The Ca2+ channel beta3 subunit differentially modulates G-protein sensitivity of alpha1A and alpha1B Ca2+ channels
UMass Chan AffiliationsTreistman Lab
Department of Pharmacology and Molecular Toxicology
Graduate School of Biomedical Sciences, Neuroscience Program
Document TypeJournal Article
KeywordsAcetylcholine; Animals; Calcium Channels; Electric Conductivity; Electric Stimulation; Ethylmaleimide; GTP-Binding Proteins; Gene Expression; Ion Channel Gating; Oocytes; Patch-Clamp Techniques; Plasmids; Receptor, Muscarinic M2; Receptors, Muscarinic; Sulfhydryl Reagents; Virulence Factors, Bordetella; Xenopus
Medicine and Health Sciences
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AbstractWe have shown previously that the Ca2+ channel beta3 subunit is capable of modulating tonic G-protein inhibition of alpha1A and alpha1B Ca2+ channels expressed in oocytes. Here we determine the modulatory effect of the Ca2+ channel beta3 subunit on M2 muscarinic receptor-activated G-protein inhibition and whether the beta3 subunit modulates the G-protein sensitivity of alpha1A and alpha1B currents equivalently. To compare the relative inhibition by muscarinic activation, we have used successive ACh applications to remove the large tonic inhibition of these channels. We show that the resulting rebound potentiation results entirely from the loss of tonic G-protein inhibition; although the currents are temporarily relieved of tonic inhibition, they are still capable of undergoing inhibition through the muscarinic pathway. Using this rebound protocol, we demonstrate that the inhibition of peak current amplitude produced by M2 receptor activation is similar for alpha1A and alpha1B calcium currents. However, the contribution of the voltage-dependent component of inhibition, characterized by reduced inhibition at very depolarized voltage steps and the relief of inhibition by depolarizing prepulses, was slightly greater for the alpha1B current than for the alpha1A current. After co-expression of the beta3 subunit, the sensitivity to M2 receptor-induced G-protein inhibition was reduced for both alpha1A and alpha1B currents; however, the reduction was significantly greater for alpha1A currents. Additionally, the difference in the voltage dependence of inhibition of alpha1A and alpha1B currents was heightened after co-expression of the Ca2+ channel beta3 subunit. Such differential modulation of sensitivity to G-protein modulation may be important for fine tuning release in neurons that contain both of these Ca2+ channels.
J Neurosci. 1998 Feb 1;18(3):878-86.
Permanent Link to this Itemhttp://hdl.handle.net/20.500.14038/32444