首页> 美国卫生研究院文献>Protein Science : A Publication of the Protein Society >Molecular dynamics studies of a DNA-binding protein: 1. A comparison of the trp repressor and trp aporepressor aqueous simulations.
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Molecular dynamics studies of a DNA-binding protein: 1. A comparison of the trp repressor and trp aporepressor aqueous simulations.

机译:DNA结合蛋白的分子动力学研究:1. trp阻遏物和trp抑藻剂水模拟的比较。

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摘要

The results of two 30-ps molecular dynamics simulations of the trp repressor and trp aporepressor proteins are presented in this paper. The simulations were obtained using the AMBER molecular mechanical force field and in both simulations a 6-A shell of TIP3P waters surrounded the proteins. The trp repressor protein is a DNA-binding regulatory protein and it utilizes a helix-turn-helix (D helix-turn-E helix) motif to interact with DNA. The trp aporepressor, lacking two molecules of the L-tryptophan corepressor, cannot bind specifically to DNA. Our simulations show that the N- and C-termini and the residues in and near the helix-turn-helix motifs are the most mobile regions of the proteins, in agreement with the X-ray crystallographic studies. Our simulations also find increased mobility of the residues in the turn-D helix-turn regions of the proteins. We find the average distance separating the DNA-binding motifs to be larger in the repressor as compared to the aporepressor. In addition to examining the protein residue fluctuations and deviations with respect to X-ray structures, we have also focused on backbone dihedral angles and corepressor hydrogen-bonding patterns in this paper.
机译:本文介绍了trp阻遏物和trp抑藻蛋白的两个30 ps分子动力学模拟的结果。模拟是使用AMBER分子机械力场获得的,在两种模拟中,TIP3P水的6-A壳都围绕着蛋白质。 trp阻遏蛋白是一种与DNA结合的调节蛋白,它利用螺旋-转-螺旋(D螺旋-转-E螺旋)基序与DNA相互作用。缺少两个L-色氨酸共加压子分子的trp无刺激子不能特异性结合DNA。我们的模拟表明,与X射线晶体学研究一致,N和C末端以及螺旋-转-螺旋基序中及其附近的残基是蛋白质最易移动的区域。我们的模拟还发现,蛋白质的D字螺旋转弯区域中残基的迁移率提高了。我们发现分隔子与DNA结合基序的平均距离比阻抑子要大。除了检查蛋白质残留物相对于X射线结构的波动和偏差外,我们还在本文中着重研究了骨架二面角和共加压子氢键的模式。

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