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小核仁RNA帽三甲基转移酶是核糖体合成和完整核仁形态所必需的。

The small nucle(ol)ar RNA cap trimethyltransferase is required for ribosome synthesis and intact nucleolar morphology.

作者信息

Colau Geoffroy, Thiry Marc, Leduc Vivian, Bordonné Rémy, Lafontaine Denis L J

机构信息

Fonds National de la Recherche Scientifique, Université Libre de Bruxelles, Institut de Biologie et de Médecine Moléculaires, Charleroi-Gosselies, Belgium.

出版信息

Mol Cell Biol. 2004 Sep;24(18):7976-86. doi: 10.1128/MCB.24.18.7976-7986.2004.

Abstract

Nucleolar morphogenesis is a poorly defined process. Here we report that the Saccharomyces cerevisiae nucleolar trimethyl guanosine synthase I (Tgs1p), which specifically selects the m(7)G cap structure of snRNAs and snoRNAs for m(2,2,7)G conversion, is required not only for efficient pre-mRNA splicing but also for pre-rRNA processing and small ribosomal subunit synthesis. Mutational analysis indicates that the requirement for Tgs1p in pre-mRNA splicing, but not its involvement in ribosome synthesis, is dependent upon its function in cap trimethylation. In addition, we report that cells lacking Tgs1p showed a striking and unexpected loss of nucleolar structural organization. Tgs1p is not a core component of the snoRNP proteins; however, in vitro, the protein interacts with the KKD/E domain present at the carboxyl-terminal ends of several snoRNP proteins. Strains expressing versions of the snoRNPs lacking the KKD/E domain were also defective for nucleolar morphology and showed a loss of nucleolar compaction. We propose that the transient and functional interactions of Tgs1p with the abundant snoRNPs, through presumed interactions with the KKD/E domain of the snoRNP proteins, contribute substantially to the coalescence of nucleolar components. This conclusion is compatible with a model of self-organization for nucleolar assembly.

摘要

核仁形态发生是一个定义尚不明确的过程。在此我们报告,酿酒酵母核仁三甲基鸟苷合酶I(Tgs1p)不仅对于有效的前体mRNA剪接是必需的,而且对于前体rRNA加工和小核糖体亚基合成也是必需的,该酶特异性地选择snRNA和snoRNA的m(7)G帽结构进行m(2,2,7)G转化。突变分析表明,Tgs1p在前体mRNA剪接中的需求,而非其在核糖体合成中的参与,取决于其在帽三甲基化中的功能。此外,我们报告缺乏Tgs1p的细胞显示出核仁结构组织显著且意外的丧失。Tgs1p不是snoRNP蛋白的核心成分;然而,在体外,该蛋白与几种snoRNP蛋白羧基末端存在的KKD/E结构域相互作用。表达缺乏KKD/E结构域的snoRNP版本的菌株在核仁形态方面也存在缺陷,并显示出核仁致密化的丧失。我们提出,Tgs1p与丰富的snoRNP通过与snoRNP蛋白的KKD/E结构域的假定相互作用而发生的瞬时和功能性相互作用,对核仁成分的聚结有很大贡献。这一结论与核仁组装的自组织模型相符。

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