US3344028A - Gelatin stabilized dry tablet streptokinase-streptodornase composition - Google Patents

Gelatin stabilized dry tablet streptokinase-streptodornase composition Download PDF

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US3344028A
US3344028A US343959A US34395964A US3344028A US 3344028 A US3344028 A US 3344028A US 343959 A US343959 A US 343959A US 34395964 A US34395964 A US 34395964A US 3344028 A US3344028 A US 3344028A
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streptokinase
streptodornase
gelatin
tablets
solution
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US343959A
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Personeus Gordon Rowland
Hawkins Samuel Richard
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Wyeth Holdings LLC
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American Cyanamid Co
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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • A61K38/16Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • A61K38/164Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
    • A61K38/166Streptokinase

Definitions

  • This invention relates to a stable composition of streptokinase and streptodornase and more particularly is concerned with a composition of matter containing streptokinase and streptodornase, preferably in the form of a tablet, which is stabilized against losses in potency by the addition of gelatin thereto.
  • Streptokinase is well known as an enzyme elaborated by certain strains of beta-hemolytic streptococci, especially those of Group A and Lancefield Group C streptococci.
  • the production of streptokinase by fermentation of these organisms is also accompanied by the formation of substantial amounts of streptodornase.
  • Combinations of streptokinase and streptodornase have been in use for some years for the liquefaction of fibrinous and purulent accumulations in the treatment of suppurative surface tissues, infected wounds and burns, chronic suppurations and the like.
  • streptokinase-streptodornase tablets have raised considerable stability problems in that the tablets are not as stable against losses in potency as are the parenteral grades of streptokinase-streptodornase. As the result, the shelf-life of a tablet must be reduced to a one year marketing period instead of the usual eighteen months. Additionally, in order to insure that the consumer buys a product up to label potency, it has been necessary to formulate the tablet using a 30% excess streptokinasestreptodornase powder. This, of course, is an unsatisfactory answer to the problem as among other things, it imposes higher operating costs.
  • the present invention is based upon the discovery that by mixing liquid streptokinasestreptodornase solution with a gelatin solution also in liquid form and which is equiva- "ice lent to at least 5% by weight of the total solids content of the streptokinase-streptodornase and phosphate diluent being treated, the resulting streptokinase-streptodornase when compressed into tablets in the usual manner is rendered stable against losses in potency for extended periods of time.
  • the gelatin be mixed with the enzyme solution while both are in a liquid phase.
  • the gelatin becomes more or less an integral part of the final powder particles setting up a protective coating for the enzyme.
  • the powder is obtained in final form by vacuum drying the gelatinized enzyme solution in a standard manner and this powder is then used in subsequent tableting procedures in the usual way.
  • an amount of liquid Q gelatin is added to the liquid solution of the enzymes equivalent to 5% by weight of the total solids of the enzymes being treated plus phosphate diluent, it has been found that the desired stability may be obtained when the amount of gelatin is as little as 1.0% by weight of the enzymes plus phosphate diluent.
