Vol 90, No 3 (2013)
- Year: 2013
- Published: 15.06.2013
- Articles: 20
- URL: https://microbiol.crie.ru/jour/issue/view/159
ANALYSIS OF EXTRACELLULAR PROTEOME OF STAPHYLOCOCCUS AUREUS 6 AT THE END OF EXPONENTIAL GROWTH PHASE
Abstract
Aim. Determine protein specter that Staphylococcus aureus synthesizes and secretes at early growth phase - the exponential phase. Materials and methods. Proteins secreted by S. aureus strain 6 into cultivation medium at the end of exponential growth phase (4.5 hours) were studied. 11 proteins were identified by liquid chromatography - mass-spectrometry method. Results. Only in 3 of these proteins the presence of signal peptides was predicted, which indicates their extracellular localization; the rest of the proteins were localized predominantly in bacterial cytoplasm. 5 of 11 proteins function as enzymes of carbohydrate metabolism. Other extracellular proteins that could indicate its contamination with proteins from disrupted bacterial cells were not detected in S. aureus cultural liquid filtrate. It has been suggested that enzymes of carbohydrate metabolism can provide bacterial cells with energy necessary for passage from lag-phase into exponential growth phase. Superoxide dismutase enzyme probably provides the course of oxidation-reduction processes. Synthesis of other proteolytic enzymes and toxins is carried out at later stages of development of bacterial population. Immunization of mice with a mixture of11 identified proteins showed their protective properties after infection by S. aureus 6 strain. Conclusion. Based on the abovementioned, the complex of isolated proteins may be perspective in development of a new strategy of prophylaxis and therapy of staphylococcus infections.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):3-12
3-12
CHARACTERISTIC OF VIRULENCE POTENTIAL OF CLINICAL ISOLATES OF ENTEROCOCCI
Abstract
Aim. Determination of virulence of enterococci strains isolated from clinical material from humans on pheno- and genotype levels. Materials and methods. 30 strains of enterococci isolated from wound exudate, urine, newborn skin lavage were used in the study. Strain identification was carried out by multiplex PCR. Hemolytic activity was determined by dish method, gelatinase - by dissolution of gelatin column, proteolytic - by biuret method; genes coding virulence factor synthesis (gelE, sprE, cylM, cylB, cylA, cylLs, cylLl, ESP, HYL, ASA) - by using PCR. Results. Clinical isolates of enterococci were assigned to E. faecalis and E. faecium species. Virulence factors on phenotype and genotype levels were detected in both species. Conclusion. Genetic determinants of virulence are more widespread among clinical isolates of E. faecalis species. Set of genes coding virulence factors in E. faecalis depends on biotope. Gene coding hyaluronidase synthesis is characteristic for E. faecium. A correlation between phenotypic manifestation of features and enterococci genotype was detected.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):12-18
12-18
FORMATION OF MICROBIAL BIOFILMS IN CAUSATIVE AGENTS OF ACUTE AND CHRONIC PYELONEPHRITIS
Abstract
Aim. Study the intensity of formation of microbial biofilms by Pseudomonas aeruginosa, Escherichia coli, Klebsiella pneumoniae, Staphylococcus aureus strains isolated during various forms of pyelonephritis. Materials and methods. 150 clinical isolates of microorganisms isolated from urine of patients with acute and chronic pyelonephritis were included into the study. Determination of intensity of film-formation was carried out by staining of the formed biofilms by crystal violet with consequent extraction of the dye and measurement of its concentration in washout solution. Results. Among causative agents of pyelonephritis P. aeruginosa isolates had the maximum film-forming ability. The intensity of biofilm formation of these isolates was 2-3 time higher than staphylococcus and enterobacteria strains. Strains isolated from patients with chronic pyelonephritis by ability to form biofilms significantly surpassed strains isolated from acute pyelonephritis patients. A higher ability to form microbial biofilms for microorganisms - causative agents of pyelonephritis progressing against the background of urolithiasis was noted. Conclusion. The ability to form biofilms is determined by both causative agent species and character of the infectious process in which this microorganism participates. Intensive formation of biofilms by E. coli, P. aeruginosa, K. pneumoniae, S. aureus clinical isolates may be an important factor of chronization of urinary tract infections.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):18-23
