比较环介导等温扩增与常规 PCR 检测对常见布鲁氏菌属的诊断价值。
Comparison of loop-mediated isothermal amplification and conventional PCR tests for diagnosis of common Brucella species.
机构信息
Department of Microbiology, Faculty of Medicine, Babol University of Medical Sciences, Babol, Iran.
Infectious Diseases and Tropical Medicine Research Center, Babol University of Medical Sciences, Babol, Iran.
出版信息
BMC Res Notes. 2020 Nov 13;13(1):533. doi: 10.1186/s13104-020-05377-8.
OBJECTIVE
Rapid, reliable, and affordable detection of Brucella species via the molecular methods remains a challenge. In recent years, loop-mediated isothermal amplification (LAMP) is a functional nucleic acid amplification technique offering a substitute to polymerase chain reaction (PCR). So, we compared the LAMP assay with the conventional PCR for the identification of common Brucella species in Iran. In this study, LAMP assay was comprehensively evaluated against the common PCR method. A group of specific LAMP primers were used to amplify a highly specific fragment from the sequence of the Brucella abortus, bcsp31 gene. Sensitivity and specificity values of tests were done with a set of 78 (50 Brucella and 28 non-Brucella) strains.
RESULTS
A dilution series of B. abortus DNA indicated that the LAMP reaction could reliably detect 10 (fg/µl) DNA target copies per reaction within 36 min, which is 10 times greater than the PCR assay. In summary, we conclude that LAMP assay provide accurate and fast test results to identify of common Brucella species in low-complexity labs, mainly in low and lower middle income countries.
目的
通过分子方法快速、可靠且经济实惠地检测布鲁氏菌属物种仍然是一项挑战。近年来,环介导等温扩增(LAMP)是一种功能性核酸扩增技术,可为聚合酶链反应(PCR)提供替代方法。因此,我们将 LAMP 检测法与常规 PCR 进行了比较,以鉴定伊朗常见的布鲁氏菌属物种。在这项研究中,我们全面评估了 LAMP 检测法与常规 PCR 方法的对比。一组特定的 LAMP 引物被用于扩增来自布鲁氏菌属 abortus 菌株 bcsp31 基因的高度特异性片段。通过一组 78 株(50 株布鲁氏菌和 28 株非布鲁氏菌)菌株进行了测试的敏感性和特异性值。
结果
B. abortus DNA 的稀释系列表明,LAMP 反应可以在 36 分钟内可靠地检测到每个反应 10 fg/µl 的 DNA 靶标拷贝,比 PCR 检测法高 10 倍。总之,我们得出结论,LAMP 检测法为鉴定低复杂度实验室中的常见布鲁氏菌属物种提供了准确、快速的检测结果,主要是在低收入和中下收入国家。
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