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The Journal of Neuroscience, April 15, 2001, 21(8):2622-2629
A Common Mechanism Underlies Vertebrate Calcium Signaling and
Drosophila Phototransduction
Irit
Chorna-Ornan1, 3,
Tamar
Joel-Almagor1, 3,
Hagit Cohen
Ben-Ami1, 3,
Shahar
Frechter1, 3,
Boaz
Gillo1, 3,
Zvi
Selinger2, 3,
Donald L.
Gill4, and
Baruch
Minke1, 3
Departments of 1 Physiology and
2 Biological Chemistry, and 3 the Kühne
Minerva Center for Studies of Visual Transduction, The Hebrew
University, Jerusalem 91120, Israel, and 4 Department of
Biochemistry and Molecular Biology, University of Maryland School of
Medicine, Baltimore, Maryland 21201
Drosophila phototransduction is an important model
system for studies of inositol lipid signaling. Light excitation in
Drosophila photoreceptors depends on phospholipase C,
because null mutants of this enzyme do not respond to light.
Surprisingly, genetic elimination of the apparently single inositol
trisphosphate receptor (InsP3R) of
Drosophila has no effect on phototransduction. This led
to the proposal that Drosophila photoreceptors do not
use the InsP3 branch of phospholipase C
(PLC)-mediated signaling for phototransduction, unlike most
other inositol lipid-signaling systems. To examine this hypothesis we
applied the membrane-permeant InsP3R antagonist
2-aminoethoxydiphenyl borate (2-APB), which has proved to be an
important probe for assessing InsP3R involvement in various
signaling systems. We first examined the effects of 2-APB on
Xenopus oocytes. We found that 2-APB is efficient at reversibly blocking the robust InsP3-mediated
Ca2+ release and store-operated
Ca2+ entry in Xenopus oocytes at a
stage operating after production of InsP3 but before the
opening of the surface membrane Cl channels by
Ca2+. We next demonstrated that 2-APB is effective
at reversibly blocking the response to light of
Drosophila photoreceptors in a light-dependent manner at
a concentration range similar to that effective in
Xenopus oocytes and other cells. We show furthermore
that 2-APB does not directly block the light-sensitive channels,
indicating that it operates upstream in the activation of these
channels. The results indicate an important link in the coupling
mechanism of vertebrate store-operated channels and
Drosophila TRP channels, which involves the
InsP3 branch of the inositol lipid-signaling pathway.
Key words:
inositol lipid signaling; InsP3 receptor; 2-APB; TRP; Drosophila phototransduction; Xenopus oocytes
Copyright © 2001 Society for Neuroscience 0270-6474/01/2182622-08$05.00/0
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