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首页> 外文期刊>Journal of Clinical Microbiology >cDNA probes for the diagnosis of bovine torovirus (Breda virus) infection.
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cDNA probes for the diagnosis of bovine torovirus (Breda virus) infection.

机译:用于诊断牛轮状病毒(Breda病毒)感染的cDNA探针。

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A genomic cDNA library of RNA from Breda virus (BRV), a bovine torovirus, was prepared. The nucleotide sequence of the 3' end of the genome was found to be highly conserved (93% identical) between BRV and Berne virus, the torovirus prototype. Cross-hybridization experiments were performed to select Berne virus cDNA clones for use as probes in a dot hybridization assay; the objective was to detect heterologous torovirus RNA in fecal material. A rapid RNA extraction method was employed to make the test applicable for routine diagnosis. Samples from calves after experimental and natural infection with BRV were assayed to establish the sensitivity and specificity of the test and to compare the test with the enzyme-linked immunosorbent assay (ELISA) for antigen detection. For this purpose, 53 samples from seven infected calves were tested with both methods. In the ELISA, BRV was detected in six fecal samples from three inoculated calves. By use of the hybridization test, 16 samples from seven calves reacted positively. With one exception, only postinoculation samples were found positive in hybridization. No signal was seen in feces from uninoculated calves or from calves infected with rotavirus or coronavirus.
机译:从牛轮状病毒布雷达病毒(BRV)制备了RNA的基因组cDNA文库。发现基因组3'端的核苷酸序列在BRV和伯恩病毒(环状病毒原型)之间高度保守(93%相同)。进行交叉杂交实验,以选择伯恩病毒cDNA克隆用作点杂交测定中的探针;目的是检测粪便中的异源轮状病毒RNA。一种快速的RNA提取方法被用于使该测试可用于常规诊断。对来自小牛的实验性和自然感染后的犊牛样品进行测定,以建立测试的敏感性和特异性,并将测试与酶联免疫吸附测定(ELISA)进行抗原检测。为此,用两种方法测试了来自七个被感染小牛的53个样品。在ELISA中,从三只接种的小牛的六个粪便样品中检测到BRV。通过杂交试验,来自七个小牛的16个样品反应阳性。除一个例外,仅发现接种后的样品在杂交中呈阳性。未接种牛犊或轮状病毒或冠状病毒感染牛犊的粪便中未见信号。

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