RU2267329C2 - Method for treating diseases accompanied with alterations of qualitative and/or quantitative composition of blood extra-cellular dna (variants) - Google Patents

Abstract

FIELD: medicine, veterinary science.

SUBSTANCE: the present innovation deals with treating malignant tumors, or infections, caused by bacteria, fungi and protozoa, or atherosclerosis, or diabetes mellitus, or diseases associated with delayed-type reaction of hypersensitivity, or diseases developed due to mutations of somatic cells' genes. For this purpose, one should introduce an agent that binds blood extra-cellular DNA, or an enzyme to alter chemical structure of blood extra-cellular DNA, or blood should be supplemented with an agent that stimulates either the synthesis or activity of endogenous desoxyribonuclease or an agent that stimulates the synthesis of antibodies that bind blood extra-cellular DNA. The innovation suggested enables to obtain high efficiency of low-toxic etiological treatment of the diseases mentioned above.

EFFECT: higher efficiency of therapy.

3 cl, 3 dwg, 14 ex, 10 tbl

Description

The invention relates to medicine and veterinary medicine and can be used to treat diseases accompanied by qualitative or quantitative changes in extracellular blood DNA, namely malignant tumors or infections caused by bacteria, fungi and protozoa, or atherosclerosis, or diabetes mellitus, or diseases associated with the reaction delayed-type hypersensitivity, as well as diseases caused by mutations in somatic cell genes.

According to modern knowledge, the listed diseases are extremely heterogeneous and painful processes that differ in etiology and pathogenesis. In accordance with these ideas, the treatment of these diseases was carried out by completely different methods. So, the main method of drug treatment of cancer is chemotherapy, see Merck Manual of Diagnosis and Therapy; 16 ^th Edition.

The main method for treating diseases caused by bacteria, fungi and protozoa is antibiotic and chemotherapy, see Merck Manual of Diagnosis and Therapy; 16 ^th Edition.

The main method of drug treatment of atherosclerosis is therapy with statin drugs that suppress cholesterol synthesis in the body, see New Concepts and Paradigms in Cardiovascular Medicine: The Noninvasive Management of Coronary Artery Disease, K. Lance Gould, THE AMERICAN JOURNAL OF MEDICINE, Volume 104, June 22, 1998, 2s-17s.

The treatment of diabetes mellitus is based on three main approaches: replacement therapy with insulin preparations, drug therapy aimed at improving the secretion of insulin by the pancreas, drug therapy aimed at increasing tissue sensitivity to insulin or accelerating tissue utilization of glucose, see Pharmacological Management of Diabetes: Recent Progress and Future Perspective in Daily Drug Treatment, Gerard Emilien et.al., Pharmacol. Ther. Vol. 81, No.1, pp. 37-51, 1999.

The basis for the treatment of allergic diseases associated with type IV hypersensitivity reactions is immunosuppressive or immunomodulating therapy, see Therapeutic Immunosupression, ed. A. W. Thomson, Ser. Immunology and Medicine vol. 29, Kluwer Acad. Publishers, Dordrecht, 2001.

Diseases developing as a result of mutations in somatic cell genes and accompanied by the development of somatic mosaicism have no etiological treatment at all, only symptomatic treatment is carried out (Youssoufian H., Pyeritz RE. Mechanisms and Consequences of Somatic Mosaicism in Humans, Nature Reviews Genetics, 2002; 3: 748-758).

The main problem of the most common chemotherapy of oncological diseases is considered its low effectiveness and high toxicity (Merck Manual of Diagnosis and Therapy; 16 ^th Edition).

The main problem of antibiotic therapy of bacterial infections is the problem of drug resistance. The circulation of antibiotic-resistant bacterial strains and their neoplasm during treatment (for example, due to the formation of biofilms in the patient's body) are the main cause of ineffective therapy (The use and resistance to antibiotics in the community. Cizman M, Int J Antimicrob Agents, 2003, Apr 21: pp. 297-307). It is generally recognized that the problem of antibiotic resistance of microorganisms is currently a global threat (Mechanisms of antimicrobial resistance: their clinical relevance in the new millennium. Sefton AM, Drugs, 2002, vol. 62: 557-66) and requires the development of new antibiotic drugs with original mechanisms of antibacterial effects and new non-antibiotic methods of influencing the infectious process. In particular, in the treatment of infection caused by penicillin and cephalosporin antibiotic-resistant gram-positive cocci, the antibiotic Vancomycin is used. Its main disadvantages include the increase in the number of vancomycin-resistant strains in the circulation; high toxicity; a relatively narrow spectrum of drug activity (The threat of vancomycin resistance. PerlTM, Am J Med, 1999, May, 106: 26S-37S).

In connection with the above, the urgent task of finding a method of antibacterial therapy is effective, low toxicity, active against a wide range of bacteria, including those resistant to antibiotic drugs.

The problems of antibiotic and chemotherapy of infections caused by fungi and protozoa are basically the same as the problems of antibiotic therapy of bacterial infections; for example, when treated with the widespread antifungal agent amphotericin (Antifungal drug resistance to azoles and polyenes. Mar Masia Canuto et.al., The Lancet Infectious Diseases, Volume 2, Issue 9, September 1, 2002, Pages 550-563; A systematic review of the antifungal effectiveness and tolerability of amphotericin In formulations, Jane P. Barrett et.al., Clinical Therapeutics, Volume 25, Issue 5, May 2003, Pages 1295-1320).

