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天然碳酸酐酶II与Co2+取代的碳酸酐酶II催化CO2水合作用机制的比较。

A comparison of the mechanisms of CO2 hydration by native and Co2+-substituted carbonic anhydrase II.

作者信息

Kogut K A, Rowlett R S

机构信息

Department of Chemistry, Colgate University, Hamilton, New York 13346.

出版信息

J Biol Chem. 1987 Dec 5;262(34):16417-24.

PMID:3119587
Abstract

We have measured the pH dependence of kcat and kcat/Km for CO2 hydration catalyzed by both native Zn2+-and metallo-substituted Co2+-bovine carbonic anhydrase II in the absence of inhibitory ions. For the Zn2+-enzyme, the pKa values controlling kcat and kcat/Km profiles are similar, but for the Co2+-enzyme the values are about 0.6 pH units apart. Computer simulations of a metal-hydroxide mechanism of carbonic anhydrase suggest that the data for both native and Co2+-carbonic anhydrase can be accounted for by the same mechanism of action, if we postulate that the substitution of Co2+ for Zn2+ in the active site causes a separation of about 0.6 pH units in the pKa values of His-64 and the metal-bound water molecule. We have also measured the activation parameters for kcat and kcat/Km for Co2+-substituted carbonic anhydrase II-catalyzed CO2 hydration and have compared these values to those obtained previously for the native Zn2+-enzyme. For kcat and kcat/Km we obtain an enthalpy of activation of 4.4 +/- 0.6 and approximately 0 kcal mol-1, respectively. The corresponding entropies of activation are -18 +/- 2 and -27 +/- 2 cal mol-1 K-1.

摘要

我们测量了天然锌离子和金属取代钴离子的牛碳酸酐酶II在无抑制离子存在时催化二氧化碳水合反应的催化常数(kcat)和催化常数与米氏常数之比(kcat/Km)对pH的依赖性。对于锌离子酶,控制kcat和kcat/Km曲线的pKa值相似,但对于钴离子酶,这些值相差约0.6个pH单位。碳酸酐酶金属氢氧化物机制的计算机模拟表明,如果我们假设活性位点中钴离子取代锌离子会使组氨酸64和金属结合水分子的pKa值相差约0.6个pH单位,那么天然和钴离子碳酸酐酶的数据都可以用相同的作用机制来解释。我们还测量了钴离子取代的碳酸酐酶II催化二氧化碳水合反应的kcat和kcat/Km的活化参数,并将这些值与之前天然锌离子酶获得的值进行了比较。对于kcat和kcat/Km,我们分别得到活化焓为4.4±0.6和约0千卡摩尔-1。相应的活化熵分别为-18±2和-27±2卡摩尔-1开尔文-1。

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