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核糖体结构控制并指导信使核糖核酸的进入、移位及退出动态过程。

The ribosome structure controls and directs mRNA entry, translocation and exit dynamics.

作者信息

Kurkcuoglu Ozge, Doruker Pemra, Sen Taner Z, Kloczkowski Andrzej, Jernigan Robert L

机构信息

Department of Chemical Engineering and Polymer Research Center, Bogazici University, 34342 Bebek, Istanbul, Turkey.

出版信息

Phys Biol. 2008 Nov 24;5(4):046005. doi: 10.1088/1478-3975/5/4/046005.

Abstract

The protein-synthesizing ribosome undergoes large motions to effect the translocation of tRNAs and mRNA; here, the domain motions of this system are explored with a coarse-grained elastic network model using normal mode analysis. Crystal structures are used to construct various model systems of the 70S complex with/without tRNA, elongation factor Tu and the ribosomal proteins. Computed motions reveal the well-known ratchet-like rotational motion of the large subunits, as well as the head rotation of the small subunit and the high flexibility of the L1 and L7/L12 stalks, even in the absence of ribosomal proteins. This result indicates that these experimentally observed motions during translocation are inherently controlled by the ribosomal shape and only partially dependent upon GTP hydrolysis. Normal mode analysis further reveals the mobility of A- and P-tRNAs to increase in the absence of the E-tRNA. In addition, the dynamics of the E-tRNA is affected by the absence of the ribosomal protein L1. The mRNA in the entrance tunnel interacts directly with helicase proteins S3 and S4, which constrain the mRNA in a clamp-like fashion, as well as with protein S5, which likely orients the mRNA to ensure correct translation. The ribosomal proteins S7, S11 and S18 may also be involved in assuring translation fidelity by constraining the mRNA at the exit site of the channel. The mRNA also interacts with the 16S 3' end forming the Shine-Dalgarno complex at the initiation step; the 3' end may act as a 'hook' to reel in the mRNA to facilitate its exit.

摘要

蛋白质合成核糖体经历大幅度运动以实现tRNA和mRNA的易位;在此,利用粗粒度弹性网络模型并通过正常模式分析来探究该系统的结构域运动。晶体结构被用于构建含有/不含有tRNA、延伸因子Tu和核糖体蛋白的70S复合物的各种模型系统。计算得到的运动揭示了大亚基众所周知的棘轮样旋转运动,以及小亚基的头部旋转和L1及L7/L12茎的高灵活性,即使在没有核糖体蛋白的情况下也是如此。这一结果表明,这些在易位过程中通过实验观察到的运动本质上是由核糖体形状控制的,并且仅部分依赖于GTP水解。正常模式分析进一步揭示,在没有E-tRNA的情况下,A位和P位tRNA的流动性增加。此外,E-tRNA的动力学受到核糖体蛋白L1缺失的影响。入口通道中的mRNA直接与解旋酶蛋白S3和S4相互作用,它们以钳状方式约束mRNA,还与蛋白S5相互作用,蛋白S5可能使mRNA定向以确保正确翻译。核糖体蛋白S7、S11和S18也可能通过在通道出口位点约束mRNA来确保翻译保真度。mRNA还在起始步骤与16S 3'端相互作用形成Shine-Dalgarno复合物;3'端可能充当“钩子”来卷入mRNA以促进其退出。

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Proc Natl Acad Sci U S A. 2007 Oct 23;104(43):16840-3. doi: 10.1073/pnas.0707850104. Epub 2007 Oct 16.
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The ribosome in focus: new structures bring new insights.聚焦核糖体:新结构带来新见解。
Trends Biochem Sci. 2007 Sep;32(9):434-41. doi: 10.1016/j.tibs.2007.08.002. Epub 2007 Aug 30.
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