Novel Wide-range Quantitative Nested Real-time PCR Assay for Mycobacterium Tuberculosis DNA: Clinical Application for Diagnosis of Tuberculous Meningitis

Overview

Journal J Clin Microbiol

Specialty Microbiology

Date 2008 Mar 14

PMID 18337387

Citations 11

Authors

Teruyuki Takahashi

Masato Tamura

Yukihiro Asami

Eiko Kitamura

Kosuke Saito

Tsukasa Suzuki

Sachiko Nonaka Takahashi

Koichi Matsumoto

Shigemasa Sawada

Eise Yokoyama

Toshiaki Takasu

Affiliations

Soon will be listed here.

Abstract

Although the "gold standard" for diagnosis of tuberculous meningitis (TBM) is bacterial isolation of Mycobacterium tuberculosis, there are still several complex issues. Recently, we developed an internally controlled novel wide-range quantitative nested real-time PCR (WR-QNRT-PCR) assay for M. tuberculosis DNA in order to rapidly diagnose TBM. For use as an internal control calibrator to measure the copy number of M. tuberculosis DNA, an original new-mutation plasmid (NM-plasmid) was developed. Due to the development of the NM-plasmid, the WR-QNRT-PCR assay demonstrated statistically significant accuracy over a wide detection range (1 to 10(5) copies). In clinical applications, the WR-QNRT-PCR assay revealed sufficiently high sensitivity (95.8%) and specificity (100%) for 24 clinically suspected TBM patients. In conditional logistic regression analysis, a copy number of M. tuberculosis DNA (per 1 ml of cerebrospinal fluid) of >8,000 was an independent risk factor for poor prognosis for TBM (i.e., death) (odds ratio, 16.142; 95% confidence interval, 1.191 to 218.79; P value, 0.0365). In addition, the copy numbers demonstrated by analysis of variance statistically significant alterations (P < 0.01) during the clinical treatment course for 10 suspected TBM patients. In simple regression analysis, the significant correlation (R(2) = 0.597; P < 0.0001) was demonstrated between copy number and clinical stage of TBM. We consider the WR-QNRT-PCR assay to be a useful and advanced assay technique for assessing the clinical treatment course of TBM.

Citing Articles

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