18-23
GENOTYPIC DIFFERENCES BETWEEN CORYNEBACTERIUM DIPHTHERIAE BIOVAR GRAVIS AND MITIS STRAINS
Abstract
Aim. Study structure of a genetic determinant of amylase activity (amy gene) in Corynebacterium diphtheriae biovar gravis and mitis strains. Materials and methods. 87 C. diphtheriae strains (31 gravis biovar strains and 56 mitis biovar strains) as well as C. diphtheriae PW8 strain were analyzed to detect structural features of C. diphtheriae strains of various biovars. 10 pairs of primers were used in PCR that flank mutually overlapping regions within DIP0357 locus as well as additional primers that flank DIP0353 - DIP0354, DIP0357 and DIP0358 loci. Results. All the C. diphtheriae biovar gravis strains were established to contain a full-size DIP0357 locus (amy gene) whereas in all the mitis biovar strains this genome fragment is absent. All the studied C. diphtheriae biovar gravis strains do not have significant changes within DIP0354 - DIP0357 loci (amy gene) whereas in genome of 57 studied C. diphtheriae biovar mitis strains the major part of this fragment including the complete nucleotide sequence of amy gene is absent. Conclusion. C. diphtheriae biovar gravis strains have a genetically determined ability to produce amylase that can be viewed as an additional pathogenicity factor giving microorganisms wider capabilities to colonize the mucous membrane of oropharynx.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):24-31
24-31
PRESENCE OF YERSINIA ENTEROCOLITICA IN CONDITIONS OF AGRO COMPLEX
Abstract
Aim. Detection of duration of existence of Yersinia enterocolitica in substrates of agro complex and formation of biofilms by causative agent during artificial semination of forage and meat products. Materials and methods. Y. enterocolitica O9 strain and its rifampicin-resistant (Rmr) mutant were used. Microbial landscape of samples was studied by seeding on selective media (HiMedia), biochemical properties of isolates were controlled on API test-systems (Bio-Merieux). The presence of yopA gene localized on virulence plasmid pCad was determined in PCR. Vital staining of biofilms was carried out by Live/Dead stain (Invitrogen, USA). Visualization of the data was registered by using GMS-510 (USA) microscope with digital camera and Skope Photo software (USA). Formation of yersinia bacterial biofilms was confirmed by using scanning electron microscope (SEM) JSM6380 (Japan). Results. Prolonged duration of existence of Y. enterocolitica in substrates of agro complex with conservation of pCad virulence plasmid by causative agent was detected. SEM demonstrated stages of biofilm formation during artificial semination of animal forage, meat products and materials of food equipment in a wide range of temperatures from 10 to 30° C, and vital stain detected viable yersinia in mature biofilms. Conclusion. Agro complexes are a variant of technogenic foci where ecological conditions for prolonged existence of saprono-sis are formed.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):31-38
31-38
FEATURES OF PROLIFERATIVE RESPONSE OF T-CELLS ON HEPATITIS C VIRUS ANTIGENS IN HEALTHY INDIVIDUALS CONTACTING WITH THIS VIRUS
Abstract
Aim. Evaluation of CD3+ and CD3-/CD56+ proliferative response on hepatitis C virus antigens in healthy medical workers. Materials and methods. The study included 15 medical workers with length of service of 2 and more years without common risk factors (blood and blood products transfusion, abdominal operations, invasive procedures, use of intravenous drugs). Control group consisted of 9 healthy individuals without risk factors. Peripheral mononuclears were isolated from blood and then incubated 72 hours in the presence of mitogen/PHA, Core+NS4 1b genotype HCV, NS4 HCV 2a+3a genotypes or medium. Proliferative activity was registered by the presence of cell division marker ki67 by using