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通过13C NMR弛豫研究SRE-RNA与VTS1p-SAM结构域结合时的动力学变化。

Changes in dynamics of SRE-RNA on binding to the VTS1p-SAM domain studied by 13C NMR relaxation.

作者信息

Oberstrass Florian C, Allain Frédéric H-T, Ravindranathan Sapna

机构信息

Institute of Molecular Biology and Biophysics, ETH Zurich, CH-8093 Zürich, Switzerland.

出版信息

J Am Chem Soc. 2008 Sep 10;130(36):12007-20. doi: 10.1021/ja8023115. Epub 2008 Aug 13.

DOI:10.1021/ja8023115
PMID:18698768
Abstract

RNA recognition by proteins is often accompanied by significant changes in RNA dynamics in addition to conformational changes. However, there are very few studies which characterize the changes in molecular motions in RNA on protein binding. We present a quantitative (13)C NMR relaxation study of the changes in RNA dynamics in the pico-nanosecond time scale and micro-millisecond time scale resulting from interaction of the stem-loop SRE-RNA with the VTS1p-SAM domain. (13)C relaxation rates of the protonated carbons of the nucleotide base and anomeric carbons have been analyzed by employing the model-free formalism, for a fully (13)C/(15)N-labeled sample of the SRE-RNA in the free and protein-bound forms. In the free RNA, the nature of molecular motions are found to be distinctly different in the stem and the loop region. On binding to the protein, the nature of motions becomes more homogeneous throughout the RNA, with many residues showing increased flexibility at the aromatic carbon sites, while the anomeric carbon sites become more rigid. Surprisingly, we also observe indications of a slow collective motion of the RNA in the binding pocket of the protein. The observation of increased motions on binding is interesting in the context of growing evidence that binding does not always lead to motional restrictions and the resulting entropy gain could favor the free energy of association.

摘要

蛋白质对RNA的识别除了会引起构象变化外,通常还伴随着RNA动力学的显著改变。然而,很少有研究对蛋白质结合时RNA分子运动的变化进行表征。我们对茎环结构的SRE-RNA与VTS1p-SAM结构域相互作用导致的皮秒至纳秒时间尺度以及微秒至毫秒时间尺度下的RNA动力学变化进行了定量的(13)C NMR弛豫研究。对于游离形式和与蛋白质结合形式的完全(13)C/(15)N标记的SRE-RNA样品,已采用无模型形式分析了核苷酸碱基的质子化碳和异头碳的(13)C弛豫率。在游离RNA中,发现茎区和环区的分子运动性质明显不同。与蛋白质结合后,整个RNA分子运动的性质变得更加均匀,许多残基在芳香族碳位点处的灵活性增加,而异头碳位点则变得更加刚性。令人惊讶的是,我们还观察到RNA在蛋白质结合口袋中存在缓慢集体运动的迹象。鉴于越来越多的证据表明结合并不总是导致运动受限,且由此产生的熵增加可能有利于结合自由能,结合时运动增加这一观察结果很有意思。

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