Bennett N, Ildefonse M, Crouzy S, Chapron Y, Clerc A
Centre National de la Recherche Scentifique, URA 520, Centre d'Etudes Nucléaires de Grenoble, France.
Proc Natl Acad Sci U S A. 1989 May;86(10):3634-8. doi: 10.1073/pnas.86.10.3634.
The cationic conductances of purified bovine retinal rod membranes were studied by incorporation of vesicles into planar lipid bilayers. When the membranes were stripped of all peripheral proteins [guanine nucleotide-binding protein (G protein) and cGMP phosphodiesterase (3',5'-cyclic-GMP 5'-nucleotidohydrolase), EC 3.1.4.35], sodium and calcium fluxes were almost only observed in the presence of cGMP. Reconstitution experiments in which purified cGMP phosphodiesterase alone or with G protein were reassociated to the vesicles in proportions similar to those found in the native rod provide evidence for a direct interaction between the cGMP-dependent channel protein and the phosphodiesterase. (i) In its inhibited state, phosphodiesterase markedly stimulates the activity of the channels in the presence of cGMP (situation in the dark-adapted rod) but is not capable of activating the channels in the absence of cGMP. (ii) In the absence of cGMP, activation of the phosphodiesterase by G protein with GTP bound (equivalent to photoexcitation) induces the opening of cation channels that have the same conductance for sodium ions as cGMP-activated channels (20-22 pS, with two sublevels of about 7 pS and 13 pS).
通过将囊泡整合到平面脂质双分子层中,对纯化的牛视网膜视杆细胞膜的阳离子电导进行了研究。当膜上所有外周蛋白(鸟嘌呤核苷酸结合蛋白(G蛋白)和cGMP磷酸二酯酶(3',5'-环鸟苷酸5'-核苷酸水解酶,EC 3.1.4.35))被去除后,几乎只有在cGMP存在时才观察到钠和钙通量。将纯化的cGMP磷酸二酯酶单独或与G蛋白以与天然视杆细胞中相似的比例重新结合到囊泡上的重建实验,为cGMP依赖性通道蛋白与磷酸二酯酶之间的直接相互作用提供了证据。(i)在其抑制状态下,磷酸二酯酶在cGMP存在时显著刺激通道活性(暗适应视杆细胞中的情况),但在没有cGMP时不能激活通道。(ii)在没有cGMP的情况下,结合GTP的G蛋白激活磷酸二酯酶(相当于光激发)会诱导阳离子通道开放,这些通道对钠离子的电导与cGMP激活的通道相同(20-22 pS,有两个约7 pS和13 pS的亚水平)。
