Gul Sheraz, Hussain Syeed, Thomas Mark P, Resmini Marina, Verma Chandra S, Thomas Emrys W, Brocklehurst Keith
Laboratory of Structural and Mechanistic Enzymology, School of Biological and Chemical Sciences, Fogg Building, Queen Mary, University of London, Mile End Road, London E1 4NS, UK.
Biochemistry. 2008 Feb 19;47(7):2025-35. doi: 10.1021/bi702126p. Epub 2008 Jan 29.
Studies on papain (EC 3.4.22.2), the most thoroughly investigated member of the cysteine proteinase superfamily, have contributed substantially to our understanding of the roles of noncovalent interactions in enzyme active center chemistry. Previously, we reported evidence that the long-held view that catalytic competence develops synchronously with formation of the catalytic site (Cys25)-S-/(His159)-Im+H ion pair is incorrect and that conformational rearrangement is necessary for each of the partners to play its role in catalysis. A decrease in the level of mutual solvation of the partners of the noncatalytic "intimate" ion pair should release the nucleophilic character of (Cys25)-S- and allow association of (His159)-Im+H with the leaving group of a substrate to provide its general acid-catalyzed elimination. Hypotheses by which this could be achieved involve electrostatic modulation of the ion pair and perturbation of its hydrophobic shielding from solvent by Trp177. The potential electrostatic modulator closest to the catalytic site is Asp158, the mutation of which to Ala substantially decreases catalytic activity. Here we report an investigation of these hypotheses by a combination of computer modeling and stopped-flow pH-dependent kinetic studies using a new series of cationic aminoalkyl 2-pyridyl disulfide time-dependent inhibitors as reactivity probes. These probes 2-4 (n = 2-4), which exist as equilibrium mixtures of H3N+-[CH2]n-S-S-2-pyridyl+H and H3N+-[CH2]n-S-S-2-pyridyl which predominate in acidic and weakly alkaline media, respectively, were shown by modeling and kinetic analysis to bind with various degrees of effectiveness near Asp158 and in some cases also near Trp177. Kinetic analysis of the reactions of 2-4 and of the reaction of CH3-[CH2]2-S-S-2-pyridyl+H <==>CH3-[CH2]2-S-S-2-pyridyl 1 and normal mode calculations lead to the conclusion that Asp158 is not involved in the generation of nucleophilic character in the ion pair and demonstrates a key role for Trp177.
木瓜蛋白酶(EC 3.4.22.2)是半胱氨酸蛋白酶超家族中研究最为深入的成员,对我们理解非共价相互作用在酶活性中心化学中的作用有重大贡献。此前,我们报道的证据表明,长期以来认为催化活性与催化位点(Cys25)-S-/(His159)-Im+H离子对的形成同步发展的观点是错误的,构象重排对于每个参与催化的伙伴发挥其作用是必要的。非催化性“紧密”离子对的伙伴之间相互溶剂化程度的降低应释放(Cys25)-S-的亲核特性,并使(His159)-Im+H与底物的离去基团结合,以提供其一般酸催化的消除作用。实现这一目标的假设涉及离子对的静电调节以及Trp177对其溶剂疏水屏蔽的扰动。最接近催化位点的潜在静电调节剂是Asp158,将其突变为Ala会显著降低催化活性。在此,我们通过计算机建模和停流pH依赖性动力学研究相结合的方法,使用一系列新的阳离子氨基烷基2-吡啶基二硫化物时间依赖性抑制剂作为反应性探针,对这些假设进行了研究。这些探针2 - 4(n = 2 - 4)分别以H3N+-[CH2]n-S-S-2-吡啶基+H和H3N+-[CH2]n-S-S-2-吡啶基的平衡混合物形式存在,在酸性和弱碱性介质中分别占主导地位,通过建模和动力学分析表明它们在Asp158附近以及某些情况下在Trp177附近以不同程度有效地结合。对2 - 4的反应以及CH3-[CH2]2-S-S-2-吡啶基+H <==>CH3-[CH2]2-S-S-2-吡啶基1的反应进行动力学分析和正常模式计算得出结论,Asp158不参与离子对亲核特性的产生,并证明了Trp177的关键作用。
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