Laboratoire de Biologie Moléculaire Eucaryote, Centre de Biologie Intégrative (CBI), Université de Toulouse, CNRS, UPS, Toulouse Cedex 9, France.
Institute for Cell and Molecular Biosciences, Newcastle University, Newcastle upon Tyne NE2 4HH, UK.
Nucleic Acids Res. 2018 May 18;46(9):4699-4714. doi: 10.1093/nar/gky116.
Ribosome biogenesis requires more than 200 trans-acting factors to achieve the correct production of the two mature ribosomal subunits. Here, we have identified Efg1 as a novel, nucleolar ribosome biogenesis factor in Saccharomyces cerevisiae that is directly linked to the surveillance of pre-40S particles. Depletion of Efg1 impairs early pre-rRNA processing, leading to a strong decrease in 18S rRNA and 40S subunit levels and an accumulation of the aberrant 23S rRNA. Using Efg1 as bait, we revealed a novel degradation pathway of the 23S rRNA. Co-immunoprecipitation experiments showed that Efg1 is a component of 90S pre-ribosomes, as it is associated with the 35S pre-rRNA and U3 snoRNA, but has stronger affinity for 23S pre-rRNA and its novel degradation intermediate 11S rRNA. 23S is cleaved at a new site, Q1, within the 18S sequence by the endonuclease Utp24, generating 11S and 17S' rRNA. Both of these cleavage products are targeted for degradation by the TRAMP/exosome complexes. Therefore, the Q1 site defines a novel endonucleolytic cleavage site of ribosomal RNA exclusively dedicated to surveillance of pre-ribosomal particles.
核糖体生物发生需要 200 多种反式作用因子来实现两个成熟核糖体亚基的正确生成。在这里,我们鉴定出 Efg1 是酿酒酵母中一种新的核仁核糖体生物发生因子,它与前 40S 颗粒的监测直接相关。Efg1 的耗竭会损害早期 pre-rRNA 的加工,导致 18S rRNA 和 40S 亚基水平的强烈下降,以及异常的 23S rRNA 的积累。利用 Efg1 作为诱饵,我们揭示了一种新的 23S rRNA 降解途径。共免疫沉淀实验表明,Efg1 是 90S 前核糖体的一个组成部分,因为它与 35S pre-rRNA 和 U3 snoRNA 相关,但与 23S pre-rRNA 及其新的降解中间产物 11S rRNA 的亲和力更强。23S 在 18S 序列内的新位点 Q1 被内切酶 Utp24 切割,生成 11S 和 17S' rRNA。这两种切割产物都被 TRAMP/exosome 复合物靶向降解。因此,Q1 位点定义了一个新的核酶切割位点,专门用于监测前核糖体颗粒。
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