CA2499686C - Solubilising polysaccharides substituted with hydrophilic and hydrophobic groups - Google Patents

Solubilising polysaccharides substituted with hydrophilic and hydrophobic groups Download PDF

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CA2499686C
CA2499686C CA2499686A CA2499686A CA2499686C CA 2499686 C CA2499686 C CA 2499686C CA 2499686 A CA2499686 A CA 2499686A CA 2499686 A CA2499686 A CA 2499686A CA 2499686 C CA2499686 C CA 2499686C
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carbohydrate polymer
solubilising
carbohydrate
groups
polymer
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CA2499686A1 (en
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Ijeoma Uchegbu
Andreas Schatzlein
Ailsa Stewart
Clive Wilson
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University College London
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University College London
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    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08BPOLYSACCHARIDES; DERIVATIVES THEREOF
    • C08B37/00Preparation of polysaccharides not provided for in groups C08B1/00 - C08B35/00; Derivatives thereof
    • C08B37/0006Homoglycans, i.e. polysaccharides having a main chain consisting of one single sugar, e.g. colominic acid
    • C08B37/0024Homoglycans, i.e. polysaccharides having a main chain consisting of one single sugar, e.g. colominic acid beta-D-Glucans; (beta-1,3)-D-Glucans, e.g. paramylon, coriolan, sclerotan, pachyman, callose, scleroglucan, schizophyllan, laminaran, lentinan or curdlan; (beta-1,6)-D-Glucans, e.g. pustulan; (beta-1,4)-D-Glucans; (beta-1,3)(beta-1,4)-D-Glucans, e.g. lichenan; Derivatives thereof
    • C08B37/00272-Acetamido-2-deoxy-beta-glucans; Derivatives thereof
    • C08B37/003Chitin, i.e. 2-acetamido-2-deoxy-(beta-1,4)-D-glucan or N-acetyl-beta-1,4-D-glucosamine; Chitosan, i.e. deacetylated product of chitin or (beta-1,4)-D-glucosamine; Derivatives thereof
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P35/00Antineoplastic agents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/30Macromolecular organic or inorganic compounds, e.g. inorganic polyphosphates
    • A61K47/34Macromolecular compounds obtained otherwise than by reactions only involving carbon-to-carbon unsaturated bonds, e.g. polyesters, polyamino acids, polysiloxanes, polyphosphazines, copolymers of polyalkylene glycol or poloxamers
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/20Pills, tablets, discs, rods
    • A61K9/2004Excipients; Inactive ingredients
    • A61K9/2022Organic macromolecular compounds
    • A61K9/2031Organic macromolecular compounds obtained otherwise than by reactions only involving carbon-to-carbon unsaturated bonds, e.g. polyethylene glycol, polyethylene oxide, poloxamers

Abstract

This invention relates to novel carbohydrate polymers with hydrophobic and hydrophilic side-groups suitable for solubilising, for example, hydrophobic drugs. The chain length of the carbohydrate polymeric backbone, and the type and number of the hydrophobic and hydrophilic side-groups are specifically chosen to improve the solubility properties of the carbohydrate polymers.

Description

SOLUBILISING POLYSACCHARIDES SUBSTITUTED WITH
HYDROPHILIC AND HYDROPHOBIC GROUPS
FIELD OF THE INVENTION
This invention relates to novel carbohydrate polymers with hydrophobic and hydrophilic side-groups suitable for solubilising, for example, hydrophobic drugs. The chain length of the carbohydrate polymeric backbone, and the type and number of the hydrophobic and hydrophilic side-groups are specifically chosen to improve the solubility properties of the carbohydrate polymers.
BACKGROUND OF THE INVENTION
Soluble polymers bearing pendant amphiphilic or hydrophobic groups, commonly known as polysoaps, have been studied for a number of years and numerous applications proposedl based on exploiting their solubilisation capacity for hydrophobic molecules ~' 3. These compounds form intramolecular micelles4'5, usually several per molecule6, and their solubilisation capacity is not lost on dilutionl unlike small molecular weight micelles, making them especially useful as solubilisers. Although these molecules are well known they have not been exploited to any great extent as pharmaceutical solubilisers.
Hydrophobic drugs are those drugs, which are practically insoluble in water. The definition of "practically insoluble" used by the British Pharmacopoeia is used here and is defined as a situation where 1g of such material requires more than 10,000 millilitres of solvent (e. g. water) to be solubilised$ or alternatively a material which has a solubility of less than 0.lmg mL-1 in water.
A few pharmaceutical solubilisers have been reported using hydrophobically and hydrophilically modified chitosans, namely: N-aryl 6-sulphated chitosanslo, quaternary ammonium palmitoyl glycol chitosan$ and alkylated ~~~T~G~ 260 / ~ (~ 4 0 6 2 poly(L-lysine citramide)11, although the effects of depolymerisation of the carbohydrate backbone was not explored in the work done on these carbohydratess' 9' 11.
However, two different molecular weights of N-lauroyl 6-carboxymethyl chitosan, with one molecular weight class being investigated at two different levels of lauroyl and carboxymethyl substitution, have been reported by Miwa and othersll as "micellar" carriers of the hydrophobic drug paclitaxel. The paclitaxel formulation described by these workers however is prepared by the probe sonication of N-lauroyl 6-carboxymethyl chitosan and paclitaxel in a 10%v/v ethanol solution. The removal of ethanol by dialysis was attempted but not confirmed by these workers and final N-lauroyl 6-carboxymethyl chitosan - paclitaxel formulations were described as "turbid" with particle size ranges of between 30 and 300nm and a mean particle size of between 32 and 82nm. In contrast, the invention disclosed herein relates to the.attributes of a solubilising polymer which produces optically clear solutions (devoid of appreciable light scattering) when hydrophobic drugs are added to an aqueous phase (devoid of organic solvents) in the presence of the solubilising polymer. Miwa and others on the other hand report that the precursor to N-lauroyl 6-carboxymethyl chitosan which contains no hydrophobic chain -carboxymethyl chitin "yielded a clear solution and the scattering phenomena detected in the case of micellar solution were not observed in the carboxymethyl chitin solution"11. The present invention thus differs from that reported by Miwa anal othersll in that an aqueous optically clear solution is prepared from the polymer and appropriate concentrations of poorly soluble drugs. Organic solvents are also not required in the preparation of the present solutions.
Hydrophobically modified chitosans soluble in dilute acid solutions have also been reportedlz, ls. Other hydrophobically modified carbohydrates have been reported to yield particulatel4''-9 dispersions in aqueous media as opposed to water soluble materialsl3 - namely palmitoyl glycol chitosani4, 15, deoxycholic acid modified chitosanl6, ~~
and cholesterol bearing pullulansl8, 19 or alternatively aqueous insoluble gel-like materialsz°' zl.
G~h.ile the advantageous influence of depolymerisation, controlled hydrophilic substitution, and controlled hydrophobic substitution of carbohydrates on the production of an optically clear solution with hydrophobic drugs has not previously been described, reports on the individual influences of depolymerisation, hydrophobic substitution and hydrophilic substitution on polymer behaviour can be found in the literature. There is an indirect relationship between the length of hydrophobic pendant groups and water solubility in the case of hydrophobised starcheszz and hydrophobised ethyl celluloses~°. This parameter also has a direct influence on the degree of polymer aggregation when in solution in the case of amphiphilic chitosans9 and dextransz3 as well as on the solubilising properties of hydrophobically modified chitosans9. The degree of hydrophobic substitution has also been reported to have an indirect influence on the aqueous solubility of starch derivatives2z and affects the flow properties of hydroxypropyl guar gums.
The balance of hydrophobic and hydrophilic substitution has also been reported to affect a number of polymer properties. An increase in hydrophobic substitution from 20 substituents in every 100 monomers to 90 substituents in every 100 monomers with an associated decrease in the level of carboxymethyl substituents from 200 substituents in. every 100 monomers to 240 substituents in every 100 monomers decreased the association of paclitaxel with the N-lauroyl 6-carboxymethyl chitosan colloidsll, indicating that a more hydrophobic polymer promoted association of paclitaxel with the chitosan based colloid. The balance between the level of hydrophobic and hydrophilic modification also affected the flow properties of amphiphilic hydroxyethylcelluloses24 and an optimum hydrophobic modification level for amphiphilic chitosans has been identified when these materials are used to prevent wool shrinkage during washings.
