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生成C/D盒和H/ACA小核仁RNA以及小核仁核糖核蛋白(snoRNP)蛋白的定位需要一种连接良好且保守的核质解旋酶。

A well-connected and conserved nucleoplasmic helicase is required for production of box C/D and H/ACA snoRNAs and localization of snoRNP proteins.

作者信息

King T H, Decatur W A, Bertrand E, Maxwell E S, Fournier M J

机构信息

Department of Biochemistry and Molecular Biology, University of Massachusetts, Amherst, 01003, USA.

出版信息

Mol Cell Biol. 2001 Nov;21(22):7731-46. doi: 10.1128/MCB.21.22.7731-7746.2001.

Abstract

Biogenesis of small nucleolar RNA-protein complexes (snoRNPs) consists of synthesis of the snoRNA and protein components, snoRNP assembly, and localization to the nucleolus. Recently, two nucleoplasmic proteins from mice were observed to bind to a model box C/D snoRNA in vitro, suggesting that they function at an early stage in snoRNP biogenesis. Both proteins have been described in other contexts. The proteins, called p50 and p55 in the snoRNA binding study, are highly conserved and related to each other. Both have Walker A and B motifs characteristic of ATP- and GTP-binding and nucleoside triphosphate-hydrolyzing domains, and the mammalian orthologs have DNA helicase activity in vitro. Here, we report that the Saccharomyces cerevisiae ortholog of p50 (Rvb2, Tih2p, and other names) is required for production of C/D snoRNAs in vivo and, surprisingly, H/ACA snoRNAs as well. Point mutations in the Walker A and B motifs cause temperature-sensitive or lethal growth phenotypes and severe defects in snoRNA accumulation. Notably, depletion of p50 (called Rvb2 in this study) also impairs localization of C/D and H/ACA core snoRNP proteins Nop1p and Gar1p, suggesting a defect(s) in snoRNP assembly or trafficking to the nucleolus. Findings from other studies link Rvb2 orthologs with chromatin remodeling and transcription. Taken together, the present results indicate that Rvb2 is involved in an early stage of snoRNP biogenesis and may play a role in coupling snoRNA synthesis with snoRNP assembly and localization.

摘要

小核仁核糖核蛋白复合体(snoRNPs)的生物发生包括小核仁RNA(snoRNA)和蛋白质成分的合成、snoRNP组装以及定位于核仁。最近,在体外观察到两种来自小鼠的核质蛋白与一个模型C/D盒小核仁RNA结合,这表明它们在snoRNP生物发生的早期阶段发挥作用。这两种蛋白在其他情况下已有描述。在snoRNA结合研究中被称为p50和p55的这两种蛋白高度保守且相互关联。它们都具有Walker A和B基序,这是ATP和GTP结合以及核苷三磷酸水解结构域的特征,并且哺乳动物的直系同源物在体外具有DNA解旋酶活性。在这里,我们报告酿酒酵母中p50的直系同源物(Rvb2、Tih2p及其他名称)在体内是产生C/D snoRNAs所必需的,而且令人惊讶的是,对于H/ACA snoRNAs也是必需的。Walker A和B基序中的点突变会导致温度敏感或致死生长表型以及snoRNA积累的严重缺陷。值得注意的是,p50(在本研究中称为Rvb2)的缺失也会损害C/D和H/ACA核心snoRNP蛋白Nop1p和Gar1p的定位,这表明在snoRNP组装或向核仁的运输过程中存在缺陷。其他研究的结果将Rvb2直系同源物与染色质重塑和转录联系起来。综上所述,目前的结果表明Rvb2参与了snoRNP生物发生的早期阶段,并且可能在将snoRNA合成与snoRNP组装和定位相偶联的过程中发挥作用。

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