RU2200327C2 - Method for diagnostics of syphilis (variants) - Google Patents

Abstract

FIELD: medicine, microbiology. SUBSTANCE: the present method could be carried out due to either immunoenzymatic or quantitative immunofluorescence assays by using ultrasound affinitypurified polyvalent treponemal antigen incubated with serum under testing. The method is characterized by application of solid-phase carrier, particularly, modified with polyglukin of composed alumosilicate magnoimmunosorbent. The suggested variants of the above- mentioned method enable to increase sensitivity and specificity of diagnostics, shorten terms and labor intensity of the assay. EFFECT: higher accuracy of diagnostics. 2 cl

Description

 The invention relates to microbiological research methods and can be used in the diagnosis of syphilis by enzyme-linked immunosorbent assay (ELISA) and quantitative enzyme-linked immunosorbent assay (KIFA).

 The complexity of the diagnosis of syphilis is due to the properties of the pathogen - spirochete Treponema pallidum, which is poorly cultured on nutrient media in vitro and not stained by microscopy. Currently, a number of methods have been developed for identifying the infection process at different stages. Existing laboratory tests can be divided into several groups: direct visualization of pale treponemas in the presence of lesions; nontreponemal tests used for screening; treponemal confirmatory tests.

 With direct visualization of microorganisms and complement binding reactions (CSCs) using cardiolipin as antigen, false-negative and false-positive results are often observed, especially in the presence of adverse infectious diseases.

 Recently, the ELISA method with the use of both pathogenic and non-pathogenic treponemas as antigens has been actively introduced into the diagnosis of syphilis. Known commercial ELISA test systems of foreign and domestic production with a set of materials and reagents necessary for the formulation of the reaction, which is carried out in two versions automatically and visually. The test results of these test systems at various stages and forms of the disease showed significant opportunities for increasing the sensitivity and specificity of the diagnosis of syphilis (G.A.Dmigrisv, E.E. Bragin, Modern methods of laboratory diagnosis of syphilis. Herald of dermatology and venereology, 2, 1996, p. 29-30, ibid., 3, 1996, pp. 33-34).

 However, with various forms of the disease, the sensitivity and specificity of the methods are ambiguous, the differentiation of antibodies with a number of autoimmune diseases is problematic.

 The sensitivity and specificity of ELISA are determined not only by the degree of purity of the ingredients used, but also by the properties of the solid phase, which should preserve the immunological properties and stability of immobilized ligands, have minimal ability to bind non-specifically the components of the analyzed system, and be convenient for phase separation.

 When using the most widespread polystyrene microplates as an immunosorbent, problems arise with their insufficient sorption ability or the presence of eluting unbound antibodies (antigens), leading to a decrease in the specificity and sensitivity of the method.

 The sensitivity of immunoassay is also determined by the purity and activity of the antigens (AH) and antibodies (AT) used. (Enzyme-linked immunosorbent assay: current status and development trends. Overview. The series "Medical genetics and immunology" V.I. Pokrovsky et al., Issue 3, M., 1986, S. 4-5).

 There is a known method for the diagnosis of syphilis by the immunofluorescence method, according to which, in order to increase the sensitivity of the method in cases of congenital disease, in case of seroresistant forms, an ultrasonically treponemal antigen is applied as a sorbent on a glass slide, and immunoglobulin M. is isolated from the test serum (Muller F., Immun. Infeet. 1977, p. 109-113).

 The method is not reliable enough with a low content of antitreponemal antibodies in the blood serum, as well as insufficiently expressed.

 As a result of the establishment of the fact that sensitization of peripheral blood neutrophils to treponemal antigen causes pronounced changes in the cell surface and intracellular structures, tested signs of neutrophil damage when exposed to ultra-voiced pale treponema for differential diagnosis of diseases at an early stage are proposed (A.S. 833206, A 61 B 10/00, G 01 N 38/16, dated 30.05.81, Bull. 20).

 The application of this method in clinical laboratories during mass screening is quite difficult.

 When detecting small amounts of pathogenic microorganisms in the studied materials, the method of selective sorption of microbes on an immunosorbent is used, followed by their immunofluorescence and enzyme immunoassay. Immunosorbents are prepared by the following methods: physical adsorption of AH or AT on red blood cells, cellulose particles, sepharose, etc .; chemical reactions of the addition of protein AT molecules, polysaccharide-protein AG molecules to solid phase sorbents; polycondensation of protein AT molecules or protein, lipopolysaccharide AG molecules using glutaraldehyde, ethyl chloroformate, borofluoride, rhodaminisothiocyanate B, diazolyl black C and others, substances (V.M. Nikitin, Handbook of immunological methods, Chisinau, 1982, pp. 233-235) .

