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首页> 外文期刊>Journal of Virological Methods >IN SITU HYBRIDIZATION TECHNIQUE FOR THE DETECTION OF SWINE ENTERIC AND RESPIRATORY CORONAVIRUSES, TRANSMISSIBLE GASTROENTERITIS VIRUS (TGEV) AND PORCINE RESPIRATORY CORONAVIRUS (PRCV), IN FORMALIN-FIXED PARAFFIN-EMBEDDED TISSUES
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IN SITU HYBRIDIZATION TECHNIQUE FOR THE DETECTION OF SWINE ENTERIC AND RESPIRATORY CORONAVIRUSES, TRANSMISSIBLE GASTROENTERITIS VIRUS (TGEV) AND PORCINE RESPIRATORY CORONAVIRUS (PRCV), IN FORMALIN-FIXED PARAFFIN-EMBEDDED TISSUES

机译:原位杂交技术,用于福尔马林固定石蜡包埋的组织中的猪肠道和呼吸道冠状病毒,可传播的胃肠炎病毒(TGEV)和猪呼吸道冠状病毒(PRCV)的检测

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摘要

The in situ hybridization (ISH) technique was developed to detect the swine coronaviruses, transmissible gastroenteritis virus (TGEV) and porcine respiratory coronavirus (PRCV), in cell culture and tissue sections from TGEV-or PRCV-infected pigs. The S-35-labeled RNA probes were generated from two plasmids pPSP.FP1 and pPSP.FP2 containing part of the S gene of TGEV. The procedure was first standardized in cell cultures. The radiolabeled pPSP.FP2 probe detected both TGEV and PRCV in virus-inoculated cell cultures, whereas pPP.FP1 probe detected TGEV but not PRCV. The probe was then used to detect TGEV or PRCV in tissues of pigs experimentally infected with TGEV or PRCV or naturally infected with TGEV. Again, the probes detected TGEV in intestines of experimentally and naturally infected pigs and PRCV in the lungs of experimentally infected pigs. TGEV RNA was detected mainly within the enterocytes at the lips of villi and, less often, within some crypt epithelial cells. PRCV was shown to replicate mainly in the bronchiolar epithelial cells and in lesser amount in type II pneumocytes, type I pneumocytes, alveolar macrophages and bronchial epithelial cells, respectively. ISH has potential applications as a diagnostic test for the detection and differentiation of TGEV and PRCV in tissues and in studies to gain a better understanding of the mechanism of pathogenesis of enteric and respiratory coronavirus infections.
机译:已开发出原位杂交(ISH)技术,以检测受TGEV或PRCV感染的猪的细胞培养和组织切片中的猪冠状病毒,可传播的胃肠炎病毒(TGEV)和猪呼吸道冠状病毒(PRCV)。 S-35标记的RNA探针是由两个含有TGEV S基因一部分的质粒pPSP.FP1和pPSP.FP2产生的。该程序首先在细胞培养中标准化。放射性标记的pPSP.FP2探针在病毒接种的细胞培养物中同时检测到TGEV和PRCV,而pPP.FP1探针检测到TGEV但未检测到PRCV。然后使用该探针检测实验感染TGEV或PRCV或自然感染TGEV的猪组织中的TGEV或PRCV。同样,这些探针在实验和自然感染的猪的肠道中检测到TGEV,在实验感染的猪的肺中检测到PRCV。 TGEV RNA主要在绒毛唇的肠上皮细胞内检测到,而在一些隐窝上皮细胞内则较少见。已显示PRCV主要在细支气管上皮细胞中复制,而在II型肺细胞,I型肺细胞,肺泡巨噬细胞和支气管上皮细胞中的复制量则较少。 ISH在诊断和鉴别组织中TGEV和PRCV以及进行研究以更好地了解肠道和呼吸道冠状病毒感染的发病机理方面具有潜在的应用价值。

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