RU2073522C1 - Medicinal preparation having antivirus effect - Google Patents

Abstract

FIELD: medicine. SUBSTANCE: proposed preparation contains human interferone and human immunoglobulins, their ratio being 1:600-300000. Human immunoglobulins are used as synergist. Recombinant human α, β or g-interferone is preferably used. Human immunoglobulins of 1GA, 1GM and 1GG types are used. Said preparation may contain pharmaceutical acceptable desired additives. EFFECT: improved quality. 4 cl, 4 tbl

Description

 The invention relates to medicine, specifically to a medicinal antiviral drug containing human interferon and synergist.

где Х кислород, С_1-6-алкокси, NH₂ или Н, или его фармацевтически приемлемая соль, ацилпроизводное и/или сложный эфир [2]
Известный препарат может содержать фармацевтически приемлемые наполнители и представлять собой таблетки, капсулы, сироп и др. лекарственные формы. Препарат растворим в воде при рН около 7,4 и включает 50-500.000 ед. интерферона на 1 мг синергиста.Known antiviral drug containing β-interferon and synergist-halogenated pyrimidine [1]
The closest analogue of the invention is an antiviral drug containing any type of interferon, including human recombinant interferon and a synergist compound of the formula

where X is oxygen, C _1-6 alkoxy, NH ₂ or H, or a pharmaceutically acceptable salt, acyl derivative and / or ester thereof [2]
A known preparation may contain pharmaceutically acceptable excipients and may be tablets, capsules, syrup, and other dosage forms. The drug is soluble in water at a pH of about 7.4 and includes 50-500,000 units. interferon per 1 mg synergist.

 A disadvantage of the known preparations is the use as a synergist of a chemical compound having a certain toxicity and causing an undesirable side effect of the known compositions.

 In addition, well-known drugs have a long latent period of action, which creates a risk of infection of the body until the peak of the protective effect of interferon develops.

 And finally, preparations based on interferon do not act on the extracellular form of microorganisms, do not suppress the bacterial component of the infection.

 The aim of the Invention is to create a new highly effective, non-toxic, non-side effects drug, acting on both the intracellular and extracellular forms of microorganisms and suppressing both the viral and bacterial components of the infection with virtually no latent period of action.

 This is achieved by the fact that the drug, including human interferon and a synergist, contains human immunoglobulins as a synergist, with a mass ratio of human interferon to human immunoglobulins equal to 1: 600-300,000.

 Preferably, as human immunoglobulins, the preparation contains a mixture of IGA, IGM and IGG.

 Currently, human immunoglobulins (antibodies) are widely used in medical practice to combat bacterial and viral infections, neutralizing exotoxins and extracellular viruses and helping to cleanse the body. A mixture of immunoglobulins can be obtained from normal or immune serum and human blood plasma.

 As a synergist in the claimed preparation, already known immunoglobulin preparations can be used, in particular, the KIP preparation (complex immunoglobulin preparation) containing a mixture of human immunoglobulins IGA, IGM, IGG obtained by treating an extract of plasma B sediment (III fraction) or human blood serum [ 3] This drug is a lyophilisate containing the specified mixture of immunoglobulins and glucose as a stabilizer. The drug is intended for the treatment of acute intestinal infections and dysbiosis.

 As human interferon, the drug contains any type of interferon (α ,,, b or g). Preferably, human interferon is obtained synthetically, namely by genetic engineering.

 According to the invention, the combination of human interferon with human immunoglobulins determines the manifestation of the claimed drug sverhdumnogo (synergistic) antiviral action with a sharp reduction in time to achieve it.

 The drug may contain pharmaceutically acceptable target additives and can be used in the form of powder, tablets, ointments and suppositories.

 The drug has a highly effective antiviral effect, is completely safe and does not detect side effects, acting on both intracellular and extracellular forms of microorganisms and suppressing both the viral and bacterial components of the infection with virtually no latent period of action, and is used for prevention and treatment a wide range of viral diseases.

 The inventive preparation is a mixture of human interferon and human immunoglobulins and can be obtained by simple mixing of the starting components. It is an amorphous product with a bluish tint, odorless and tasteless, readily soluble in water and a 20-30% solution of dimethyl sulfoxide. The drug is used in the form of powder, tablets, ointments and suppositories.

 Example 1. The preparation in the form of a powder includes human interferon and human immunoglobulins in a mass ratio of 1: 600-300 000.

 Example 2. The inventive preparation in the form of tablets includes the ingredients in the ratio shown in table 1.

 Example 3. The inventive preparation in the form of an ointment includes the ingredients in the ratio shown in table.2.

 Example 4. The inventive drug in the form of candles includes the ingredients in the ratio shown in table.3.

 Biological tests were carried out using human recombinant a-, b- and g- interferon preparations and CIP as components of the claimed drug.

