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本文引用的文献

1
Crystal structure of the eukaryotic ribosome.真核生物核糖体的晶体结构。
Science. 2010 Nov 26;330(6008):1203-9. doi: 10.1126/science.1194294.
2
A molecular clamp ensures allosteric coordination of peptidyltransfer and ligand binding to the ribosomal A-site.分子夹确保了肽基转移和配体与核糖体 A 位结合的变构协调。
Nucleic Acids Res. 2010 Nov;38(21):7800-13. doi: 10.1093/nar/gkq641. Epub 2010 Jul 21.
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Ribosome dynamics and tRNA movement by time-resolved electron cryomicroscopy.利用时间分辨电子 cryomicroscopy 研究核糖体动力学和 tRNA 运动。
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Enhanced purity, activity and structural integrity of yeast ribosomes purified using a general chromatographic method.采用通用色谱法纯化酵母核糖体,提高其纯度、活性和结构完整性。
RNA Biol. 2010 May-Jun;7(3):354-60. doi: 10.4161/rna.7.3.11648. Epub 2010 May 22.
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Single ribosome dynamics and the mechanism of translation.单个核糖体动力学与翻译机制。
Annu Rev Biophys. 2010;39:491-513. doi: 10.1146/annurev.biophys.093008.131427.
6
Elongation in translation as a dynamic interaction among the ribosome, tRNA, and elongation factors EF-G and EF-Tu.翻译延伸作为核糖体、tRNA 以及延伸因子 EF-G 和 EF-Tu 之间的动态相互作用。
Q Rev Biophys. 2009 Aug;42(3):159-200. doi: 10.1017/S0033583509990060.
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Comprehensive molecular structure of the eukaryotic ribosome.真核生物核糖体的综合分子结构。
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The structure of the ribosome with elongation factor G trapped in the posttranslocational state.核糖体与延长因子 G 在易位后状态下的结构。
Science. 2009 Oct 30;326(5953):694-9. doi: 10.1126/science.1179709.
9
Structures of the ribosome in intermediate states of ratcheting.棘轮运动中间状态下核糖体的结构
Science. 2009 Aug 21;325(5943):1014-7. doi: 10.1126/science.1175275.
10
Architecture and secondary structure of an entire HIV-1 RNA genome.完整HIV-1 RNA基因组的结构与二级结构
Nature. 2009 Aug 6;460(7256):711-6. doi: 10.1038/nature08237.

使用 hSHAPE 对酵母核糖体进行高通量结构分析。

High throughput structural analysis of yeast ribosomes using hSHAPE.

机构信息

Department of Cell Biology and Molecular Genetics, University of Maryland, College Park, MD, USA.

出版信息

RNA Biol. 2011 May-Jun;8(3):478-87. doi: 10.4161/rna.8.3.14453. Epub 2011 May 1.

DOI:10.4161/rna.8.3.14453
PMID:21508682
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3360075/
Abstract

Global mapping of rRNA structure by traditional methods is prohibitive in terms of time, labor and expense. High throughput selective 2' hydroxyl acylation analyzed by primer extension (hSHAPE) bypasses these problems by using fluorescently labeled primers to perform primer extension reactions, the products of which can be separated by capillary electrophoresis, thus enabling long read lengths in a cost effective manner. The data so generated is analyzed in a quantitative fashion using SHAPEFinder. This approach was used to map the flexibility of nearly the entire sequences of the 3 largest rRNAs from intact, empty yeast ribosomes. Mapping of these data onto near-atomic resolution yeast ribosome structures revealed the binding sites of known trans-acting factors, as well as previously unknown highly flexible regions of yeast rRNA. Refinement of this technology will enable nucleotide-specific mapping of changes in rRNA structure depending on the status of tRNA occupancy, the presence or absence of other trans-acting factors, due to mutations of intrinsic ribosome components or extrinsic factors affecting ribosome biogenesis, or in the presence of translational inhibitors.

摘要

采用传统方法对 rRNA 结构进行全局映射在时间、劳动力和费用方面都是不可行的。通过使用荧光标记的引物进行引物延伸反应,高吞吐量选择性 2' 羟基酰化分析(hSHAPE)可以绕过这些问题,其产物可以通过毛细管电泳进行分离,从而以具有成本效益的方式实现长读长。使用 SHAPEFinder 以定量方式分析生成的数据。该方法用于绘制完整、空酵母核糖体中 3 个最大 rRNA 的几乎整个序列的灵活性。将这些数据映射到接近原子分辨率的酵母核糖体结构上,揭示了已知反式作用因子的结合位点,以及先前未知的酵母 rRNA 高度灵活区域。该技术的改进将能够根据 tRNA 占据状态、其他反式作用因子的存在与否、内在核糖体成分的突变或影响核糖体生物发生的外在因素,以及翻译抑制剂的存在,对 rRNA 结构的变化进行核苷酸特异性映射。