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Molecular dissection of the pseudoknot governing the translational regulation of Escherichia coli ribosomal protein S15.

机译:假性结的分子解剖控制大肠杆菌核糖体蛋白S15的翻译调控。

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摘要

The ribosomal protein S15 controls its own translation by binding to a mRNA region overlapping the ribosome binding site. That region of the mRNA can fold in two mutually exclusive conformations that are in dynamic equilibrium: a structure with two hairpins and a pseudoknot. A mutational analysis provided evidence for the existence and requirement of the pseudoknot for translational control in vivo and S15 recognition in vitro. In this study, we used chemical probing to analyze the structural consequences of mutations and their effect on the stem-loop/pseudoknot equilibrium. Interactions between S15 and the pseudoknot structure were further investigated by footprinting experiments. These data, combined with computer modelling and the previously published data on S15 binding and in vivo control, provide important clues on pseudoknot formation and S15 recognition. An unexpected result is that the relevant control element, here the pseudoknot form, can exist in a variety of topologically equivalent structures recognizable and shapable by S15. S15 sits on the deep groove of the co-axial stack and makes contacts with both stems, shielding the bridging adenine. The only specific sequence determinants are found in the helix common to the pseudoknot and the hairpin structures.
机译:核糖体蛋白S15通过结合与核糖体结合位点重叠的mRNA区域来控制自身的翻译。 mRNA的该区域可以动态平衡的两个互斥构象折叠:具有两个发夹和假结的结构。突变分析为假结的存在和在体内的翻译控制以及在体外的S15识别提供了证据。在这项研究中,我们使用化学探针分析了突变的结构后果及其对茎环/假单胞菌平衡的影响。通过足迹实验进一步研究了S15和假结结构之间的相互作用。这些数据与计算机模型以及先前发布的有关S15结合和体内控制的数据相结合,为假结形成和S15识别提供了重要线索。出乎意料的结果是,相关的控制元素(这里为伪结形式)可以存在于S15可以识别和可变形的各种拓扑等效结构中。 S15位于同轴堆叠的深槽上,并与两个阀杆接触,从而屏蔽了桥接的腺嘌呤。在假结和发夹结构共有的螺旋中发现了唯一的特定序列决定簇。

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