Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors

Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors

Abstract We have examined the regulation of mutually exclusive Cav2.2 exon 37a and b variants by the mouse μ-opioid receptor (mMOR) C-terminal splice variants 1, 1C and 1O in tsA-201 cells. Electrophysiological analyses revealed that both channel isoforms exhibit DAMGO-induced voltage-dependent (Gβγ...

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Main Authors: Maria A. Gandini, Ivana A. Souza, Dvij Raval, Jin Xu, Ying-Xian Pan, Gerald W. Zamponi
Format: Article
Language:English
Published: BMC 2019-11-01
Series:Molecular Brain
Subjects:
N-type
Calcium channel
Cav2.2
Opioid receptor
Splicing
G proteins
Online Access:http://link.springer.com/article/10.1186/s13041-019-0524-6
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spelling doaj-6f54790b247b45bcaf1af0b60c0e4d0b2020-11-25T00:02:53ZengBMCMolecular Brain1756-66062019-11-0112111110.1186/s13041-019-0524-6Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptorsMaria A. Gandini0Ivana A. Souza1Dvij Raval2Jin Xu3Ying-Xian Pan4Gerald W. Zamponi5Department of Physiology and Pharmacology, Alberta Children’s Hospital Research Institute, Hotchkiss Brain Institute, Cumming School of Medicine, University of CalgaryDepartment of Physiology and Pharmacology, Alberta Children’s Hospital Research Institute, Hotchkiss Brain Institute, Cumming School of Medicine, University of CalgaryDepartment of Physiology and Pharmacology, Alberta Children’s Hospital Research Institute, Hotchkiss Brain Institute, Cumming School of Medicine, University of CalgaryDepartment of Neurology and the Molecular Pharmacology Program, Memorial Sloan-Kettering Cancer CenterDepartment of Neurology and the Molecular Pharmacology Program, Memorial Sloan-Kettering Cancer CenterDepartment of Physiology and Pharmacology, Alberta Children’s Hospital Research Institute, Hotchkiss Brain Institute, Cumming School of Medicine, University of CalgaryAbstract We have examined the regulation of mutually exclusive Cav2.2 exon 37a and b variants by the mouse μ-opioid receptor (mMOR) C-terminal splice variants 1, 1C and 1O in tsA-201 cells. Electrophysiological analyses revealed that both channel isoforms exhibit DAMGO-induced voltage-dependent (Gβγ-mediated) inhibition and its recovery by voltage pre-pulses, as well as a voltage-independent component. However, the two channel isoforms differ in their relative extent of voltage-dependent and independent inhibition, with Cav2.2-37b showing significantly more voltage-dependent inhibition upon activation of the three mMOR receptors studied. In addition, coexpression of either mMOR1 or mMOR1C results in an agonist-independent reduction in the peak current density of Cav2.2-37a channels, whereas the peak current density of Cav2.2-37b does not appear to be affected. Interestingly, this decrease is not due to an effect on channel expression at the plasma membrane, as demonstrated by biotinylation experiments. We further examined the mechanism underlying the agonist-independent modulation of Cav2.2-37a by mMOR1C. Incubation of cells with pertussis toxin did not affect the mMOR1C mediated inhibition of Cav2.2-37a currents, indicating a lack of involvement of Gi/o signaling. However, when a Src tyrosine kinase inhibitor was applied, the effect of mMOR1C was lost. Moreover, when we recorded currents using a Cav2.2-37a mutant in which tyrosine 1747 was replaced with phenylalanine (Y1747F), the agonist independent effects of mMOR1C were abolished. Altogether our findings show that Cav2.2-37a and Cav2.2-37b isoforms are subject to differential regulation by C-terminal splice variants of mMORs, and that constitutive mMOR1C activity and downstream tyrosine kinase activity exert a selective inhibition of the Cav2.2-37a splice variant, an N-type channel isoform that is highly enriched in nociceptors. Our study provides new insights into the roles of the MOR full-length C-terminal variants in modulating Cav2.2 channel isoform activities.http://link.springer.com/article/10.1186/s13041-019-0524-6N-typeCalcium channelCav2.2Opioid receptorSplicingG proteins
collection DOAJ
language English
format Article
sources DOAJ
author Maria A. Gandini
Ivana A. Souza
Dvij Raval
Jin Xu
Ying-Xian Pan
Gerald W. Zamponi
spellingShingle Maria A. Gandini
Ivana A. Souza
Dvij Raval
Jin Xu
Ying-Xian Pan
Gerald W. Zamponi
Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
Molecular Brain
N-type
Calcium channel
Cav2.2
Opioid receptor
Splicing
G proteins
author_facet Maria A. Gandini
Ivana A. Souza
Dvij Raval
Jin Xu
Ying-Xian Pan
Gerald W. Zamponi
author_sort Maria A. Gandini
title Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
title_short Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
title_full Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
title_fullStr Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
title_full_unstemmed Differential regulation of Cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
title_sort differential regulation of cav2.2 channel exon 37 variants by alternatively spliced μ-opioid receptors
publisher BMC
series Molecular Brain
issn 1756-6606
publishDate 2019-11-01
description Abstract We have examined the regulation of mutually exclusive Cav2.2 exon 37a and b variants by the mouse μ-opioid receptor (mMOR) C-terminal splice variants 1, 1C and 1O in tsA-201 cells. Electrophysiological analyses revealed that both channel isoforms exhibit DAMGO-induced voltage-dependent (Gβγ-mediated) inhibition and its recovery by voltage pre-pulses, as well as a voltage-independent component. However, the two channel isoforms differ in their relative extent of voltage-dependent and independent inhibition, with Cav2.2-37b showing significantly more voltage-dependent inhibition upon activation of the three mMOR receptors studied. In addition, coexpression of either mMOR1 or mMOR1C results in an agonist-independent reduction in the peak current density of Cav2.2-37a channels, whereas the peak current density of Cav2.2-37b does not appear to be affected. Interestingly, this decrease is not due to an effect on channel expression at the plasma membrane, as demonstrated by biotinylation experiments. We further examined the mechanism underlying the agonist-independent modulation of Cav2.2-37a by mMOR1C. Incubation of cells with pertussis toxin did not affect the mMOR1C mediated inhibition of Cav2.2-37a currents, indicating a lack of involvement of Gi/o signaling. However, when a Src tyrosine kinase inhibitor was applied, the effect of mMOR1C was lost. Moreover, when we recorded currents using a Cav2.2-37a mutant in which tyrosine 1747 was replaced with phenylalanine (Y1747F), the agonist independent effects of mMOR1C were abolished. Altogether our findings show that Cav2.2-37a and Cav2.2-37b isoforms are subject to differential regulation by C-terminal splice variants of mMORs, and that constitutive mMOR1C activity and downstream tyrosine kinase activity exert a selective inhibition of the Cav2.2-37a splice variant, an N-type channel isoform that is highly enriched in nociceptors. Our study provides new insights into the roles of the MOR full-length C-terminal variants in modulating Cav2.2 channel isoform activities.
topic N-type
Calcium channel
Cav2.2
Opioid receptor
Splicing
G proteins
url http://link.springer.com/article/10.1186/s13041-019-0524-6
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