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[Identification and evaluation of a new nucleic acid amplification test target for specific detection of Mycobacterium tuberculosis complex]. | LitMetric
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[Identification and evaluation of a new nucleic acid amplification test target for specific detection of Mycobacterium tuberculosis complex].

Shi-hui Gao Ying-wei Zhao Zhong-yi Hu Jie Wang Jun-mei Lu Li-ping Yan Qi Guo Hui Ma Lian-hua Qin

Zhonghua Jie He He Hu Xi Za Zhi

Shanghai Key Laboratory of Tuberculosis, Shanghai Pulmonary Hospital, Tongji University School of Medicine, Shanghai 200433, China.

Published: December 2012

AI Article Synopsis

  • The study aimed to find a new nucleic acid amplification test target for accurately detecting Mycobacterium tuberculosis complex (MTC).
  • Using ISSR genotyping technology, researchers obtained a specific 588 bp fragment from the MTC genome and designed primer pairs to test various mycobacterial strains.
  • Results showed that the new test could effectively distinguish MTC strains from non-tuberculous mycobacteria, with high accuracy in identifying MTC using the developed primer pairs.

Article Abstract

Objective: To identify and evaluate a new nucleic acid amplification (NAA) test target for specific detection of Mycobacterium tuberculosis (MTB) complex (MTC).

Methods: MTC-specific fragment was obtained by ISSR genotyping technology. Primer pairs were designed based on the sequences of MTC-specific fragment and tested in 211 mycobacterial strains including 107 MTC strains and 104 nontuberculous mycobacteria (NTM) strains. IS6110 element (specific identification of MTC strains) and 16s rRNA gene (specific identification of Mycobacterium) amplification were used as a control to evaluate the efficacy of the NAA test target in the detection of MTC strains.

Results: One MTC-specific fragment with the length of 588 bp, located in 315947 - 316534 of the genome from MTB reference strain H(37) Rv, were obtained, cloned and sequenced. MTC-specific primer pairs MTCF/R were designed based on these sequences. All 211 mycobacterial strains accurately produced the genus-specific 16s rRNA amplicon. All MTC strains were positive in the MTCF/R PCR amplification while 99% MTC strains (106/107) were positive in the amplification of IS6110 sequences. All NTM strains were negative in both IS6110 and MTCF/R PCR amplification.

Conclusions: The MTC-specific fragment developed in this study can be used as a new NAA test target to correctly distinguish MTC from NTM.

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