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采用高分辨率熔解曲线分析快速检测结核分枝杆菌临床分离株中的异烟肼、利福平及氧氟沙星耐药性。

Rapid detection of isoniazid, rifampin, and ofloxacin resistance in Mycobacterium tuberculosis clinical isolates using high-resolution melting analysis.

机构信息

Centre for Infectious Diseases and Microbiology-Public Health, Institute of Clinical Pathology and Medical Research, Westmead, New South Wales, Australia.

出版信息

J Clin Microbiol. 2011 Oct;49(10):3450-7. doi: 10.1128/JCM.01068-11. Epub 2011 Aug 10.

Abstract

A high-resolution melting analysis (HRMA) assay was developed to detect isoniazid, rifampin, and ofloxacin resistance in Mycobacterium tuberculosis by targeting resistance-associated mutations in the katG, mabA-inhA promoter, rpoB, and gyrA genes. A set of 28 (17 drug-resistant and 11 fully susceptible) clinical M. tuberculosis isolates was selected for development and evaluation of HRMA. PCR amplicons from the katG, mabA-inhA promoter, rpoB, and gyrA genes of all 28 isolates were sequenced. HRMA results matched well with 18 mutations, identified by sequencing, in 17 drug-resistant isolates and the absence of mutations in 11 susceptible isolates. Among 87 additional isolates with known resistance phenotypes, HRMA identified katG and/or mabA-inhA promoter mutations in 66 of 69 (95.7%) isoniazid-resistant isolates, rpoB mutations in 51 of 54 (94.4%) rifampin-resistant isolates, and gyrA mutations in all of 41 (100%) ofloxacin-resistant isolates. All mutations within the HRMA primer target regions were detected as variant HRMA profiles. The corresponding specificities were 97.8%, 100%, and 98.6%, respectively. Most false-positive results were due to synonymous mutations, which did not affect susceptibility. HRMA is a rapid, sensitive method for detection of drug resistance in M. tuberculosis which could be used routinely for screening isolates in countries with a high prevalence of tuberculosis and drug resistance or in individual isolates when drug resistance is suspected.

摘要

建立了一种高分辨率熔解分析(HRMA)assay,通过针对 katG、mabA-inhA 启动子、rpoB 和 gyrA 基因中的耐药相关突变,检测结核分枝杆菌中的异烟肼、利福平、和氧氟沙星耐药性。选择了一组 28 个(17 个耐药和 11 个完全敏感)临床结核分枝杆菌分离株,用于 HRMA 的开发和评估。对所有 28 个分离株的 katG、mabA-inhA 启动子、rpoB 和 gyrA 基因的 PCR 扩增子进行测序。HRMA 结果与 17 个耐药分离株的 18 个测序鉴定的突变以及 11 个敏感分离株的无突变吻合良好。在 87 个具有已知耐药表型的额外分离株中,HRMA 在 66 个(95.7%)异烟肼耐药分离株中鉴定出 katG 和/或 mabA-inhA 启动子突变,在 51 个(94.4%)利福平耐药分离株中鉴定出 rpoB 突变,在所有 41 个(100%)氧氟沙星耐药分离株中鉴定出 gyrA 突变。HRMA 引物靶区内的所有突变均被检测为变异 HRMA 图谱。相应的特异性分别为 97.8%、100%和 98.6%。大多数假阳性结果是由于同义突变,这不影响药敏性。HRMA 是一种快速、敏感的检测结核分枝杆菌耐药性的方法,可在结核病和耐药性高发国家常规用于筛选分离株,也可在怀疑耐药性时用于单个分离株。

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