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用于评估麻疹病毒免疫力的中和酶联免疫吸附测定

Neutralization enzyme-linked immunosorbent assay for evaluation of immunity to measles virus.

作者信息

Nates S V, Rey G Y, Giordano M O, Depetris A R, Boshell J

机构信息

Instituto de Virología Dr. J.M. Vanella, Facultad de Ciencias Médicas, Universidad Nacional de Córdoba, Argentina.

出版信息

Viral Immunol. 1995;8(1):47-52. doi: 10.1089/vim.1995.8.47.

Abstract

A neutralization enzyme-linked immunosorbent (Nt-ELISA) assay for determination of protective immunity to measles virus was developed and evaluated. This procedure uses the same initial steps as performed to determine antibody titers by seroneutralization (Nt) test. However, a reduction in virus infectivity by neutralizing antibody was determined by quantitation of viral antigen using ELISA. The serum dilution that resulted in neutralization of 50% of infectious virus could be determined from the absorbance values. To be able to screen a large number of specimens, the conditions of the Nt-ELISA test were adjusted such that negative sera for measles antibodies and the positive ones were clearly distinguished on the basis of a single dilution (1:4). This test showed similar sensitivity (88.3%) and equal specificity as the Nt test when screening 136 serum samples from normal subjects. The estimation of protective antibody titers by Nt and Nt-ELISA methods was strongly correlated (correlation coefficient = 0.91). Thus, the measles Nt-ELISA test is rapid, reproducible, sensitive, and specific for detection of protective measles antibodies.

摘要

开发并评估了一种用于测定对麻疹病毒保护性免疫的中和酶联免疫吸附(Nt-ELISA)试验。该程序使用与通过血清中和(Nt)试验测定抗体滴度相同的初始步骤。然而,通过使用ELISA定量病毒抗原来确定中和抗体对病毒感染性的降低。可以从吸光度值确定导致50%感染性病毒被中和的血清稀释度。为了能够筛选大量标本,调整了Nt-ELISA试验的条件,以便在单一稀释度(1:4)的基础上清楚地区分麻疹抗体阴性血清和阳性血清。在筛选136份正常受试者血清样本时,该试验显示出与Nt试验相似的敏感性(88.3%)和相同的特异性。通过Nt和Nt-ELISA方法估计的保护性抗体滴度高度相关(相关系数=0.91)。因此,麻疹Nt-ELISA试验对于检测保护性麻疹抗体具有快速、可重复、灵敏和特异的特点。

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