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      Genotyping markers used for multi locus VNTR analysis with ompA (MLVA- ompA) and multi sequence typing (MST) retain stability in Chlamydia trachomatis

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          Abstract

          We aimed to evaluate the stability of the Chlamydia trachomatis multi locus VNTR analysis (MLVA- ompA) and multi sequence typing (MST) systems through multiple passages in tissue culture. Firstly, we analyzed the stability of these markers through adaptation of C. trachomatis to tissue culture and secondly, we examined the stability of a four-locus MLVA- ompA and a five-locus MST system after multiple passages in tissue culture. Marker sequences were monitored through successive chlamydial developmental cycles to evaluate the stability of the individual DNA markers through many bacterial divisions and this, in turn, informed us of the usefulness of using such typing systems for short and long-term molecular epidemiology. Southampton genitourinary medicine (GUM) clinic isolates from endocervical swabs collected from C. trachomatis positive women were passaged through tissue culture. MLVA- ompA typing was applied to primary swab samples and to the same samples after C. trachomatis had been passaged through cell culture (eight passages). Sequence data from time-zero and passage-eight isolates were aligned with reference sequences to determine the stability of the markers. The Swedish new variant (nvCT) underwent 72 passages in cell culture and the markers of the two schemes were similarly analyzed. Analysis of genetic markers of the MLVA- ompA typing system before and after the isolates were introduced to tissue culture showed no change in the dominant sequence. The nvCT that had been passaged 72 times over the duration of a year also showed no variation in the dominant sequence for both the genotyping schemes. MLVA- ompA and MST markers are stable upon adaptation of C. trachomatis to tissue culture following isolation of strains from primary endocervical swab samples. These markers remain stable throughout multiple rounds of cell-division in tissue culture, concomitant with the incubation period and appearance of symptoms normally associated with host-infection. Both genotyping schemes are, therefore, suitable for epidemiology of C. trachomatis.

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          Guidelines for the validation and application of typing methods for use in bacterial epidemiology.

          A. van Belkum, P. T. Tassios, L Dijkshoorn (2007)
          For bacterial typing to be useful, the development, validation and appropriate application of typing methods must follow unified criteria. Over a decade ago, ESGEM, the ESCMID (Europen Society for Clinical Microbiology and Infectious Diseases) Study Group on Epidemiological Markers, produced guidelines for optimal use and quality assessment of the then most frequently used typing procedures. We present here an update of these guidelines, taking into account the spectacular increase in the number and quality of typing methods made available over the past decade. Newer and older, phenotypic and genotypic methods for typing of all clinically relevant bacterial species are described according to their principles, advantages and disadvantages. Criteria for their evaluation and application and the interpretation of their results are proposed. Finally, the issues of reporting, standardisation, quality assessment and international networks are discussed. It must be emphasised that typing results can never stand alone and need to be interpreted in the context of all available epidemiological, clinical and demographical data relating to the infectious disease under investigation. A strategic effort on the part of all workers in the field is thus mandatory to combat emerging infectious diseases, as is financial support from national and international granting bodies and health authorities.
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            Multiple-locus variable number tandem repeats analysis for genetic fingerprinting of pathogenic bacteria.

            Bjørn-Arne Lindstedt (2005)
            DNA fingerprinting has attracted considerable interest as means for identifying, tracing and preventing the dissemination of infectious agents. Various methods have been developed for typing of pathogenic bacteria, which differ in discriminative power, reproducibility and ease of interpretation. During recent years a typing method, which uses the information provided by whole genome sequencing of bacterial species, has gained increased attention. Short sequence repeat (SSR) motifs are known to undergo frequent variation in the number of repeated units through cellular mechanisms most commonly active during chromosome replication. A class of SSRs, named variable number of tandem repeats (VNTRs), has proven to be a suitable target for assessing genetic polymorphisms within bacterial species. This review attempts to give an overview of bacterial agents where VNTR-based typing, or multiple-locus variant-repeat analysis (MLVA) has been developed for typing purposes, together with addressing advantages and drawbacks associated with the use of tandem repeated DNA motifs as targets for bacterial typing and identification.
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              Multiple-Locus Variable Number Tandem Repeat Analysis of Staphylococcus Aureus: Comparison with Pulsed-Field Gel Electrophoresis and spa-Typing

