in water and in the majority of organic solvents. The spectrum shown in FIG. 10 shows the presence of 9 resonance peaks whose values are shown in Table 3 below.

Displacement function (ppm)

⁼ CH-, -CH ₂ -, - CH ₃ 14.29, 22.93, 29.81

C2 55.35

C6 60.96

C3-C5 73.87

C 83.85 Cl 104.03

C = 0 amide and ester 173.79

Table 3: Displacements obtained in solid-carbon NMR of O-oleoyl-chitin expressed in ppm and the corresponding functions

Example 10 Synthesis of heparin grafted with palmitic acid DSI

Introduce 1 g of heparin in 11 ml of anhydrous DMF. Heat gradually to 60 ° C with magnetic stirring. Add 5 mL of anhydrous pyridine and then 2.5 g of palmitoyl chloride in 6 mL of anhydrous DMF. Leave the mixture under magnetic stirring for 2 h at 60 ° C. and then 1 h at room temperature. Pour the mixture into 100 mL of cold ethanol to obtain a precipitate. Extract and wash the precipitate with 100 mL of ethanol and then 100 mL of diethyl ether.

Example 10a: Synthesis and Characterization of Heparin Grafted with Palmitic Acid DS2

Synthesis: Heparin (2 g) is dissolved in 10 ml of dichloromethane and 2 ml of palmitic acid chloride contained in a flask. The flask is refluxed under continuous magnetic stirring for 72 h at room temperature. Afterwards, 20 ml of a solution of sodium acetate in methanol is added to the reaction mixture. The precipitate formed is recovered on a sintered glass filter of porosity No. 4 and then washed with 100 ml of methanol and then 100 ml of acetone. The solid is dried under vacuum at room temperature. The heparin esterified with palmitic acid is purified by dissolving in 10 ml of distilled water and adding NaCl until a NaCl concentration of 10% w / v is reached. Afterwards, 20 ml of methanol are added and the precipitate formed is recovered on a sintered glass filter and then washed with 100 ml of ethanol and then 100 ml of acetone. The solid is dried under vacuum at room temperature.

Characterization of O-palmitoyl-heparin: The infrared spectroscopy analysis (Figure 11) showed the presence of 1620 and 1724 cm- ¹ bands which correspond to the carbonyl groups of the ester function The 1135 and 1187 cm bands ^"1 correspond to the C-O groups of the ester function. The O-palmitoyl-heparin spectrum also showed bands at 2849 and 2916 cm ^-1 corresponding to the alkyl groups of palmitic acid.

Example 11 Synthesis and Characterization of Carrageenan Grafted with Palmitic Acid

Synthesis: Carrageenan (2 g) is suspended in 10 ml of dichloromethane and 1, 2 or 3 ml of palmitic acid chloride contained in a flask. We call the O-palmitoyl-carrageenans obtained DSI, DS2 and DS3 in relation to the amount of acid chloride reacted. The flask is refluxed under continuous magnetic stirring for 72 h at 30 ° C. Afterwards, the solid is recovered on a sintered glass filter and then washed twice with 100 mL of ethanol. The solid is dried under vacuum at room temperature for 12 hours.

Infrared Characterization (Figure 12): The characterization by infrared spectroscopy of o-palmitoyl-carrageenan showed the presence of bands at 1699 cm ^-1 and 1739 cm ^-1, which correspond to the carbonyl groups of the ester function. The bands at 1047 cm ^-1 and 1207 cm ^-1 correspond to the C-O groups of the ester function. The O-palmitoyl-carrageenan spectrum also showed bands at 2848 cm- ¹ and 2916 cm- ¹ corresponding to the alkyl groups of palmitic acid.

Example 12 Synthesis and Characterization of Hyaluronic Acid Grafted with Palmitic Acid

Hyaluronic acid (2 g) is mixed with 10 ml of dichloromethane and 2 ml of palmitic acid chloride contained in a flask. The flask is refluxed under continuous magnetic stirring for 5 days at 30 ° C. Afterwards, the solid is recovered on a sintered glass filter and then washed twice with 100 ml of acetone. The solid is dried under vacuum at room temperature for 12 hours. Infrared characterization (Figure 13): Characterization by infrared spectroscopy of ΓΟ-palmitoyl-hyaluronic acid showed the presence of bands corresponding to the carbonyl groups of the ester function. The bands at 1048 and 1207 cm ^-1 correspond to the C-O groups of the ester function, and the O-palmitoyl-hyaluronic acid spectrum also showed bands at 2848 and 2915 cm ^-1 corresponding to the alkyl groups of the palmitic.

