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5'-对氟磺酰苯甲酰腺苷对Ⅱ型钙调蛋白依赖性蛋白激酶ATP结合位点的亲和标记

Affinity labeling of the ATP-binding site of type II calmodulin-dependent protein kinase by 5'-p-fluorosulfonylbenzoyl adenosine.

作者信息

King M M, Shell D J, Kwiatkowski A P

机构信息

Department of Chemistry, Ohio State University, Columbus 43210.

出版信息

Arch Biochem Biophys. 1988 Dec;267(2):467-73. doi: 10.1016/0003-9861(88)90052-5.

DOI:10.1016/0003-9861(88)90052-5
PMID:2850765
Abstract

Modification of the type II calmodulin-dependent protein kinase by 5'-p-fluorosulfonylbenzoyl adenosine (FSBA) resulted in a time-dependent inactivation of the enzyme. The reaction followed pseudo-first-order kinetics and showed a nonlinear dependence on reagent concentration. The rate of inactivation was sensitive to Mg2+- and calmodulin-induced conformational changes on the enzyme. However, the enhancing effects of these ligands were not additive; indeed, the kinetic parameters of the Mg2+-stimulated inactivation reaction with FSBA (Kinact = 2.4 mM; kappa max = 0.12 min-1) were almost unaffected by the simultaneous addition of calmodulin (Kinact = 1.5 mM; kappa max = 0.086 min-1). Protection from inactivation by FSBA was provided by Mg2+-ADP which is consistent with modification of the catalytic site. An analysis of the protective effect of Mg2+-ADP in the absence (Kd = 590 microM) and presence (Kd = 68 microM) of calmodulin demonstrated that binding of the modulator protein to the enzyme increases the affinity of the protein kinase for nucleotides. Modification by FSBA resulted in labeling of both Tyr and Lys residues but only labeling of Lys was decreased by Mg2+-ADP which is consistent with the hypothesis that a conserved Lys residue is important in nucleotide binding to the protein kinase. However, the kinetic results of the inactivation reaction suggest that this Lys is not involved in mediating the calmodulin-promoted increase in the affinity of the enzyme for Mg2+-nucleotide complexes.

摘要

用5'-对氟磺酰苯甲酰腺苷(FSBA)修饰II型钙调蛋白依赖性蛋白激酶会导致该酶随时间失活。该反应遵循假一级动力学,并且对试剂浓度呈非线性依赖。失活速率对Mg2+和钙调蛋白诱导的酶构象变化敏感。然而,这些配体的增强作用并非相加的;实际上,FSBA引发的Mg2+刺激失活反应的动力学参数(Kinact = 2.4 mM;kappa max = 0.12 min-1)几乎不受同时添加钙调蛋白的影响(Kinact = 1.5 mM;kappa max = 0.086 min-1)。Mg2+-ADP可保护酶不被FSBA失活,这与催化位点的修饰一致。对Mg2+-ADP在无钙调蛋白(Kd = 590 microM)和有钙调蛋白(Kd = 68 microM)时的保护作用分析表明,调节蛋白与酶的结合增加了蛋白激酶对核苷酸的亲和力。FSBA修饰导致Tyr和Lys残基均被标记,但只有Lys的标记被Mg2+-ADP降低,这与保守的Lys残基在核苷酸与蛋白激酶结合中起重要作用的假设一致。然而,失活反应的动力学结果表明,该Lys不参与介导钙调蛋白促进酶对Mg2+-核苷酸复合物亲和力的增加。

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