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The structure of Rpf2–Rrs1 explains its role in ribosome biogenesis

机译:Rpf2-Rrs1的结构解释了其在核糖体生物发生中的作用

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摘要

The assembly of eukaryotic ribosomes is a hierarchical process involving about 200 biogenesis factors and a series of remodeling steps. The 5S RNP consisting of the 5S rRNA, RpL5 and RpL11 is recruited at an early stage, but has to rearrange during maturation of the pre-60S ribosomal subunit. Rpf2 and Rrs1 have been implicated in 5S RNP biogenesis, but their precise role was unclear. Here, we present the crystal structure of the Rpf2–Rrs1 complex from Aspergillus nidulans at 1.5 Å resolution and describe it as Brix domain of Rpf2 completed by Rrs1 to form two anticodon-binding domains with functionally important tails. Fitting the X-ray structure into the cryo-EM density of a previously described pre-60S particle correlates with biochemical data. The heterodimer forms specific contacts with the 5S rRNA, RpL5 and the biogenesis factor Rsa4. The flexible protein tails of Rpf2–Rrs1 localize to the central protuberance. Two helices in the Rrs1 C-terminal tail occupy a strategic position to block the rotation of 25S rRNA and the 5S RNP. Our data provide a structural model for 5S RNP recruitment to the pre-60S particle and explain why removal of Rpf2–Rrs1 is necessary for rearrangements to drive 60S maturation.
机译:真核生物核糖体的组装是一个分级过程,涉及约200个生物发生因子和一系列重塑步骤。由5S rRNA,RpL5和RpL11组成的5S RNP在早期被募集,但在60S前核糖体亚基成熟期间必须重新排列。 Rpf2和Rrs1已牵涉5S RNP生物发生,但它们的确切作用尚不清楚。在这里,我们介绍来自构巢曲霉的Rpf2-Rrs1复合物的晶体结构,分辨率为1.5Å,并将其描述为由Rrs1完成的Rpf2的Brix结构域,形成两个具有重要功能尾的反密码子结合结构域。将X射线结构拟合到先前描述的60S之前的粒子的冷冻EM密度与生化数据相关。异二聚体与5S rRNA,RpL5和生物发生因子Rsa4形成特异性接触。 Rpf2–Rrs1的柔性蛋白尾巴位于中央突起。 Rrs1 C末端尾部的两个螺旋占据重要位置,以阻止25S rRNA和5S RNP的旋转。我们的数据为5S RNP募集到60S之前的颗粒提供了结构模型,并解释了为什么去除Rpf2-Rrs1对于重新排列驱动60S成熟是必要的。

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