With regard to amphiphilic polymer molecular weight alone this has been shown to have an indirect effect on the emulsifying activity of hydrophobised starches~6 and an optimum molecular weight has been identified for amphiphilic chitosans bearing deoxycholic acid pendant groups in the context of DNA - chitosan nanoparticles fabricated for gene delivery'. Also the molecular weight of hydrophobised (C6-aryl) dextrans influenced the phase separation of these systems with the high molecular weight material being more likely to phase separate23. The molecular weight of hydrophobic hydroxypropyl guar gums28 was found to influence their flow properties. However, the molecular weight of N-lauroyl 6-carboxymethyl chitosan polymers did not affect their ability to encapsulate paclitaxel within. the chitosan based colloidll.
Returning to the work of Zhang and others on aryl dextrans23, the main purpose of this work was to "prepare a family of polymer pairs in which the compatibility in aqueous solution could be varied in subtle ways" with a view to applying the results to the development of adhesives. The authors conclude that the tendency for dextran and hydrophobically modified dextran to phase separate increases with molecular weight, degree of hydrophobic substitution and hydrophobic chain length23. It should be noted that Zhang and others~3 did not explore the effect of molecular weight on the phase separation of hydrophobically and hydrophilically modified dextrans.
It is an object of embodiments of the present invention to obviate or mitigate at least one or more of 5 the aforementioned problems.
It is a further object of embodiments of the present invention to provide a polymer for solubilising hydrophobic materials such as drugs.
SUi~IARY OF THE INVENTION
According to a first aspect of the present invention there is provided a solubilising carbohydrate polymer of average molecular weight of about 2 - 30 kD according to the following formula:
CH20R' CHZOR"
__O.__ O __O___ _ HO HO
N+
R~ ~~R, wherein m is 0.010 to 10.OOa;
n is 0.010 to 99.980;
p is O.OOo to 99.980;
X is any linear or branched, substituted or unsubstituted, or cyclo form of an alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol or acyl group;
R~ , R~ ~ , R~ ~ ~ are independently any linear or branched, substituted or unsubstituted, or cyclo form of an alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol, acyl group, any sugar substitutent or oligo polyoxa C1 - C3 alkylene units; and R1, R2 and R3 are independently any linear or branched, substituted or unsubstituted, or Cyclo forms of any alkyl, alkenyl, alkynyl, aryl or acyl group.
It is understood that m + n + p will be equal to 100%.
5. It should also be understood that m, n and p may form any arrangement in the solubilising carbohydrate polymer. The arrangement of the m, n and p units may therefore be random or in a block copolymer form such as mnpmnpmnp etC. This is identified in the structure shown above by the dashed line between the different monomer units.
The carbohydrate polymer may be positively charged with a counter ion. The counter ion may be represented by any negative ion. Typically the counter ion may be ions of any of the following: chloride, iodide, acetate and glucoronide.
If the monomer unit identified by n is uncharged (i.e.
the hydrophilic side group is uncharged) then the carbohydrate polymer may loe uncharged and there will therefore be no counter ion.
Typically, X may be selected from any of the following linear or branched, substituted or unsubstituted, or cyclo groups : C1-C3o ; Cs-Cz4 i or C~.z-Cla .
The X group may be selected from any of the following:
any type of fatty acid derivative of, for example, steariC
acid, oleic acid, palmitic acid; N-hydroxysuccinimide acid and any other activated aryl compounds; and anhydrides.
In particular, X may be CH3 (CHI) 14CONH, or CH3 (CHI) 15NH.
Rl, Rz and R3 may independently be any linear or branched, substituted or unsubstituted, or CyClo form of the following alkyl, alkenyl, alkynyl, aryl or aryl groups:
C2-'C30 i C1-C12 i C1"C6 i Or C1 .
Typically, R1, R~ and R3 may be C1 - C4 linear alkyl groups.
Conveniently, all of R1, Rz and R3 may be CH3 .
On some monomers the C2 nitrogen may not be fully substituted and may be present as a secondary or tertiary amine.
R~ , R~ ~ and R~ ~ ~ may independently be any linear or branched, substituted or unsubstituted, or cyclo form of the following alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol or aryl groups: C1-C3o; C1-C1~; and C1-C6.
Typically, R~ , R~ ~ and R~ ~ ~ may be C1 - C4 linear glycol based groups.
Typically, R~ , R~ ~ and R~ ~ ~ are any of the following sugar substituents: glucose, galactose, fructose and muramic acid.
R~ , R~ ~ and R~ ~ ~ may be oligo polyoxa C1 - C3 alkylene units such as ethylene glycol oligomers.
All of R~ , R~ ~ and R~ ~ ~ may be CH20CH2CH20H or CHaCH~OH.
The carbohydrate polymer starting material to which additional hydrophobic and hydrophilic groups are attached may have an average molecular weight of about 2 to 30 kD.
Preferably, the carbohydrate polymer starting material has a molecular weight of about 5 to 17 kD.
Conveniently, the X group may be hydrophobic.
Conveniently, the Rl, RZ and R3 groups form a quaternary ammonium group which is hydrophilic.
Hydrophilic groups are groups, which are well hydrated by water and associate on a molecular level with water. A
further non-ionic hydrophilic group may replace NR1RZR3, providing R~ , R~ ~ and R~ ~ ~ are equal to CHaO-Y and Y is a hydrophilic substituent. In that case both hydrophilic substituents on the carbohydrate polymer may be selected from mono and oligo hydroxy C1-C6 alkyl, mono and oligo hydroxy substituted C2-C6 acyl, C1-C2 alkoxy alkyl optionally having one or more of the hydroxy groups substituted on the alkoxy or alkylene groups, oligo or poly-(oxa C1-C2 alkylene), preferably polyethylene glycol comprising up to 120 ethylene oxide units (i.e. a molecular weight of 5,000), and C1-C4 alkyl (oligo or poly oxa C1-C3 alkylene) optionally hydroxy substituted preferably oligo or polyglycerol ethers; wherein the replacement group for NR1RZR3 is joined via an ether linkage to a saccharide unit of the polysaccharide. The aryl group may contain alkyl, alkenyl or alkynyl groups.
The R' , R~ ~ and R~ ~ ~ groups may also be hydrophilic .
Typically, the ratio of m:n:p may have the following range: 0.1:1:98.9 to 9:91:0; 1:5:96 to 8:50:42; or 3:10:87 to 5:19:76.
The total number of monomer units of m+n+p may be about 10 to 100. Preferably, the total number of monomer units of m+n+p may be less than about 200.
Typically, the number of X groups may not exceed 10 for every 100 monomer groups in the carbohydrate backbone.
The solubilising carbohydrate polymer may also contain additional targeting groups such as peptides, antibodies and other ligands, for example, folate and transferrin ligands which may allow the polymer to target endogenous receptors and thus target its drug payload to such endogenous receptors at the site of pathology.
According to a second aspect of the present invention there is provided a method of forming a solubilising carbohydrate polymer according to the first aspect wherein the method comprises;
depolymerising a carbohydrate polymer to form depolymerised carbohydrate;
reacting the depolymerised carbohydrate with a first reactive compound to form hydrophobic side-groups on the carbohydrate backbone and thus form hydrophobically substituted depolymerised carbohydrate; and adding a second reactive compound to the hydrophobically substituted depolymerised carbohydrate to quaternarise an amine group and thereby form the solubilising carbohydrate polymer.
The carbohydrate polymer may be selected from the following: glycol chitosans, dextrans, alginic acids, starches, dextran, guar gums and all other carbohydrate polymers.
The carbohydrate polymer may be depolymerised with any of the following: an acid, a base, or enzyme.
The acid used to depolymerise the carbohydrate polymer may be selected from any of the following: HC1, H~S04, HN03 or HF.