Atherosclerosis is a systemic disease, accompanied by the formation of specific atherosclerotic plaques in the walls of large and medium arteries. Depending on the place of occurrence, stage of development and magnitude of atherosclerotic plaques, the disease has various clinical manifestations (coronary heart disease, stroke, etc.). It is the manifestations of systemic atherosclerosis at the level of one or another organ that are subjected to drug and surgical treatment. Atherosclerosis as a systemic disease does not have methods of drug treatment. The most common prevention method that slows down the progression of the disease is the treatment with 3-hydroxy-3-methylglutaryl coenzyme A (HMGCoA) reductase inhibitors (Lovastatin, Parvastatin, etc.), which inhibits the synthesis of endogenous cholesterol and accelerates the clearance of low density lipoproteins from blood plasma, which slows the development of atherosclerosis (New Concepts and Paradigms in Cardiovascular Medicine: The Noninvasive Management of Coronary Artery Disease, K. Lance Gould, THE AMERICAN JOURNAL OF MEDICINE, Volume 104, June 22, 1998, 2s-17s). The disadvantages of this treatment are serious side effects (A safety look at currently available statins., Moghadasian MH, Expert Opin Drug Saf, 2002, Sep 1: pp. 269-74) and limited effectiveness (Statins: balancing benefits, efficacy and safety., Clearfield MB, Expert Opin Pharmacother, 2002, May 3: pp. 469-77).

The main cause of disability and death in patients with type 1 and type 2 diabetes are complications associated with the development of micro- and macroangiopathies. It is believed that achieving effective metabolic control (maintaining normal glucose and glycosylated hemoglobin levels at physiological boundaries for a long time) prevents the development of complications. Insulin therapy, including intensive, is the method of choice in situations where metabolic control with other drugs cannot be achieved (Outpatient insulin therapy in type 1 and type 2 diabetes mellitus: scientific review, DeWitt DE, Hirsch IB, JAMA, 2003, May 289: pp. 2254-64). However, even with intensive treatment regimens, the risk of developing complications, including fatal ones, remains high (Cause-specific mortality in a population with diabetes: South Tees Diabetes Mortality Study., Roper NA, et.al., Diabetes Care, 2002, Jan 25 : pp. 43-8). In connection with the above, the urgent and generally recognized task of finding new drugs for the treatment of type 1 and type 2 diabetes, including those capable of preventing the development of complications, is relevant and recognized.

One of the most widely used methods in clinical practice for treating conditions associated with delayed hypersensitivity reactions is the administration of the Cyclosporin A peptide, see Therapeutic Immunosupression, ed. AW Thomson, Ser. Immunology and Medicine vol. 29, Kluwer Acad. Publishers, Dordrecht, 2001. Well-known disadvantages of this method include serious side effects - nephrotoxicity, hypertension and a high risk of infection (Cyclosporine: mechanisms of action and toxicity, Graham RM, Cleve Clin J Med, 1994, Jul-Aug 61: pp. 308-13). Another problem is the loss of effectiveness with prolonged use of the drug, which manifests itself, for example, in an increased likelihood of transplant rejection (Renal transplantation, past, present and future, Ponticelli C, et.al. J Nephrol, 1999, Jul-Aug 12, Suppl 2: S105-10).

Thus, for the treatment of diseases accompanied by changes in the qualitative and / or quantitative composition of extracellular blood DNA, a wide range of different methods are used that have similar disadvantages:

1) toxicity;

2) the development of side effects;

3) low effectiveness of therapy.

Meanwhile, in real clinical practice, the diseases under consideration often accompany one another. For example, therapy with immunosuppressive drugs for diseases associated with a delayed hypersensitivity reaction, significantly increases the risk of developing infectious diseases (Recent advances in the diagnosis and management of infection in the organ transplant recipient. Tolkoff-Rubin NE, Rubin RH; Semin Nephrol, 2000, Mar 20: 148-63); atherosclerosis is a common complication of diabetes (Diabetes and atherosclerosis: epidemiology, pathophysiology and management. Beckman JA, Creager MA, Libby P; JAMA, 2002, May 287: 2570-81), and often its development is accompanied by a systemic infection process (Infection and atherosclerosis: potential roles of pathogen burden and molecular mimicry, Epstein SE, Zhu J, Bumett MS, Zhou YF, Vercelotti G, Hajjar D, Arterioscler Thromb Vasc Biol, 2000, Jun 20: 1417-20); a number of forms of diabetes develop as a result of the development of a delayed-type hypersensitivity reaction (Evidence of islet cell autoimmunity in elderly patients with type 2 diabetes, Pietropaolo M, Barinas-Mitchell E, Pietropaolo SL, Kuller LH, Trucco M, Diabetes, 2000, Jan 49: 32- 8), or against the background of an infectious process (Systemic diseases caused by oral infection. Li X, Kolltveit KM, Tronstad L, Olsen I, Clin Microbiol Rev 2000 Oct 13: 547-58) and, in turn, leads to a high risk of development infections (Diabetes and the risk of infection-related mortality in the US, Bertoni AG, Saydah S, Brancati FL, Diabetes Care, 2001, June, 24: 6 1044-9).

Currently, there are no methods that would allow to treat the above diseases in combination. In this regard, there is no opportunity to take any well-known technical solution for the prototype of the present invention.

