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Molecular Detection of the mcr Genes by Multiplex PCR

机译:通过多重PCR分子检测MCR基因

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Background: The emergence and prevalence of plasmid-mediated colistin-resistant bacterial strains in recent years have raised great concerns in clinical medicine. It is urgently needed to develop a cheaper, faster, simpler, sensitive, and specific molecular detection method to identify and monitor the dissemination of the transferable resistant determinants. Methods and Results: Herein, eight pairs of primers were designed to set up a multiplex PCR method for the rapid and efficient determination of reported mcr genes. This assay can give results within 85 min (35 min for amplification and 50 min for electrophoresis). We validated the feasibility of this assay by testing the presence of mcr genes in 60 colistin-resistant isolates. Conclusion: Our multiplex PCR technique exhibits remarkable advantages in the light of clear identification, efficiency of amplification, as well as the time consuming for detection, and thus could be useful for the surveillance and epidemiological research of plasmid-mediated colistin resistance, particularly for the under-resourced laboratories.
机译:背景:近年来质粒介导的耐药性细菌菌株的出现和患病率在临床医学中提出了极大的担忧。迫切需要开发更便宜,更快,更简单,敏感和特定的分子检测方法,以识别和监测可转移的抗性决定簇的传播。方法和结果:本文,设计了八对引物以建立多重PCR方法,用于快速有效地测定报告的MCR基因。该测定可以在85分钟内给出结果(35分钟的放大,电泳50分钟)。我们通过在耐菌落抗性分离物中测试MCR基因的存在来验证该测定的可行性。结论:我们的多重PCR技术鉴于明确的鉴定,放大效率以及检测效率的效率,因此对质粒介导的乳蛋白抗性的监测和流行病学研究有用,特别是对于资源不足的实验室。

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