              Leo Schouls, Emile Spalburg, Martijn van Luit (2009)
              Background Molecular typing of methicillin-resistant Staphylococcus aureus (MRSA) is required to study the routes and rates of transmission of this pathogen. Currently available typing techniques are either resource-intensive or have limited discriminatory ability. Multiple-locus variable number tandem repeat analysis (MLVA) may provide an alternative high throughput molecular typing tool with high epidemiological resolution. Methodology/Principal Findings A new MLVA scheme for S. aureus was validated using 1681 S. aureus isolates collected from Dutch patients and 100 isolates from pigs. MLVA using 8 tandem repeat loci was performed in 2 multiplex PCRs and the fluorescently labeled PCR products were accurately sized on an automated DNA sequencer. The assessed number of repeats was used to create MLVA profiles consisting of strings of 8 integers that were used for categorical clustering. MLVA yielded 511 types that clustered into 11 distinct MLVA complexes which appeared to coincide with MLST clonal complexes. MLVA was at least as discriminatory as PFGE and twice as discriminatory as spa-sequence typing. There was considerable congruence between MLVA, spa-sequence typing and PFGE, at the MLVA complex level with group separation values of 95.1% and 89.2%. MLVA could not discriminate between pig-related MRSA strains isolated from humans and pigs, corroborating the high degree of relationship. MLVA was also superior in the grouping of MRSA isolates previously assigned to temporal-spatial clusters with indistinguishable SpaTypes, demonstrating its enhanced epidemiological usefulness. Conclusions The MLVA described in this study is a high throughput, relatively low cost genotyping method for S. aureus that yields discrete and unambiguous data that can be used to assign biological meaningful genotypes and complexes and can be used for interlaboratory comparisons in network accessible databases. Results suggest that MLVA offsets the disadvantages of other high discriminatory typing approaches and represents a promising tool for hospital, national and international molecular epidemiology.
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                Author and article information

                Journal
                Journal ID (nlm-ta): Front Cell Infect Microbiol
                Journal ID (iso-abbrev): Front Cell Infect Microbiol
                Journal ID (publisher-id): Front. Cell. Inf. Microbio.
                Title: Frontiers in Cellular and Infection Microbiology
                Publisher: Frontiers Media S.A.
                ISSN (Electronic): 2235-2988
                Publication date (Electronic): 17 May 2012
                Publication date Collection: 2012
                Volume: 2
                Electronic Location Identifier: 68
                Affiliations
                [1] 1simpleMolecular Microbiology and Infection, School of Medicine, University of Southampton, Southampton Hampshire, UK
                [2] 2simpleDepartment of Clinical Microbiology, Malmö University Hospital Malmö, Sweden
                [3] 3simpleDepartment of Obstetrics and Gynaecology, Malmö University Hospital Malmö, Sweden
                [4] 4simpleDepartment of Medical Sciences, Section of Clinical Bacteriology, Uppsala University Uppsala, Sweden
                [5] 5simpleHealth Protection Agency, Microbiology Services, Public Health Laboratory Southampton, Southampton General Hospital, Southampton Hampshire, UK
                Author notes

                Edited by: Yasuko Rikihisa, Ohio State University, USA

                Reviewed by: Ted Hackstadt, Rocky Mountain Laboratories/NIAID/NIH, USA; Yajun Song, Beijing Institute of Microbiology and Epidemiology, China; João P. Gomes, National Institute of Health, Portugal

                *Correspondence: Peter Marsh, Health Protection Agency, Microbiology Services, Public Health Laboratory Southampton, Southampton General Hospital, Tremona Road, Southampton, SO16 6YD, Hampshire, UK. e-mail: peter.marsh@ 123456uhs.nhs.uk
                Article
                DOI: 10.3389/fcimb.2012.00068
                PMC ID: 3417530
                PubMed ID: 22919659
                SO-VID: b2320dfd-7a50-43b3-94e4-cfbc37002bc9
                Copyright © Copyright © 2012 Labiran, Clarke, Cutcliffe, Wang, Skilton, Persson, Bjartling, Herrmann, Christerson and Marsh.
                License:

                This is an open-access article distributed under the terms of the Creative Commons Attribution Non Commercial License, which permits non-commercial use, distribution, and reproduction in other forums, provided the original authors and source are credited.

                History
                Date received : 20 January 2012
                Date accepted : 30 April 2012
                Page count
                Figures: 1, Tables: 2, Equations: 0, References: 23, Pages: 7, Words: 5652
                Categories
                Subject: Microbiology
                Subject: Original Research Article

                ScienceOpen disciplines: Infectious disease & Microbiology
                Keywords: tissue culture,multi sequence typing,marker stability,chlamydia trachomatis,mlva-ompa
                Data availability:
                ScienceOpen disciplines: Infectious disease & Microbiology
                Keywords: tissue culture, multi sequence typing, marker stability, chlamydia trachomatis, mlva-ompa

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