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灵长类肉瘤病毒克隆分离株 gag 基因产物差异表达所涉及的分子机制。

Molecular mechanisms involved in the differential expression of gag gene products by clonal isolates of a primate sarcoma virus.

作者信息

Robbins K C, Okabe H, Tronick S R, Gilden R V, Aaronson S A

出版信息

J Virol. 1978 Feb;25(2):471-8. doi: 10.1128/JVI.25.2.471-478.1978.

Abstract

Clonal isolates of an early passage stock of woolly monkey sarcoma virus (WSV) have been shown to code for different numbers of woolly monkey helper leukemia virus gag gene products. In the present report, the molecular mechanisms responsible for their differential expression of gag gene products have been analyzed. Three WSV RNA genomes were shown to possess sedimentation coefficients consistent with the differences demonstrated in their allotments of helper viral sequences. The WSV variant (WSV clone 9) that expressed no detectable proteins was shown to contain the largest amount of helper viral information. Moreover, there was no additive hybridization of the WLV complementary DNA probe by RNA of this WSV clone and that of a WSV clone coding for several gag gene products. These results suggest that the lack of expression of gag gene products by WSV clone 9 is not due to a major deletion of helper viral gag gene sequences. Similar levels of WLV-specific RNA were demonstrated in cells nonproductively transformed by each WSV clone, arguing that the ability to express gag gene proteins was not related to the magnitude of viral RNA transcription. Taken together, the results are most consistent with a mechanism by which small deletions or point mutations in the genomes of some WSV variants result in premature termination of translation or synthesis of immunologically nonreactive gag gene proteins. The present findings have implications concerning the effects of evolutionary selective pressures on helper viral genetic information in mammalian transforming viruses.

摘要

绒毛猴肉瘤病毒(WSV)早期传代毒株的克隆分离物已被证明编码不同数量的绒毛猴辅助白血病病毒gag基因产物。在本报告中,已对其gag基因产物差异表达的分子机制进行了分析。三种WSV RNA基因组的沉降系数与它们在辅助病毒序列分配中所显示的差异一致。不表达可检测蛋白质的WSV变体(WSV克隆9)被证明含有最多的辅助病毒信息。此外,该WSV克隆的RNA与编码几种gag基因产物的WSV克隆的RNA之间不存在WLV互补DNA探针的加成杂交。这些结果表明,WSV克隆9缺乏gag基因产物表达并非由于辅助病毒gag基因序列的重大缺失。在由每个WSV克隆非生产性转化的细胞中,显示出相似水平的WLV特异性RNA,这表明表达gag基因蛋白的能力与病毒RNA转录的程度无关。综上所述,这些结果最符合一种机制,即某些WSV变体基因组中的小缺失或点突变导致翻译过早终止或合成免疫无反应性的gag基因蛋白。本研究结果对进化选择压力对哺乳动物转化病毒中辅助病毒遗传信息的影响具有启示意义。

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