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基于核蛋白基因的巢式逆转录聚合酶链反应检测法在诊断自发性和实验性牛呼吸道合胞体病毒感染中的应用评估

Evaluation of a nested reverse transcription-PCR assay based on the nucleoprotein gene for diagnosis of spontaneous and experimental bovine respiratory syncytial virus infections.

作者信息

Valarcher J F, Bourhy H, Gelfi J, Schelcher F

机构信息

UMR Institut National de la Recherche Agronomique-Ecole Nationale Vétérinaire de Toulouse de Physiopathologie Infectieuse et Parasitaire des Ruminants, ENVT, 31076 Toulouse cedex 3, France.

出版信息

J Clin Microbiol. 1999 Jun;37(6):1858-62. doi: 10.1128/JCM.37.6.1858-1862.1999.

Abstract

The first nested reverse transcription (RT)-PCR based on the nucleoprotein gene (n RT-PCR-N) of the bovine respiratory syncytial virus (BRSV) has been developed and optimized for the detection of BRSV in bronchoalveolar lavage fluid cells of calves. This test is characterized by a low threshold of detection (0.17 PFU/ml), which is 506 times lower than that obtained by an enzyme immunosorbent assay (EIA) test (RSV TESTPACK ABBOTT). During an experimental infection of 17 immunocompetent calves less than 3 months old, BRSV RNA could be detected up to 13 days after the onset of symptoms whereas isolation in cell culture was possible only up to 5 days. Compiling results obtained by conventional techniques (serology, antigen detection, and culture isolation) for 132 field samples collected from calves with acute respiratory signs revealed that n RT-PCR-N showed the highest diagnostic sensitivity and very good specificity. This n RT-PCR-N with its long period of detection during BRSV infection thus provides a valuable tool for diagnostic and epidemiological purposes.

摘要

基于牛呼吸道合胞体病毒(BRSV)核蛋白基因的首个巢式逆转录(RT)-PCR(n RT-PCR-N)已被开发并优化,用于检测犊牛支气管肺泡灌洗细胞中的BRSV。该检测方法的特点是检测阈值低(0.17 PFU/ml),比酶免疫吸附测定(EIA)检测(RSV TESTPACK ABBOTT)获得的阈值低506倍。在对17头3个月龄以下免疫功能正常的犊牛进行实验性感染期间,症状出现后长达13天可检测到BRSV RNA,而细胞培养中仅在5天内可分离到病毒。对从有急性呼吸道症状的犊牛采集的132份现场样本采用常规技术(血清学、抗原检测和培养分离)获得的结果进行汇总分析,结果显示n RT-PCR-N具有最高的诊断敏感性和非常好的特异性。因此,这种在BRSV感染期间检测期长的n RT-PCR-N为诊断和流行病学目的提供了一种有价值的工具。

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