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BIV TAR RNA与Tat肽相互作用的热力学和溶剂化动力学

Thermodynamics and solvation dynamics of BIV TAR RNA-Tat peptide interaction.

作者信息

Goel Teena, Kumar Santosh, Maiti Souvik

机构信息

Proteomics and Structural Biology Unit, Institute of Genomics and Integrative Biology, CSIR, Mall Road, New Delhi 110 007, India.

出版信息

Mol Biosyst. 2013 Jan 27;9(1):88-98. doi: 10.1039/c2mb25357g. Epub 2012 Oct 31.

Abstract

The interaction of the trans-activation responsive (TAR) region of bovine immunodeficiency virus (BIV) RNA with the Tat peptide is known to play important role in viral replication. Despite being thoroughly studied through a structural point of view, the nature of binding between BIV TAR RNA and the BIV Tat peptide requires information related to its thermodynamics and the nature of hydration around the TAR-Tat complex. In this context, we carried out the thermodynamic study of binding of the Tat peptide to the BIV TAR RNA hairpin through different calorimetric and spectroscopic measurements. Fluorescence titration of 2-aminopurine tagged BIV TAR RNA with the Tat peptide gives their binding affinity. The isothermal titration calorimetric experiment reveals the enthalpy of binding between BIV TAR RNA and the Tat peptide to be largely exothermic with the value of -11.7 (SEM 0.2) kcal mol(-1). Solvation dynamics measurements of BIV TAR RNA having 2-AP located at the bulge region have been carried out in the absence and presence of the BIV Tat peptide using the time correlated single photon counting technique. The solvent cage around the Tat binding site of RNA appears to be more rigid in the presence of the Tat peptide as compared to the free RNA. The displacement of solvent and ions on RNA due to peptide binding influences the entropic contributions to the total binding energy.

摘要

已知牛免疫缺陷病毒(BIV)RNA的反式激活应答(TAR)区域与Tat肽的相互作用在病毒复制中起重要作用。尽管从结构角度进行了深入研究,但BIV TAR RNA与BIV Tat肽之间的结合性质需要有关其热力学以及TAR-Tat复合物周围水化性质的信息。在此背景下,我们通过不同的量热和光谱测量对Tat肽与BIV TAR RNA发夹的结合进行了热力学研究。用Tat肽对2-氨基嘌呤标记的BIV TAR RNA进行荧光滴定可得出它们的结合亲和力。等温滴定量热实验表明,BIV TAR RNA与Tat肽之间的结合焓在很大程度上是放热的,值为-11.7(标准误0.2)kcal mol⁻¹。使用时间相关单光子计数技术,在不存在和存在BIV Tat肽的情况下,对位于凸起区域的具有2-AP的BIV TAR RNA进行了溶剂化动力学测量。与游离RNA相比,在存在Tat肽的情况下,RNA上Tat结合位点周围的溶剂笼似乎更刚性。由于肽结合导致RNA上溶剂和离子的置换影响了对总结合能的熵贡献。

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