Title of Invention

A METHOD FOR PREVENTING COLORATION OF A FREEZE-DRY COMPOSITION

Abstract "A METHOD FOR PREVENTING COLORATION OF A FREEZE-DRY COMPOSITION" A method for preventing coloration of a freeze-dry composition containing a saccharide and a pharmacologically active proteinaceous substance, said method comprising adding hydrophobic amino acid having a hydropathy index of not less that 3.8 to a solution containing a saccharide and a pharmacologically active proteinaceous substance, wherein said hydrophobic amino acid is added in a total amount of from 0.1 parts by weight to 200 parts by weight per 100 parts by weight of said saccharide, and freeze-drying the solution to obtain said freeze-dry composition, thereby, preventing coloration of said freeze-dry composition.
Full Text FORM 2
THE PATENTS ACT 1970
[39 OF 1970]
8B
THE PATENTS RULES, 2003
as amended by
THE PATENTS (AMENDMENT) RULES, 2006
COMPLETE SPECIFICATION
[See Section 10; rule 13]
"A METHOD FOR PREVENTING COLORATION OF A FREEZE-DRY COMPOSITION"
OTSUKA PHARMACEUTICAL CO., LTD., a Japanese company of 9 Kandatsukasa-cho 2-chome, Chiyoda-ku, Tokyo 101-8535, Japan
The following specification particularly describes the invention and the manner in which it is to be performed:

The present invention relates to a method for preventing coloration of a freeze-dry composition.
TECHNICAL FIELD
The present invention relates to a method for reducing and/or preventing coloration caused by a combined use of saccharide and amino acid. Specifically, the invention provides, as an amino acid usable with a saccharide, an amino acid having an anti-coloring effect when combined with a saccharide. The invention also provides a method for preventing coloration achieved by using the amino acid.
The invention further relates to a method for stabilizing a dry composition containing a pharmacologically active proteinaceous substance. Specifically, the invention relates to a dry composition containing a pharmacologically active proteinaceous substance to which a saccharide and an amino acid are added.
BACKGROUND ART
Pharmaceutical compositions, particularly in dry compositions containing a pharmacologically active proteinaceous substance as an active ingredient, sucrose, glucose, fructose, maltose and like saccharides (Japanese

Unexamined Patent Publications Nos. 1983-92619, 1985-48933 and 1990-138222, etc.), glycine, alanine and like amino acids (Japanese Unexamined Patent Publications No. 1983 — 146504) have generally been used as stabilizers effective on the active ingredient.
However, it is generally known that when these saccharides, which are used as stabilizers for pharmacologically active proteinaceous substances, are used with an amino acid, coloration caused by the Maillard reaction, etc. results. Therefore, pharmaceutical compositions containing a saccharide and an amino acid have the drawback of coloration with the passage of time.
An object of the present invention is to provide an amino acid having an anti-coloring effect for reducing and/or preventing coloration caused by the combined use of saccharide and amino acid. Specifically, the invention provides an anti-coloring agent containing the amino acid as an essential ingredient suitable for preventing the coloration caused by the change with the passage of time of a dry composition containing a saccharide, and a method for preventing coloration where the amino acid is used.
Another object of the invention is to provide an amino acid useable as a stabilizer for a dry composition containing a saccharide, particularly, a proteinaceous dry composition containing a saccharide. More specifically,

the invention provides a dry composition containing a saccharide and the amino acid.
DISCLOSURE OF THE INVENTION
The inventor has conducted extensive research to achieve the above objects. Consequently, the inventor has found that, in dry compositions containing a saccharide, specifically, dry compositions containing a saccharide and a pharmacologically active proteinaceous substance, use of specific amino acid enables the significant reduction and/or prevention of coloration attributable to saccharide. He has also found that dry compositions containing a saccharide as a stabilizer, even dry compositions containing a pharmacologically active proteinaceous substance, can further be improved in stability by adding the specific amino acid. The invention has been accomplished based on the above findings.
In other words, the invention firstly relates to use of a hydrophobic amino acid preventing the coloration caused by the combined use of saccharide and amino acid, specifically, the following embodiments are included. 1. Anti-coloring agent
Item 1. An anti-coloring agent comprising a hydrophobic amino acid as an essential ingredient suitably preventing coloration of a dry composition containing a