Example 13: Formation of microparticles and nanoparticles from α-cyclodextrin and acylated polysaccharides: N-palmitoyl-chitosan and O-oleoyl-chitosan

The microparticles and nanoparticles were formed from α-cyclodextrin and polysaccharide grafted with fatty acids. The examples of the polysaccharides used are grouped in the table below. The protocol consists of weighing α-cyclodextrin and the O- or N-acyl polysaccharide in a small flask. Subsequently, the distilled water is added to the mixture of α-cyclodextrin and the polysaccharide O- or N-acylated. The mixture is kept under magnetic stirring for 3 days. polysaccharide Mass Acid DS Percentage Percentage Percentage Size of fatty molar (%) mass of mass mass particles polysaccharid of water (nm) *

(kDa) e amphiphilic cyclodextrin

chitosan N-250 AP 13.1 1 10 89 7320 ± acylated 2 1823 chitosan 0- 250 AO 4.64 1 10 89 2090 ± acylated 367

* Hydrodynamic diameter expressed in volume.

Table 4: Sizes of particles obtained from N-acylated or O-acylated chitosan An example of an image of particles observed by electron transmission microscopy is shown in FIG. 14.

^■ 5

Example 14 Encapsulation of Water-Soluble Active Ingredients

The protocol adopted for encapsulating the hydrophilic active principles is to dissolve the active principle in water at an initial concentration as indicated in Table 5 and then to add the amphiphilic polysaccharide and Γα-cyclodextrin. The mixture is kept under magnetic stirring for 3 days. After the 3 days of mixing, the concentration of the active ingredient that has not been encapsulated is determined in the supernatant of the preparation. The supernatant is separated either by simple sedimentation or by centrifugation of the microparticles, or after ultracentrifugation in the case of nanoparticles.

Table 5: Example of encapsulated active molecules. Example 15 Preparation and Characterization of Nanoparticles Comprising O-Palmitoyl Heparin DSI

The protocol consists of weighing O-palmitoyl heparin DSI and α-cyclodextrin in a vial. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature thanks to a magnetic bar. The O-palmitoyl heparin DSI concentrations of α-cyclodextrin are shown in Table 6. The results of hydrodynamic diameter measurements are shown in Table 6 and Figure 16.

Table 6: Effect of O-palmitoyl heparin concentration variation on the hydrodynamic diameter of nanoparticles composed of heparin DS2

Example 16 Preparation and Characterization of Nanoparticles Composed of O-Palmitoyl Heparin DS2

O-palmitoyl heparin DS2 and Γα-cyclodextrin were weighed into a vial. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature thanks to a magnetic bar. The concentrations of α-cyclodextrin α-palmitoyl heparin DS 2 are shown in Table 7. The results of hydrodynamic diameter measurements are shown in Table 7 and Figure 17.

Table 7: Effect of the variation of the concentration of α-CD on the hydrodynamic diameter of nanoparticles composed of heparin DS2 Figure 18 shows an example of images obtained by electron transmission electron microscopy observations of nanoparticles composed of heparin DS2. These images obtained without contrast agents, show that these nanoparticles self-organized in a well structured manner in the form of a hexagon.

Example 17 Preparation and Characterization of O-Palmitoyl Carrageenan DSI Microparticles

The 0-palmitoyl-carrageenan DSI and Γα-cyclodextrin are weighed in a bottle. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature thanks to a magnetic bar. The O-palmitoyl-carrageenan deα-cyclodextrin concentrations and the hydrodynamic diameter measurement results are shown in Table 8.

