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.
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1 November 1986
Article|
November 01 1986
Light-dependent binding of G-protein to outer segment membranes of toad photoreceptors.
N J Mangini
,
D R Pepperberg
,
W Baehr
Online ISSN: 1540-7748
Print ISSN: 0022-1295
J Gen Physiol (1986) 88 (5): 675–694.
Citation
N J Mangini, D R Pepperberg, W Baehr; Light-dependent binding of G-protein to outer segment membranes of toad photoreceptors.. J Gen Physiol 1 November 1986; 88 (5): 675–694. doi: https://doi.org/10.1085/jgp.88.5.675
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