CA2020654A1 - Stabilized fgf composition and production thereof - Google Patents
Stabilized fgf composition and production thereofInfo
- Publication number
- CA2020654A1 CA2020654A1 CA002020654A CA2020654A CA2020654A1 CA 2020654 A1 CA2020654 A1 CA 2020654A1 CA 002020654 A CA002020654 A CA 002020654A CA 2020654 A CA2020654 A CA 2020654A CA 2020654 A1 CA2020654 A1 CA 2020654A1
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- Canada
- Prior art keywords
- composition
- fgf
- accordance
- fgf protein
- hydroxypropyl cellulose
- Prior art date
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Classifications
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
- A61K38/16—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- A61K38/17—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- A61K38/18—Growth factors; Growth regulators
- A61K38/1825—Fibroblast growth factor [FGF]
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K47/00—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
- A61K47/30—Macromolecular organic or inorganic compounds, e.g. inorganic polyphosphates
- A61K47/36—Polysaccharides; Derivatives thereof, e.g. gums, starch, alginate, dextrin, hyaluronic acid, chitosan, inulin, agar or pectin
- A61K47/38—Cellulose; Derivatives thereof
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/48—Preparations in capsules, e.g. of gelatin, of chocolate
- A61K9/50—Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals
- A61K9/5073—Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals having two or more different coatings optionally including drug-containing subcoatings
- A61K9/5078—Microcapsules having a gas, liquid or semi-solid filling; Solid microparticles or pellets surrounded by a distinct coating layer, e.g. coated microspheres, coated drug crystals having two or more different coatings optionally including drug-containing subcoatings with drug-free core
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P43/00—Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P7/00—Drugs for disorders of the blood or the extracellular fluid
- A61P7/02—Antithrombotic agents; Anticoagulants; Platelet aggregation inhibitors
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P9/00—Drugs for disorders of the cardiovascular system
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P9/00—Drugs for disorders of the cardiovascular system
- A61P9/10—Drugs for disorders of the cardiovascular system for treating ischaemic or atherosclerotic diseases, e.g. antianginal drugs, coronary vasodilators, drugs for myocardial infarction, retinopathy, cerebrovascula insufficiency, renal arteriosclerosis
Abstract
TITLE: STABILIZED FGF COMPOSITION AND
PRODUCTION THEREOF
ABSTRACT
Disclosed are (1) a stabilized FGF protein composition which comprises an FGF protein and water-insoluble hydroxypropyl cellulose; (2) a method for preparing a stabilized FGF protein composition, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose; and (3) a method for stabilizing an FGF protein which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose, whereby the stabilized FGF protein can be provided. The composition is obtained in a solid state which has improved stability.
PRODUCTION THEREOF
ABSTRACT
Disclosed are (1) a stabilized FGF protein composition which comprises an FGF protein and water-insoluble hydroxypropyl cellulose; (2) a method for preparing a stabilized FGF protein composition, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose; and (3) a method for stabilizing an FGF protein which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose, whereby the stabilized FGF protein can be provided. The composition is obtained in a solid state which has improved stability.
Description
2~2~
STABILIZED FGF COMPOSITION AND PRODUCTION THEREOF
BACKGROUND OF THE INVENTION
The present invention relates to a stabilized fibroblast growth factor thereinafter briefly referred to as FGF) protein composition, a method for preparing a stabilized FGF protein composition, and a method for stabilizing an FGF protein.
FGF was first isolated as a factor exhibiting strong growth promoting action on fibroblasts such as BAL~/c3T3 cells [D. Gospodarowicz, Nature 249, 123 (1974)3. It is now known that the FGF exhibits growth promoting action on almost all cells derived from mesoblast~ FGF is classified into basic FGF (hereinafter briefly referred to as bFGF) and acidic FGF (hereinafter briefly referred to as aFGF), based on the isoelectric point thereof. bFGF and aFGF both have strong growth promoting action and plasminogen activator inducing action on vascular endothelial cells. Together, these actions suggest a potential for the application thereof as a drug for promoting angiogenesis, as a therapeutic drug for traumas, and as a preventive and therapeutic drug for thrombosis, arteriosclerosis, etc.
Previously, the FGFs were purified to homogeneity from organs derived from animals, such as bovine pituitary.
However, supply o~ these F'GFs was limited, and there was a Eear of antigenicity due to their hetel^ozoic origin.
Recently, there has been developed a method for producing ., ' : ,.
2~2~6~
FGF in large quantities. The method involves using recombinant DNA techniques to express a cloned human FGF
gene in microorganisms or in animal cells. [FEBS Letters 213, 189-194 (1987); Buropean Patent Publication (hereinafter also referred to as EP Publication) No.
237,966)].
In other way, in order to stabilize polypeptide producing factors, an aqueous medical composition characteri~ed by comprising water-soluble polysaccharides in enough amount for stabilizing a growth factor was provided, and it is stated that the composition is effective against declining of activities of mitogen of the polypeptide growing factor and declining of bioactivities [Japanese Unexamined Patent Publication No. 63-152324/1988 corresponding to EP Publication ~o. 267/015].
Since most of the FGF proteins are very unstable, not only they are rapidly inactivated in aqueous solution, but also thier bioactivity easily reduces even by lyophilization. Further, when the FGF proteins are administered for many hours as intravenous drip, a reduction in titer during that time is unavoidable, which causes a major problem.
l`he above-de~cribed aqueous medical composition comprising water-soluble polysaccharides, especially in the ca~e of cellulose derivatives of a degree of ether substitution of at least 0.35 of ether groups per anhydro-glucose unit in the cellulose chain ~ln the case of hydroxy-propyl cellulose, the degree of substitution of hydroxypropoxyl , ~
:
~o~
~ 3 ~ 27580-51 residue is at least 35~)~ it is difficult to form solid medical composition in powder when the base is an FGF protein.
Titer of the composition is lowered during mixing and drying process.
SUMMARY OF THE INVENTION
The present inventors have discovered that the stability of FGF pro~eins is surprisingly increased by admixing an FGF protein with a water-insoluble hydroxypropyl cellulose.
In particlular, the present inventors have succeeded in obtaining a solid composition having an improved stability of FGF protein as compared with that of the above-described aqueous medical composition comprising FGF protein and water-soluble polysaccharides.
In accordance with the present inven~ion, there is provided (1) a stabilized FGF protein composition which comprises an F~F protein and water-insoluble hydroxypropyl cellulose; ~2) a method for preparing a stabilized FGF
protein composition, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose; and (3) a method for stabilizing an FGF protein, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose.
DESCRIPTIO`N OF THE PREF~RRED EMBODIMENTS
The FGF proteins used in the present invention may include basie FGF ~hereina~ter also referred to as bFGF) and acidic FGF ~hereina~ter also referred to as aFGF). The FGF
.
. .
~, - . .- , 2 fJ~
protein used in the present invention include those derived from mammals. The mammals include human, monkey, pig, bovine, sheep and horse.
The FGF proteins include those extracted from various organs in which the presence of FGFs is already known, such as brain and pituitary.
Further, the FGF proteins include tho6e obtained by the recombinant DNA technique ~FEBS Letters 213, 189-194 ~1987~;
EP Publication No. 237,966~.
Hereinafter, the recombinant human basic FGF may be referred to as rhbFGF.
The FG~ proteins used in the present invention include a FGF mutein.
Examples of the muteins of the FGFs used in the present invention include the muteins disclosed in Biochemical_and Bivphysical Research Communications 151, 701-708 (1988), EP
No. 281,822 A2, EP Publication No. 326,907 Al; and there may be included the muteins introduced by at least one glycosylation site diclosed in Japanese Patent Application No. 109014/1990 ~filed on April 25, l990j which corresponds to European Pa~ent Application No. 90107737.0 and U.S. Patent Application Ser. No. 511,469.
For example, the FGF muteins used in the present invention are obtained essentially by variations o~ the amino acid se~uences oE the original peptides or proteins.
Such variations include addition o~ amino acid~s), deletion : -.
~`
~ ": ' '' of constituent amino acid(s) and substitution of constituent amino acid(s) by different amino acid(s). Further, FGF
muteins introduced by glycosylation site are included in such variations.
Such addition of amino acid(s) includes addition of at least one amino acid.
Such deletion of constituent amino acid(s) includes deletion of at least one FGF-constituent amino acid.
Such substitution of constituent amino acid(s) by different amino acid~s) includes substitution of at least one FGF-constituent amino acid by at least one different amino acid.
At least one amino acid in the mutein which has at least one amino acid added to the FGF excludes methionine lS derived from the initiation codon used for peptide expression and a signal peptide.
The number of the added amino acid(s) is at least one.
However, it may be any number as long as FGF characteristics are not lost. More preferable amino acids include some or all of the amino acid sequences of proteins which have homology with the FGFs and which exhibit activities similar to those of the FGFs.
As for the number of the deleted FGF-constituent amino acid(s) in the mutein which lacks at least one FGF-con~tituent amino acid, it may be any number as long as FGFcharacteristics are not lost.
Example~ oE the deleted constituent amino acid include ~ . - : : ,:: :, :,.-,. . :
- , . ~. . . , ;; , : .:.: . , , , . :........... ::: : :.. ., - - .: . . .................. . . .
.
~20~
the 10 residues on the amino termial side of the human bFGF:
Met-Pro-Ala-Leu-Pro-Glu-~sp Gly-Gly-Ser, the 14 residues on the amino terminal side of the human bFGF:
Met-Pro-Ala-Leu-Pro-Glu-Asp-Gly-Gly-Ser-Gly-Ala-Phe-Pro, -the 41 residues on the amino terminal side of the human bFGF:
Met-Pro-Ala-Leu~ .. -Val, the 61 residues on the carboxyl terminal side of the human bFGF:
Lys-Cys- -Val-Ser.
The muteins further include muteins lacking the 7 to 46 amino acid residues on the carboxyl side of the original peptide or protein of the bFGF.
Preferred examples of such deletion include deletion of the following amino acid sequences of the rhbFGF:
~nino acid sequence from amino acid No. 102 on Amino acid sequence from amino acid No. 105 on Amino acid sequence from amino acid ~o. 115 on Amino acid sequence from amino acid No. 119 on Amino acid sequence from amino acid No. 124 on Amino acid sequence from amino acid No. 130 on ~nino acid sequence from arnino acid No. 138 on As for the number of FGF-constituent amino acids prior , ~ . . . :. .; ~. , : .. : . -2~20~
to substitution in the mutein, which has at least one FGF-constituent amino acid substituted by at least one different amino acid, it may be any number as long as FGF
characteristics are not lost.
Examples of the constituent amino acids prior to substitution include cysteine and cystine, but c~steine is preferable~ The constituent amino acids other than cysteine prior to substitution include aspartic acid, arginine, gl~cine and valine.
When the constituent amino acid prior to substitution is cysteine, neutral amino acids are preferable as the substituted amino acids. The neutral amino acids include glycine, valine, alanine/ leucine, isoleucine, tyrosine, phenylalanine, histidine, tryptophan, serine, threonine and methionine. Serine and threonine are particularly preferred.
When the constituent amino acid prior to substitution is any one other t'nan cysteine, amino acids which are different, for example, in hydrophilicity, hydrophobicity or electric charge from the amino acid prior to substitution are selected as the substituting different amino acids.
Speciically, when the amino acid prior to substitution is aspartic acid, the substituting amino acids include asparagine, threonine, valine, phenylalanine and arginine.
~n particular, asparagine and arginine are preEerable.
When the amino acid prior to substitution is arginine, the substituting amino acids includes glutamine, threonine, . - . . . :: -:
.. .. . ....
, . :- :
2`i~2 ~
leucine~ phenylalanine and aspartic acid. Glutamine is especially preferableO
When the amino acid prior to substitution is glycine, the substituting amino acids include threonine, leucine, phenylalanine, serine, glutamic acid and arginine.
Threonine i5 particularly preferred.
When the amino ~cid prior to substitution is serine, the substituting amino acids include methionine, alanine, leucine, cysteine, glutamine, arginine and aspartic acid.
In particular, methionine is preferable.
When the amino acid prior to substitution is valine, the substituting amino acids include serine, leuciner proline, glycine, lysine and aspartic acid. Serine is especially preferred.
As the original constituent amino acids prior to substitution, aspartic acid, arginine, glycine, serine and valine are preferably selected.
As the substituting amino acids, asparagine, glutamine, arginine~ threonine, methionine, serine and leucine are preferably selected.
The most preferred substituted muteins include a mutein in which cysteine, the constituent amino acid, is substituted by serine.
In the above substitution, the substitution of at least ~5 two constituent amlno acids may be simultaneously carried out. In particular, it is pr~ferable to substitute two or three constituent amino acids.
.. , . . . . ~, . .
.~ . ~ , . . ~. , , . - : . - - ... .
Q6~
g The muteins may be obtained by a combination of two or three of the above-mentioned addition, deletion and substitution.
A mutein is preferable in which at least one human bFGF-constituent amino acid is substituted by at least one different amino acid. In particular, rhbFGF mutein CS23 is preferable in which cysteine residues at the 70- and 88-positions of human bFGF are substituted by serine residues, respectively.
The EGF mutein has had introduced at least one glycosylation site. And the mutein may further have sugar chain(s).
The glycosylation sites include a site in which an amino acid sequence constituting the glycosylation site is represented by the following the formula:
Asn-X~Y
(wherein X may be any amino acid residue, and Y is Thr, Ser or Cys).
X is preferably an amino acid other than Pro, and more preferably Gly, Tyr, Arg, Ser, Iys, Val or Ala and more preferably Gly, Lys, Val or Ala. Y is preferably Thr or Ser.
The sugar which is added to a FGF mutein may be any one ~ound in known glycosylated proteins. Examples of such sugars include N-acetyl glycosamine, N-acetyl galactosarnine, mannose, galactose, ~ucose and cyalic acid.
The number of sugars in a glycosyl chain is preferably ., .. . : ..
'. ~
.:
:~: . . ~ . :
~ ~2.~
at least one, and more preferably 10 to 20~
In order to produce the muteins, site-directed mutagenesis is employed. This technique is ~ell-known and described in R. F. Lather and J. P. Lecoq, Genetic Enqineerinq, pp. 31-50, Academic Press (1983). Mutagenesis directed to oligonucleotide is described in M. Smith and S.
Gillam, Genetic ~nqi~eerinq: Principles and Methods, Vol. 3, pp. 1-32, Plenum Press (1981).
The production of a structural gene which encodes the mutein is carried out, for example, by the steps o~:
(a) hybridizing a single-stranded DNA comprising a single strand of the structural gene of FGF with a mutagenic oligonucleotide pximer(the above-mentioned primer is complementary to a region, including a codon for cysteine, to be replaced by this single strand, or including an anti-sense triplet which forms a pair with this codon in some cases, provided this does not apply to disparity with other codon ~or the amino acid than the above codon, or with the anti-sense triplet in some cases.), (b) elongating the primer using DNA polymerase to Eorm a mutational heteroduplex, and (c) replicating this mutational heteroduplex.
q`hent phage DN~ for transferring the mutagenized gene is isolated and introduced into a plasmid.