saccharide.
Item 2. The anti-coloring agent according to item 1, wherein the hydrophobic amino acid has a hydropathy index of not less than 2.
Item 3. The anti-coloring agent according to item 1, wherein the hydrophobic amino acid has a hydropathy index of not less than 3.8.
Item 4. The anti-coloring agent according to item 1, wherein the hydrophobic amino acid has a hydropathy index in the range of from 3.8 to 4.5.
Item 5. The anti-coloring agent according to item 1, wherein the hydrophobic amino acid is at least one member selected from the group consisting of valine, leucine, isoleucine and phenylalanine.
Item 6. The anti-coloring agent according to item 1, wherein the hydrophobic amino acid content is in the range of from 0.1 part by weight to 200 parts by weight per 100 parts by weight of saccharide contained in the dry composition.
Item 7. The anti-coloring agent according to item 1, wherein the saccharide is at least one member selected from the group consisting of reducing sugars, sucrose, trehalose, mannitol and dextran 40.
Item 8. The anti-coloring agent according to item 1, wherein the hydrophobic amino acid is used in such

a manner that its concentration becomes in the range of from 0.1 wt.% to 70 wt.% per 100 wt.% of the total weight of the dry composition.
Item 9. The anti-coloring agent according to item 1, wherein the dry composition is a freeze-dried composition comprising a pharmacologically active proteinaceous substance as an active ingredient.
Item 10. The anti-coloring agent according to item 1, wherein the pharmacologically active proteinaceous substance is at least one member selected from the group consisting of antiviral polypeptides, immunomodulator polypeptides and hematinic polypeptides.
Item 11. The anti-coloring agent according to item 1, wherein the pharmacologically active proteinaceous substance is interferon. 2. Method for preventing coloration
Item 12. A method for preventing coloration of a dry composition containing a saccharide comprising adding a hydrophobic amino acid to the dry composition containing a saccharide.
Item 13. The method for preventing coloration according to item 12, wherein the hydrophobic amino acid has a hydropathy index of not less than 2.
Item 14. The method for preventing coloration according to item 12, wherein the hydrophobic amino acid

has a hydropathy index of not less than 3.8.
Item 15. The method for preventing coloration according to item 12, wherein the hydrophobic amino acid has a hydropathy index in the range of from 3.8 to 4.5.
Item 16. The method for preventing coloration according to item 12, wherein the hydrophobic amino acid is at least one member selected from the group consisting of valine, leucine, isoleucine and phenylalanine.
Item 17. The method for preventing coloration according to item 12, wherein the hydrophobic amino acid is used in such a manner that its concentration becomes in the range of from 0.1 part by weight to 200 parts by weight per 100 parts by weight of saccharide contained in the dry composition.
Item 18. The method for preventing coloration according to item 12, wherein the saccharide is at least one member selected from the group consisting of reducing sugars, sucrose, trehalose, mannitol and dextran 40.
Item 19. The method for preventing coloration according to item 12, wherein the hydrophobic amino acid is used in such a manner that its concentration becomes in the range of from 0.1 wt.% to 70 wt.% per 100 wt.% of the total weight of the dry composition.
Item 20. The method for preventing coloration according to item 12, wherein the dry composition is a

freeze-dried composition comprising a pharmacologically active proteinaceous substance as an active ingredient.
Item 21. The method for preventing coloration according to item 20, wherein the pharmacologically active proteinaceous substance is at least one member selected from the group consisting of antiviral polypeptides, immunomodulator polypeptides and hematinic polypeptides.
Item 22. The method for preventing coloration according to item 12, wherein the pharmacologically active proteinaceous substance is interferon. 3. Use of hydrophobic amino acid
Item 23. Use of a hydrophobic amino acid for preventing coloration of a dry composition containing a saccharide.
Item 24. The use of a hydrophobic amino acid according to item 23, wherein the hydrophobic amino acid has a hydropathy index of not less than 2.
Item 25. The use of a hydrophobic amino acid according to item 23, wherein the hydrophobic amino acid has a hydropathy index of not less than 3.8.
Item 26. The use of a hydrophobic amino acid according to item 23, wherein the hydrophobic amino acid has a hydropathy index in the range of from 3.8 to 4.5.
Item 27. The use of a hydrophobic amino acid according to item 23, wherein the hydrophobic amino acid

is at least one member selected from the group consisting of valine, leucine, isoleucine and phenylalanine.
Item 28 . The use of a hydrophobic amino acid according to item 23, wherein the concentration of the hydrophobic amino acid is in the range of from 0.1 part by weight to 200 parts by weight per 100 parts by weight of saccharide contained in the dry composition.
Item 29. The use of a hydrophobic amino acid according to item 23, wherein the saccharide is at least one member selected from the group consisting of reducing sugars, sucrose, trehalose, mannitol and dextran 40.
Item 30 . The use of a hydrophobic amino acid according to item 23, wherein the concentration of the hydrophobic amino acid is in the range of from 0.1 wt.% to 70 wt.% per 100 wt.% of the total weight of the dry composition.
Item 31 . The use of a hydrophobic amino acid according to item 23, wherein the dry composition is a freeze-dried composition containing a pharmacologically active proteinaceous substance as an active ingredient.
Item 32. The use of a hydrophobic amino acid according to item 23, wherein the pharmacologically active proteinaceous substance is at least one member selected from the group consisting of antiviral polypeptides, immunomodulator polypeptides and hematinic polypeptides.

