Mahaney J E, Autry J M, Jones L R
Department of Biochemistry, West Virginia University School of Medicine, Morgantown, West Virginia 26506-9142, USA.
Biophys J. 2000 Mar;78(3):1306-23. doi: 10.1016/S0006-3495(00)76686-0.
Kinetics studies of the cardiac Ca-ATPase expressed in Sf21 cells (Spodoptera frugiperda insect cells) have been carried out to test the hypotheses that phospholamban inhibits Ca-ATPase cycling by decreasing the rate of the E1.Ca to E1'.Ca transition and/or the rate of phosphoenzyme hydrolysis. Three sample types were studied: Ca-ATPase expressed alone, Ca-ATPase coexpressed with wild-type phospholamban (the natural pentameric inhibitor), and Ca-ATPase coexpressed with the L37A-phospholamban mutant (a more potent monomeric inhibitor, in which Leu(37) is replaced by Ala). Phospholamban coupling to the Ca-ATPase was controlled using a monoclonal antibody against phospholamban. Gel electrophoresis and immunoblotting confirmed an equivalent ratio of Ca-ATPase and phospholamban in each sample (1 mol Ca-ATPase to 1.5 mol phospholamban). Steady-state ATPase activity assays at 37 degrees C, using 5 mM MgATP, showed that the phospholamban-containing samples had nearly equivalent maximum activity ( approximately 0.75 micromol. nmol Ca-ATPase(-1).min(-1) at 15 microM Ca(2+)), but that wild-type phospholamban and L37A-phospholamban increased the Ca-ATPase K(Ca) values by 200 nM and 400 nM, respectively. When steady-state Ca-ATPase phosphoenzyme levels were measured at 0 degrees C, using 1 microM MgATP, the K(Ca) values also shifted by 200 nM and 400 nM, respectively, similar to the results obtained by measuring ATP hydrolysis at 37 degrees C. Measurements of the time course of phosphoenzyme formation at 0 degrees C, using 1 microM MgATP and 268 nM ionized [Ca(2+)], indicated that L37A-phospholamban decreased the steady-state phosphoenzyme level to a greater extent (45%) than did wild-type phospholamban (33%), but neither wild-type nor L37A-phospholamban had any effect on the apparent rate of phosphoenzyme formation relative to that of Ca-ATPase expressed alone. Measurements of inorganic phosphate (P(i)) release concomitant with the phosphoenzyme formation studies showed that L37A-phospholamban decreased the steady-state rate of P(i) release to a greater extent (45%) than did wild-type phospholamban (33%). However, independent measurements of Ca-ATPase dephosphorylation after the addition of 5 mM EGTA to the phosphorylated enzyme showed that neither wild-type phospholamban nor L37A-phospholamban had any effect on the rate of phosphoenzyme decay relative to Ca-ATPase expressed alone. Computer simulation of the kinetics data indicated that phospholamban and L37A-phospholamban decreased twofold and fourfold, respectively, the equilibrium binding of the first Ca(2+) ion to the Ca-ATPase E1 intermediate, rather than inhibiting rate of the E.Ca to E'.Ca transition or the rate of phosphoenzyme decay. Therefore, we conclude that phospholamban inhibits Ca-ATPase cycling by decreasing Ca-ATPase Ca(2+) binding to the E1 intermediate.
对在Sf21细胞(草地贪夜蛾昆虫细胞)中表达的心脏钙-ATP酶进行了动力学研究,以验证磷蛋白通过降低E1.Ca到E1'.Ca转变的速率和/或磷酸化酶水解的速率来抑制钙-ATP酶循环的假说。研究了三种样本类型:单独表达的钙-ATP酶、与野生型磷蛋白(天然五聚体抑制剂)共表达的钙-ATP酶,以及与L37A-磷蛋白突变体(一种更有效的单体抑制剂,其中Leu(37)被Ala取代)共表达的钙-ATP酶。使用抗磷蛋白的单克隆抗体来控制磷蛋白与钙-ATP酶的偶联。凝胶电泳和免疫印迹证实每个样本中钙-ATP酶和磷蛋白的比例相同(1摩尔钙-ATP酶比1.5摩尔磷蛋白)。在37℃下,使用5 mM MgATP进行稳态ATP酶活性测定,结果表明含磷蛋白的样本具有几乎相同的最大活性(在15 μM Ca(2+)时约为0.75微摩尔·纳摩尔钙-ATP酶(-1)·分钟(-1)),但野生型磷蛋白和L37A-磷蛋白分别使钙-ATP酶的K(Ca)值增加了200 nM和400 nM。当在0℃下使用1 μM MgATP测量稳态钙-ATP酶磷酸化酶水平时,K(Ca)值也分别移动了200 nM和400 nM,这与在37℃下测量ATP水解得到的结果相似。在0℃下,使用1 μM MgATP和268 nM游离[Ca(2+)]测量磷酸化酶形成的时间进程,结果表明L37A-磷蛋白比野生型磷蛋白更显著地降低了稳态磷酸化酶水平(45%比33%),但野生型和L37A-磷蛋白相对于单独表达的钙-ATP酶对磷酸化酶形成的表观速率均无影响。与磷酸化酶形成研究同时进行的无机磷酸盐(P(i))释放测量表明,L37A-磷蛋白比野生型磷蛋白更显著地降低了稳态P(i)释放速率(45%比33%)。然而,在向磷酸化酶中添加5 mM EGTA后对钙-ATP酶去磷酸化的独立测量表明,野生型磷蛋白和L37A-磷蛋白相对于单独表达的钙-ATP酶对磷酸化酶衰变速率均无影响。动力学数据的计算机模拟表明,磷蛋白和L37A-磷蛋白分别使第一个Ca(2+)离子与钙-ATP酶E1中间体的平衡结合降低了两倍和四倍,而不是抑制E.Ca到E'.Ca转变的速率或磷酸化酶衰变的速率。因此,我们得出结论,磷蛋白通过降低钙-ATP酶与E1中间体的Ca(2+)结合来抑制钙-ATP酶循环。