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LAS1L interacts with the mammalian Rix1 complex to regulate ribosome biogenesis

机译:LAS1L与哺乳动物Rix1复合物相互作用以调节核糖体的生物发生

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The coordination of RNA polymerase I transcription with pre-rRNA processing, preribosomal particle assembly, and nuclear export is a finely tuned process requiring the concerted actions of a number of accessory factors. However, the exact functions of some of these proteins and how they assemble in subcomplexes remain poorly defined. LAS1L was first described as a nucleolar protein required for maturation of the 60S preribosomal subunit. In this paper, we demonstrate that LAS1L interacts with PELP1, TEX10, and WDR18, the mammalian homologues of the budding yeast Rix1 complex, along with NOL9 and SENP3, to form a novel nucleolar complex that cofractionates with the 60S preribosomal subunit. Depletion of LAS1L-associated proteins results in a p53-dependent G1 arrest and leads to defects in processing of the pre-rRNA internal transcribed spacer 2 region. We further show that the nucleolar localization of this complex requires active RNA polymerase I transcription and the small ubiquitin-like modifier–specific protease SENP3. Taken together, our data identify a novel mammalian complex required for 60S ribosomal subunit synthesis, providing further insight into the intricate, yet poorly described, process of ribosome biogenesis in higher eukaryotes.
机译:RNA聚合酶I转录与前rRNA加工,核糖体颗粒组装和核输出的协调是一个微调的过程,需要许多辅助因素的共同作用。但是,其中一些蛋白质的确切功能以及它们在亚复合物中的组装方式仍然不清楚。 LAS1L首先被描述为60S核糖体前亚基成熟所需的核仁蛋白。在本文中,我们证明了LAS1L与PELP1,TEX10和WDR18(萌芽的酵母Rix1复合物的哺乳动物同源物)以及NOL9和SENP3相互作用,形成了与60S核糖体前亚基共馏的新型核仁复合物。 LAS1L相关蛋白的消耗导致p53依赖性G1阻滞,并导致pre-rRNA内部转录间隔区2区域加工中的缺陷。我们进一步表明,这种复合物的核仁定位需要活性RNA聚合酶I转录和小的泛素样修饰物特异性蛋白酶SENP3。综上所述,我们的数据确定了60S核糖体亚基合成所需的新型哺乳动物复合物,从而提供了对高级真核生物中核糖体生物发生过程的复杂但尚未充分描述的进一步了解。

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