Item 33. The use of a hydrophobic amino acid according to item 23, wherein the pharmacologically active proteinaceous substance is interferon.
The present invention can effectively reduce or prevent the coloration caused by the change with the passage of time of dry compositions containing a saccharide, especially compositions containing a saccharide and a pharmacologically active proteinaceous substance. Thereby, it can provide dry compositions excellent in stability.
Secondly, the invention relates to dry compositions containing a pharmacologically active proteinaceous substance in a stable manner including the prevention of coloring. 4. Dry compositions
Item 34. A dry composition containing a pharmacologically active proteinaceous substance whereto a saccharide and a hydrophobic amino acid are added as a stabilizer.
Item 35. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the hydrophobic amino acid has a hydropathy index of not less than 2.
Item 36. The dry composition containing a pharmacologically active proteinaceous substance according

to item 34, wherein the hydrophobic amino acid has a hydropathy index of not less than 3.8.
Item 37. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the hydrophobic amino acid has a hydropathy index in the range of from 3.8 to 4.5.
Item 38. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the hydrophobic amino acid is at least one member selected from the group consisting of valine, leucine, isoleucine and phenylalanine.
Item 39. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the concentration of the hydrophobic amino acid is in the range of from 0.1 part by weight to 200 parts by weight per 100 parts by weight of saccharide contained in the dry composition.
Item 40. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the saccharide is at least one member selected from the group consisting of reducing sugars, sucrose, trehalose, mannitol and dextran 40.
Item 41. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the concentration of the hydrophobic

amino acid is in the range of from 0.1 wt.% to 70 wt.% per 100 wt.% of the total weight of the dry composition.
Item 42. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, which is a freeze-dried composition.
Item 43. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the pharmacologically active proteinaceous substance is at least one member selected from the group consisting of antiviral polypeptides, immunomodulator polypeptides and hematinic polypeptides.
Item 44. The dry composition containing a pharmacologically active proteinaceous substance according to item 34, wherein the pharmacologically active proteinaceous substance is interferon.
The present invention can provide, by combining a saccharide with a hydrophobic amino acid, dry compositions containing a pharmacologically active proteinaceous substance as an active ingredient in a stable condition even after completion of drying (freeze-drying, etc.) and during storage.
BEST MODE FOR CARRYING OUT THE INVENTION The anti-coloring agent of the invention comprises a hydrophobic amino acid as an essential

ingredient. The anti-coloring agent of the invention significantly prevents coloration with the passage of time, especially when used with a dry composition containing a saccharide.
The hydrophobic amino acids to be used in the invention are those having a hydropathy index of about 2 or larger (Jack Kyte and Russel F. Doolittel, "A Simple Method for Displaying the Hydropathic Character of a Protein." J. Mol. Biol. 157(1982): 105-132). Any amino acids having the above property may be used in the invention whether or not they are protein-constituting amino acids. The hydrophobic amino acids may preferably be those having a hydropathy index of about 2.8 or larger such as valine, leucine, isoleucine and phenylalanin; more preferably those having a hydropathy index of about 3.8 or larger; and even more preferably those having a hydropathy index in the range of from about 3.8 to about 4.5 such as valine, leucine and isoleucine.
The hydrophobic amino acids to be used in the invention may be in the form of dipeptides, tripeptides, salts or amides. Examples of the dipeptides of hydrophobic amino acids are leucyl-valine, isoleucyl-valine, isoleucyl-leucine, leucyl-glycine, etc. Examples of the tripeptides of hydrophobic amino acids are isoleucyl-leucyl-valine, leucyl-glicyl-glycine, etc. The

salts of hydrophobic amino acids include salts thereof with sodium, potassium and like alkali metals or with calcium, magnesium and like alkaline earth metals; adduct salts thereof with phosphoric acid, hydrochloric acid, hydrobromic acid and like inorganic acids or with organic acids such as a sulfonic acid, etc. More specific examples of the salts of hydrophobic amino acids are an L-leucic amide hydrochloride, L-isoleucyl-β-naphthylamide hydrobromide, L-valine-β-naphthylamide, etc.
These hydrophobic amino acids (including those in a form of a salt or amide) may be used singularly or in an arbitrary combination.
The anti-coloring agent of the invention targets saccharides generally known to cause coloration with the passage of time due to the Maillard reaction and the like when combined with amino acid. Specifically, the targeted saccharides include those generally used as stabilizers for dry pharmaceutical compositions, particularly pharmaceutical compositions containing a pharmacologically active proteinaceous substance. More specifically, glucose, fructose, maltose and like reducing sugars; sucrose, trehalose, mannitol, dextran 40 and the like are included. These saccharides can be added to a dry composition singularly or in an arbitrary combination. Among those preferable are sucrose and maltose.

