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Comparison of an Internally Controlled Large-Volume LightCycler Assay for Detection of Mycobacterium tuberculosis in Clinical Samples with the COBAS AMPLICOR Assay

机译:使用COBAS AMPLICOR测定法比较用于临床样品中结核分枝杆菌检测的内部控制大容量LightCycler测定法的比较

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摘要

We present a sensitive and specific assay for reliable and flexible detection of members of the Mycobacterium tuberculosis complex (MTBC) in clinical samples. This real-time PCR assay, which uses the LightCycler 2.0 instrument and 100-μl glass capillaries, can provide a result within 1 h after DNA extraction. The primers amplify a 206-bp fragment of the MTBC 16S rRNA gene. The sensor hybridization probe targets a region highly specific to members of the MTBC. The assay also includes a novel type of internal control that monitors the function of the reaction components and can detect potential inhibitors. Template DNA was extracted by the same procedure used for the COBAS AMPLICOR M. tuberculosis assay, so the LightCycler assay could be directly compared to the COBAS AMPLICOR assay. The LightCycler assay was evaluated with 146 clinical samples of various types. Very good agreement (100% sensitivity, 98.6% specificity) could be shown between the LightCycler and COBAS AMPLICOR assays. Specificity was checked with a panel of nontuberculous mycobacteria, as well as a large panel of bacterial and fungal organisms.
机译:我们提出了一种灵敏而特异性的检测方法,用于可靠,灵活地检测临床样品中结核分枝杆菌复合物(MTBC)成员。该实时PCR分析使用LightCycler 2.0仪器和100μl玻璃毛细管,可在DNA提取后1小时内提供结果。引物扩增MTBC 16S rRNA基因的206 bp片段。传感器杂交探针靶向MTBC成员高度特异的区域。该测定还包括新型类型的内部对照,其监控反应组分的功能并可以检测潜在的抑制剂。模板DNA的提取方法与COBAS AMPLICOR结核分枝杆菌测定方法相同,因此可以将LightCycler测定法与COBAS AMPLICOR测定法直接比较。使用146种不同类型的临床样品对LightCycler分析进行了评估。在LightCycler和COBAS AMPLICOR分析之间可以显示出非常好的一致性(100%灵敏度,98.6%特异性)。用一组非结核分枝杆菌以及一大批细菌和真菌生物检查特异性。

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