  • the upper limit of gelatin does not appear to be especially critical and in general it has not been found necessary to exceed 5% by weight based on the weight of the enzymes plus phosphate diluent. In terms of a commercial oral or buccal tablet and which usually contains 12,500 units of active ingredient, the amount of gelatin in such tablets would be about 0.0001 to 0.0005% by weight.
  • the dosage quantity need not be limited to 12,500 units of streptokinase as the dosage quantity may range from about 500 to 12,500 units, a unit of streptokinase being that amount which activates suflicient plasmin to bring about dissolution of a standard fibrin cloth in 10 minutes at 35 C. Usually, however, a single dose ranging from about 10,000 to 20,000 units of streptokinase is satisfactory.
  • the dried enzyme solution containing the gelatin may be formed into water-soluble tablets by standard tableting procedures.
  • the active ingredients may be incorporated with pharmaceutical excipients in a standard manner.
  • Such compositions should contain at least 12,500 units of streptokinase and streptodornase.
  • the potency of the active ingredient is normally in the range of 3000 to 6000 units of streptokinase per milligram of powder. Therefore, the weight of the active ingredient may be between 0.8% and 1.7% of the weight of the tablet.
  • the amount of active ingredient in such compositions is such that a suitable dosage may be obtained.
  • the tablets may contain the following: a binder such as gum tragacanth, acacia, corn starch or gelatin, a disintegrating agent such as corn starch, potato starch, alginic acid, or the like; a lubricant such as stearic acid, magnesium stearate, talc, or the like; and a sweetening agent such as sucrose or saccharin may be added, as well as flavoring such as peppermint, oil of Wintergreen, or cherry flavoring.
  • a binder such as gum tragacanth, acacia, corn starch or gelatin
  • a disintegrating agent such as corn starch, potato starch, alginic acid, or the like
  • a lubricant such as stearic acid, magnesium stearate, talc, or the like
  • a sweetening agent such as sucrose or saccharin may be added, as well as flavoring such as peppermint, oil of Wintergreen, or cherry flavoring.
  • EXAMPLE 1 phosphate buffer diluent is known. Based on the combined total solids, a gelatin solution is prepared which is equivalent to by weight of the total solids of the enzyme one-half gelatin treated; the remaining half served as control portion).
  • the powder is then assayed for temperature In thls Instance 45% loss m q q Str t d t t d t t h f b 0 was observed in the control lot whereas the gelatrmzed 5 rep 0 Omase con en e Ore emg tablets showed a loss of only from original potency ma e mto ta during a period of 4 months at 37 C.
  • EXAMPLE 2 The powder produced as in Example 1 1s bllended ka Example 2 is repeated with the exception that (l) the compressed lflto tablets y aPPmPna te ma mg gelatinized powder and the tablets prepared therefrom Procedures Sing the fOHPWmg formulatloflare compared for stability purposes, as well as the con- (a) An aqueous solution of 205 g- 261211111 l trol powder and tablets, and (2) two separate lots of bulk in 2 liters of hot water is prepared concurrently Wfi liquid streptokin-ase-streptodornase chosen at random are (b) A phosphate solution comprising 2648 g.
  • Weight of lyophillized product 3.00 kg. Each mg. of this gelatinized product is equivalent to about 4200 units of SK/SD.
  • the above product was tableted in the following manner. About 1.5 kg. of the above gelatinized S-K/SD, containing approximately 6.5 billion units of SK, was mixed with 89.5 kg. of sprayed-dried lactose and 1 kg. of magnesium stearate. The well-mixed blend was compressed into 500,000 tablets. Each tablet contained about 12,500 units of SK/SD (3 mg. per tablet).
  • the method of increasing the stability of streptokinase-streptodornase tablets which comprises adding a liquid gelatin solution to a liquid solution containing the 0 enzymes streptokin-ase and streptodorn'ase equivalent to about 5% based on the weight of the total solids in the enzyme solution, and thereafter heating the resulting solution to dryness.

