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通过间接酶免疫测定法检测唾液中针对重组诺沃克病毒抗原的抗体来诊断诺沃克病毒感染。

Diagnosis of norwalk virus infection by indirect enzyme immunoassay detection of salivary antibodies to recombinant norwalk virus antigen.

作者信息

Moe Christine L, Sair Arnie, Lindesmith Lisa, Estes Mary K, Jaykus Lee-Ann

机构信息

Department of International Health, Rollins School of Public Health of Emory University, 1518 Clifton Rd. NE, Room 716, Atlanta, GA 30322, USA.

出版信息

Clin Diagn Lab Immunol. 2004 Nov;11(6):1028-34. doi: 10.1128/CDLI.11.6.1028-1034.2004.

Abstract

Simple diagnostic tests are needed for the detection of norovirus (NoV) outbreaks. Salivary antibody assays provide an attractive alternative to collecting and testing serum or stool samples. Antibodies to Norwalk virus (NV) in oral fluid samples were compared with NV antibodies in serum collected from 38 volunteers challenged with NV inoculum. Pre- and postchallenge (day 4, 8, 14, and 21) saliva and serum samples were examined by enzyme immunoassay (EIA) using recombinant NV antigen. Of 18 infected subjects (those who shed NV in stool or who demonstrated immunoglobulin G [IgG] seroconversion), 15 (83%) had > or =4-fold increases in NV-specific salivary IgA and 15 (83%) had > or =4-fold increases in NV-specific salivary IgG when prechallenge and postchallenge saliva samples were compared. When the results of the IgA and IgG assays were combined, all 18 infected subjects showed > or =4-fold increases in NV-specific salivary IgG or IgA postchallenge titers compared to their prechallenge titers. One of 19 uninfected subjects had a > or =4-fold increase in NV-specific salivary IgG. The sensitivity of the combined assay results was 100%, and the specificity was 95%. NV-specific salivary IgA titers peaked around 14 days postchallenge. NV-specific salivary IgG and serum IgG titers continued to rise through 21 days postchallenge. The application of this EIA to an elementary school outbreak indicated that 67% of the subjects with confirmed infections had >4-fold rises in anti-NoV IgA when an antigen in the same genetic cluster as the outbreak virus was used. This is the first documented mucosal antibody response to NoV in children. This EIA provides a useful approach for diagnosing NoV outbreaks.

摘要

检测诺如病毒(NoV)暴发需要简单的诊断测试。唾液抗体检测为采集和检测血清或粪便样本提供了一种有吸引力的替代方法。将口腔液体样本中针对诺沃克病毒(NV)的抗体与38名接受NV接种物攻击的志愿者所采集血清中的NV抗体进行了比较。使用重组NV抗原,通过酶免疫测定(EIA)对攻击前和攻击后(第4、8、14和21天)的唾液和血清样本进行检测。在18名感染受试者(即粪便中排出NV或显示免疫球蛋白G [IgG] 血清转化的受试者)中,当比较攻击前和攻击后的唾液样本时,15名(83%)受试者的NV特异性唾液IgA增加了≥4倍,15名(83%)受试者的NV特异性唾液IgG增加了≥4倍。当将IgA和IgG检测结果合并时,所有18名感染受试者在攻击后NV特异性唾液IgG或IgA滴度与其攻击前滴度相比均增加了≥4倍。19名未感染受试者中有1名NV特异性唾液IgG增加了≥4倍。合并检测结果的敏感性为100%,特异性为95%。NV特异性唾液IgA滴度在攻击后约14天达到峰值。NV特异性唾液IgG和血清IgG滴度在攻击后21天内持续上升。将这种EIA应用于一所小学的暴发疫情表明,当使用与暴发病毒处于同一基因簇的抗原时,67%确诊感染的受试者抗NoV IgA增加了>4倍。这是首次记录到儿童对NoV的黏膜抗体反应。这种EIA为诊断NoV暴发提供了一种有用的方法。

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