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A simple method for the determination of individual rate constants for substrate hydrolysis by serine proteases.

机译:一种简单的测定丝氨酸蛋白酶水解底物速率常数的方法。

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摘要

A simple method is presented for the determination of individual rate constants for substrate hydrolysis by serine proteases and other enzymes with similar catalytic mechanism. The method does not require solvent perturbation like viscosity changes, or solvent isotope effects, that often compromise nonspecifically the activity of substrate and enzyme. The rates of substrate diffusion into the active site (k1), substrate dissociation (k-1), acylation (k2), and deacylation (k3) in the accepted mechanism of substrate hydrolysis by serine proteases are derived from the temperature dependence of the Michaelis-Menten parameters kcat/Km and kcat. The method also yields the activation energies for these molecular events. Application to wild-type and mutant thrombins reveals how the various steps of the catalytic mechanism are affected by Na+-binding and site-directed mutations of the important residues Y225 in the Na+ binding environment and L99 in the S2 specificity site. Extension of this method to other proteases should enable the derivation of detailed information on the kinetic and energetic determinants of protease function.
机译:提出了一种简单的方法,用于测定丝氨酸蛋白酶和其他具有相似催化机理的酶水解底物的各个速率常数。该方法不需要诸如粘度变化或溶剂同位素效应之类的溶剂扰动,这些扰动通常非特异性地损害底物和酶的活性。底物扩散到活性位点(k1),底物解离(k-1),酰化(k2)和脱酰化(k3)的速率是丝氨酸蛋白酶对底物水解的公认机制,这取决于米氏菌的温度依赖性-Menten参数kcat / Km和kcat。该方法还产生了这些分子事件的活化能。对野生型和突变型凝血酶的应用揭示了催化机制的各个步骤如何受到Na +结合和Na +结合环境中重要残基Y225和S2特异性位点L99的定点突变的影响。将该方法扩展到其他蛋白酶应该能够获得有关蛋白酶功能的动力学和能量决定因素的详细信息。

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