依赖 RNA 的蛋白激酶 PKR 和 Z-DNA 结合直系同源物 PKZ 在介导起始因子 eIF2α 依赖性蛋白质合成抑制和病毒诱导的应激颗粒形成方面的能力不同。
RNA-dependent protein kinase PKR and the Z-DNA binding orthologue PKZ differ in their capacity to mediate initiation factor eIF2α-dependent inhibition of protein synthesis and virus-induced stress granule formation.
机构信息
Department of Molecular, Cellular and Developmental Biology, University of California, Santa Barbara, California 93106, USA.
出版信息
Virology. 2013 Aug 15;443(1):48-58. doi: 10.1016/j.virol.2013.04.020. Epub 2013 May 23.
Abstract
Protein kinase R (PKR), a regulator of translation in mammalian cells, possesses two ds-RNA binding domains responsible for kinase activation. Protein kinase Z (PKZ), a PKR-like kinase present in fish, possesses two Z-DNA binding domains. A complementation strategy with cells stably deficient in PKR was used to compare the functions of PKR and PKZ. We found reporter expression was inhibited by wildtype (WT) PKR but not by either catalytic (K296R) or RNA-binding (K64E) mutants. PKZ, like PKR, more potently inhibited 5' cap-dependent compared to IRES-dependent reporter expression. However, in contrast to PKR-expressing cells, phosphorylation of initiation factor eIF2α was not detectably increased in PKZ-expressing cells. Furthermore, virus-induced stress granule formation was observed in PKR-deficient cells complemented with WT PKR but not K296R mutant PKR or WT PKZ. These results suggest that PKR and PKZ function by distinguishable mechanisms to modulate host responses including protein synthesis inhibition and stress granule formation.
摘要
蛋白激酶 R(PKR)是哺乳动物细胞中翻译的调节因子,具有两个 ds-RNA 结合结构域,负责激酶的激活。蛋白激酶 Z(PKZ)是一种存在于鱼类中的 PKR 样激酶,具有两个 Z-DNA 结合结构域。我们使用稳定缺乏 PKR 的细胞的互补策略来比较 PKR 和 PKZ 的功能。我们发现野生型(WT)PKR 抑制报告基因表达,但催化(K296R)或 RNA 结合(K64E)突变体则不抑制。PKZ 与 PKR 一样,更强烈地抑制 5' 帽依赖性而不是 IRES 依赖性报告基因表达。然而,与表达 PKR 的细胞不同,在表达 PKZ 的细胞中,起始因子 eIF2α 的磷酸化没有明显增加。此外,在补充 WT PKR 的 PKR 缺陷型细胞中观察到病毒诱导的应激颗粒形成,但在补充 K296R 突变体 PKR 或 WT PKZ 的细胞中则没有观察到。这些结果表明,PKR 和 PKZ 通过不同的机制发挥作用,以调节宿主反应,包括蛋白质合成抑制和应激颗粒形成。
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