Johnson Erik C B, Malito Enrico, Shen Yuequan, Pentelute Brad, Rich Dan, Florián Jan, Tang Wei-Jen, Kent Stephen B H
Department of Biochemistry and Molecular Biology, The University of Chicago, IL 60637, USA.
J Mol Biol. 2007 Oct 26;373(3):573-86. doi: 10.1016/j.jmb.2007.07.054. Epub 2007 Aug 2.
The human immunodeficiency virus 1 (HIV-1) protease (PR) is an aspartyl protease essential for HIV-1 viral infectivity. HIV-1 PR has one catalytic site formed by the homodimeric enzyme. We chemically synthesized fully active HIV-1 PR using modern ligation methods. When complexed with the classic substrate-derived inhibitors JG-365 and MVT-101, the synthetic HIV-1 PR formed crystals that diffracted to 1.04- and 1.2-A resolution, respectively. These atomic-resolution structures revealed additional structural details of the HIV-1 PR's interactions with its active site ligands. Heptapeptide inhibitor JG-365, which has a hydroxyethylamine moiety in place of the scissile bond, binds in two equivalent antiparallel orientations within the catalytic groove, whereas the reduced isostere hexapeptide MVT-101 binds in a single orientation. When JG-365 was converted into the natural peptide substrate for molecular dynamic simulations, we found putative catalytically competent reactant states for both lytic water and direct nucleophilic attack mechanisms. Moreover, free energy perturbation calculations indicated that the insertion of catalytic water into the catalytic site is an energetically favorable process.
人类免疫缺陷病毒1型(HIV-1)蛋白酶(PR)是一种对HIV-1病毒感染性至关重要的天冬氨酸蛋白酶。HIV-1 PR具有一个由同二聚体酶形成的催化位点。我们使用现代连接方法化学合成了具有完全活性的HIV-1 PR。当与经典的底物衍生抑制剂JG-365和MVT-101复合时,合成的HIV-1 PR形成了分别衍射至1.04埃和1.2埃分辨率的晶体。这些原子分辨率结构揭示了HIV-1 PR与其活性位点配体相互作用的更多结构细节。七肽抑制剂JG-365在催化凹槽内以两个等效的反平行方向结合,其具有羟乙胺部分取代了可裂解键,而还原的等排体六肽MVT-101以单一方向结合。当将JG-365转化为天然肽底物用于分子动力学模拟时,我们发现了裂解水和直接亲核攻击机制的假定催化活性反应物状态。此外,自由能扰动计算表明催化水插入催化位点是一个能量有利的过程。
