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在最小 rRNA 和核糖体蛋白 S4 共孵育过程中稳定复合物的缓慢形成。

Slow formation of stable complexes during coincubation of minimal rRNA and ribosomal protein S4.

机构信息

Program in Cell, Molecular and Developmental Biology and Biophysics, Johns Hopkins University, 3400 North Charles Street, Baltimore, MD 21218, USA.

出版信息

J Mol Biol. 2011 Sep 23;412(3):453-65. doi: 10.1016/j.jmb.2011.07.048. Epub 2011 Jul 29.

DOI:10.1016/j.jmb.2011.07.048
PMID:21821049
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3167742/
Abstract

Ribosomal protein S4 binds and stabilizes a five-helix junction or five-way junction (5WJ) in the 5' domain of 16S ribosomal RNA (rRNA) and is one of two proteins responsible for nucleating 30S ribosome assembly. Upon binding, both protein S4 and 5WJ reorganize their structures. We show that labile S4 complexes rearrange into stable complexes within a few minutes at 42 °C, with longer coincubation leading to an increased population of stable complexes. In contrast, prefolding the rRNA has a smaller effect on stable S4 binding. Experiments with minimal rRNA fragments show that this structural change depends only on 16S residues within the S4 binding site. SHAPE (selective 2'-hydroxyl acylation analyzed by primer extension) chemical probing experiments showed that S4 strongly stabilizes 5WJ and the helix (H) 18 pseudoknot, which become tightly folded within the first minute of S4 binding. However, a kink in H16 that makes specific contacts with the S4 N-terminal extension, as well as a right-angle motif between H3, H4, and H18, requires a minute or more to become fully structured. Surprisingly, S4 structurally reorganizes the 530-loop and increases the flexibility of H3, which is proposed to undergo a conformational switch during 30S assembly. These elements of the S4 binding site may require other 30S proteins to reach a stable conformation.

摘要

核糖体蛋白 S4 结合并稳定了 16S 核糖体 RNA(rRNA)5' 结构域中的五螺旋结(5WJ),是负责引发 30S 核糖体组装的两种蛋白质之一。结合后,蛋白质 S4 和 5WJ 都会重新组织其结构。我们发现不稳定的 S4 复合物在 42°C 下几分钟内重新排列成稳定的复合物,而更长时间的共孵育会导致稳定复合物的比例增加。相比之下,rRNA 的预折叠对稳定 S4 结合的影响较小。使用最小 rRNA 片段的实验表明,这种结构变化仅取决于 S4 结合位点内的 16S 残基。SHAPE(通过引物延伸选择性 2'-羟基酰化分析)化学探测实验表明,S4 强烈稳定 5WJ 和 H18 假结,这些结构在 S4 结合的最初一分钟内变得紧密折叠。然而,H16 中的一个拐点与 S4 N 端延伸形成特定接触,以及 H3、H4 和 H18 之间的直角模体,需要一分钟或更长时间才能完全形成结构。令人惊讶的是,S4 对 530 环进行了结构重组,并增加了 H3 的灵活性,这被提议在 30S 组装过程中发生构象转换。S4 结合位点的这些元素可能需要其他 30S 蛋白才能达到稳定构象。

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