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水泡性口炎病毒感染细胞的RNA合成:复制的体内调节

RNA synthesis of vesicular stomatitis virus-infected cells: in vivo regulation of replication.

作者信息

Simonsen C C, Batt-Humphries S, Summers D F

出版信息

J Virol. 1979 Jul;31(1):124-32. doi: 10.1128/JVI.31.1.124-132.1979.

Abstract

Pulse-labeling of vesicular stomatitis virus-infected HeLa and BHK cells with [3H]uridine throughout the infectious cycle demonstrated two peaks of uridine incorporation into virus-specific RNA molecules. By separating total RNA synthesis into replication and transcription products, we showed that replication occurs over a shorter period of time in one peak synthesis. The biphasic nature of uridine incorporation is in part due to a general membrane phenomenon of reduced metabolite transport during vesicular stomatis virus infection and in part due to the apparent uncoupling of replication and transcription. A change in the ratio of newly synthesized plus and minus strands of the genome length (42S) RNA was found as the infection proceeded. Early in the infection, plus-stranded 42S RNA comprised 40% of the total genome length RNA synthesis, whereas late in infection, only 15 to 20% of the 42S RNA synthesized was complementary to the virion minus strand. Our data suggest that the rate of synthesis of plus-stranded 42S RNA was constant throughout the infection. The rate of virus release was determined by monitoring the uptake of [3H]uridine into released virus particles. Virus maturation and release are closely associated with the assembly of 42S RNA-containing nucleocapsids.

摘要

在整个感染周期中,用[3H]尿苷对感染水疱性口炎病毒的HeLa细胞和BHK细胞进行脉冲标记,结果显示尿苷掺入病毒特异性RNA分子有两个峰值。通过将总RNA合成分为复制产物和转录产物,我们发现复制在一个峰值合成中发生的时间较短。尿苷掺入的双相性质部分归因于水疱性口炎病毒感染期间代谢物转运减少的一般膜现象,部分归因于复制和转录明显的解偶联。随着感染的进行,发现基因组长度(42S)RNA新合成的正链和负链比例发生了变化。在感染早期,正链42S RNA占总基因组长度RNA合成的40%,而在感染后期,合成的42S RNA中只有15%至20%与病毒粒子负链互补。我们的数据表明,在整个感染过程中正链42S RNA的合成速率是恒定的。通过监测[3H]尿苷掺入释放的病毒颗粒中的情况来确定病毒释放速率。病毒成熟和释放与含42S RNA核衣壳的组装密切相关。

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