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Role of the closing base pair for d(GCA) hairpin stability: free energy analysis and folding simulations

机译:闭合碱基对对d(GCA)发夹稳定性的作用:自由能分析和折叠模拟

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摘要

Hairpin loops belong to the most important structural motifs in folded nucleic acids. The d(GNA) sequence in DNA can form very stable trinucleotide hairpin loops depending, however, strongly on the closing base pair. Replica-exchange molecular dynamics (REMD) were employed to study hairpin folding of two DNA sequences, d(gcGCAgc) and d(cgGCAcg), with the same central loop motif but different closing base pairs starting from single-stranded structures. In both cases, conformations of the most populated conformational cluster at the lowest temperature showed close agreement with available experimental structures. For the loop sequence with the less stable G:C closing base pair, an alternative loop topology accumulated as second most populated conformational state indicating a possible loop structural heterogeneity. Comparative-free energy simulations on induced loop unfolding indicated higher stability of the loop with a C:G closing base pair by ~3 kcal mol−1 (compared to a G:C closing base pair) in very good agreement with experiment. The comparative energetic analysis of sampled unfolded, intermediate and folded conformational states identified electrostatic and packing interactions as the main contributions to the closing base pair dependence of the d(GCA) loop stability.
机译:发夹环属于折叠核酸中最重要的结构基序。 DNA中的d(GNA)序列可以形成非常稳定的三核苷酸发夹环,但是强烈依赖于闭合碱基对。副本交换分子动力学(REMD)用于研究两个DNA序列d(gcGCAgc)和d(cgGCAcg)的发夹折叠,它们具有相同的中心环基序,但从单链结构开始的闭合碱基对不同。在这两种情况下,在最低温度下人口最多的构象簇的构象都与可用的实验结构密切相关。对于具有不太稳定的G:C封闭碱基对的环序列,替代的环拓扑累积为第二填充的构象状态,表明可能的环结构异质性。诱导环展开的自由比较能量模拟表明,在非常高的C:G闭合碱基对条件下,环的稳定性更高,相对于G:C闭合碱基对约为3〜kcal mol -1 。与实验良好的协议。采样的展开,中间和折叠构象状态的比较能量分​​析确定,静电和堆积相互作用是d(GCA)回路稳定性对闭合碱基对的依赖性的主要贡献。

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