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Chinese Journal of Antituberculosis ›› 2025, Vol. 47 ›› Issue (6): 687-693.doi: 10.19982/j.issn.1000-6621.20250031

• Original Articles • Previous Articles     Next Articles

Multicenter evaluation study on the application of a novel PCR fluorescence probe technology for early diagnosis of tuberculosis

Ou Xichao1, Teng Chong2, Song Yuanyuan1, Zheng Yang1, Chen Lei3, Zhu Jun4, Wang Jianguo5, Pan Zhaobao3, Kang Haitao4, Wang Yan5, Yao Hongyan6, Huang Fei1()   

  1. 1National Key Laboratory of Intelligent Tracking and Forecasting for Infectious Diseases, National Center for Tuberculosis Control and Prevention, Chinese Center for Disease Control and Prevention, Beijing 102206, China
    2Department of Tuberculosis, Beijing Dongcheng District Center for Disease Control and Prevention, Public Health Emergency Management Innovation Center, Beijing 100050, China
    3Department of Laboratory Medicine, The Second People’s Hospital of Weifang, Shandong Province, Weifang 261041, China
    4Clinical Laboratory, Zhoukou Communicable Disease Hospital (Zhoukou Tuberculosis Dispensary), Henan Province, Zhoukou 466001, China
    5Clinical Laboratory, Affiliated Hospital of Hebei University, Baoding 071000, China
    6Department of Education and Training, Chinese Center for Disease Control and Prevention, Beijing 102206, China
  • Received:2025-01-20 Online:2025-06-10 Published:2025-06-11
  • Contact: Huang Fei, Email: huangfei@chinacdc.cn
  • Supported by:
    National Key Research and Development Program(2022YFC2305204);National Key Research and Development Program(2023YFC2307301);Key Research and Development Plan of Xizang Autonomous Region(XZ202201ZY0007N-01);2528 Tuberculosis Prevention and Control Project

Abstract:

Objective: To evaluate the reliability of the novel PCR fluorescence probe technique (DiagMed qPCR, abbreviated as “qPCR”) in diagnosing tuberculosis among tuberculosis suspected patients and provide foundational data support for its clinical application in early tuberculosis diagnosis. Methods: Prospective studies were conducted at The Second People’s Hospital of Weifang, Zhoukou Communicable Disease Hospital, and Affiliated Hospital of Hebei University. Patients meeting inclusion criteria who presented with suspected initial TB diagnosis between June and October 2024 were consecutively enrolled. Laboratory staff performed smear staining microscopy, MGIT 960 liquid culture, GeneXpert MTB/RIF (abbreviated as “Xpert”), and qPCR on sputum or bronchoalveolar lavage fluid (BALF) samples from enrolled patients. Results: A total of 563 patients with suspected initial TB diagnosis were included. The smear microscopy positivity rate was 38.01% (214/563), liquid culture positivity rate was 50.80% (286/563), Xpert positivity rate was 54.53% (307/563), and qPCR positivity rate was 58.79% (331/563). Both qPCR and Xpert positivity rates were significantly higher than that of liquid culture (χ2=22.000, P<0.001; χ2=9.468, P=0.003). Using liquid culture as the reference standard, qPCR demonstrated a sensitivity of 92.31% (264/286) and specificity of 75.74% (206/272), while Xpert showed a sensitivity of 91.07% (255/280) and specificity of 80.60% (216/268). Using clinical diagnosis as the reference standard, qPCR exhibited a sensitivity of 68.05% (328/482) and specificity of 96.30% (78/81), whereas Xpert demonstrated a sensitivity of 65.04% (307/472) and specificity of 100.00% (78/78). Conclusion: The qPCR technique demonstrates excellent diagnostic performance for Mycobacterium tuberculosis detection. It can be utilized for active case finding in key populations and for early TB diagnosis in general healthcare institutions and designated TB medical facilities.

Key words: Mycobacterium tuberculosis, Polymerase chain reaction, Diagnosis, differential, Evaluation studies

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