• Variation in the amount of α-cyclodextrin (Figure 19)

Effect of the variation of the concentration of a-CD on the hydrodynamic diameter of the microparticles composed of carrageenan DSI

• Variation of O-palmitoyl-carrageenan DSI (Figure 20)

Name Concentration Concentration Ratio of D _h (nm)

0-palmitoyl-α-carrageenan CD-0-DSI (g / L) palmitoyl-carrageenan α-CD (g / L)

DSI

Carr5 100 2.5 40 1089 ± 272

Carr6 100 5 20 1277 ± 218 Carr7 100 10 10 1196 ± 242

Carr8 100 20 5 1384 ± 225

Carr9 100 30 3.3 1658 ± 403

TABLE 9 Effect of the variation of the O-palmitoye-carrageenan concentration on the hydrodynamic diameter of the microparticles composed of Carrageenan DSI Example 18 Preparation and Characterization of O-Palmitoyl-Carrageenan DS2 Microparticles and Nanoparticles

LO-palmitoyl-carrageenan DS2 as well as Γα-cyclodextrin are weighed into a vial. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature thanks to a magnetic bar. The O-palmitoyl-carrageenan deα-cyclodextrin concentrations and hydrodynamic diameter measurement results are shown in Table 10.

• Variation in the amount of α-cyclodextrin (Figure 21)

Table 10: Effect of the variation of the concentration of α-CD on the hydrodynamic diameter of the microparticles and nanoparticles composed of carrageenan DS2. EXAMPLE 19 Preparation and Characterization of O-Palmitoyl-Carrageenan DS3 Microparticles

LO-palmitoyl-carrageenan DS3 as well as Γα-cyclodextrin are weighed into a vial. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature. The ΓΟ-palmitoyl-carrageenan concentrations of α-cyclodextrin and the results of hydrodynamic diameter measurements are shown in Table 11. • Variation of the amount of fl-palmitoyl-carrageenan DS3.

Table 11: Effect of variation of O-palmitoyl-carrageenan concentration on the hydrodynamic diameter of microparticles composed of carrageenan DS3

Example 20 Manufacture of Microparticles and Nanoparticles Comprising N-Palmitoyl-Chitosan in the Presence of Castor Oil

The microparticles and nanoparticles were formed from α-cyclodextrin and N-palmitoyl-chitosan CM9. The concentrations used are summarized in the table below. The protocol consists of weighing N-palmitoyl-chitosan, Ρα-cyclodextrin and castor oil previously marked by Sudan III. The addition of Sudan III makes it possible to detect the instability phenomena of the preparations. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature.

The preparations observed with the eye did not show phenomena of instability. The results of the size measurements are summarized in the table below.

Table 12: Effect of variation of castor oil concentration on the hydrodynamic diameter of microparticles and nanoparticles composed of chitosan CM9

Example 21 Manufacture of Microparticles Comprising O-Oleoyl-Chitin in the Presence of Castor Oil

The microparticles were formed from α-cyclodextrin and O-oleoyl-chitin DS 0.68%. The concentrations used are grouped in the table below. The protocol consists of weighing O-oleoyl-cliitin, α-cyclodextrin and castor oil previously marked by Sudan ΠΙ. The addition of Sudan III makes it possible to detect the instability phenomena of the preparations. Subsequently, the water is added to the mixture. Everything is mixed for 72 hours at room temperature. The preparations observed with the eye did not show phenomena of instability. The results of the size measurements are summarized in the table below.

Table 13: Effect of variation of castor oil concentration and O-oleoyl-chitin concentration on the hydrodynamic diameter of the microparticles

Example 22 Absence of Particle Formation Using Native Chitosan, Not Grafted with Palmitic Acid

Α-cyclodextrin (100 mg) and native chitosan (10 mg) were weighed in a vial. Subsequently, the water is added to the mixture so as to reach a total volume of 1 mL. The whole is mixed thanks to a magnetic bar for 72 hours at room temperature. FIG. 23 (1) is an image obtained after observation by electron transmission microscopy which shows the absence of formation of nanoparticles or microparticles in comparison with the images of nanoparticles obtained with O-palmitoyl-chitosan CM6 / α-cyclodextrin / water (1/10/89)%.

Example 23 Drying of Particles by Freeze-drying

Lyophilization is a vacuum drying process at low temperature. The product containing water is previously frozen. Even today freeze-drying remains the method of choice for drying heat-sensitive products.

The microparticles were prepared from α-cyclodextrin and N-oleoyl-chitosan, CM4, DS 13.47%. The protocol consists of weighing N-oleoyl-chitosan and α-cyclodextrin. The concentrations used are shown in Table 14. Thereafter, water is added to the mixture. The whole is mixed for 72 hours at room temperature.

