首页> 外文期刊>The American Journal of Tropical Medicine and Hygiene >Detection of Mycoplasma pneumoniae and Legionella pneumophila in Patients Having Community-Acquired Pneumonia: A Multicentric Study from New Delhi, India
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Detection of Mycoplasma pneumoniae and Legionella pneumophila in Patients Having Community-Acquired Pneumonia: A Multicentric Study from New Delhi, India

机译:检测肺炎肺炎肺炎肺炎患者患有社区肺炎的患者:印度新德里的多中心研究

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摘要

Atypical pathogens including Mycoplasma pneumoniae and Legionella pneumophila are increasingly recognized as important causes of community-acquired pneumonia (CAP). Mycoplasma pneumoniae accounts for 20-40% of all CAP and L. pneumophila is responsible for 3-15% of cases. The paucity of data from India in this regard prompted us to conduct this prospective multicentric analysis to detect the prevalence of M. pneumoniae and L. pneumophila in our geographical region. A total of 453 patients with symptoms of pneumonia and 90 controls with no history of lower respiratory tract infections were included in the study. A duplex polymerase chain reaction (PCR) targeting 543 bp region of P1 adhesin gene of M. pneumoniae and 375 bp region of macrophage infectivity potentiator (mip) gene of L. pneumophila was standardized for simultaneous detection of these atypical pathogens. Respiratory secretions, blood, and urine samples were collected from each patient and control and were subjected to duplex PCR, culture and serology for M. pneumoniae and L. pneumophila. Urine samples were subjected for detecting L. pneumophila antigen. Among the 453 patients investigated for M. pneumoniae, 52 (11.4%) were positive for IgM antibodies, 17 were positive by culture, and seven tested positive by PCR (P1 gene). Similarly for L. pneumophila, 50 cases (11%) were serologically positive for IgM antibodies, one was positive by PCR (mip gene) and urine antigen detection. A total of eight samples were positive by duplex PCR for M. pneumoniae P1 gene (N = 7) and L. pneumophila mip gene (N = 1). Of the 90 controls, two samples (2.2%) showed IgM positivity, and 15 (16.7%) showed IgG positivity for M. pneumoniae. For L. pneumophila, three samples (3.3%) tested positive for IgM, and 12 (13.3%) tested positive for IgG antibodies. The study findings indicate the presence of M. pneumoniae and L. pneumophila in our geographical region, and a combination of laboratory approaches including PCR, culture, and serology is required for effective detection of these agents.
机译:包括支原体肺炎和军团菌肺炎的非典型病原体越来越被认为是社区肺炎(帽)的重要原因。肺炎肺炎患者占所有帽的20-40%,L.Pneumophila占3-15%的案件。在这方面,来自印度的数据的缺乏促使我们进行这一前瞻性多中心分析,以检测我们地理区域中M.肺炎和L.Pneumophila的患病率。研究共有453例患有肺炎和90例对照的患者,没有历史历史,没有降低呼吸道感染历史。用于同时检测这些非典型病原体的双工聚合酶链式反应(PCR)P1粘粘剂基因的P1粘粘剂基因和375bp型巨噬细胞感染增强剂(MIP)基因的375bp区域。从每个患者和对照中收集呼吸分泌物,血液和尿液样品,对M. pneumoniae和L.Pneumophila进行双相PCR,培养和血清学。进行尿液样品检测L.肺炎罗拉抗原。在对M.肺炎的453名患者中,52例(11.4%)为IgM抗体阳性,17次通过培养阳性,并通过PCR(P1基因)阳性阳性阳性。类似地,对于L.Pneumophila,50例(11%)为IgM抗体阳性阳性,通过PCR(MIP基因)和尿抗原检测是阳性的。通过双链体PCR用于M.肺炎料P1基因(N = 7)和L.Pneumophila MIP基因(n = 1),总共八个样品。在90个对照中,两个样品(2.2%)显示IgM积极性,并且15(16.7%)显示了M.肺炎的IgG阳性。对于L. pneumophila,三种样品(3.3%)测试阳性IgM,12(13.3%)测试阳性IgG抗体。该研究结果表明我们的地理区域中的M.肺炎和L.Pneumophila的存在,并且需要在包括PCR,培养和血清学中的实验室方法的组合来有效检测这些药剂。

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