Pandhare Jui, Dash Chandravanu, Rao Mala, Deshpande Vasanti
Division of Biochemical Sciences, National Chemical Laboratory, Pune-411 008, India.
J Biol Chem. 2003 Dec 5;278(49):48735-44. doi: 10.1074/jbc.M308976200. Epub 2003 Sep 24.
The kinetics of slow onset inhibition of Proteinase K by a proteinaceous alkaline protease inhibitor (API) from a Streptomyces sp. is presented. The kinetic analysis revealed competitive inhibition of Proteinase K by API with an IC50 value 5.5 +/- 0.5 x 10-5 m. The progress curves were time-dependent, consistent with a two-step slow tight binding inhibition. The first step involved a rapid equilibrium for formation of reversible enzyme-inhibitor complex (EI) with a Ki value 5.2 +/- 0.6 x 10-6 m. The EI complex isomerized to a stable complex (EI*) in the second step because of inhibitor-induced conformational changes, with a rate constant k5 (9.2 +/- 1 x 10-3 s-1). The rate of dissociation of EI* (k6) was slower (4.5 +/- 0.5 x 10-5 s-1) indicating the tight binding nature of the inhibitor. The overall inhibition constant Ki* for two-step inhibition of Proteinase K by API was 2.5 +/- 0.3 x 10-7 m. Time-dependent dissociation of EI* revealed that the complex failed to dissociate after a time point and formed a conformationally altered, irreversible complex EI**. These conformational states of enzyme-inhibitor complexes were characterized by fluorescence spectroscopy. Tryptophanyl fluorescence of Proteinase K was quenched as a function of API concentration without any shift in the emission maximum indicating a subtle conformational change in the enzyme, which is correlated to the isomerization of EI to EI*. Time-dependent shift in the emission maxima of EI* revealed the induction of gross conformational changes, which can be correlated to the irreversible conformationally locked EI** complex. API binds to the active site of the enzyme as demonstrated by the abolished fluorescence of 5-iodoacetamidofluorescein-labeled Proteinase K. The chemoaffinity labeling experiments lead us to hypothesize that the inactivation of Proteinase K is because of the interference in the electronic microenvironment and disruption of the hydrogen-bonding network between the catalytic triad and other residues involved in catalysis.
本文介绍了一种来自链霉菌属的蛋白质碱性蛋白酶抑制剂(API)对蛋白酶K的缓慢起效抑制动力学。动力学分析表明,API对蛋白酶K具有竞争性抑制作用,IC50值为5.5±0.5×10-5 m。进程曲线与时间相关,符合两步缓慢紧密结合抑制。第一步涉及形成可逆酶-抑制剂复合物(EI)的快速平衡,Ki值为5.2±0.6×10-6 m。由于抑制剂诱导的构象变化,EI复合物在第二步异构化为稳定复合物(EI*),速率常数k5为(9.2±1×10-3 s-1)。EI的解离速率(k6)较慢(4.5±0.5×10-5 s-1),表明抑制剂具有紧密结合的性质。API对蛋白酶K两步抑制的总体抑制常数Ki为2.5±0.3×10-7 m。EI的时间依赖性解离表明,复合物在某个时间点后未能解离,并形成了构象改变的不可逆复合物EI。酶-抑制剂复合物的这些构象状态通过荧光光谱进行了表征。蛋白酶K的色氨酸荧光随着API浓度的增加而猝灭,发射最大值没有任何偏移,表明酶发生了细微的构象变化,这与EI异构化为EI相关。EI*发射最大值的时间依赖性变化揭示了总体构象变化的诱导,这与不可逆的构象锁定EI**复合物相关。如5-碘乙酰氨基荧光素标记的蛋白酶K荧光消失所示,API与酶的活性位点结合。化学亲和标记实验使我们推测,蛋白酶K的失活是由于对电子微环境的干扰以及催化三联体与其他参与催化的残基之间氢键网络的破坏。
Zotero 插件