Nested PCR in lung tissue for diagnosis of pulmonary tuberculosis

Kang, Young Ae; Kwon, Sung Youn; Yoon, Ho Il; Chung, Jin-Haeng; Lee, Choon-Taek; Lee, Jae Ho

doi:10.1183/09031936.00067209

Cited by 26 publications

(26 citation statements)

References 23 publications

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“…High sensitivity and specificity of real time PCR in diagnosing pulmonary tuberculosis has been reported by several studies although the sensitivity of PCR is lower in smear negative cases in comparison to the smear positive cases. [7][8][9] Seven of our cases )6.8%( which were AFB smear and culture MTB negative but were positive on PCR for MTB were treated with antituberculosis drugs with good clinico-radiological response thereby suggesting that PCR is also useful in some culture MTB negative patients to diagnose pulmonary tuberculosis ) Table 4(. PCR for MTB was falsely positive in only one patient with history of antituberculosis treatment in the last one year and this may have occurred due to cross contamination or due to the presence of dead bacilli in the patient.…”

Section: Resultsmentioning

confidence: 74%

Comparison of real time PCR with phenotypic methods in bronchoalveolar lavage in diagnosis of sputum smear negative pulmonary tuberculosis patients

et al. 2018

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Background: Early diagnosis of pulmonary tuberculosis is of utmost importance for proper control of the disease in the patient. Diagnosis of pulmonary tuberculosis is usually by acid fast bacilli (AFB) smear examination and culture Mycobacterium tuberculosis (MTB). In this study, we have employed polymerase chain reaction (PCR) for MTB in bronchoalveolar lavage (BAL) along with AFB smear and culture MTB for early diagnosis of pulmonary tuberculosis.Methods: A prospective observational study was conducted in the Department of Pulmonary Medicine, Era’s Lucknow medical college and Hospital, Lucknow over a period of two years. A total of 123 previously treated cases of pulmonary tuberculosis were enrolled for the study whose two sputum smear samples were negative for AFB. These patients underwent fibreoptic bronchoscopy and BAL was obtained which was sent for AFB smear, culture MTB and PCR for MTB.Results: The examination of BAL revealed the highest sensitivity for culture MTB at 87.4% followed by PCR for MTB at 73.8% and then AFB smear at 61.2%. PCR for MTB helped in diagnosing an additional 12% patients of pulmonary tuberculosis which were negative on AFB smear and an additional 6.8% patients which were negative on culture MTB.Conclusions: PCR for MTB is useful in making an early diagnosis of pulmonary tuberculosis especially in paucibacillary cases negative on AFB smear and also in some culture MTB negative patients.

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Section: Resultsmentioning

confidence: 74%

Comparison of real time PCR with phenotypic methods in bronchoalveolar lavage in diagnosis of sputum smear negative pulmonary tuberculosis patients

et al. 2018

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“…The recent WHOendorsed Xpert MTB/RIF assay (Cepheid, Sunnyvale, CA), has shown a sensitivity for nonrespiratory tissue specimens ranging from 53% to 100% and a specificity ranging from 97.3% to 100% (2,10,13,31). However, with various degrees of sensitivity being reported for different assays (8), the clinical utility of PCR-based tests for diagnosing EPTB in tissue samples is still uncertain (17). We investigated another molecular assay for application in diagnosing EPTB, the LightCycler mycobacterium detection assay (LCTB) (Roche Diagnostics, GmbH, Germany), which has the added advantage of simultaneously diagnosing three species, Mycobacterium tuberculosis, M. avium, and M. kansasii.…”

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confidence: 99%

“…Possibly, the poorer performance of the LCTB with other tissue types may be due to poor quality of tissues, uneven distribution of bacteria, difficulty in extracting M. tuberculosis DNA or loss of DNA during extraction, or the presence of PCR-inhibitory substances (6,29). Similar studies have employed phenol-chloroform with ethanol precipitation (7,22,23) or manual commercial kit extraction (6,17), which are labor intensive and time-consuming. Since an automated extraction method was used, a tissue homogenization step was performed preextraction to liquefy the solid tissue specimens and release any bacteria present.…”

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confidence: 99%

“…Conventional diagnosis of EPTB hinges on identification of acid-fast bacilli, histopathological examination of tissues, or culture (6,17). These methods are time-consuming, require expertise, can be nonspecific, and are frequently delayed.…”

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confidence: 99%

“…The shift is toward newer molecular diagnostic tools for detecting either RNA or DNA to improve sensitivity and speed up the diagnostic process (30). A number of studies have reported on performance of PCR-based assays for diagnosis of EPTB in formalinfixed paraffin-embedded tissues (3,9,14,18,26), bone marrow, and lymph node (22,23) and lung (17) tissue. The recent WHOendorsed Xpert MTB/RIF assay (Cepheid, Sunnyvale, CA), has shown a sensitivity for nonrespiratory tissue specimens ranging from 53% to 100% and a specificity ranging from 97.3% to 100% (2,10,13,31).…”

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confidence: 99%

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Performance of the Roche LightCycler Real-Time PCR Assay for Diagnosing Extrapulmonary Tuberculosis

Gous¹,

Scott²,

Wong³

et al. 2012

J Clin Microbiol

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The Roche LightCycler mycobacterium detection molecular assay for Mycobacterium tuberculosis , M. avium , and M. kansasii , was applied to tissue specimens. It performed well on lymph node and cerebrospinal fluid specimens and less well on lung, liver, and bone marrow core biopsy specimens, but used in conjunction with a clinical suspicion of tuberculosis, it could augment patient management.

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An Appraisal of PCR-Based Technology in the Detection of Mycobacterium tuberculosis

et al. 2011

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Tuberculosis is an under-recognized yet catastrophic health problem, particularly in developing countries. The HIV pandemic has served to increase the number of susceptible individuals, and multidrug-resistance and poor socioeconomic conditions also augment the prevalence and the consequences of the disease. To control the disease and its spread, it is vital that tuberculosis diagnostics are accurate and rapid. Whereas microscopy and culture have several limitations (low sensitivity is a problem for the former, while the latter has a delayed turnaround time), PCR-based techniques targeting regions of the Mycobacterium tuberculosis genome such as IS6110 have proved to be useful. The purpose of this review is to assess the use of PCR-RFLP, nested PCR and real-time PCR protocols and the choice of target regions for the detection of M. tuberculosis. Real-time PCR for the detection of M. tuberculosis target genes in clinical specimens has contributed to improving diagnosis and epidemiologic surveillance in the past decade. However, targeting one genome sequence such as IS6110 may not by itself be sufficiently sensitive to reach 100% diagnosis, especially in the case of pulmonary tuberculosis. Additional testing for target genome sequences such as hsp65 seems encouraging. An interesting approach would be a multiplex real-time PCR targeting both IS6110 and hsp65 to achieve comprehensive and specific molecular diagnosis. This technology needs development and adequate field testing before it becomes the acceptable gold standard for diagnosis.

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Nested PCR in lung tissue for diagnosis of pulmonary tuberculosis

Cited by 26 publications

References 23 publications

Comparison of real time PCR with phenotypic methods in bronchoalveolar lavage in diagnosis of sputum smear negative pulmonary tuberculosis patients

Comparison of real time PCR with phenotypic methods in bronchoalveolar lavage in diagnosis of sputum smear negative pulmonary tuberculosis patients

Performance of the Roche LightCycler Real-Time PCR Assay for Diagnosing Extrapulmonary Tuberculosis

An Appraisal of PCR-Based Technology in the Detection of Mycobacterium tuberculosis

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