FACS. Results. The initial immunogram of medical workers differed from the control group by a significantly lower quantity of CD3+ lymphocytes, in particular CD3+/CD8 + population. Incubation with PHA resulted in a decrease of quantity ofCD3+/ ki67+, CD4+/ki67+ and CD3-/CD56+/ki67+ in the medical workers group. Cultivation with HCV antigens resulted in a significant decrease of Treg (CD3+/CD25high/FoxP3+) and activated T-lymphocytes population in the case of stimulation by Core and NS4 1b genotype antigens. Analysis of cell response on virus antigens based on proliferative activity index detected significant differences only for CD8+/ki67+. Stimulation by Core and NS4 1b genotype antigens resulted in an increase of quantity of these cells whereas in the case of NS4 2a+3a genotypes their decrease was observed. Conclusion. The described changes may reflect exhaustion of cell reactivity due to extra antigen load in the group of medical workers, while differentiated immunologic shifts on hepatitis C viruses of various genotypes are noted.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):38-44
38-44
MONITORING OF ENTEROVIRUS CIRCULATION IN IRKUTSK REGION
Abstract
Aim. Monitoring of circulation of enteroviruses (EVI) in Irkutsk Region and study of regional specter of circulating enteroviruses. Materials and methods. 1419 samples from patients with suspected EVI, contact in foci of enterovirus infection, acute intestine infections and 964 samples of sewage water were studied in total. In 2011 isolation of viral agents from 97 samples positive on enterovirus by RT-PCR from patients with preliminary EVI diagnosis and 5 samples of sewage water of Irkutsk city was carried out. Transplantable line of human rhabdomyosarcoma RD cell culture was used for isolation of enteroviruses. Infection of cells and 2 serial passages of the studied material were carried out. The isolates were typed in neutralization reaction (NR) with a set of 32 diagnostic type-specific immune sera against viral poliomyelitis I-III; Coxsackie B1-6; Coxsackie А2, А4, А7, А9, А10; ЕСНО 68-71; ЕСНО 2, 4, 7, 8, 9, 12, 16, 20, 25, 26, 27, 29, 31, 33. Results. In 2011 circulation of enterovirus serotypes that were previously absent on the territory of the region was established: ЕСНО 68, ЕСНО 70, ECHO 71. These strains were isolated from patients, circulation of ECHO 70 serotype was established also in samples of sewage water. The analysis of enterovirus landscape carried out showed the possibility of complication of epidemic situation on the territory of the region due to change of serovariants of causative agents of non-polioenterovirus infections and detection of epidemically significant enteroviruses - ECHO 68, 70 and 71 serotypes. Conclusion. Determination of specter of enterovirus serotypes, detection of serotypes that had not previously circulated in Irkutsk Region allows to prognose epidemic situation on morbidity of enterovirus infections and timely develop and make decisions for ensuring epidemiologic welfare of the population.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):45-51
45-51
REACTOGENICITY, SAFETY, IMMUNOGENICITY AND PROPHYLACTIC EFFECTIVENESS OF POLYSACCHARIDE PNEUMOCOCCUS VACCINE DURING IMMUNIZATION OF HIV-INFECTED PATIENTS
Abstract
Aim. Study safety, reactogenicity, immunogenicity and prophylactic effectiveness of polysaccharide pneumococcus vaccines during immunization of adult HIV-infected patients. Materials and methods. 200 HIV-infected patients at stages 3 to 4A of the disease aged 20 to 50 years with the quantity of CD 4+ T-lymphocytes in blood of no less than 500 μl -1 took part in the study. 100 individuals immunized with polysaccharide 23-valent pneumococcus vaccine (Pneumo 23, Sanofi Pasteur, France) constituted the observation group. 