The saccharide content of the dry composition varies depending on the kind of saccharide contained and cannot be generalized. However, a general amount of the saccharide used is 10 wt.% to 90 wt.%, in some cases 20 Wt.% to 80 wt.% and in other cases 40 wt.% to 80 wt.% per 100 wt.% of the dry composition. The above proportion is suitably applied when the saccharide used is sucrose.
Content of the hydrophobic amino acid in the dry composition varies depending on the kind of saccharide contained in the dry composition and cannot be generalized. However, per 100 wt.% of the dry composition, the hydrophobic amino acid can be contained generally about 0.1 wt.% to about 70 wt.%, preferably about 0.25 wt.% to about 60 wt.%, more preferably about 0.5 wt.% to about 50 wt.%, and even more preferably about 1 wt.% to about 50
Wt . "o .
There is no limitation on the ratio of the hydrophobic amino acid to the saccharide contained in the dry composition. However, the amount of amino acid used is generally about 0.1 part by weight to about 200 parts by weight, preferably about 0.2 part by weight to about 100 parts by weight and more preferably about 1 part by weight to about 100 parts by weight per 100 parts by weight of the saccharide contained in the dry composition.
Dry compositions in which the anti-coloring

agents of the invention are usable include compositions containing a pharmacologically active proteinaceous substance as an active ingredient.
There is no limitation on the pharmacologically active proteinaceous substances to be used as long as they are pharmacologically effective proteins or peptides (including polypeptides). Examples thereof are enzymes, hemoglobin, immunoglobulins, hormones, blood coagulation factors and like proteins, antiviral polypeptides (ex. interferons-α , -β , -γ , etc.), immunomodulator polypeptides (ex. interleukins-1, 2, 3, 4, 5, 6, 7, 8, etc.), hematinic polypeptides (ex. erythropoietin, granulocyte colony stimulating factor, macrophage-colony stimulating factor and granulocyte-macrophage-colony stimulating factor) and like polypeptides, etc. The proteins and peptides may be contained in the dry composition singularly or in an arbitrary combination. Among these, preferable are interferons.
The above proteins and peptides include those existing in nature, produced by recombinant DNA techniques or chemical syntheses.
There is no limitation on the proportion of the pharmacologically active proteinaceous substance to the dry composition. The amount of the pharmacologically active proteinaceous substance used varies depending on

the kind to be used; however, specific examples of the concentrations thereof are generally not more than 20 wt.%, in some cases 0.00001 wt.% to 10 wt.%, in some cases 0.0001 wt.% to 10 wt.%, in some cases 0.001 wt.% to 10 wt.% and in some cases 0.001 wt.% to 5 wt.%, per 100 wt.% of the dry composition.
The dry compositions in which the anti-coloring agents of the invention are used may further contain human serum albumin, a polar amino acid(s) or a salt(s) thereof (ex. an amino acid(s) having a hydropathy index of not larger than 0 or a salt thereof), an inorganic salt(s), gelatin, a surfactant(s) , a buffer(s), etc.
The usage of the anti-coloring agents of the invention is not limited as long as they are used in the above dry compositions. Preferably, they are added to a solution containing saccharide(s) and/or pharmacologically active proteinaceous substance(s) prior to the preparation of (i.e., before drying) the dry composition (dried product) or mixed into a solution together with saccharide(s) and/or pharmacologically active proteinaceous substance(s).
There is no limitation on the ratio of the anti-coloring agent to the dry composition. However, per 100 wt.% of the dry composition, hydrophobic amino acid is generally about 0. 1 wt.% to about 70 wt.%, preferably

about 0.25 wt. % to about 60 wt.%, more preferably about 0.5 wt.% to about 50 wt.%, and even more preferably about 1 wt.% to about 50 wt.%.
The content of hydrophobic amino acid per 100 parts by weight of saccharides contained in the dry composition is generally about 0.1 part by weight to about 200 parts by weight, preferably about 0.2 part by weight to about 100 parts by weight, and more preferably about 1 part by weight to about 100 parts by weight.
The invention relates to a method for preventing coloration of dry compositions containing a saccharide comprising use of hydrophobic amino acid. Specific examples of hydrophobic amino acids, saccharides, dry compositions and usage of hydrophobic amino acids are as described above.
Furthermore, the invention provides use of hydrophobic amino acid as a stabilizer. The hydrophobic amino acid suitably functions as a stabilizer when combined with a saccharide and is particularly effective as a stabilizer for dry compositions containing a pharmacologically active proteinaceous substance.
The invention also relates to a dry composition containing a pharmacologically active proteinaceous substance in which a stabilizer composed of hydrophobic
amino acid and saccharide is used.