Freeze-drying is carried out on 1 ml of preparation containing the microparticles previously frozen at (-20 ° C.) for 12 h, then placed in the freeze-dryer for 24 h. After freeze-drying, the preparations are resuspended in 1 mL of MilliQ ^® water, we note that the macroscopic appearance of the samples has not changed. In order to ensure that the lyophilization step did not modify the physicochemical characteristics of the particles, measurements of the hydrodynamic diameter were made after lyophilization and compared with those obtained before lyophilization (Table 14).

Table 14: Measurement of Hydrodynamic Diameters of Particles (CM4 Chitosan)

N-acylated kDa with PAO and a 13.47% DS before and after freeze drying Example 24: Scaling of Scale-up

Scaling up is a necessity to develop this process on an industrial scale. We designed a pilot consisting of a reactor stirred by a mechanical propeller type agitator. The stirring speed is set at 350 rpm. The regulation of the temperature at 25 ° C is ensured by a circulation of fluid (water / ethylene glycol) connected to a thermostat.

The batches of 100 ml of microparticles are obtained by successively adding to the reactor (1 g) chitosan of molecular weight 250 kDa N-acylated with 10 equivalents of palmitic acid (CM9, DS 17.01%), 10 g of a-cyclodextrin and MilliQ ^® water qs 100 mL.

The results obtained at pilot scale are grouped in Table 15 and compared to those obtained at the laboratory scale.

obtained on a pilot scale compared to those obtained at the laboratory scale

No significant change in D _¾ has been reported. MET images showed that my microparticles retained their hexagonal structures. Example 25 Manufacture of Microparticles with a Mixture of Two Polysaccharides

Table 16: Hydrodynamic diameters of microparticles composed of a mixture of O-.

palmitoyl-chitosan and O-palmitoyl-dextran

Table 17: Hydrodynamic Diameters of the Microparticles Comprising a Mixture of O-Palmitoyl-Chitosan and O-Palmitoyl-Pullulan

Table 18: Hydrodynamic Diameters of Microparticles Comprising a Mixture of O-Palmitoyl-Chitin and O-Palmitoyl Dextran

Table 20: Hydrodynamic Diameters of the Microparticles Comprising a Mixture of O-Palmitoyl-Chitin and O-Palmitoyl-Pullulan

Example 26: Antiviral activity of nanoparticles composed of O-palmitoyl heparin Cells. Kidney epithelial cells extracted from an African green monkey (cells

Vero, (ATCC CCL-81), Hep-2 and (ATCC CCL-23) human epithelial cells and kidney epithelial cells extracted from an African green monkey (MA-104, ATCC CRL-2378.1) are grown in monolayers. in Eagle's Minimum Essential Environment (MEAT) (Gibco BRL, Gaithersburg, MD) supplemented with 10% heat-inactivated fetal bovine serum and 1% antibiotic-antifungal solution (Zell Shield, Minerva Biolabs GmbH, Berlin, Germany). The 293TT cell line, derived from human kidney embryonic cells transformed with simian virus 40 large T antigen (SV40), is cultured in Dulbecco's Modified Minimal Eagle Medium (DMEM) (Gibco-BRL, Gaithersburg, MD). ) supplemented with 10% fetal bovine serum (FCS; Gibco-BRL), 1% Glutamax-I (Invitrogen, Carlsbad, CA) and 1% non-essential amino acids (Sigma Aldrich, Steinheim, Germany). 293TT cells allow the expression of a high level of proteins from vectors containing the SV40 origin of replication due to over-replication of the expression vectors (Buck et al, 2004).

Virus. Clinical isolates of HSV-1 and HSV-2 have been provided by Professor M. Pistello (University of Pisa, Italy). The HSV-1 and HSV-2 strains were propagated and titrated by the Vero cell plate technique. The RSV strain A2 (ATCC VR-1540) was propagated and titrated by the Reed-Muench method on Hep-2 cells described previously (Donalisio et al, 2012). The human rotavirus strain Wa (ATCC VR-2018) was active with 5μg / ml with porcine type IX pork trypsin (Sigma, St. Louis, Mo.) for 30 min at 37 ° C and propagated in patients. MA104 cells using MEM medium containing 0.5 μg trypsin per ml as previously described (Coulson et al, 1986). Virus stocks were kept frozen (-80 ° C).