The carbohydrate polymer may be depolymerised for a few days, for example, 48 hours, then isolated and subjected to further depolymerisation dependent on the average molecular weight of solubilising carbohydrate polymer required.
The average molecular weight of carbohydrate polymer to be depolymerised is about 3 to 30 kD and is preferably about 15 kD.
The first reactive compound which forms the hydrophobic side-groups on the depolymerised carbohydrate polymer may be selected from any of the following: any type of fatty acid derivative of, for example, stearic acid, oleic acid, palmitic acid; organo halides such as alkyl, alkenyl, alkynyl, cyclic or non-aromatic halides, acyl chlorides, anhydrides, N-hydroxysuccinimide and other activated acyl compounds capable of being attacked on the C1 carbon by a compound capable of nucleophilic attack. By nucleophilic attack is meant compounds which attack atoms with a low electron density. The aryl groups may also contain an alkyl, alkenyl or alkynyl group.
Preferably, the first reactive compound which forms the hydrophobic side-groups on the depolymerised glycol chitosan may be selected form any of the following:

hexadecyl bromide, dodecyl bromide, myristic acid N-hydroxysuccinimide.
Preferably, the fatty acid derivative may be palmitic acid N-hydroxysuccinimide; palmitic acid benzotriazole 5 carbonate; palmitaldehyde; palmitoyl chloride; and palmitic acid p-nitro phenyl carbonate.
The second reactive compound may be an organo halide wherein the organo may be selected from any linear or branch, substituted or unsubstituted, or cyclo form of any 10 alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol or acyl group.
Typically, the second reactive compound may be any linear or branched, substituted or unsubstituted, or cyclo form of the following alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol or aryl groups: C1-C3p; C1-C12; C~-C6; or C1.
Typically, the organo group of the organo halides may be short chain linear alkyl groups.
The organo group of the organo halides may be CH3.
The solubilising carbohydrate polymer obtained may be purified by column chromatography, dialysis and freeze drying.
According to a third aspect of the present invention there is provided a carbohydrate polymer according to the first aspect and a pharmaceutically acceptable carrier.
Pharmaceutically acceptable carriers are well known to those skilled in the art and include, but are not limited to, 0.1 M, or preferably 0.05 M phosphate buffer or 0.9%
saline. Additionally, such pharmaceutically acceptable carriers may be aqueous or non-aqueous solutions, suspensions, arid emulsions. Examples of non-aqueous solvents are propylene glycol, polyethyleneglycol, vegetable oils such as olive oil, and injectable organic esters such as ethyl oleate. Aqueous carriers include water, alcoholiclaqueous solutions, emulsions or suspensions, including saline and buffered media.
Parenteral vehicles include sodium chloride solution, Ringer's dextrose, dextrose and sodium chloride, lactated Ringer's or fixed oils. Preservatives and other additives may also be present, such as, for example, anti-microbial, anti-oxidants, chelating agents, inert gases and the like.
Typically, the ratio of carbohydrate polymer to pharmaceutical acceptable carrier ranges from 0.05 wt. % to o.
wt.
10 According to a fourth aspect of the present invention there is provided a pharmaceutical composition comprising a carbohydrate polymer according to a first aspect and a drug .
The drug may be poorly soluble in aqueous solvents such as water.
The drug may be selected from any of the following:
prednisolone; cyclosporine; oestradiol, testosterone, drugs with multicyclic ring structures which lack polar groups such as paclitaxel and drugs such as etoposide.
Typically, the ratio of carbohydrate polymer to the drug may be 10 wt. % . 5000 wt. o.
Typically, the ratio of carbohydrate polymer to drug to pharmaceutically acceptable carrier may be about 1 mg .
1-5 mg . 1 g.
The pharmaceutical composition may be in the form of any of the following: tablets, suppositories, liquid capsule, powder form, or a form suitable for pulmonary delivery.
When tablets are used for oral administration, typically used carriers include sucrose, lactose, mannitol, maltitol, dextran, corn starch, typical lubricants such as magnesium stearate, preservatives such as paraben, sorbin, anti-oxidants such as ascorbic acid, a-tocopheral, cysteine, disintegrators or binders. When administered orally as capsules, effective diluents include lactose and dry corn starch. A liquid for oral use includes syrup, suspension, solution and emulsion, which may contain a typical inert diluent used in this field, such as water, in addition, sweeteners or flavours may be contained.
Suppositories may be prepared by admixing the compounds of the present invention with a suitable non-irritative excipient such as those that are solid at normal temperature but become liquid at the temperature in the intestine and melt in the rectum to release the active ingredient, such, as cocoa butter and polyethyleneglycols.
The dose can be determined on age, body weight, administration time, administration method, combination of drugs, the level or condition of which a patient is undergoing therapy and other factors. While the daily doses may vary depending on the conditions and body weight of patients, the species or active ingredient, and administration route, in the case of oral use, the daily doses may be about 0.1-2 mg/person/day, preferably 0.5-100 mg/person/day.
According to a fifth aspect of the present invention there is provided a method of dissolving poorly soluble drugs in a carbohydrate polymer wherein the solubilising carbohydrate polymer has a specifically designed average molecular weight, and specific type and amount of hydrophilic and hydrophobic side-groups substituted on a carbohydrate polymeric backbone whereby on dissolving a poorly soluble drug in the solubilising carbohydrate polymer a substantially clear solution is obtained.
By substantially optically clear solution herein is meant an optically clear solution which is devoid of appreciable light scattering and is clear to the naked eye.
By poorly soluble drugs is meant where one gram of a drug requires more than 10,000 ml of solvent (waterj to be solublised. Alternatively, this means a drug which has a solubility of less than 0.1 mg mL-1 in water.
Typically, the solubilising carbohydrate polymer is selected from any derivatives of the following: chitosans, dextrans, alginic acids, starches, dextran, guar gums and all other carbohydrate polymers.
Tn particular, the carbohydrate polymer according to the first aspect may be used.
The poorly soluble drug may be selected from any of the following: cyclosporin, steroids such as prednisolone, oestradiol, testosterone, drugs with multicyclic ring structures which lack polar groups such as paclitaxel and drugs such as etoposide.
BRIEF DESCRIPTION OF THE DRA~nIINGS
Embodiments of the present invention will now be described, by way of example only, with reference to the accompanying drawings in which:
Figure 1a is a representation of quaternary ammonium palmitoyl glycol chitosan (GCPQ);
Figure 1b is a representation of quaternary ammonium hexadecyl glycol chitosan (GCHQ);
Figure 2a is a representation of the haemolytic activity of GCPQ prepared from glycol chitosan which has been subjected to an initial 48 hours acid degradation and a further 8 hours acid degradation, followed by acylation with palmitic acid N-hydroxysuccinimide and alkylation with methyl iodide (i.e. GCPQ488);
Figure 2b is a representation of the haemolytic activity of GCPQ488 and cyclosporine in a 1:1 ratio;
Figure 2c is a representation of the haemolytic activity of GCHQ prepared from glycol chitosan which has been subjected to an initial 48 hours acid degradation and a further 8 hours degradation, followed by alkylation with hexadecyl bromide and alkylation with methyl iodide (i.e.
GCHQ4$8);
Figure 2d is a representation of the haemolytic activity of GCHQ488 and prednisolone in a 1:5 ratio;
Figure 3a is a representation of the cyctotoxicity to A549 cell lines after incubation with GCPQ488;
Figure 3b is a representation of the cyctotoxicity to A549 cell lines after incubation with GCPQ488 and cyclosporine;
Figure 3c is a representation of the cyctotoxicity to A549 cell lines after incubation with GCHQ488;
Figure 3d is a representation of the cytotoxicity to A549 cell lines after incubation with GCHQ488 and prednisolone in a 1:5 ratio;
Figure 3e is a representation of the cyctotoxicity to A431 cell lines after incubation with GCPQ488 and cyclosporine;
Figure 3f is a representation of the cyctotoxicity to A431 cell lines after incubation with GCHQ488; and Figure 3g is a representation of the cyctotoxicity to A431 cell lines after incubation with GCHQ488 and prednisolone in a 1:5 ratio.
