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Vol. 63, Issue 4, 832-843, April 2003

Modulation of CaV2.2 Calcium Channels: Probed by the Use of
Receptor-G
Tandems
Department of Pharmacology, University College London, London,
United Kingdom (F.B., P.V., A.C.D.); and Molecular Pharmacology Group,
Division of Biochemistry and Molecular Biology, Institute of Biomedical
and Life Sciences, University of Glasgow, Glasgow, United Kingdom
(R.J.W., G.M.)
The stable interaction of a G-protein coupled receptor and a particular
partner G-protein was made possible by creating tandems between the
2A adrenergic receptor (
2A-R) and
pertussis toxin-resistant mutants of different G
subunits of
heterotrimeric G-proteins. Both
2A-R-G
o
and
2A-R-G
i proved able to reconstitute
agonist-induced voltage-dependent inhibition of N-type calcium channels
(CaV2.2) similar to the wild-type
2A-R when
expressed in COS-7 cells. The interaction of Gq with the
Gi/o signaling pathways was studied by expressing either
G
q or a chimeric construct based on G
q containing the last five amino acids of G
z, which is
activated by
2A-R. It was found that G
qz5
activated by the wild-type
2A-R inhibited
CaV2.2 currents in a voltage-independent fashion.
Furthermore, G
qz5 counteracted the voltage-dependent
inhibition resulting from
2A-R-G
o
activation. We subsequently investigated the basis for the behavior of
G
qz5. Our evidence suggests that this occurs as a result
of a downstream effect of activation of G
qz5 because it
was blocked by C-terminal construct of phospholipase C
1. Furthermore it is likely to occur in part via protein kinase C (PKC) activation, because the PKC activator phorbol dibutyrate mimicked the effects of
G
qz5 in
2A-R-G
o-transfected cells. Conversely,
cells expressing both
2A-R-G
o and
G
qz5 exhibited a partial restoration of
voltage-dependent inhibition in the presence of the PKC inhibitor
bisindolylmaleimide I (GF 109203X). The potential sites of
phosphorylation are discussed.
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