Ghomashchi F, Yu B Z, Berg O, Jain M K, Gelb M H
Department of Chemistry, University of Washington, Seattle 98195.
Biochemistry. 1991 Jul 23;30(29):7318-29. doi: 10.1021/bi00243a037.
The binding equilibrium of phospholipase A2 (PLA2) to the substrate interface influences many aspects of the overall kinetics of interfacial catalysis by this enzyme. For example, the interpretation of kinetic data on substrate specificity was difficult when there was a significant kinetic contribution from the interfacial binding step to the steady-state catalytic turnover. This problem was commonly encountered with vesicles of zwitterionic phospholipids, where the binding of PLA2 to the interface was relatively poor. The action of PLA2 on phosphatidylcholine (PC) vesicles containing a small amount of anionic phospholipid, such as phosphatidic acid (PA), was studied. It was shown that the hydrolysis of these mixed lipid vesicles occurs in the scooting mode in which the enzyme remains tightly bound to the interface and only the substrate molecules present on the outer monolayer of the target vesicle became hydrolyzed Thus the phenomenon of scooting mode hydrolysis was not restricted to the action of PLA2 on vesicles of pure anionic phospholipids, but it was also observed with vesicles of zwitterionic lipids as long as a critical amount of anionic compound was present. Under such conditions, the initial rate of hydrolysis of PC in the mixed PC/PA vesicles was enhanced more than 50-fold. Binding studies of PLA2 to vesicles and kinetic studies in the scooting mode demonstrated that the enhancement of PC hydrolysis in the PC/PA covesicles was due to the much higher affinity of the enzyme toward covesicles compared to vesicles of pure PC phospholipids. A novel and technically simple protocol for accurate determination of the substrate specificity of PLA2 at the interface was also developed by using a double-radiolabel approach. Here, the action of PLA2 in the scooting mode was studied on vesicles of the anionic phospholipid 1,2-dimyristoyl-sn-glycero-3-phosphomethanol that contained small amounts of 3H- and 14C-labeled phospholipids. From an analysis of the 3H and 14C radioactivity in the released fatty acid products, the ratio of substrate specificity constants (kcat/KMS) was obtained for any pair of radiolabeled substrates. These studies showed that the PLA2s from pig pancreas and Naja naja naja venom did not discriminate between phosphatidylcholine and phosphatidylethanolamine phospholipids or between phospholipids with saturated versus unsaturated acyl chains and that the pig enzyme had a slight preference for anionic phospholipids (2-3-fold). The described protocol provided an accurate measure of the substrate specificity of PLA2 without complications arising from the differences in binding affinities of the enzyme to vesicles composed of pure phospholipids.
磷脂酶A2(PLA2)与底物界面的结合平衡影响着该酶界面催化整体动力学的许多方面。例如,当界面结合步骤对稳态催化周转有显著的动力学贡献时,就难以解释关于底物特异性的动力学数据。这种问题在两性离子磷脂囊泡中很常见,在这种情况下PLA2与界面的结合相对较差。研究了PLA2对含有少量阴离子磷脂(如磷脂酸,PA)的磷脂酰胆碱(PC)囊泡的作用。结果表明,这些混合脂质囊泡的水解以“滑动模式”发生,即酶保持紧密结合在界面上,只有靶囊泡外单层上存在的底物分子被水解。因此,“滑动模式”水解现象并不局限于PLA2对纯阴离子磷脂囊泡的作用,只要存在临界量的阴离子化合物,在两性离子脂质囊泡中也能观察到。在这种条件下,PC/PA混合囊泡中PC的初始水解速率提高了50多倍。PLA2与囊泡的结合研究以及“滑动模式”下的动力学研究表明,与纯PC磷脂囊泡相比,PC/PA共混囊泡中PC水解的增强是由于该酶对共混囊泡具有更高的亲和力。通过使用双放射性标记方法,还开发了一种新颖且技术简单的方案,用于准确测定界面处PLA2的底物特异性。在此,研究了PLA2在“滑动模式”下对含有少量3H和14C标记磷脂的阴离子磷脂1,2 - 二肉豆蔻酰 - sn - 甘油 - 3 - 磷酸甲醇囊泡的作用。通过分析释放的脂肪酸产物中的3H和14C放射性,可获得任意一对放射性标记底物的底物特异性常数(kcat/KMS)之比。这些研究表明,来自猪胰腺和眼镜蛇毒的PLA2在磷脂酰胆碱和磷脂酰乙醇胺磷脂之间,或在具有饱和与不饱和酰基链的磷脂之间没有区分,并且猪源酶对阴离子磷脂有轻微偏好(2 - 3倍)。所描述的方案提供了对PLA2底物特异性的准确测量,而不会因该酶对由纯磷脂组成的囊泡的结合亲和力差异而产生复杂情况。
