Young P R, Briedis A V
Department of Chemistry, University of Illinois, Chicago 60680.
Biochem J. 1989 Jan 15;257(2):541-8. doi: 10.1042/bj2570541.
The major glutathione S-transferase isoenzyme from bovine brain was isolated and purified approx. 500-fold. The enzyme has a pI of 7.39 +/- 0.02 and consists of two non-identical subunits having apparent Mr values of 22,000 and 24,000. The enzyme is uniformly distributed in brain, and kinetic data at pH 6.5 with 1-chloro-2,4-dinitrobenzene (CDNB) as substrate suggest a random rapid-equilibrium mechanism. The kinetics of inhibition by product, by GSH analogues and by NADH are consistent with the suggested mechanism and require inhibitor binding to several different enzyme forms. Long-chain fatty acids are excellent inhibitors of the enzyme, and values of 1nKi for hexanoic acid, octanoic acid, decanoic acid and lauric acid form a linear series when plotted as a function of alkyl chain length. A free-energy change of -1900 J/mol (-455 cal/mol) per CH2 unit is calculated for the contribution of hydrophobic binding energy to the inhibition constants. The turnover number of the purified enzyme dimer is approx. 3400/min. When compared with the second-order rate constant for the reaction between CDNB and GSH, the enzyme is providing a rate acceleration of about 1000-fold. The role of entropic contributions to this small rate acceleration is discussed.
从牛脑中分离并纯化出主要的谷胱甘肽S-转移酶同工酶,纯化倍数约为500倍。该酶的等电点为7.39±0.02,由两个不同的亚基组成,其表观分子量分别为22,000和24,000。该酶在脑中均匀分布,以1-氯-2,4-二硝基苯(CDNB)为底物在pH 6.5下的动力学数据表明其为随机快速平衡机制。产物、谷胱甘肽类似物和NADH的抑制动力学与所提出的机制一致,且需要抑制剂与几种不同的酶形式结合。长链脂肪酸是该酶的优良抑制剂,己酸、辛酸、癸酸和月桂酸的1nKi值作为烷基链长度的函数绘制时形成一个线性系列。计算出每个CH2单元的疏水结合能对抑制常数的贡献的自由能变化为-1900 J/mol(-455 cal/mol)。纯化的酶二聚体的周转数约为3400/分钟。与CDNB和谷胱甘肽之间反应 的二级速率常数相比,该酶提供了约1000倍的速率加速。讨论了熵贡献对这种小速率加速的作用。
