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Energetic basis for selective recognition of T·G mismatched base pairs in DNA by imidazole-rich polyamides

机译:富含咪唑的聚酰胺选择性识别DNA中T·G错配碱基对的能量基础

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摘要

To complement available structure and binding results and to develop a detailed understanding of the basis for selective molecular recognition of T·G mismatches in DNA by imidazole containing polyamides, a full thermodynamic profile for formation of the T·G–polyamide complex has been determined. The amide-linked heterocycles f-ImImIm and f-PyImIm (where f is formamido group, Im is imidazole and Py is pyrrole) were studied by using biosensor-surface plasmon resonance (SPR) and isothermal titration calorimetry (ITC) with a T·G mismatch containing DNA hairpin duplex and a similar DNA with only Watson–Crick base pairs. Large negative binding enthalpies for all of the polyamide–DNA complexes indicate that the interactions are enthalpically driven. SPR results show slower complex formation and stronger binding of f-ImImIm to the T·G than to the match site. The thermodynamic analysis indicates that the enhanced binding to the T·G site is the result of better entropic contributions. Negative heat capacity changes for the complex are correlated with calculated solvent accessible surface area changes and indicate hydrophobic contributions to complex formation. DNase I footprinting analysis in a long DNA sequence provided supporting evidence that f-ImImIm binds selectively to T·G mismatch sites.
机译:为了补充可用的结构和结合结果,并发展出对含咪唑的聚酰胺对DNA中T·G错配进行选择性分子识别的基础的详细理解,已确定了形成T·G-聚酰胺复合物的完整热力学曲线。使用生物传感器表面等离子体激元共振(SPR)和等温滴定热法(ITC),用T·进行了酰胺连接的杂环f-ImImIm和f-PyImIm(其中f为甲酰胺基,Im为咪唑,Py为吡咯)的研究。 G错配包含DNA发夹双链体和仅带有Watson-Crick碱基对的类似DNA。所有聚酰胺-DNA复合物的大的负结合焓表明相互作用是由焓驱动的。 SPR结果显示,与匹配位点相比,复合物形成较慢,f-ImImIm与T·G的结合更强。热力学分析表明,与T·G位点的结合增强是更好的熵贡献的结果。配合物的负热容变化与计算得出的溶剂可及表面积变化相关,并表明疏水对配合物形成的贡献。 DNase I在长DNA序列中的足迹分析提供了支持性证据,表明f-ImImIm选择性结合到T·G错配位点。

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