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Reverse ELISA for the detection of anti West Nile virus IgG antibodies in humans.

机译:反向ELISA用于检测人类抗西尼罗河病毒IgG抗体。

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We have developed a specific reverse ELISA to investigate the potential of the domain III of the West Nile virus envelope protein to detect virus-specific antibodies. For this purpose, the domain III antigen was expressed in Escherichia coli, refolded and directly labelled with peroxidase. By mixing serum samples with the enzyme-labelled antigen, immune complexes will form that are simultaneously recognized by rheumatoid factor coated microtiter plates. Specific antibodies to the domain III were found in 160 out of 206 sera of patients with neutralising antibodies to West Nile virus (77.6% sensitivity). The antigen differentiated reliably between sera of West Nile virus- and dengue virus-infected patients. In combination with indirect immunofluorescence, to exclude four false-positive samples, the specificity was 100% (280 samples). Assuming a prevalence rate of anti-West-Nile virus antibodies of 5%, the positive and negative predictive values were 93.3% and 98.8% respectively. These results indicate that the reverse ELISA using a specific portion of the envelope antigen of West Nile virus is especially suitable for studies on the prevalence of West Nile infections in affected countries.
机译:我们已经开发了一种特异性的反向ELISA,以研究西尼罗河病毒包膜蛋白III结构域检测病毒特异性抗体的潜力。为此目的,结构域III抗原在大肠杆菌中表达,重新折叠并直接用过氧化物酶标记。通过将血清样品与酶标记的抗原混合,将形成免疫复合物,同时被类风湿因子包被的微量滴定板识别。在针对西尼罗河病毒的中和抗体的206名患者中,有160名血清中发现了针对结构域III的特异性抗体(敏感性为77.6%)。该抗原可在西尼罗河病毒感染者和登革热病毒感染者的血清之间可靠区分。与间接免疫荧光结合,排除了四个假阳性样品,特异性为100%(280个样品)。假设抗西尼罗河病毒抗体的流行率为5%,阳性和阴性预测值分别为93.3%和98.8%。这些结果表明,使用西尼罗河病毒包膜抗原的特定部分进行的反向ELISA特别适合于在受影响国家/地区研究西尼罗河感染的患病率。

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