Description

United States Patent 3,344,028 GELATIN STABILIZED DRY TABLET STREPTO- KINASE-STREPTODORNASE COMPOSITION Gordon Rowland Personeus, Old Tappan, NJ., and Samnel Richard Hawkins, Pearl River, N.Y., assignors to American Cyanamid Company, Stamford, Conn.
No Drawing. Filed Feb. 11, 1964, Ser. No. 343,959
3 Claims. (Cl. 167-73) This invention relates to a stable composition of streptokinase and streptodornase and more particularly is concerned with a composition of matter containing streptokinase and streptodornase, preferably in the form of a tablet, which is stabilized against losses in potency by the addition of gelatin thereto.
Streptokinase is well known as an enzyme elaborated by certain strains of beta-hemolytic streptococci, especially those of Group A and Lancefield Group C streptococci. The production of streptokinase by fermentation of these organisms is also accompanied by the formation of substantial amounts of streptodornase. Combinations of streptokinase and streptodornase have been in use for some years for the liquefaction of fibrinous and purulent accumulations in the treatment of suppurative surface tissues, infected wounds and burns, chronic suppurations and the like.
Until recently, it has been proposed to introdce streptokinase into the system by intravenous or intramuscular injection. Each of those modes of administration is subject, however, to serious disadvantages and limitations. Attendance by, or a visit to a physician is necessary and patient acceptance is very poor. Pain and tenderness are experienced at the site of injection and administration by either of these routes may be accompanied by such undesirable side effects as elevation of temperature, nodule formation and allergic reactions. The side effects attending intravenous administration are apt to be particularly serious and may include shock, chills and high fever. Evidently the side effects that accompanying the administration of streptokinase by injection result from the fact that, when a sufiicient quantity is administered by this route to be effective at the site of an injury, there is also produced an undesirably high level in the blood.
Recently, it has been found possible to administer systemically streptokinase in buccal form, that is by absorption of the streptokinase through the mucous membrane, or even more recently by the oral route. The side effects previously noted with intramuscular and intravenous injection have been obviated by these newer dosage forms. Tablets for both oral and buccal administration containing streptokinase-streptodornase have been found to be useful therapeutic agents for accelerating the liquefaction of purulent exudates and lysis of blood clots as Well as efficacious in the reversal of inflammatory processes of diverse origin.
The production of streptokinase-streptodornase tablets, however, has raised considerable stability problems in that the tablets are not as stable against losses in potency as are the parenteral grades of streptokinase-streptodornase. As the result, the shelf-life of a tablet must be reduced to a one year marketing period instead of the usual eighteen months. Additionally, in order to insure that the consumer buys a product up to label potency, it has been necessary to formulate the tablet using a 30% excess streptokinasestreptodornase powder. This, of course, is an unsatisfactory answer to the problem as among other things, it imposes higher operating costs.
The present invention is based upon the discovery that by mixing liquid streptokinasestreptodornase solution with a gelatin solution also in liquid form and which is equiva- "ice lent to at least 5% by weight of the total solids content of the streptokinase-streptodornase and phosphate diluent being treated, the resulting streptokinase-streptodornase when compressed into tablets in the usual manner is rendered stable against losses in potency for extended periods of time. It is not known with certainty how the addition of liquid gelatin to the liquid streptokinase-streptodornase solution results in a product which, when dried, is much more stable than tablets produced by the current operating conditions but it is believed that in some manner the enzyme solutions have been gelatinized by the addition of gelatin which keeps the enzymes from undergoing loss in potency upon storage for extended periods of time.
It is essential that the gelatin be mixed with the enzyme solution while both are in a liquid phase. By this procedure the gelatin becomes more or less an integral part of the final powder particles setting up a protective coating for the enzyme. The powder is obtained in final form by vacuum drying the gelatinized enzyme solution in a standard manner and this powder is then used in subsequent tableting procedures in the usual way.
While as indicated above, preferably an amount of liquid Q gelatin is added to the liquid solution of the enzymes equivalent to 5% by weight of the total solids of the enzymes being treated plus phosphate diluent, it has been found that the desired stability may be obtained when the amount of gelatin is as little as 1.0% by weight of the enzymes plus phosphate diluent. The upper limit of gelatin does not appear to be especially critical and in general it has not been found necessary to exceed 5% by weight based on the weight of the enzymes plus phosphate diluent. In terms of a commercial oral or buccal tablet and which usually contains 12,500 units of active ingredient, the amount of gelatin in such tablets would be about 0.0001 to 0.0005% by weight. Obviously, the dosage quantity need not be limited to 12,500 units of streptokinase as the dosage quantity may range from about 500 to 12,500 units, a unit of streptokinase being that amount which activates suflicient plasmin to bring about dissolution of a standard fibrin cloth in 10 minutes at 35 C. Usually, however, a single dose ranging from about 10,000 to 20,000 units of streptokinase is satisfactory.
