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核糖体蛋白S8和S15的RNA结合位点结构。

The structure of the RNA binding site of ribosomal proteins S8 and S15.

作者信息

Müller R, Garrett R A, Noller H F

出版信息

J Biol Chem. 1979 May 25;254(10):3873-8.

PMID:108264
Abstract

Proteins S8 and S15 from the 30 S ribosomal subunit of Escherichia coli were bound to 16 S RNA and digested with ribonuclease A. A ribonucleoprotein complex was isolated which contained the two proteins and three noncontiguous RNA subfragments totaling 93 nucleotides, that could be unambiguously located in the 16 S RNA sequence. We present a secondary structural model for the RNA moiety of the binding site complex, in which the two smaller fragments are extensively base-paired, respectively, to the two halves of the large fragment, to form two disconnected duplexes. Each of the two duplexes is interrupted by a small internal loop. This model is supported by (i) minimum energy considerations, (ii) sites of cleavage by ribonuclease A, and (iii) modification by the single strand-specific reagent kethoxal. The effect of protein binding on the topography of the complex is reflected in the kethoxal reactivity of the RNA moiety. In the absence of the proteins, 5 guanines are modified; 4 of these, at positions 663, 732, 733, and 741, are strongly protected from kethoxal when protein S15 is bound.

摘要

来自大肠杆菌30 S核糖体亚基的蛋白质S8和S15与16 S RNA结合,并用核糖核酸酶A消化。分离出一种核糖核蛋白复合物,它包含这两种蛋白质和三个不连续的RNA亚片段,总共93个核苷酸,这些亚片段可以明确地定位在16 S RNA序列中。我们提出了结合位点复合物RNA部分的二级结构模型,其中两个较小的片段分别与大片段的两半广泛碱基配对,形成两个不相连的双链体。两个双链体中的每一个都被一个小的内部环中断。该模型得到以下支持:(i)最小能量考虑,(ii)核糖核酸酶A的切割位点,以及(iii)单链特异性试剂乙二醛的修饰。蛋白质结合对复合物拓扑结构的影响反映在RNA部分的乙二醛反应性上。在没有蛋白质的情况下,5个鸟嘌呤被修饰;当结合蛋白质S15时,其中位于663、732、733和741位的4个鸟嘌呤受到乙二醛的强烈保护。

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