EXAMPLES
Example 1 Materials Glycol chitosan, palmitic acid N-hydroxysuccinimde, methyl iodide, 1-bromohexadecane, pyrene and paclitaxel were all obtained from Sigma Aldrich Co, UK. Prednisolone acetate, prednisolone and cyclosporine were all obtained from Allergan, USA. Hydrochloric acid was obtained from Merck, UK and all organic solvents were purchased from the Department of Pure and Applied Chemistry, University of Strathclyde.
METHODS
Degradation of glycol chitosan (GC) 5 Acid degradation of glycol chitosan (GC) was carried out as previously describedl5. Glycol chitosan (2g) was dissolved in hydrochloric acid (4 M, 150 mL) and the solution filtered to remove insoluble impurities. The filtered solution was placed in a pre-heated water bath set 10 at 50°C. After 48h the reaction was stopped and the products isolated and purified as described below. The reaction solution was exhaustively dialysed (Visking Seamless Cellulose Tubing, molecular weight cut off -12,400 for cytochrome c) against distilled water (5 L with 15 6 changes over 24h). The dialysate at the end of the dialysis procedure had a neutral pH. The dialysate was subsequently freeze-dried and the material was recovered as cream coloured cotton wool like material. The acid degradation step was repeated for either 4h, 8h, 24h or 48h to give materials, which were further depolymerised.
Synthesis of low molecular weight palmitoyl glycol chitosan (PGC) Palmitoyl glycol chitosan (PGC) was synthesised as previously describedl4. Glycol chitosan (500mg), sodium bicarbonate (376mg) in a mixture of absolute ethanol (24mL) and water (76mL) was reacted with palmitic acid ~N
hydroxysuccinimide (198mg) in absolute ethanol (150mL).
Palmitic acid N-hydroxysuccinimide solution was added drop wise. The product was isolated after stirring for 72h by evaporating off most of the ethanol, extraction of the remaining liquid Wlth three volumes of diethyl ether (100mL), exhaustive dialysis against water and freeze dried to give a white cotton wool like solid.
Synthesis of low molecular weight hexadeayl glycol chitosan tGCH) Hexadecyl glycol chitosan (GCH) was synthesised based on a modification of the method of Wakita and Hashimotoa9.
Glycol chitosan (500mg) was dissolved in a 1:1 mixture of methanol and N-methyl pyrrolzdinone (20mL) and to this was added drop wise a solution of sodium bicarbonate (376mg) dissolved in absolute ethanol (20mL). 1-bromhexadecane (3.5mL) was freshly dissolved in a mixture of methanol, N-methyl pyrrolidinone, absolute ethanol (5mL:5mL:10mL) and this solution was added to the basic glycol. chitosan solution drop wise over a 1h time period. The resulting reaction mixture was refluxed at 70-85°C in an oil bath with stirring over a period of 4 hours and then filtered and the filtrate retained. The ethanol was then evaporated off under reduced pressure at 50°C and the residue produced dissolved in distilled water (30mL). This solution was then dialysed against 5L of water with 6 changes over 24 hours and freeze dried to give an off white solid.
Synthesis of low molecular weight quaternary ammonium palmitoyl glycol chitosan (GCPQ) arid low molecular weight quaternary ammonium hexadecyl glycol chitosan (GCHQ) Quaternisation was carried out using essentially the same method as reported by Domard and others3°. PGC or GCH
(300 mg) was dispersed in N-methyl-2-pyrrolidone (25 ml) overnight for 12 h at room temperature. Sodium hydroxide (40 mg), methyl iodide (1.0 g) and sodium iodide (45 mg) were added and the reaction stirred under a stream of nitrogen at 36°C for 3 h. The quaternary ammonium product was recovered by precipitation with diethyl ether, filtered and washed with copious amounts of absolute ethanol followed by copious amounts of diethyl ether to give a brown hygroscopic solid. The solid was dissolved in water (100 ml) to give a yellow viscous solution. The resultant aqueous solution was exhaustively dialysed against water (5L) with six changes over a 24 h period and the product freeze-dried to give a white cotton-like solid which was present as the iodide salt. The quaternary ammonium iodide was then dissolved in water (150 ml) to give a clear solution and the solution passed through a column (1 x 6 cm) packed with Amberlite IRA-93 Cl-. Before use the column was packed with resin and subsequently with one volume of the resin (30 ml) and subsequently washed with hydrochloric acid solution (90 ml, 1 M) followed by distilled water (500 ml) to give a neutral pH. The clear eluate from the column was freeze-dried to give GCPQ as a transparent fibrous solid.
zH NMR
1H NMR scans (with integration) and 1H correlation spectroscopy experiments were performed on GCPQ and GCHQ
samples solubilised in deuterated methanol and the level of palmitoylation and quaternisation determined by integrating the palmitoyl methyl, alkyl methyl or quaternary ammonium methyl peaks relative to the sugar peaks3l. The mole%
palmitoylation, alkylation or quaternisation refers to the number of moles of sugar monomers bearing a palmitoyl, alkyl or quaternary ammonium group per 100 moles of sugar monomers respectively.
MW Determination The molecular weight of degraded glycol chitosan (GC) was determined by GPC-MALLS (i.e. gel permeation chromatography - multi angle laser light scattering).
Polymers were dissolved in an acetate buffer (sodium acetate 0.3M, acetic acid 0.2M) and filtered (0.2~,m) samples (200~.L, 1 - 2mg mL-1) injected onto GPC columns using a Waters 717 plus Autosampler. Samples were chromatographed over a PSS HEMA-BIO 300 (330 X 8mm, particle size = 10 ~,m, exclusion limit for dextran = 5 x 105) and a PSS HEMA-BIO 40 (330 X 8mm, particle size - 10 Vim, exclusion limit for dextran - 3 ~e 106) column (Polymer Standards Services, Mainz, Germany). The mobile phase was an acetate buffer (sodium acetate 0.3M, acetic acid 0.2M) and molecular weights were determined using a DAWN EOS MALLS detector (18 angles at 20 - 150° - Wyatt Technology, USA) equipped with a 30 mV linearly polarized gallium arsenide laser (~,= 690 nm) and an Optilab DSP interferometric refractometer (~,= 690 nm, Wyatt Technology, USA). All the measurements were carried out at room temperature. Molecular weights, molecular weight distribution and molecular size in solution were obtained from GPC graphs using Astra for Windows (v4.73) software.
The refractive index increment (dn/dc) of GC in the mobile phase was measured with an Optilab DSP
interferometric refractometer (~, = 690nm, Wyatt Technology, USA,) at 25°C. A Rheodyne 7725 sample injector was used to load filtered (0.45 ~,m) polymer solutions of various concentrations and the data were processed using DNDC for Windows (v5.31) software.
Fluorescence Spectroscopy A dilute aqueous solution of pyrene (2E.tM) was prepared by initially dissolving pyrene in ethanol (0.4mg/mL). 100,1 of this solution was pipetted into a volumetric flask (100mL) and the ethanol dried under a stream of nitrogen gas. The solution was then made up in distilled water.
Using the aqueous pyrene solution as the solvent, polymer solutions were made at various concentrations. The fluorescence emission spectra were recorded (340nm - 600nm) at an excitation wavelength of 335nm. The I3/ I1 ratio was calculated from the intensity of the third (383nm) and first (375nm) vibronic peaks in the pyrene emission spectra3z and an increase in the size of the I3 peak relative to the I1 peak indicates a more hydrophobic environment32. In polar solvents such as water this value is approximately 0.67.
Solubilisation Studies Various levels of the GCPQ and GCHQ samfles were dissolved in water and a weighed amount of drug added with probe sonication (MSE Soniprep 150, Sanyo, UK with the instrument set at 60 - 85% of its maximum output) for about 5 minutes or until a clear solution is obtained. The presence of a clear solution was verified by optical density measurements (~, - 600nm, UV1 Spectrophotometer, ThermoUnicam, UK). The samples were stored at refrigeration (4 - 8°C) or room (22°C) temperature. At various time intervals liquid samples were filtered (0.45[am, 25mm in diameter) and the first millilitre discarded. The subsequent filtrate was retained and analysed for dissolved drug using HPLC.