HPV PsV production. Plasmids and 293TT cells used for pseudovirus (PsV) production were provided by John Schiller (National Cancer Institute, Bethesda, MD). The protocol details and plasmid maps of this study can be found at the following link: http://home.ccr.cancer.gov/lco/default.asp. HPV-16 pseudoviruses were produced according to previously described methods (Buck et al, 2005). Briefly, 293TT cells are transfected with plasmids expressing the major and minor capsid proteins of papillomavirus (respectively L1 and L2) and a reporter plasmid expressing secreted alkaline phosphatase (SEAP), pYSEAP. The capsids were matured overnight in a cell lysate, the clarified supernatant was then loaded over a density gradient of 27 to 33 to 39%, Optiprep (Sigma-Aldrich, St. Louis, MO), at room temperature for 4 hours. The material was then centrifuged at 340,000 g for 3.5 hours at 16 ° C in an SW50.1 rotor (Beckman Coulter, Inc., FuUerton, CA) and then collected by puncture at the bottom of the tubes. Fractions are assayed for purity in glycine-10% Tris-Sodium Dodecyl Sulfate (SDS) gels, titrated on 293TT cells for SEAP detection, and then pooled and frozen at -80 °. C for the desired duration. The L1 protein content of PsV stocks was determined by comparison with standard bovine serum albumin on SDS-polyacrylamide gels stained with Coomassie Blue.

EXAMPLE 27 Absence of Particle Formation Using the Derivatives of β-Cyclodextrin and O-Palmitoyl-Chitosan (CM12)

Table 22: Absence of Particle Formation by Mixing O-Palmitoyl-Chitosan

(CM12) with ΓΗΡ-β-CD or Με-β-CD Example 28 Absence of Particle Formation Using the Derivatives of β-Cyclodextrin and O-oleoyl-Chitin

Table 23: Absence of _x formation

O-oleoyl-chitin

Example 29 Absence of Particle Formation Using p-Cyclodextrin and O-Palmitoyl-Pullulan Derivatives

Table 24: Absence of Particle Formation Using the β-Cyclodextrin and O-Palmitoyl-Pullulan Derivatives Example 30 Preparation and Characterization of O-Palmitoyl Microparticles-Hyaluronic Acid

O-palmitoyl-hyaluronic acid and Γα-cyclodextrin are weighed in a bottle. Subsequently, the water is added to the mixture. The whole is mixed for 72 hours at room temperature. The concentration of α-cyclodextrin and the results of measurements of the hydrodynamic diameters are shown in Table 25.

compounds (-palmitoyl-hyaluronic acid Example 31: Encapsulation of active ingredients in the presence of a solvent

The protocol adopted for encapsulating the hydrophobic active principles is to dissolve the active ingredient in an ethanol / water mixture at an initial concentration as indicated in Table 26 and then to add the amphiphilic polysaccharide and α-cyclodextrin. The mixture is kept under magnetic stirring for 3 days. After the 3 days of mixing, the concentration of the active ingredient that has not been encapsulated is determined in the supernatant of the preparation. The supernatant is separated either by simple sedimentation or by centrifugation of the microparticles, or after ultracentrifugation in the case of nanoparticles.

Table 26: Example of encapsulated active molecules.

Claims

An inclusion complex according to claim 1 formed by the interaction between at least

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinan, polymannuronic acid, and derivatives thereof, said polysaccharide having hydrophobic groups selected from alkyl groups, linear or branched, containing from 2 to 1000 carbon atoms, or linear or branched, especially linear alkenyl groups, which may contain at least 1 double bond C = C, said hydrophobic groups being covalently bonded to said polysaccharide,

And an α-cyclodextrin (CD) in the form of a monomer,

the polysaccharide and the cyclodextrin being non-covalently bound.

2. Inclusion complex according to claim 1 wherein the polysaccharide is composed of at least 3 saccharide units, its molar mass being in particular between 100 Da to 1000000 kDa, and in particular equal to 20 kDa, 145 kDa or 250 kDa ,

and in particular in which the degree of substitution of the polysaccharide by the hydrophobic groups is between 0.001 and 100%, in particular between 0.05 and 50%.

3. Inclusion complex according to claim 1 or 2 wherein the ratio between the concentration of the cyclodextrin in g / L and that of the polysaccharide is from 10 ^"6 to 900,000, in particular from 4 to 15, and especially equal to to 10.

