Shurtz R, Dolev S, Aboud M, Salzberg S
J Virol. 1979 Sep;31(3):668-76. doi: 10.1128/JVI.31.3.668-676.1979.
When NIH/3T3 mouse fibroblasts were infected with the Moloney strain of murine leukemia virus, part of the viral genome RNA molecules were detected in polyribosomes of the infected cells early in the infectious cycle. The binding appears to be specific, since we could demonstrate the release of viral RNA from polyribosomes with EDTA. Moreover, when infection occurred in the presence of cycloheximide, most viral RNA molecules were detected in the free cytoplasm. Size analysis on polyribosomal viral RNA molecules indicated that two size class molecules, 38S and 23S, are present in polyribosomes at 3 h after infection. Analysis of the polyriboadenylate [poly(rA)] content of viral RNA extracted from infected polyribosomes demonstrated that such molecules bind with greatest abundance at 3 h after infection, as has been detected with total viral RNA. No molecules lacking poly(rA) stretches could be detected in polyribosomes. Furthermore, when a similar analysis was performed on unbound molecules present in the free cytoplasm, identical results were obtained. We conclude that no selection towards poly(rA)-containing viral molecules is evident on binding to polyribosomes. These findings suggest that the incoming viral genome of the Moloney strain of murine leukemia virus may serve as a messenger for the synthesis of one or more virus-specific proteins early after infection of mouse fibroblasts.
当用莫洛尼鼠白血病病毒株感染NIH/3T3小鼠成纤维细胞时,在感染周期早期,在被感染细胞的多核糖体中检测到部分病毒基因组RNA分子。这种结合似乎具有特异性,因为我们可以用乙二胺四乙酸(EDTA)证明病毒RNA从多核糖体中释放出来。此外,当在放线菌酮存在的情况下发生感染时,大多数病毒RNA分子在游离细胞质中被检测到。对多核糖体病毒RNA分子的大小分析表明,感染后3小时,多核糖体中存在两种大小类别的分子,即38S和23S。对从感染的多核糖体中提取的病毒RNA的聚腺苷酸[poly(rA)]含量分析表明,与总病毒RNA检测结果一样,此类分子在感染后3小时结合最为丰富。在多核糖体中未检测到缺乏poly(rA)延伸的分子。此外,当对游离细胞质中存在的未结合分子进行类似分析时,也得到了相同的结果。我们得出结论,在与多核糖体结合时,没有明显选择含poly(rA)的病毒分子。这些发现表明,莫洛尼鼠白血病病毒株进入的病毒基因组在感染小鼠成纤维细胞后早期可能作为一种信使,用于合成一种或多种病毒特异性蛋白质。
