首页> 美国卫生研究院文献>Journal of Virology >Cell-free translation of virion RNA from nondefective and transformation-defective Rous sarcoma viruses.
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Cell-free translation of virion RNA from nondefective and transformation-defective Rous sarcoma viruses.

机译:来自无缺陷和转化缺陷的劳斯肉瘤病毒的病毒粒子RNA的无细胞翻译。

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摘要

Nondefective and transformation-defective virion subunit RNAs from two strains of Rous sarcoma virus (RSV) were translated in cell-free systems derived from Krebs IIA ascites cells, wheat germ, and L-cells. In each case the predominant viral-specific product was a polypeptide of molecular weight 76,000 that is related to the internal viral group-specific antigens, as judged by immunoprecipitation with monospecific antisera and tryptic peptide fingerprinting. No difference could be detected between the translation products of 35S RNA from nondefective and transformation-defective RSV virions, nor of 35S RNA from different strains of RSV. The 76,000-molecular-weight polypeptide synthesized in response to 35S RNA in vitro was labeled with formyl-methionine from initiator tRNA. Models for viral protein synthesis are discussed in the light of these results, and arguments positioning the group-specific antigen gene at the 5' end of the 35S RNA are presented.
机译:在来自Krebs IIA腹水细胞,小麦胚芽和L细胞的无细胞系统中翻译了来自两个劳斯肉瘤病毒(RSV)菌株的无缺陷和转化缺陷的病毒体亚基RNA。在每种情况下,主要的病毒特异性产物都是分子量为76,000的多肽,该多肽与内部病毒组特异性抗原有关,通过单特异性抗血清和胰蛋白酶肽指纹图谱的免疫沉淀来判断。没有缺陷的和转化缺陷的RSV病毒体的35S RNA的翻译产物,以及来自不同的RSV株的35S RNA的翻译产物都没有检测到差异。在体外响应35S RNA合成的76,000分子量的多肽用起始物tRNA的甲酰基甲硫氨酸标记。根据这些结果,讨论了病毒蛋白质合成的模型,并提出了将群特异性抗原基因定位在35S RNA 5'端的论点。

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