首页> 外文期刊>Clinical microbiology and infection: European Society of Clinical Microbiology and Infectious Diseases >The molecular epidemiology and evolution of the Panton-Valentine leukocidin-positive, methicillin-resistant Staphylococcus aureus strain USA300 in Western Australia.
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The molecular epidemiology and evolution of the Panton-Valentine leukocidin-positive, methicillin-resistant Staphylococcus aureus strain USA300 in Western Australia.

机译:西澳大利亚州Panton-Valentine leukocidin阳性,耐甲氧西林金黄色葡萄球菌菌株USA300的分子流行病学和进化。

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摘要

Between 2003 and 2008, 76 clinical isolates of the Panton-Valentine leukocidin-positive Staphylococcus aureus strain 'West Australian methicillin-resistant Staphylococcus aureus (MRSA)-12' (WA MRSA-12) were recovered from 72 patients living in the Perth area in Western Australia. These isolates were found to belong to multilocus sequence type 8, and had a USA300-like pulsed-field gel electrophoresis pulsotype. All isolates were genotyped using diagnostic DNA arrays covering species markers, resistance factors, virulence-associated, as well as MSCRAMM (microbial surface components recognizing adhesive matrix molecules) genes to prove the identity between WA MRSA-12 and the pandemic strain USA300, as well as to detect possible genetic variability. In general, WA MRSA-12 isolates were similar to USA300, and the most common variant was identical to USA300-TC1516. From this clone, most of the other variants may have evolved by a limited number of gene losses or acquisitions. Variations in carriage of virulence and resistance-associated genes allow distinction of variants or sub-clones. Altogether, 16 variants could be distinguished. They differed in the carriage of resistance genes (blaZ/I/R, ermC, msrA + mpbBM, aadD + mupR, aphA3 + sat, tetK, qacC, merA/B/R/T) of beta-haemolysin-converting phages and of enterotoxins (sek + seq, which were deleted in four isolates). Notably, the arginine catabolic mobile element (ACME) was absent in 12 isolates (15.8%). The mercury resistance (mer) operon, which is usually associated with SCCmec type III elements, was found in several ACME-negative isolates. The present study emphasises the importance of genotyping in detecting the introduction and evolution of significant MRSA strains within a community.
机译:在2003年至2008年之间,从居住在珀斯地区珀斯地区的72例患者中回收了76株Panton-Valentine白细胞介素阳性金黄色葡萄球菌菌株“西澳大利亚耐甲氧西林金黄色葡萄球菌(MRSA)-12”(WA MRSA-12)。澳洲西部。发现这些分离物属于多基因座序列类型8,并具有USA300样脉冲场凝胶电泳脉冲型。使用诊断DNA阵列对所有分离物进行基因分型,这些阵列包括物种标记,抗性因子,毒力相关以及MSCRAMM(识别粘附基质分子的微生物表面成分)基因,以证明WA MRSA-12与大流行毒株USA300之间的身份以检测可能的遗传变异。通常,WA MRSA-12分离株与USA300类似,最常见的变体与USA300-TC1516相同。从这个克隆中,大多数其他变体可能是由于有限数量的基因丢失或获取而进化出来的。毒力和抗性相关基因携带的变异允许区分变异或亚克隆。总共可以区分16个变体。它们在抗性基因(blaZ / I / R,ermC,msrA + mpbBM,aadD + mupR,aphA3 + sat,tetK,qacC,merA / B / R / T)的抗性基因携带方面有所不同。肠毒素(sek + seq,已在四个分离株中删除)。值得注意的是,在12个分离株(15.8%)中不存在精氨酸分解代谢移动元件(ACME)。在几种ACME阴性分离物中发现了通常与SCCmec III型元素相关的耐汞操纵子。本研究强调基因分型在检测社区内重大MRSA菌株的引入和进化中的重要性。

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