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Development of a multiplex real-time quantitative PCR assay to detect Chlamydia pneumoniae, Legionella pneumophila and Mycoplasma pneumoniae in respiratory tract secretions.

机译:开发用于检测呼吸道分泌物中肺炎衣原体,肺炎军团菌和肺炎支原体的实时荧光定量PCR检测方法。

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摘要

Atypical pathogens such as Chlamydia pneumoniae, Legionella pneumophila and Mycoplasma pneumoniae are an important cause of community-acquired pneumonia. The available detection methods (culture and serology) either lack sensitivity or give only a retrospective diagnosis. In order to improve their detection and quantification in respiratory samples, a real-time multiplex PCR, performed in two separate reactions, was developed for these three pathogens. The comparison of multiplex real-time and conventional PCR assay on 73 respiratory specimens showed an overall agreement of 98.3%, corresponding to 95.8%, 100% and 100% agreement for C. pneumoniae, L. pneumophila and M. pneumoniae, respectively. Clinical application of this multiplex real-time PCR was done on 40 respiratory samples from 38 patients with respiratory tract infections. Of 19 serology-positive patients, 14 were confirmed by the multiplex real-time PCR to be infected by either one of the three pathogens. All samples from serology-negative patients were negative with the multiplex real-time PCR.
机译:非典型病原体,例如肺炎衣原体,肺炎军团菌和肺炎支原体,是社区获得性肺炎的重要原因。可用的检测方法(文化和血清学)要么缺乏敏感性,要么仅提供回顾性诊断。为了改善它们在呼吸道样品中的检测和定量,针对这三种病原体开发了在两个单独的反应中进行的实时多重PCR。在73个呼吸道标本上进行的实时荧光定量PCR和常规PCR分析的比较显示,总体一致性为98.3%,分别对应于肺炎衣原体,肺炎支原体和肺炎支原体的95.8%,100%和100%一致。这种多重实时PCR的临床应用是对来自38例呼吸道感染患者的40份呼吸样品进行的。在19位血清学阳性患者中,通过多重实时PCR确认了14位被三种病原体之一感染。血清学阴性患者的所有样品在多重实时PCR中均为阴性。

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