| Literature DB >> 27450004 |
Ryota Ushio1, Masaki Yamamoto2, Kentaro Nakashima1, Hiroki Watanabe1, Kenjiro Nagai1, Yuji Shibata1, Ken Tashiro1, Toshinori Tsukahara1, Hideyuki Nagakura1, Nobuyuki Horita1, Takashi Sato1, Masaharu Shinkai3, Makoto Kudo3, Atsuhisa Ueda4, Takeshi Kaneko1.
Abstract
Nucleic acid amplification tests are a major diagnostic tool for pulmonary tuberculosis (PTB). Recently, digital PCR (dPCR) assay has improved sensitivity for the detection of small copy numbers of target molecules. The aim of this study is to explore the utility of dPCR for detecting Mycobacterium tuberculosis (MTB) DNA in PTB patient plasma. Total DNA was purified from plasma samples of newly diagnosed sputum smear-positive PTB patients. Copy numbers of MTB-specific genes in the samples were quantified with dPCR assays targeted for IS6110 or gyrB. A total of 33 PTB patients were enrolled. Significant differences between PTB patients and controls were observed in copy numbers of both targets: IS6110 mean ± SD, 144.8 ± 538.3 vs 0.44 ± 0.49 (copies/20 μL, p = 0.004; Mann-Whitney U test) and gyrB mean ± SD, 359.0 ± 2116 vs 0.07 ± 0.28 (copies/20 μL, p = 0.011; Mann-Whitney U test), respectively. This test had sensitivities of 65% or 29% and a specificity of 93% or 100% with the IS6110-targeted or gyrB-targeted assays, respectively. A dPCR assay successfully detected MTB DNA in PTB patient plasma. This minimally invasive and accurate method has potential to become an alternative diagnostic option.Entities:
Keywords: Circulating DNA; Digital PCR; IS6110; Plasma; Tuberculosis; gyrB
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Year: 2016 PMID: 27450004 DOI: 10.1016/j.tube.2016.04.004
Source DB: PubMed Journal: Tuberculosis (Edinb) ISSN: 1472-9792 Impact factor: 3.131