The saccharide(s) used in the invention is not limited but may include those generally used or function as stabilizers for dry pharmaceutical compositions, specifically, pharmaceutical compositions containing a pharmacologically active proteinaceous substance. Specific examples are sucrose, maltose, lactose, trehalose and like disaccharides; mannitol, xylitol and like sugar alcohols; dextran 40, dextran 70; chondroitin sulfuric acid and like polysaccharides. These saccharides can be added to the dry compositions singularly or in an arbitrary combination. Among those, preferable are sucrose, maltose, lactose, trehalose and like disaccharides, and more preferable is sucrose.
The saccharide content of the targeted dry composition is not limited and may be generally about 10 wt.% to about 90 wt.%, in some cases about 20 wt.% to about 80 wt.%, and in some other cases about 40 wt.% to about 80 wt.% per 100 wt.% of dry composition. The above proportion is suitably applied when sucrose or like disaccharides is used.
The hydrophobic amino acid content in the dry composition is not limited and may be, per 100 wt.% of dry composition, generally about 0.1 wt.% to about 70 wt.%, preferably about 0.25 wt.% to about 60 wt.%, more preferably about 0.5 wt.% to about 50 wt.%, and even more

preferably about 1 wt.% to about 50 wt.%. The proportion of hydrophobic amino acid to saccharide contained in the dry composition is, per 100 parts by weight of saccharide, generally about 0.1 part by weight to about 200 parts by weight, preferably about 0.2 part by weight to about 100 parts by weight, and more preferably about 1 part by weight to about 100 parts by weight.
Examples
The present invention will be described below in more detail with reference to Examples. However, the scope of the present invention is not limited to these Examples. Examples 1 to 3
In each Example, a mixture was prepared so as to contain 0.25 ml of an interferon-α bulk solution (hereinafter referred to as "IFN-α bulk solution"; titer: 2 x 107 IU/ml) , 1 mg of Tween 80, 5 mg of sucrose, and 5 mg of an amino acid (isoleucine (Example 1), valine (Example 2), or leucine (Example 3)) per vial (1 ml capacity). A suitable amount of distilled water for injection was added to dissolve them. The mixture was freeze-dried using a shelf-type lyophilizer (LYOVAC GT-4: LEYBOLD). The resultant freeze-dried composition was allowed to stand at 70°C. The extent of coloration and

the titer of the freeze-dried composition were observed with the passage of time, and then the remaining IFN-a activity was estimated by the ratio of the measured IFN-a activity to the IFN-a activity (100%) of the composition immediately after freeze-drying. For comparison, as an amino acid, 5 mg of glycine (Comparative Example 1) or arginine hydrochloride (Comparative Example 2) was used for evaluating the coloration. Furthermore, for evaluating the stability of IFN-a, a test was conducted in the same manner as mentioned above except that a system with no amino acid added was used (Comparative Example 3). The results, including the degree of coloration and the stability of the IFN-a of the compositions obtained in Examples and Comparative Examples, are shown in Table 1 and Table 2.


Table 1

Evaluation of coloration:
No coloration was observed
± Slight coloration was observed
+ Little coloration was observed ++ Much coloration was observed +++ Extreme coloration was observed

Table 2

Preparation Remaining IFN-α Activity (%)


Week 0 Week
1 Week 2
Examples 1. IFN-α + sucrose
+ isoleucine
2. IFN-α + sucrose
+ valine
3. IFN-α + sucrose
+ leucine 100.0 100.0 100.0 71.6 59.2 75.6 51.8 47.1 72.3
Comp. Example 1. IFN-α + sucrose 100.0 48.6 38.7
As shown in Table 1, the combined use of sucrose and glycine and the combined use of sucrose and arginine hydrochloride caused coloration of the freeze-dried composition with the passage of time. Using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger prevented coloration of the freeze-dried composition. Furthermore, as shown in Table 2, the stability of IFN-a improved when using sucrose with hydrophobic amino acid having a hydropathy index (HP-INDEX) of 3.8 or larger compared to the stability when using sucrose singularly.

Examples 4 to 6
In each Example, a mixture was prepared so as to contain 0.25 ml of an IFN-α bulk solution (titer: 2 x 107 IU/ml), 1 mg of Tween 80, 5 mg of maltose, and 5 mg of an amino acid (isoleucine (Example 4), valine (Example 5), or leucine (Example 6)) per vial (1 ml capacity). A suitable amount of distilled water for injection was added to dissolve them. The mixture was freeze-dried using a shelf-type lyophilizer (LYOVAC GT-4: LEYBOLD). The resultant freeze-dried composition was allowed to stand at 70 °C. The extent of coloration of the freeze-dried composition was observed with the passage of time. For comparison, as an amino acid, 5 mg of glycine (Comparative Example 4) or arginine hydrochloride (Comparative Example 5) was used for evaluating the coloration, and the test was conducted in the same manner as mentioned above. The results of the Examples and Comparative Examples are shown in Table 3.