The dried enzyme solution containing the gelatin may be formed into water-soluble tablets by standard tableting procedures. Thus, the active ingredients may be incorporated with pharmaceutical excipients in a standard manner. Such compositions should contain at least 12,500 units of streptokinase and streptodornase. The potency of the active ingredient is normally in the range of 3000 to 6000 units of streptokinase per milligram of powder. Therefore, the weight of the active ingredient may be between 0.8% and 1.7% of the weight of the tablet. The amount of active ingredient in such compositions is such that a suitable dosage may be obtained.
The tablets may contain the following: a binder such as gum tragacanth, acacia, corn starch or gelatin, a disintegrating agent such as corn starch, potato starch, alginic acid, or the like; a lubricant such as stearic acid, magnesium stearate, talc, or the like; and a sweetening agent such as sucrose or saccharin may be added, as well as flavoring such as peppermint, oil of Wintergreen, or cherry flavoring.
The invention will be described in greater detail in conjunction with the following specific examples.
EXAMPLE 1 phosphate buffer diluent is known. Based on the combined total solids, a gelatin solution is prepared which is equivalent to by weight of the total solids of the enzyme one-half gelatin treated; the remaining half served as control portion).
TABLE 1 Initial Months, Rfl. Months, 37 0. Lot Potency (SK units/ tablet) 1 2 4 5 1 3 4 Gelatinizcd 11, 600 10.900 14, 400 11, 900 9, 600 12. 600 11, 900 9, 375 Non-gelatinired control 12, 0 0, 900 10,240 8, 800 8, 550 6, 700 6, 675
solution and phosphate being treated. The gelatin is heated It can readily be seen that at the end of five months to form a solution and then cooled below 37 C. The at room temperature there W E an 8% greater 1055 in gelatin solution is then transferred to the liquid bulk soluthe potfincy (lathe f i 01 was tion with thorough mixing. The Smtreated solution is served in the gelatmlzed tablets. The stabilizing effect than vacuum dried to yield a White fluffy powder which of the gelatin is even more dramatic in the accelerated is thoroughly mixed. The powder is then assayed for temperature In thls Instance 45% loss m q q Str t d t t d t t h f b 0 was observed in the control lot whereas the gelatrmzed 5 rep 0 Omase con en e Ore emg tablets showed a loss of only from original potency ma e mto ta during a period of 4 months at 37 C.
EXAMPLE 2 EXAMPLE 3 The powder produced as in Example 1 1s bllended ka Example 2 is repeated with the exception that (l) the compressed lflto tablets y aPPmPna te ma mg gelatinized powder and the tablets prepared therefrom Procedures Sing the fOHPWmg formulatloflare compared for stability purposes, as well as the con- (a) An aqueous solution of 205 g- 261211111 l trol powder and tablets, and (2) two separate lots of bulk in 2 liters of hot water is prepared concurrently Wfi liquid streptokin-ase-streptodornase chosen at random are (b) A phosphate solution comprising 2648 g. of an used in this experimental comparison. The testing interequimolar mixture of monobasic sodium phosphate with 1 W115 are 0 l 9 mimihs and 14 months at room water of crystallization and dibasic sodium phosphate with Permre on 12 waters of crystallization (.06 7 mole of each), disi can readfly be seen that at the end fli 14 month 1 d t d t 80 H r Th 1489 a fbulk period at room temperature, the non-gelatlmzed powder so m Wa F e 16 en 0 and the tablets prepared therefrom show a loss of potency u'mts) added to the pliosphate 50111 of 3 3% and 34% respectively, while the gelatinized powder tlOIl Wlih Stirring SK/SD bulk POWdt?r 1S madfi P Of and the corresponding lot of tablets show no loss of poabout 20% SK) and the solution clarified by filtration. tency.
TABLE 2 Original Qmonths R.T., 14 months 14 months Percent Loss Tablet Lot No. Potency SK SK units/ R.T., SK R.T., SK from units/tablet tablet units/tablet units/tablet theoretical I (gel) 12, 735 13, 125 12, 000 13, 035 0 II (control) 10, 500 s, 325 9, 300 s, 600 34 SK-SD Powder N0. Tablet N 0. Initial Potency 9months R.T., 14 months Percent Loss SK units/mg. units/mg. R.T., units/mg Potency I (5% gel) I 3,867 3,720 3,875 0 II (control) 11 3,611 3,300 2,607 33 1 4% loss. 9% loss.
(c) The gelatin solution (a) is added to the phosphate We claim:
SK/SD solution (b) above, with stirring and the combined solutions lyophillized.
Weight of lyophillized product, 3.00 kg. Each mg. of this gelatinized product is equivalent to about 4200 units of SK/SD.
The above product was tableted in the following manner. About 1.5 kg. of the above gelatinized S-K/SD, containing approximately 6.5 billion units of SK, was mixed with 89.5 kg. of sprayed-dried lactose and 1 kg. of magnesium stearate. The well-mixed blend was compressed into 500,000 tablets. Each tablet contained about 12,500 units of SK/SD (3 mg. per tablet).
At the same time a control lot of tablets is made from powder not treated with gelatin. The initial potencies of both lots of tablets are determined. The potencies of the tablets are then determined at various time intervals and temperatures, that is, at 1, 2, 4 and 5 months at room temperature and at 1, 3 and 4 months at 37 C. Table 1 below shows the results obtained (one bulk liquid split;
1. The method of increasing the stability of streptokinase-streptodornase tablets which comprises adding a liquid gelatin solution to a liquid solution containing the 0 enzymes streptokin-ase and streptodorn'ase equivalent to about 5% based on the weight of the total solids in the enzyme solution, and thereafter heating the resulting solution to dryness.
2. The method according to claim 1 in which the re sulting dried powder is compressed into tablets.
LEWIS GOTTS, Primary Examiner.
S. K. ROSE, Assistant Examiner.

