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首页> 外文期刊>Journal of Clinical Microbiology >Comparative Sequencing of the Serine-Aspartate Repeat-Encoding Region of the Clumping Factor B Gene (clfB) for Resolution within Clonal Groups of Staphylococcus aureus
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Comparative Sequencing of the Serine-Aspartate Repeat-Encoding Region of the Clumping Factor B Gene (clfB) for Resolution within Clonal Groups of Staphylococcus aureus

机译:克隆因子B基因(clfB)的丝氨酸-天冬氨酸重复编码区的比较测序以解决金黄色葡萄球菌的克隆组中。

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Molecular techniques such as spa typing and multilocus sequence typing use DNA sequence data for differentiating Staphylococcus aureus isolates. Although spa typing is capable of detecting both genetic micro- and macrovariation, it has less discriminatory power than the more labor-intensive pulsed-field gel electrophoresis (PFGE) and costly genomic DNA microarray analyses. This limitation hinders strain interrogation for newly emerging clones and outbreak investigations in hospital or community settings where robust clones are endemic. To overcome this constraint, we developed a typing system using DNA sequence analysis of the serine-aspartate (SD) repeat-encoding region within the gene encoding the keratin- and fibrinogen-binding clumping factor B (clfB typing) and tested whether it is capable of discriminating within clonal groups. We analyzed 116 S. aureus strains, and the repeat region was present in all isolates, varying in sequence and in length from 420 to 804 bp. In a sample of 36 well-characterized genetically diverse isolates, clfB typing subdivided identical spa and PFGE clusters which had been discriminated by whole-genome DNA microarray mapping. The combination of spa typing and clfB typing resulted in a discriminatory power (99.5%) substantially higher than that of spa typing alone and closely approached that of the whole-genome microarray (100.0%). clfB typing also successfully resolved genetic differences among isolates differentiated by PFGE that had been collected over short periods of time from single hospitals and that belonged to the most prevalent S. aureus clone in the United States. clfB typing demonstrated in vivo, in vitro, and interpatient transmission stability yet revealed that this locus may be recombinogenic in a primarily clonal population structure. Taken together, these data show that the SD repeat-encoding region of clfB is a highly stable marker of microvariation, that in conjunction with spa typing it may serve as a DNA sequence-based alternative to PFGE for investigating genetically similar strains, and that it is useful for analyzing collections of isolates in both long-term population-based and local epidemiologic studies.
机译:诸如 spa 分型和多基因座序列分型的分子技术使用DNA序列数据来区分金黄色葡萄球菌分离株。尽管 spa 分型能够检测遗传的微观和宏观变异,但与劳动强度大的脉冲场凝胶电泳(PFGE)和昂贵的基因组DNA微阵列分析相比,它的辨别力较小。这种限制阻碍了对新出现的克隆的菌株询问和在健壮的克隆为地方病的医院或社区环境中的暴发调查。为了克服这一限制,我们开发了一种利用角蛋白和纤维蛋白原结合聚簇因子B( clfB 分型)编码基因中丝氨酸-天冬氨酸(SD)重复编码区的DNA序列分析开发分型系统)并测试了它是否能够在克隆组中进行区分。我们分析了116个 S。金黄色葡萄球菌菌株,其重复区存在于所有分离株中,序列和长度在420至804bp之间变化。在36个特征明确的遗传多样性分离株的样本中, clfB 分型细分了相同的 spa 和PFGE簇,这些簇已通过全基因组DNA微阵列作图进行了区分。 spa 类型和 clfB 类型的组合产生的辨别力(99.5%)明显高于单独的 spa 类型,并且非常接近全基因组微阵列的比例(100.0%)。 clfB 分型还成功解决了由PFGE分离的分离株之间的遗传差异,这些分离株是在短时间内从单一医院收集的,属于最流行的 S。美国的aureus 克隆。 clfB 分型显示出体内,体外和患者间的传播稳定性,但仍表明该基因座可能在主要的克隆种群结构中具有重组作用。综上所述,这些数据表明 clfB 的SD重复编码区是微变异的高度稳定标记,与 spa 键入结合,它可以作为DNA序列PFGE的替代品,可用于研究遗传相似的菌株,在长期的基于群体的流行病学研究和局部流行病学研究中,对分析分离株的收集有用。

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