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Binding mechanisms of TATA box-binding proteins: DNA kinking is stabilized by specific hydrogen bonds.

机译:TATA盒结合蛋白的结合机制:DNA扭结通过特定的氢键稳定。

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摘要

One of the common mechanisms of DNA bending by minor groove-binding proteins is the insertion of protein side chains between basepair steps, exemplified in TBP (TATA box-binding protein)/DNA complexes. At the central basepair step of the TATA box TBP produces a noticeable decrease in twist and an increase in roll, while engaging in hydrogen bonds with the bases and sugars. This suggests a mechanism for the stabilization of DNA kinks that was explored here with ab initio quantum mechanical calculations and molecular dynamics/potential of mean force calculations. The hydrogen bonds are found to contribute the energy necessary to drive the conformational transition at the central basepair step. The Asn, Thr, and Gly residues involved in hydrogen bonding to the DNA bases and sugar oxygens form a relatively rigid motif in TBP. The interaction of this motif with DNA is found to be responsible for inducing the untwisting and rolling of the central basepair step. Notably, direct readout is shown not to be capable of discriminating between AA and AT steps, as the strength of the hydrogen bonds between TBP and the DNA are the same for both sequences. Rather, the calculated free energy cost for an equivalent conformational transition is found to be sequence-dependent, and is calculated to be higher for AA steps than for AT steps.
机译:较小的沟结合蛋白引起的DNA弯曲的常见机制之一是在碱基对步骤之间插入蛋白侧链,例如TBP(TATA盒结合蛋白)/ DNA复合物。在TATA盒的中央碱基对步骤中,TBP产生明显的扭曲减少和侧翻增加,同时与碱基和糖类进行氢键结合。这表明了DNA纽结稳定的机制,这里从头开始进行了量子力学计算和分子动力学/平均力计算潜力。发现氢键在中央碱基对步骤中贡献了驱动构象转变所需的能量。氢键结合到DNA碱基和糖氧上的Asn,Thr和Gly残基在TBP中形成一个相对刚性的基序。发现该基序与DNA的相互作用是引起中央碱基对步骤解旋和旋转的原因。值得注意的是,由于两个序列的TBP和DNA之间的氢键强度相同,因此直接读数显示无法区分AA和AT步骤。而是,对于等效构象转变,所计算的自由能成本被发现是与序列有关的,并且对于AA步骤而言,其计算出的自由能成本要比对于AT步骤而言更高。

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