Department of Molecular, Cellular, and Developmental Biology, University of California, Santa Barbara, CA 93106, USA.
Proc Natl Acad Sci U S A. 2010 Feb 16;107(7):2884-9. doi: 10.1073/pnas.0912718107. Epub 2010 Feb 1.
CDK5/p35 is a cyclin-dependent kinase essential for normal neuron function. Proteolysis of the p35 subunit in vivo results in CDK5/p25 that causes neurotoxicity associated with a number of neurodegenerative diseases. Whereas the mechanism by which conversion of p35 to p25 leads to toxicity is unknown, there is common belief that CDK5/p25 is catalytically hyperactive compared to CDK5/p35. Here, we have compared the steady-state kinetic parameters of CDK5/p35 and CDK5/p25 towards both histone H1, the best known substrate for both enzymes, and the microtubule-associated protein, tau, a physiological substrate whose in vivo phosphorylation is relevant to Alzheimer's disease. We show that the kinetics of both enzymes are the same towards either substrate in vitro. Furthermore, both enzymes display virtually identical kinetics towards individual phosphorylation sites in tau monitored by NMR. We conclude that conversion of p35 to p25 does not alter the catalytic efficiency of the CDK5 catalytic subunit by using histone H1 or tau as substrates, and that neurotoxicity associated with CDK5/p25 is unlikely attributable to CDK5 hyperactivation, as measured in vitro.
CDK5/p35 是一种细胞周期蛋白依赖性激酶,对正常神经元功能至关重要。体内 p35 亚基的蛋白水解导致 CDK5/p25 的产生,从而引起与许多神经退行性疾病相关的神经毒性。虽然将 p35 转化为 p25 导致毒性的机制尚不清楚,但人们普遍认为 CDK5/p25 的催化活性比 CDK5/p35 更高。在这里,我们比较了 CDK5/p35 和 CDK5/p25 对组蛋白 H1(这两种酶最著名的底物)和微管相关蛋白 tau(一种生理底物,其体内磷酸化与阿尔茨海默病有关)的稳态动力学参数。我们发现,两种酶在体外对任一底物的动力学都是相同的。此外,通过 NMR 监测 tau 中单个磷酸化位点,两种酶均表现出几乎相同的动力学。我们得出结论,p35 转化为 p25 并没有改变 CDK5 催化亚基的催化效率,无论是使用组蛋白 H1 还是 tau 作为底物,并且与 CDK5/p25 相关的神经毒性不太可能归因于 CDK5 的过度激活,如在体外测量的那样。
