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核糖核酸酶A催化的能量学。1. 胞苷2',3'-环磷酸水解的pH值、离子强度和溶剂同位素依赖性。

Energetics of ribonuclease A catalysis. 1. pH, ionic strength, and solvent isotope dependence of the hydrolysis of cytidine cyclic 2',3'-phosphate.

作者信息

Eftink M R, Biltonen R L

出版信息

Biochemistry. 1983 Oct 25;22(22):5123-34. doi: 10.1021/bi00291a011.

DOI:10.1021/bi00291a011
PMID:6317013
Abstract

The pH, ionic strength, and solvent deuterium isotope dependence of the steady-state kinetics of the ribonuclease A catalyzed hydrolysis of cytidine cyclic 2',3'-phosphate has been investigated by using, primarily, the technique of flow microcalorimetry to monitor the kinetics. The pH dependence of the Michaelis-Menten parameters has been analyzed by assuming the participation of His-12 and -119 of the enzyme and a third ionizing group, postulated to be on the pyrimidine ring of the substrate, to determine the pH-independent rate constant kc, and Michaelis constant Km. The reported pH analysis, together with existing NMR data and chemical modification studies, allows an assignment of the functional roles of His-12 and -119 as being those of general acid and general base catalytic residues, respectively. At high pH, the apparent Km value is found to increase to unity. This drop in affinity between the enzyme and the substrate at high pH indicates that the substrate binds to the enzyme primarily through an electrostatic interaction with the active-site histidine residues, particularly His-12. The apparent absence of an interaction with the riboside portion of the substrate is suggested to be due to the fact that the substrate exists in a syn conformation about its glycosidic bond and thus cannot interact optimally with the enzyme's binding pocket. This will result in a relative destabilization of the enzyme-substrate complex, which can then be relieved upon the formation of the transition state. The ionic strength dependence of ribonuclease activity is shown to be primarily a result of its effect on the pKa of the histidine residues and a concomitant change in the value of Km.

摘要

主要采用流动微量热法监测动力学,研究了核糖核酸酶A催化胞苷2',3'-环磷酸水解的稳态动力学对pH、离子强度和溶剂氘同位素的依赖性。通过假设酶的His-12和-119以及假定位于底物嘧啶环上的第三个电离基团参与反应,分析了米氏参数对pH的依赖性,以确定与pH无关的速率常数kc和米氏常数Km。所报道的pH分析,连同现有的核磁共振数据和化学修饰研究,使得能够分别将His-12和-119的功能作用确定为一般酸催化残基和一般碱催化残基。在高pH下,发现表观Km值增加到1。在高pH下酶与底物之间亲和力的下降表明,底物主要通过与活性位点组氨酸残基,特别是His-12的静电相互作用与酶结合。底物与核苷部分明显缺乏相互作用被认为是由于底物以其糖苷键的顺式构象存在,因此不能与酶的结合口袋最佳地相互作用。这将导致酶-底物复合物相对不稳定,然后在过渡态形成时得以缓解。核糖核酸酶活性对离子强度的依赖性主要表现为其对组氨酸残基pKa的影响以及Km值的相应变化。

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