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人肌肉肌酸激酶活性位点中半胱氨酸282的异常低pK(a)值

An unusually low pK(a) for Cys282 in the active site of human muscle creatine kinase.

作者信息

Wang P F, McLeish M J, Kneen M M, Lee G, Kenyon G L

机构信息

College of Pharmacy, University of Michigan, Ann Arbor, Michigan 48109-1065, USA.

出版信息

Biochemistry. 2001 Oct 2;40(39):11698-705. doi: 10.1021/bi011208f.

DOI:10.1021/bi011208f
PMID:11570870
Abstract

All phosphagen kinases contain a conserved cysteine residue which has been shown by crystallographic studies, on both creatine kinase and arginine kinase, to be located in the active site. There are conflicting reports as to whether this cysteine is essential for catalysis. In this study we have used site-directed mutagenesis to replace Cys282 of human muscle creatine kinase with serine and methionine. In addition, we have replaced Cys282, conserved across all creatine kinases, with alanine. No activity was found with the C282M mutant. The C282S mutant showed significant, albeit greatly reduced, activity in both the forward (creatine phosphorylation) and reverse (MgADP phosphorylation) reactions. The K(m) for creatine was increased approximately 10-fold, but the K(m) for phosphocreatine was relatively unaffected. The V and V/K pH-profiles for the wild-type enzyme were similar to those reported for rabbit muscle creatine kinase, the most widely studied creatine kinase isozyme. However, the V/K(creatine) profile for the C282S mutant was missing a pK of 5.4. This suggests that Cys282 exists as the thiolate anion, and is necessary for the optimal binding of creatine. The low pK of Cys282 was also determined spectrophotometrically and found to be 5.6 +/- 0.1. The S284A mutant was found to have reduced catalytic activity, as well as a 15-fold increase in K(m) for creatine. The pK(a) of Cys282 in this mutant was found to be 6.7 +/- 0.1, indicating that H-bonding to Ser284 is an important, but not the sole, factor contributing to the unusually low pK(a) of Cys282.

摘要

所有磷酸原激酶都含有一个保守的半胱氨酸残基,晶体学研究表明,在肌酸激酶和精氨酸激酶中,该残基都位于活性位点。关于这个半胱氨酸对于催化是否必不可少,存在相互矛盾的报道。在本研究中,我们利用定点诱变技术将人肌肉肌酸激酶的Cys282分别替换为丝氨酸和甲硫氨酸。此外,我们还将所有肌酸激酶中保守的Cys282替换为丙氨酸。C282M突变体没有活性。C282S突变体在正向(肌酸磷酸化)和反向(MgADP磷酸化)反应中均表现出显著活性,尽管活性大幅降低。肌酸的K(m)增加了约10倍,但磷酸肌酸的K(m)相对未受影响。野生型酶的V和V/K pH曲线与报道的兔肌肉肌酸激酶(研究最广泛的肌酸激酶同工酶)相似。然而,C282S突变体的V/K(肌酸)曲线缺少一个5.4的pK值。这表明Cys282以硫醇盐阴离子形式存在,是肌酸最佳结合所必需的。通过分光光度法也测定了Cys282的低pK值,发现为5.6±0.1。发现S284A突变体的催化活性降低以及肌酸的K(m)增加了15倍。发现该突变体中Cys282的pK(a)为6.7±0.1,表明与Ser284的氢键作用是导致Cys282异常低pK(a)的一个重要但非唯一因素。

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