Department of Structural Cell Biology, Max Planck Institute of Biochemistry, Munich, Germany.
Elife. 2020 Nov 16;9:e61467. doi: 10.7554/eLife.61467.
The yeast THO complex is recruited to active genes and interacts with the RNA-dependent ATPase Sub2 to facilitate the formation of mature export-competent messenger ribonucleoprotein particles and to prevent the co-transcriptional formation of RNA:DNA-hybrid-containing structures. How THO-containing complexes function at the mechanistic level is unclear. Here, we elucidated a 3.4 Å resolution structure of THO-Sub2 by cryo-electron microscopy. THO subunits Tho2 and Hpr1 intertwine to form a platform that is bound by Mft1, Thp2, and Tex1. The resulting complex homodimerizes in an asymmetric fashion, with a Sub2 molecule attached to each protomer. The homodimerization interfaces serve as a fulcrum for a seesaw-like movement concomitant with conformational changes of the Sub2 ATPase. The overall structural architecture and topology suggest the molecular mechanisms of nucleic acid remodeling during mRNA biogenesis.
酵母 THO 复合物被招募到活性基因上,并与 RNA 依赖性 ATP 酶 Sub2 相互作用,以促进成熟的具有出口能力的信使核糖核蛋白颗粒的形成,并防止 RNA:DNA 杂交结构的共转录形成。THO 包含的复合物在机制水平上如何发挥作用尚不清楚。在这里,我们通过冷冻电子显微镜解析了 THO-Sub2 的 3.4Å 分辨率结构。THO 亚基 Tho2 和 Hpr1 相互缠绕形成一个平台,该平台被 Mft1、Thp2 和 Tex1 结合。所得复合物以不对称的方式同源二聚化,每个原聚体上都附着有一个 Sub2 分子。同源二聚化界面充当一个支点,与 Sub2 ATP 酶的构象变化相伴发生跷跷板式运动。整体结构架构和拓扑结构表明了 mRNA 生物发生过程中核酸重塑的分子机制。
Zotero 插件
