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Indian Journal of Medical Microbiology
Medknow Publications on behalf of Indian Association of Medical Microbiology
ISSN: 0255-0857
EISSN: 0255-0857
Vol. 28, No. 3, 2010, pp. 227-232
Bioline Code: mb10069
Full paper language: English
Document type: Research Article
Document available free of charge

Indian Journal of Medical Microbiology, Vol. 28, No. 3, 2010, pp. 227-232

 en Evaluation of a nested PCR targeting IS6110 of Mycobacterium tuberculosis check for this species in other resources for detection of the organism in the leukocyte fraction of blood samples
Nandagopal, B; Sankar, S; Lingesan, K; Appu, K C.; Sridharan, G & Gopinathan, A K.

Abstract

Purpose: Tuberculosis poses a serious health problem in resource-poor settings such as India. Polymerase chain reaction (PCR) is presently seen as a promising alternative to conventional smear microscopy and culture techniques. Undiagnosed fever is a condition where the aetiology could include tuberculosis in a significant percentage. This paper evaluates a nested PCR (nPCR) using Hotstar Taq for the detection of M. tuberculosis check for this species in other resources in patients with febrile illness using insertion element, IS6110 as a target.
Material and Methods:A total of 355 samples (301 HIV status unknown and 54 HIV seropositives) from patients primarily with febrile illness were tested for the presence of M. tuberculosis. Blood culture was done in a commercial automated blood culture system and nPCR in DNA extracts from buffy coat samples. Hotstar Taq polymerase was used to enhance the sensitivity of nPCR and the lower limit of detection was determined by using cloned plasmid.
Results: Among the patients tested, 2% were positive by automated culture system and 6.8% of patients were positive by nPCR. Majority of the positives were from HIV seropositive individuals. The sensitivity of the nPCR was 100% and the specificity was 95.1%. The lower limit of detection was less than 1 genome copy per microlitre. Among the nPCR positives, patients from rural community were significantly higher than from the peri-urban community.
Conclusions: The nPCR had a high sensitivity and specificity on buffy coat samples using Hotstar Taq polymerase in the reaction mix. Thus the technique is a valuable tool in the diagnosis of tuberculosis.

Keywords
Buffy coat, Mycobacterium tuberculosis, nested PCR, IS6110, rural

 
© Copyright 2010 Indian Journal of Medical Microbiology.
Alternative site location: http://www.ijmm.org

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