All variants of the present invention are based on the solution of the problem of creating a highly effective and low-toxic method for treating malignant tumors, infectious diseases caused by bacteria, fungi and protozoa, atherosclerosis, diabetes mellitus, diseases associated with a delayed hypersensitivity reaction, diseases caused by mutations in somatic cell genes.

According to the first embodiment of the invention, this problem is solved due to the fact that for the treatment of malignant tumors, or infectious diseases caused by bacteria, fungi and protozoa, or atherosclerosis, or diabetes mellitus, or allergic diseases associated with a delayed hypersensitivity reaction, or diseases caused by mutations in somatic cell genes, an agent that binds extracellular blood DNA is injected into the blood.

According to a second embodiment of the invention, this problem is solved due to the fact that an enzyme is introduced into the blood that alters the chemical structure of the extracellular DNA of the blood.

According to a third embodiment of the invention, this problem is solved by introducing into the blood an agent that stimulates the synthesis or activity of endogenous deoxyribonuclease, or an agent that stimulates the synthesis of antibodies that bind extracellular blood DNA.

The development of these diseases is accompanied by qualitative and quantitative changes in extracellular blood DNA, however, sources known to the applicant lack knowledge on the genetic repertoire of extracellular blood DNA of patients with the diseases under consideration, the biological role of extracellular blood DNA in the diseases under consideration, and the possible therapeutic effect of its binding or modification for the treatment of these diseases .

According to the applicants, the extracellular DNA of the blood of patients with the diseases under consideration contains a unique in its qualitative and quantitative composition repertoire of genes and regulatory genetic elements, which differs sharply from the DNA repertoire described in the human genome. In contrast to intracellular DNA, extracellular blood DNA of patients with the diseases under consideration contains mainly unique human genes. The presence of bacterial extracellular DNA and extracellular DNA of fungi in the biofilm matrix and in the blood plasma of an infected person has been established.

It has been established that extracellular DNA of blood, including extracellular DNA of bacteria, fungi and parasites in the diseases under consideration, contributes to their development.

It has been established that the binding and modification of extracellular blood DNA, as well as the stimulation of the synthesis or activity of endogenous biopolymers that bind, or destroy, or modify the chemical composition and / or conformation and / or polymerization of extracellular blood DNA without its destruction, leads to therapeutic effect.

The above new properties of the claimed invention, based on fundamentally new ideas about the role of extracellular DNA of blood plasma in the development of the diseases under consideration, allow us to conclude that the claimed method meets the criterion of "inventive step".

The claimed method is implemented as follows.

Materials and methods.

In the first embodiment, antibodies against DNA isolated from the blood of patients with systemic lupus erythematosus according to the method of Shuster A.M. were used as a DNA binding agent. (Shuster A.M. et.al., Science, v. 256.1992, pp. 665-667). Similar anti-DNA antibodies are capable of binding DNA.

In the second embodiment, bacterial Sss I Methylase (CpG Methylase), (NewEngland Biolabs) was used as a DNA modifying agent. In the Sss I experiments, methylase was included in the composition of small unilamellar liposomes (SUVs) in the ratio of 1u enzyme per 1 μg of lipids (enzymesosomes), as well as T4 ligase enzyme (Fermentas).

In the third embodiment, anti-Gf actin antibodies (Calbiochem) were used as an agent that stimulates the synthesis and / or activity of endogenous biopolymers that bind, or destroy, or modify the chemical composition and / or conformation and / or polymerization of extracellular blood DNA without its destruction. . G-Actin is an inhibitor of the activity of endogenous DNase I. The binding of actin to antibodies increases the activity of endogenous DNase I.

Plasma DNA was isolated as follows: fresh (no more than 3-4 hours after collection) blood plasma with an added anticoagulant (sodium citrate) was unscrewed on a pillow of Ficoll-PlaquePlus (Amersham-Pharmacia) at 1500 g for 20 minutes at room temperature. Plasma (1/2 of the total amount) was carefully selected without touching the remainder of the cells on the Ficoll pillow, and unscrewed at 10,000 g for 30 minutes to get rid of cell debris and debris. The supernatant was collected without affecting the precipitate, up to 1% sarcosyl, up to 50 mM Tris-HCl, pH 7.6, up to 20 mM EDTA, up to 400 mM NaCl and an equal volume of 1: 1 phenol-chloroform mixture were added. The resulting emulsion was incubated at 65 ° C for 2 hours, then phenol-chloroform was separated by centrifugation at 5000g for 20 minutes at room temperature. The phenol-chloroform deproteinization procedure was repeated in the same way three times, after which the aqueous phase was treated with chloroform and then diethyl ether. Separation from organic solvents was carried out by centrifugation at 5000 g for 15 minutes. An equal volume of isopropanol was added to the resulting aqueous phase and incubated overnight at 0 ° C. After precipitation, nucleic acids were separated by centrifugation at 0 ° C, 10,000 g for 30 minutes. The nucleic acid precipitate was dissolved in a buffer containing 10 mM Tris-HCl, pH 7.6, 5 mM EDTA, and applied onto a cushion of step cesium chloride (1 M, 2.5 M, 5.7 M) in a centrifuge tube for the SW60Ti rotor. The DNA volume was 2 ml, the volume of each step of CsCl - 1 ml. Ultracentrifugation was performed in an L80-80 (Beckman) instrument for 3 hours at 250,000 g. DNA was collected from the surface of the 5.7 M step in fractions. Fractions were dialyzed for 12 hours at 4 ° C. The presence of DNA in the fractions was determined by agarose electrophoresis, with visualization of DNA with ethidium bromide. The amount of DNA was determined spectrophotometrically (Beckman DU70) in a 100 μl cuvette, taking a spectrum from 220 to 320 nm.

