RU2429781C1 - Diagnostic technique for remitted genital and urogenital herpetic infection - Google Patents

Abstract

FIELD: medicine. ^ SUBSTANCE: diagnosing immune response failure associating remitted genital and urogenital herpetic infection is ensured by evaluating T-lymphocyte levels in heparinised venous blood of CD4+, CD8+, CD16+ cluster differentiation by laser flow cytofluorimetry. It is combined with cytokine levels: interleukin-2, tumour necrosis factor-alpha, alpha interferon, gamma interferon of venous blood plasma. ^ EFFECT: method enables evaluating immunopathogenic mechanisms of remitted genital and urogenital herpetic infection. ^ 2 ex

Description

The invention relates to medicine, namely to the diagnosis of the characteristics of the immunological response in cases of herpetic infection of the genitals and urogenital tract in remission.

The main feature of herpesvirus infections is their tendency to a chronic course with periods of exacerbation and remission, the immune-mediated pathogenesis of the disease.

A known method for the diagnosis of genital herpes and immunological disorders, including the following laboratory examinations: a clinical analysis of urine, a microscopic examination of unpainted preparations, a study of smears stained by Gram, the selection and identification of viruses in blood and saliva, the determination of antibodies against HIV antigens, lymphotoxic test with B-lymphocytes, determination of antibodies to normal tissue species, other immunofluorescence methods, clinical blood test, determination of T-suppressor in / killer cells with monoclonal antibodies in lymphocytotoxic test, determining the ratio of T-lymphocyte subpopulations, identification ratios of large and small lymphocytes (1).

The disadvantage of this method is the high economic cost of the examination, due, inter alia, to the need for 2-, 3-fold implementation of laborious methods that do not fully disclose the main immunopathogenetic mechanisms of the patient's response. There is no indication of differentiated treatment.

A known diagnostic method for herpes, including microbiological examination of the material, detection and isolation of herpes simplex virus, direct immunofluorescence of smears for herpes simplex virus, determination of antibodies to herpes simplex virus in the reaction of indirect immunofluorescence, enzyme immunoassay for determination of antibodies to herpes simplex virus, determination interferon alpha-1, beta-1 blood serum, clinical blood test, determination of the number of T-lymphocytes, B-lymphocytes, subpopulations of T-lymphocytes comrade (2).

The disadvantage of this method is the high cost of the examination due, including the need for 2-fold conducting high-tech techniques. It also does not take into account that people with a diagnosis are not required to carry out the full volume of recommended laboratory techniques.

A known diagnostic method for herpetic infection, including clinical analysis of urine, the determination of antibodies against HIV antigens, the study of scraping from vesicles on the herpes simplex virus by direct and indirect immunofluorescence, the study of saliva on the herpes simplex virus by direct and indirect immunofluorescence, the determination of antibodies in the reaction of passive hemagglutination , determination of serum immunoglobulins of the main classes (IgA, M, G), determination of the level of immunoglobulin M by enzyme-linked immunosorbent assay, analysis of clinical study (3).

The disadvantage of this method is the high cost of the examination, not revealing the main pathogenetic mechanisms of the immunological response of the patient's body during the remission of the disease.

This method is taken as a prototype.

The aim of the invention is to reduce economic costs and the disclosure of the immunopathogenetic mechanisms of herpetic infection of the genitals and urogenital tract in remission for the further selection of pathogenetically optimized, individual immunocorrective therapy.

This goal is achieved by the fact that during the period of remission of a herpetic infection of the genitals and genitourinary tract, the patient's blood is taken in the morning, on an empty stomach from the ulnar vein in the treatment room into a test tube with heparin.

The levels of T-lymphocytes with the phenotype of the differentiation cluster CD4 +, CD8 +, CD16 + are determined by laser flow cytofluorimetry. Quantitative determination of interleukin-2 is carried out by the enzyme-linked immunosorbent assay using test systems of the Protein circuit LLC (St. Petersburg), alpha interferon, tumor necrosis factor-alpha by the enzyme immunoassay using reagents of Vector-Best CJSC (Novosibirsk).

