应用多重PCR方法快速鉴定结核分枝杆菌复合群与非结核分枝杆菌的研究

中国防痨杂志 ›› 2013, Vol. 35 ›› Issue (9): 686-689.

应用多重PCR方法快速鉴定结核分枝杆菌复合群与非结核分枝杆菌的研究

王桂荣付育红梁倩尚媛媛姜广路赵立平于霞陈素婷黄海荣

101149 首都医科大学附属北京胸科医院北京市结核病胸部肿瘤研究所国家结核病临床实验室

收稿日期:2013-03-26 出版日期:2013-09-10 发布日期:2013-09-08
通信作者: 黄海荣 E-mail:hairong.huangcn@gmail.com
基金资助:
北京市自然科学基金（7132049）

Study on rapid differentiation of Mycobacterium tuberculosis complex from non-tuberculous mycobacteria by a multiplex PCR

WANG Gui-rong, FU Yu-hong, LIANG Qian, SHANG Yuan-yuan, JIANG Guang-lu, ZHAO Li-ping, YU Xia, CHEN Su-ting, HUANG Hai-rong

National Tuberculosis Clinical Laboratory, Beijing Tuberculosis and Thoracic Tumor Institute, Beijing Chest Hospital, Capital Medical University, Beijing 101149,China

Received:2013-03-26 Online:2013-09-10 Published:2013-09-08
Contact: HUANG Hai-rong E-mail:hairong.huangcn@gmail.com

摘要/Abstract

摘要： 目的建立并评估快速鉴定结核分枝杆菌复合群（MTBC）与非结核分枝杆菌（NTM）的多重PCR方法。方法应用分别针对MTBC的oxyR-ahpC基因间隔区、MTBC和NTM的rpoB基因可变区的3对分枝杆菌特异性引物进行多重PCR扩增，扩增产物分别为473 bp、235 bp和136 bp。应用该多重PCR方法对6株MTBC标准株、50株NTM标准株、312株MTBC临床分离株和300株NTM临床分离株进行了初步菌种鉴定。结果经多重PCR 扩增后进行凝胶电泳，MTBC标准株473 bp和235 bp片段均可见，NTM标准株仅见136 bp片段。312株MTBC临床分离株中，310株扩增出473 bp和235 bp片段，敏感度为99.36%（310/312），特异度为99.32%（294/296）；300株NTM临床分离株中，294株扩增出136 bp片段，敏感度为98.00%（294/300），特异度为100.00%（310/310）。结论该多重PCR方法可检测并鉴别MTBC及NTM，具有高度的特异度和敏感度，有可能作为鉴别MTBC与NTM的有价值的检测手段。

关键词: 分枝杆菌, 结核, 分枝杆菌属, 多重聚合酶链反应

Abstract: Objective To establish and evaluate a multiplex PCR technique to rapid differentiate Mycobacterium tuberculosis complex (MTBC) from non-tuberculous mycobacteria (NTM). Methods Three pairs of oligo nucleotide primers were used in the multiplex PCR reaction. A 473 bp DNA fragment encoding oxyR-ahpC intergenic region in MTBC, a 235 bp and 136 bp DNA fragment encoding variable rpoB gene region from MTBC and NTM, respectively, were amplified. The multiplex PCR was assessed in 6 reference strains of MTBC, 50 reference strains of NTM, 312 clinical strains of MTBC and 300 clinical strains of NTM. Results The multiplex PCR produced two DNA fragments at the size 473 bp and 235 bp for MTBC reference strains, and one DNA fragment with the size 136 bp for NTM reference strains. Among 312 MTBC clinical samples, the sensitivity was 99.36% (310/312) and specificity was 99.32% (294/296). Among 300 NTM clinical samples, the sensitivity and specificity were 98.00% (294/300) and 100.00% (310/310) respectively. Conclusion The multiplex PCR can differentiate MTBC and NTM efficiently, and might be a valuable technique for clinical use.

Key words: Mycobacterium tuberculosis, Mycobacterium, Multiplex polymerase chain reaction

王桂荣付育红梁倩尚媛媛姜广路赵立平于霞陈素婷黄海荣. 应用多重PCR方法快速鉴定结核分枝杆菌复合群与非结核分枝杆菌的研究[J]. 中国防痨杂志, 2013, 35(9): 686-689.

WANG Gui-rong, FU Yu-hong, LIANG Qian, SHANG Yuan-yuan, JIANG Guang-lu, ZHAO Li-ping, YU Xia, CHEN Su-ting, HUANG Hai-rong. Study on rapid differentiation of Mycobacterium tuberculosis complex from non-tuberculous mycobacteria by a multiplex PCR[J]. Chinese Journal of Antituberculosis, 2013, 35(9): 686-689.

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