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首页> 外文期刊>Journal of Clinical Microbiology >Assessment of Two New Molecular Methods for Identification of Candida parapsilosis Sensu Lato Species
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Assessment of Two New Molecular Methods for Identification of Candida parapsilosis Sensu Lato Species

机译:鉴定两种新型分子鉴定假丝酵母念珠菌的方法

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Candida parapsilosis sensu stricto, C. orthopsilosis, and C. metapsilosis replaced C. parapsilosis groups I, II, and III in 2005. Since then, an increased interest in studying their epidemiology has arisen based on the observed differences in antifungal susceptibilities and virulence the three species. A strict differentiation of these species cannot be achieved by phenotypic methods. We evaluate two new molecular methodologies to differentiate among these species by the use of a collection of 293 bloodstream infection isolates of C. parapsilosis sensu lato. For the first method, the isolates were studied using PCR amplification of a fragment of the C. parapsilosis sensu lato FKS1 gene and a universal primer pair followed by EcoRI enzyme digestion. The other method used the allele discrimination ability of molecular beacons in a multiplex real-time PCR format. Both methods of identification showed 100% concordance with internal transcribed spacer 1 (ITS1)/ITS2 sequencing and proved to be effective for clinical applications, even with mixed-species DNAs.
机译:念珠菌性念珠菌,正念念珠菌和间位念珠菌在2005年取代了副念珠菌I,II和III组。从那时起,基于观察到的抗真菌药敏性和毒力的差异,人们对其研究流行病学的兴趣日益浓厚。三种。这些物种的严格区分不能通过表型方法实现。我们评估了两种新的分子方法,以通过使用293种C. parapsilosis sensu lato血流感染分离株的集合来区分这些物种。对于第一种方法,分离株的研究是使用PCR扩增副翼念珠菌 FKS1 基因片段和通用引物对,然后进行EcoRI酶消化。另一种方法是使用多重实时PCR格式的分子信标的等位基因识别能力。两种鉴定方法均显示出与内部转录间隔区1(ITS1)/ ITS2测序的100%一致性,并且即使对于混合物种DNA也被证明对临床应用有效。

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