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用于检测实验室和临床样本中黄热病毒的灵敏且特异的单克隆免疫测定法。

Sensitive and specific monoclonal immunoassay for detecting yellow fever virus in laboratory and clinical specimens.

作者信息

Monath T P, Hill L J, Brown N V, Cropp C B, Schlesinger J J, Saluzzo J F, Wands J R

出版信息

J Clin Microbiol. 1986 Jan;23(1):129-34. doi: 10.1128/jcm.23.1.129-134.1986.

Abstract

A solid-phase radioimmunoassay (RIA) was developed for the detection of yellow fever (YF) virus in infected cell culture supernatant fluid and clinical samples. The test employed a flavivirus group-reactive monoclonal antibody attached to a polystyrene bead support and a radiolabeled type-specific antibody probe in a simultaneous sandwich RIA format. Optimal assay conditions specified a 16-h incubation at high temperature (45 degrees C). Monoclonal antibody to tetanus toxoid was added to the radiolabeled probe to inhibit nonspecific binding. The sensitivity of the assay for cell culture-propagated virus was 2.0 log10 50% mosquito infectious doses per 100 microliters or 100 pg of gradient-purified virion protein per 100 microliters. Specificity, assessed with human sera from 512 patients with liver diseases other than YF, including acute viral hepatitis, showed a false-positive rate of 0.0 to 0.6%. Sera from experimentally infected rhesus macaques containing greater than 3.0 log10 units/100 microliter of YF virus were positive by RIA. Sera and liver tissue from human patients were found to be positive.

摘要

已开发出一种固相放射免疫测定法(RIA),用于检测感染细胞培养上清液和临床样本中的黄热病(YF)病毒。该检测采用附着于聚苯乙烯珠载体上的黄病毒属群反应性单克隆抗体和放射性标记的型特异性抗体探针,采用同时夹心RIA形式。最佳检测条件规定在高温(45℃)下孵育16小时。将破伤风类毒素单克隆抗体添加到放射性标记的探针中以抑制非特异性结合。该检测对细胞培养增殖病毒的灵敏度为每100微升2.0 log10 50%蚊感染剂量或每100微升100 pg梯度纯化病毒粒子蛋白。用512例非黄热病肝病患者(包括急性病毒性肝炎)的人血清评估特异性,假阳性率为0.0%至0.6%。来自实验感染恒河猴的血清,若每100微升含大于3.0 log10单位的YF病毒,则通过RIA检测呈阳性。发现人类患者的血清和肝组织呈阳性。

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本文引用的文献

6
Summary of a symposium on yellow fever.
J Infect Dis. 1981 Jul;144(1):87-91. doi: 10.1093/infdis/144.1.87.

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