Pitcher David, Chalker Victoria J, Sheppard Carmen, George Robert C, Harrison Timothy G
Respiratory and Systemic Infection Laboratory, Health Protection Agency Centre for Infections, 61 Colindale Avenue, London NW9 5EQ, UK.
J Med Microbiol. 2006 Feb;55(Pt 2):149-155. doi: 10.1099/jmm.0.46281-0.
Real-time PCR was employed to detect a region of the P1 cytadhesin gene of Mycoplasma pneumoniae in clinical samples. An internal processing control was included that could be co-amplified simultaneously in the same reaction tube. The assay could reproducibly detect 1 x 10(3) M. pneumoniae organisms ml(-1) in clinical samples. There was no amplification of DNA or signal production from 15 other species of human mycoplasmas and 19 other bacterial species. Using a panel of 175 respiratory samples taken from patients with pneumonia of proven aetiology, the sensitivity was found to be 60 % and the specificity of the assay 96.7 % when compared with serology. This assay is suitable for same-day diagnosis of M. pneumoniae infection and batch processing of respiratory samples for clinical screening.
采用实时聚合酶链反应(Real-time PCR)检测临床样本中肺炎支原体P1黏附素基因的一个区域。实验包含一个内部处理对照,可在同一反应管中同时进行共扩增。该检测方法可重复性地检测临床样本中每毫升1×10³个肺炎支原体。15种其他人类支原体和19种其他细菌均未出现DNA扩增或信号产生。使用一组从病因已明确的肺炎患者中采集的175份呼吸道样本进行检测,与血清学检测相比,该检测方法的灵敏度为60%,特异性为96.7%。该检测方法适用于肺炎支原体感染的当日诊断以及对呼吸道样本进行批量处理以用于临床筛查。
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