首页> 美国卫生研究院文献>The Journal of General Physiology >Light-dependent binding of G-protein to outer segment membranes of toad photoreceptors published erratum appears in J Gen Physiol 1987 May;89(5):following 837
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Light-dependent binding of G-protein to outer segment membranes of toad photoreceptors published erratum appears in J Gen Physiol 1987 May;89(5):following 837

机译:G蛋白与蟾蜍感光细胞外节膜的光依赖性结合已发表的勘误表载于J Gen Physiol 1987 May; 89(5):following 837

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摘要

Light-dependent changes in the binding of G-protein were analyzed in outer segment disk membranes obtained from photoreceptors of the toad (Bufo marinus) retina. Isolated, intact retinas, incubated in oxygenated Ringer's solution at 23 +/- 1 degree C, were subjected to various conditions of illumination and then incubated in darkness for specified periods. The retinas were then chilled (0-4 degrees C) and the receptor outer segments (ROS) were isolated. Binding of the alpha- and beta-subunits of G-protein to the ROS membranes was analyzed by quantitating G alpha and G beta extracted from the membranes with hypotonic medium lacking GTP vs. hypotonic medium containing GTP (H and HG extracts, respectively). For retinas illuminated and then immediately chilled for analysis, the extent of G binding (relative abundance of G alpha, beta in the HG extract) increased with the extent of bleaching of the visual pigment. Near-maximal binding was observed after bleaches of greater than or equal to 30%. With an increasing period of incubation in darkness after approximately 70% bleaching, the extent of binding declined gradually to low levels characteristic of unbleached retinas. The period required for half-completion of the decline was approximately 10(3) s. A gradual decline in G binding, from a rapidly developing peak value, was also observed with an increasing period of exposure to intense light. Viewed in the context of previous electrophysiological data, our results indicate that sustained bleaching desensitization of the rods does not depend upon a persisting state of "tight binding" (immobilization) of G-protein by bleached visual pigment.
机译:分析了从蟾蜍(Bufo marinus)视网膜的感光器获得的外段盘状膜中G蛋白结合的光依赖性变化。将分离的完整视网膜在23 +/- 1摄氏度的含氧林格氏液中孵育,然后置于各种光照条件下,然后在黑暗中孵育指定的时间。然后将视网膜冷却(0-4摄氏度),并分离受体外部片段(ROS)。通过定量从缺乏GTP的低渗培养基与含有GTP的低渗培养基(分别为H和HG提取物)从膜中提取的Gα和G beta来分析G蛋白的α和β亚基与ROS膜的结合。对于先照射视网膜然后立即冷却以进行分析的视网膜,G结合的程度(HG提取物中Gα,β的相对丰度)随着视觉色素的漂白程度而增加。漂白度大于或等于30%后,观察到近乎最大的结合。在约70%的漂白后,随着在黑暗中孵育时间的增加,结合的程度逐渐降低至未漂白的视网膜所特有的低水平。下降完成一半所需的时间约为10(3)s。随着暴露于强光的时间增加,也观察到了G结合从快速发展的峰值逐渐下降。在先前的电生理数据的上下文中查看,我们的结果表明,棒的持续漂白脱敏不依赖于漂白可视色素对G蛋白的“紧密结合”(固定化)的持久状态。

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