Table 3

Preparation HP-INDEX of
Amino Acid Coloration (70 °C)



Week 0 Week 1 Wee k 2
Examples 4. IFN~cx + maltose
+ isoleucine
5. IFN-a + maltose
+ valine
6. IFN-a + maltose
+ leucine 4. 5 4 . 2 3 . 8 - _ -
Comp. Examples 3. IFN-a + maltose
+ glycine
4. IFN-a + maltose
+ arginine
hydrochloride -0. 4
-4 . 5 - + + + + + + + + + +
Evaluation of coloration:
No coloration was observed ± Slight coloration was observed + Little coloration was observed ++ Much coloration was observed +++ Extreme coloration was observed
As shown in Table 3, the combined use of maltose and glycine and the combined use of maltose and arginine hydrochloride caused coloration of the freeze-dried composition with the passage of time. Using maltose with

hydrophobic amino acid having a hydropathy index of 3.8 or larger prevented coloration of the freeze-dried composition.
Examples 7 to 9
In each Example, a mixture was prepared so as to contain 0.25 ml of an IFN-α bulk solution (titer: 2 x 107 IU/ml), 1 mg of Tween 80, 5 mg of trehalose, and 5 mg of an amino acid (isoleucine (Example 7), valine (Example 8), or leucine (Example 9) ) per vial (1 ml capacity) . A suitable amount of distilled water for injection was added to dissolve them. The mixture was freeze-dried using a shelf-type lyophilizer (LYOVAC GT-4: LEYBOLD). The resultant freeze-dried composition was allowed to stand at 70 °C. The titer of the freeze-dried composition was observed with the passage of time, and then the remaining IFN-a activity was estimated by the ratio of the measured IFN-a activity to the IFN-a activity (100%) of the composition immediately after freeze-drying. For comparison, the test was conducted in the same manner as mentioned above except that a system with no amino acid added was used (Comparative Example 6) for evaluating the stability of IFN-a. The results of the Examples and Comparative Example are shown in Table 4.

Table 4

As shown in Table 4, the stability of IFN-a improved when using trehalose with hydrophobic amino acid having a hydropathy index (HP-INDEX) of 3.8 or larger compared to the stability when using sucrose singularly.
Examples 10 to 12
In each Example, a mixture was prepared so as to contain 0.25 ml of an IFN-a bulk solution (titer: 2 x 107 IU/ml), 1 mg of Tween 80, 40 mg of sucrose, and 5 mg of an amino acid (isoleucine (Example 10), valine (Example 11), or leucine (Example 12)) per vial (1 ml capacity). A suitable amount of distilled water for injection was added to dissolve them. The mixture was freeze-dried using a shelf-type lyophilizer (LYOVAC GT - 4: LEYBOLD). The

resultant freeze-dried composition was allowed to stand at 70 °C. The extent of coloration of the freeze-dried composition was observed with the passage of time. For comparison, as an amino acid, 5 mg of glycine (Comparative Example 7) or arginine hydrochloride (Comparative Example 8) was used for evaluating the coloration, and the test was conducted in the same manner as mentioned above. The results of the Examples and Comparative Examples are shown in Table 5.
Table 5


Evaluation of coloration:
No coloration was observed ± Slight coloration was observed + Little coloration was observed ++ Much coloration was observed +++ Extreme coloration was observed
As shown in Table 5, the combined use of sucrose and glycine and the combined use of sucrose and arginine hydrochloride caused coloration of the freeze-dried composition with the passage of time. Using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger significantly prevented coloration of the freeze-dried composition.
Examples 13 to 15
A freeze-dried composition was obtained in the same manner as in Examples 1 to 3 except that 0.25 ml of IFN-β bulk solution (titer: 2 x 107 IU/ml) was used
7
instead of 0.25 ml of IFN-α bulk solution (titer: 2 x 10 IU/ml). The resultant freeze-dried composition was allowed to stand at 70 °C, and the coloration thereof was observed with the passage of time. The results show that, as Examples 1 to 3, coloration of the freeze-dried composition can be prevented by using sucrose with

hydrophobic amino acid having a hydropathy index of 3.8 or larger.
Examples 16 to 18
A freeze-dried composition was obtained in the same manner as in Examples 10 to 12 except that 0.25 ml of IFN-jJ bulk solution (titer: 2 x 107 IU/ml) was used instead of 0.25 ml of IFN-α bulk solution (titer: 2 x 10 IU/ml). The resultant freeze-dried composition was allowed to stand at 70 °C, and the coloration thereof was observed with the passage of time. The results show that, as Examples 10 to 12, coloration of the freeze-dried composition can be prevented by using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger.
Examples 19 to 21
A freeze-dried composition was obtained in the same manner as in Examples 1 to 3 except that 0.25 ml of IFN-y bulk solution (titer: 2 x 107 IU/ml) was used instead of 0.25 ml of IFN-a bulk solution (titer: 2 x 10 IU/ml). The resultant freeze-dried composition was allowed to stand at 7 0 °C, and the coloration thereof was observed with the passage of time. The results show that, as Examples 1 to 3, coloration of the freeze-dried

