人源U2B" 蛋白复合物与U2小核RNA发夹IV在水溶液中的分子动力学模拟
Molecular dynamics simulation of the human U2B" protein complex with U2 snRNA hairpin IV in aqueous solution.
作者信息
Guo J X, Gmeiner W H
机构信息
Eppley Institute, University of Nebraska Medical Center, Omaha, Nebraska, 68198-6805 USA.
出版信息
Biophys J. 2001 Aug;81(2):630-42. doi: 10.1016/s0006-3495(01)75728-1.
A 2200-ps molecular dynamics (MD) simulation of the U2 snRNA hairpin IV/U2B" complex was performed in aqueous solution using the particle mesh Ewald method to consider long-range electrostatic interactions. To investigate the interaction and recognition process between the RNA and protein, the free energy contributions resulting from individual amino acids of the protein component of the RNA/protein complex were calculated using the recently developed glycine-scanning method. The results revealed that the loop region of the U2 snRNA hairpin IV interacted mainly with three regions of the U2B" protein: 1) beta 1-helix A, 2) beta 2-beta 3, and 3) beta 4-helix C. U2 snRNA hairpin IV bound U2B" in a similar orientation as that previously described for U1 snRNA with the U1A' protein; however, the details of the interaction differed in several aspects. In particular, beta 1-helix A and beta 4-helix C in U2B" were not observed to interact with RNA in the U1A' protein complex. Most of the polar and charged residues in the interacting regions had larger mutant free energies than the nonpolar residues, indicating that electrostatic interactions were important for stabilizing the RNA/protein complex. The interaction was further stabilized by a network of hydrogen bonds and salt bridges formed between RNA and protein that was maintained throughout the MD trajectory. In addition to the direct interactions between RNA and the protein, solvent-mediated interactions also contributed significantly to complex stability. A detailed analysis of the ordered water molecules in the hydration of the RNA/protein complex revealed that bridged water molecules reside at the interface of RNA and protein as long as 2100 ps in the 2200-ps trajectory. At least 20 bridged water molecules, on average, contributed to the instantaneous stability of the RNA/protein complex. The stabilizing interaction energy due to bridging water molecules was obtained from ab initio Hartree-Fock and density functional theory calculations.
使用粒子网格埃瓦尔德方法在水溶液中对U2 snRNA发夹IV/U2B”复合物进行了2200皮秒的分子动力学(MD)模拟,以考虑长程静电相互作用。为了研究RNA与蛋白质之间的相互作用和识别过程,使用最近开发的甘氨酸扫描方法计算了RNA/蛋白质复合物蛋白质组分中各个氨基酸产生的自由能贡献。结果表明,U2 snRNA发夹IV的环区主要与U2B”蛋白质的三个区域相互作用:1)β1-螺旋A,2)β2-β3,以及3)β4-螺旋C。U2 snRNA发夹IV与U2B”的结合方向与先前描述的U1 snRNA与U1A'蛋白质的结合方向相似;然而,相互作用的细节在几个方面有所不同。特别是,在U1A'蛋白质复合物中未观察到U2B”中的β1-螺旋A和β4-螺旋C与RNA相互作用。相互作用区域中的大多数极性和带电残基的突变自由能比非极性残基大,表明静电相互作用对于稳定RNA/蛋白质复合物很重要。RNA与蛋白质之间形成的氢键和盐桥网络在整个MD轨迹中得以维持,进一步稳定了这种相互作用。除了RNA与蛋白质之间的直接相互作用外,溶剂介导的相互作用对复合物稳定性也有显著贡献。对RNA/蛋白质复合物水合作用中有序水分子的详细分析表明,在2200皮秒的轨迹中,桥连水分子在RNA与蛋白质的界面处存在长达2100皮秒。平均而言,至少20个桥连水分子有助于RNA/蛋白质复合物的瞬时稳定性。桥连水分子产生的稳定相互作用能是通过从头算哈特里-福克和密度泛函理论计算得到的。
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