 The mass ratio of the starting drugs during the tests varied in the range of the preparation of interferon, the preparation of immunoglobulins, equal to 1:10 - 1000, which in terms of the corresponding substances is 1: 600-300 000. Such a conversion of the ratios was made taking into account the fact that 3 mg of lyophilized starting drugs interferon contains 10-50 micrograms of pure protein.

 The ratio of active components in the claimed preparation is established taking into account the maximum antiviral activity achieved by it and economic feasibility.

 Studies of the antiviral activity of the claimed drug was performed on cell cultures of SPEV and Wish against 100 TCD (50% tissue cytopathic dose) of vesicular stomatitis virus, EMC virus, influenza virus and Sendai virus. In all experiments, similar results were obtained, confirming the presence of a super-total (synergistic) antiviral effect and a sharp reduction in the time it was reached.

 Evaluation of the antiviral effect of the claimed drug and its ingredients was carried out in accordance with VFS 42-227 BC-89, in terms of antiviral activity titer. The antiviral activity titer was taken as the reciprocal of the dilution of the test drug, in which the cell culture in 50% of the plate wells was visually completely protected from the cytopathic effect of the virus.

 Examples of biological tests are presented below. The ratio of active components in the tested variants of the claimed drug in the table. 4.

Example 5. 3 mg of a lyophilized preparation of a-interferon with an activity of 1x10 ⁶ IU was dissolved in 1 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 1000 times, triturated and introduced into the wells of a flat-bottomed 96-well plate with a monolayer cell culture Wish. Incubation was carried out at 37 ^o C in an atmosphere with 5% CO ₂ for 18 hours. After that, a dose of vesicular stomatitis virus corresponding to 100 TCD 50 in 0.1 ml, where TCD 50 - 50%, was added to each well with the test materials. tissue cytopathic dose. After the introduction of the indicator virus, the cell culture was incubated for 2 days at 37 ^o C in an atmosphere with 5% carbon dioxide. The determination of the activity of interferon in the preparation was taken into account when the dose of the introduced virus corresponded to 100 TCD 50. For the titer of interferon, the reciprocal of the preparation was taken, at which the cell culture in 50% of the holes was visually completely protected from the cytopathic effect of the virus.

 The titer of antiviral activity of a-interferon was 1: 64000. In a titer of 1: 128,000, the cytopathic effect of the virus was observed.

Example 6. 3 mg of a lyophilized preparation of b-interferon with an activity of 1x10 ⁶ IU was dissolved in 1 ml of medium 199 with 2% serum of cow fruit and antibiotics, then diluted 1000 times, triturated and introduced into the wells of a flat-bottomed 96-well plate with a monolayer cell culture Wish. The incubation was carried out at 37 ^o C in an atmosphere with 5% CO ₂ for 18 hours. After that, a dose of vesicular stomatitis virus corresponding to 100 TCD50 in 0.1 ml was added to each well with test materials, where TCD50 is a 50% tissue cytopathic dose. After the introduction of the indicator virus, the cell culture was incubated for 2 days at 37 ^o C in an atmosphere with 5% carbon dioxide. Accounting for the determination of interferon activity in the preparation was carried out when the dose of the introduced virus corresponded to 100 TCD50. For the interferon titer, the reciprocal of the preparation was taken, in which the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

 The titer of the antiviral activity of b-interferon was 1:64 000. In the titer of 1: 128 000 the cytopathic effect of the virus was observed.

Example 7. 4 mg of a lyophilized preparation of g-interferon with an activity of 1x10 ⁵ IU was dissolved in 1 ml of medium 109 with 2% serum of cow fruit and antibiotics, then diluted 1000 times, triturated and introduced into the wells of a flat-bottomed 96-well plate with a monolayer cell culture Wish. Incubation was carried out at 37 ^o C in an atmosphere with 5% CO ₂ for 18 hours. After that, a dose of vesicular stomatitis virus corresponding to 100 TCD50 in 0.1 ml was added to each well with test materials, where TCD50 is a 50% tissue cytopathic dose. After the introduction of the indicator virus, the cell culture was incubated for 2 days at 37 ^o C in an atmosphere with 5% carbon dioxide. Accounting for the determination of interferon activity in the preparation was carried out when the dose of the introduced virus corresponded to 100 TCD50. For the titer of interferon, the reciprocal of the preparation was taken, in which the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

 The titer of the antiviral activity of g-interferon was 1:32 000. In the titer of 1:64 000 the cytopathic effect of the virus was observed.

