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Cbf5p是一种潜在的假尿嘧啶合酶,Nhp2p是一种假定的RNA结合蛋白,它们与Gar1p共同存在于所有H BOX/ACA基序的小核仁核糖核蛋白中,并构成一种常见的二分结构。

Cbf5p, a potential pseudouridine synthase, and Nhp2p, a putative RNA-binding protein, are present together with Gar1p in all H BOX/ACA-motif snoRNPs and constitute a common bipartite structure.

作者信息

Watkins N J, Gottschalk A, Neubauer G, Kastner B, Fabrizio P, Mann M, Lührmann R

机构信息

Institut für Molekularbiologie und Tumorforschung, Philipps-Universität Marburg, Germany.

出版信息

RNA. 1998 Dec;4(12):1549-68. doi: 10.1017/s1355838298980761.

Abstract

The eukaryotic nucleolus contains a large number of small nucleolar RNAs (snoRNAs) that are involved in preribosomal RNA (pre-rRNA) processing. The H box/ACA-motif (H/ACA) class of snoRNAs has recently been demonstrated to function as guide RNAs targeting specific uridines in the pre-rRNA for pseudouridine (psi) synthesis. To characterize the protein components of this class of snoRNPs, we have purified the snR42 and snR30 snoRNP complexes by anti-m3G-immunoaffinity and Mono-Q chromatography of Saccharomyces cerevisiae extracts. Sequence analysis of the individual polypeptides demonstrated that the three proteins Gar1p, Nhp2p, and Cbf5p are common to both the snR30 and snR42 complexes. Nhp2p is a highly basic protein that belongs to a family of putative RNA-binding proteins. Cbf5p has recently been demonstrated to be involved in ribosome biogenesis and also shows striking homology with known prokaryotic psi synthases. The presence of Cbf5p, a putative psi synthase in each H/ACA snoRNP suggests that this class of RNPs functions as individual modification enzymes. Immunoprecipitation studies using either anti-Cbf5p antibodies or a hemagglutinin-tagged Nhp2p demonstrated that both proteins are associated with all H/ACA-motif snoRNPs. In vivo depletion of Nhp2p results in a reduction in the steady-state levels of all H/ACA snoRNAs. Electron microscopy of purified snR42 and snR30 particles revealed that these two snoRNPs possess a similar bipartite structure that we propose to be a major structural determining principle for all H/ACA snoRNPs.

摘要

真核生物的核仁包含大量参与前核糖体RNA(pre-rRNA)加工的小核仁RNA(snoRNA)。最近已证明,H框/ACA基序(H/ACA)类snoRNA作为引导RNA,靶向pre-rRNA中的特定尿苷以合成假尿苷(ψ)。为了表征这类snoRNP的蛋白质成分,我们通过对酿酒酵母提取物进行抗m3G免疫亲和层析和Mono-Q层析,纯化了snR42和snR30 snoRNP复合物。对各个多肽的序列分析表明,Gar1p、Nhp2p和Cbf5p这三种蛋白质在snR30和snR42复合物中都存在。Nhp2p是一种高度碱性的蛋白质,属于推定的RNA结合蛋白家族。最近已证明Cbf5p参与核糖体生物合成,并且与已知的原核ψ合成酶也有显著的同源性。每个H/ACA snoRNP中都存在推定的ψ合成酶Cbf5p,这表明这类RNP作为单独的修饰酶发挥作用。使用抗Cbf5p抗体或血凝素标记的Nhp2p进行的免疫沉淀研究表明,这两种蛋白质都与所有H/ACA基序snoRNP相关。体内消耗Nhp2p会导致所有H/ACA snoRNA的稳态水平降低。对纯化的snR42和snR30颗粒的电子显微镜观察显示,这两种snoRNP具有相似的二分结构,我们认为这是所有H/ACA snoRNP的主要结构决定原则。

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