Assay for Prednisolone Prednisolone levels were analysed in filtered samples of the polymer - drug formulation by HPLC. Samples (20~,L), appropriately diluted with the mobile phase (acetonitrile, water 36: 64) were injected onto a reverse phase Symmetry C18, 3.5~.m column (4.6mm X 75mm, Waters Instruments, UK) by means of a Waters 717 autosampler and a Waters 515 isocratic pump. Peak detection was via a Waters 486 variable wavelength UV detector with the wavelength set at 243nm and data was Collected using a Waters 746 data module. The mobile phase was set at a flow rate of 1ml miry 1. A standard curve was prepared with samples of prednisolone solubilised in the mobile phase (0.1 - l.Omg 5 Ml-~ ) .
Assa3r For CSraX osporine Cyclosporine was analysed by HPLC on the same instrumentation as above except that the column was a 10 Waters Spherisorb 5~.tm, 4.6mm X 250mm column, maintained at 80°C with a Jones Chromatography Column Heater model 7971.
Filtered Samples (20~.L) dissolved in acetonitrile, water (1:
1) were injected onto the column and the mobile phase was acetonitrile: water: tart-butyl-methyl-ether: phosphoric 15 acid (600:350:50:1) at a flow rate of l.2mL miril. Peaks were detected by UV detection at a wavelength of 210nm. A
standard curve was prepared using solutions of the drug (1 _ 10~g mL_'~) .
20 Haemoaompatibi.Zty~ Studies Approximately 5ml of human blood was centrifuged (1000g x 10 min), the supernatant removed and the erythrocyte pellet recovered. The pellet was washed twice by resuspending in PBS (pH 7.4, 4°C) and centrifuging (1000g x 10 min). The pellet was then weighed and a 3% w/w dispersion of the erythrocytes was prepared in PBS (pH
7.4). 100~.L of this erythrocyte suspension was placed into each well of a 96 well plate. To this erythrocyte suspension was added 100~.L of varying concentrations of the sample formulations. Sample formulations were either prepared in phosphate buffered saline (PBS, pH = 7.4) or water. PBS (pH = 7.4) and Triton X-100 (1% wlv) served as negative and positive controls respectively. The plate was incubated at 37°C for 4h after which the plate was centrifuged (1000g x l0min) and 100~.L of the supernatant removed and placed in a new microtitre plate. The absorbance was measured at 570nm and the results expressed as percentage haemolysis assuming Triton X-100 gave 1000 haemolysis and PBS (pH = 7,4) gave 0% haemolysis.
Cytotoxi,city Studies A human lung carcinoma cell line (A549, ATCC CCL
185) and a human epidermoid carcinoma cell line (A431, ATCC
CRL - 1555) were both maintained in Dulbecco's minimum essential medium (DMEM) supplemented with 10% foetal calf serum (FCS) and 2mM glutamine (GibcoBRL, U.K) at 10% C0~ and 37°C.
To measure the cytotoxicity of the formulations, a standard MTT (3-[4,5-dimethylthiazol-2-yl]2,5-diphenyltetrazolium bromide thiazolyl blue indicator dye) assay was carried out33. 96 well microtitre plates, 1 per formulation, were seeded with about 800 cells per well and incubated at 37°C with 10% C02 for 72 hours. The medium was then removed from the wells and varying concentrations of each formulation (200~,L, prepared in 6% dextrose and diluted in medium) were added to the wells. DMEM alone and Triton X-100 (1ow/v) were used as positive and negative controls respectively. The plates were incubated under the standard conditions for 4 hours and the drug solutions then removed from the wells, replaced with DMEM and the cells further incubated for 72 hours, The indicator dye (50~.L, 50mg mL-1) was then added to the cells, which were subsequently incubated in the dark for a further 4 hours. At the end of the incubation time, the dye was removed and the cells lysed by addition of dimetlzylsulfoxide (200~,L) . To the lysed cells was then added Sorensen's glycine buffer (25~.L) and the absorbance measured at 570nm. Values are expressed as a percentage of the control minus the background obtained from the wells containing just DMEM.
The structures of GCPQ and GCHQ are shown in Figures 1a and 1b, respectively. GCPQ and GCHQ were recovered as white fibrous solids. With the glycol chitosan starting material as has been reported previouslyl5, an increase in the acid degradation time led to an increase in the degree of depolymerisation (Table 1), however after the initial 48h there is a slowing down in the level of depolymerisation (Table 1).
Table 1: Molecular Weights of Glycol Chitosan Samples POLYMER Acid Molecular Polydispersity Degradation Weight (kD) Mw/Mn Time GCO Oh 104 1.05 GC48 48h 19.3 1.20 GC484 48h + 4h 17.9 1.23 GC488 48h +8h 17.2 1.28 GC4824 48h + 24h - -GC4848 48h + 48h 15.2 1.08 The lipidic and quaternary ammonium derivatives of these glycol chitosan polymers are able to solubilise hydrophobic drugs such as prednisolone and cyclosporine in aqueous media as shown in Table 2.
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v~z ~ ~ ~ u ~ a All solutions were clear transparent liquids with optical density readings of less than 0.001 against distilled water which had an optical density of 0.000.
Solutions remained optically clear on dilution ten 5 times with water. These solutions are in contrast to the chitosan - paclitaxel colloids reported by Miwa and othersll where liquids with "turbidity" were obtained and the hydrophobic drug was added to the polymer formulation in the presence of l0ov/v of ethanol, with the removal of 10 ethanol being attempted but not confirmed.
1H NMR was used to quantify the level of quaternisation, acylation and alkylation and a value for the hydrophilicity index (HI) is quoted in Table 2. The HI (derived from the 1H NMR data) is a term used here to characterise the 15 hydrophilicity of the polymers and this value quantifies the relationship between additional ionic hydrophilic substituents and hydrophobic substituents added to a previously aqueous soluble polymer or aqueous soluble polymer derivative. Aqueous soluble polymers are described 20 as polymers soluble in water at a level of above 1mg mL-18.
These carbohydrate polymers may be additionally substituted with non-ionic hydrophilic units as is shown here.
The data in Table 3 shown below, shows that the 25 polymers aggregate in aqueous media to produce hydrophobic domains as evidenced by the increase in the I3/ I1 ratio.
TABLE 3: I3/I1 data for GCPQ and GCHQ Polymers Polymer C
t ti on oncen GCPQ488BGCPQ4824BGCPQ4848BGCHQ488B GCHQ4824B
ra 0 0.67 0.67 0.67 0.67 0.67 0,25 - - 0.91 - -0,5 0.67 0.82 0.88 0.80 0.85 1 0.97 0.85 1.02 0.86 1.02 1.5 1.02 - - 0.91 1.18 2.0 1.28 0.86 0.92 1 1.25 [B merely means a different batch of polymer]
These hydrophobic domains provide areas for the solubilisation of hydrophobic solutes while the hydrophilic substituents increase the affinity of the polymer with the aqueous solvent and prevent phase separation.
As shown in Table 3 the hydrophobicity of the polymer aggregates when present at a polymer concentration of 1mg mL-1 (as determined using a pyrene probe) followed the trend GCHQ4824 = GCPQ4848 > GCPQ488 > GCHQ488 = GCPQ4824. This hydrophobicity ranking obtained by the use of the pyrene probe is similar to the hydrophobicity ranking obtained using the HI: GCPQ4848 - 1.58, GCPQ488 - 3.33, GCHQ488#1 (i.e. different batch of polymer) - 4.22 and GCPQ4824 -4.44. (Table 2). Additionally the maximum level of drug solubilised in the case of the more polar drug prednisolone is solubilised by GCHQ488 (Tables 2&4), one of the more polar polysoaps (Table 2).