~ suitable host is transEormed with the plasmid thus obtained, and the obtained transformant is cultivated in a medium, thereby beinq capable o~ producing the mutein.
. .
- . : : - ; . ..
~ 75~0-51 Examples of the water-insoluble hydroxypropyl cellulose include a low-substituted hydroxypropyl ether of celluloseO
The low-substituted hydroxypropyl cellulose contains not less than 5.0~ and not more than 16.0% by weight hydroxypro-poxyl group on a dry basis (i.e. when dried at 105C for 1 hour).
(Refer to the Japanese Pharmacopeia, the 11th revision D-733 to D-780; and The U.S. Pharmacopeia, the 21st revision, Supplement, pages 5180 to 5181).
Examples of low-substituted hydroxypropyl cellulose used in the present invention include low-substituted hydroxy-propyl cellulose ~LH-ll, LH-20, LH 21, LH-22 and L~I-31, Shin-Etsu Chemical, Japan).
In the present invention, the weight ratio of the FGF
protein to water-insoluble hydroxypropyl cellulose is preferably about 1 : 0.01 to 1,000,000, more preferably about 1 : 1 to 100l000, still more preferably about 1 : 500 to 20,000, and especially preferably about 1 : 500 to 10,000.
Further, the composition of the present invention may further contain one or more members selected from sugars, proteins, amino acids, sodium chloride and gum arabic.
The sugars include, for example~ sucrose, trehalose, maltose, fructose, inositole and amylose. The proteins include, for example, casein, albumine, gelatin and egg white. The amino acids include, Eor example, cysteine, phenylalanine, leucine and glycine.
In the present invention~ the weight ratio oE FGF
protein to sugars, proteins, aminc~ acids, sodium chloride 2 ~ 5 ~
- 12 - 2758o-5l and/or gum arabic is preferably about 1:0.01 to 1,000,000, more preferably about 1:1 to 100,000, still more preferably about 1:500 to 20,000, and especially preferably about 1:500 to 10,000.
The compositions of the present invention are obtained by admixing the FGF protein with the water-insoloble hydroxypropyl cellulose, for example, by adding an aqueous solution of the FGF protein to water-insoluble hydroxypropyl cellulose in powder, followed by mixing. The pH of the aqueous solution of the FGF protein is preferably adjusted to about 3 to 10, more preferably to about 5 to 9.
The addition and th~ mixing are carried out, for example, at about 10 to 30C, preferably at about 10 to 20C.
The mixing is sufficiently performed by devices generally used for stirring and granulation [such as a mortar, a Pony*mixer (Hosokawa Tekkosho, Japan), a Vertical*
granulator (Fuji Sangyo) and a Super*mixer (Hosokawa Tekkosho)], by devices used for fluidized granulation [such as Glad*(Okawara Seisakusho)] and by devices used for rolling granulation [such as CF (Freund)].
The compositions thus mixed are, for example, driecl or lyophilized at room temperature (about 10 to 30C) under : reduced pressure (about 10 mmHg or less), whereby the solid compositions stabilized in bioac~ivity can be obtained.
Sugars, proteins, amino acids, sodium chloride and/or gum arabic may be simultaneously added when water-insoluble *Trade-mark .
.. . .
' . ` . "'`' ' ' . ' ' .' : ` .
.` ` ` ' ~ ""` ~` :' 2 ~
hydroxypropyl cellulose and FGF protein are mixed, or they may be mixed with water-insoluble hydroxypropyl cellulose, followed by adding FGF protein. The production method of the composition is carried out by similar method with that of the composition comprising water-insoluble hydroxypropyl cellulose and FGF protein.
In the above mixing, the aqueous solution of the FGF
proteln stabilized with glucan sulfate may be used.
Examples of the glucan sulfate include dextran sulfates, cyclodextrin sulfates and ~-1,3 glucan sulfates.
All of these are sulfuric ester derivative of polymer of D-glucose. The sulfur content in the glucan sulfate is preferably not less than about 3% by weight, more preferably about 12 to 20~ by weight, most preferably about 16 to 20%
by weight. In particular, dextran sulfate is preferable.
The dextran sulfates include a sulfate of dextran produced from sucrose by the action of a microorganism such as Leuconostoc mesenteroi es. The dextran sulfate is a partial sulfates of dextran mainly containing ~(lt6) linkage, and the sulfur content therein is usually at least about 12% by weight, preferably about 16 to 20% by weight.
The average molecular weight thereof is in the range of about 1,000 to 40,000,000, preferably in the range of 3,000 to S00,000. The dextran sulfate is very easily soluble in water, and is a compound already known in the art, which is manufactured by known methods ~er se.
Cyclodextrin in the cyclodextrin sulfate includes t`
~o~
cyclodextrin produced from starch by the action of a microorganism such as Bacillus macerans. The cyclodextrin has ring structure of D-glucose molecules linked by ~ 4) linkage, and includes an ~-type (6 molecules) r a ~-type (7 molecules) and a y-type (8 molecules). In this invention, any of these forms may be used.
The cyclodextrin sulfate is obtained by sulfation of the cyclodextrin, and the sulfation is conducted according to methods already known in the art. The methods for sulfation include the methods described in U.S. Patent No.
2,923,704 and Japanese Patent Unexamined Publication No.
50-36422/lg75, The sulfur content in the cyclodextrin sulfate is usually at least about 3% by weight, preferably about 12 to 24% by weight. The cyclodextrin sulfate has the property of being very soluble in water.
The degree of sulfation of the cyclodextrin sulfate may be any degree as long as the sulfur content is at least about 12~ by weight. In particular, the cyclodextrin sulfate whose sulfur content is about 16 to 21% by weight are advantageously used. Mixtures of the sulfates different from one another in degree of sulfation may be used as such, or the purified sulfates having the single degree of sulfation may be used. The puriEication can be conducted, ~5 for example, by concentrating a reaction solution containing an alkali metal salt of ~-cyclodextrin sulfate, evaporating it to dryness, dissolving the condensate in water, and :. . :
-` 2~Q~
mixing the resulting aqueous solution with a hydrophilic solvent to separate a desired product.
~ -1,3-glucan in the ~-1,3-glucan sulfate includes straight-chain ~-1,3-glucans, which are produced by microorganisms belonging to Alcaliqenes or Agrobacterium.
There may be in the form of a low molecular weight polymer obtained by hydrolysis of the straight-chain ~ 1,3-glucans and similarly having a straight-chain ~-1J3-glucan structure.
Curdlan (also known as a thermogelable polysaccharide PS and available from Wako Pure Chemical Industries Ltd.
Japan) is known as a water-insoluble, thermogelable~
unbranched glucan, and has straight-chain ~-1, 3-glucan linkage alone which is produced from a microbial strain belonging to Alcaligenes or Aqrobacterium [Japanese Patent Publication Nos. 43- 7000/1968, 48-32673/1973 and 48-32674/1976].
The Alcaligenes faecalis var. Myxo~enes NTK-u strain, the Aqrobacterium radiobacter strain and the Agrobacterium ._ radiobacter U-l9 strain, which produce Curdlan, are cited in ~merican Type Culture Collection Cataloque of Strains, the 15th edition (1982), as ATCC- 21680, ATCC-6466 and ATCC-21679, respectively.
The properties o~ partially hydrolyzate oE Curdlan and the method for preparation thereof have already been described in detail in Japanese Patent Unexamined Publication No. 55- 83798/1980.
: :
.,, Thus, the straight-chain ~-1,3-glucan is a compound represented by the following formula:
~ ~ j H~\ I ON
wherein n is an integer of 4 to about 1,000.
Any of the ~-1,3-glucans described above may be used as -long as the average degree of polymerization (DP) thereof is not more than 1,000. In particular, there are advantageously used the partically hydrolyzed products thereof having an average degree of polymerization tDP) of 6 I5 to about 300, more preferably 15 to about 200.
n in the formula (I) has a relation to DP represented by the following equation:
DP - 2 = n.
The sul~ate of the straight-chain ~-1,3-glucan is produced by sulfonation of the three hydroxyl groups of the intermediate monosaccharide unit of the ~-1,3-glucan or its lower polymers and the hydroxyl groups of the monosaccharide units at both ends thereof. The sulfates having an average degree of substitution ~DS) of 0~5 to 3 per monosaccharide unit are usually usedr and preferably ones having an average degree oE substitution (DS) of 1 to 2 are advantageously used.
, .
", . ~ ' ,' -Sulfation of straight-chain ~-1,3-glucans or its low molecular weight polymer can be achieved by allowing a sulfating agent such as chlorosulfonic acid or sulfuric anhydride to act thereon, or by reacting a complex of sulfuric anhydride and an organic base such as pyridine, dimethylformamide, trimethylamine or dimethylaniline therewith [J. Biol. Chem. ~39, 2986 (1964)].
The ~-1,3-glucan sulEate is very soluble in water and low in toxicity. The sulfur content in ~-1,3-glucan sulfates is usually at least about 5% by weight, preferably about 10 to 24% by weight.
The glucan sulfate is very low in toxicity to warm-blooded animals. This is therefore advantageous for ;
parenteral or oral administration of the stabili~ed compositions comprising the FGF protein and the glucan sulfate to the warm-blooded animals.
The glucan sulfate may be used in the state of free or salt. Examples of such salts include sodium salts, potassium salts, ammonium salts and trimethylammonium salts.
When the glucan sulfate is brought into contact with the FGF protein in aqueous media, the free glucan sulfate may be added thereto, followed by addition of proper amount of an alkali or acid to give the desired pH. By the addition of alkali, the glucan su].fate may be exist in the 2~ aqueous media in khe ~orm o~ either its salt or a mixture of the free dextran sulfate and its salt.
If the FGF protein is brought into con-tact with glucan .,~ ......... .
.
:. . -, ~: :
:~ . . :~: . -- 18 - ~
sulfate in aqueous media in the presence of an additional dlbasic or tribasic carboxylic acid, the FGF protein is advantageously more stabilized.
Examples of the dibasic carboxylic acids include tartaric acid, maleic acid, malic acid and fumaric acid~
The tribasic carboxylic acids include, for example, citric acid and isocitric acid.
The above carboxylic acids may be used in the form of either free compounds or their salts. E~amples of such salts include sodium salts, potassium salts and ammonium salts~
Further, the free carboxylic acid may be added thereto, followed by addition of proper amounts of an alkali or acid to give the desired pH. By the addition of the alkali, the carboxylic acid may be exist in the aqueous media in the form of either its salt or a mixture of the free acid and its salt.
When the FGF protein is brought into contact with the glucan sulfate in aqueous media, it is preferred that the glucan sulfate is a~ded in an amount of about 0.1 to 100 mol/mol, more preferably about 0.5 to ~ mol relative to 1 mol of FGF protein.
The concentration of the glucan su~fate in the aqueous media is preferably about 0.0005 to 5% by w/v, more pre~erably about 0.01 to ]% by w/v.
The concentration o~ the FGF protein in the aqueous media i9 preferably about 0.0005 to 5~ by w/v, more ;:
, ' ' ' ' . ' ~
- 2~2~
preferably about 0.01 to 1% by w/v.
The concentration of the carboxylic acid in the aqueous media is preferably about 1 mM to lM, more preferably about 10 mM to 500 mM.
For their contact in the aqueous medium, the object can be attained only by mixing the FGF protein, the glucan sulfate and the carboxylic acid as required with one another in the aqueous medium.
The aqueous media may be any media such as distilled water, physiological saline solution and glucose solution are preferably used. As the aqueous media, there can also be used buffers such as phosphate buffer and tris~hydroxymethyl)aminomethane-HCl buffer.
When the FSF protein, the glucan sulfate and the carboxylic acid as required are mixed with one anotherl they may be mixed as aqueous solutions, respectively, or may be mixed as solids, respectively, followed by dissolution in the aqueous medium. In mixing, the temperature is preferably about 0 to 40C, and the pH is preferably in the range of about 3 to 10, more preferably in the range of about 5 to 9. The time taken to mix is usually about 1 to 30 minutes.
Thus, the aqueous solution of the FGF protein stabilized with glucan sulfate is obtained.
In the present invention, the above-described composition comprising FGF protein and water-in~oluble hydroxypropyl cellulose may be further coated by an enteric polymer.
.... ,., ~ : :: :... . ;, .
21~1D6~
Examples of the enteric polymers used in the present invention include hydroxypropyl methyl cellulose phthalate, carboxymethyl ethyl cellulose, cellulose acetate phthalate, hydroxymethyl cellulose acetate succinate and acrylic polymers [such as methacrylic acid-ethyl acrylate copolymers (Eudragit*L30D-55 and Eudragit*L100-55~, methacrylic acid-methyl acrylate copolymers (Eudragit L-100) and methacrylic acid-met-hyl methacrylate copolymers (Eudragit S100~, Rohm, West Germany].
The coating is conducted by known methods per se.
Namely, dispersions or solutions obtained by dispersing or dissolving the coating bases in water or organic solvents are sprayed on the tablets, the granules or the fine grains by pan coating methods, fluidized coating methods, the rolling coating methods or the like. When the compositions are coated with the coating agents, it is desirable that the temperature of the composition to be coated is about 25 to 70C, preferably about 25 to 50C. The coating amounts are about ~0 to 300%, preferably 50 to 100~ as the intestinally soluble polymers based on the compositions.
Further, the solid composition ~powder) vf the present invention and fatty acid ester of polyglycerol granules can also be heated and fluidized to obtain granules. According to the granules, the eE~ective 1ngredient tE'G~ protein) of the solid composition o~ the present invention is stably eluted and released, and stabilized for a long time.
When the fatty acid ester oE polyglycerol is a mi~ture, *Trade-mark , it does not show a clear melting point and is softened at a specific temperature in some cases. In this specification, the "melting point" includes a softening point which such a mixture shows.
The fatty acid ester of polyglycerol used above may be any of a monoester, a diester and a polyester as long as it is an ester formed by the combination of a polyglycerol with a fatty acid. The fatty acid ester of polyglycerol , unlike hardened oil and so on, has the characteristics of showing no crystal polymorphism and having little interaction with effective ingredients such as drugs.
The polyglycerin is "a polyhydric alcohol having n (in a cyclic polyglycerin) to n + 2 (in a straight or branched polyglycerin) hydroxyl groups and n - 1 (in a straight or branched polyglycerin) to n (in a cyclic polyglycerin) ether combinations in one molecule" [Polyqlycerin Ester, p. 12, edited and published by Sa~amoto Yakuhin Kogyo Co. Ltd., Japan ~May 2, 1986)]. For example, compounds represented by the following formula can be used.
20 HO(cH2_1cH_cH2_O)nH
OH
wherein n indicates a degree of polymerization and is an integer of 2 or more. n is normally 2 to 50l preferably 2 to 20, more preferably 2 to 10. The polyglycerol is straight or branched.
