This proposal describes an unique approach for a detailed analysis of the
activation process of the retinal rod cyclic GMP-gated channel. The light
response in retinal photoreceptors causes intracellular levels of cGMP
to drop, thereby closing cGMP-gated channels and generating an electrical
signal to the brain. Structural and kinetic studies indicate that two
different subunits assemble into heteromeric channels, but it is not
known how each binding event contributes to activation. A photoaffinity
cGMP analog will be used to freeze the channel in different states of
activation. Single channel analysis will allow the following questions
to be addressed:
1. What are the details of channel activation? This includes identifying
the states the channel goes through during activation, and how
cooperativity is achieved.
2. How does the P subunit effect activation and at which steps? Results
from homomeric channels (formed from subunits) and heteromeric channels
will be compared with native channels which express a 240 kD 13 subunit.
3. Do different patterns of subunit occupancy by cGMP lead to different
channel behaviors?
A detailed analysis of the steps leading to activation of this channel
will give insight into how it participates in phototransduction. Cyclic
nucleotide-gated channel isoforms have been identified in rods, cones,
olfactory neuroepithelium, heart, sperm, and kidney. Knowledge of the
contribution of different elements to activation might help to understand
the roles these isoforms play in different tissues, and facilitate tissue
specific targeting in therapeutic applications.
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