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利用选择性核糖体谱研究酵母中转录核糖体的相互作用。

Selective ribosome profiling to study interactions of translating ribosomes in yeast.

机构信息

Center for Molecular Biology of Heidelberg University (ZMBH), DKFZ-ZMBH Alliance, Heidelberg, Germany.

German Cancer Research Center (DKFZ), Heidelberg, Germany.

出版信息

Nat Protoc. 2019 Aug;14(8):2279-2317. doi: 10.1038/s41596-019-0185-z. Epub 2019 Jul 22.

DOI:10.1038/s41596-019-0185-z
PMID:31332354
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7115923/
Abstract

A number of enzymes, targeting factors and chaperones engage ribosomes to support fundamental steps of nascent protein maturation, including enzymatic processing, membrane targeting and co-translational folding. The selective ribosome profiling (SeRP) method is a new tool for studying the co-translational activity of maturation factors that provides proteome-wide information on a factor's nascent interactome, the onset and duration of binding and the mechanisms controlling factor engagement. SeRP is based on the combination of two ribosome-profiling (RP) experiments, sequencing the ribosome-protected mRNA fragments from all ribosomes (total translatome) and the ribosome subpopulation engaged by the factor of interest (factor-bound translatome). We provide a detailed SeRP protocol, exemplified for the yeast Hsp70 chaperone Ssb (stress 70 B), for studying factor interactions with nascent proteins that is readily adaptable to identifying nascent interactomes of other co-translationally acting eukaryotic factors. The protocol provides general guidance for experimental design and optimization, as well as detailed instructions for cell growth and harvest, the isolation of (factor-engaged) monosomes, the generation of a cDNA library and data analysis. Experience in biochemistry and RNA handling, as well as basic programing knowledge, is necessary to perform SeRP. Execution of a SeRP experiment takes 8-10 working days, and initial data analysis can be completed within 1-2 d. This protocol is an extension of the originally developed protocol describing SeRP in bacteria.

摘要

许多酶、靶向因子和伴侣蛋白与核糖体结合,以支持新生蛋白成熟的基本步骤,包括酶加工、膜靶向和共翻译折叠。选择性核糖体谱(SeRP)方法是一种研究成熟因子共翻译活性的新工具,它提供了因子新生相互作用组、结合起始和持续时间以及控制因子结合机制的蛋白质组范围信息。SeRP 基于两种核糖体谱(RP)实验的结合,即从所有核糖体(总翻译组)和感兴趣因子结合的核糖体亚群(因子结合翻译组)中测序核糖体保护的 mRNA 片段。我们提供了一个详细的 SeRP 方案,以酵母 Hsp70 伴侣 Ssb(应激 70B)为例,用于研究因子与新生蛋白的相互作用,该方案易于适应鉴定其他共翻译作用的真核因子的新生相互作用组。该方案为实验设计和优化提供了一般指导,以及细胞生长和收获、(因子结合)单体的分离、cDNA 文库的生成和数据分析的详细说明。执行 SeRP 实验需要生化和 RNA 处理方面的经验,以及基本的编程知识。执行 SeRP 实验需要 8-10 个工作日,初始数据分析可以在 1-2 天内完成。该方案是最初在细菌中描述 SeRP 的方案的扩展。

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Ribosome pausing in amylase producing Bacillus subtilis during long fermentation.在长时间发酵过程中,产淀粉酶枯草芽孢杆菌中的核糖体暂停现象。
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Chp1 is a dedicated chaperone at the ribosome that safeguards eEF1A biogenesis.Chp1 是核糖体上的一种专门伴侣蛋白,可保护 eEF1A 的生物发生。
Nat Commun. 2024 Feb 15;15(1):1382. doi: 10.1038/s41467-024-45645-w.
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