TABLE 4: Prednisolone Stability Studies Polymer Polymer Age of Storage Original Prednisolone ConcentrationFormulatiConditionsPrednisoloneDetected (mg mI: on Concentrations(mg mL
l) (mg mL'1) l) GCPQ488 1 25 weeksRT 1.0 0.2 GCPQ488 1 15 weeks4pC 0.75 0.2 GCHQ488 1 12 weeksRT 5.0 4.5 GCHQ488A*1 2 weeks 4C 2.5 2.4 GCHQ488A*1 10 weeks4aC 2.5 2.4 GCHQ488A*1 2 weeks 4QC 5.0 4.4 GCHQ488A*1 10 weeks4QC 5.0 4.3 * = different batch of GCHQ488 Also the least polar polysoaps (with the lowest HI
value) and the highest molecular weight i,e. - GCPQ484 and GCHQ484 are insoluble in water at a level of 1mg mL-1 (Tables 1 and 2).
Relatively high levels of hydrophobicity also hamper (albeit to a lesser extent) the solubilisation of CyClosporine, as evidenced by the rather low maximum levels of cyclosporine solubilised by GCPQ4848 and GCHQ4824. This is shown in Table 5 below.
TABLE 5: Cyclosporine Stability Studies Lymer Polymer Age of Storage Initial Cyclosporine ConcetrationsformulationConditionsLevel Detected of (mg mLi) Cyclosporine (mg mL 1) GCPQ4881 1 day 49C 1 0.95 GCPg4881 3 days 4QC 2 0.92 GCPQ4881 1 week 4qC 2 1.10 GCPQ4881 2 weeks 4QC 1 1.10 GCPQ4881 4 weeks 4QC 1 0.90 GCPg4881 8 weeks 4aC 1 0.80 GCPQ4881 12 weeks 4QC 1 0.70 GCPQ4881 15 weeks 4QC 1 0.80 GCPQ4881 22 weeks 4QC 1 0.70 The solubilising polymer must thus be depolymerised as well as substituted with a controlled number of hydrophobic and hydrophilic moieties. Within the molecular weight range (10 - 20kD), HI (when calculated from the 1H NMR) values of above about 2 appear to be the most efficient polymers in the case of the more polar palmitoyl substituent and HT values above about 3 appear to be the most efficient solubilisers in the case of the less polar hexadecyl substituents (Table 2). Clearly in the case of prednisolone and cyclosporine, a high level of quaternisation and low level of hydrophobic modification favours solubilisation with these polymers (Tables 1 -4) .

With the N-lauroyl 6-carboxymethyl chitosan polymers prepared previouslyll, a shift to a higher level of the carboxymethyl groups and a lower level of lauroyl.groups resulted in a decreased association of paclitaxel with the 5 chitosan based colloid. In the present invention, the ability of the polymer molecule to be fully hydrated by water molecules (presence of ionic quaternary ammonium groups) plays a more important role than the ability of the polymer to aggregate into polymeric micelles (presence of 10 hydrophobic groups) and provide a hydrophobic cavity within which hydrophobic solutes may be shielded.
The solubilising polymer should be prepared from an aqueous soluble and depolymexised carbohydrate and the most effective polymers have a degree of polymerisation of less 15 than 200 monomer units. The solubilising polymer may further have a level of hydrophobic substitution not exceeding 10 substituents per every 100 monomers and finally an additional ionic hydrophilic substitution level of equal to or more than 1 substituent per polymer chain.
20 There may be an optional additional hydrophilic substituent of at least 1 hydrophilic substituent per polymer chain.
Previous work with N-lauroyl 6-carboxymethyl chitosan has shown that there is no increase in the association of paclitaxel with the chitosan based colloid on reducing the 25 degree of polymerisation from a molecular weight of 50kD to 2kD11. However, it is shown. herewith that even small changes in molecular weight affect the solubilising properties of the polymers as evidenced by the data presented on GCPQ484 and GCPQ4848 (Table 2).
30 Finally, in the work described using N-lauroyl 6-carboxymethylchitosan, polymers encapsulating paclitaxel had a level of hydrophobic substitution exceeding 20 substituents per 100 monomers and a minimum level of 140 carboxymethyl groups per 100 monomersll. In contrast the present invention relates to a maximum level of 10 hydrophobic substituents per 100 monomer units.
The solubilising polymer of the present invention may contain additional targeting groups such as peptides, antibodies and other ligands e.g. folate and transferrin ligands which will allow the polymer to target endogenous receptors and thus target its drug payload to such endogenous receptors at the site of pathology.
With the HPLC assays used the retention time of prednisolone was 2.7min and the standard curve had a correlation coefficient of 0.998 while the retention time for cyclosporine was 13.7min and the standard curve had a correlation coefficient of 0.98. Solubilised material was stable for up to 12 weeks with chitosan based polymer formulations retaining up to 9Oo of solubilised drug for this length of time (Tables 4 and 5).
The solubilising polymers presented herein are biocompatible. Solutions of the GCPQ488 and GCPQ488, cyclosporine samples in water resulted in a maximum 40%
cell lysis, while formulations within isotonic PBS (pH -7.4) gave about 10% cell lysis up to a polymer concentration of 1mg mL-1 (Figure 2). The hypotonic water environment is thus responsible for the observed cell lysis. While the inclusion of up to 1mg mL-1 cyclosporine within polymer formulations appeared to protect the cells from lysis (especially in the presence of water as the solvent), the inclusion of 5mg mL-~ prednisolone increased the level of lysis observed with the polymers (Figure 2).
It is concluded that these glycol chitosan polysoaps show no appreciable levels of haemolysis to cells. However, what should be noted here is the observation of drug activity in the presence of the polysoaps.
Below a level of 0.lmg mL-1 none of the glycol chitosan based polysoaps are particularly cytotoxic in both the A431 and the A549 cell lines (Figure 3). However the addition of either prednisolone or cyclosporine does cause the appearance of some cytotoxicity although none of the formulations resulted in the observation of less than 500 cell survival below a polymer concentration of 0.01mg mL-1.
It may be concluded that the glycol chitosan polysoaps are not particularly cytotoxic polymers and any toxicity seen with the drug formulations is largely due to the addition of drug and not due to the toxicity of the polymer per se.
Once again what should be noted here is the observation of drug activity in the presence of the polysoaps.
Example 2 This Example relates to a high throughput method of selection of carbohydrate solubilisers Materials Glycol chitosan, palmitic acid N-hydroxysuccinimide, methyl iodide, N-methyl pyrrolidone, sodium iodide, sodium hydroxide, prednisolone and 6-methyl prednisolone were all obtained from Sigma-Aldrich Co. UK. Absolute ethanol was supplied by Bamford Laboratories, UK and diethyl ether by BDH Laboratories, UK. Acetonitrile was supplied by Riedel de-Haen, Germany.
Me thods Degradation of Glycol Cha.tosan (GC) Glycol chitosan (GC) was degraded for 48h as described abovez5. 25 quaternary ammonium palmitoyl glycol chitosan polymers were synthesised from the degraded material with differing levels of hydrophobic (palmitoyl) and hydrophilic (quaternary ammonium) substitution.
Solutions of palmitic acid N-hydroxysuccinimide (PNS) in ethanol ( 5 . 2 8mg mL-~ ) , sodium iodide ( 2mg mL-1 ) in N-methyl pyrrolidone (NMP), sodium hydroxide in absolute ethanol (l0mg mL-1) , glycol chitosan (l0mg mL'1, GC) in a solution of sodium bicarbonate (7.53mg mL-1) and prednisolone (l0mg mL'1) in methanol were prepared.
25 different polymers were synthesised by adding a solution of palmitic acid N-hydroxysuccinimide at the levels shown in Table 1 to the glycol chito~san - sodium bicarbonate solution (1mL) contained in a 25mL test tube.
The tubes were shaken for 16h at room temperature and subsequently heated at 85°-C for 4h to evaporate off the ethanol.
The residues in the tubes were extracted with diethyl ether (3 X l5mL) to remove unreacted palmitic acid and subsequently washed with absolute ethanol to remove polar contaminants. Ethanol was removed and residual ethanol was dried under a stream of nitrogen. For the quaternisation reaction the solution of sodium iodide in NMP was added to the test tubes in the quantities shown in Table 1. This was followed by the addition of the solution of sodium hydroxide and the addition of methyl iodide in the quantities shown in Table 1.
