Ca2+ channel currents and contraction in CaVbeta3-deficient ileum smooth muscle from mouse

Brigitte Held; Volodymyr Tsvilovskyy; Marcel Meissner; Lars Kaestner; Andreas Ludwig; Sven Mossmang; Peter Lipp; Marc Freichel; Veit Flockerzi

doi:10.1016/j.ceca.2007.04.013

Ca2+ channel currents and contraction in CaVbeta3-deficient ileum smooth muscle from mouse

Cell Calcium. 2007 Oct-Nov;42(4-5):477-87. doi: 10.1016/j.ceca.2007.04.013. Epub 2007 Jun 18.

Authors

Brigitte Held¹, Volodymyr Tsvilovskyy, Marcel Meissner, Lars Kaestner, Andreas Ludwig, Sven Mossmang, Peter Lipp, Marc Freichel, Veit Flockerzi

Affiliation

¹ Institut für Experimentelle und Klinische Pharmakologie und Toxikologie, Medizinische Fakultät, Universität des Saarlandes, D-66421 Homburg, Germany. brigitte.held@uks.eu

PMID: 17580090
DOI: 10.1016/j.ceca.2007.04.013

Abstract

Voltage activated L-type Ca(2+) channels are the principal Ca(2+) channels in intestinal smooth muscle cells. They comprise the ion conducting Ca(V)1 pore and the ancillary subunits alpha(2)delta and beta. Of the four Ca(V)beta subunits Ca(V)beta(3) is assumed to be the relevant Ca(V)beta protein in smooth muscle. In protein lysates isolated from mouse ileum longitudinal smooth muscle we could identify the Ca(V)1.2, Ca(V)alpha(2), Ca(V)beta(2) and Ca(V)beta(3) proteins, but not the Ca(V)beta(1) and Ca(V)beta(4) proteins. Protein levels of Ca(V)1.2, Ca(V)alpha(2) and Ca(V)beta(2) are not altered in ileum smooth muscle obtained from Ca(V)beta(3)-deficient mice indicating that there is no compensatory increase of the expression of these channel proteins. Neither the Ca(V)beta(2) nor the other Ca(V)beta proteins appear to substitute for the lacking Ca(V)beta(3). L-type Ca(2+) channel properties including current density, inactivation kinetics as well as Cd(2+)- and dihydropyridine sensitivity were identical in cells of both genotypes suggesting that they do not require the presence of a Ca(V)beta(3) protein. However, a key hallmark of the Ca(V)beta modulation of Ca(2+) current, the hyperpolarisation of channel activation is slightly but significantly reduced by 4 mV. In addition to L-type Ca(2+) currents T-type Ca(2+) currents could be recorded in the murine ileum smooth muscle cells, but T-type currents were not affected by the lack of Ca(V)beta(3). Both proteins, Ca(V)beta(2) and Ca(V)beta(3) are localized near the plasma membrane and the localization of Ca(V)beta(2) is not altered in Ca(V)beta(3) deficient cells. Spontaneous contractions and potassium and carbachol induced contractions are not significantly different between ileum longitudinal smooth muscle strips from mice of both genotypes. In summary the data show that in ileum smooth muscle cells, Ca(V)beta(3) has only subtle effects on L-type Ca(2+) currents, appears not to be required for spontaneous and potassium induced contraction but might have a function beyond being a Ca(2+) channel subunit.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Calcium Channels / analysis
Calcium Channels / genetics
Calcium Channels / physiology*
Calcium Channels, L-Type / analysis
Calcium Channels, L-Type / genetics
Calcium Channels, L-Type / metabolism
Calcium Channels, L-Type / physiology*
Electric Conductivity
Ileum / physiology*
Inositol 1,4,5-Trisphosphate Receptors / metabolism
Mice
Mice, Knockout
Muscle Contraction*
Muscle, Smooth / chemistry
Muscle, Smooth / metabolism
Muscle, Smooth / physiology*
Patch-Clamp Techniques

Substances

Cacnb2 protein, mouse
Cacnb3 protein, mouse
Calcium Channels
Calcium Channels, L-Type
Inositol 1,4,5-Trisphosphate Receptors