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聚合酶链反应在鼻咽拭子中用于鉴定引起社区获得性肺炎的呼吸道细菌的效用。

Utility of Polymerase Chain Reaction in Nasopharyngeal Swabs for Identifying Respiratory Bacteria Causing Community-Acquired Pneumonia.

机构信息

Infectious Diseases Service, University Hospital and University of Lausanne, Lausanne, Switzerland.

Department of Diagnostic and Interventional Radiology, University Hospital and University of Lausanne, Lausanne, Switzerland.

出版信息

Microbiol Spectr. 2022 Jun 29;10(3):e0037922. doi: 10.1128/spectrum.00379-22. Epub 2022 May 18.

DOI:10.1128/spectrum.00379-22
PMID:35583335
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9241648/
Abstract

Timely identification of a pathogen in lower respiratory tract infections (LRTI) can support appropriate antibiotics use. The difficulty of obtaining lower respiratory tract (LRT) samples limits the utility of point-of-care syndromic molecular assays. We assessed the performance of the FilmArray Pneumonia plus panel (FilmArray PP) in nasopharyngeal (NP) swab for detection of Streptococcus pneumoniae, Haemophilus influenzae, and Moraxella catarrhalis. Patients in the study included retrospectively consenting adults who attended the emergency department of Lausanne University Hospital between February 2019 and August 2020 for a community-acquired LRTI, with available NP swab and a high-quality LRT sample. These samples were tested with the FilmArray PP (cutoff of ≥10 copies/mL). Positive (PPA) and negative percent agreement (NPA) of FilmArray PP in NP swab were calculated, using (i) FilmArray PP in LRT sample and (ii) standard microbiological tests as reference standards. To assess the performance of a lower detection cutoff, NP samples were also tested with an in-house PCR (cutoff of ≥10 copies/mL) for S. pneumoniae and H. influenzae. Overall, 118 patients were included. FilmArray PP in LRT sample and standard microbiology tests detected S. pneumoniae in 19/118 and 12/118, H. influenzae in 44/118 and 19/118, and M. catarrhalis in 14/118 and 0/118, respectively. Using LRT FilmArray PP as reference, PPA and NPA of FilmArray PP on NP were 58% and 100% for S. pneumoniae, 61% and 100% for H. influenzae, and 57% and 99% for M. catarrhalis. Using standard diagnostic tests as reference, PPA and NPA were 58% and 96% for S. pneumoniae, 74% and 87% for H. influenzae, and indefinite and 92% for M. catarrhalis. Using a lower cutoff on NP (≥10 copies/mL), PPA was 68% for S. pneumoniae and 77% for H. influenzae with LRT FilmArray PP as reference. FilmArray PP in NP swabs has a limited PPA for identifying the most common etiologies of community-acquired LRTI irrespective of the reference standard, preventing its use for withholding antibiotics. The PCR detection cutoff does not explain the low PPA. The excellent NPA suggests the use of NP PCR results for rapidly targeted antimicrobial therapy. Timely identification of a pathogen in patients with lower respiratory tract infections is of paramount importance to avoid inappropriate antibiotic prescription. We aimed to evaluate the performance of a rapid syndromic molecular assay in nasopharyngeal swabs for identifying the most common bacterial causes of lower respiratory tract infections in adults (Streptococcus pneumoniae, Haemophilus influenzae, and Moraxella catarrhalis). Our data show that nasopharyngeal molecular assay has a good concordance with lower respiratory tract sample when positive but not when negative. A positive result is therefore concordant with a lower respiratory tract infection and can be used to target antibiotics. Nevertheless, a negative result does not have a good concordance, so it cannot be used to withhold antibiotics. Our findings illustrate the potential utility of these easily collected samples for the management of patients with lower respiratory tract infections.

摘要

及时鉴定下呼吸道感染(LRTI)中的病原体有助于合理使用抗生素。由于难以获取下呼吸道(LRT)样本,床边即时检测的基于综合征的分子检测方法的应用受到限制。我们评估了 FilmArray Pneumonia plus 检测试剂盒(FilmArray PP)在鼻咽(NP)拭子中检测肺炎链球菌、流感嗜血杆菌和卡他莫拉菌的性能。该研究纳入了 2019 年 2 月至 2020 年 8 月期间因社区获得性 LRTI 而在洛桑大学医院急诊科就诊的、经回顾性同意的成年患者。这些患者同时提供了 NP 拭子和高质量的 LRT 样本。使用 FilmArray PP(≥10 拷贝/mL 为阳性界限值)检测这些样本。使用(i)LRT 样本中的 FilmArray PP 和(ii)标准微生物学检测作为参考标准,计算 FilmArray PP 在 NP 拭子中的阳性预测值(PPA)和阴性预测值(NPA)。为评估较低检测界限值的性能,我们还使用了一种针对 S. pneumoniae 和 H. influenzae 的实验室自建 PCR(≥10 拷贝/mL 为阳性界限值)检测 NP 样本。总体上,共有 118 名患者入组。FilmArray PP 在 LRT 样本和标准微生物学检测中分别检测到 19/118 和 12/118 例肺炎链球菌、44/118 和 19/118 例流感嗜血杆菌、14/118 和 0/118 例卡他莫拉菌。使用 LRT FilmArray PP 作为参考,FilmArray PP 在 NP 上的 PPA 和 NPA 分别为 58%和 100%用于肺炎链球菌、61%和 100%用于流感嗜血杆菌、57%和 99%用于卡他莫拉菌。使用标准诊断测试作为参考,PPA 和 NPA 分别为 58%和 96%用于肺炎链球菌、74%和 87%用于流感嗜血杆菌、不确定和 92%用于卡他莫拉菌。使用 NP(≥10 拷贝/mL)上的较低界限值,当以 LRT FilmArray PP 作为参考时,PPA 分别为 68%用于肺炎链球菌和 77%用于流感嗜血杆菌。FilmArray PP 在 NP 拭子中的 PPA 有限,无论参考标准如何,均可用于识别社区获得性 LRTI 的最常见病因,从而防止其用于避免抗生素的使用。PCR 检测界限值并不能解释较低的 PPA。极好的 NPA 提示可使用 NP PCR 结果进行快速靶向抗菌治疗。及时鉴定下呼吸道感染患者的病原体对于避免不适当的抗生素处方至关重要。我们旨在评估快速综合征分子检测在成人下呼吸道感染中的常见细菌病原体(肺炎链球菌、流感嗜血杆菌和卡他莫拉菌)中的鼻拭子中的性能。我们的数据表明,当结果为阳性时,下呼吸道分子检测与下呼吸道样本具有良好的一致性,但当结果为阴性时则不一致。因此,阳性结果与下呼吸道感染一致,可用于靶向抗生素。然而,阴性结果的一致性不好,因此不能用于避免抗生素。我们的研究结果说明了这些易于采集的样本在管理下呼吸道感染患者方面的潜在应用价值。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ad3a/9241648/55ce9ed4bccc/spectrum.00379-22-f002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ad3a/9241648/f7828ea6dafd/spectrum.00379-22-f001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ad3a/9241648/55ce9ed4bccc/spectrum.00379-22-f002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ad3a/9241648/f7828ea6dafd/spectrum.00379-22-f001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ad3a/9241648/55ce9ed4bccc/spectrum.00379-22-f002.jpg

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