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A novel subtyping assay for detection of clostridium difficile virulence genes

机译:用于检测艰难梭菌毒力基因的新型亚型分析

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摘要

This proof-of-concept study demonstrates the application of a novel nucleic acid detection platform to detect Clostridium difficile in subjects presenting with acute diarrheal symptoms. This method amplifies three genes associated with C. difficile infection, including genes and deletions (cdtB and tcdC) associated with hypervirulence attributed to the NAP1/027/BI strain. Amplification of DNA from the tcdB, tcdC, and cdtB genes was performed using a droplet-based sandwich platform with quantitative real-time PCR in microliter droplets to detect and identify the amplified fragments of DNA. The device and identification system are simple in design and can be integrated as a point-of-care test to help rapidly detect and identify C. difficile strains that pose significant health threats in hospitals and other health-care communities.
机译:这项概念验证研究证明了新型核酸检测平台在患有急性腹泻症状的受试者中检测艰难梭菌的应用。此方法扩增了与艰难梭菌感染相关的三个基因,包括与归因于NAP1 / 027 / BI菌株的高毒力相关的基因和缺失(cdtB和tcdC)。使用基于液滴的夹心平台和定量实时PCR在微升液滴中检测tcdB,tcdC和cdtB基因的DNA,以检测和鉴定DNA的扩增片段。该设备和识别系统设计简单,可以集成为即时检验,以帮助快速检测和识别艰难梭菌菌株,这些菌株对医院和其他医疗保健领域构成重大健康威胁。

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