Specific examples oE such polyglycerols include diglycerol, triglycerol, tetraglycerol, pentaglycerol, ,: ... . ..
, . . .
.. - .... ..
hexaglycerol, heptaglycerol, octaglycerol, nonaglycerol, decaglycerol, pentadecaglycerol, eicosaglycerol and triacontaglycerol. Of these polyglycerols, for example, tetraglycerol, hexaglycerol and decaglycerol are frequently used.
The fatty acids include, for example, saturated or unsaturated higher fatty acids having 8 to 40 carbon atoms, preferably 12 to 22 carbon atoms. Examples of such fatty acids include palmitic acid, stearic acid, oleic acid, l~ linolic acid, linolenic acid, myristic acid, lauric acid, ricinolic acid, caprylic acid, capric acid and behenic acid.
of these fatty acids, for example, stearic acid, oleic acid, lauric acid and ricinolic acid are preferable.
Specific examples of the fatty acid ester of polyglycerol include caprylyl mono(deca)glyceride, caprylyl di(tri)glyceride, lauryl mono(tetra)glyceride, lauryl mono(hexa)glyceride, lauryl mono(deca)glyceride, oleyl mono(tetra)glyceride, oleyl mono(hexa)-glyceride, oleyl mono(deca)glyceride, oleyl di(tri)glyceride, oleyl di(tetra)glyceride, oleyl sesqui(deca)glyceride, oleyl penta(tetra)glyceride, oleyl penta(hexa)glyceride, oleyl deca(deca)glyceride, linolyl mono(hepta)glyceride, linolyl di~tri)glyceride, linolyl di(tetra)glyceride, linolyl di~hexa)glyceride, stearyl mono~tetra)g].yceride, stearyl rnono~hexa)glyceride, stearyl mono~deca)glyceride, stearyl tri(tetra)glyceride, stearyl tri(hexa)glyceride, stearyl sesqui(hexa)glyceride, stearyl penta(tetra)glyceride, ,~,: . :
: . , . : . :
~i~ 2 ~
stearyl penta(hexa~glycedride, stearyl deca(deca)glyceride/
palmityl mono(tetra)glyceride, palmityl mono(hexa)glyceride, palmityl mono(deca)glyceride, palmityl tri(tetra)glyceride, palmityl tri(hexa)glyceride, palmityl sesqui~hexa)glycoride, palmityl penta(tetra)glyccride, palmityl penta(hexa)-glyceride and palmityl deca(deca)glyceride. Examples of the preferred fatty acid ester of polyglycerol include stearyl penta(tetra)glyceride (for example, PS-310, Sakamoto Yakuhin Co., Japan), stearyl mono(tetra)glyceride (for example, MS-310, Sakamoto ~akuhin Co.), stearyl penta(hexa)~
glyceride (for example, PS-500, Sakamoto Yakuhin Co.), stearyl acid sesqui(hexa)glyceride (for example, SS-500, Sakamoto Yakuhin Co.) and stearyl mono(deca)glyceride~
These fatty acid ester of polyglycerol are used alone or as mixtures of two or more kinds.
The melting point of the fatty acid ester of polyglycerol is about 40 to 80C, preferably about 40 to 60C.
The molecular weight of the fatty acid ester of polyglycerol is usually 200 to 5,000, preferably 300 to 2,000. The hydrophile-lypophile balance (~LB) thereof is l to 22, preferably l to 15, and the elution rate of the effective ingredient of the powder can be controlled by adjusting the HLB. The H~B can also be ad~usted by mixing two or rnore kinds o~ atty acid ester of polyglycerol.
The fatty acid ester of polyglycerol can also be used together with lipids. ~s the lipids are used water-.. . , ~. ................................ .
: ' . ' . ~ :' . , ~2~
insoluble materials permissible depending on the purpose of preparations and the like. The preferred softening point or melting point of the lipids is about 40 to 120C, particularly about 40 to 90C.
Specific examples of the lipids include the hardened products of fats and oils such as castor oil, cotton seed oil, soybean oil, rapeseed oil and beef tallow; waxes such as beeswax, carnauba wax, spermaceti, lecitin, paraffin and microcrystalline wax; fat~y acids such as ~tearic acid and palmitic acid, or fatty acid salts such as sodium sa].ts and potassium salts of fatty acids; fatty alcohols such as stearyl alcohol and cetyl alcohol; and glycerides. Of these lipids, there are preferable, for example, hardened cotton seed oil, hardened castor oil, hardened soybean oil, carnauba wax, microcrystalline wax, stearic acid and stearyl alcohol.
The ratio of the lipid to the fatty acid ester of polyglycerol is usually 100 parts by weight or less of lipid per 100 parts by weight of fatty acid ester oE polyglycerol, and can be suitably selected within the above range.
In the preparation of the granulated compositions, spherical fatty acid ester of polyglycerol granules are preferably used to adhere the powders (the solid compositions o.E the present invention) in large amounts to the fatty ac.id ester of polyglycerol or to allow the esters to contain the powders in large amounts, and to obtain the granulated compositions corresponding to the shape and the , : . , . : , ~ .
. .
- - 2~2~
size of the fatty acid ester of polyglycerol granules. When the spherical fatty acid ester of polyglycerol granules are used, large amounts of powders (the solid compositions of the present invention), for example, the powder constituting about 80% by weight of the whole granulated composition, can be incorporated therein. Moreover, the spherical granulated compositions relatively smooth in surface and narrow in size distribution can be obtained. In some cases, the powder can be incorporated therein so as to constitute more than ~0~ by weight, for example, about 85% by weight, of the whole granulated composition.
The spherical fatty acid ester of polyglycerol granules can be obtained, for example, by spray cooling, preferably spray chilling. The spray chilling can be carried out by rotating a disk such as an aluminum disk having a smooth sur~ace and dripping the molten fatty acid ester of polyglycerol thereon. The rotary disk is not particularly limited in size, but is about 5 to lO0 cm, preferably about lO to 20 cm in di.ameter. The rotational speed of the rotary ~ disk and the dripping rate of the molten fatty acid ester of polyglycerol can be dekermined depending on the desired size and the like of the granules. The rotational number of the rotary dis]c is usually abouk lO to 6,000 rpm, preferably 900 to 6,000 rpm, more preferably 1,000 to 3,000 rpm. The molten fatty acid ester of po:LygLycerol can be dripped at a constant rate, for example, of about 2 to 200 g/min, preferably about 5 to lO0 g/min.
~;
.,: ; , :, , .:, - i ; ~ , -. , :
~, ,, ; ~ -: :, : :
; ~ ' ' ! , The size of the fatty acid ester of polyglycerol granules can be selected according to the desired size of the granulated composition and is not particularly limited, but is usually about 10 to 150 meshes, preferably about 25 to 100 meshes.
The solid compositions (powders) of the present invention can be used together with powdery diluents.
Examples of such diluents include excipients such as lactose, cornstarch, Avicel*(microcrystalline cellulose:
Asahi Chemical Industry, Japan), powder sugar and magnesium stearate; binders such as starch, gelatin, gum arabic powder, methyl cellulose, carboxymethyl cellulose sodium, hydroxypropyl methyl cellulose and polyvinyl pyrrolidon;
disintegrators such as carboxymethyl cellulose calcium and low substituted-hydroxypropyl cellulose; coloring agents;
flavoring agents; absorbents; preservatives; wetting agents antistatic agents; and d.isintegration delaying agents.
rrhe ratio of the powder (the solid cornposition of the present invention) to the above fatty acid ester of polyglycerol can be established depending on the desired size of the granulated composition, the content of the drug active ingredient and the like, but is usually 10 to 1,000 parts by weight, preferably 50 to 500 parts by weight of the powder per 100 parts by weight o the fatty acid ester of polyglycerol.
The granulation by heating and fluidizing can be conducted according to conventional 1uidized-bed *rrrade-mark ~ : .
. . ~. .
granulating methods. The heating temperature in the granulating methods is near the melting point of the above ~atty acid ester oE polyglycerol ester, preferably within the range from the melting point of the fatty acid ester of polyglycerol to the temperature 5C lower than the melting point. If the heating temperature is too high, the fatty acid ester of polygly-cerol granules tend to coalesce by fusion to form a granulated composition wide in size distribution. On the other hand, if the heating temperature is too low, it is difficult to granulate the powder (the solid composition of the present invention) with the fatty acid ester of polyglycerol granules.
The granulation can be performed by floating the fatty acid ester of polyglycerol granules and the powder (the solid composition o~ the present invention) to form a fluidized bed, and by heating and fluidizing them at a required temperature. It can be confirmed by the presence or absence of the powder particles whether or not the granulation is completed.
The granulated compositions thus obtained are usually ine-grained or granular.
When the granulated composition is observed under a microscope, it usually has a shape corresponding to the shape oE the ~atty acid ester oE polyglycerol granule, and ~5 1t seems that the powder (solid composition of the present invention) is at least partially embedded in the fatty acid ester of polyglycerol granulel pre~erably involved therein ; to coaleace.
' ` ~ , '`' ' ' , ,' ' .
, . ,' ~ ': ' ~", . ' . ` ' ' ' ' ' ` ' '~
,~ :
:' :
2 ~
The compositions of the present invention thus obtained are solid.
The compositions of the present invention include pharmaceutical compositions containin~ the above solid compositions (Eor example, ointments and suppositories)~
Namely, in the case of the ointments, the solid compositions of the present invent-ion are dispersed in bases for the ointments. In the case of the suppositoriesr the solid compositions of the present invention are dispersed in bases for the suppositorie5.
As the present FGF composition is stabilized, it can be advantageously used as a medicine.
The stabilized FGF protein compositions of the present invention can be safely administered parenterally or orally to warm-blooded animals (such as human, mouse, rat, hamster, rabbit, dog and cat) as such or with pharmacologically permissible additives (such as carriers, excipients and diluents), as pharmaceutical compositions tsuch as tablets, capsules, granules, fine grains, powders, ointments and suppositories)-Such preparations can be formulated into the formssuitable for oral administration such as tablets, capsules, powders, granules and fine grains in accordance with known methods per se, In these cases, as additives are used 23 excipients (such as lactose, cornstarch, light silica and ~ine crystalline cellulose), binders (such as alpha starch, methyl cellulose, carboxymethyl cellulose, hydroxypropyl ~ , ' P2~
cellulose, hydroxypropyl methyl celulose and polyvinyl pyrrolidone), disintegrators (such as carboxymethyl cellulose calcium, starch and low-substituted hydroxypropyl cellulose), surface active agents [such as Tween*80 (~ao Atlas, Japan), Pluronic*F68 (Asahi Denka Kogyo, Japan) and polyoxyethylene-polyoxypropylene copolymer], antioxidants (such as L-cysteine, sodium sulfite and sodium ascorbate) and lubricants (such as magnesium stearate and talc).
As to the tablets, the granules and the fine grains, coating may be carried out in accordance with known methods per se for the purpose of masking tastes or giving intragastric solubility, intestinal solubility or increasing :~
sustained release. As the coating agents are used, for example, hydroxypropyl methyl cellulose, ethyl cellulose, hydroxymethyl cellulose, hydroxypropyl cellulose, polyoxyethylene glycol, Tween 80, Pluronic*F68, castor oil, cellulose acetate phthalate, hydroxypropyl methyl cellulose phthalate, hydroxypropyl methyl cellulose acetate succinate, acrylic polymers (~udragitkL100-SS and L-100, Rohm, West Germany), carboxymethyl ethyl cellulose, polyvinyl acetal diethylamino acetate, waxes and pigments such as talc, titanium oxide and iron oxide red. These coating agents may be applied in one or more layers, alone or in combination of two or more agents.
The coat.ing is conducted by known method9 per se~
Namely, d.ispersions or so].utions obtained by dispersing or dis~olving the coating bases in water or organic solvents *Trade-mark , .,, ~ ' ` i , : , ,...................... .
` ~ ID 2 f~
are sprayed on the tablets, the granules or the fine grains by pan coating methods, fluidized coating methods or rolling coating methods. The tablets, the granules and the fine grains are preferably coated at about 25 to 70C, more preferably at about 25 to 50C.
Further, ointments and suppositories can be prepared according to known methods per se using the following additives.
Examples of the additives used when the ointments are prepared include vaseline, beweswax, paraffin, liquid paraffin, cholesterol, stearyl alcohol, lanolin, cetyl alcohol and polyethylene glycol.
Examples of the additives used when the suppositories are prepared include cacao butter, hydrogenated vegetable oils, monoglycerides, triglycerides, glycerogelatin and polyethylene glycol.
The FGF protein compositions of the present invention have growth promoting action on ibroblasts, high stability and low toxicity. Therefore, the FGF protein compositions can be used as therapeutic promoting drugs for burns, traumas, postoperative tissues and the like, or therapeutic drugs for thrombosis, arteriosclerosis and the like by arterializing action~ Also, they can be used as reagents ~or promotin~ cell cultivation.
When the FGF protein compositions of the present invention are used as the above-mentioned drugs, they are administered, for example, to the above-mentioned .
::
^ 2021D6~
warm-blooded animals in an approprlate amount ranging from about 1 ng/kg to 100 ~g/kg daily as the FGF protein, taking into account the route of administration, symptoms, etc.
Recombinant human bFGF mutein CS23 (hereinafter also referred to as rhbFGF mutein CS23) used in Examples hereinafter described is prepared by the method described in Biochemical and Biophysical Research Communications 151 r 701-708 (1988) or the method described in European Patent Publication No~ 281,822 A2. The rhbFGF mutein CS23 used in Examples hereinafter described was prepared and purified by the methods described in European Patent Publication No.
281,822 A2, Examples 1, ~, 7 and 24, using transformant Escherichia coli MM294/pTB76~ (IFO 14613, FERM BP-1645).
The transformant Escherichia coli MM294/pTB762 described above was deposited with the Institute for Fermentation, Osaka (IFO), Japan and with the Fermentation Research Institute, Agency of Industrial Science and Technology, Ministry oE International Trade and Industry tFRI), Japan. 'rhe accession number and the deposit date are shown in Table 1. As to the deposit in FRI, the deposit was initially made under accession number denoted by FERM P
number. Said deposit was converted to the deposit under Budapest Treaty and the transformant has been stored at FRI
under acces~ion number denoted by FERM BP.
Table 1 Transforman _ _ IFO _ FRI
E. coli MM29A/ IFO 14613 FERM P-9409 FER~ BP-1645 _p'rB762 (May 27,1987) (June 11, 1987) ,. : ,. :
- . ~ , :
Reference Example 1 The FGF activity in Examples described below was measured by the following method.
