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通过整合基因到蛋白质功能的方法,快速检测痰标本中与 pncA 突变相关的结核分枝杆菌和吡嗪酰胺药敏性。

Rapid detection of Mycobacterium tuberculosis and pyrazinamide susceptibility related to pncA mutations in sputum specimens through an integrated gene-to-protein function approach.

机构信息

State Key Laboratory of Virology, Wuhan Institute of Virology, Chinese Academy of Sciences, Wuhan, China.

出版信息

J Clin Microbiol. 2014 Jan;52(1):260-7. doi: 10.1128/JCM.02285-13. Epub 2013 Nov 13.

Abstract

Testing the pyrazinamide (PZA) susceptibility of Mycobacterium tuberculosis isolates is challenging. In a previous paper, we described the development of a rapid colorimetric test for the PZA susceptibility of M. tuberculosis by a PCR-based in vitro-synthesized-pyrazinamidase (PZase) assay. Here, we present an integrated approach to detect M. tuberculosis and PZA susceptibility directly from sputum specimens. M. tuberculosis was detected first, using a novel long-fragment quantitative real-time PCR (LF-qPCR), which amplified a fragment containing the whole pncA gene. Then, the positive amplicons were sequenced to find mutations in the pncA gene. For new mutations not found in the Tuberculosis Drug Resistance Mutation Database (www.tbdreamdb.com), the in vitro PZase assay was used to test the PZA resistance. This approach could detect M. tuberculosis within 3 h with a detection limit of 7.8 copies/reaction and report the PZA susceptibility within 2 days. In an initial testing of 213 sputum specimens, the LF-qPCR found 53 positive samples with 92% sensitivity and 97% specificity compared to the culture test for M. tuberculosis detection. DNA sequencing of the LF-qPCR amplicons revealed that 49 samples were PZA susceptible and 1 was PZA resistant. In the remaining 3 samples, with new pncA mutations, the in vitro PZase assay found that 1 was PZA susceptible and 2 were PZA resistant. This integrated approach provides a rapid, efficient, and relatively low-cost solution for detecting M. tuberculosis and PZA susceptibility without culture.

摘要

测试分枝杆菌属结核分枝杆菌分离株的吡嗪酰胺(PZA)敏感性具有挑战性。在之前的一篇论文中,我们描述了一种基于 PCR 的体外合成吡嗪酰胺酶(PZase)测定法,用于快速比色法检测分枝杆菌属结核分枝杆菌的 PZA 敏感性。在这里,我们提出了一种从痰标本中直接检测分枝杆菌属结核分枝杆菌和 PZA 敏感性的综合方法。首先,使用一种新的长片段定量实时 PCR(LF-qPCR)检测分枝杆菌属结核分枝杆菌,该 PCR 扩增包含整个 pncA 基因的片段。然后,对阳性扩增子进行测序以发现 pncA 基因中的突变。对于在结核病耐药基因突变数据库(www.tbdreamdb.com)中未发现的新突变,使用体外 PZase 测定法测试 PZA 耐药性。这种方法可以在 3 小时内检测到分枝杆菌属结核分枝杆菌,检测限为 7.8 拷贝/反应,并在 2 天内报告 PZA 敏感性。在对 213 份痰标本的初步测试中,LF-qPCR 发现 53 份阳性样本,与分枝杆菌属结核分枝杆菌检测的培养试验相比,敏感性为 92%,特异性为 97%。LF-qPCR 扩增子的 DNA 测序显示,49 份样本对 PZA 敏感,1 份样本对 PZA 耐药。在其余 3 份样本中,有新的 pncA 突变,体外 PZase 测定法发现 1 份样本对 PZA 敏感,2 份样本对 PZA 耐药。这种综合方法提供了一种快速、高效且相对低成本的解决方案,无需培养即可检测分枝杆菌属结核分枝杆菌和 PZA 敏感性。

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