Wallick E T, Lindenmayer G E, Lane L K, Allen J C, Pitts B J, Schwartz A
Fed Proc. 1977 Aug;36(9):2214-8.
Na+,K+-ATPase has been purified from lamb kidney and consists of two polypeptide peaks on polyacrylamide gel electrophoresis with an enzyme activity of 1,000 mumole Pi/mg pro per hr. A scheme depicting the interaction of cardiac glycoside with the enzyme and ligand effects on binding has been constructed. Under all ligand conditions, ouabain binding tends to reach the same maximum if sufficient ouabain is present. Initial rates vary with ligand conditions. Using a chase method, the rate of dissociation of the glycoside from the enzyme is not influenced by the ligands present, although with separation of the enzyme-glycoside complex from the binding medium, differences are noted. The effect of ouabain on Na binding demonstrated two classes of sites, KD = 0.2 mM and KD = 18 mM. Denaturation decreased the high affinity sites. There was also a good correlation between ouabain binding and inhibition of Na binding. Clearly, ligands are critical in regulating cardiac glycoside interaction with the enzyme.
钠钾ATP酶已从羊肾中纯化出来,在聚丙烯酰胺凝胶电泳上由两个多肽峰组成,酶活性为每小时每毫克蛋白1000微摩尔无机磷。已经构建了一个描述强心苷与该酶相互作用以及配体对结合影响的示意图。在所有配体条件下,如果存在足够的哇巴因,哇巴因结合往往会达到相同的最大值。初始速率随配体条件而变化。使用追踪法,糖苷从酶上解离的速率不受存在的配体影响,尽管在将酶 - 糖苷复合物与结合介质分离时会注意到差异。哇巴因对钠结合的影响表明存在两类位点,解离常数(KD)分别为0.2毫摩尔和18毫摩尔。变性降低了高亲和力位点。哇巴因结合与钠结合抑制之间也存在良好的相关性。显然,配体在调节强心苷与酶的相互作用中至关重要。