Samples diluted in 2-fold step with DMEM medium S containing 10% calf serum were added to a Nunc*96-well microtiter plate (flat base) in an amount of 50 ~1 per well, and then each well wa-s seeded with 50 ~1 (2 X 103 cells) of fetal bovine cardiac endotherial cells (CRL139S) purchased from American Type Culture Clollection, followed by cultivation for 3 days. Then, to each well was added 20 ~1 of MTT [ 3-(4,5-dimethyazolyl-2-yl~-2,5-diphenyltetr~zolium bromide] [Journal of Immunological Method 93, 1S7 (1986)~
solution (5 mg/ml PBS, Sigma). After 4.5 hours, 100 ~1 o 10% SDS-0.01 N HCl was added thereto, and then the microtiter plate was allowed to stand overnight.
Thereafter, the absorbance at 590 nm was measured by using Titertek Multiscan [Tada et al., Journal of Immu _loqical Method 93, 157 (1986)~
Example 1 Sodium dextran sulfate having a mean molecular weight of 7,500 (Seikagaku Kogyo, Japan) was added to a 50 mM
sodium citrate solution ~pH 8.0) containing rhbFGF mutein CS23 in a concentration of 450 ~g/ml so as to give a concentration of 210 ~g/ml. ~hen, 1 ml of the resulting solution was adde~ to 5 g of low-substituted hydroxypropyl cellulose (hereinafter referred to as L-HPC) (LH-2or Conterlt of hydroxypropyl group: 13.0 to 16.0~, Shin-Etsu *Trade-mark - , ~ -. . .... . .
,: : :
:, : ~ i . , .:: ,. , :
:: .: : .
2 ~ % ~
Chemical), followed by sufficient stirring. The rnixture thus obtained was dried at room temperature (about 20C) under reduced pressure (about 5 mm Hg~ for 20 hours to obtain a crude powder composition containing rhbFGF mutein CS23 and L-HPC.
As a control, a powder composition containing rhbFGF
mutein CS23 and lactose was prepared in the same manner as the above method except that 5 g of lactose was used in place of L-HPC.
The remaining activity of these compositions was measured by the method described in Reference Example 1.
The results are shown in Table 2.
Table 2 Additive Remaining FGF Activitv (%) Lactose _ 8 Example 2 Sodium dextran sulfate having a mean molecular weight of 7,500 was added to a 50 mM sodium citrate solution (pH
8.0) containing rhbFGF mutein CS23 in a concentration of 500 ~Ig/ml so as to give a concentration vf 233 ~g/ml. Then/ 1 ml portions of the resulting solution were added to 5 g of L-~PC (LH-ll, Corl~ent of hydroxypropoxyl group: 10.0 to 13.0~, Shin-Etsu Chemical) and to 5 g of lactose, respectively, ollowed by sufficient stirring. The mixtures thus obtained were lyophili2ed to obtain powder compositions containing rhbFGF mutein CS23 and L-HPC, and rhbFGF mutein CS23 and lactose, respectively.
:: . ~ ' ,~ , : .-''.'. :.
2~2~
STABILIZED FGF COMPOSITION AND PRODUCTION THEREOF
BACKGROUND OF THE INVENTION
The present invention relates to a stabilized fibroblast growth factor thereinafter briefly referred to as FGF) protein composition, a method for preparing a stabilized FGF protein composition, and a method for stabilizing an FGF protein.
FGF was first isolated as a factor exhibiting strong growth promoting action on fibroblasts such as BAL~/c3T3 cells [D. Gospodarowicz, Nature 249, 123 (1974)3. It is now known that the FGF exhibits growth promoting action on almost all cells derived from mesoblast~ FGF is classified into basic FGF (hereinafter briefly referred to as bFGF) and acidic FGF (hereinafter briefly referred to as aFGF), based on the isoelectric point thereof. bFGF and aFGF both have strong growth promoting action and plasminogen activator inducing action on vascular endothelial cells. Together, these actions suggest a potential for the application thereof as a drug for promoting angiogenesis, as a therapeutic drug for traumas, and as a preventive and therapeutic drug for thrombosis, arteriosclerosis, etc.
Previously, the FGFs were purified to homogeneity from organs derived from animals, such as bovine pituitary.
However, supply o~ these F'GFs was limited, and there was a Eear of antigenicity due to their hetel^ozoic origin.
Recently, there has been developed a method for producing ., ' : ,.
2~2~6~
FGF in large quantities. The method involves using recombinant DNA techniques to express a cloned human FGF
gene in microorganisms or in animal cells. [FEBS Letters 213, 189-194 (1987); Buropean Patent Publication (hereinafter also referred to as EP Publication) No.
237,966)].
In other way, in order to stabilize polypeptide producing factors, an aqueous medical composition characteri~ed by comprising water-soluble polysaccharides in enough amount for stabilizing a growth factor was provided, and it is stated that the composition is effective against declining of activities of mitogen of the polypeptide growing factor and declining of bioactivities [Japanese Unexamined Patent Publication No. 63-152324/1988 corresponding to EP Publication ~o. 267/015].
Since most of the FGF proteins are very unstable, not only they are rapidly inactivated in aqueous solution, but also thier bioactivity easily reduces even by lyophilization. Further, when the FGF proteins are administered for many hours as intravenous drip, a reduction in titer during that time is unavoidable, which causes a major problem.
l`he above-de~cribed aqueous medical composition comprising water-soluble polysaccharides, especially in the ca~e of cellulose derivatives of a degree of ether substitution of at least 0.35 of ether groups per anhydro-glucose unit in the cellulose chain ~ln the case of hydroxy-propyl cellulose, the degree of substitution of hydroxypropoxyl , ~
:
~o~
~ 3 ~ 27580-51 residue is at least 35~)~ it is difficult to form solid medical composition in powder when the base is an FGF protein.
Titer of the composition is lowered during mixing and drying process.
SUMMARY OF THE INVENTION
The present inventors have discovered that the stability of FGF pro~eins is surprisingly increased by admixing an FGF protein with a water-insoluble hydroxypropyl cellulose.
In particlular, the present inventors have succeeded in obtaining a solid composition having an improved stability of FGF protein as compared with that of the above-described aqueous medical composition comprising FGF protein and water-soluble polysaccharides.
In accordance with the present inven~ion, there is provided (1) a stabilized FGF protein composition which comprises an F~F protein and water-insoluble hydroxypropyl cellulose; ~2) a method for preparing a stabilized FGF
protein composition, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose; and (3) a method for stabilizing an FGF protein, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose.
DESCRIPTIO`N OF THE PREF~RRED EMBODIMENTS
The FGF proteins used in the present invention may include basie FGF ~hereina~ter also referred to as bFGF) and acidic FGF ~hereina~ter also referred to as aFGF). The FGF
.
. .
~, - . .- , 2 fJ~
protein used in the present invention include those derived from mammals. The mammals include human, monkey, pig, bovine, sheep and horse.
The FGF proteins include those extracted from various organs in which the presence of FGFs is already known, such as brain and pituitary.
Further, the FGF proteins include tho6e obtained by the recombinant DNA technique ~FEBS Letters 213, 189-194 ~1987~;
EP Publication No. 237,966~.
Hereinafter, the recombinant human basic FGF may be referred to as rhbFGF.
The FG~ proteins used in the present invention include a FGF mutein.
Examples of the muteins of the FGFs used in the present invention include the muteins disclosed in Biochemical_and Bivphysical Research Communications 151, 701-708 (1988), EP
No. 281,822 A2, EP Publication No. 326,907 Al; and there may be included the muteins introduced by at least one glycosylation site diclosed in Japanese Patent Application No. 109014/1990 ~filed on April 25, l990j which corresponds to European Pa~ent Application No. 90107737.0 and U.S. Patent Application Ser. No. 511,469.
For example, the FGF muteins used in the present invention are obtained essentially by variations o~ the amino acid se~uences oE the original peptides or proteins.
Such variations include addition o~ amino acid~s), deletion : -.
~`
~ ": ' '' of constituent amino acid(s) and substitution of constituent amino acid(s) by different amino acid(s). Further, FGF
muteins introduced by glycosylation site are included in such variations.
Such addition of amino acid(s) includes addition of at least one amino acid.
Such deletion of constituent amino acid(s) includes deletion of at least one FGF-constituent amino acid.
Such substitution of constituent amino acid(s) by different amino acid~s) includes substitution of at least one FGF-constituent amino acid by at least one different amino acid.
At least one amino acid in the mutein which has at least one amino acid added to the FGF excludes methionine lS derived from the initiation codon used for peptide expression and a signal peptide.
The number of the added amino acid(s) is at least one.
However, it may be any number as long as FGF characteristics are not lost. More preferable amino acids include some or all of the amino acid sequences of proteins which have homology with the FGFs and which exhibit activities similar to those of the FGFs.
As for the number of the deleted FGF-constituent amino acid(s) in the mutein which lacks at least one FGF-con~tituent amino acid, it may be any number as long as FGFcharacteristics are not lost.
Example~ oE the deleted constituent amino acid include ~ . - : : ,:: :, :,.-,. . :
- , . ~. . . , ;; , : .:.: . , , , . :........... ::: : :.. ., - - .: . . .................. . . .
.
~20~
the 10 residues on the amino termial side of the human bFGF:
Met-Pro-Ala-Leu-Pro-Glu-~sp Gly-Gly-Ser, the 14 residues on the amino terminal side of the human bFGF:
Met-Pro-Ala-Leu-Pro-Glu-Asp-Gly-Gly-Ser-Gly-Ala-Phe-Pro, -the 41 residues on the amino terminal side of the human bFGF:
Met-Pro-Ala-Leu~ .. -Val, the 61 residues on the carboxyl terminal side of the human bFGF:
Lys-Cys- -Val-Ser.
The muteins further include muteins lacking the 7 to 46 amino acid residues on the carboxyl side of the original peptide or protein of the bFGF.
Preferred examples of such deletion include deletion of the following amino acid sequences of the rhbFGF:
~nino acid sequence from amino acid No. 102 on Amino acid sequence from amino acid No. 105 on Amino acid sequence from amino acid ~o. 115 on Amino acid sequence from amino acid No. 119 on Amino acid sequence from amino acid No. 124 on Amino acid sequence from amino acid No. 130 on ~nino acid sequence from arnino acid No. 138 on As for the number of FGF-constituent amino acids prior , ~ . . . :. .; ~. , : .. : . -2~20~
to substitution in the mutein, which has at least one FGF-constituent amino acid substituted by at least one different amino acid, it may be any number as long as FGF
characteristics are not lost.
Examples of the constituent amino acids prior to substitution include cysteine and cystine, but c~steine is preferable~ The constituent amino acids other than cysteine prior to substitution include aspartic acid, arginine, gl~cine and valine.
When the constituent amino acid prior to substitution is cysteine, neutral amino acids are preferable as the substituted amino acids. The neutral amino acids include glycine, valine, alanine/ leucine, isoleucine, tyrosine, phenylalanine, histidine, tryptophan, serine, threonine and methionine. Serine and threonine are particularly preferred.
When the constituent amino acid prior to substitution is any one other t'nan cysteine, amino acids which are different, for example, in hydrophilicity, hydrophobicity or electric charge from the amino acid prior to substitution are selected as the substituting different amino acids.
Speciically, when the amino acid prior to substitution is aspartic acid, the substituting amino acids include asparagine, threonine, valine, phenylalanine and arginine.
~n particular, asparagine and arginine are preEerable.
When the amino acid prior to substitution is arginine, the substituting amino acids includes glutamine, threonine, . - . . . :: -:
.. .. . ....
, . :- :
2`i~2 ~
leucine~ phenylalanine and aspartic acid. Glutamine is especially preferableO
When the amino acid prior to substitution is glycine, the substituting amino acids include threonine, leucine, phenylalanine, serine, glutamic acid and arginine.
Threonine i5 particularly preferred.
When the amino ~cid prior to substitution is serine, the substituting amino acids include methionine, alanine, leucine, cysteine, glutamine, arginine and aspartic acid.
In particular, methionine is preferable.
When the amino acid prior to substitution is valine, the substituting amino acids include serine, leuciner proline, glycine, lysine and aspartic acid. Serine is especially preferred.
As the original constituent amino acids prior to substitution, aspartic acid, arginine, glycine, serine and valine are preferably selected.
As the substituting amino acids, asparagine, glutamine, arginine~ threonine, methionine, serine and leucine are preferably selected.
The most preferred substituted muteins include a mutein in which cysteine, the constituent amino acid, is substituted by serine.
In the above substitution, the substitution of at least ~5 two constituent amlno acids may be simultaneously carried out. In particular, it is pr~ferable to substitute two or three constituent amino acids.
.. , . . . . ~, . .
.~ . ~ , . . ~. , , . - : . - - ... .
Q6~
g The muteins may be obtained by a combination of two or three of the above-mentioned addition, deletion and substitution.
A mutein is preferable in which at least one human bFGF-constituent amino acid is substituted by at least one different amino acid. In particular, rhbFGF mutein CS23 is preferable in which cysteine residues at the 70- and 88-positions of human bFGF are substituted by serine residues, respectively.
The EGF mutein has had introduced at least one glycosylation site. And the mutein may further have sugar chain(s).
The glycosylation sites include a site in which an amino acid sequence constituting the glycosylation site is represented by the following the formula:
Asn-X~Y
(wherein X may be any amino acid residue, and Y is Thr, Ser or Cys).
X is preferably an amino acid other than Pro, and more preferably Gly, Tyr, Arg, Ser, Iys, Val or Ala and more preferably Gly, Lys, Val or Ala. Y is preferably Thr or Ser.
The sugar which is added to a FGF mutein may be any one ~ound in known glycosylated proteins. Examples of such sugars include N-acetyl glycosamine, N-acetyl galactosarnine, mannose, galactose, ~ucose and cyalic acid.
The number of sugars in a glycosyl chain is preferably ., .. . : ..
'. ~
.:
:~: . . ~ . :
~ ~2.~
at least one, and more preferably 10 to 20~
In order to produce the muteins, site-directed mutagenesis is employed. This technique is ~ell-known and described in R. F. Lather and J. P. Lecoq, Genetic Enqineerinq, pp. 31-50, Academic Press (1983). Mutagenesis directed to oligonucleotide is described in M. Smith and S.
Gillam, Genetic ~nqi~eerinq: Principles and Methods, Vol. 3, pp. 1-32, Plenum Press (1981).
The production of a structural gene which encodes the mutein is carried out, for example, by the steps o~:
(a) hybridizing a single-stranded DNA comprising a single strand of the structural gene of FGF with a mutagenic oligonucleotide pximer(the above-mentioned primer is complementary to a region, including a codon for cysteine, to be replaced by this single strand, or including an anti-sense triplet which forms a pair with this codon in some cases, provided this does not apply to disparity with other codon ~or the amino acid than the above codon, or with the anti-sense triplet in some cases.), (b) elongating the primer using DNA polymerase to Eorm a mutational heteroduplex, and (c) replicating this mutational heteroduplex.
q`hent phage DN~ for transferring the mutagenized gene is isolated and introduced into a plasmid.
~ suitable host is transEormed with the plasmid thus obtained, and the obtained transformant is cultivated in a medium, thereby beinq capable o~ producing the mutein.
. .
- . : : - ; . ..
