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Calcium Modulation of Ligand Affinity in the Cyclic GMP–gated Ion Channels of Cone Photoreceptors

机译:锥形感光体的循环GMP门控离子通道中的钙配体亲和力的钙调制。

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摘要

To investigate modulation of the activation of cGMP-gated ion channels in cone photoreceptors, we measured currents in membrane patches detached from the outer segments of single cones isolated from striped bass retina. The sensitivity of these channels to activation by cGMP depends on the history of exposure to divalent cations of the membrane's cytoplasmic surface. In patches maintained in 20 μM Ca++ and 100 μM Mg++ after excision, the current amplitude dependence on cGMP is well described by a Hill equation with average values of K 1/2, the concentration necessary to activate half the maximal current, of 86 μM and a cooperativity index, n, of 2.57. Exposing the patch to a solution free of divalent cations irreversibly increases the cGMP sensitivity; the average value of K 1/2 shifts to 58.8 μM and n shifts to 1.8. Changes in cGMP sensitivity do not affect other functional parameters of the ion channels, such as the interaction and permeation of mono- and divalent cations. Modulation of cGMP activation depends on the action of an endogenous factor that progressively dissociates from the channel as Ca++ concentration is lowered below 1 μM. The activity of the endogenous modulator is not well mimicked by exogenously added calmodulin, although this protein competes with the endogenous modulator for a common binding site. Thus, the modulation of cGMP affinity in cones depends on the activity of an unidentified molecule that may not be calmodulin.
机译:为了研究锥体感光器中cGMP门控离子通道激活的调节,我们测量了从斑块状低音视网膜分离出的单个锥体外部部分分离的膜片中的电流。这些通道对cGMP激活的敏感性取决于暴露于膜细胞质表面二价阳离子的历史。在切除后维持在20μMCa ++ 和100μMMg ++ 中的贴片中,当前振幅对cGMP的依赖性可以通过Hill方程很好地描述,其Hill平均值为K 1/2,即激活最大电流一半(86μM)和协同指数n(2.57)所需的浓度。将贴剂暴露于不含二价阳离子的溶液中会不可逆转地提高cGMP敏感性; K 1/2的平均值变为58.8μM,n变为1.8。 cGMP灵敏度的变化不会影响离子通道的其他功能参数,例如一价和二价阳离子的相互作用和渗透。 cGMP激活的调节取决于内源性因子的作用,随着Ca ++ 浓度降低到1μM以下,内源性因子逐渐从通道解离。内源调节剂的活性不能被外源添加的钙调蛋白很好地模仿,尽管该蛋白与内源调节剂竞争一个共同的结合位点。因此,视锥细胞中cGMP亲和力的调节取决于可能不是钙调蛋白的未鉴定分子的活性。

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