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2009年纽约市一场特征明确的腮腺炎疫情中实验室诊断方法的敏感性比较。

Comparison of the sensitivity of laboratory diagnostic methods from a well-characterized outbreak of mumps in New York city in 2009.

作者信息

Rota Jennifer S, Rosen Jennifer B, Doll Margaret K, McNall Rebecca J, McGrew Marcia, Williams Nobia, Lopareva Elena N, Barskey Albert E, Punsalang Amado, Rota Paul A, Oleszko William R, Hickman Carole J, Zimmerman Christopher M, Bellini William J

机构信息

Division of Viral Diseases, National Center for Immunization and Respiratory Diseases, Centers for Disease Control and Prevention, Atlanta, GA, USA.

出版信息

Clin Vaccine Immunol. 2013 Mar;20(3):391-6. doi: 10.1128/CVI.00660-12. Epub 2013 Jan 16.

Abstract

A mumps outbreak in upstate New York in 2009 at a summer camp for Orthodox Jewish boys spread into Orthodox Jewish communities in the Northeast, including New York City. The availability of epidemiologic information, including vaccination records and parotitis onset dates, allowed an enhanced analysis of laboratory methods for mumps testing. Serum and buccal swab samples were collected from 296 confirmed cases with onsets from September through December 2009. All samples were tested using the Centers for Disease Control and Prevention (CDC) capture IgM enzyme immunoassay (EIA) and a real-time reverse transcription-PCR (rRT-PCR) that targets the short hydrophobic gene. A subset of the samples (n = 205) was used to evaluate 3 commercial mumps IgM assays and to assess the sensitivity of using an alternative target gene (nucleoprotein) in the rRT-PCR protocol. Among 115 cases of mumps with 2 documented doses of measles, mumps, and rubella (MMR) vaccine, the CDC capture IgM EIA detected IgM in 51% of serum samples compared to 9% to 24% using three commercial IgM assays. The rRT-PCR that targeted the nucleoprotein gene increased RNA detection by 14% compared to that obtained with the original protocol. The ability to detect IgM improved when serum was collected 3 days or more after symptom onset, whereas sensitivity of RNA detection by rRT-PCR declined when buccal swabs were collected later than 2 days after onset. Selection of testing methods and timing of sample collection are important factors in the ability to confirm infection among vaccinated persons. These results reinforce the need to use virus detection assays in addition to serologic tests.

摘要

2009年,纽约州北部一个东正教犹太男孩夏令营爆发腮腺炎疫情,并蔓延至东北部的东正教犹太社区,包括纽约市。由于可获取包括疫苗接种记录和腮腺炎发病日期在内的流行病学信息,因此能够对腮腺炎检测的实验室方法进行强化分析。收集了296例确诊病例的血清和口腔拭子样本,这些病例的发病时间为2009年9月至12月。所有样本均使用疾病控制与预防中心(CDC)的捕获IgM酶免疫测定法(EIA)以及针对短疏水基因的实时逆转录聚合酶链反应(rRT-PCR)进行检测。一部分样本(n = 205)用于评估3种商用腮腺炎IgM检测方法,并评估在rRT-PCR方案中使用替代靶基因(核蛋白)的敏感性。在115例有2剂麻疹、腮腺炎和风疹(MMR)疫苗接种记录的腮腺炎病例中,CDC捕获IgM EIA在51%的血清样本中检测到IgM,相比之下,三种商用IgM检测方法的检测率为9%至24%。与原始方案相比,针对核蛋白基因的rRT-PCR使RNA检测率提高了14%。症状出现3天或更长时间后采集血清时,IgM的检测能力有所提高,而发病2天后采集口腔拭子,rRT-PCR检测RNA的敏感性则会下降。检测方法的选择和样本采集时间是确认接种疫苗者是否感染的重要因素。这些结果进一步表明,除了血清学检测外,还需要使用病毒检测方法。

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