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首页> 外文期刊>The Journal of Antimicrobial Chemotherapy >A novel reverse-line hybridization assay for identifying genotypes of CTX-M-type extended-spectrum beta-lactamases.
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A novel reverse-line hybridization assay for identifying genotypes of CTX-M-type extended-spectrum beta-lactamases.

机译:一种新颖的反向杂交测定法,用于鉴定CTX-M型超广谱β-内酰胺酶的基因型。

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OBJECTIVES: To develop a reverse-line hybridization assay to identify CTX-M genotypes, potentially useful for large-scale investigation of surveillance collections. METHODS: Isolates carrying previously characterized bla(CTX-M) genes were used to develop the method. In addition, 334 isolates from five separate surveys were used to validate the method. CTX-M group was known from an independent multiplex PCR for 122 isolates and genotype was confirmed for 80 isolates by DNA sequencing. A multiplex PCR was designed to amplify a genotype-specific region within the bla(CTX-M) open-reading frame. Oligonucleotides were designed to hybridize to regions within each amplicon, covering mutations that distinguish among bla(CTX-M) genotypes. RESULTS: CTX-M phylogenetic groups were identified by the multiplex PCR with 100% concordance. The reverse-line hybridization assay specifically identified commonly-reported variants within these groups (98.7% concordance). CONCLUSIONS: The hybridization method enabled precise identification of CTX-M genes, rather than just to group level, without the need for DNA sequencing. In its present format, the method enables 43 isolates to be processed per membrane, giving results within one working day. It is a useful tool for the epidemiological investigation of bla(CTX-M) genes among survey collections of Enterobacteriaceae.
机译:目的:开发一种反向杂交杂交技术,以鉴定CTX-M基因型,可能对大规模收集监视资料有用。方法:使用携带先前鉴定的bla(CTX-M)基因的分离株开发该方法。此外,使用了来自五个独立调查的334个分离株来验证该方法。通过独立的多重PCR已知122个分离物的CTX-M组,并且通过DNA测序确认了80个分离物的基因型。设计了多重PCR,以扩增bla(CTX-M)开放阅读框内的基因型特异性区域。设计寡核苷酸以与每个扩增子内的区域杂交,涵盖区分bla(CTX-M)基因型的突变。结果:通过多重PCR鉴定出CTX-M系统发育群体,一致性为100%。反向杂交测定法明确鉴定了这些组中普遍报道的变异(98.7%的一致性)。结论:杂交方法能够精确鉴定CTX-M基因,而不仅仅是组水平,而无需进行DNA测序。以目前的格式,该方法可使每个膜处理43个分离株,从而在一个工作日内得出结果。它是肠杆菌科调查集合中bla(CTX-M)基因的流行病学调查的有用工具。

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