Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection

Background: Several nucleic acid amplification techniques (IS6110, 16S rRNA, and 85B mRNA) were developed for the rapid, direct detection of Mycobacterium tuberculosis. We aimed to assess the diagnostic performance of 85B mRNA-based RT-qPCR by comparing with the real-time PCR COBAS TaqMan MTB Kit wh...

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Main Authors: Mehmet Demirci, Suat Saribas, Nigar Ozer, Sezer Toprak, Emel Caglar, Gonenc Ortakoylu, Pelin Yuksel, Gulsel Ayaz, Hrisi B. Tokman, Omer Uysal, Harika O. Dinc, Tevhide Ziver, Bekir Kocazeybek
Format: Article
Language:English
Published: Elsevier 2018-09-01
Series:Journal of Infection and Public Health
Online Access:http://www.sciencedirect.com/science/article/pii/S1876034118300273
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spelling doaj-49c08f9c6f6240f39cffedd585ef6cf82020-11-25T02:26:50ZengElsevierJournal of Infection and Public Health1876-03412018-09-01115662666Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infectionMehmet Demirci0Suat Saribas1Nigar Ozer2Sezer Toprak3Emel Caglar4Gonenc Ortakoylu5Pelin Yuksel6Gulsel Ayaz7Hrisi B. Tokman8Omer Uysal9Harika O. Dinc10Tevhide Ziver11Bekir Kocazeybek12Beykent University Medical Faculty, Department of Medical Microbiology, Istanbul, TurkeyIstanbul University, Cerrahpasa Medical Faculty, Department of Medical Microbiology, Istanbul, TurkeyIstanbul University, Cerrahpasa Medical Faculty, Department of Medical Microbiology, Istanbul, TurkeyYedikule Chest Disease Education and Research Hospital, Istanbul, TurkeyYedikule Chest Disease Education and Research Hospital, Istanbul, TurkeyYedikule Chest Disease Education and Research Hospital, Istanbul, TurkeyIstanbul University, Cerrahpasa Medical Faculty, Department of Medical Microbiology, Istanbul, TurkeyCerrahpasa Medical Faculty, Department of Medical Biology, Istanbul, TurkeyIstanbul University, Cerrahpasa Medical Faculty, Department of Medical Microbiology, Istanbul, TurkeyDepartment of Biostatistics, Medical School of Bezmialem Vakif University, Istanbul, TurkeyIstanbul University, Cerrahpasa Medical Faculty, Department of Medical Microbiology, Istanbul, TurkeyEastern Mediterranean University Faculty of Health Sciences, Nutrition and Dietetic Department, Famagusta, CyprusIstanbul University, Cerrahpasa Medical Faculty, Department of Medical Microbiology, Istanbul, Turkey; Corresponding author at: Istanbul University, Cerrahpasa Faculty of Medicine, Department of Medical Microbiology, Cerrahpasa Street, 34098 Istanbul, Turkey.Background: Several nucleic acid amplification techniques (IS6110, 16S rRNA, and 85B mRNA) were developed for the rapid, direct detection of Mycobacterium tuberculosis. We aimed to assess the diagnostic performance of 85B mRNA-based RT-qPCR by comparing with the real-time PCR COBAS TaqMan MTB Kit while using the BACTEC MGIT 960 method as the gold standard. Methods: 60 patients with confirmed pulmonary TB and 60 individuals without TB were included as the study and control groups, respectively. Sputum specimens were cultured using LJ and BACTEC MGIT 960 systems. Extracted DNA was used for COBAS PCR in a CONAS TaqMan 48 analyzer. 85B mRNA detection was performed by RT-qPCR. Results: The sensitivity, specificity, positive predictive value, negative predictive value, and accuracy of COBAS TaqMan MTB Test were detected as 93.3%, 83.3%, 84.8%, 92.6%, and 88.3%, respectively. The same diagnostic parameters of RT-qPCR were: 98.3%, 95.0%, 95.2%, 98.3%, and 96.7%, respectively. According to the binary logistic regression analysis, RT-qPCR (OR: 19,924, p < 0.001) was identified as the more optimal test. Conclusion: RT-qPCR targeting the 85B gene of M. tuberculosis seems to be a more useful and rapid technique than DNA-based methods for detecting live M. tuberculosis bacilli from sputum specimens. Keywords: 85B mRNA, Mycobacterium tuberculosis, RT-qPCR, BACTEC MGIT 960http://www.sciencedirect.com/science/article/pii/S1876034118300273
collection DOAJ
language English
format Article
sources DOAJ
author Mehmet Demirci
Suat Saribas
Nigar Ozer
Sezer Toprak
Emel Caglar
Gonenc Ortakoylu
Pelin Yuksel
Gulsel Ayaz
Hrisi B. Tokman
Omer Uysal
Harika O. Dinc
Tevhide Ziver
Bekir Kocazeybek
spellingShingle Mehmet Demirci
Suat Saribas
Nigar Ozer
Sezer Toprak
Emel Caglar
Gonenc Ortakoylu
Pelin Yuksel
Gulsel Ayaz
Hrisi B. Tokman
Omer Uysal
Harika O. Dinc
Tevhide Ziver
Bekir Kocazeybek
Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection
Journal of Infection and Public Health
author_facet Mehmet Demirci
Suat Saribas
Nigar Ozer
Sezer Toprak
Emel Caglar
Gonenc Ortakoylu
Pelin Yuksel
Gulsel Ayaz
Hrisi B. Tokman
Omer Uysal
Harika O. Dinc
Tevhide Ziver
Bekir Kocazeybek
author_sort Mehmet Demirci
title Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection
title_short Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection
title_full Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection
title_fullStr Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection
title_full_unstemmed Diagnostic performance of the RT-qPCR method targeting 85B mRNA in the diagnosis of pulmonary Mycobacterium tuberculosis infection
title_sort diagnostic performance of the rt-qpcr method targeting 85b mrna in the diagnosis of pulmonary mycobacterium tuberculosis infection
publisher Elsevier
series Journal of Infection and Public Health
issn 1876-0341
publishDate 2018-09-01
description Background: Several nucleic acid amplification techniques (IS6110, 16S rRNA, and 85B mRNA) were developed for the rapid, direct detection of Mycobacterium tuberculosis. We aimed to assess the diagnostic performance of 85B mRNA-based RT-qPCR by comparing with the real-time PCR COBAS TaqMan MTB Kit while using the BACTEC MGIT 960 method as the gold standard. Methods: 60 patients with confirmed pulmonary TB and 60 individuals without TB were included as the study and control groups, respectively. Sputum specimens were cultured using LJ and BACTEC MGIT 960 systems. Extracted DNA was used for COBAS PCR in a CONAS TaqMan 48 analyzer. 85B mRNA detection was performed by RT-qPCR. Results: The sensitivity, specificity, positive predictive value, negative predictive value, and accuracy of COBAS TaqMan MTB Test were detected as 93.3%, 83.3%, 84.8%, 92.6%, and 88.3%, respectively. The same diagnostic parameters of RT-qPCR were: 98.3%, 95.0%, 95.2%, 98.3%, and 96.7%, respectively. According to the binary logistic regression analysis, RT-qPCR (OR: 19,924, p < 0.001) was identified as the more optimal test. Conclusion: RT-qPCR targeting the 85B gene of M. tuberculosis seems to be a more useful and rapid technique than DNA-based methods for detecting live M. tuberculosis bacilli from sputum specimens. Keywords: 85B mRNA, Mycobacterium tuberculosis, RT-qPCR, BACTEC MGIT 960
url http://www.sciencedirect.com/science/article/pii/S1876034118300273
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