composition can be prevented by using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger.
Examples 22 to 24
A freeze-dried composition was obtained in the same manner as in Examples 10 to 12 except that 0.25 ml of IFN-(3 bulk solution (titer: 2 x 107 IU/ml) was used instead of 0.25 ml of IFN-a bulk solution (titer: 2 x 107 IU/ml). The resultant freeze-dried composition was allowed to stand at 70 °C, and the coloration thereof was observed with the passage of time. The results show that, as Examples 10 to 12, coloration of the freeze-dried composition can be prevented by using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger.
Examples 25 to 27
A freeze-dried composition was obtained in the same manner as in Examples 1 to 3 except that 0.25 ml of erithropoietin bulk solution (titer: 2 x 10 IU/ml) was used instead of 0.25 ml of IFN-a bulk solution (titer: 2 x 107 IU/ml). The resultant freeze-dried composition was allowed to stand at 70 °C, and the coloration thereof was observed with the passage of time. The results show that,

as Examples 1 to 3, coloration of the freeze-dried composition can be prevented by using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger.
Examples 28 to 30
A freeze-dried composition was obtained in the same manner as in Examples 10 to 12 except that 0.25 ml of erithropoietin bulk solution (titer: 2 x 107 IU/ml) was used instead of 0.25 ml of IFN-a bulk solution (titer: 2 x 10 IU/ml). The resultant freeze-dried composition was allowed to stand at 70 °C, and the coloration thereof was observed with the passage of time. The results show that, as Examples 10 to 12, coloration of the freeze-dried composition can be prevented by using sucrose with hydrophobic amino acid having a hydropathy index of 3.8 or larger.
Examples 31 to 33
One vial (1 ml capacity) of mixture solution was prepared in such a manner that it comprised 0.25 ml of IFN-a bulk solution (titer: 2 x 107 IU/ml), 40 mg of sucrose, and 5 mg each of two kinds of amino acid (glycine + isoleucine (Example 31), glycine + valine (Example 32), or glycine + leucine (Example 33)). A suitable amount of

distilled water for injection was added to dissolve them. Thereafter, freeze-drying was conducted in the same manner as in Examples 10 to 12 obtaining a freeze-dried composition. The resultant freeze-dried composition was allowed to stand at 70 °C. The extent of coloration of the freeze-dried composition was observed with the passage of time. For comparison, the test was conducted in the same manner as mentioned above except that 5 mg of glycine alone (Comparative Example 7) was used as the amino acid. The results of the Examples and Comparative Example are shown in Table 6.
Table 6


Evaluation of coloration:
No coloration was observed ± Slight coloration was observed + Little coloration was observed ++ Much coloration was observed +++ Extreme coloration was observed
As shown in Table 6, the freeze-dried composition containing sucrose and glycine caused coloration with the passage of time. However, coloration of the freeze-dried composition can significantly prevented by using hydrophobic amino acid having a hydropathy index of 3.8 or larger in addition to sucrose and glycin.
INDUSTRIAL APPLICABILITY The anti-coloring agent of the invention can significantly reduce and/or prevent the coloration of a dry composition with the passage of time caused by the combined use of saccharide and amino acid. Such an anti-coloring agent is specifically useful for preventing the coloration of a dry composition comprising a saccharide and a pharmacologically active proteinaceous substance. From another point of view, the anti-coloring agent is also useful as a stabilizer for a dry composition

containing a saccharide and a pharmacologically active proteinaceous substance. Therefore, the invention can provide dry compositions containing a pharmacologically active proteinaceous substance and an anti-coloring agent or a stabilizer, i.e., dry compositions containing a pharmacologically active proteinaceous substance to which a saccharide and an amino acid are added, which exhibits excellent stability by significantly preventing the coloration and lowered activity observed with the passage of time.

