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艰难梭菌感染的实验室检测:隧道尽头的曙光。

Laboratory testing for Clostridium difficile infection: light at the end of the tunnel.

机构信息

Department of Medicine, NorthShore University HealthSystem, University of Chicago, Evanston, IL, USA.

出版信息

Am J Clin Pathol. 2011 Sep;136(3):372-80. doi: 10.1309/AJCPTP5XKRSNXVIL.

Abstract

Clostridium difficile infection (CDI) is changing as evidenced by increasing virulence, rising incidence, unresponsiveness to metronidazole therapy, and worse outcomes. Thus, it is critical that CDI diagnosis be accurate so ongoing epidemiology, disease prevention, and treatment remain satisfactory. We tested 10 diagnostic assays, including 1 commercial real-time polymerase chain reaction (qPCR) test for the laboratory detection of toxigenic C difficile on 1,000 stool samples. Sensitive culture for toxigenic C difficile using 2 types of media with broth enrichment defined the reference standard. For the study, 1,000 tests were performed on samples from 919 patients. Of the samples, 146 contained evidence for toxigenic C difficile and represented the true-positive results. Only the US Food and Drug Administration-cleared qPCR assay (Becton Dickinson, Franklin Lakes, NJ) and 1 glutamate dehydrogenase test (TechLab, Blacksburg, VA) were not statistically inferior to culture in sensitivity. The common enzyme immunoassay tests all had sensitivity values less than 50%. Clinical laboratory professionals need to seriously consider their diagnostic testing and use the assays that perform best for the detection of CDI.

摘要

艰难梭菌感染(CDI)正在发生变化,其表现为毒力增加、发病率上升、对甲硝唑治疗无反应以及预后更差。因此,准确诊断 CDI 至关重要,这样才能持续进行流行病学、疾病预防和治疗。我们测试了 10 种诊断检测方法,包括针对实验室检测产毒艰难梭菌的一种商业实时聚合酶链反应(qPCR)检测法,共对 1000 份粪便样本进行了检测。采用两种含肉汤增菌的培养基进行产毒艰难梭菌的敏感培养,将其作为参考标准。在这项研究中,对 919 名患者的 1000 个样本进行了检测。在这些样本中,有 146 份样本含有产毒艰难梭菌的证据,这是真正的阳性结果。只有美国食品和药物管理局批准的 qPCR 检测法(Becton Dickinson,Franklin Lakes,NJ)和 1 种谷氨酸脱氢酶检测法(TechLab,Blacksburg,VA)在敏感性方面与培养法没有统计学差异。常见的酶联免疫吸附试验检测法的敏感性值均小于 50%。临床实验室专业人员需要认真考虑他们的诊断检测,并使用性能最佳的检测法来检测 CDI。

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