 Of interest is the method of selective concentration of microorganisms on the surface of magnetic immunosorbents (MIS), which is intensively developing in the field of epidemiological monitoring of environmental objects. This solves the problem of identifying the causative agent of infection at a low concentration in the test material. Devices and devices have been developed for manipulating MIS, starting with the collection, transportation, storage of samples, transferring MIS, to carry out an immunological reaction (RF Patent 2098828, G 01 N 33/553, C 12 M 1/00, dated 10.12.97, Bull . 34).

 An enzyme-linked immunosorbent diagnostic test system for the detection of hepatitis A virus using as a solid carrier of magnetosorbents sensitized with antihepatitis (A) immunoglobulins (RF Patent 2065164, G 01 N 33/53, from 10.08.96, Bull. 22).

 The advantages of this test system compared to the traditional ELISA method are the ability to detect the presence of the virus during its discrete entry and low concentration, selectively concentrate viruses directly from the secretions of patients or other contaminated samples and reduce the analysis time from 4 to 1 hour due to the phased transfer of MIS .

 Constraining factors for the use of MIS in diagnostic test systems are the technological difficulties of their production.

 Known methods for epidemiological monitoring and diagnosis of hepatitis A virus use MIS based on polyacrylamide granules, which are obtained by emulsion polymerization of a mixture of polyacrylamide comonomers and a catalyst with magnetic powder, followed by activation of the surface of the magnetosorbents with glutaraldehyde for 18-20 hours and treatment with an albumin solution for 1 -3 hours (RF Patent 2068703, A 61 K 39/395, C 12 N 11/00 // G 01 N 33/53, dated 10.11.96, Bull. 31).

 The duration and multi-stage process using expensive imported toxic reagents inhibits the organization of IIA production. In addition, glutaraldehyde is hydrolyzed in an aqueous medium, which leads to nonspecific sorption and a decrease in stability in biospecific processes.

 A known method of producing an immunosorbent in which a silochrome is used as a carrier is treated with aminopropyltriethoxysilane and activated with n-benzoquinone, followed by immobilization of the aminoacylase and an additional stabilizing treatment with glyoxal solution. A.S. USSR 1060676, C 12 N 11/14; C 12 N 9/78, dated 12.15.83, Bull. 46).

 The method does not provide for immunosorbent with magnetic properties.

 Closest to the claimed method is an enzyme-linked immunosorbent assay system for detecting antibodies to the causative agent of syphilis in human serum (Ovchinnikov N.M., Bednova V.N., Delektorsky V.V. Laboratory diagnosis of sexually transmitted diseases. - M., 1987 .-- 303 p.).

Diagnostic test system is as follows. The test serum is added to the wells of a polystyrene plate sensitized with an ultra-sonic antigen from pathogenic pale treponema, in parallel control solutions and inhibited for 30 minutes at 37 ^° C, washed, the enzyme anti-species conjugate is introduced and the mixture is kept in an incubator for 30 minutes, the wells are washed and introduced the substrate is an indicator reagent, the tablet is incubated for 1 hour at room temperature in a darkened place. The reaction results are taken into account by changing the color of the substrate mixture.

 The advantages of the prototype diagnostic test system are manifested in an increase in its sensitivity due to an enzyme conjugate capable of detecting in the blood serum of patients with syphilis antibodies to Pallidum Teronema, which affinity interact with highly specific cell structures of treponemal antigen adsorbed on the surface of a polystyrene tablet.

 However, the immunosorbent, which is an antigen-sensitized polystyrene tablet, does not have a sorption capacity sufficient for reliable indication of microorganisms in small quantities. In addition, an increased concentration of immunoglobulins in the solid phase leads to the adsorption of freely bound antibodies, which elute in the subsequent stages of incubation and washing and thereby reduce the sensitivity and specificity of diagnosis. The sorption process is reversible, therefore, antigen-sensitized tablets are not subject to long-term storage (their shelf life is 20 days in the cold under sealing conditions).

 ELISA test system does not provide sufficient diagnostic rapidity necessary for mass examinations. The duration of the analysis, excluding preparatory measures, is more than 2 hours.