WE CLAIM:
1. A method for preventing coloration of a freeze-dry composition
containing a saccharide and a pharmacologically active proteinaceous
substance, said method comprising
adding hydrophobic amino acid having a hydropathy index of not less than 3.8 to a solution containing a saccharide and a pharmacologically active proteinaceous substance, wherein said hydrophobic amino acid is added in a total amount of from 0.1 parts by weight to 200 parts by weight per 100 parts by weight of said saccharide,
and freeze-drying the solution to obtain said freeze-dry composition, thereby, preventing coloration of said freeze-dry composition.
2. The method for preventing coloration as claimed in claim 1, wherein the hydrophobic amino acid has a hydropathy index in the range of from 3.8 to 4.5.
3. The method for preventing coloration as claimed in claim 1, wherein the hydrophobic amino acid is at least one member selected from the group consisting of valine, leucine and isoleucine.
4. The method for preventing coloration as claimed in claim 1, wherein the saccharide is at least one member selected from the group consisting of reducing sugars, sucrose, trehalose, mannitol and dextran 40.
5. The method for preventing coloration as claimed in claim 1, wherein the hydrophobic amino acid is used in such a manner that its concentration becomes in the range of from 0.1 wt.% to 70 wt% of the total weight of the dry composition.

6. The method for preventing coloration as claimed in claim 1, wherein the pharmacologically active proteinaceous substance is at least one member selected from the group consisting of antiviral polypeptides, immunomodulator polypeptides and hematinic polypeptides.
7. The method for preventing coloration as claimed in claim 1, wherein the pharmacologically active proteinaceous substance is interferon.
Dated this 19th day of June, 2002.
[VINEET ROHILLA]
OF REMFRY & SAGAR
ATTORNEY FOR THE APPLICANTS]

Documents:

00148-mumnp-2006-abstract(31-03-2008).doc

00148-mumnp-2006-abstract(31-03-2008).pdf

00148-mumnp-2006-claims(granted)-(31-03-2008).doc

00148-mumnp-2006-claims(granted)-(31-03-2008).pdf

00148-mumnp-2006-correspondence(11-09-2008).pdf

00148-mumnp-2006-correspondence(ipo)-(18-05-2007).pdf

00148-mumnp-2006-form 1(31-03-2008).pdf

00148-mumnp-2006-form 13(16-10-2008).pdf

00148-mumnp-2006-form 13(31-03-2008).pdf

00148-mumnp-2006-form 18(07-07-2006).pdf

00148-mumnp-2006-form 2(granted)-(31-03-2008).doc

00148-mumnp-2006-form 2(granted)-(31-03-2008).pdf

00148-mumnp-2006-form 3(05-03-2007).pdf

00148-mumnp-2006-form 3(06-02-2006).pdf

00148-mumnp-2006-form 3(07-02-2006).pdf

00148-mumnp-2006-form 3(12-04-2006).pdf

00148-mumnp-2006-form 3(31-03-2008).pdf

00148-mumnp-2006-form 5(07-02-2006).pdf

00148-mumnp-2006-petition under rule 137(31-03-2008).pdf

00148-mumnp-2006-petition under rule 138(31-03-2008).pdf

00148-mumnp-2006-power of authority(23-03-2006).pdf

00148-mumnp-2006-power of authority(31-03-2008).pdf

148-mumnp-2006-claims.doc

148-mumnp-2006-claims.pdf

148-MUMNP-2006-CORRESPONDENCE(11-9-2008).pdf

148-mumnp-2006-correspondence-received-ver-050406.pdf

148-mumnp-2006-correspondence-received-ver-060206.pdf

148-mumnp-2006-correspondence-received-ver-070206.pdf

148-mumnp-2006-correspondence-received-ver-100406.pdf

148-mumnp-2006-correspondence-received-ver-230506.pdf

148-mumnp-2006-correspondence-received.pdf

148-mumnp-2006-description (complete).pdf

148-mumnp-2006-form-1.pdf

148-mumnp-2006-form-2.doc

148-mumnp-2006-form-2.pdf

148-mumnp-2006-form-26.pdf

148-mumnp-2006-form-3.pdf

148-mumnp-2006-form-5.pdf

184-mumnp-2006-claims(23-12-2010).pdf

abstract1.jpg


Patent Number 224549
Indian Patent Application Number 148/MUMNP/2006
PG Journal Number 02/2009
Publication Date 09-Jan-2009
Grant Date 16-Oct-2008
Date of Filing 06-Feb-2006
Name of Patentee OTSUKA PHARMACEUTICAL CO., LTD.
Applicant Address OF 9 KANDATSUKASA-CHO 2-CHOME, CHIYODA-KU, TOKYO 10-8535, JAPAN
Inventors:
# Inventor's Name Inventor's Address
1 CHIKAMASA YAMASHITA OF 11-5, AZA KAWAMUKAINISHINOKOSHIM TOKUNAGA, OTSU-CHO, NARUTO-AHI, TOKUSHIMA 772-0034, JAPAN
2 MASAAKI ODOMI 101-14, AZA NAKATA, OTOZE, AIZUMI-CHO, ITANO-GUN, TOKUSHIMA 771-1240, JAPAN.
PCT International Classification Number C09K 15/16
PCT International Application Number N/A
PCT International Filing date 2000-12-22
PCT Conventions:
# PCT Application Number Date of Convention Priority Country
1 1999-368053 1999-12-24 Japan