A New Lab Developed Real Time PCR Assay for Direct Detection of C. Difficle from Stool Sample without DNA Extraction

Brandon Y. Li
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Abstract

Clostridium difficile is a major cause of nosocomial antibiotic-associated infectious diarrhea and pseudomembranous colitis. Detection of C. difficile by anaerobic bacterial culture and/or cytotoxicity assays has been largely replaced by rapid enzyme immunoassays (EIA). However, due to the lack of sensitivity of stool EIA, we developed a multiplex real-time PCR assay targeting the C. difficile toxin genes tcdB. stool samples from hospitalized pediatric patients suspected of having C. difficile-associated disease were prospectively collected. Three testing modalities were evaluated, including enriched culture, cepheid Xpert and real-time Pcr (tcdB) on stool samples performed with tcdB gene-specific primers and hydrolysis probes. A total of 150 de-identified clinical specimen were analyzed. The sensitivities of stool real-time Pcr were 95% against cepheid Xpert C. difficile and 93% against enriched culture respectively, with a specificity of 97% and 94%. The lower limit of detection of the stool real-time PCR was 0.5 cFU/ml of per reaction for tcdB. Direct detection of C. difficile toxin genes in stool samples by real-time Pcr showed performance comparable to enriched culture. Real-time PCR of DNA from stool samples is a rapid and cost-effective diagnostic modality for patients that should facilitate appropriate patient management.
建立了一种无需提取DNA直接检测粪便中艰难梭菌的实时PCR方法
艰难梭菌是院内抗生素相关感染性腹泻和假膜性结肠炎的主要原因。通过厌氧细菌培养和/或细胞毒性试验检测艰难梭菌已在很大程度上被快速酶免疫测定(EIA)所取代。然而,由于粪便EIA缺乏敏感性,我们开发了一种针对艰难梭菌毒素基因tcdB的多重实时PCR检测方法。前瞻性收集怀疑患有艰难梭菌相关疾病的住院儿科患者的粪便样本。利用tcdB基因特异性引物和水解探针对粪便样本进行富集培养、造父变星Xpert和实时Pcr (tcdB)三种检测方式进行评估。对150例去鉴定临床标本进行分析。粪便实时Pcr对造父变星Xpert艰难梭菌的敏感性为95%,对富集培养物的敏感性为93%,特异性为97%和94%。粪便实时荧光定量PCR对tcdB的检测下限为0.5 cFU/ml。通过实时荧光定量Pcr直接检测粪便样品中的艰难梭菌毒素基因,其性能与富集培养相当。对患者而言,粪便样本DNA的实时PCR是一种快速且具有成本效益的诊断方式,应有助于对患者进行适当的管理。
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