 The aim of the invention is to increase the sensitivity and specificity of diagnosis at all stages of syphilis, ensuring the reliability of detection of infection with a low content of antibodies in the test serum of the patient, reducing analysis time and reducing its complexity.

 The goal is achieved in two ways: IFA and KIFA. According to the first option, ELISA involves sensitization of a solid-phase carrier by an ultra-sonic affinity-purified multivalent treponemal antigen, its incubation with test serum, and then with peroxidase monoclonal antispecies immunoglobulins, followed by application of a substrate-indicator reagent and intermittent washing of the carrier with the transfer of the medium and by transferring the medium to a separate transfer of the carrier .

 According to the second option, KIFA includes sensitization of a solid-phase carrier by an ultra-sonicated affinity-purified multivalent treponemal antigen, its incubation with the test serum, and then with immunoglobulins luminescent against human globulins, and intermediate washing of the carrier during phased transfer of the solid-phase carrier.

 In relation to the prototype of the inventive diagnostic method, according to the first embodiment, has the following distinctive features. The use of magnetic immunosorbents sensitized with treponemal antigen as a solid-phase carrier provides selective concentration of anti-infection antibodies on them, including at their low concentration in the test material.

 The choice of organosilicon sorbent - aluminosilicate with a loose structure and a well-developed surface provides a fairly stable incorporation of magnetic particles into the sorbent structure and a large reaction surface and sorption capacity during gel formation with dextran. Together with the use for immobilization of a highly specific treponemal antigen and conjugate of immunoperoxidase monoclonal against human globulins for the formation of the immune complex, the proposed solid-phase carriers provide increased reliability, sensitivity and specificity of diagnosis. The possibility of phased transfer of the solid-phase carrier into the test material, conjugating and substrate reagents, in the washing solutions due to their magnetic properties, reduces the analysis time and reduces the complexity.

 In addition, the composite magnetic immunosorbents (KIIS) used during their freeze drying are much more stable in storage than polystyrene tablets.

The method of obtaining KIIS consists in the following: a mixture consisting of 2.5 g of aluminosilicate filler and 0.5 g of magnetic powder was suspended in 40 ml of a 0.2-0.4% aqueous solution of polyglucin and then kept at room temperature for one hour . The resulting sorbent was dried at 100-110 ^o C for 30 minutes. To one gram of the resulting preparation was added 12 ml of a 23% sodium chloride solution and 1 ml of secondary sodium alkyl sulfate. The mixture was incubated for 1-2 hours at a temperature of 37 ^o C, then the sorbent was washed with 100 ml of 0.9% sodium chloride solution and 100 ml of distilled water. To 0.1 g of activated sorbent was added 1 ml of UZTA with a protein content of 3.5 mg / ml. The mixture was left at 37 ^{° C.} for one hour. Next, the supernatant was removed, and the carrier was washed with 0.9% sodium chloride solution to “0” extinction on a spectrophotometer. Magnoimmunosorbents were lyophilized.

 The obtained composite aluminosilicate magnetoimmunosorbents were highly dispersed irregularly shaped microspheres with pronounced magnetic properties, with good wettability and effective sedimentation in solution, and lack of tendency to conglomeration. Sorbents had granule sizes from 20 to 100 microns. The average value of their specific surface is 117 m / g, the average pore radius is 35 nm, and the pore volume is 1.7 cm / g.

A method for diagnosing syphilis is carried out as follows: according to the first embodiment, 0.1 ml of a 10% suspension of Trep-KMIS is added to vials (such as penicillin). Why 0.2 ml of test sera were added to the test bottles, 0.2 ml of phosphate-buffered saline (FSB) to the bottles with the negative control, and 0.2 ml of the positive reacting serum to the bottles with the positive control. After 20-30 min of incubation at a temperature of 37 ^o C after thorough washing of the sorbent granules with a permanent magnet, 0.2 ml of immunoperoxidase monoclonal conjugate against human globulins in working dilution was added to all bottles (experimental and control). After 20-30 minutes after washing the granules, 0.2 ml of substrate-indicator solution was added to the vials (10 ml of orthophenylenediamine and 40 μl of 33% hydrogen peroxide per 10 ml of citrate buffer solution). The reaction was stopped by adding 0.05 ml of 2M sulfuric acid to the vials. Analysis was carried out visually after 1-5 minutes. With a positive result, an orange-brown staining occurred, with a negative solution of the reaction ingredients remained colorless. To take into account the results on a Multiskap scanning device, the contents of the vials after stopping the reaction were transferred to microplates and the readings were taken at 492 nm. Samples were considered positive, the color indices of which were 1.5 times or more higher than the control ones.