Example 1. The effect of the destruction, binding and modification of extracellular DNA on its pathogenic properties

C57B1 mice were vaccinated with a high metastatic or low metastatic LLC tumor strain. On the 9th day after the inoculation, the animals were euthanized and the total blood plasma of mice was collected. The total fraction of extracellular blood DNA after isolation was stored at -20 ° C in phosphate buffer.

The experiment involved 7 groups of mice inoculated with a low metastatic LLC strain.

Group 1-6 mice with a low metastatic LLC strain inoculated.

A group of 2-6 mice with a grafted low metastatic LLC strain + double intravenous (on the seventh and eighth day after transplantation) administration of the total extracellular DNA fraction of mice with a grafted high metastatic strain (0.05 μg of DNA was dissolved in 500 μl of fresh heparinized blood before administration).

A group of 3-6 mice with a grafted low metastatic LLC strain + double intravenous (on the seventh and eighth day after transplantation) administration of the total DNA fraction of mice with a grafted high metastatic strain (0.05 μg of DNA was dissolved in 500 μl of fresh plasma before administration). Before the introduction, the DNA sample was subjected to photochemical disinfection (addition of 1 μM methylene blue, followed by red light exposure for 10 minutes (~ 60,000 Lux).

A group of 4-6 mice with a grafted low metastatic LLC strain + double intravenous (on the seventh and eighth day after grafting) administration of the total DNA fraction of mice with a grafted high metastatic strain (0.05 μg of DNA was dissolved in 500 μl of fresh plasma before administration). Before administration, the DNA sample was mixed with 10 μg of anti-DNA antibodies.

A group of 5-6 mice with a grafted low metastatic LLC strain + intravenous twofold (on the seventh and eighth day after grafting) administration of the total DNA fraction of mice with a grafted high metastatic strain (0.05 μg of DNA was dissolved in 500 μl of fresh heparinized blood before administration). Before introducing into the sample, 1 μg of Ricin plant toxin fragment A was added and incubated for 1 hour at 37 ° C. Ricin is a member of the RIP family (ribosome inactivating proteins) of toxins that are widely used to create immunotoxins. In addition to the ability to inactivate ribosomes, these proteins have the ability to deadenylate DNA. To realize the toxic effect, the catalytic unit A of RIP type II toxins must be delivered to the cell by subunit B. In the absence of subunit B, chain A is not toxic, however, the polynucleotide adeninglycosidase activity of chain A can be used to inactivate DNA circulating in plasma.

A group of 6-6 mice with a grafted low metastatic LLC strain + intravenous twofold (on the seventh and eighth day after grafting) administration of the total DNA fraction of mice with a grafted high metastatic strain (0.05 μg of DNA was dissolved in 500 μl of fresh heparinized blood before administration). The DNA sample was enzymatically methylated prior to administration (I. Muiznieks et.al., FEBS Letters, 1994, v. 344, pp. 251-254).

Group 7 - 6 mice with a low metastatic LLC strain inoculated + double intravenous (on the seventh and eighth day after transplantation) administration of the total extracellular DNA fraction of mice inoculated with a low metastatic LLC strain.

A group of 8–6 mice with a grafted low metastatic LLC strain + intravenous twofold (on the seventh and eighth day after grafting) administration of the total DNA fraction of mice with a grafted high metastatic strain (0.05 μg DNA was dissolved in 500 μl of fresh heparinized blood before administration. DNA sample before the introduction was incubated in the presence of 100U ligase for 30 minutes at 37 ° C.

The number of metastatic nodes in the lungs was evaluated on day 15 after inoculation.

The experimental results are shown in table 1.

Table 1 Group Ncp one 12.0 2 22.5 3 14.1 four 15,5 5 15.1 6 12.3 7 13.3 8 14.5

Thus, the extracellular DNA of the blood of mice with a high-grade tumor strain enhances the metastasis of a less malignant tumor. The binding and modification of extracellular DNA of the blood prevents this according to the claimed method.

Example 2. The effect of binding and modification on the pathogenicity of the extracellular DNA of a patient with atherosclerosis and diabetes

Human embryonic pancreatic beta cells and human aortic endothelial cells were used to form the primary cell culture. 24 hours after passage in the experimental series, extracellular DNA isolated from the plasma of a patient with severe type 2 diabetes and systemic atherosclerosis (0.0025 μg DNA per ml of culture medium) was added to the cell cultures.

In the first experimental series, anti-DNA antibodies were added to the culture at a concentration of 5 μg / ml.

In the second experimental series, enzymes in a concentration of 20 μg / ml were additionally added to the culture.

After 24 hours, the content of viable cells was evaluated by the inclusion of trypan blue dye.

The experimental results are shown in table 2.

