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转化和回复野生田鼠细胞中劳斯肉瘤病毒特异性RNA的性质

Nature of Rous sarcoma virus-specific RNA in transformed and revertant field vole cells.

作者信息

Krzyzek R A, Lau A F, Faras A J

出版信息

J Virol. 1979 Feb;29(2):507-15. doi: 10.1128/JVI.29.2.507-516.1979.

Abstract

Cytoplasmic and polyribosomal RNAs from Rous sarcoma virus-transformed and phenotypically reverted field vole cells were fractionated by rate-zonal sedimentation and hybridized with a (3)H-labeled complementary DNA viral probe to determine the size classes of virus-specific RNA present in these cell types. In contrast to Rous sarcoma virus-infected permissive avian cells, only two of three discrete species of virus-specific RNA were detected in the cytoplasm of these vole cells. These included genome-length 35S RNA and a 21S RNA. However, viral 28S RNA, routinely detected in the cytoplasm of productively infected avian cells, could not be found in cytoplasmic RNA from vole cells. In addition, a low-molecular-weight viral RNA sedimenting less than 16S was detected in both infected avian and vole cells. Because of its heterogeneity this latter species is most likely generated from the intracellular degradation of the larger viral RNAs. Both the viral 35S and 21S RNA were also found to be associated with total polyribosomes from these vole cells. Studies were also performed to determine the distribution of both total viral genomic and sarcoma-specific RNA sequences among the size classes of fractionated total polyribosomes. In both vole cell types the majority of cytoplasmic viral RNA sequences were also associated with polyribosomes and were similarly distributed among the size classes of total polyribosomes. Sarcoma-specific sequences were present on both the 35S and 21S RNA species. These data suggest that the expression of the viral transforming gene in revertant field vole cells may be controlled at some stage subsequent to translation of the viral RNA.

摘要

通过速率区带沉降法对来自劳氏肉瘤病毒转化的和表型回复的田鼠细胞的细胞质RNA和多核糖体RNA进行分级分离,并用3H标记的互补DNA病毒探针进行杂交,以确定这些细胞类型中存在的病毒特异性RNA的大小类别。与感染劳氏肉瘤病毒的允许性禽类细胞不同,在这些田鼠细胞的细胞质中仅检测到三种离散的病毒特异性RNA中的两种。这些包括基因组长度的35S RNA和21S RNA。然而,在生产性感染的禽类细胞的细胞质中常规检测到的病毒28S RNA,在田鼠细胞的细胞质RNA中未发现。此外,在感染的禽类和田鼠细胞中均检测到沉降小于16S的低分子量病毒RNA。由于其异质性,后一种RNA很可能是由较大病毒RNA的细胞内降解产生的。病毒35S和21S RNA也被发现与这些田鼠细胞的总多核糖体相关。还进行了研究以确定分级分离的总多核糖体的大小类别中总病毒基因组和肉瘤特异性RNA序列的分布。在两种田鼠细胞类型中,大多数细胞质病毒RNA序列也与多核糖体相关,并且在总多核糖体的大小类别中分布相似。肉瘤特异性序列存在于35S和21S RNA种类上。这些数据表明,病毒转化基因在回复的田鼠细胞中的表达可能在病毒RNA翻译后的某个阶段受到控制。

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