Genotyping Mycoplasma synoviae: Development of a multi-locus variable number of tandem-repeats analysis and comparison with current molecular typing methods

滑膜支原体 多位点VNTR分析 生物 打字 可变数串联重复 多位点序列分型 基因分型 遗传学 串联重复 基因座(遗传学) 基因型 支原体 基因组 基因 鸡败血症支原体
作者
Zsuzsa Kreizinger,Kinga M. Sulyok,Katinka Bekő,Áron Botond Kovács,Dénes Grózner,Orsolya Felde,Szilvia Marton,Krisztián Bànyai,Salvatore Catania,Dušan Benčina,Miklós Gyuranecz
出处
期刊:Veterinary Microbiology [Elsevier BV]
卷期号:226: 41-49 被引量:9
标识
DOI:10.1016/j.vetmic.2018.10.012
摘要

Control of one of the most important avian mycoplasmas, Mycoplasma synoviae, and tracing the spread of the infection can be challenging as the pathogen is transmissible by both horizontal and vertical routes, and it can be disseminated through long distances via the hatching eggs, day-old chicks or pullets during intensive international trade. Genetic information provided by molecular typing methods support control programmes and epizootiologic studies. The aims of the present study were to develop a multi-locus variable number of tandem-repeats analysis (MLVA) method for the typing of M. synoviae isolates and to evaluate the currently used molecular typing methods which are applicable directly on clinical samples. Tandem repeat (TR) regions were selected from the whole genome sequence of the M. synoviae type strain (WVU1853) to characterise the genetic diversity of 86 M. synoviae strains originating from 15 countries. The strains were also submitted to multi-locus sequence typing (MLST) assays, vlhA gene sequence analysis and to assays designed to differentiate live vaccine strains from field strains. The developed MLVA involves the examination of seven TR regions and provides similar genetic resolution as the tested MLST assays by identifying 35 genotypes among the tested strains. Differentiation of the live vaccine strains from field strains was also successful with the developed assay. The provided MLVA method proved to be a highly discriminative, rapid and cost-effective alternative typing technique for the genetic characterisation of M. synoviae and it is also suitable for the complementation of live vaccine strain differentiating assays in ambiguous cases.

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