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Carbon Dioxide Hydration Activity of Carbonic Anhydrase: Kinetics of Alkylated Anhydrases B and C from Humans*

机译:碳酸酐酶的二氧化碳水化活性:人类烷基化酸酐酶B和C的动力学*

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摘要

A stop-flow kinetic study was performed on the carbon dioxide hydration activity of the human carbonic anhydrase B isoenzyme carboxymethylated at its histidine200, and of the human C isoenzyme carboxyketoethylated at its histidine63. The Michaelis-Menten parameters determined between pH 5.6 and 8.7 showed striking differences between the native and the alkylated enzymes, as well as between the modified enzymes themselves. The alkylations caused: (i) a decrease in the kcat values, particularly marked for the carboxymethylated B isoenzyme, (ii) a change in the apparent pK of the kcat curves, and (iii) a dependence of Km on pH, for the alkylated enzymes, in contrast to the pH-independent Km values of the native enzymes. The CO2 hydration and esterase activities of the carboxymethyl B isoenzyme differ markedly in their pH dependence. A kinetic mechanism, which is found to be compatible with all the present observations, is proposed. The results indicate that the modifiable histidine residues do not play an essential role in the catalytic mechanism of the native carbonic anhydrases, but they may well influence the enzyme activity in a secondary role.
机译:对在其组氨酸200处羧甲基化的人碳酸酐酶B同工酶和在其组氨酸63处羧甲基化的人碳同工酶B的二氧化碳水合活性进行了停止流动动力学研究。在pH值5.6和8.7之间确定的Michaelis-Menten参数显示出天然和烷基化酶之间以及修饰的酶本身之间的显着差异。烷基化导致:(i)烷基化的kcat值降低,特别是对于羧甲基化的B同功酶而言是明显的;(ii)kcat曲线的表观pK的变化;以及(iii)Km对pH的依赖性。不同于天然酶的pH依赖性Km值。羧甲基B同工酶的CO2水合和酯酶活性在其pH依赖性方面明显不同。提出了一种动力学机理,发现该动力学机理与所有当前的观察结果都相容。结果表明,可修饰的组氨酸残基在天然碳酸酐酶的催化机理中不发挥重要作用,但它们可能在次要作用中很好地影响酶的活性。

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