Spontaneous and induced gamma-interferon, alpha-interferon of venous blood are also determined. Blood of the patient is taken in the morning, on an empty stomach from the cubital vein in the treatment room in a test tube with heparin. To determine the levels of cytokines (spontaneous and stimulated production), 1 ml of heparinized blood is added to a vial of medium (maintenance medium supplemented with heparin, L-glutamine, gentamicin) in a ratio of 1: 4. Mixed. Pour 1 ml of the mixture into a bottle with PHA (mitogen, 10 μg / ml). Pour 1 ml of the mixture into a bottle with PHA (mitogen, 10 μg / ml). Pour 1 ml of the mixture into a bottle with PHA (mitogen, 10 μg / ml). Pour 1 ml of the mixture into a bottle with PHA (mitogen, 10 μg / ml). Both vials are incubated for a day at 37 ° C. After incubation, the contents of both vials are centrifuged at 3000 G for 10 minutes. The supernatant is collected and the concentration of the desired cytokines is determined in it. A bottle of medium is an indicator of the spontaneous production of the Central Committee. A bottle with PHA is an indicator of the stimulated production of the Central Committee.

Comparison of the proposed method with other methods known in the field of medicine shows compliance with the criteria of the invention.

The inventive method examined 1654 patients.

Example 1

Patient S., 30 years old.

He complained of relapses of genital herpes with localization of rashes in the foreskin. The area of skin lesion is 2-3 cm, the relapse rate is 10-14 times a year, the duration of exacerbation is 7-10 days. Relapse was accompanied by severe paresthesia in the form of “tingling,” “burning,” an increase in inguinal lymph nodes. He considers himself a patient for 5 years, was treated only with an exacerbation of the disease. Used acyclovir tablets and local form (cream "Zovirax"). He came into remission of the disease, which, according to the patient, lasted 3 weeks. Earlier, the etiological role of the herpes simplex virus in the development of the disease was proved by polymerase chain reaction and enzyme immunoassay methods.

Inspection data - general condition is satisfactory. There are no rashes of herpes on the skin of the foreskin. An increase in inguinal lymph nodes up to 1.5 cm, soft-elastic consistency, painless on palpation. The skin over the lymph nodes is not changed. Zev - without signs of inflammation, the tongue is clean. The vesicular breathing, heart tones are clear, rhythmic. Liver at the edge of the costal arch, intestinal palpation painless. Pasternatsky’s symptom is negative. Body temperature 36.5. Physiological administration is normal.

On the eve of treatment, during the period of remission of the disease, an immunological examination was performed. General clinical analysis from venous blood: leukocytes - 3.2 × 10 ³ L, stab neutrophils - 1%, segmented neutrophils - 64%, eosinophils - 4%, monocytes - 11%, lymphocytes - 20%. Cellular immunity (differentiation clusters): CD4 + 32%, CD8 + 20%, CD16 + 10%. Cytokines: interleukin-2 0, alpha interferon 0, alpha interferon spontaneous 0, alpha interferon induced 0, gamma interferon 0, gamma interferon spontaneous 0, gamma interferon induced 1000, tumor necrosis factor 0.

Diagnosed with: Secondary immunodeficiency state of the combined type (cellular with cytokine deficiency). Infectious Syndrome. Chronic recurrent herpetic infection of the genitals and urogenital tract, stage of remission.

Prescribed treatment with an antiviral drug with immunomodulatory effect "Ferrovir", a course of 10 injections. After the treatment, a stable remission was observed for 3 months.

In control blood tests performed 3 months after the end of treatment, there is a positive trend. General clinical blood test: leukocytes - 4.5 × 10 ³ L, stab neutrophils - 0%, segmented neutrophils - 51%, eosinophils - 5%, monocytes - 7%, lymphocytes - 37%. Cellular immunity (differentiation clusters): CD4 + 38%, CD8 + 24%, CD16 + 12%. Cytokines: interleukin-2 10, alpha-interferon 5, alpha-interferon spontaneous 6, alpha-interferon induced 10, gamma-interferon 12.4, gamma-interferon spontaneous 2, gamma-interferon-induced 5, alpha tumor necrosis factor 0.

Example 2

Patient P., 20 years old.

She complained of rashes of herpes on the labia 5-7 times a year, both against the background of provoking factors (hypothermia, stress), and for no apparent reason. Rashes are “migratory” in the inguinal region, an area of about 1 cm, periodically - rash is staged, several localizations. Vesicles appeared on the site of hyperemia, bursting, shrinking into a “crust” with cracks and erosion. The duration of relapse is 5-10 days. Rashes were accompanied by an increase and soreness of the inguinal lymph nodes, an increase in body temperature to subfebrile values. Sick for 2 years. Used in the period of exacerbation "Acyclovir", locally - in the area of rashes "3oviraks". Examined by a dermatologist in exacerbation: positive polymerase chain reaction and specific immunoglobulins of classes M, G (enzyme immunoassay) to the herpes simplex virus.

