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建立一种双重实时荧光定量 PCR 方法,用于同时检测环境和临床样本中的嗜肺军团菌和新型纳氏支原体。

Development of a duplex q-PCR for the simultaneous detection of Parachlamydia acanthamoebae and Simkania negevensis in environmental and clinical samples.

机构信息

Laboratoire de Génie Enzymatique et Microbiologie, Equipe de Biotechnologie des Algues, Ecole Nationale d'Ingénieurs de Sfax, Université de Sfax, 3038, Sfax, Tunisia.

Laboratory of Microbiology, Faculty of Medicine of Sfax, Habib Bourguiba University Hospital, University of Sfax, Tunisia.

出版信息

Anal Biochem. 2023 Apr 15;667:115080. doi: 10.1016/j.ab.2023.115080. Epub 2023 Feb 10.

DOI:10.1016/j.ab.2023.115080
PMID:36775111
Abstract

Parachlamydia acanthamoebae and Simkania negevensis, two Chlamydia-like bacteria, have been recently recognized as emerging human respiratory pathogens. The prevalence and frequency of these bacteria in the environment and among atypical pneumonia patients are still underestimated by classical cultures, immunohistochemistry and serology which are non-specific, long and tedious methods. This study aims to develop a new duplex probe-based q-PCR assay for the simultaneous detection and quantification of P. acanthamoebae and S. negevensis. The selected hydrolysis probes displayed no cross-reaction with the closely related Chlamydia or the other tested waterborne pathogens. The assay achieved a large dynamic range for quantification (from 5 × 10 to 5 DNA copies/reaction). Efficiencies of FAM and JOE label probes weren't affected when they were combined. They were close to 100%, indicating the linear amplification. The application of this diagnostic tool resulted in 9/47 (19%) and 4/47 (8.5%) positive water samples for P. acanthamoebae and S. negevensis, respectively. P. acanthamoebae was also covered from 2/78 (2.5%) respiratory specimens and only one case (1/200 = 0.5%) of P. acanthamoebae and SARS-CoV-2 co-infection was noticed. While S. negevensis wasn't detected in clinical samples, the developed duplex q-PCR was shown to be an accurate, highly sensitive, and robust diagnostic tool for the detection and quantification of P. acanthamoebae and S. negevensis.

摘要

类立克次体副衣原体和辛型支原体,两种类似衣原体的细菌,最近被认为是新兴的人类呼吸道病原体。这些细菌在环境中的流行率和频率以及非典型肺炎患者中的流行率和频率仍被经典培养、免疫组织化学和非特异性、冗长和繁琐的血清学方法所低估。本研究旨在开发一种新的基于双探针 q-PCR 检测方法,用于同时检测和定量检测类立克次体副衣原体和辛型支原体。所选的水解探针与密切相关的衣原体或其他测试的水生病原体没有交叉反应。该检测方法的定量动态范围较大(从 5×10 到 5 DNA 拷贝/反应)。FAM 和 JOE 标记探针的效率不受组合影响,接近 100%,表明线性扩增。该诊断工具的应用导致 9/47(19%)和 4/47(8.5%)的水样分别为类立克次体副衣原体和辛型支原体阳性。类立克次体副衣原体还从 2/78(2.5%)呼吸道标本中检出,仅 1 例(1/200=0.5%)同时感染类立克次体副衣原体和 SARS-CoV-2。虽然辛型支原体未在临床样本中检出,但所开发的双 q-PCR 被证明是一种准确、高度敏感、强大的检测和定量检测类立克次体副衣原体和辛型支原体的诊断工具。

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