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一种疱疹病毒遗传元件,其在缺乏病毒GADD34功能的情况下影响翻译。

A herpesvirus genetic element which affects translation in the absence of the viral GADD34 function.

作者信息

Mohr I, Gluzman Y

机构信息

Wyeth-Ayerst Research, Lederle Laboratories, Pearl River, NY 10965, USA.

出版信息

EMBO J. 1996 Sep 2;15(17):4759-66.

PMID:8887567
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC452208/
Abstract

Novel suppressor variants of conditionally lethal HSV-1 gamma34.5 deletion mutants have been isolated which exhibit restored ability to grow on neoplastic neuronal cells. Deletion of the viral gamma34.5 genes, whose products share functional similarity with the cellular GADD34 gene, renders the virus non-neurovirulent and imposes a block to viral replication in neuronal cells. Protein synthesis ceases at late times post-infection and the translation initiation factor eIF2alpha is phosphorylated by the cellular PKR kinase [Chou et al. (1990) Science, 252, 1262-1266; (1995) Proc. Natl Acad. Sci. USA, 92, 10516-10520]. The suppressor mutants have overcome the translational block imposed by PKR. Multiple, independent isolates all contain rearrangements within a 595 bp element in the HSV-1 genome where the unique short component joins the terminal repeats. This alteration, which affects the production of the viral mRNA and protein from the Us11 and Us12 genes, is both necessary and sufficient to confer the suppressor phenotype on gamma34.5 mutant viruses. HSV-1 thus encodes a specific element which inhibits ongoing protein synthesis in the absence of the viral GADD34-like function. Since this inhibition involves the accumulation of phosphorylated eIF2alpha, the element identified by the suppressor mutations may be a discrete PKR activator. Activation of the PKR kinase thus does not proceed through a general, cellular 'antiviral' sensing mechanism. Instead, the virus deliberately activates PKR and encodes a separate function which selectively prevents the phosphorylation of at least one PKR target, eIF2alpha. The nature of this potential activator element, and how analogous cellular elements could affect PKR pathways which affect growth arrest and differentiation are discussed.

摘要

已分离出有条件致死性单纯疱疹病毒1型γ34.5缺失突变体的新型抑制变体,这些变体在肿瘤性神经元细胞上表现出恢复的生长能力。病毒γ34.5基因的缺失使其产物与细胞GADD34基因具有功能相似性,导致病毒无神经毒性,并在神经元细胞中阻止病毒复制。感染后期蛋白质合成停止,翻译起始因子eIF2α被细胞PKR激酶磷酸化[Chou等人(1990年)《科学》,252卷,1262 - 1266页;(1995年)《美国国家科学院院刊》,92卷,10516 - 10520页]。抑制突变体克服了PKR施加的翻译阻断。多个独立分离株均在单纯疱疹病毒1型基因组中一个595 bp元件内发生重排,该元件位于独特短片段与末端重复序列相连处。这种改变影响了Us11和Us12基因的病毒mRNA和蛋白质的产生,对于赋予γ34.5突变病毒抑制表型而言既必要又充分。因此,单纯疱疹病毒1型编码一种特定元件,在缺乏病毒GADD34样功能时抑制正在进行的蛋白质合成。由于这种抑制涉及磷酸化eIF2α的积累,抑制突变鉴定出的元件可能是一种离散的PKR激活剂。因此,PKR激酶的激活并非通过一般的细胞“抗病毒”传感机制进行。相反,病毒故意激活PKR并编码一种单独的功能,选择性地阻止至少一个PKR靶点eIF2α的磷酸化。本文讨论了这种潜在激活元件的性质,以及类似的细胞元件如何影响影响生长停滞和分化的PKR途径。

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本文引用的文献

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The carboxyl terminus of the murine MyD116 gene substitutes for the corresponding domain of the gamma(1)34.5 gene of herpes simplex virus to preclude the premature shutoff of total protein synthesis in infected human cells.小鼠MyD116基因的羧基末端替代单纯疱疹病毒γ(1)34.5基因的相应结构域,以防止感染的人类细胞中总蛋白质合成过早终止。
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The US 9, 10, 11, and 12 genes of herpes simplex virus type 1 are of no importance for its neurovirulence and latency in mice.单纯疱疹病毒1型的美国9、10、11和12基因对其在小鼠中的神经毒性和潜伏性并不重要。
Virology. 1993 May;194(1):419-23. doi: 10.1006/viro.1993.1279.
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Host Innate Immune Response and Viral Immune Evasion During Alphaherpesvirus Infection.α疱疹病毒感染过程中的宿主固有免疫应答与病毒免疫逃逸。
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