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酿酒酵母U3A小核仁核糖核蛋白颗粒的体内和体外结构-功能分析:蛋白质-RNA相互作用以及与核糖体前体RNA的碱基配对相互作用

An in vivo and in vitro structure-function analysis of the Saccharomyces cerevisiae U3A snoRNP: protein-RNA contacts and base-pair interaction with the pre-ribosomal RNA.

作者信息

Méreau A, Fournier R, Grégoire A, Mougin A, Fabrizio P, Lührmann R, Branlant C

机构信息

Laboratoire d'Enzymologie et de Génie Génétique, URA CNRS 457, Université de Nancy 1, Boulevard des Aiguillettes, 54506 Vandoeuvre les Nancy cedex, BP239, France.

出版信息

J Mol Biol. 1997 Oct 31;273(3):552-71. doi: 10.1006/jmbi.1997.1320.

DOI:10.1006/jmbi.1997.1320
PMID:9356246
Abstract

The structure and accessibility of the S. cerevisiae U3A snoRNA was studied in semi-purified U3A snoRNPs using both chemical and enzymatic probes and in vivo using DMS as the probe. The results obtained show that S. cerevisiae U3A snoRNA is composed of a short 5' domain with two stem-loop structures containing the phylogenetically conserved boxes A' and A and a large cruciform 3' domain containing boxes B, C, C' and D. A precise identification of RNA-protein contacts is provided. Protection by proteins in the snoRNP and in vivo are nearly identical and were exclusively found in the 3' domain. There are two distinct protein anchoring sites: (i), box C' and its surrounding region, this site probably includes box D, (ii) the boxes B and C pair and the bases of stem-loop 2 and 4. Box C' is wrapped by the proteins. RNA-protein interactions are more loose at the level of boxes C and D and a box C and D interaction is preserved in the snoRNP. In accord with this location of the protein binding sites, an in vivo mutational analysis showed that box C' is important for U3A snoRNA accumulation, whereas mutations in the 5' domain have little effect on RNA stability. Our in vivo probing experiments strongly suggest that, in exponentially growing cells, most of the U3A snoRNA molecules are involved in the 10-bp interaction with the 5'-ETS region and in two of the interactions recently proposed with 18S rRNA sequences. Our experimental study leads to a slightly revised version of the model of interaction proposed by J. Hughes. Single-stranded segments linking the heterologous helices are highly sensitive to DMS in vivo and their functional importance was tested by a mutational analysis.

摘要

利用化学和酶促探针,在半纯化的U3A小核仁核糖核蛋白颗粒(snoRNPs)中研究了酿酒酵母U3A小核仁RNA(snoRNA)的结构和可及性,并在体内以二甲基亚砜(DMS)作为探针进行了研究。所得结果表明,酿酒酵母U3A snoRNA由一个短的5'结构域和一个大的十字形3'结构域组成,5'结构域有两个茎环结构,包含系统发育保守的A'盒和A盒,3'结构域包含B、C、C'和D盒。提供了RNA与蛋白质相互作用位点的精确鉴定。snoRNP中的蛋白质和体内的蛋白质所提供的保护几乎相同,且仅在3'结构域中发现。有两个不同的蛋白质锚定位点:(i),C'盒及其周围区域,该位点可能包括D盒;(ii)B盒和C盒对以及茎环2和4的碱基。C'盒被蛋白质包裹。在C盒和D盒水平上,RNA与蛋白质的相互作用较为松散,并且在snoRNP中保留了C盒和D盒之间的相互作用。与蛋白质结合位点的这种定位一致,体内突变分析表明,C'盒对U3A snoRNA的积累很重要,而5'结构域中的突变对RNA稳定性影响很小。我们的体内探测实验强烈表明,在指数生长的细胞中,大多数U3A snoRNA分子参与了与5'-外部转录间隔区(ETS)区域的10个碱基对的相互作用,以及最近提出的与18S rRNA序列的两种相互作用。我们的实验研究导致了J. Hughes提出的相互作用模型的一个略有修订的版本。连接异源螺旋的单链片段在体内对DMS高度敏感,并且通过突变分析测试了它们的功能重要性。

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