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Detection of transmissible gastroenteritis virus by RT-PCR and differentiation from porcine respiratory coronavirus

机译:RT-PCR检测猪传染性胃肠炎病毒及其与猪呼吸道冠状病毒的鉴别

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摘要

An RT-PCR method was developed that amplified genetic material from the 5′ end of the S protein gene of both transmissible gastroenteritis virus (TGEV) and porcine respiratory coronavirus (PRCV), but discriminated between the two by the size of the product generated. A number of restriction endonuclease enzymes were assessed for recognition of the amplicons so produced. The assay was shown to detect viral RNA from all of the 26 different TGEV and PRCV isolates examined, covering a period from 1946 to 1996. Detection of TGEV in clinical specimens was possible using a spin column method to extract RNA and sensitivity was compared to virus isolation and antigen detection ELISA. The method could provide a means of confirming positive results from immunological screening tests such as FAT and ELISA, reducing the need for virus isolation and convalescent serology.
机译:开发了一种RT-PCR方法,该方法从可传播的胃肠炎病毒(TGEV)和猪呼吸道冠状病毒(PRCV)的S蛋白基因的5'末端扩增遗传物质,但通过产生的产物大小区分两者。评估了许多限制性核酸内切酶以识别如此产生的扩增子。结果表明,该方法可检测到从所检查的26种不同TGEV和PRCV分离物中的所有病毒RNA,涵盖1946年至1996年。使用旋转柱法提取RNA可以检测临床标本中的TGEV,并将敏感性与病毒进行了比较分离和抗原检测ELISA。该方法可以提供一种方法,用于确认免疫筛选测试(例如FAT和ELISA)的阳性结果,从而减少了对病毒分离和恢复期血清学的需求。

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