~ 75~0-51 Examples of the water-insoluble hydroxypropyl cellulose include a low-substituted hydroxypropyl ether of celluloseO
The low-substituted hydroxypropyl cellulose contains not less than 5.0~ and not more than 16.0% by weight hydroxypro-poxyl group on a dry basis (i.e. when dried at 105C for 1 hour).
(Refer to the Japanese Pharmacopeia, the 11th revision D-733 to D-780; and The U.S. Pharmacopeia, the 21st revision, Supplement, pages 5180 to 5181).
Examples of low-substituted hydroxypropyl cellulose used in the present invention include low-substituted hydroxy-propyl cellulose ~LH-ll, LH-20, LH 21, LH-22 and L~I-31, Shin-Etsu Chemical, Japan).
In the present invention, the weight ratio of the FGF
protein to water-insoluble hydroxypropyl cellulose is preferably about 1 : 0.01 to 1,000,000, more preferably about 1 : 1 to 100l000, still more preferably about 1 : 500 to 20,000, and especially preferably about 1 : 500 to 10,000.
Further, the composition of the present invention may further contain one or more members selected from sugars, proteins, amino acids, sodium chloride and gum arabic.
The sugars include, for example~ sucrose, trehalose, maltose, fructose, inositole and amylose. The proteins include, for example, casein, albumine, gelatin and egg white. The amino acids include, Eor example, cysteine, phenylalanine, leucine and glycine.
In the present invention~ the weight ratio oE FGF
protein to sugars, proteins, aminc~ acids, sodium chloride 2 ~ 5 ~
- 12 - 2758o-5l and/or gum arabic is preferably about 1:0.01 to 1,000,000, more preferably about 1:1 to 100,000, still more preferably about 1:500 to 20,000, and especially preferably about 1:500 to 10,000.
The compositions of the present invention are obtained by admixing the FGF protein with the water-insoloble hydroxypropyl cellulose, for example, by adding an aqueous solution of the FGF protein to water-insoluble hydroxypropyl cellulose in powder, followed by mixing. The pH of the aqueous solution of the FGF protein is preferably adjusted to about 3 to 10, more preferably to about 5 to 9.
The addition and th~ mixing are carried out, for example, at about 10 to 30C, preferably at about 10 to 20C.
The mixing is sufficiently performed by devices generally used for stirring and granulation [such as a mortar, a Pony*mixer (Hosokawa Tekkosho, Japan), a Vertical*
granulator (Fuji Sangyo) and a Super*mixer (Hosokawa Tekkosho)], by devices used for fluidized granulation [such as Glad*(Okawara Seisakusho)] and by devices used for rolling granulation [such as CF (Freund)].
The compositions thus mixed are, for example, driecl or lyophilized at room temperature (about 10 to 30C) under : reduced pressure (about 10 mmHg or less), whereby the solid compositions stabilized in bioac~ivity can be obtained.
Sugars, proteins, amino acids, sodium chloride and/or gum arabic may be simultaneously added when water-insoluble *Trade-mark .
.. . .
' . ` . "'`' ' ' . ' ' .' : ` .
.` ` ` ' ~ ""` ~` :' 2 ~
hydroxypropyl cellulose and FGF protein are mixed, or they may be mixed with water-insoluble hydroxypropyl cellulose, followed by adding FGF protein. The production method of the composition is carried out by similar method with that of the composition comprising water-insoluble hydroxypropyl cellulose and FGF protein.
In the above mixing, the aqueous solution of the FGF
proteln stabilized with glucan sulfate may be used.
Examples of the glucan sulfate include dextran sulfates, cyclodextrin sulfates and ~-1,3 glucan sulfates.
All of these are sulfuric ester derivative of polymer of D-glucose. The sulfur content in the glucan sulfate is preferably not less than about 3% by weight, more preferably about 12 to 20~ by weight, most preferably about 16 to 20%
by weight. In particular, dextran sulfate is preferable.
The dextran sulfates include a sulfate of dextran produced from sucrose by the action of a microorganism such as Leuconostoc mesenteroi es. The dextran sulfate is a partial sulfates of dextran mainly containing ~(lt6) linkage, and the sulfur content therein is usually at least about 12% by weight, preferably about 16 to 20% by weight.
The average molecular weight thereof is in the range of about 1,000 to 40,000,000, preferably in the range of 3,000 to S00,000. The dextran sulfate is very easily soluble in water, and is a compound already known in the art, which is manufactured by known methods ~er se.
Cyclodextrin in the cyclodextrin sulfate includes t`
~o~
cyclodextrin produced from starch by the action of a microorganism such as Bacillus macerans. The cyclodextrin has ring structure of D-glucose molecules linked by ~ 4) linkage, and includes an ~-type (6 molecules) r a ~-type (7 molecules) and a y-type (8 molecules). In this invention, any of these forms may be used.
The cyclodextrin sulfate is obtained by sulfation of the cyclodextrin, and the sulfation is conducted according to methods already known in the art. The methods for sulfation include the methods described in U.S. Patent No.
2,923,704 and Japanese Patent Unexamined Publication No.
50-36422/lg75, The sulfur content in the cyclodextrin sulfate is usually at least about 3% by weight, preferably about 12 to 24% by weight. The cyclodextrin sulfate has the property of being very soluble in water.
The degree of sulfation of the cyclodextrin sulfate may be any degree as long as the sulfur content is at least about 12~ by weight. In particular, the cyclodextrin sulfate whose sulfur content is about 16 to 21% by weight are advantageously used. Mixtures of the sulfates different from one another in degree of sulfation may be used as such, or the purified sulfates having the single degree of sulfation may be used. The puriEication can be conducted, ~5 for example, by concentrating a reaction solution containing an alkali metal salt of ~-cyclodextrin sulfate, evaporating it to dryness, dissolving the condensate in water, and :. . :
-` 2~Q~
mixing the resulting aqueous solution with a hydrophilic solvent to separate a desired product.
~ -1,3-glucan in the ~-1,3-glucan sulfate includes straight-chain ~-1,3-glucans, which are produced by microorganisms belonging to Alcaliqenes or Agrobacterium.
There may be in the form of a low molecular weight polymer obtained by hydrolysis of the straight-chain ~ 1,3-glucans and similarly having a straight-chain ~-1J3-glucan structure.
Curdlan (also known as a thermogelable polysaccharide PS and available from Wako Pure Chemical Industries Ltd.
Japan) is known as a water-insoluble, thermogelable~
unbranched glucan, and has straight-chain ~-1, 3-glucan linkage alone which is produced from a microbial strain belonging to Alcaligenes or Aqrobacterium [Japanese Patent Publication Nos. 43- 7000/1968, 48-32673/1973 and 48-32674/1976].
The Alcaligenes faecalis var. Myxo~enes NTK-u strain, the Aqrobacterium radiobacter strain and the Agrobacterium ._ radiobacter U-l9 strain, which produce Curdlan, are cited in ~merican Type Culture Collection Cataloque of Strains, the 15th edition (1982), as ATCC- 21680, ATCC-6466 and ATCC-21679, respectively.
The properties o~ partially hydrolyzate oE Curdlan and the method for preparation thereof have already been described in detail in Japanese Patent Unexamined Publication No. 55- 83798/1980.
: :
.,, Thus, the straight-chain ~-1,3-glucan is a compound represented by the following formula:
~ ~ j H~\ I ON
wherein n is an integer of 4 to about 1,000.
Any of the ~-1,3-glucans described above may be used as -long as the average degree of polymerization (DP) thereof is not more than 1,000. In particular, there are advantageously used the partically hydrolyzed products thereof having an average degree of polymerization tDP) of 6 I5 to about 300, more preferably 15 to about 200.
n in the formula (I) has a relation to DP represented by the following equation:
DP - 2 = n.
The sul~ate of the straight-chain ~-1,3-glucan is produced by sulfonation of the three hydroxyl groups of the intermediate monosaccharide unit of the ~-1,3-glucan or its lower polymers and the hydroxyl groups of the monosaccharide units at both ends thereof. The sulfates having an average degree of substitution ~DS) of 0~5 to 3 per monosaccharide unit are usually usedr and preferably ones having an average degree oE substitution (DS) of 1 to 2 are advantageously used.
, .
", . ~ ' ,' -Sulfation of straight-chain ~-1,3-glucans or its low molecular weight polymer can be achieved by allowing a sulfating agent such as chlorosulfonic acid or sulfuric anhydride to act thereon, or by reacting a complex of sulfuric anhydride and an organic base such as pyridine, dimethylformamide, trimethylamine or dimethylaniline therewith [J. Biol. Chem. ~39, 2986 (1964)].
The ~-1,3-glucan sulEate is very soluble in water and low in toxicity. The sulfur content in ~-1,3-glucan sulfates is usually at least about 5% by weight, preferably about 10 to 24% by weight.
The glucan sulfate is very low in toxicity to warm-blooded animals. This is therefore advantageous for ;
parenteral or oral administration of the stabili~ed compositions comprising the FGF protein and the glucan sulfate to the warm-blooded animals.
The glucan sulfate may be used in the state of free or salt. Examples of such salts include sodium salts, potassium salts, ammonium salts and trimethylammonium salts.
When the glucan sulfate is brought into contact with the FGF protein in aqueous media, the free glucan sulfate may be added thereto, followed by addition of proper amount of an alkali or acid to give the desired pH. By the addition of alkali, the glucan su].fate may be exist in the 2~ aqueous media in khe ~orm o~ either its salt or a mixture of the free dextran sulfate and its salt.
If the FGF protein is brought into con-tact with glucan .,~ ......... .
.
:. . -, ~: :
:~ . . :~: . -- 18 - ~
sulfate in aqueous media in the presence of an additional dlbasic or tribasic carboxylic acid, the FGF protein is advantageously more stabilized.
Examples of the dibasic carboxylic acids include tartaric acid, maleic acid, malic acid and fumaric acid~
The tribasic carboxylic acids include, for example, citric acid and isocitric acid.
The above carboxylic acids may be used in the form of either free compounds or their salts. E~amples of such salts include sodium salts, potassium salts and ammonium salts~
Further, the free carboxylic acid may be added thereto, followed by addition of proper amounts of an alkali or acid to give the desired pH. By the addition of the alkali, the carboxylic acid may be exist in the aqueous media in the form of either its salt or a mixture of the free acid and its salt.
When the FGF protein is brought into contact with the glucan sulfate in aqueous media, it is preferred that the glucan sulfate is a~ded in an amount of about 0.1 to 100 mol/mol, more preferably about 0.5 to ~ mol relative to 1 mol of FGF protein.
The concentration of the glucan su~fate in the aqueous media is preferably about 0.0005 to 5% by w/v, more pre~erably about 0.01 to ]% by w/v.
The concentration o~ the FGF protein in the aqueous media i9 preferably about 0.0005 to 5~ by w/v, more ;:
, ' ' ' ' . ' ~
- 2~2~
preferably about 0.01 to 1% by w/v.
The concentration of the carboxylic acid in the aqueous media is preferably about 1 mM to lM, more preferably about 10 mM to 500 mM.
For their contact in the aqueous medium, the object can be attained only by mixing the FGF protein, the glucan sulfate and the carboxylic acid as required with one another in the aqueous medium.
The aqueous media may be any media such as distilled water, physiological saline solution and glucose solution are preferably used. As the aqueous media, there can also be used buffers such as phosphate buffer and tris~hydroxymethyl)aminomethane-HCl buffer.
When the FSF protein, the glucan sulfate and the carboxylic acid as required are mixed with one anotherl they may be mixed as aqueous solutions, respectively, or may be mixed as solids, respectively, followed by dissolution in the aqueous medium. In mixing, the temperature is preferably about 0 to 40C, and the pH is preferably in the range of about 3 to 10, more preferably in the range of about 5 to 9. The time taken to mix is usually about 1 to 30 minutes.
Thus, the aqueous solution of the FGF protein stabilized with glucan sulfate is obtained.
In the present invention, the above-described composition comprising FGF protein and water-in~oluble hydroxypropyl cellulose may be further coated by an enteric polymer.
.... ,., ~ : :: :... . ;, .
21~1D6~
Examples of the enteric polymers used in the present invention include hydroxypropyl methyl cellulose phthalate, carboxymethyl ethyl cellulose, cellulose acetate phthalate, hydroxymethyl cellulose acetate succinate and acrylic polymers [such as methacrylic acid-ethyl acrylate copolymers (Eudragit*L30D-55 and Eudragit*L100-55~, methacrylic acid-methyl acrylate copolymers (Eudragit L-100) and methacrylic acid-met-hyl methacrylate copolymers (Eudragit S100~, Rohm, West Germany].
The coating is conducted by known methods per se.
Namely, dispersions or solutions obtained by dispersing or dissolving the coating bases in water or organic solvents are sprayed on the tablets, the granules or the fine grains by pan coating methods, fluidized coating methods, the rolling coating methods or the like. When the compositions are coated with the coating agents, it is desirable that the temperature of the composition to be coated is about 25 to 70C, preferably about 25 to 50C. The coating amounts are about ~0 to 300%, preferably 50 to 100~ as the intestinally soluble polymers based on the compositions.
Further, the solid composition ~powder) vf the present invention and fatty acid ester of polyglycerol granules can also be heated and fluidized to obtain granules. According to the granules, the eE~ective 1ngredient tE'G~ protein) of the solid composition o~ the present invention is stably eluted and released, and stabilized for a long time.
When the fatty acid ester oE polyglycerol is a mi~ture, *Trade-mark , it does not show a clear melting point and is softened at a specific temperature in some cases. In this specification, the "melting point" includes a softening point which such a mixture shows.
The fatty acid ester of polyglycerol used above may be any of a monoester, a diester and a polyester as long as it is an ester formed by the combination of a polyglycerol with a fatty acid. The fatty acid ester of polyglycerol , unlike hardened oil and so on, has the characteristics of showing no crystal polymorphism and having little interaction with effective ingredients such as drugs.
The polyglycerin is "a polyhydric alcohol having n (in a cyclic polyglycerin) to n + 2 (in a straight or branched polyglycerin) hydroxyl groups and n - 1 (in a straight or branched polyglycerin) to n (in a cyclic polyglycerin) ether combinations in one molecule" [Polyqlycerin Ester, p. 12, edited and published by Sa~amoto Yakuhin Kogyo Co. Ltd., Japan ~May 2, 1986)]. For example, compounds represented by the following formula can be used.
20 HO(cH2_1cH_cH2_O)nH
OH
wherein n indicates a degree of polymerization and is an integer of 2 or more. n is normally 2 to 50l preferably 2 to 20, more preferably 2 to 10. The polyglycerol is straight or branched.
Specific examples oE such polyglycerols include diglycerol, triglycerol, tetraglycerol, pentaglycerol, ,: ... . ..
, . . .
.. - .... ..
hexaglycerol, heptaglycerol, octaglycerol, nonaglycerol, decaglycerol, pentadecaglycerol, eicosaglycerol and triacontaglycerol. Of these polyglycerols, for example, tetraglycerol, hexaglycerol and decaglycerol are frequently used.
