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30S核糖体亚基的纯化及其生化与冷冻电镜分析

30S Ribosomal Subunit Purification and Its Biochemical and Cryo-EM Analysis.

作者信息

Belinite Margarita, Khusainov Iskander, Marzi Stefano

机构信息

Institut de Génétique et de Biologie Moléculaire et Cellulaire (IGBMC), INSERM U964, CNRS UMR7104, Université de Strasbourg, Illkirch, France.

Architecture et Réactivité de l'ARN, CNRS 9002, Université de Strasbourg, Strasbourg, France.

出版信息

Bio Protoc. 2022 Oct 20;12(20). doi: 10.21769/BioProtoc.4532.

Abstract

The ribosome is a complex cellular machinery whose solved structure allowed for an incredible leap in structural biology research. Different ions bind to the ribosome, stabilizing inter-subunit interfaces and structurally linking rRNAs, proteins, and ligands. Besides cations such as K and Mg , polyamines are known to stabilize the folding of RNA and overall structure. The bacterial ribosome is composed of a small (30S) subunit containing the decoding center and a large (50S) subunit devoted to peptide bond formation. We have previously shown that the small ribosomal subunit of is sensitive to changes in ionic conditions and polyamines concentration. In particular, its decoding center, where mRNA codons and tRNA anticodons interact, is prone to structural deformations in the absence of spermidine. Here, we report a detailed protocol for the purification of the intact and functional 30S, achieved through specific ionic conditions and the addition of spermidine. Using this protocol, we obtained the cryo-electron microscopy (cryo-EM) structure of the 30S-mRNA complex from at 3.6 Å resolution. The 30S-mRNA complex formation was verified by a toeprinting assay. In this article, we also include a description of toeprinting and cryo-EM protocols. The described protocols can be further used to study the process of translation regulation. Graphical abstract.

摘要

核糖体是一种复杂的细胞机制,其解析结构使结构生物学研究实现了惊人的飞跃。不同的离子与核糖体结合,稳定亚基间的界面,并在结构上连接rRNA、蛋白质和配体。除了钾离子和镁离子等阳离子外,多胺也已知能稳定RNA的折叠和整体结构。细菌核糖体由一个包含解码中心的小(30S)亚基和一个负责肽键形成的大(50S)亚基组成。我们之前已经表明,[具体细菌名称未给出]的小核糖体亚基对离子条件和多胺浓度的变化敏感。特别是,其解码中心(mRNA密码子和tRNA反密码子相互作用之处)在没有亚精胺的情况下容易发生结构变形。在这里,我们报告了一种通过特定离子条件和添加亚精胺来纯化完整且有功能的30S的详细方案。使用该方案,我们获得了来自[具体细菌名称未给出]的30S - mRNA复合物的冷冻电子显微镜(cryo - EM)结构,分辨率为3.6 Å。通过足迹法验证了30S - mRNA复合物的形成。在本文中,我们还包括了足迹法和冷冻电子显微镜方案的描述。所描述的方案可进一步用于研究翻译调控过程。图形摘要。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/34fb/9606446/0eceef6f08e1/BioProtoc-12-20-4532-ga001.jpg

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本文引用的文献

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