ABSTRACT
INTRODUCTION: Following the successful eradication of smallpox, mass vaccination against this disease was discontinued in 1980. The unvaccinated population continues to be at risk of infection due to military use of variola virus or exposure to monkeypox virus in Africa and non-endemic areas. In cases of these diseases, rapid diagnosis is of great importance, since the promptness and effectiveness of therapeutic and quarantine measures depend on it. The aim of work is to develop a kit of reagents for enzyme-linked immunosorbent assay (ELISA) for fast and highly sensitive detection of orthopoxviruses (OPV) in clinical samples. MATERIALS AND METHODS: The efficiency of virus detection was evaluated by single-stage ELISA in the cryolisate of CV-1 cell culture samples infected with vaccinia, cowpox, rabbitpox, and ectromelia viruses, as well as in clinical samples of infected rabbits and mice. RESULTS: The method of rapid ELISA was shown to allow the detection of OPV in crude viral samples in the range of 5.0 1025.0 103 PFU/ml, and in clinical samples with a viral load exceeding 5 103 PFU/ml. CONCLUSIONS: The assay involves a minimum number of operations and can be performed within 45 minutes, which makes it possible to use it in conditions of a high level of biosecurity. Rapid ELISA method was developed using polyclonal antibodies, which significantly simplifies and reduces the cost of manufacturing a diagnostic system.
Subject(s)
Ectromelia virus , Orthopoxvirus , Variola virus , Rabbits , Animals , Mice , Orthopoxvirus/genetics , Vaccinia virus , Variola virus/genetics , Enzyme-Linked Immunosorbent AssayABSTRACT
INTRODUCTION: The abolition of smallpox vaccination has led to the disappearance of population immunity to pox viruses. However, the threat of infection by pathogenic orthopoxviruses persists and determines the need to develop sensitive and operational methods for indicating pathogens. OBJECTIVES: Development of a sensitive, fast and easy-to-use immunochemical test for the detection of orthopoxviruses in the «point of care¼ format. MATERIAL AND METHODS: We used preparations of cultural vaccinia virus (VV) with varying degrees of purification, polyclonal antibodies from hyperimmune rabbit serum, and equipment from a previously developed autonomous kit for dot-immunoassay on flat protein arrays. RESULTS AND DISCUSSION: It has been established that rabbit polyclonal antibodies can be used in a single-stage dotanalysis, both as a capture agent immobilized on a substrate and as a detection reagent bound with colloidal gold particles. It is shown that the effectiveness of the detection of VV is inversely related to the degree of purification of viruses from sub-viral structures. The sensitivity of the rapid detection of viruses in a crude preparation was about 30 times higher than in pure viral material. The increase in sensitivity, presumably, occurs due to binding to the capture antibodies of subviral structures, which form large aggregates of sensitized gold particles. The test does not detect cross-reactions with heterogeneous viruses (measles, rubella and chickenpox) that cause exantematous diseases. CONCLUSION: The one-stage variant of the dot-immunoassay reduces the analysis time to 40 minutes and improves the detection sensitivity of orthopoxviruses in crude viral preparations to the range of 105-104 PFU / ml. Full makeup, ease of analysis and the ability to visually accounting for results allow the test to be used outside of laboratories.
Subject(s)
Antibodies, Viral/blood , Immunoblotting/methods , Immunohistochemistry , Orthopoxvirus/immunology , Poxviridae Infections/diagnosis , Animals , Humans , Orthopoxvirus/isolation & purification , Poxviridae Infections/blood , Poxviridae Infections/immunology , Poxviridae Infections/virology , Rabbits , Reagent Kits, Diagnostic/standards , Sensitivity and Specificity , Smallpox Vaccine/analysis , Time FactorsABSTRACT
The study was targeted to the investigation of possibilities of using in immunological analysis the sols on basis of bivalent cobalt compounds as a catalytic marker to ensure the trusted visual registration of analysis results in immunology reactions plats. The results of comparative evaluation of immune-enzyme and immune catalytic tests on the basis of several commercial diagnostic test systems of various national manufacturers are presented. The conclusion is derived that by the sensitivity and specificity the cobaltferous immunosols are not inferior to immuneperoxidase conjugated metabolites and even have an advantage due to the relative simplicity of immunosol preparation and the possibility of trusted non-instrument registration of results. The application of cobaltferous immunosols permits to develop the diagnostic test systems with trusted visual registration of results following the "yes-no" principle to ensure the immunodiagnostics in poorly equipped laboratories.