The fatty acids include, for example, saturated or unsaturated higher fatty acids having 8 to 40 carbon atoms, preferably 12 to 22 carbon atoms. Examples of such fatty acids include palmitic acid, stearic acid, oleic acid, l~ linolic acid, linolenic acid, myristic acid, lauric acid, ricinolic acid, caprylic acid, capric acid and behenic acid.
of these fatty acids, for example, stearic acid, oleic acid, lauric acid and ricinolic acid are preferable.
Specific examples of the fatty acid ester of polyglycerol include caprylyl mono(deca)glyceride, caprylyl di(tri)glyceride, lauryl mono(tetra)glyceride, lauryl mono(hexa)glyceride, lauryl mono(deca)glyceride, oleyl mono(tetra)glyceride, oleyl mono(hexa)-glyceride, oleyl mono(deca)glyceride, oleyl di(tri)glyceride, oleyl di(tetra)glyceride, oleyl sesqui(deca)glyceride, oleyl penta(tetra)glyceride, oleyl penta(hexa)glyceride, oleyl deca(deca)glyceride, linolyl mono(hepta)glyceride, linolyl di~tri)glyceride, linolyl di(tetra)glyceride, linolyl di~hexa)glyceride, stearyl mono~tetra)g].yceride, stearyl rnono~hexa)glyceride, stearyl mono~deca)glyceride, stearyl tri(tetra)glyceride, stearyl tri(hexa)glyceride, stearyl sesqui(hexa)glyceride, stearyl penta(tetra)glyceride, ,~,: . :
: . , . : . :
~i~ 2 ~
stearyl penta(hexa~glycedride, stearyl deca(deca)glyceride/
palmityl mono(tetra)glyceride, palmityl mono(hexa)glyceride, palmityl mono(deca)glyceride, palmityl tri(tetra)glyceride, palmityl tri(hexa)glyceride, palmityl sesqui~hexa)glycoride, palmityl penta(tetra)glyccride, palmityl penta(hexa)-glyceride and palmityl deca(deca)glyceride. Examples of the preferred fatty acid ester of polyglycerol include stearyl penta(tetra)glyceride (for example, PS-310, Sakamoto Yakuhin Co., Japan), stearyl mono(tetra)glyceride (for example, MS-310, Sakamoto ~akuhin Co.), stearyl penta(hexa)~
glyceride (for example, PS-500, Sakamoto Yakuhin Co.), stearyl acid sesqui(hexa)glyceride (for example, SS-500, Sakamoto Yakuhin Co.) and stearyl mono(deca)glyceride~
These fatty acid ester of polyglycerol are used alone or as mixtures of two or more kinds.
The melting point of the fatty acid ester of polyglycerol is about 40 to 80C, preferably about 40 to 60C.
The molecular weight of the fatty acid ester of polyglycerol is usually 200 to 5,000, preferably 300 to 2,000. The hydrophile-lypophile balance (~LB) thereof is l to 22, preferably l to 15, and the elution rate of the effective ingredient of the powder can be controlled by adjusting the HLB. The H~B can also be ad~usted by mixing two or rnore kinds o~ atty acid ester of polyglycerol.
The fatty acid ester of polyglycerol can also be used together with lipids. ~s the lipids are used water-.. . , ~. ................................ .
: ' . ' . ~ :' . , ~2~
insoluble materials permissible depending on the purpose of preparations and the like. The preferred softening point or melting point of the lipids is about 40 to 120C, particularly about 40 to 90C.
Specific examples of the lipids include the hardened products of fats and oils such as castor oil, cotton seed oil, soybean oil, rapeseed oil and beef tallow; waxes such as beeswax, carnauba wax, spermaceti, lecitin, paraffin and microcrystalline wax; fat~y acids such as ~tearic acid and palmitic acid, or fatty acid salts such as sodium sa].ts and potassium salts of fatty acids; fatty alcohols such as stearyl alcohol and cetyl alcohol; and glycerides. Of these lipids, there are preferable, for example, hardened cotton seed oil, hardened castor oil, hardened soybean oil, carnauba wax, microcrystalline wax, stearic acid and stearyl alcohol.
The ratio of the lipid to the fatty acid ester of polyglycerol is usually 100 parts by weight or less of lipid per 100 parts by weight of fatty acid ester oE polyglycerol, and can be suitably selected within the above range.
In the preparation of the granulated compositions, spherical fatty acid ester of polyglycerol granules are preferably used to adhere the powders (the solid compositions o.E the present invention) in large amounts to the fatty ac.id ester of polyglycerol or to allow the esters to contain the powders in large amounts, and to obtain the granulated compositions corresponding to the shape and the , : . , . : , ~ .
. .
- - 2~2~
size of the fatty acid ester of polyglycerol granules. When the spherical fatty acid ester of polyglycerol granules are used, large amounts of powders (the solid compositions of the present invention), for example, the powder constituting about 80% by weight of the whole granulated composition, can be incorporated therein. Moreover, the spherical granulated compositions relatively smooth in surface and narrow in size distribution can be obtained. In some cases, the powder can be incorporated therein so as to constitute more than ~0~ by weight, for example, about 85% by weight, of the whole granulated composition.
The spherical fatty acid ester of polyglycerol granules can be obtained, for example, by spray cooling, preferably spray chilling. The spray chilling can be carried out by rotating a disk such as an aluminum disk having a smooth sur~ace and dripping the molten fatty acid ester of polyglycerol thereon. The rotary disk is not particularly limited in size, but is about 5 to lO0 cm, preferably about lO to 20 cm in di.ameter. The rotational speed of the rotary ~ disk and the dripping rate of the molten fatty acid ester of polyglycerol can be dekermined depending on the desired size and the like of the granules. The rotational number of the rotary dis]c is usually abouk lO to 6,000 rpm, preferably 900 to 6,000 rpm, more preferably 1,000 to 3,000 rpm. The molten fatty acid ester of po:LygLycerol can be dripped at a constant rate, for example, of about 2 to 200 g/min, preferably about 5 to lO0 g/min.
~;
.,: ; , :, , .:, - i ; ~ , -. , :
~, ,, ; ~ -: :, : :
; ~ ' ' ! , The size of the fatty acid ester of polyglycerol granules can be selected according to the desired size of the granulated composition and is not particularly limited, but is usually about 10 to 150 meshes, preferably about 25 to 100 meshes.
The solid compositions (powders) of the present invention can be used together with powdery diluents.
Examples of such diluents include excipients such as lactose, cornstarch, Avicel*(microcrystalline cellulose:
Asahi Chemical Industry, Japan), powder sugar and magnesium stearate; binders such as starch, gelatin, gum arabic powder, methyl cellulose, carboxymethyl cellulose sodium, hydroxypropyl methyl cellulose and polyvinyl pyrrolidon;
disintegrators such as carboxymethyl cellulose calcium and low substituted-hydroxypropyl cellulose; coloring agents;
flavoring agents; absorbents; preservatives; wetting agents antistatic agents; and d.isintegration delaying agents.
rrhe ratio of the powder (the solid cornposition of the present invention) to the above fatty acid ester of polyglycerol can be established depending on the desired size of the granulated composition, the content of the drug active ingredient and the like, but is usually 10 to 1,000 parts by weight, preferably 50 to 500 parts by weight of the powder per 100 parts by weight o the fatty acid ester of polyglycerol.
The granulation by heating and fluidizing can be conducted according to conventional 1uidized-bed *rrrade-mark ~ : .
. . ~. .
granulating methods. The heating temperature in the granulating methods is near the melting point of the above ~atty acid ester oE polyglycerol ester, preferably within the range from the melting point of the fatty acid ester of polyglycerol to the temperature 5C lower than the melting point. If the heating temperature is too high, the fatty acid ester of polygly-cerol granules tend to coalesce by fusion to form a granulated composition wide in size distribution. On the other hand, if the heating temperature is too low, it is difficult to granulate the powder (the solid composition of the present invention) with the fatty acid ester of polyglycerol granules.
The granulation can be performed by floating the fatty acid ester of polyglycerol granules and the powder (the solid composition o~ the present invention) to form a fluidized bed, and by heating and fluidizing them at a required temperature. It can be confirmed by the presence or absence of the powder particles whether or not the granulation is completed.
The granulated compositions thus obtained are usually ine-grained or granular.
When the granulated composition is observed under a microscope, it usually has a shape corresponding to the shape oE the ~atty acid ester oE polyglycerol granule, and ~5 1t seems that the powder (solid composition of the present invention) is at least partially embedded in the fatty acid ester of polyglycerol granulel pre~erably involved therein ; to coaleace.
' ` ~ , '`' ' ' , ,' ' .
, . ,' ~ ': ' ~", . ' . ` ' ' ' ' ' ` ' '~
,~ :
:' :
2 ~
The compositions of the present invention thus obtained are solid.
The compositions of the present invention include pharmaceutical compositions containin~ the above solid compositions (Eor example, ointments and suppositories)~
Namely, in the case of the ointments, the solid compositions of the present invent-ion are dispersed in bases for the ointments. In the case of the suppositoriesr the solid compositions of the present invention are dispersed in bases for the suppositorie5.
As the present FGF composition is stabilized, it can be advantageously used as a medicine.
The stabilized FGF protein compositions of the present invention can be safely administered parenterally or orally to warm-blooded animals (such as human, mouse, rat, hamster, rabbit, dog and cat) as such or with pharmacologically permissible additives (such as carriers, excipients and diluents), as pharmaceutical compositions tsuch as tablets, capsules, granules, fine grains, powders, ointments and suppositories)-Such preparations can be formulated into the formssuitable for oral administration such as tablets, capsules, powders, granules and fine grains in accordance with known methods per se, In these cases, as additives are used 23 excipients (such as lactose, cornstarch, light silica and ~ine crystalline cellulose), binders (such as alpha starch, methyl cellulose, carboxymethyl cellulose, hydroxypropyl ~ , ' P2~
cellulose, hydroxypropyl methyl celulose and polyvinyl pyrrolidone), disintegrators (such as carboxymethyl cellulose calcium, starch and low-substituted hydroxypropyl cellulose), surface active agents [such as Tween*80 (~ao Atlas, Japan), Pluronic*F68 (Asahi Denka Kogyo, Japan) and polyoxyethylene-polyoxypropylene copolymer], antioxidants (such as L-cysteine, sodium sulfite and sodium ascorbate) and lubricants (such as magnesium stearate and talc).
As to the tablets, the granules and the fine grains, coating may be carried out in accordance with known methods per se for the purpose of masking tastes or giving intragastric solubility, intestinal solubility or increasing :~
sustained release. As the coating agents are used, for example, hydroxypropyl methyl cellulose, ethyl cellulose, hydroxymethyl cellulose, hydroxypropyl cellulose, polyoxyethylene glycol, Tween 80, Pluronic*F68, castor oil, cellulose acetate phthalate, hydroxypropyl methyl cellulose phthalate, hydroxypropyl methyl cellulose acetate succinate, acrylic polymers (~udragitkL100-SS and L-100, Rohm, West Germany), carboxymethyl ethyl cellulose, polyvinyl acetal diethylamino acetate, waxes and pigments such as talc, titanium oxide and iron oxide red. These coating agents may be applied in one or more layers, alone or in combination of two or more agents.
The coat.ing is conducted by known method9 per se~
Namely, d.ispersions or so].utions obtained by dispersing or dis~olving the coating bases in water or organic solvents *Trade-mark , .,, ~ ' ` i , : , ,...................... .
` ~ ID 2 f~
are sprayed on the tablets, the granules or the fine grains by pan coating methods, fluidized coating methods or rolling coating methods. The tablets, the granules and the fine grains are preferably coated at about 25 to 70C, more preferably at about 25 to 50C.
Further, ointments and suppositories can be prepared according to known methods per se using the following additives.
Examples of the additives used when the ointments are prepared include vaseline, beweswax, paraffin, liquid paraffin, cholesterol, stearyl alcohol, lanolin, cetyl alcohol and polyethylene glycol.
Examples of the additives used when the suppositories are prepared include cacao butter, hydrogenated vegetable oils, monoglycerides, triglycerides, glycerogelatin and polyethylene glycol.
The FGF protein compositions of the present invention have growth promoting action on ibroblasts, high stability and low toxicity. Therefore, the FGF protein compositions can be used as therapeutic promoting drugs for burns, traumas, postoperative tissues and the like, or therapeutic drugs for thrombosis, arteriosclerosis and the like by arterializing action~ Also, they can be used as reagents ~or promotin~ cell cultivation.
When the FGF protein compositions of the present invention are used as the above-mentioned drugs, they are administered, for example, to the above-mentioned .
::
^ 2021D6~
warm-blooded animals in an approprlate amount ranging from about 1 ng/kg to 100 ~g/kg daily as the FGF protein, taking into account the route of administration, symptoms, etc.
Recombinant human bFGF mutein CS23 (hereinafter also referred to as rhbFGF mutein CS23) used in Examples hereinafter described is prepared by the method described in Biochemical and Biophysical Research Communications 151 r 701-708 (1988) or the method described in European Patent Publication No~ 281,822 A2. The rhbFGF mutein CS23 used in Examples hereinafter described was prepared and purified by the methods described in European Patent Publication No.
281,822 A2, Examples 1, ~, 7 and 24, using transformant Escherichia coli MM294/pTB76~ (IFO 14613, FERM BP-1645).
The transformant Escherichia coli MM294/pTB762 described above was deposited with the Institute for Fermentation, Osaka (IFO), Japan and with the Fermentation Research Institute, Agency of Industrial Science and Technology, Ministry oE International Trade and Industry tFRI), Japan. 'rhe accession number and the deposit date are shown in Table 1. As to the deposit in FRI, the deposit was initially made under accession number denoted by FERM P
number. Said deposit was converted to the deposit under Budapest Treaty and the transformant has been stored at FRI
under acces~ion number denoted by FERM BP.
Table 1 Transforman _ _ IFO _ FRI
E. coli MM29A/ IFO 14613 FERM P-9409 FER~ BP-1645 _p'rB762 (May 27,1987) (June 11, 1987) ,. : ,. :
- . ~ , :
Reference Example 1 The FGF activity in Examples described below was measured by the following method.
Samples diluted in 2-fold step with DMEM medium S containing 10% calf serum were added to a Nunc*96-well microtiter plate (flat base) in an amount of 50 ~1 per well, and then each well wa-s seeded with 50 ~1 (2 X 103 cells) of fetal bovine cardiac endotherial cells (CRL139S) purchased from American Type Culture Clollection, followed by cultivation for 3 days. Then, to each well was added 20 ~1 of MTT [ 3-(4,5-dimethyazolyl-2-yl~-2,5-diphenyltetr~zolium bromide] [Journal of Immunological Method 93, 1S7 (1986)~
solution (5 mg/ml PBS, Sigma). After 4.5 hours, 100 ~1 o 10% SDS-0.01 N HCl was added thereto, and then the microtiter plate was allowed to stand overnight.
