4.6 Article

Cav1.3 and BK Channels for Timing and Regulating Cell Firing

Journal

MOLECULAR NEUROBIOLOGY
Volume 42, Issue 3, Pages 185-198

Publisher

SPRINGER
DOI: 10.1007/s12035-010-8151-3

Keywords

L-type calcium channels; Pacemaking currents; Action potential firing; Neurons; Chromaffin cells

Categories

Funding

  1. Marie Curie Research Training Network CavNET [MRTN-CT-2006-035367]
  2. Italian M.I.U.R. [PRIN 2007SYRBBH_001]
  3. San Paolo Company [2008.2191]

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L-type Ca2+ channels (LTCCs, Ca(v)1) open readily during membrane depolarization and allow Ca2+ to enter the cell. In this way, LTCCs regulate cell excitability and trigger a variety of Ca2+-dependent physiological processes such as: excitation-contraction coupling in muscle cells, gene expression, synaptic plasticity, neuronal differentiation, hormone secretion, and pacemaker activity in heart, neurons, and endocrine cells. Among the two major isoforms of LTCCs expressed in excitable tissues (Ca(v)1.2 and Ca(v)1.3), Ca(v)1.3 appears suitable for supporting a pacemaker current in spontaneously firing cells. It has steep voltage dependence and low threshold of activation and inactivates slowly. Using Ca(v)1.3(-/-) KO mice and membrane current recording techniques such as the dynamic and the action potential clamp, it has been possible to resolve the time course of Ca(v)1.3 pacemaker currents that regulate the spontaneous firing of dopaminergic neurons and adrenal chromaffin cells. In several cell types, Ca(v)1.3 is selectively coupled to BK channels within membrane nanodomains and controls both the firing frequency and the action potential repolarization phase. Here we review the most critical aspects of Ca(v)1.3 channel gating and its coupling to large conductance BK channels recently discovered in spontaneously firing neurons and neuroendocrine cells with the aim of furnishing a converging view of the role that these two channel types play in the regulation of cell excitability.

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