The percentage of viable cells 48 hours after passage:

table 2 Cells The control DNA of the patient Patient DNA + anti-DNA antibodies DNA of the patient + enzymesosomes B cells 73% 43% 65% 59% Endothelium 62% 35% 49% fifty%

Thus, the extracellular DNA of the blood of a patient with severe type II diabetes and atherosclerosis has a negative effect on both healthy pancreatic B cells and healthy endothelial cells. The binding and modification of the extracellular DNA of the patient’s blood prevents this according to the claimed method.

Example 3. Treatment of a malignant tumor.

Group 1 - 7 mice vaccinated with Ehrlich carcinoma - control.

Group 2 - 6 mice vaccinated with Ehrlich carcinoma, received on the third day after transplantation of the tumor an intravenous injection of a fraction of human anti-DNA antibodies of 200 μg per animal.

A group of 3 to 6 mice vaccinated with Ehrlich carcinoma, received on the third day after transplantation of the tumor an intravenous injection of “enzymes” at a dose of 700 mcg per animal.

The effect was determined by the size of the tumor on day 7 after inoculation.

Tumor size 7 days after inoculation:

Table 3 Group Tumor volume, mm ³ one 105 +/- 12 2 57 +/- 11 3 65 +/- 15

The data presented indicate that the binding and modification of extracellular blood DNA has an antitumor effect.

Example 4. Treatment of bacterial and fungal infections.

In the experiment used white outbred mice weighing 23-25 grams.

Group 1 (10 mice) - the mice were injected into the retroorbital sinus with bacteria of the pathogenic strain of Staphylococcus aureus VT-2003R at a dose of 1 × 10 ¹⁰ bacterial cells per mouse. 2 hours after infection, the anti-DNA antibody was administered intravenously to the mice at a dose of 300 μg / mouse.

Group 2 (10 mice) - the mice were injected into the retroorbital sinus with bacteria of the pathogenic strain of Staphylococcus aureus VT-2003R at a dose of 1 × 10 ¹⁰ bacterial cells per mouse. 2 hours after infection, mice were injected intravenously with enzymesosomes at a dose of 1000 μg / mouse.

Group 3 (10 mice) - mice were injected into the retroorbital sinus with bacteria of the pathogenic strain of Staphylococcus aureus VT-2003R at a dose of 1 × 10 ¹⁰ bacterial cells per mouse. Phosphate buffer was administered intravenously 2 hours after infection.

The survival rate of animals was evaluated 32 hours after infection.

The results are shown in table 4.

The survival of mice at different times after infection:

Table 4 0 h 2 h 4 h 6 h 8 h 12 h 24 h 28 h 32 h Group 1 one hundred% one hundred% one hundred% 80% 70% 60% 60% fifty% 40% Group 2 one hundred% one hundred% 70% 70% fifty% 40% thirty% twenty% twenty% Group 3 one hundred% one hundred% 70% fifty% 40% thirty% twenty% 10% 10%

Group 4 (10 mice) - mice were injected intravenously with fungi subcultured from a pathogenic clinical isolate of Candida Albicans at a dose of LD50. On the third day after infection, 300 μg / mouse anti-DNA antibodies were intravenously administered to mice.

Group 5 (10 mice) - mice were injected intravenously with fungi subcultured from a pathogenic clinical isolate of Candida Albicans at a dose of LD50. Enzyosomes were administered intravenously to mice at a dose of 1000 μg / mouse 3 days after infection.

Group 6 (10 mice) - mice were injected intravenously with fungi subcultured from a pathogenic clinical isolate of Candida Albicans at a dose of LD50. As a negative control, phosphate buffer was administered intravenously 3 days after infection.

The survival and weight of the mice were evaluated on day 7 after infection.

The results are shown in table 5.

The survival of mice at different times after infection:

Table 5 1 day 3 day 5 day 7 day Group 4 one hundred% 90% 90% 90% Group 5 one hundred% 80% 80% 80% Group 6 one hundred% 80% fifty% fifty%

Thus, the binding and modification of the extracellular DNA of the blood of infected animals has a therapeutic effect in both bacterial and fungal infections.

Example 5. Treatment of an autoimmune disease.

30 C57B1 mice were immunized with a suspension of Mycobacterium Smegmatis (100 μg antigen in 50 μl aluminum alum) subcutaneously in the paw pad. After 4 weeks, a resolving dose of antigen (50 μg) was injected into the mice of the opposite paw.

The mice of the first group (10 mice) were injected anti-DNA antibodies intravenously at a dose of 200 μg per mouse 30 minutes before the resolution dose.

Mice of the second group (10 mice) 30 minutes before the administration of the resolving dose were given intravenous enzymes at a dose of 750 μg per mouse.

Mice in the control group (10 mice) were injected with phosphate buffer 30 minutes before the resolution dose.

The intensity of paw edema was evaluated at 1, 2, 5, and 24 hours after the administration of the resolving dose of antigen.

The results are shown in table 6.

The intensity of paw edema at different times after the introduction of a resolving dose of antigen.

Table 6 In 30 minutes 1 hour 2 hours 5 o'clock 24 hours The control 2.1 3.6 3,7 4.1 4.2 Group 1 2.1 2,8 3.0 2.9 2.9 Group 2 2.1 3.0 3,1 3.4 3.0

Thus, the binding and modification of extracellular blood DNA has an inhibitory effect on the development of a delayed-type hypersensitivity reaction.

Example 6. Treatment of autoimmune diabetes and malignant tumors.

In the experiment, 20 female NOD mice and 20 female C3H mice were used.

