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在虫草素(3'-脱氧腺苷)存在的情况下,痘苗病毒感染细胞中宿主蛋白质合成的抑制作用

Inhibition of host protein synthesis in vaccinia virus-infected cells in the presence of cordycepin (3'-deoxyadenosine).

作者信息

Person A, Beaud G

出版信息

J Virol. 1978 Jan;25(1):11-8. doi: 10.1128/JVI.25.1.11-18.1978.

Abstract

Cordycepin inhibited efficiently viral mRNA and polyadenylic acid syntheses in vaccinia virus-infected cells, but allowed the shutoff of host protein synthesis to occur. Therefore, cordycepin was used to study this shutoff in the absence of gene expression. Ribosome transit time was increased in infected cells, revealing an inhibition at the level of elongation and/or release of polypeptide chains. However, the disappearance of heavy polysomes in vaccinia virus-infected cells showed that the inhibition of host protein synthesis resulted predominantly from a block at the stage of initiation. This conclusion was confirmed by the recovery of heavy polyribosomes when low levels of cycloheximide were added to slow down ribosome release from the mRNA. Similar amounts of cellular mRNA (present in the polyribosomes) were found in vaccinia virus-infected cells and in mock-infected cels (exposed to cordycepin), showing that the cellular mRNA was not inactivated in these conditions. It was concluded that a component of the vaccinia virion inhibits, in the absence of viral RNA and polyadenylic acid syntheses, host protein synthesis at the level of initiation and, to a lesser extent, at the level of elongation (and/or release) of polypeptide chains.

摘要

虫草素能有效抑制痘苗病毒感染细胞中病毒mRNA和聚腺苷酸的合成,但却允许宿主蛋白合成的关闭发生。因此,在不存在基因表达的情况下,虫草素被用于研究这种关闭现象。感染细胞中的核糖体转运时间增加,这表明在多肽链的延伸和/或释放水平上存在抑制作用。然而,痘苗病毒感染细胞中重多聚核糖体的消失表明,宿主蛋白合成的抑制主要是由起始阶段的阻断导致的。当加入低水平的环己酰亚胺以减缓核糖体从mRNA上的释放时,重多聚核糖体的恢复证实了这一结论。在痘苗病毒感染细胞和模拟感染细胞(暴露于虫草素)中发现了相似数量的细胞mRNA(存在于多聚核糖体中),这表明细胞mRNA在这些条件下没有失活。得出的结论是,在不存在病毒RNA和聚腺苷酸合成的情况下,痘苗病毒粒子的一种成分在起始水平上抑制宿主蛋白合成,在较小程度上也在多肽链的延伸(和/或释放)水平上抑制宿主蛋白合成。

相似文献

本文引用的文献

1
MESSENGER RNA IN CELLS INFECTED WITH VACCINIA VIRUS.感染痘苗病毒的细胞中的信使核糖核酸
Proc Natl Acad Sci U S A. 1964 Apr;51(4):577-85. doi: 10.1073/pnas.51.4.577.

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