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Understanding the molecular mechanism of umami recognition by T1R1-T1R3 using molecular dynamics simulations

机译:用分子动力学模拟了解T1R1-T1R3对鼠疫识别的分子机制

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摘要

Taste receptor T1R1-T1R3 can be activated by binding to several natural ligands, e.g., L-glutamate and 5'-ribonucleotides etc., thereby stimulating the umami taste. The molecular mechanism of umami recognition at atomic details, however, remains elusive. Here, using homology modeling, molecular docking and molecular dynamics (MD) simulations, we investigate the effects of five natural umami ligands on the structural dynamics of T1R1-T1R3. Our work identifies the key residues that are directly involved in recognizing the binding ligands. In addition, two adjacent binding sites in T1R1 are determined for substrate binding, and depending on the molecular size and chemical properties of the incoming ligand, one or both binding sites can be occupied. More interestingly, the ligand binding can modulate the pocket size, which is likely correlated with the closing and opening motions of T1R1. We then classify these five ligands into two groups according to their different binding effects on T1R1, which likely associate with the distinct umami signals stimulated by various ligands. This work warrants new experimental assays to further validate the theoretical model and provides guidance to design more effective umami ligands.
机译:味道受体T1R1-T1R3可以通过结合几种天然配体,例如L-谷氨酸和5'-核糖核苷酸等来激活,从而刺激肌瘤。然而,原子细节的乌马姆识别的分子机制仍然难以捉摸。这里,使用同源造型,分子对接和分子动力学(MD)模拟,我们研究了五种天然umami配体对T1R1-T1R3结构动力学的影响。我们的作品识别直接参与识别结合配体的关键残留物。另外,T1R1中的两个相邻的结合位点用于底物结合,并且取决于进入配体的分子尺寸和化学性质,可以占据一个或两个结合位点。更有趣的是,配体结合可以调节口袋尺寸,这可能与T1R1的闭合和打开运动相关。然后,根据其对T1R1的不同结合效应,将这五种配体分为两组,这可能与各种配体刺激的不同umami信号相关联。这项工作保证了新的实验测定,以进一步验证理论模型,并为设计更有效的幼虫配体提供指导。

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