Diabetes in NOD mice occurs due to the development of autoimmune damage to pancreatic b cells. Mice of the first group (10 females of the NOD line) received an intravenous injection of a fraction of mouse anti-G-f actin antibodies (Calbiochem) at 200 μg per mouse at the age of 6, 7, 8, 9, and 10 weeks. 10 mice of the control third group received injections of phosphate buffer from 6 to 10 weeks. Starting from week 15, the level of glucose in the blood of mice was measured every three days. If the glucose level exceeded 250 mg / dl in two subsequent measurements, diabetes was detected. Estimated the number of cases at 15, 18, 24 and 28 weeks of mice.

The results are shown in table 7.

The ratio of healthy and sick mice (The first digit is the number of healthy animals in the group; the second digit is the number of sick animals in the group):

Table 7 15 week 18 week 24 week 28 week Group 1 9/1 8/2 6/4 6/4 Group 2 7/3 5/5 3/7 3/7

Tumors were induced by intradermal injection of 3-methylcholanthrene (1 mg of 3-methylcholanthrene dissolved in 50 μl of olive oil per mouse) at 4 weeks of age. The number of mice with developing tumors was estimated at 10 weeks after carcinogen administration.

Mice of the third group (10 females of the C3H line) received intravenous injections of a 200 μg mouse anti-G-f actin antibody fraction per mouse at 5, 6, 7, 8, 9, and 10 weeks old.

Mice of the fourth group (10 females of the SZN line) received intravenous injections of phosphate buffer at the age of 5, 6, 7, 8, 9, and 10 weeks.

The presence of tumors in animals at the age of 14 weeks was determined. The results are shown in table 8.

The ratio of healthy and sick mice (The first digit is the number of healthy animals in the group; the second digit is the number of sick animals in the group):

Table 8 14 week Group 3 2/8 Group 4 4/6

Thus, suppressing the activity of intrinsic inhibitors of endogenous DNase I has a therapeutic effect in the development of autoimmune diabetes and cancer.

Example 7. Suppression of the spread of a mutant gene. A number of human diseases arise due to the development of the state of somatic mosaicism - expansion of a mutant gene in a population of somatic cells (Youssoufian H, Pyeritz RE. Mechanisms and Consequences of Somatic Mosaicism in Humans. Nature Reviews Genetics 2002; 3: 748-758).

As a model for the development of somatic mosaicism, the mutation frequency of the HPRT gene in blood T-lymphocytes was studied. The human HPRT gene (Chromosome Xq26) encodes a constitutively expressed but not essential enzyme involved in the metabolism of purine bases. Cloning was performed according to the method described by Bigbee W (Bigbee W. Et al., Mutation Res., 1998, v.397, pp. 119-136). The peripheral blood lymphocytes were cloned in 8 patients who received a course of three-week immunostimulating therapy with Neovir after surgical removal of the tumor. Of 8 patients, 4 patients additionally received human recombinant DNase I (Genetech) therapy (200 μg / kg intravenously, 4 times a day for 3 weeks). The frequency of occurrence of HPRT-deficient clones in the blood of patients receiving DNase I therapy was on average 3 times lower than that in the blood of patients receiving only immunostimulating therapy. The addition of extracellular DNA from the blood of patients who did not receive DNase into the culture medium during the cloning of T-lymphocytes of patients treated with DNase increases the frequency of occurrence of HPRT-deficient clones during cloning of the latter. Pre-incubation of extracellular DNA of blood of patients who did not receive DNase with anti-DNA antibodies or with enzymes (0.1 μg of antibodies or 5 μg of enzymes per 0.1 μg of DNA in 1 ml of plasma for 30 minutes at 37 ° C), before being added to the culture medium when cloned, deprives her of the ability to increase the frequency of occurrence of HPRT-deficient clones.

Thus, the binding and modification of extracellular blood DNA reduces the frequency of the mutant gene in the cell population and prevents the development of somatic mosaicism.

Example 8. The treatment of the disease of Markiafava-Mikeli

Markiafava disease - Mikeli is a very rare disease associated with the presence of a somatic gene mutation at the PI gene locus (phosphatidyl glycan class A). Patient O., 17 years old, suffers from this disease for 3 years. Over the past 2 years, the disease has been able to compensate for the use of glucocorticosteroid hormones. Over the past year, the symptoms of the disease reappeared and began to intensify: episodes of hemolysis (2-3 times a month), hemoglobinuria, hepatosplenomegaly, macrocytosis, anisocytosis. 4 blood transfusions were performed. Four months ago, the patient developed an episode of acute renal failure (creatinine - 8, 2 mg / dl) due to an intense episode of intravascular hemolysis against a background of purulent tonsillitis. Within a week, the patient underwent hemodialysis procedures. After compensating for kidney function, with the patient's consent, she was prescribed weekly infusions of human donor DNA-binding antibodies isolated in patients with systemic lupus erythematosus in a single dose of 500 mg (1, 2, 3 and 4 weeks). During this month, there was only one disease paroxysm (2 weeks) of significantly lower intensity than the previous one. The crisis was easily stopped by a three-day course of prednisone at a dose of 50 mg per day. At week 5, the patient was prescribed daily single intramuscular injections of DNase I at a dose of 2,000,000 units. Kunza per day. Over the next three months of observation, the patient returned to normal blood count, jaundice and hepatosplenomegaly disappeared. Paroxysms of the disease were not repeated (figure 1).