100 individuals not immunized against pneumococcus infection constituted the comparison group. The groups were standardized by sex, age and disease stage. Vaccine reactogenicity was evaluated by detection of general and local postvaccination reactions, degree of their intensity and duration. Vaccine safety was evaluated based on comparative evaluation of results of general clinical and biochemical studies of blood, general urine analysis, determination of IgE in blood sera, CD 4+ T-lymphocytes level, quantity of HIV RNA (viral load) before vaccination and 28 days after the immunization. Vaccine immunogenicity was evaluated by determination in blood sera ofIgG against a mixture of Streptococcus рneumoniaе polysaccharides comprising Pneumo 23. Prophylaxis effectiveness of the preparation was evaluated by juxtaposition of acute respiratory illness morbidity in observation and control groups. Results. During immunization of HIV-infected patients against pneumococcus infection postvaccination complications, severe local and general postvaccination reactions were not detected, laboratory studies carried out before and after the immunization gave evidence on the lack of progression of the main disease and activization of the infectious process. After the immunization the geometric mean antibody titer against S. рneumoniaе increased by 2 times and reached protective level. Index of prophylactic effectiveness of Pneumo 23 vaccines during immunization of HIV-positive patients was 5.6, and relative risk of the disease in the immunized group - 0.07, in the control group - 0.42. Conclusion. The data provided give evidence on the high prophylactic effect of vaccination of immune compromised HIV-positive patients with a lack of deterioration of the main disease course.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):52-60
52-60
ACTIVATING EFFECT OF A GERMANIUM-ORGANIC COMPOUND ON IMMUNOCOMPETENT CELLS DURING INTRANASAL IMMUNIZATION OF MICE WITH A LIVE INFLUENZA VACCINE
Abstract
Aim. Detailed characteristic of results of intranasal immunization of mice with one of two variants of vaccinating influenza virus, particularly in combination with a low molecular weight germanium-organic compound (LMW-GOC). An additional aim is evaluation of effect of LMW-GOC on the parameters of immune system in case of intranasal administration of the preparation without the addition of vaccinating virus. Materials and methods. The study was carried out in female CBA mice (18-20 g, 6 animals per group). Intranasal immunization was carried out by 2 different variants of B/Victoria influenza virus - once or twice with a 2 week interval. Cells for study were obtained from spleen and nasal- and bronchial-associated lymphoid tissue (NALT/ BALT) 24 hours and 7 days after intranasal administration of the preparations. The main method of the study - determination of the level of expression of various markers of lymphocytes in comparison with the level of the same markers in the cells of control group animals by using flow cytometry method. The mean parameters obtained were determined by using program package WinMDI 2.8. Results. The main results were the increase of level of expression of various lymphocyte markers obtained from mice after intranasal administration of the vaccines and their combination with LMW-GOC or LMW-GOC only without the participation of the vaccines. A significant increase of the expression of TLR9 marker compared with other parameters was noted. Administration to mice of wild B/Victoria strain notably more frequently conditioned the decrease of expression of some parameters compared with administration of the cold adapted strain. Effect of LMW-GOC without the vaccine also conditioned the increase of levels of markers however a combination of the preparations with the vaccine was more effective. Conclusion. The increase of level of expression of a number of lymphocyte markers may serve as a sign of successful intranasal vaccination against influenza. LMW-GOC preparation increases immune stimulating effect of intranasally administered vaccines and in none of the cases weakens the stimulating result of effect of the vaccines, and in many cases increases it. LMW-GOC may be studied as a main or additional adjuvant for intranasal application of influenza vaccines.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):60-68
60-68
EXPRESSION OF TLR2 AND TLR9 GENES BY EPITHELIAL CELLS OF CERVICAL CANAL MUCOUS MEMBRANE IN WOMEN WITH INFLAMMATORY DISEASES OF SMALL PELVIS ORGANS
Abstract
