Ma Shuhua, Devi-Kesavan Lakshmi S, Gao Jiali
Department of Chemistry and Supercomputing Institute, Digital Technology Center, University of Minnesota, 207 Pleasant Street SE, Minneapolis, MN 55455, USA.
J Am Chem Soc. 2007 Nov 7;129(44):13633-45. doi: 10.1021/ja074222+. Epub 2007 Oct 13.
Molecular dynamics simulations using a combined QM/MM potential have been performed to study the catalytic mechanism of human cathepsin K, a member of the papain family of cysteine proteases. We have determined the two-dimensional free energy surfaces of both acylation and deacylation steps to characterize the reaction mechanism. These free energy profiles show that the acylation step is rate limiting with a barrier height of 19.8 kcal/mol in human cathepsin K and of 29.3 kcal/mol in aqueous solution. The free energy of activation for the deacylation step is 16.7 kcal/mol in cathepsin K and 17.8 kcal/mol in aqueous solution. The reduction of free energy barrier is achieved by stabilization of the oxyanion in the transition state. Interestingly, although the "oxyanion hole" has been formed in the Michaelis complex, the amide units do not donate hydrogen bonds directly to the carbonyl oxygen of the substrate, but they stabilize the thiolate anion nucleophile. Hydrogen-bonding interactions are induced as the substrate amide group approaches the nucleophile, moving more than 2 A and placing the oxyanion in contact with Gln19 and the backbone amide of Cys25. The hydrolysis of peptide substrate shares a common mechanism both for the catalyzed reaction in human cathepsin K and for the uncatalyzed reaction in water. Overall, the nucleophilic attack by Cys25 thiolate and the proton-transfer reaction from His162 to the amide nitrogen are highly coupled, whereas a tetrahedral intermediate is formed along the nucleophilic reaction pathway.
利用结合量子力学/分子力学势的分子动力学模拟研究了半胱氨酸蛋白酶木瓜蛋白酶家族成员人组织蛋白酶K的催化机制。我们确定了酰化和脱酰步骤的二维自由能表面,以表征反应机制。这些自由能分布图表明,酰化步骤是限速步骤,在人组织蛋白酶K中的势垒高度为19.8千卡/摩尔,在水溶液中为29.3千卡/摩尔。脱酰步骤的活化自由能在组织蛋白酶K中为16.7千卡/摩尔,在水溶液中为17.8千卡/摩尔。通过稳定过渡态中的氧阴离子实现了自由能垒的降低。有趣的是,尽管在米氏复合物中已经形成了“氧阴离子洞”,但酰胺单元并不直接向底物的羰基氧提供氢键,而是稳定硫醇盐阴离子亲核试剂。当底物酰胺基团接近亲核试剂时,会诱导氢键相互作用,移动超过2埃,并使氧阴离子与Gln19和Cys25的主链酰胺接触。肽底物的水解对于人组织蛋白酶K中的催化反应和水中的非催化反应具有共同的机制。总体而言,Cys25硫醇盐的亲核攻击和从His162到酰胺氮的质子转移反应高度耦合,而在亲核反应途径中形成了四面体中间体。