Example 9. Treatment of diabetes

The study included 2 patients (Patient Sh. And Patient I.) with severe insulin-dependent diabetes mellitus, with a high daily requirement for insulin and a lack of adequate glycemic control, which manifested itself in frequent episodes of hyperglycemia. Patient III noted complaints of pain behind the sternum, salivation, belching and heartburn, which did not respond to standard antacid therapy (soars 0.01 g / day). When fibrogastroduodenoscopy revealed candidiasis of the distal esophagus.

Patients were injected with an immunoglobulin preparation obtained by fractionating the plasma of healthy volunteer donors 3 times previously immunized with calf thymus DNA. The drug was administered intravenously 1 time per week in the amount of 1000 mg. A total of 4 injections of the drug were carried out. The daily insulin requirement was calculated (as an indicator of the activity of the underlying disease) and the number of weekly episodes of hyperglycemia (blood glucose level was monitored by the instrument method 5 times a day).

The results of the study are shown in table 9.

The effect of anti-DNA antibody treatment on the course of insulin-dependent diabetes mellitus.

Table 9 Before treatment In 2 weeks In 3 weeks After 4 weeks Episodes of hyperglycemia (per week) W 17 9 6 6 AND 10 7 5 5 Insulin requirement U / kg body weight W 1.91 1,63 1.31 1.15 AND 1.55 1.42 1.21 0.9 Extracellular DNA DNA content; ng \ ml W 195 66 45 57 AND 98 73 55 22

By the end of the study, patient III noted the complete disappearance of complaints of dyspeptic phenomena. With repeated fibrogastroscopy, no signs of esophageal candidiasis were detected.

Example 10. Treatment of a malignant tumor.

In January 2004, in a clinic for thoracic surgery, two patients (a man aged 57 years old and a woman aged 55 years old) with a diagnosis of lung cancer in the T4N2M + stage underwent palliative surgery to remove the affected lung. All patients previously received chemotherapy and radiation treatment. After surgery, patients with their consent underwent a procedure for the mobilization of peripheral blood stem cells (GM-CSF of 5 μg / kg subcutaneously three times within 3 days), followed by stem cell isolation by cytapheresis on a Haemonetic apparatus. The isolated cells were transfected with cDNA of the human dornase-alpha gene (Deoxyribonuclease I) by cationic liposomes and 50,000,000 cells were injected intravenously. The procedure was repeated after 3, 6 and 9 months. To date (observation period -14 months, follow-up examinations every 3 months), none of the observed patients showed signs of disease progression. At the same time, the data of retrospective control indicate that the likelihood of developing a relapse by this time and in such patients is approaching 100%. The drawing shows information about the content of extracellular DNA of the blood of patients before treatment and during treatment by the present method (figure 2).

Example 11. The treatment of malaria

Patient D., 49 years old, was admitted to the hospital on the 20th day from the onset of the disease with complaints of fever up to 40-41 ° C, tremendous chills in the morning and afternoon, repeated after 48 hours, lasting 2.5-3 hours, changing to fever for 4 hours, without sweating, weakness, intense diffuse headache, poor appetite, intermittent sleep. 2 months ago I came from India, where I spent my vacation. Microscopy revealed Plasmodium Vivax (3-5 in the field of view). The patient was prescribed Delagil at a course dose of 2.5 g and Primakvin at 0.015 g per day at a course dose of 0.2 g. On the fourth day from the start of treatment with microscopy, Plasmodium Vivax remained in the blood, fever attacks and hepatosplenomegaly persisted. With the patient’s consent, she received intradermal injections of DNA from a calf thymus mixed with Freund’s incomplete adjuvant (50 mg / 50 mg). Only 3 injections with an interval of 48 hours. Symptomatic treatment was carried out for 2 weeks. After 2 weeks, a repeated course of Delagil was prescribed, at the end of which there was a sanation of blood from the parasite, the disappearance of fever attacks and normalization of well-being.

The table shows information about the content of extracellular DNA of the patient’s blood and the titer of anti-DNA antibodies in the course of treatment.

(Day 0 - upon admission to the hospital)

Table 10 Days from the start of treatment
in blood DNA ng \ ml 0 four 8 12 fourteen eighteen 22 26 thirty 117 123 155 138 73 46 12 7 5 Anti-DNA antibody titer (1:50 dilution) 0.113 0.124 0.354 0.614 1,534 2,211 2,655 2,644 2,520

Example 12. The treatment of sepsis.

A 32-year-old patient was admitted to the hospital 80 hours after the onset of the disease with a diagnosis of acute appendicitis. On examination, the condition is serious, inhibited. The skin and mucous membranes are pale. Respiratory rate 25 per minute. Pulse - 142 beats. per minute, weak filling, irregular. CVP is negative. HELL 70/50 mm Hg Heart sounds are deaf. The abdomen is uniformly swollen, does not participate in the act of breathing. Positive symptoms of peritoneal irritation, intestinal motility are absent. Diuresis is sharply reduced. In blood tests, toxic changes. The patient was operated on for emergency reasons. When opening the abdominal cavity - gangrenous, perforated appendicitis, diffuse purulent peritonitis. Appenectomy, debridement and drainage of the abdominal cavity, nasogastrointestinal intubation were performed. In the postoperative period, an infectious toxic shock developed. The patient started antibacterial therapy: cefepime 100 mg / kg / day iv, vancomycin 60 mg / kg / day iv, ofloxacin 20 mg / kg / day iv. Since the nature of the changes in the abdominal region did not preclude the presence of an aerobic-anaerobic association of pathogens, iv administration of metronidazole at a dose of 22.5 mg / kg / day was started.