An inclusion complex according to claim 1 to 3 wherein:

the polysaccharide is a chitosan carrying hydrophobic groups at oxygen atoms originating from -OH groups and / or -CH ₂ OH groups attached to the chitosan ring, and having the formula

in which

■ R represents

• a hydrogen atom, or

• a group of

in which

R ⁴ represents the hydrophobic group and is chosen from:

A linear or branched alkyl group containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₁ -CH ₃ or - (CH ₂ ) ₁₆ -CH ₃ ,

A linear or branched alkenyl group containing 2 to 1000 carbon atoms and containing at least one C doubleC double bond, in particular the groups - (C¾) 7 -CH =CH-CH ₂ - (CH ₂ ) ₇ -CH ₃ or - CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ .with the proviso that R represents at

minus a group of formula

m m represents the number of units of D-glucosamine units,

N represents the number of units of N-acetyl-D-glucosamine units,

* and Γα- cyclodextrin CD

in which

P is equal to 6, 1 2 3

^• R, R and R, identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, chosen from methyl, ethyl, propyl, isopropyl, amino -NH ₂ groups, ammonium groups -NH ₃ ⁺ , or sulfate groups -SO4 ^{2 "} , and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

and in particular in which the cyclodextrin is functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins, biotin or its derivatives.

5. Inclusion complex according to one of claims 1 to 3, wherein

in which

^D R ⁴ has the meanings given in claim 4,

D * represents dextran,

■ the cyclodextrin is the a-CD,

or wherein the polysaccharide is hyaluronic acid bearing hydrophobic groups, attached by oxygen atoms of said hyaluronic acid and representing groups of formula

in which

R ⁴ has the meanings given in claim 4,

n * represents hyaluronic acid,

■ the cyclodextrin is the a-CD,

or wherein the polysaccharide is an amylopectin having hydrophobic groups attached by oxygen atoms of said amlopectin and representing groups of formula

in which ⁿ R ⁴ has the meaning designated in Claim 4,

* * Represents an amylopectin,

■ the cyclodextrin is Γ a-CD,

or wherein the polysaccharide is a pullulan bearing hydrophobic groups attached by oxygen atoms of said pullulan and representing groups of formula

* O - ^^ R ⁴

O

in which

R ⁴ has the meanings given in claim 5,

* * Represents pullulan,

■ the cyclodextrin is Γ a-CD,

or wherein the polysaccharide is a heparin bearing hydrophobic groups attached by nitrogen atoms of said heparin and representing groups of formula

in which

R ⁴ has the meanings given in claim 4,

* * Represents heparin,

or in which the polysaccharide is a heparin bearing hydrophobic groups attached by oxygen atoms of said heparin, these oxygens possibly coming from the hydroxyl or carboxyl groups of heparin, and representing groups of formula

in which

^D R ⁴ has the meanings given in claim 4,

α * represents heparin,

■ and the cyclodextrin is Γ a-CD,

or wherein the polysaccharide is a carrageenan having hydrophobic groups attached by nitrogen atoms of said group having groups of formula in which

° R ⁴ has the meanings given above,

* * Represents carrageenan,

. Or else the polysaccharide is a carrageenan bearing hydrophobic groups attached by oxygen atoms of said carrageenan, these oxygens possibly coming from hydroxyl or carboxyl groups of carrageenan, and representing groups of formula

in which

° R ⁴ has the meanings given above,

D * represents carrageenan,

■ and the cyclodextrin is Γ a-CD.

6. Particle size ranging from 1 nm to 100000 nm containing inclusion complexes according to claims 1 to 5 by interaction between at least

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, cellulose derivatives, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyguluronic acid, xanthan, arabinane, polymannuronic acid, and derivatives thereof, comprising hydrophobic groups selected from linear or branched alkyl groups or linear or branched alkenyl groups and carrying from 1 to 4 C = C double bonds, conjugated or otherwise, said hydrophobic groups being covalently bonded to said polysaccharide, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives,

An α-cyclodextrin in the form of a monomer, optionally functionalized with a ligand chosen from antibodies, antibody fragments, receptors, lectins or biotin or its derivatives.

7. encapsulation system containing one or more particles according to claim 6, and a substance used for its properties in the pharmaceutical, medical, paramedical, medical devices, cosmetic, veterinary, food, food animal, agrochemical, pesticides, cosmeto-textiles, perfumery, environmental, including water depollution, in the paint, building and / or automobile industry.