Claims (1)

1. THE METHOD OF INCREASING THE STABILITY OF STREPTOKINASE-STREPTODORNASE TABLETS WHICH COMPRISES ADDING A LIQUID GELATIN SOLUTION TO A LIQUID SOLUTION CONTAINING THE ENZYMES STREPTOKINASE AND STREPTODORNASE EQUIVALENT TO ABOUT 5% BASED ON THE WEIGHT OF THE TOTAL SOLIDS IN THE ENZYME SOLUTION, AND THEREAFTER HEATING THE RESULTING SOLUTION TO DRYNESS.
US343959A 1964-02-11 1964-02-11 Gelatin stabilized dry tablet streptokinase-streptodornase composition Expired - Lifetime US3344028A (en)

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Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3515642A (en) * 1965-12-06 1970-06-02 Takeda Chemical Industries Ltd Method for preparing a stabilized enzyme composition
US3726969A (en) * 1971-06-09 1973-04-10 Abbott Lab Accelerating the lysis of blood clots with urokinase and a benzylamine derivative
US4690816A (en) * 1982-09-20 1987-09-01 Fujisawa Pharmaceutical Co., Ltd. Type soft capsule
US4914020A (en) * 1985-02-05 1990-04-03 Konishiroku Photo Industry Co., Ltd. Multi-layer analytical element with preserved enzyme containing spreading layer

Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2930736A (en) * 1957-01-07 1960-03-29 Nat Drug Co Stabilized trypsin compositions containing partially hydrolyzed gelatin and method of making
US3019167A (en) * 1959-05-01 1962-01-30 Innerfield Irving Method of administering streptokinase systemically

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2930736A (en) * 1957-01-07 1960-03-29 Nat Drug Co Stabilized trypsin compositions containing partially hydrolyzed gelatin and method of making
US3019167A (en) * 1959-05-01 1962-01-30 Innerfield Irving Method of administering streptokinase systemically

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3515642A (en) * 1965-12-06 1970-06-02 Takeda Chemical Industries Ltd Method for preparing a stabilized enzyme composition
US3726969A (en) * 1971-06-09 1973-04-10 Abbott Lab Accelerating the lysis of blood clots with urokinase and a benzylamine derivative
US4690816A (en) * 1982-09-20 1987-09-01 Fujisawa Pharmaceutical Co., Ltd. Type soft capsule
US4914020A (en) * 1985-02-05 1990-04-03 Konishiroku Photo Industry Co., Ltd. Multi-layer analytical element with preserved enzyme containing spreading layer

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