Example 8. 300 mg of a lyophilized preparation of immunoglobulins was dissolved in 1 ml of medium 199 with 2% serum of cow fruits and antibiotics, triturated and introduced into the wells of a flat-bottomed 96-well plate with a monolayer Wish cell culture. Incubation was carried out at 37 ^o C in an atmosphere with 5% CO ₂ for 18 hours. After that, a dose of vesicular stomatitis virus corresponding to 100 TCD 50 in 0.1 ml, where TCD 50 is 50% tissue, was added to each well with the test materials. cytopathic dose. After the introduction of the indicator virus, the cell culture was incubated for 2 days at 37 ^o C in an atmosphere with 5% carbon dioxide. The determination of the activity of immunoglobulins was carried out when the dose of the introduced virus corresponded to 100 TCD 50. For the titer of immunoglobulins, the reciprocal of the preparation was taken, in which the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

 The titer of antiviral activity of immunoglobulins was 1:16. In the titer of 1:32, the cytopathic effect of the virus was observed.

 Example 9. The test was carried out analogously to example 8 with the exception that 3 g of a lyophilized immunoglobulin preparation was used. The titer of antiviral activity of immunoglobulins was 1: 160. In a titer of 1: 320, the cytopathic effect of the virus was observed.

Example 10. 3 mg of a lyophilized preparation of a-interferon with an activity of 1x10 ⁶ IU 300 mg of a lyophilized preparation of immunoglobulins was dissolved in 1 ml of medium 199 with 2% serum of cow fruit and antibiotics, then diluted 1000 times, titrated and in a titer of 1: 128 000 interferon was introduced into a well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 5.

 In a titer of 1: 128,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 11. 3 mg of a lyophilized preparation of b-interferon with an activity of 1x10 ⁶ IU and 300 mg of a lyophilized preparation of immunoglobulins were dissolved in 1 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 1000 times, titrated and in a titer of 1: 128 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 6.

 At a titer of 1: 128,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 12. 3 mg of a lyophilized preparation of g-interferon with an activity of 1x10 ⁵ IU 300 mg of a lyophilized preparation of immunoglobulins was dissolved in 1 ml of medium 199 with 2% serum of cow fruit and antibiotics, then diluted 1000 times, titrated and in a titer of 1:64 000 interferon was introduced into a well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 7.

 At a titer of 1:64,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 13. 3 mg of a lyophilized preparation of a-interferon with an activity of 1x10 ⁶ IU and 30 mg of a lyophilized preparation of immunoglobulins were dissolved in 1 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 1000 times, titrated and in a titer of 1: 128 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 5. In a titer of 1: 128,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 14. 3 mg of a lyophilized preparation of b-interferon with an activity of 1x10 ⁶ IU and 30 mg of a lyophilized preparation of immunoglobulins were dissolved in 1 ml of medium 199 with 2% serum of cow fruit and antibiotics, then diluted 1000 times, titrated and in a titer of 1: 128 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 6.

 At a titer of 1: 128,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 15. 3 mg of a lyophilized preparation of g-interferon with an activity of 1x10 ⁵ IU and 30 mg of a lyophilized preparation of immunoglobulins were dissolved in 1 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 1000 times, titrated and in a titer of 1:64 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 7.

 At a titer of 1:64,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 16. 3 mg of a lyophilized preparation of a-interferon with an activity of 1x10 ⁶ IU and 3 g of a lyophilized preparation of immunoglobulins were dissolved in 10 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 100 times, titrated and in a titer of 1: 128 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 5.

 At a titer of 1: 128,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 17. 3 mg of a lyophilized preparation of b-interferon with an activity of 1x10 ⁶ IU and 3 g of a lyophilized preparation of immunoglobulins were dissolved in 10 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 100 times, titrated and in a titer of 1: 128 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 6.

 At a titer of 1: 128,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 18. 3 mg of a lyophilized preparation of g-interferon with an activity of 1 × 10 ⁵ IU and 3 g of a lyophilized preparation of immunoglobulins were dissolved in 10 ml of medium 199 with 2% serum of cow fruits and antibiotics, then diluted 100 times, titrated and in a titer of 1:64 000 interferon was introduced into the well of a flat-bottomed 96-well plate with a monolayer culture of Wish cells. Further tests were carried out analogously to example 7.

 At a titer of 1:64,000, the cell culture in 50% of the wells was completely protected from the cytopathic effect of the virus.

Example 19. The expressed antiviral effect of a-, b- and g-interferon in the culture of Wish cells after their preincubation at 37 ^° C for 40 minutes with the vesicular stomatitis virus develops only after 18 hours, while when using the inventive preparation the antiviral effect reached after 40 minutes.

 Thus, in the inventive preparation, the mass ratio of interferon immunoglobulins is 1: 600-300000.

Claims (4)

 1. The antiviral drug, including human interferon and a synergist, characterized in that as a synergist it contains human immunoglobulins in a mass ratio of human interferon: synergist 1: 600 300000.  2. The drug according to claim 1, characterized in that as a human interferon, it contains recombinant alpha, or beta, or gamma interferon human.  3. The drug according to claim 1, characterized in that as a human immunoglobulin it contains a mixture of IGA, IGM and IGG.  4. The drug according to claims 1 to 3, characterized in that it further comprises pharmaceutically acceptable target additives.

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