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快速检测耐异烟肼和/或利福平的结核分枝杆菌菌株:多重聚合酶链反应分析的标准化

Rapid Detection of Mycobacterium tuberculosis Strains Resistant to Isoniazid and/or Rifampicin: Standardization of Multiplex Polymerase Chain Reaction Analysis.

作者信息

Collantes Jimena, Solari Francesca Barletta, Rigouts Leen

机构信息

Instituto de Medicina Tropical Alexander von Humboldt, Lima, Peru.

Universidad Peruana Cayetano Heredia, Lima, Peru.

出版信息

Am J Trop Med Hyg. 2016 Dec 7;95(6):1257-1264. doi: 10.4269/ajtmh.16-0120. Epub 2016 Oct 24.

DOI:10.4269/ajtmh.16-0120
PMID:27928076
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5154436/
Abstract

Drug susceptibility testing using molecular techniques can enhance the identification of drug-resistant Mycobacterium tuberculosis Two multiplex real-time polymerase chain reaction (qPCR) assays were developed to detect the most common resistance-associated mutations to isoniazid (katGS315T, inhA-15C → T), and rifampicin (rpoBH526Y and rpoBS531L). To assess the species specificity of the qPCR, we selected 31 nontuberculous mycobacteria (NTM) reference strains belonging to 17 species from the public collection of mycobacterial cultures (BCCM/ITM). Additionally, we tested 17 isoniazid and/or rifampicin-resistant strains with other mutations in the target genes to assess mutation specificity. The limit of detection for all the targeted mutations was 20 bacilli/reaction. Multiplex 1 showed 90%, 95%, and 100% efficiency for wild type (WT), Mut katGS315T, and Mut rpoBS531L, respectively; whereas Multiplex 2 showed 97%, 94%, and 90% efficiency for WT, Mut inhA-15, and Mut rpoBH526Y, respectively. Three of 17 strains that presented other mutations in the target genes were identified as rifampicin resistant and only 3/31 NTM showed a similar melting temperature to rpoBL531 and/or katGT315 mutants. Thus, our proposed cascade of specific tuberculosis detection followed by drug resistance testing showed sensitivities for katGS315T, rpoBS531L, rpoBH526Y, and inhA-15 detection of 100%, 100%, 100%, and 96%, respectively; and specificities of 98%, 95%, 100%, and 100, respectively.

摘要

使用分子技术进行药物敏感性测试可以提高对耐药结核分枝杆菌的识别。开发了两种多重实时聚合酶链反应(qPCR)检测方法,以检测与异烟肼(katGS315T、inhA - 15C→T)和利福平(rpoBH526Y和rpoBS531L)最常见的耐药相关突变。为了评估qPCR的物种特异性,我们从分枝杆菌培养物的公共收藏(BCCM/ITM)中选择了31株属于17个物种的非结核分枝杆菌(NTM)参考菌株。此外,我们测试了17株在靶基因中有其他突变的异烟肼和/或利福平耐药菌株,以评估突变特异性。所有靶向突变的检测限为20个杆菌/反应。多重检测1对野生型(WT)、突变型katGS315T和突变型rpoBS531L的检测效率分别为90%、95%和100%;而多重检测2对WT、突变型inhA - 15和突变型rpoBH526Y的检测效率分别为97%、94%和90%。在17株在靶基因中有其他突变的菌株中,有3株被鉴定为利福平耐药,只有3/31的NTM显示出与rpoBL531和/或katGT315突变体相似的熔解温度。因此,我们提出的先进行特异性结核检测然后进行耐药性测试的级联检测方法对katGS315T、rpoBS531L、rpoBH526Y和inhA - 15检测的敏感性分别为100%、100%、100%和96%;特异性分别为98%、95%、100%和100%。

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