Aim. Determine subpopulation composition of blood lymphocytes and the level of expression of TLR2 and TLR9 by epithelial cells of cervical canal mucous membrane in women of reproductive age with inflammatory disease of small pelvis organs (IDSPO) at exacerbation stage and remission period. Materials and methods. Clinical-laboratory and gynecological examination of 105 women was carried out and 3 groups were formed based on the results: patients at IDSPO exacerbation stage; patients at remission stage; clinically healthy women. By using real time PCR, TLR2, TLR9 gene expression levels were determined in epithelial cells of cervical canal mucous membrane in women of all the 3 groups. Subpopulation composition of blood lymphocytes was determined by flow cytofluorimetry by using monoclonal antibodies with CD45+ CD3+ -T-cell, CD45+ CD3+ CD4+ -Т-helper, CD45+, CD3 + , CD8+ -Т-suppressors-cytotoxic killers, CD45 + , CD3-, CD16+, CD56+ natural killers, CD45+, CD3-, CD19+ -В-lymphocytes. Immune fluorescence reaction evaluation was carried out in flow cytofluorimeter Cytomics FC 500 (Becton Coulter, USA). Results. The level of expression of TLR2 gene in the studied groups of patients was established not to differ significantly from parameters in the comparison groups, however it should be noted that this parameter in women with IDSPO at exacerbation stage (causative agents of the infectious process - ureaplasma, staphylococcus, candida) was somewhat higher than in the comparison group. Significantly high level of TLR9 gene expression in cervical canal epithelial cells was detected to correlate with the presence of infectious causative agents. In the group of women with exacerbation of the infectious process the expression of TLR9 was 14.5 times higher compared with the group of women without IDSPO. Among groups of women with IDSPO significant differences in relation to control group in relative and absolute levels of CD3 + T-lymphocytes; CD4+ T-helpers; CD8+ cytotoxic killer T-suppressors, B-lymphocytes compared with the same parameters in clinically healthy women were not detected. Conclusion. The increase of TLR9 gene expression level in cervical canal cells of women with IDSPO may serve as an additional diagnostic feature of the presence and degree of severity of the disease.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):68-72
68-72
EVALUATION OF SIGNIFICANCE OF BORRELIA GARINII SPIROCHETE RECOMBINANT PROTEIN DbpB FOR SERODIAGNOSTICS OF IXODES TICK-BORNE BORRELIOSIS
Abstract
Aim. Obtaining recombinant protein DbpB of West Siberia Borrelia garinii 20047 isolate and evaluation of its antigen activity for the possible use in serodiagnostics of ixodes tick-borne bor-reliosis (ITB). Materials and methods. Coding region of dbpB gene of novosibirsk B. garinii 20047 isolate was amplified by PCR and cloned as part of expressing pETm vector in Escherichia coli BL21(DE3) strain cells. Recombinant protein DbpB produced by the selected clone was studied by EIA method for its ability to react with sera antibodies oflTB patients. Results. E. coli BL21(DE3) clone producing recombinant protein DbpB in quantity of 30% of total E. coli cell protein was obtained. Homology of amino acid sequence of recombinant protein DbpB of novosibirsk B.garinii 20047 isolate with primary structures of B. garinii, B. afzelii and B. burgdorferi sensu stricto spirochete genospieces DbpB proteins presented in GenBank database was 98.4, 77 and 73%, respectively. Sensitivity of immune enzyme detection in sera of ITB patients with migrating erythema of IgM and IgG reacting with DbpB antigen was 13.9 and 20.0%, respectively. Frequency of detection of IgM and IgG against DbpB in patient sera with disseminated ITB form was 15.7 and 43.8%, respectively. Specificity ofimmune enzyme detection ofantibodies against recombinant antigen DbpB in which sera of syphilis, rheumatoid arthritis patients and healthy donors used as control sera was 100%. Conclusion. DbpB recombinant protein of novosibirsk B. garinii 20047 isolate may be used as one of antigens for highly specific serodiagnostics of ITB disseminated stage.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):73-79
73-79
SEROLOGIC STUDY OF EXPERIMENTAL CHOLERA POLYMER ANTIGEN DIAGNOSTICUMS
Abstract