Thereafter, the absorbance at 590 nm was measured by using Titertek Multiscan [Tada et al., Journal of Immu _loqical Method 93, 157 (1986)~
Example 1 Sodium dextran sulfate having a mean molecular weight of 7,500 (Seikagaku Kogyo, Japan) was added to a 50 mM
sodium citrate solution ~pH 8.0) containing rhbFGF mutein CS23 in a concentration of 450 ~g/ml so as to give a concentration of 210 ~g/ml. ~hen, 1 ml of the resulting solution was adde~ to 5 g of low-substituted hydroxypropyl cellulose (hereinafter referred to as L-HPC) (LH-2or Conterlt of hydroxypropyl group: 13.0 to 16.0~, Shin-Etsu *Trade-mark - , ~ -. . .... . .
,: : :
:, : ~ i . , .:: ,. , :
:: .: : .
2 ~ % ~
Chemical), followed by sufficient stirring. The rnixture thus obtained was dried at room temperature (about 20C) under reduced pressure (about 5 mm Hg~ for 20 hours to obtain a crude powder composition containing rhbFGF mutein CS23 and L-HPC.
As a control, a powder composition containing rhbFGF
mutein CS23 and lactose was prepared in the same manner as the above method except that 5 g of lactose was used in place of L-HPC.
The remaining activity of these compositions was measured by the method described in Reference Example 1.
The results are shown in Table 2.
Table 2 Additive Remaining FGF Activitv (%) Lactose _ 8 Example 2 Sodium dextran sulfate having a mean molecular weight of 7,500 was added to a 50 mM sodium citrate solution (pH
8.0) containing rhbFGF mutein CS23 in a concentration of 500 ~Ig/ml so as to give a concentration vf 233 ~g/ml. Then/ 1 ml portions of the resulting solution were added to 5 g of L-~PC (LH-ll, Corl~ent of hydroxypropoxyl group: 10.0 to 13.0~, Shin-Etsu Chemical) and to 5 g of lactose, respectively, ollowed by sufficient stirring. The mixtures thus obtained were lyophili2ed to obtain powder compositions containing rhbFGF mutein CS23 and L-HPC, and rhbFGF mutein CS23 and lactose, respectively.
:: . ~ ' ,~ , : .-''.'. :.
2~2~
- 3~ -The remaining activity of these compositions is shown in Table 3.
Table 3 Additive _Remaining FGF Activity (%) Lactose ll Example 3 -Using the powder composition containing rhbFGF mutein CS23 and L-HPC obtained in Example l, granules were prepared by the following method.
Namely, 85 g of nonpareils (20 to 28 meshes) was placed in a mini CF device (Freund), and coated with the powder having the following composition by sprinkling at a rat~ of 5 g/min at a rotational speed of a rotor of 400 rpm while spraying 50 ml of a 1% (w/v) hydroxypropyl cellulose (Content of hydroxy~ropoxyl group : 53.4 to 77.5 %~
solution at a rate of 2.5 ml/min. The resulting product was dried under vacuum at 40C for 16 hours, followed by sieving khrough a round sieve to obtain ~pherical granules having a particle size of 12 to 32 meshes.
[Powder]
Powder composition containing the rhbFGF
mutein CS23 obtained in Example 1 20 g Fine granulaked sugar 20 g Corn Starch 20 g Then, 60 g of the granules thus obtained was placed in a mini CF device ~Freund), and provided wikh an intestinally ~oluble coating by spraying the intestinally soluble filTn 2 [3 ~
solution having the following composition at a rate of 5 ml/min at a rotational speed of a rotor of 400 rpm, adjusting the air temperature to 40C and the granule temperature to 35C, to obtain intestinally soluble granules.
[Intestinally Soluble Film Solution]
Hydroxypropyl methyl cellulose phthalate 20 g Castor oil 2 g Tale 0.4g Acetone 200 ml Example 4 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to 2 g of L-HPC tLH-20, Shin-Etsu Chemical~, and the mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a powder composition. The remaining activity oE the resulting composition was 100%.
Example 5 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration oE 1 mg/ml was added to a mixtura of 1.6 g of L-HPC (LH-20, Shin-Etsu Chemical) and 0.4 g of powder sugar (pulverized sucrose) as a saccharide, and the resulting mixture was suff:iciently stirred, ollowad by drying at room temperature (about 20C) under reduced pressure (about 5 mm ~CJ ) :Eor 20 hours to obtain a powder composition. The composition thus obtained showed the following remaining activity immediately after preparation, after 2 months at 40C and after 6 months at 40C.
L-HPC + Sugar Powder Immediately after preparation 95 After 2 months at 40C 81~
After 6 months at 40C 81%
Example 6 -~ 1) 500 g of stearyl mono(tetra)glycerlde (MS-310, Sakamoto Yakuhin Co.) was added to 500 g of stearyl penta(tetra)glyceride (PS-310, Sakamoto Yakuhin Co.), and the mixture was heated at 90C to melt it. The resulting melt was dripped at a rate of 20 g/minute on an aluminum disk 15 cm in diameter rotating at 1lO00 rpm to prepare spherical fatty acid ester of polyglycerol granules which pass through a 32-mesh sieve, but does not pass through a 42-mesh sieve.
100 g of the spherical Eatty acid ester of polyglycerol granules obtained above, 5 g of the powder composition obtained in Example 4 and 95 y of L-HPC (LH-20, Shin-Etsu Chemical) were placed in a fluidized granulator (type FD 3S, Fuji Sangyo). Setting the supply air temperature to 54C, the mixture was heated and fluidized. A~ter it was confirmed that L-HPC particles floating in a fluidized bed had disappeared, the supply oE heat was stopped and the cooling was carried out, thereby obtaining yranules.
(2) 100 g o~ the granules of rhbFGF mutein CS23 obtained in the above item (1) was placed in the fluidized , 2~2~6~l~
granulator (type FD-3S, Fuji Sangyo), and coated with a coating solution [a solution of 100 g of hydroxypropyl methyl cellulose phthalate HP-55S (Shin-Etsu Chemical) in 1 litre of a 1:1 mixture of acetone and ethanol) at a solution supply rate of 2 g/minute at a supply air temperature of ~8C to obtain a coated granule composition containing rhbFGF mutein CS23.
Example 7 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to a mixture oE 1.6 g of L-HPC tLH-20, Shin-Etsu Chemical) and 0.4 g of human serum albumin (HSA), casein or purified gelatin as a protein, and the resulting mixture was ..
sufficiently stirred, ollowed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a respective powder compositions.
Example 8 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to a mixture of 1.6 g of L-HPC (LH-20, Shin-Etsu Chemical) and 0.~ g of sodium chloride, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) Eor 20 hours to obtain a powder compo5ition.
2S ~
2 ml of 50 mM sodlum citrate ~olution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml , :
;~ 'i 2 ~11 2 ~
was added to a mixture of 1.6 g of L-HPC ~LH-20, Shin-Etsu Chemical) and 0.4 g of L-cysteine as an amino acid, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) ~or 20 hours to obtain a powder composition.
Example 10 -~
2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml 10 was added to a mixture of 1.2 g of L-HPC (LH-20, Shin-Etsu ::
Chemical), 0.4 g of L-cysteine and 0.4 g of sodium chloride, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a powder composition.
Exam~le 11 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to a mixture of 1~2 g of I,-HPC (LH-20, Shin-Etsu Chemical), 0.4 g of L-cysteine and 0.4 g of powder sugar, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reducecl pressure (about 5 mm ~Ig) for 20 hours to obtain a powder composition.
~ le 12 2 ml o~ 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml ::, . .
was added to a mixture of 1.6 g of L-HPC (LH-20, Shin-Etsu Chemical) and 0.4 g of gum arabic, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a powder composition.
`:
Experimental Example-~l Sodium dextran sulfate having an average molecular weight of 7,500 was added to a 50 mM sodium citrate solution (pH 8.0) containing rhbFGF mutein CS23 in a concentration of 200 ~g/ml so as to give a concentration of 93.2 ~g/ml.
Then, 1 ml portions of the resulting solution were added to 1 g of L-HPC~ ~L~-20) and to 1 g of hydroxypropyl cellulose ~hydroxypropoxyl group : 61 %), respectively.
The resulting solution was stirred sufficiently. The mixtures thus obtained were dried at room temperature for 20 hours under reduced pressure (about 20C, about 5 mmHg) to give powder compositions containing rhbFGF mutein CS23 and L-HPC, and rhbFGF mutein CS23 and hydroxypropyl cellulose, respectivelyc The remaining activity of these compositions is shown in Table 4.
Table 4 _ _Additive _ _ _ Remaininq ~GF Actlvity (%) 25 Hydroxypropyl cellul se 44
Table 3 Additive _Remaining FGF Activity (%) Lactose ll Example 3 -Using the powder composition containing rhbFGF mutein CS23 and L-HPC obtained in Example l, granules were prepared by the following method.
Namely, 85 g of nonpareils (20 to 28 meshes) was placed in a mini CF device (Freund), and coated with the powder having the following composition by sprinkling at a rat~ of 5 g/min at a rotational speed of a rotor of 400 rpm while spraying 50 ml of a 1% (w/v) hydroxypropyl cellulose (Content of hydroxy~ropoxyl group : 53.4 to 77.5 %~
solution at a rate of 2.5 ml/min. The resulting product was dried under vacuum at 40C for 16 hours, followed by sieving khrough a round sieve to obtain ~pherical granules having a particle size of 12 to 32 meshes.
[Powder]
Powder composition containing the rhbFGF
mutein CS23 obtained in Example 1 20 g Fine granulaked sugar 20 g Corn Starch 20 g Then, 60 g of the granules thus obtained was placed in a mini CF device ~Freund), and provided wikh an intestinally ~oluble coating by spraying the intestinally soluble filTn 2 [3 ~
solution having the following composition at a rate of 5 ml/min at a rotational speed of a rotor of 400 rpm, adjusting the air temperature to 40C and the granule temperature to 35C, to obtain intestinally soluble granules.
[Intestinally Soluble Film Solution]
Hydroxypropyl methyl cellulose phthalate 20 g Castor oil 2 g Tale 0.4g Acetone 200 ml Example 4 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to 2 g of L-HPC tLH-20, Shin-Etsu Chemical~, and the mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a powder composition. The remaining activity oE the resulting composition was 100%.
Example 5 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration oE 1 mg/ml was added to a mixtura of 1.6 g of L-HPC (LH-20, Shin-Etsu Chemical) and 0.4 g of powder sugar (pulverized sucrose) as a saccharide, and the resulting mixture was suff:iciently stirred, ollowad by drying at room temperature (about 20C) under reduced pressure (about 5 mm ~CJ ) :Eor 20 hours to obtain a powder composition. The composition thus obtained showed the following remaining activity immediately after preparation, after 2 months at 40C and after 6 months at 40C.
L-HPC + Sugar Powder Immediately after preparation 95 After 2 months at 40C 81~
After 6 months at 40C 81%
Example 6 -~ 1) 500 g of stearyl mono(tetra)glycerlde (MS-310, Sakamoto Yakuhin Co.) was added to 500 g of stearyl penta(tetra)glyceride (PS-310, Sakamoto Yakuhin Co.), and the mixture was heated at 90C to melt it. The resulting melt was dripped at a rate of 20 g/minute on an aluminum disk 15 cm in diameter rotating at 1lO00 rpm to prepare spherical fatty acid ester of polyglycerol granules which pass through a 32-mesh sieve, but does not pass through a 42-mesh sieve.
100 g of the spherical Eatty acid ester of polyglycerol granules obtained above, 5 g of the powder composition obtained in Example 4 and 95 y of L-HPC (LH-20, Shin-Etsu Chemical) were placed in a fluidized granulator (type FD 3S, Fuji Sangyo). Setting the supply air temperature to 54C, the mixture was heated and fluidized. A~ter it was confirmed that L-HPC particles floating in a fluidized bed had disappeared, the supply oE heat was stopped and the cooling was carried out, thereby obtaining yranules.
(2) 100 g o~ the granules of rhbFGF mutein CS23 obtained in the above item (1) was placed in the fluidized , 2~2~6~l~
granulator (type FD-3S, Fuji Sangyo), and coated with a coating solution [a solution of 100 g of hydroxypropyl methyl cellulose phthalate HP-55S (Shin-Etsu Chemical) in 1 litre of a 1:1 mixture of acetone and ethanol) at a solution supply rate of 2 g/minute at a supply air temperature of ~8C to obtain a coated granule composition containing rhbFGF mutein CS23.
Example 7 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to a mixture oE 1.6 g of L-HPC tLH-20, Shin-Etsu Chemical) and 0.4 g of human serum albumin (HSA), casein or purified gelatin as a protein, and the resulting mixture was ..
sufficiently stirred, ollowed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a respective powder compositions.
Example 8 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to a mixture of 1.6 g of L-HPC (LH-20, Shin-Etsu Chemical) and 0.~ g of sodium chloride, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) Eor 20 hours to obtain a powder compo5ition.
2S ~
2 ml of 50 mM sodlum citrate ~olution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml , :
;~ 'i 2 ~11 2 ~
was added to a mixture of 1.6 g of L-HPC ~LH-20, Shin-Etsu Chemical) and 0.4 g of L-cysteine as an amino acid, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) ~or 20 hours to obtain a powder composition.
Example 10 -~
2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml 10 was added to a mixture of 1.2 g of L-HPC (LH-20, Shin-Etsu ::
Chemical), 0.4 g of L-cysteine and 0.4 g of sodium chloride, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a powder composition.
Exam~le 11 2 ml of 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml was added to a mixture of 1~2 g of I,-HPC (LH-20, Shin-Etsu Chemical), 0.4 g of L-cysteine and 0.4 g of powder sugar, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reducecl pressure (about 5 mm ~Ig) for 20 hours to obtain a powder composition.
~ le 12 2 ml o~ 50 mM sodium citrate solution (pH 7.0) containing rhbFGF mutein CS23 at a concentration of 1 mg/ml ::, . .
was added to a mixture of 1.6 g of L-HPC (LH-20, Shin-Etsu Chemical) and 0.4 g of gum arabic, and the resulting mixture was sufficiently stirred, followed by drying at room temperature (about 20C) under reduced pressure (about 5 mm Hg) for 20 hours to obtain a powder composition.
`:
Experimental Example-~l Sodium dextran sulfate having an average molecular weight of 7,500 was added to a 50 mM sodium citrate solution (pH 8.0) containing rhbFGF mutein CS23 in a concentration of 200 ~g/ml so as to give a concentration of 93.2 ~g/ml.
Then, 1 ml portions of the resulting solution were added to 1 g of L-HPC~ ~L~-20) and to 1 g of hydroxypropyl cellulose ~hydroxypropoxyl group : 61 %), respectively.
