Otto-Bruc A, Antonny B, Vuong T M, Chardin P, Chabre M
CNRS, Institut de Pharmacologie Moléculaire et Cellulaire, Valbonne, France.
Biochemistry. 1993 Aug 24;32(33):8636-45. doi: 10.1021/bi00084a035.
In the retinal cyclic GMP phosphodiesterase (PDE), catalysis by the alpha beta-heterodimer is inhibited in the dark by two identical gamma-subunits and stimulated in the light by the GTP-bearing alpha-subunit of the heterotrimeric G-protein transducin (T beta gamma-T alpha GDP). Two T alpha GTP molecules, dissociated from T beta gamma, bind to and displace the PDE gamma subunits from their inhibitory sites on PDE alpha beta. With GTP gamma S in lieu of GTP, this association becomes persistent. Under physiological conditions, the PDE alpha beta (gamma T alpha)2 active complex stays on the membrane. But in low-salt buffers, it becomes soluble and dissociates into a partially active PDE alpha beta catalytic moiety and two PDE gamma-T alpha GTP gamma S complexes. This indicates that T alpha binds preferentially to PDE gamma. We have studied the interaction of recombinant bovine PDE gamma with purified T alpha in solution or with retinal rod outer segments (ROS) containing both T beta gamma-T alpha GDP and PDE alpha beta gamma 2. When added to dark ROS, recombinant PDE gamma did not bind to inactive PDE alpha beta gamma 2 but extracted T alpha GDP from membrane-bound holo-transducin to form a soluble PDE gamma-T alpha GDP complex. PDE gamma also bound to purified T alpha GDP in solution. The kinetics and affinity of the interaction between PDE gamma and T alpha GDP or T alpha GTP gamma S were determined by monitoring changes in the proteins' tryptophan fluorescence. The Kd's for the binding of recombinant PDE gamma to soluble T alpha GTP gamma S and T alpha GDP are < or = 0.1 and 3 nM, respectively. PDE gamma-T alpha GDP falls apart in 3 s. This slow dissociation means that, in situ, T alpha-PDE gamma cannot physically leave the active PDE alpha beta, since after GTP hydrolysis, an isolated T alpha-PDE gamma complex would dissociate too slowly to allow a fast PDE reinhibition by the liberated PDE gamma. When recombinant PDE gamma was added to PDE that had been persistently activated by T alpha GTP gamma S, reinhibition occurred and T alpha GTP gamma S, complexed to the native PDE gamma, was released, indicating that both had hitherto stayed bound to PDE alpha beta. The mutation W70F does not prevent recombinant PDE gamma from inhibiting PDE alpha beta but diminishes its affinity for T alpha GTP and T alpha GDP 100-fold.(ABSTRACT TRUNCATED AT 400 WORDS)
在视网膜环鸟苷酸磷酸二酯酶(PDE)中,αβ异二聚体的催化作用在黑暗中受到两个相同γ亚基的抑制,而在光照下受到异三聚体G蛋白转导素(Tβγ - TαGDP)中携带GTP的α亚基的刺激。从Tβγ解离的两个TαGTP分子结合并取代PDEγ亚基在PDEαβ上的抑制位点。用GTPγS代替GTP时,这种结合会持续存在。在生理条件下,PDEαβ(γTα)2活性复合物保留在膜上。但在低盐缓冲液中,它会变得可溶并解离成部分活性的PDEαβ催化部分和两个PDEγ - TαGTPγS复合物。这表明Tα优先与PDEγ结合。我们研究了重组牛PDEγ与溶液中纯化的Tα或与含有Tβγ - TαGDP和PDEαβγ2的视网膜杆状外段(ROS)的相互作用。当添加到黑暗的ROS中时,重组PDEγ不与无活性的PDEαβγ2结合,但从膜结合的全转导素中提取TαGDP以形成可溶性PDEγ - TαGDP复合物。PDEγ也与溶液中纯化的TαGDP结合。通过监测蛋白质色氨酸荧光的变化来确定PDEγ与TαGDP或TαGTPγS之间相互作用的动力学和亲和力。重组PDEγ与可溶性TαGTPγS和TαGDP结合的解离常数(Kd)分别≤0.1和3 nM。PDEγ - TαGDP在3秒内解离。这种缓慢的解离意味着,在原位,Tα - PDEγ不能从活性PDEαβ上物理离开,因为在GTP水解后,分离的Tα - PDEγ复合物解离得太慢,无法使释放的PDEγ快速重新抑制PDE。当将重组PDEγ添加到已被TαGTPγS持续激活的PDE中时,会发生重新抑制,并且与天然PDEγ复合的TαGTPγS被释放,表明两者此前一直与PDEαβ结合。W70F突变并不阻止重组PDEγ抑制PDEαβ,但会使其对TαGTP和TαGDP的亲和力降低100倍。(摘要截断于400字)