The tubes were heated for 3h at 36°-C and diethyl ether added to the tubes (5mL). This caused the quaternary ammonium product to precipitate. The supernatant was decanted from the tubes and the residues washed with diethyl ether (3 X 5mL). The residue was then left to dry overnight and water (2mL) subsequently added to each tube to produce polymer solutions known herein as "concentrated polymer solutions". To a separate set of 25 tubes was added 0.lmL of the prednisolone solution in methanol.
Methanol was removed under a stream of nitrogen and to each tube was added a sample of one of the 25 quaternary ammonium palmitoyl glycol chitosan solutions (1mL) from above.
This mixture was probe sonicated (MSE Instruments, Sanyo, UK) filtered using a 0.45[am filter and analysed by high performance liquid chromatography (HPLC). The polymer solutions obtained from the synthesis step above were diluted by adding to 1mL each of the 25 solutions to an additional volume of water (1mL) to produce what are termed here as "dilute polymer solutions" and the prednisolone solubilisation procedure described above repeated once more with a more dilute solution of the synthesised polymer.
Prednisolone levels were analysed in filtered (0.450 samples of the polymer - drug formulation by HPLC. Samples (20~,L), appropriately diluted with the mobile phase (acetonitrile, water 36: 64) and containing 6-methyl prednisolone (l~,g mL-1) were injected onto a reverse phase Symmetry C18, 3.5~m column (4.6mm X 75mm, Waters 5 Instruments, UK) by means of a Waters 717 autosampler and a Waters 515 isocratic pump. Peak detection was via a Waters 486 variable wavelength W detector with the wavelength set at 243nm and data was collected using Waters Empower software. The mobile phase was set at a flow rate of 1ml 10 min-1. A standard curve was prepared with 6-methyl prednisolone (1~g mL-1) as the internal standard and with samples of prednisolone solubilised in the mobile phase ( 0 .1 - 2 0 ~.g mL-1 ) .

Table 6: High throughput polymer synthesis - reagent volumes (mL) T -Increas ing palmitic acid N-Increasing hydroxys uccinimide (hydrophobic methyl iodide substitu tion) (hydrophilic Polymer Polymer Polymer Polymer Polymer substitution) E1 E2 E3 E4 E5 PNS - PNS - PNS - PNS - PNS -0.5 1 2 3 4 NaI - NaI - NaI - NaI - NaI -3.0 3.0 3.0 3.0 3.0 NaOH - NaOH - NaOH - NaOH - NaOH -0.6 0.6 0.6 0.6 0.6 0.062 0.062 0.062 0.062 0.062 Polymer Polymer Polymer Polymer Polymer PNS - PNS - PNS - PNS - PNS -0.5 1 2 3 4 NaI - NaI - NaI - NaI - Na2 -2.5 2.5 2.5 2.5 2.5 NaOH - NaOH - NaOH - NaOH - NaOH -0.5 0.5 0.5 0.5 0.5 0.052 0.052 0.052 0.052 0.052 Polymer Polymer Polymer Polymer Polymer PNS - PNS - PNS - PNS - PNS -0.5 1 2 3 4 NaI - NaI - NaI - NaI - NaI -NaOH - NaOH - NaOH - NaOH - NaOH -0.4 0.4 0.4 0.4 0.4 0.042 0.042 0.042 0.042 0.042 Polymer Polymer Polymer Polymer Polymer B1. B2 B3 B4 B5 PNS - PNS - PNS - PNS - PNS -0.5 1 2 3 4 NaI - NaI - NaI - NaI - NaI -1.5 1.5 1.5 1.5 1.5 NaOH - NaOH - NaOH - NaOH - NaOH -0.3 0.3 0.3 0.3 0.3 0.032 0.032 0.032 0.032 0.032 Polymer Polymer Polymer Polymer Polymer PNS - PNS - PNS - PNS - PNS -0.5 1 2 3 4 NaI - NaI - NaI - NaI - NaI -NaOH - NaOH - NaOH - NaOH - NaOH -0.2 0.2 0.2 0.2 0.2 0.022 0.022 0.022 0.022 0.022 All values are in ml.

Results Table 7: High throughput polymer synthesis - prednisoloae solubilities with concentrated polymer solutions (mg mL-1) T -Increas ing palmitic acid N-Tncreasing hydroxys uccinimide (hydrophobic methyl iodide substitu tion) (hydrophilic Polymer Polymer Polymer Polymer Polymer substitution) E1 E2 E3 E4 E5 0.472 0.613 0.632 - -Polymer Polymer Polymer Polymer Polymer 0.984 0.978 0.828 0.847 0.906 Polymer Polymer Polymer Polymer Polymer Cl C2 C3 C4 C5 0.433 0.374 0.346 0.399 0.374 Polymer Polymer Polymer Polymer Polymer .373 0.166 0.128 0.369 0.367 _ Polymer Polymer Polymer Polymer Polymer 0.598 0.590 - - 0.512 Table 8: High throughput polymer synthesis - prednisolone solubilities with dilute polymer solutions (mg mh"1) T Increas ing palmitic acid N-Increasing hydroxys uccinimide (hydrophobic methyl iodide substitu tion) (hydrophilic Polymer Polymer Polymer Polymer Polymer substitution) E1 E2 E3 E4 E5 0.987 0.830 - - -Polymer Polymer Polymer Polymer Polymer 0.954 0.802 0.847 0.713 0.633 Polymer Polymer Polymer Polymer Polymer 0.831 0.700 0.625 0.776 0.731 Polymer Polymer Polymer Polymer Polymer 0.816 0.785 0.860 0.680 0.626 Polymer Polymer Polymer Polymer Polymer 0.993 0.956 0.691 0.644 0.646 Comment on Results The high through put method outlined above was able to select polymers with a high solubilising ability (e. g.
Polymer E1) for a particular drug which in this case was prednisolone. Polymer E1 may then be synthesised in bulk quantities. Lower concentrations of the polymer (dilute polymer solutions) of about 0.01 - 5m m 1 were superior solubilisers of the model drug than higher concentrations (of about 5 - 10 mg mL-1) of the polymer.

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Claims (45)

1. A solubilising carbohydrate polymer of average molecular weight of about 2 - 30 kD according to the following formula:

wherein m is 0.01% to 10.00%;
n is 0.01% to 99.98%;
p is 0.00% to 99.98%
X is any linear or branched, substituted or unsubstituted, or cyclo form of an alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol or acyl group;
R', R", R'" are independently any linear or branched, substituted or unsubstituted, or cyclo form of an alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol, acyl group, any sugar substituent or oligo polyoxa C1 - C3 alkylene units; and R1, R2 and R3 are independently any linear or branched, substituted or unsubstituted, or cyclo forms of any alkyl, alkenyl, alkynyl, aryl or acyl group;
Wherein the x group is hydrophobic, and wherein the R1, R2 and R3 groups form a quaternary ammonium group which is hydrophilic.
2. A solubilising carbohydrate polymer according to claim 1 wherein the arrangement of the m, n and p units are in a block copolymer form.
3. A solubilising carbohydrate polymer according to claim 2 wherein the block copolymer is mnpmnpmnp.
4. A solubilising carbohydrate polymer according to claim 1, 2 or 3 wherein the carbohydrate polymer is positively charged with a counter ion.
5. A solubilising carbohydrate polymer according to claim 4 wherein the counter ion is ions of any of the following:
chloride, iodide, acetate and glucoronide.
6. A solubilising carbohydrate polymer according to any one of claims 1 to 5 where X is selected from any C1-C30;
C8-C24; or C12-CI8 group which is in linear or branched, substituted or unsubstituted, or cyclo form.
7. A solubilising carbohydrate polymer according to any one of claims 1 to 6 wherein the X group is selected from any of the following: any type of fatty acid derivative of stearic acid, oleic acid, palmitic acid;
N-hydroxysuccinimide activated acyl compounds; and anhydrides.
