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延伸中的核糖体结构:转位前后两个tRNA的排列

Structure of the elongating ribosome: arrangement of the two tRNAs before and after translocation.

作者信息

Nierhaus K H, Wadzack J, Burkhardt N, Jünemann R, Meerwinck W, Willumeit R, Stuhrmann H B

机构信息

MPI für Molekulare Genetik, AG Ribosomen, Ihnestrasse 73, D-14195 Berlin, Germany.

出版信息

Proc Natl Acad Sci U S A. 1998 Feb 3;95(3):945-50. doi: 10.1073/pnas.95.3.945.

Abstract

The ribosome uses tRNAs to translate the genetic information into the amino acid sequence of proteins. The mass ratio of a tRNA to the ribosome is in the order of 1:100; because of this unfavorable value it was not possible until now to determine the location of tRNAs within the ribosome by neutron-scattering techniques. However, the new technique of proton-spin contrast-variation improves the signal-to-noise ratio by more than one order of magnitude, thus enabling the direct determination of protonated tRNAs within a deuterated ribosome for the first time. Here we analyze a pair of ribosomal complexes being either in the pre- or post-translocational states that represent the main states of the elongating ribosome. Both complexes were derived from one preparation. The orientation of both tRNAs within the ribosome and their mutual arrangement are determined by using an electron microscopy model for the Escherichia coli ribosome and the tRNA structure. The mass center of gravity of the (tRNA)2mRNA complex moves within the ribosome by 12 +/- 4 A in the course of translocation as previously reported. The main results of the present analysis are that the mutual arrangement of the two tRNAs does not change on translocation and that the angle between them is, depending on the model used, 110 degrees +/- 10 degrees before and after translocation. The translocational movement of the constant tRNA complex within the ribosome can be described as a displacement toward the head of the 30S subunit combined with a rotational movement by about 18 degrees.

摘要

核糖体利用转运RNA(tRNA)将遗传信息转化为蛋白质的氨基酸序列。tRNA与核糖体的质量比约为1:100;由于这个不利的值,直到现在还无法通过中子散射技术确定tRNA在核糖体中的位置。然而,质子自旋对比度变化新技术将信噪比提高了一个多数量级,从而首次能够直接确定氘代核糖体中质子化的tRNA。在这里,我们分析了一对处于转位前或转位后状态的核糖体复合物,它们代表了延伸核糖体的主要状态。这两种复合物都来自同一份制备物。利用大肠杆菌核糖体的电子显微镜模型和tRNA结构,确定了核糖体中两种tRNA的方向及其相互排列。如先前报道,(tRNA)2mRNA复合物的质心在转位过程中在核糖体内移动了12±4埃。本分析的主要结果是,两种tRNA的相互排列在转位时不会改变,并且根据所使用的模型,它们之间的角度在转位前后分别为110°±10°。核糖体中恒定tRNA复合物的转位运动可以描述为朝着30S亚基头部的位移以及大约18°的旋转运动。

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本文引用的文献

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Three-dimensional reconstruction of the Escherichia coli 30 S ribosomal subunit in ice.
J Mol Biol. 1996 Sep 13;262(1):43-52. doi: 10.1006/jmbi.1996.0497.
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