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首页> 外文期刊>Journal of Clinical Microbiology >Vibrio cholerae Strain Typing and Phylogeny Study Based on Simple Sequence Repeats
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Vibrio cholerae Strain Typing and Phylogeny Study Based on Simple Sequence Repeats

机译:基于简单序列重复的霍乱弧菌菌株分型和系统发育研究

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Vibrio cholerae is the etiological agent of cholera. Its natural reservoir is the aquatic environment. To date, practical typing of V. cholerae is mainly serological and requires about 200 antisera. Simple sequence repeats (SSR), also termed VNTR (for variable number of tandem repeats), provide a source of high genomic polymorphism used in bacterial typing. Here we describe an SSR-based typing method that combines the variation in highly mutable SSR loci, with that of shorter, relatively more stable mononucleotide repeat (MNR) loci, for accurate and rapid typing of V. cholerae. In silico screening of the V. cholerae genome revealed thousands of perfect SSR tracts with an average frequency of one SSR every 152 bp. A panel of 32 V. cholerae strains, representing both clinical and environmental isolates, was tested for polymorphism in SSR loci. Two strategies were applied to identify SSR variation: polymorphism of SSR tracts longer than 12 bp (L-SSR) assessed by capillary fragment-size analysis and MNR polymorphism assessed by sequencing. The nine L-SSR loci tested were all polymorphic, displaying 2 to 13 alleles per locus. Sequence analysis of eight MNR-containing loci (MNR-multilocus sequence typing [MLST]) provided information on both variations in the MNR tract itself, and single nucleotide polymorphism (SNP) in their flanking sequences. Phylogenetic analysis of the combined SSR data showed a clear discrimination between the clinical strains belonging to O1 and O139 serogroups, and the environmental isolates. Furthermore, discrimination between 27 strains of the 32 strains was achieved. SSR-based typing methods combining L-SSR and MNR-MLST were found to be efficient for V. cholerae typing.
机译:霍乱弧菌是霍乱的病原体。它的天然水库是水生环境。迄今为止, V的实际键入。霍乱主要是血清学,需要约200种抗血清。简单序列重复(SSR),也称为VNTR(用于可变数目的串联重复),提供了用于细菌分型的高基因组多态性来源。在这里,我们描述了一种基于SSR的分型方法,该方法结合了高度易变SSR基因座中的变异与较短,相对更稳定的单核苷酸重复(MNR)基因座中的变异,可准确快速地鉴定V。霍乱。在计算机上筛选 V。霍乱弧菌基因组揭示了数千条完美的SSR片段,平均频率为每152 bp一个SSR。 32个 V的面板。测试了代表临床和环境分离株的霍乱菌菌株在SSR位点的多态性。应用了两种策略来鉴定SSR变异:通过毛细管片段大小分析评估的长于12 bp的SSR片段多态性(L-SSR)和通过测序评估的MNR多态性。测试的9个L-SSR基因座均为多态性,每个位点显示2至13个等位基因。八个包含MNR的基因座(MNR-多基因座序列类型[MLST])的序列分析提供了有关MNR区域本身的变异以及其侧翼序列中的单核苷酸多态性(SNP)的信息。综合SSR数据的系统发育分析表明,属于O1和O139血清群的临床菌株与环境分离株之间存在明显的区别。此外,在32个菌株中的27个菌株之间进行了区分。发现结合了L-SSR和MNR-MLST的基于SSR的键入方法对于 V是有效的。霍乱

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