A pharmaceutical composition containing as an active substance a substance encapsulated in inclusion complexes according to one of claims 1 to 5 or in particles according to claim 6, in association with a pharmaceutically acceptable carrier, in solid form, or as a solution or suspension in a physiological medium, usable by the routes:

parenteral, oral, cutaneous, subcutaneous, nasal, pulmonary or ocular and, for any administration at the level of a mucous membrane,

especially in the form of pills (tablets), soft capsules, hard capsules (capsules), powders, granules, soluble or dispersible tablets, patch, implant, suppositories, solutions, suspension, syrup, pastes, creams, gels, emulsions, sprays, lotions , or ointments.

9. Process for the preparation of an inclusion complex according to claims 1 to 5, comprising a step of mixing at least:

And an α-cyclodextrin (CD) in monomeric form, preferably in suspension in a solvent, in particular water,

and in particular comprising a mixing step

A polysaccharide chosen from chitosan, dextran, hyaluronic acid, amylose, amylopectin, pullulan, heparin, chitin, heparan sulfate, dermatan sulfate, keratan sulfate, chondroitin sulfate, cellulose sulfate, dextran sulfate, dextrin sulfate, starch, pectin, alginates, carrageenans, fucan, curdlan, xylan, polyglucuronic acid, xanthan, arabinan, polymannuronic acid, and their derivatives,

said polysaccharide having hydrophobic groups of formula O

in which

- * represents the polysaccharide,

- R ⁴ represents

An alkyl group, linear or branched, containing from 1 to 1000 carbon atoms, in particular the groups - (CH ₂ ) ₁₄ -CH 3 or - (CH 2) ₁₆ -CH 3,

• a linear or branched alkenyl group containing from 2 to 1000 carbon atoms and having at least one double bond C = C, such as - (CH ₂₎ ₇ - CH = CH-CH ₂ - (CH ₂₎ ₇ -CH ₃ or - (CH ₂ ) ₇ -CH = CH- (CH ₂ ) ₇ -CH ₃ ,

An α-cyclodextrin (CD) having the formula

in which

P is equal to 6,

R ¹ , R ² and R ³ , identical or different, in particular identical, are hydrogen atoms, alkyl groups having 1 to 3 carbon atoms, selected from methyl, ethyl, propyl, isopropyl, amino groups -NH ₂ , ammonium groups - NH ₃ ⁺ , or sulfate groups -SO ₄ ^{2 -} , and are in particular hydrogen atoms or methyl groups,

said CD being alpha-cyclodextrin (α-CD) in monomeric form,

10. Polysaccharide selected from

II

a pullulan bearing hydrophobic groups having the formula

a hyaluronic acid bearing hydrophobic groups having the formula

a chitin carrying hydrophobic groups having the formula

in which

■ R represents

a hydrogen atom,

a group of formula

in which

■ R ⁴ represents

provided that R represents at least one group of formula

■ m represents the number of N-glucosamine units,

■ n represents the number of N-acetyl-glucosamine units,

provided that the percentage of units n in relation to the total number of units is greater than 50%,

11. Particles according to claim 6, comprising an inclusion complex according to claims 1 to 5 for their use as medicaments, especially as adjuvants for vaccination, treatment of burns, and / or for healing.

12. Particles according to claim 6, comprising an inclusion complex according to claims 1 to 5, for their use in the preparation of medicaments having at least an activity for preventing, inhibiting and / or treating fungal, bacterial, viral and / or parasitic infections on biotic or abiotic surfaces.

13.. Particles according to claim 6, comprising an inclusion complex according to claims 1 to 5 for their use as veterinary medicaments, especially as adjuvants for vaccination.

14. Use of the particles according to claim 6, comprising an inclusion complex according to claims 1 to 5 as a cosmetic agent, especially as an anti-aging agent, depigmenting, healing, moisturizing, perfuming, deodorant, anti-transpirant, cleanser, dye , conservative.

15. Use of the particles according to claim 6 comprising an inclusion complex according to one of claims 1 to 5 for the implementation of a method for preparing devices, including wound dressings, said devices comprising said particles, and being capable of releasing said particles or one or more active substance (s) of interest contained in said particles.