The resulting solution was stirred sufficiently. The mixtures thus obtained were dried at room temperature for 20 hours under reduced pressure (about 20C, about 5 mmHg) to give powder compositions containing rhbFGF mutein CS23 and L-HPC, and rhbFGF mutein CS23 and hydroxypropyl cellulose, respectivelyc The remaining activity of these compositions is shown in Table 4.
Table 4 _ _Additive _ _ _ Remaininq ~GF Actlvity (%) 25 Hydroxypropyl cellul se 44
Claims (29)
1. A stabilized FGF protein composition which comprises an FGF protein and water-insoluble hydroxypropyl cellulose.
2. A composition in accordance with claim 1, wherein the water-insoluble hydroxypropyl cellulose is low-substituted hydroxypropyl cellulose.
3. A composition in accordance with claim 2, in which the low-substituted hydroxypropyl cellulose contains not less than 5.0% and not more than 16.0% of hydroxypropoxyl group.
4. A composition in accordance with claim 1, wherein the FGF protein is an FGF mutein.
5. A composition in accordance with claim 4, wherein the FGF protein is a mutein at least one human basic FGF-constituent amino acid of which is substituted by at least one different amino acid.
6. A composition in accordance with claim 1, which is further coated by an enteric polymer.
7. A method for preparing a stabilized FGF protein composition, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose.
8. A method in accordance with claim 7, wherein the water-insoluble hydroxypropyl cellulose is low-substituted hydroxypropyl cellulose.
9. A method in accordance with claim 8, wherein the low-substituted hydroxypropyl cellulose contains not less than 5.0% and not more than 16.0% of hydroxypropoxyl group.
10. A method in accordance with claim 7, wherein the FGF protein is an FGF mutein.
11. A method in accordance with claim 10, wherein the FGF protein is a mutein at least one human basic FGF-constituent amino acid of which is substituted by at least one different amino acid.
12. A method in accordance with claim 7, which comprises further coating the composition by an enteric polymer.
13. A method for stabilizing an FGF protein, which comprises admixing an FGF protein with a water-insoluble hydroxypropyl cellulose.
14. A method in accordance with claim 13, wherein the water-insoluble hydroxypropyl cellulose is low-substituted hydroxypropyl cellulose.
15. A method in accordance with claim 14, wherein the low-substituted hydroxypropyl cellulose contains not less than 5.0% and not more than 16.0% of hydroxypropoxyl group.
16. A method in accordance with claim 13, wherein the FGF protein is an FGF mutein.
17. A method in accordance with claim 16, wherein the FGF protein is a mutein at least one human basic FGF-constituent amino acid of which is substituted by at least one different amino acid.
18. A method in accordance with claim 13, which comprises further coating the composition by an enteric polymer.
19. A dry powdery pharmaceutical composition which comprises:
an FGF protein in an amount sufficient to promote growth of fibroblasts; and a water-insoluble hydroxypropyl cellulose having a degree of substitution of hydroxypropyl group of 5 to 16%;
wherein the amount of the water-insoluble hydroxyl cellulose is such that a weight ratio of the FGF protein: the water-insoluble hydroxypropyl cellulose is within the range from 1:0.01 to 1.1,000,000 and that the stability of the FGF protein is increased.
an FGF protein in an amount sufficient to promote growth of fibroblasts; and a water-insoluble hydroxypropyl cellulose having a degree of substitution of hydroxypropyl group of 5 to 16%;
wherein the amount of the water-insoluble hydroxyl cellulose is such that a weight ratio of the FGF protein: the water-insoluble hydroxypropyl cellulose is within the range from 1:0.01 to 1.1,000,000 and that the stability of the FGF protein is increased.
20. A composition in accordance with claim 19, in which the FGF protein: the water-insoluble hydroxypropyl cellulose weight ratio is from 1:1 to 1:100,000.
21. A composition in accordance with claim 19, in which the FGF protein: the water-insoluble hydroxypropyl cellulose weight ratio is from 1:500 to 1:20,000.
22. A composition in accordance with claim 20, which fur-ther comprises:
at least one member selected from the group consisting of sugars, proteins, amino acids, sodium chloride and gum arabic in a weight ratio of the FGF protein: the said member of from 1:1 to 100,000.
at least one member selected from the group consisting of sugars, proteins, amino acids, sodium chloride and gum arabic in a weight ratio of the FGF protein: the said member of from 1:1 to 100,000.
23. A composition in accordance with claim 20, which further comprises:
a glucan sulfate having a sulfur content of 3 to 20%
by weight.
a glucan sulfate having a sulfur content of 3 to 20%
by weight.
24. A composition in accordance with claim 20, wherein the FGF protein is a recombinant human basic FGF or a mutein thereof.
25. A pharmaceutical dry granulated composition comprising granules of a C12-C22 fatty acid ester of a polyglycerol having a melting point of about 40 to 80°C and the powdery dry composition of any one of claims 19 to 24 attached to the granules.
26. An enteric pharmaceutical composition which comprises the powdery dry composition of any one of claims 19 to 24 as it is or granules, fine grains or tablets made therefrom coated with an enteric polymer.
27. A process for producing a powdery dry composition of an FGF protein of increased stability, which comprises:
admixing an aqueous solution of the FGF protein having a pH value of about 3 to 10 with a water-insoluble hydroxy-propyl cellulose in powder form at a temperature of 10 to 30°C, wherein the water-insoluble hydroxypropyl cellulose has a degree of substitution of hydroxypropyl group of 5 to 16% and is used in such an amount that a weight ratio of the FGF protein: the water-insoluble hydroxypropyl cellulose is within the range from 1:0.01 to 1:1,000,000 and that the stability of the FGF protein in the powdery dry composition is increased; and drying or lyophilizing the resulting mixture at a temperature not more than 30°C under reduced pressure.
admixing an aqueous solution of the FGF protein having a pH value of about 3 to 10 with a water-insoluble hydroxy-propyl cellulose in powder form at a temperature of 10 to 30°C, wherein the water-insoluble hydroxypropyl cellulose has a degree of substitution of hydroxypropyl group of 5 to 16% and is used in such an amount that a weight ratio of the FGF protein: the water-insoluble hydroxypropyl cellulose is within the range from 1:0.01 to 1:1,000,000 and that the stability of the FGF protein in the powdery dry composition is increased; and drying or lyophilizing the resulting mixture at a temperature not more than 30°C under reduced pressure.
28. A process in accordance with claim 27, wherein:
the aqueous solution of the FGF protein further con-tains a glucan sulfate or a pharmaceutically acceptable salt thereof having a sulfur content of 3 to 20% by weight in an amount of 0.1 to 100 mol per mol of the FGF protein.
the aqueous solution of the FGF protein further con-tains a glucan sulfate or a pharmaceutically acceptable salt thereof having a sulfur content of 3 to 20% by weight in an amount of 0.1 to 100 mol per mol of the FGF protein.
29. A process in accordance with claim 28 wherein:
the aqueous solution of the FGF protein further con-tains a dibasic or tribasic carboxylic acid or a pharmaceutically acceptable salt thereof in a concentration of from 1 mM to 1M.
the aqueous solution of the FGF protein further con-tains a dibasic or tribasic carboxylic acid or a pharmaceutically acceptable salt thereof in a concentration of from 1 mM to 1M.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP17622889 | 1989-07-07 | ||
| JP176228/1989 | 1989-07-07 | ||
| JP13633390 | 1990-05-24 | ||
| JP136333/1990 | 1990-05-24 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2020654A1 true CA2020654A1 (en) | 1991-01-08 |
Family
ID=26469955
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002020654A Abandoned CA2020654A1 (en) | 1989-07-07 | 1990-06-06 | Stabilized fgf composition and production thereof |
Country Status (14)
| Country | Link |
|---|---|
| US (1) | US5189148A (en) |
| EP (1) | EP0406856B1 (en) |
| JP (1) | JP2536247B2 (en) |
| CN (1) | CN1049106A (en) |
| AT (1) | ATE102044T1 (en) |
| AU (1) | AU632344B2 (en) |
| CA (1) | CA2020654A1 (en) |
| DE (1) | DE69006947T2 (en) |
| DK (1) | DK0406856T3 (en) |
| ES (1) | ES2062206T3 (en) |
| FI (1) | FI903440A0 (en) |
| HU (1) | HU205862B (en) |
| IE (1) | IE902470A1 (en) |
| NO (1) | NO902995L (en) |
Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US6174529B1 (en) | 1991-06-21 | 2001-01-16 | University Of Cincinnati | Oral therapy for the treatment of allergies and method of manufacture |
| US6613332B1 (en) | 1991-06-21 | 2003-09-02 | The University Of Cincinnati | Oral administration of therapeutic proteins |
Families Citing this family (48)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5763394A (en) * | 1988-04-15 | 1998-06-09 | Genentech, Inc. | Human growth hormone aqueous formulation |
| US5981485A (en) | 1997-07-14 | 1999-11-09 | Genentech, Inc. | Human growth hormone aqueous formulation |
| US5202311A (en) * | 1988-08-19 | 1993-04-13 | Children's Medical Center Corporation | Stabilized fgf composition |
| GB9015824D0 (en) * | 1990-07-18 | 1990-09-05 | Erba Carlo Spa | Stable pharmaceutical compositions containing a fibroblast growth factor |
| US5714458A (en) * | 1990-07-18 | 1998-02-03 | Farmitalia Carlo Erba S.R.L. | Stable pharmaceutical compositions containing a fibroblast growth factor |
| US5500409A (en) * | 1990-10-01 | 1996-03-19 | Thomas Jefferson University | Method for inhibiting collagen synthesis by keloid fibroblasts |
| TW209174B (en) * | 1991-04-19 | 1993-07-11 | Takeda Pharm Industry Co Ltd | |
| DE4121043A1 (en) * | 1991-06-26 | 1993-01-07 | Merck Patent Gmbh | BONE REPLACEMENT MATERIAL WITH FGF |
| CA2080538A1 (en) * | 1991-10-21 | 1993-04-22 | Joseph V. Bondi | Lyophilized acidic fibroblast growth factor |
| CA2080537A1 (en) * | 1991-10-21 | 1993-04-22 | David B. Volkin | Stabilized topical acidic fibroblast growth factor formulation |
| US5580578A (en) * | 1992-01-27 | 1996-12-03 | Euro-Celtique, S.A. | Controlled release formulations coated with aqueous dispersions of acrylic polymers |
| US5482929A (en) * | 1991-12-26 | 1996-01-09 | Kaken Pharmaceutical Co., Ltd. | Composition of stabilized fibroblast growth factor |
| US7070806B2 (en) * | 1992-01-27 | 2006-07-04 | Purdue Pharma Lp | Controlled release formulations coated with aqueous dispersions of acrylic polymers |
| US5348941A (en) * | 1992-04-01 | 1994-09-20 | Merck & Co., Inc. | Stabilizers for fibroblast growth factors |
| SE9201073D0 (en) * | 1992-04-03 | 1992-04-03 | Kabi Pharmacia Ab | PROTEIN FORMULATION |
| DE4242889A1 (en) * | 1992-12-18 | 1994-06-23 | Merck Patent Gmbh | Hollow endoprostheses with filling that promotes bone growth |
| JP3349535B2 (en) * | 1993-01-12 | 2002-11-25 | フロイント産業株式会社 | Method for producing spherical granules |
| US5331095A (en) * | 1993-04-12 | 1994-07-19 | Scios Nova Inc. | Process for purification of basic fibroblast growth factor |
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Family Cites Families (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| NZ222413A (en) * | 1986-11-05 | 1991-06-25 | Ethicon Inc | Compositions containing a polypeptide growth factor and a water-soluble cellulose polymer stabiliser |
| US4717717A (en) * | 1986-11-05 | 1988-01-05 | Ethicon, Inc. | Stabilized compositions containing epidermal growth factor |
| JP2526965B2 (en) * | 1987-02-24 | 1996-08-21 | 武田薬品工業株式会社 | Muteins, DNAs and their uses |
| NZ226171A (en) * | 1987-09-18 | 1990-06-26 | Ethicon Inc | Gel formulation containing polypeptide growth factor |
| NZ226170A (en) * | 1987-09-18 | 1990-07-26 | Ethicon Inc | Stable freeze-dried pharmaceutical composition containing epidermal growth factor |
-
1990
- 1990-06-06 CA CA002020654A patent/CA2020654A1/en not_active Abandoned
- 1990-07-03 US US07/547,454 patent/US5189148A/en not_active Expired - Fee Related
- 1990-07-04 NO NO90902995A patent/NO902995L/en unknown
- 1990-07-05 JP JP2178917A patent/JP2536247B2/en not_active Expired - Lifetime
- 1990-07-05 EP EP90112850A patent/EP0406856B1/en not_active Expired - Lifetime
- 1990-07-05 DK DK90112850.4T patent/DK0406856T3/en active
- 1990-07-05 AT AT90112850T patent/ATE102044T1/en not_active IP Right Cessation
- 1990-07-05 ES ES90112850T patent/ES2062206T3/en not_active Expired - Lifetime
- 1990-07-05 DE DE69006947T patent/DE69006947T2/en not_active Expired - Fee Related
- 1990-07-06 IE IE247090A patent/IE902470A1/en unknown
- 1990-07-06 AU AU58799/90A patent/AU632344B2/en not_active Ceased
- 1990-07-06 HU HU904116A patent/HU205862B/en not_active IP Right Cessation
- 1990-07-06 FI FI903440A patent/FI903440A0/en not_active IP Right Cessation
- 1990-07-06 CN CN90103391A patent/CN1049106A/en active Pending
Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US6174529B1 (en) | 1991-06-21 | 2001-01-16 | University Of Cincinnati | Oral therapy for the treatment of allergies and method of manufacture |
| US6613332B1 (en) | 1991-06-21 | 2003-09-02 | The University Of Cincinnati | Oral administration of therapeutic proteins |
Also Published As
| Publication number | Publication date |
|---|---|
| DE69006947D1 (en) | 1994-04-07 |
| NO902995D0 (en) | 1990-07-04 |
| JP2536247B2 (en) | 1996-09-18 |
| HU205862B (en) | 1992-07-28 |
| HU904116D0 (en) | 1990-12-28 |
| HUT54895A (en) | 1991-04-29 |
| DK0406856T3 (en) | 1994-07-04 |
| EP0406856A3 (en) | 1991-04-10 |
| FI903440A0 (en) | 1990-07-06 |
| EP0406856B1 (en) | 1994-03-02 |
| ATE102044T1 (en) | 1994-03-15 |
| AU5879990A (en) | 1991-01-10 |
| DE69006947T2 (en) | 1994-08-25 |
| AU632344B2 (en) | 1992-12-24 |
| US5189148A (en) | 1993-02-23 |
| EP0406856A2 (en) | 1991-01-09 |
| IE902470A1 (en) | 1991-02-13 |
| JPH04128239A (en) | 1992-04-28 |
| ES2062206T3 (en) | 1994-12-16 |
| CN1049106A (en) | 1991-02-13 |
| NO902995L (en) | 1991-01-08 |
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Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| FZDE | Discontinued |