 Thus, in contact with specific antibodies, magneto-immunosorbents carried out their dynamic, selective concentration, forming an immune complex, which is further determined by the peroxidase reaction.

 A comparative assessment of the effectiveness and sensitivity of the developed test system was carried out with 539 blood serums of patients with various forms of syphilis: before treatment, during and after treatment. Trep-KIIS with serodiagnosis of syphilis in ELISA is 0.9% higher in the complete discrepancy between the results and 2.3% in the degree of positivity of the test compared to the ultra-sonic treponemal antigen in the complement binding reaction (CSC). Including, with primary seronegative syphilis, the complete discrepancy between the results in favor of Trep-KIIS was 8.3% of cases, and with primary seropositive syphilis - 1.8% of cases.

 In the study of 230 sera of patients with syphilis during and at the end of treatment, it was found that the test positiveness when using Trep-KIIS in ELISA is higher by 4.3% of cases compared with CSC and 1.7% higher by a complete discrepancy of results.

 The control group was the serum of 209 individuals free of syphilitic infection. The specificity of the test was found to be 99.7%, while the test sera in RSCs with USTA were specific in 99.2% of cases.

The method for the diagnosis of syphilis according to the second variant (CIFA) in vials (such as penicillin) was introduced into 0.1 ml of 10% suspension Trep-KMIS. Then, 0.2 ml of the tested sera were added to the test bottles, 0.2 ml of phosphate-buffered saline (FSB) to the bottles with the negative control and 0.2 ml of the positively reacting serum to the bottles with the positive control. After 20-30 minutes of incubation at a temperature of 37 ^° C after thorough washing of the sorbent granules with a permanent magnet, 0.2 ml of immunoglobulins luminescent against human globulins were introduced into all bottles (experimental and control). They were incubated for 30 minutes, washed with PBS three times and once in distilled water, the contents of the vials were transferred to glass and the results were recorded.

 Quantitative accounting of the fluorescence intensity of granules of magnetic sorbents was carried out using a luminescent microscope with a photometric nozzle. The difference between the luminescence of the granules and the background, determined using a probe sequentially directed to the sorbent granules, and the gap between them were expressed in relative units and were taken as a value characterizing the intensity of fluorescence of the granules. More than two times the difference in the fluorescence intensity of granules of magnetic sorbents and control samples was considered a positive result.

 Thus, the advantages of the proposed diagnostic method in comparison with commercial test systems for the diagnosis of syphilis are manifested in an increase in sensitivity by 1.5-1.7%, specificity by 0.4-0.6%. Analysis time reduced from 2 to 1 hour. Used KIIS will organize the release of highly sensitive and specific test systems for the diagnosis of syphilis by ELISA and KIFA methods.

Claims (2)

 1. A method for the diagnosis of syphilis by enzyme-linked immunosorbent assay (ELISA), which includes sensitization of a solid-phase carrier by an ultra-sounding affinity-purified multivalent treponemal antigen, its incubation with the test serum, and then with antispecies monoclonal immunoglobulins peroxidase, the application of substrate-dependent reagent-sensitive reagent reaction results, characterized in that as a solid-phase carrier using a modified polyglucin composition aluminosilicate magnimoimmunosorbent, which is placed in vials where the test serum is added sequentially, conjugating reagent, substrate-indicator solution, while doing intermediate washing of the sorbent granules with a permanent magnet, while samples in which orange-brown staining are considered positive - where the solution remains colorless.  2. A method for the diagnosis of syphilis by the method of quantitative immunofluorescence analysis (CIFA), which includes sensitizing a solid-phase carrier with an ultrasonically purified affinity-purified multivalent treponemal antigen, incubating it with the test serum, and then with luminescent anti-human serum, intermediate washing of the reaction results with subsequent that as a solid-phase carrier, a polyglucin-modified composite aluminosilicate magneto-immunosorbent is used, which is placed in vials, where the test serum, which luminesces anti-human serum, is successively added, intermittently washing the sorbent granules using a permanent magnet, then transfer the contents of the vials to the glass and quantify the fluorescence intensity of the magnetic sorbent granules using a luminescent microscope with a photometric nozzle , while a positive result is considered the difference in the intensity of fluorescence of granules of magnetic sorbents and control samples more than doubled.