Came into remission. Inspection data: general condition satisfactory, skin integument of usual color. There are no rashes of herpes on the mucous membranes of the genital organs. The oral cavity is sanitized. Lymph nodes: inguinal enlarged to 1-2 cm, soft-elastic consistency, painless, not fused with surrounding tissues. Vesicular breathing. No wheezing. Heart tones are clear, rhythmic. Body temperature 36.8.

Examination data: general clinical blood test: leukocytes - 3.8 × 10 ³ L, stab neutrophils - 1%, segmented neutrophils - 70%, eosinophils - 5%, monocytes - 6%, lymphocytes - 18%. Cellular immunity (differentiation clusters): CD4 + 22%, CD8 + 20%, CD16 + 19%. Cytokines: interleukin-2 14.2, alpha-interferon 0, alpha-interferon spontaneous 1, alpha-interferon induced 0, gamma-interferon 0, gamma-interferon spontaneous 0, gamma-interferon induced 1000, alpha tumor necrosis factor 0.

Diagnosed with: Secondary immunodeficiency state of the combined type (cellular with cytokine deficiency). Infectious Syndrome. Chronic recurrent herpetic infection of the genitals and urogenital tract, stage of remission.

P. is recommended to carry out immunocorrective and antiviral therapy from the moment the “precursors” of relapse appear: “Famvir” 500 mg, topically to the rash area “Viferon-gel”, 2 weeks after the onset of clinical manifestations of relapse, into the muscle, “Ferrovir”, course 10 injection.

At the next visit, P. said that the treatment was effective: on the first day of the exacerbation, the manifestations of "paresthesia" were stopped, there was no infiltrate, no vesicles, the lymph nodes did not increase, their pain was not. Body temperature did not rise. Remission after treatment was 4 months.

In control analyzes conducted after 3 months, positive dynamics were revealed. General clinical blood test: leukocytes - 4.7 × 10 ³ L, stab neutrophils - 2%, segmented neutrophils - 62%, eosinophils - 3%, monocytes - 8%, lymphocytes - 25%. Cellular immunity (differentiation clusters): CD4 + 40%, CD8 + 25%, CD16 + 10%. Cytokines: interleukin-2 10, alpha interferon 0, alpha interferon spontaneous 0, alpha interferon induced 0, gamma interferon 14.3, gamma interferon spontaneous 10, gamma interferon induced 1000, tumor necrosis factor 5, gamma interferon 0.

Clinical trials have shown that the use of a method for diagnosing disorders of the immunological response in cases of herpetic infection of the genitals and urogenital tract during remission by a combination of laboratory methods for studying T-lymphocyte levels with the phenotype of the differentiation cluster SD4 +, SD8 +, SD16 + by laser flow cytofluorimetry, and interleukin-2 cytokine levels , alpha-interferon, gamma-interferon, alpha-factor of tumor necrosis leads to a refinement of the pathogenetic characteristics of the immunological first line of response for selecting the most appropriate and effective therapies.

The method can be recommended in the practical activities of allergists, immunologists, infectious disease specialists, dermatovenerologists, gynecologists, urologists, outpatient therapists and hospitals.

Information sources

1. Order of the Ministry of Health of the Russian Federation of 08.04.1996 N134 "On temporary industry standards for the volume of medical care" (together with "Methodological recommendations for the use of temporary industry standards for the volume of medical care"). Appendix 1. Code ICD-10: A 60.0.

2. Order of the Ministry of Health of the Russian Federation of 08.04.1996 N134 "On temporary industry standards for the volume of medical care" (together with the "Methodological recommendations for the use of temporary industry standards for the volume of medical care"). Appendix 1. Code ICD-10: B00.

3. Order of the Ministry of Health of the Russian Federation of 08.04.1996 N134 "On temporary industry standards for the volume of medical care" (together with "Methodological recommendations for the use of temporary industry standards for the volume of medical care"). Appendix 1. Code ICD-10: В00.9.

Claims (1)

A method for diagnosing disorders of the immunological response during a herpetic infection of the genitals and urogenital tract, characterized in that during the period of remission of the herpetic infection of the genitals and urogenital tract, the levels of T-lymphocytes of heparinized venous blood with the phenotype of the differentiation cluster CD4 +, CD8 +, CD16 + are determined by laser flow cytometry simultaneous determination of cytokine levels: interleukin-2, tumor necrosis factor alpha, interferon alpha, interferon gamma from venous plasma blood.