Despite the treatment, the patient's condition continued to deteriorate, intoxication and respiratory failure persisted and increased; hyperthermia, azotemia.

Given the severity of the patient’s condition and the lack of response to antibiotic therapy, it was decided to carry out hemosorption using a sorbent containing an immobilized enzyme methylase. 18 hours after surgery, 6 hemosorption was performed with an interval of 6 hours. The patient’s condition after the first hemosorption improved slightly. The phenomena of encephalopathy disappeared, body temperature decreased to 37.3 C, tachycardia, respiratory rate decreased, and flaccid peristalsis appeared. In blood tests, leukocytosis with a neutrophilic shift to the left, hypoproteinemia with hypoalbuminemia, persisted. A significant decrease in the level of urea was noted.

After repeated procedures, the patient's condition improved. Hemodynamics stabilized. After the 3rd hemosorption, active peristalsis appeared, there was a stool. Normalized diuresis. A gradual normalization of the general analysis of blood and urea was noted, and an increase in the concentration of total protein and albumin in blood plasma was also noted. The behavior of complex therapy according to the described scheme led to a rapid involution of the inflammatory process in the abdominal cavity, restoration of the functions of parenchymal organs and homeostasis. 3 days after the start of treatment, the patient in satisfactory condition was transferred to the surgical department.

On the 20th day I was discharged for outpatient treatment

The level of methylation of extracellular blood DNA was measured according to the method J. Worm (In-Tube DNA Methylation Profiling by Fluorescence Melting Curve Analysis Clinical Chemistry 47: 1183-1189, 2001).

The results are presented in figure 3.

A significantly higher level of methylation of extracellular blood DNA is detected after the start of treatment according to the claimed method.

Example 13. The treatment of atherosclerosis

Patient A., 32 years old, with a diagnosis of hereditary hypercholesterolemia, suffered myocardial infarction at 24 years old, suffers from angina pectoris of 2-3 functional class, is in disability. Against the background of a diet, taking 40 mg of lovastatin and cholestyramine, the level of total cholesterol is 450 mg%. The content of extracellular blood DNA is 64 ng / ml. According to VEM, the test is positive, depression of the ST segment. According to coronary angiography in 2 coronary arteries 3 stenosis 60, 60 and 70%. The patient began to administer an immunoglobulin preparation obtained by fractionating the plasma of healthy volunteer donors 3 times previously immunized with calf thymus DNA. The drug was administered intravenously 1 time per week in the amount of 1000 mg. A total of 20 injections of the drug were made. By the time the treatment was completed according to the claimed method, xanthom regression was noted, there were no episodes of angina pectoris. The level of total cholesterol is about 160 mg%, the content of extracellular blood DNA is 12 ng / ml. According to bicycle ergometry, the test is negative, there is no depression of the ST segment. According to angiography, a decrease in the degree of stenosis of the coronary arteries (40, 40 and 30%) and the absence of new stenoses were noted. The patient's condition is satisfactory.

Example 14. Treatment of systemic lupus erythematosus

The study included 4 patients with an established diagnosis of systemic lupus erythematosus and laboratory symptoms of glomerulonephritis (proteinuria, microhematuria). All patients received standard therapy (non-steroidal anti-inflammatory drugs, chloroquine and daily drip infusions of 6% DEAE-dextran solution (400 ml of 6% solution) for 15 days. We studied the concentration of DNA in the blood plasma before and after treatment. Patients were evaluated. according to the SLAM (Sustemic Lupus Activity Measure) scale. The plasma DNA content in patients decreased by 50% at the end of the 15-day course of treatment. The disease activity in 4 control patients who received only standard therapy decreased by 20% (average value about the beginning of therapy - 9.7; after the end of therapy - 7.2). The disease activity in patients receiving DEAE-dextran therapy decreased by 40% (the average value before therapy was 9.2; after the end of therapy - 5.3 )

Claims (5)

1. A method for the treatment of malignant tumors or infections caused by bacteria, fungi and protozoa, or atherosclerosis, or diabetes mellitus, or diseases associated with a delayed-type hypersensitivity reaction, or diseases developing due to mutations in somatic cell genes, characterized in that blood is introduced into the blood extracellular blood DNA binding agent. 2. A method for the treatment of malignant tumors or infections caused by bacteria, fungi and protozoa, or atherosclerosis, or diabetes mellitus, or diseases associated with a delayed-type hypersensitivity reaction, or diseases developing due to mutations in somatic cell genes, characterized in that they are introduced into the blood an enzyme that changes the chemical structure of extracellular blood DNA. 3. A method of treating malignant tumors or infections caused by bacteria, fungi and protozoa, or atherosclerosis, or diabetes mellitus, or diseases associated with a delayed-type hypersensitivity reaction, or diseases developing due to mutations in somatic cell genes, characterized in that they are introduced into the blood an agent that stimulates the synthesis or activity of endogenous deoxyribonuclease, or an agent that stimulates the synthesis of antibodies that bind extracellular blood DNA. Priority on points: 07/14/2003 according to claims 1-2; 03/12/2004 according to claim 3.

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