Gérard Emilie F, Mokkawes Thirakorn, Johannissen Linus O, Warwicker Jim, Spiess Reynard R, Blanford Christopher F, Hay Sam, Heyes Derren J, de Visser Sam P
Manchester Institute of Biotechnology, The University of Manchester, 131 Princess Street, Manchester M1 7DN, United Kingdom.
Department of Chemical Engineering, The University of Manchester, Oxford Road, Manchester M13 9PL, United Kingdom.
ACS Catal. 2023 Jun 6;13(12):8247-8261. doi: 10.1021/acscatal.3c00761. eCollection 2023 Jun 16.
Vanadium haloperoxidases (VHPOs) are unique enzymes in biology that catalyze a challenging halogen transfer reaction and convert a strong aromatic C-H bond into C-X (X = Cl, Br, I) with the use of a vanadium cofactor and HO. The VHPO catalytic cycle starts with the conversion of hydrogen peroxide and halide (X = Cl, Br, I) into hypohalide on the vanadate cofactor, and the hypohalide subsequently reacts with a substrate. However, it is unclear whether the hypohalide is released from the enzyme or otherwise trapped within the enzyme structure for the halogenation of organic substrates. A substrate-binding pocket has never been identified for the VHPO enzyme, which questions the role of the protein in the overall reaction mechanism. Probing its role in the halogenation of small molecules will enable further engineering of the enzyme and expand its substrate scope and selectivity further for use in biotechnological applications as an environmentally benign alternative to current organic chemistry synthesis. Using a combined experimental and computational approach, we elucidate the role of the vanadium haloperoxidase protein in substrate halogenation. Activity studies show that binding of the substrate to the enzyme is essential for the reaction of the hypohalide with substrate. Stopped-flow measurements demonstrate that the rate-determining step is not dependent on substrate binding but partially on hypohalide formation. Using a combination of molecular mechanics (MM) and molecular dynamics (MD) simulations, the substrate binding area in the protein is identified and even though the selected substrates (methylphenylindole and 2-phenylindole) have limited hydrogen-bonding abilities, they are found to bind relatively strongly and remain stable in a binding tunnel. A subsequent analysis of the MD snapshots characterizes two small tunnels leading from the vanadate active site to the surface that could fit small molecules such as hypohalide, halide, and hydrogen peroxide. Density functional theory studies using electric field effects show that a polarized environment in a specific direction can substantially lower barriers for halogen transfer. A further analysis of the protein structure indeed shows a large dipole orientation in the substrate-binding pocket that could enable halogen transfer through an applied local electric field. These findings highlight the importance of the enzyme in catalyzing substrate halogenation by providing an optimal environment to lower the energy barrier for this challenging aromatic halide insertion reaction.
卤化钒过氧化物酶(VHPOs)是生物学中独特的酶,可催化具有挑战性的卤素转移反应,并利用钒辅因子和过氧化氢将强芳香族C-H键转化为C-X(X = Cl、Br、I)。VHPO催化循环始于过氧化氢和卤化物(X = Cl、Br、I)在钒酸盐辅因子上转化为次卤化物,随后次卤化物与底物反应。然而,尚不清楚次卤化物是从酶中释放出来,还是以其他方式被困在酶结构内用于有机底物的卤化反应。从未确定过VHPO酶的底物结合口袋,这对蛋白质在整个反应机制中的作用提出了质疑。探究其在小分子卤化反应中的作用将有助于对该酶进行进一步改造,并进一步扩大其底物范围和选择性,以便在生物技术应用中作为当前有机化学合成的环境友好替代品使用。通过结合实验和计算方法,我们阐明了钒卤过氧化物酶蛋白在底物卤化中的作用。活性研究表明,底物与酶的结合对于次卤化物与底物的反应至关重要。停流测量表明,速率决定步骤不依赖于底物结合,而是部分依赖于次卤化物的形成。通过结合分子力学(MM)和分子动力学(MD)模拟,确定了蛋白质中的底物结合区域,尽管所选底物(甲基苯基吲哚和2-苯基吲哚)的氢键结合能力有限,但发现它们结合相对较强,并在结合通道中保持稳定。对MD快照的后续分析表明,有两条从小的钒酸盐活性位点通向表面的小通道,可容纳次卤化物、卤化物和过氧化氢等小分子。使用电场效应的密度泛函理论研究表明,特定方向上的极化环境可大幅降低卤素转移的势垒。对蛋白质结构的进一步分析确实表明,底物结合口袋中存在较大的偶极取向,这可通过施加局部电场实现卤素转移。这些发现突出了该酶在催化底物卤化反应中的重要性,即通过提供最佳环境来降低这一具有挑战性的芳香族卤化物插入反应的能垒。