Aim. Evaluation of quality indicators of constructed cholera antigen polymer diagnosticums by using a complex of specific anti-cholera sera. Materials and methods. Cell lysates of cholera vibrio strains Vibrio cholerae cholerae 1395, V. eltor Ogawa 2044, V. eltor Inaba 13020, V. cholerae О139 16064 were sensitins for experimental preparations. 3 sera from cholera patients, normal human sera, cholera O1 (Ogawa, Inaba) commercial horse, cholera O139 commercial rabbit and heterologic sera against shigella, salmonella, escherichia and yersinia as well as experimental cholera rabbit sera against O1 and O139 were used as control. Results. The study established that diagnosticums based on V. cholerae cholerae 1395 and V. cholerae О139 16064 strain sensitins by quality indicators may be used in the future for construction of these diagnosticums. Conclusion. Antibody containing preparations - commercial horse O1 sera, rabbit experimental and commercial sera and MCA O139 demonstrating titers not lower than 1/5120-1/10240 may serve as a control of experimental diagnosticums in the absence of human sera from cholera patients.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):79-83
79-83
DETECTION OF UNCULTIVABLE BACTERIA FORMS IN PROBIOTIC LYOPHILIZED PREPARATIONS
Abstract
Aim. Detection of viable but uncultivable forms among lyophilized cells of commercial probiotics. Materials and methods. 9 series of probiotic preparations (colibacterin, bificol, bifidumbacterin, bifiform) with expired (up to 30 years of storage) or valid shelf life were objects of the study. Total quantity of the bacteria was calculated under the microscope in Goryaev chamber, the number of viable cells was determined in luminescence microscope after staining by an array of fluorescent dyes, the quantity of CFU/ml was evaluated by method of seeding into the respective solid or semi-liquid cultivation medium. Results. Juxtaposition of the specified parameter values allowed to establish that in lyophilized preparations of colibacterin with expired shelf life the amount of viable but not forming colonies (uncultivable forms) cells varied from 4.13 to 99.73% depending on date of production. For bifidumbacterin with unexpired shelf life live cells constituted 95.45 and 70.73%. The amount of viable bifidobacteria forming colonies was on the level of 100 and 50%, respectively. In bifidopreparations micro colonies that may possibly be formed spontaneously by awakened uncultivable forms were noted. A possibility of growth stimulation of these cells by 1 and 10% aminopeptide was shown. Conclusion. The presence ofuncultivable forms in lyophilized preparations of probiotics was proven experimentally.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):83-88
83-88
PATHOGENIC PROPERTIES OF FUNGI FUSARIUM GENUS ISOLATED FROM PATIENTS WITH ATOPIC DERMATITIS
Abstract
Aim. Study of adhesive activity and growth speed of fungi Fusarium genus isolated from the surface of cutaneous covering in patients with atopic dermatitis (AD). Materials and methods. Clinical and museum F. oxysporum, F. solani strains were used in the study. Seeding was carried out into agarized Czapek and Sabouraud medium. The cultures were studied for 9 days at 30+2°C. adhesive properties of fungi were determined by using model based on nitrocellulose film (S.A.Li-sovskaya et al., 2006). Results. The studies carried out showed statistically significant differences in adhesive properties and intergrowth intensity of various Fusarium spp. Adhesion level of F. solani microconidia was almost 2.5 times higher compared with F. oxysporum. Formation of the first germ tube by F. solani microconidia was noted during the first 10 hours whereas by F. oxysporum - only at day 2. Conclusion. The data obtained confirm species differences of Fusarium spp. pathogenic properties that emphasize the importance of species identification of fungi.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):88-92
88-92
FEATURES OF DYNAMICS OF GROWTH AND FORMATION OF UNCULTIVABLE FORMS IN LACTOCOCCUS LACTIS
Abstract