8. A solubilising carbohydrate polymer according to claim 7 wherein the activated acyl compound is N-hydroxysuccinimide.
9. A solubilising carbohydrate polymer according to any one of claims 1 to 5 wherein X is CH3(CH2)14CONH, or CH3 ( CH2 ) 15NH.
10. A solubilising carbohydrate polymer according to any one of claims 1 to 9 wherein R1, R2 and R3 are independently any C1-C30; C1-C6; or C1 linear or branched, substituted or unsubstituted, or cyclo form of the following groups:
alkyl; alkenyl; alkynyl; aryl; acyl.
11. A solubilising carbohydrate polymer according to any one of claims 1 to 9 wherein R1, R2 and R3 are C1 - C4 linear alkyl groups.
12. A solubilising carbohydrate polymer according to any one of claims 1 to 9 wherein all of R1, R2 and R3 are CH3.
13. A solubilising carbohydrate polymer according to any one of claims 1 to 12 wherein R', R" and R"' are independently any C1-C30; C1-C12; and C1-C6 linear or branched, substituted or unsubstituted, or cyclo form of the following groups: alkyl; alkenyl; alkynyl; aryl; amine;
amide; alcohol; acyl.
14. A solubilising carboyhydrate polymer according to any one of claims 1 to 12 wherein R', R'' and R'll are C1 - C4 linear glycol based groups.
15. A solubilising carbohydrate polymer according to any one of claims 1 to 12 wherein R', R" and R''' are any of the following sugar substituents: glucose, galactose, fructose and muramic acid.
16. A solubilising carbohydrate polymer according to any one of claims 1 to 12 wherein R', R'' and R''' are oligo polyoxa C1 - C3 alkylene units such as ethylene glycol oligomers.
17. A solubilising carbohydrate polymer according to any one of claims 1 to 12 wherein all of R', R" and R''' are CH2OCH2CH2OH or CH2CH2OH.
18. A solubilising carbohydrate polymer according to any one of claims 1 to 17 wherein a carbohydrate polymer starting material to which additional hydrophobic and hydrophilic groups are attached has an average molecular weight of about 2 to 30 kD.
19. A solubilising carbohydrate polymer according to any one of claims 1 to 17 wherein a carbohydrate polymer starting material has a molecular weight of about 5 to 17 kD.
20. A solubilising carbohydrate polymer according to any one of claims 1 to 19 wherein the ratio of m:n:p have the following range: 0.1:1:98.9 to 9:91:0; 1:5:96 to 8:50:42;
or 3:10:87 to 5:19:76.
21. A solubilising carbohydrate polymer according to any one of claims 1 to 20 wherein the total number of monomer units of m+n+p are about 10 to 100.
22. A solubilising carbohydrate polymer according to any one of claims 1 to 21 wherein the total number of monomer units of m+n+p is less than about 200.
23. A solubilising carbohydrate polymer according to any one of claims 1 to 22 wherein the number of x groups does not exceed 10 for every 100 monomer groups in the carbohydrate backbone.
24. A solubilising carbohydrate polymer according to any one of claims 1 to 23 wherein the solubilising carbohydrate polymer also contains additional targetting groups namely peptides, antibodies and other ligands which allow the polymer to target endogenous receptors and thus target its drug payload to such endogenous receptors at the site of pathology.
25. A method of forming a solubilising carbohydrate polymer according to any one of claims 1 to 24 wherein the method comprises;
depolymerising a carbohydrate polymer to form depolymerised carbohydrate;
reacting the depolymerised carbohydrate with a first reactive compound to form hydrophobic side-groups on the carbohydrate backbone and thus form hydrophobically substituted depolymerised carbohydrate; and adding a second reactive compound to the hydrophobically substituted depolymerised carbohydrate to quaternarise an amine group and thereby form the solubilising carbohydrate polymer.
26. A method according to claim 25 wherein the carbohydrate polymer is selected from the following: glycol chitosans, dextrans, alginic acids, starches, dextran, guar gums and all other carbohydrate polymers.
27. A method according to claim 25 or 26 wherein the carbohydrate polymer is depolymerised with any of the following: an acid, a base, or enzyme.
28. A method according to claim 27 wherein the acid used to depolymerise the carbohydrate polymer is selected from any of the following: HCl, H2SO4, HNO3 or HF.
29. A method according to any one of claims 25 to 28 wherein the carbohydrate polymer is depolymerised for a few days, for example, 48 hours, then isolated and subjected to further depolymerisation dependent on the average molecular weight of solubilising carbohydrate polymer required.
30. A method according to any one of claims 25 to 29 wherein the average molecular weight of carbohydrate polymer to be depolymerised is about 3 to 30 kD.
31. A method according to any one of claims 25 to 30 wherein the first reactive compound which forms the hydrophobic side-groups on the depolymerised carbohydrate polymer is selected from any of the following: any type of fatty acid derivative of stearic acid, oleic acid, palmitic acid; organo halides, acyl chlorides, anhydrides, and activated acyl compounds capable of being attacked on the Cl carbon by a compound capable of nucleophilic attack.
32. A method according to claim 31 wherein the activated acyl compound is N-hydroxysuccinimide.
33. A method according to any one of claims 25 to 30 wherein the first reactive compound which forms the hydrophobic side-groups on the depolymerised glycol chitosan is selected from any of the following: hexadecyl bromide, dodecyl bromide, myristic acid N-hydroxysuccinimide.
34. A method according to claim 31 wherein the fatty acid derivative is palmitic acid N-hydroxysuccinimide; palmitic acid benzotriazole carbonate; palmitaldehyde; palmitoyl chloride; or palmitic acid p-nitro phenyl carbonate.
35. A method according to any one of claims 25 to 34 wherein the second reactive compound is an organo halide wherein the organo is selected from any linear or branched, substituted or unsubstituted, or cyclo form of any alkyl, alkenyl, alkynyl, aryl, amine, amide, alcohol or acyl group.
36. A method according to any one of claims 25 to 34 wherein the second reactive compound is any C1-C30; C1-C12;
C1-C6; or C1 linear or branched, substituted or unsubstituted, or cyclo form of the following groups:
alkyl; alkenyl; alkynyl; aryl; amine; amide; alcohol; acyl.
37. A carbohydrate polymer according to any one of claims 1 to 24 and a pharmaceutically acceptable carrier
38. A carbohydrate polymer according to claim 37 wherein the ratio of carbohydrate polymer to pharmaceutical acceptable carrier ranges from 0.05 wt. % to 10 wt. %.
39. A pharmaceutical composition comprising a carbohydrate polymer according to any one of claims 1 to 24 and a drug.
40. A pharmaceutical composition according to claim 39 wherein the drug is selected from any of the following:
prednisolone; cyclosporine; oestradiol, testosterone, drugs with multicyclic ring structures which lack polar groups such as paclitaxel and drugs such as etoposide.
41. A pharmaceutical composition according to claim 39 or 40 wherein the ratio of carbohydrate polymer to the drug is wt. % : 5000 wt. %.
42. A pharmaceutical composition according to claim 39 or 40 wherein the composition includes a pharmaceutically acceptable carrier, and wherein the ratio of carbohydrate polymer to drug to pharmaceutically acceptable carrier is about 1 mg : 1-5 mg : 1 g.
43. A pharmaceutical composition according to any one of claims 39 to 42 wherein the pharmaceutical composition is in the form of any of the following: tablets, suppositories, liquid capsule, powder form, or a form suitable for pulmonary delivery.
44. A method of dissolving poorly soluble drugs in a carbohydrate polymer according to any one of claims 1 to 24 wherein the solubilising carbohydrate polymer has a specifically designed average molecular weight, and specific type and amount of hydrophilic and hydrophobic side-groups substituted on a carbohydrate polymeric backbone whereby on dissolving a poorly soluble drug in the solubilising carbohydrate polymer a substantially clear solution is obtained.
45. A method according to claim 44 wherein the poorly soluble drug is selected from any of the following:
cyclosporin, steroids, oestradiol, testosterone, drugs with multicyclic ring structures which lack polar groups and etoposide.
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