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G 补丁激活剂内的抑制段在核糖体组装过程中调节 Prp43-ATP 酶的活性。

An inhibitory segment within G-patch activators tunes Prp43-ATPase activity during ribosome assembly.

机构信息

Institute of Medical Microbiology, University of Zurich, Zurich, Switzerland.

Cryo-EM Knowledge Hub, ETH Zurich, Zurich, Switzerland.

出版信息

Nat Commun. 2024 Nov 22;15(1):10150. doi: 10.1038/s41467-024-54584-5.

Abstract

Mechanisms by which G-patch activators tune the processive multi-tasking ATP-dependent RNA helicase Prp43 (DHX15 in humans) to productively remodel diverse RNA:protein complexes remain elusive. Here, a comparative study between a herein and previously characterized activators, Tma23 and Pxr1, respectively, defines segments that organize Prp43 function during ribosome assembly. In addition to the activating G-patch, we discover an inhibitory segment within Tma23 and Pxr1, I-patch, that restrains Prp43 ATPase activity. Cryo-electron microscopy and hydrogen-deuterium exchange mass spectrometry show how I-patch binds to the catalytic RecA-like domains to allosterically inhibit Prp43 ATPase activity. Tma23 and Pxr1 contain dimerization segments that organize Prp43 into higher-order complexes. We posit that Prp43 function at discrete locations on pre-ribosomal RNA is coordinated through toggling interactions with G-patch and I-patch segments. This could guarantee measured and timely Prp43 activation, enabling precise control over multiple RNA remodelling events occurring concurrently during ribosome formation.

摘要

G 斑激活剂调节具有多任务功能的依赖于 ATP 的 RNA 解旋酶 Prp43(人类中的 DHX15)以有效地重塑各种 RNA:蛋白质复合物的机制仍不清楚。在这里,分别对本研究中和以前表征的激活剂 Tma23 和 Pxr1 进行了比较研究,确定了在核糖体组装过程中组织 Prp43 功能的片段。除了激活 G 斑外,我们还在 Tma23 和 Pxr1 中发现了一个抑制片段 I 斑,它抑制 Prp43 ATP 酶活性。低温电子显微镜和氘氚交换质谱显示了 I 斑如何结合到催化 RecA 样结构域以变构抑制 Prp43 ATP 酶活性。Tma23 和 Pxr1 包含二聚化片段,将 Prp43 组织成更高阶的复合物。我们假设,通过与 G 斑和 I 斑片段的切换相互作用,在 pre-rRNA 上的离散位置上的 Prp43 功能被协调。这可以保证 Prp43 的激活得到精确控制,从而能够在核糖体形成过程中同时发生的多个 RNA 重塑事件中进行精确控制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a020/11584650/77ececc6db72/41467_2024_54584_Fig1_HTML.jpg

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