Aim. Study strain differences in dynamics of viability and formation of uncultivable forms of Lactococcus lactis. Materials and methods. 3 strains of L. lactis - MSU, 729 and F116 were used in the study. Uncultivable forms were obtained by prolonged incubation of cultures of lactococcus in synthetic medium under conditions of carbohydrate deprivation. Medium was inoculated by cultures grown in Elliker broth, washed by saline and without washing. The populations obtained were incubated at 30°C without mixing for 4 months. Samples of cultures were studied periodically for viability and cultivability. Results. In cultures obtained by using unwashed inoculate active growth of quantity of bacteria in the first days after seeding was noted. Speed of formation of uncultivable forms is the faster the higher the level of metabolic activity of cells in the population. A fact of phenotypic dissociation in lactococcus culture under stress was detected. Conclusion. The speed of formation of uncultivable forms of L. lactis, as well as stability of their existence may probably depend on the strain, cultivation conditions and metabolic activity of cells in the population.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):92-96
92-96
IMMUNOGENETIC FACTORS OF INTERACTION OF HEPATITIS C VIRUS AND HUMAN AND POSSIBILITIES OF DEVELOPMENT OF THERAPEUTIC TACTIC
Abstract
Various macroorganism factors influence spontaneous and therapy induced elimination of hepatitis C virus. Standard therapy is application of a combination of pegylated interfernos and ribavirin. However such tactics results in attainment of a resistant virological response in approximately half the cases during infection by genotype 1 virus. The future of viral hepatitis C therapy lies most probably in the sphere of application of specific antiviral preparations such as protease and/or polymerase inhibitors as an addition to standard therapy. The aim of this review was to describe mechanisms of resistance to therapy in light of reaction of innate and adaptive immune response as well as an attempt to determine factors capable of prognosing response to therapy.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):97-103
97-103
EPIDEMIC PROCESS AND VACCINE PROPHYLAXIS OF PERTUSSIS
Abstract
Analysis of data on epidemic process of pertussis infection in conditions of wide coverage of population by prophylactic vaccination is presented. Post-vaccination immunity against pertussis was shown to reduce with age; therefore a large part of vaccinated children becomes susceptible to this infection already in primary school age. Epidemic process of pertussis continues both as manifest form and as subclinical and atypical forms. The main reservoir of pertussis infection is older age population groups. The necessity to implement programs of revaccination against pertussis in older children, adolescents and adults is justified. Characteristics of vaccines for immune prophylaxis of pertussis infection are given.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):103-110
103-110
PROTEIN COMPONENTS OF INNATE IMMUNITY IN PROTECTION FROM PATHOGENIC INVASION (LITERATURE REVIEW)
Abstract
System of innate immunity is a set of effector molecules and cells counteracting invasion of pathogens and their products. AIpha-2-macroglobulin (a2-MG) and lactoferrin (LF) play a significant role in primary protection of organism. A wide spectrum of transport and regulatory functions, high affinity to endocytosis receptor as well as structural features of these proteins allow them not only to effectively protect the organism during direct contact with pathogen but also to have an immunomodulatory impact on immunocompetent cells of adaptive immunity. However despite a common receptor and a number of ligands, mechanisms of realization of protective functions of a2-MG and LF differ significantly. The aim of this review is to system-ize knowledge on means and mechanisms of protection of a2-MG and LF against invasion.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):111-117
111-117
BOLIVIAN HEMORRHAGIC FEVER
Abstract
Analysis of data of the available literature on epidemiology of Bolivian hemorrhagic fever, manifestations of human disease, biological properties of the causative agent and development carried out abroad of means and methods of diagnostics, prophylaxis and therapy of this infection that presents a potential threat for the population and economy of the Russian Federation in case of introduction of the causative agent is presented.
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):118-126
118-126
CONTENTS
Journal of microbiology, epidemiology and immunobiology. 2013;90(3):127-128
127-128