Abstract

Ion channel currents are the fundamental units of electrical activity in most organisms. In our nervous system, K+ and Ca2+ channels are critical, and their regulation provides a way to directly control neuronal excitability and release of neurotransmitter (NT) at synapses. The modulations are crucial to basic nervous function and their understanding should contribute to novel modes of medical interventions for a range of disorders involving the brain, nerves and muscles. We focus primarily on the family of KCNQ (Kv7/M-type) K+ channels that underlie several neuronal K+ currents, and also on CaV2.2 (N-type) Ca2+ channels. In particular, we seek to elucidate the molecular mechanisms of Gq/11- mediated pathways that act on these ion channels, and the functional effect of these pathways on release of NT. Both KCNQ and CaV2.2 channels have emerged as being regulated by PIP2, and this project studies the molecular mechanisms of the PIP2-mediated regulation. We use heterologous systems in which the channels, receptors and signaling molecules are expressed in mammalian tissue- culture cells or oocytes, preparations of rodent sympathetic superior cervical ganglion (SCG) neurons, hippocampal neurons grown on astrocyte """"""""micro-islands"""""""" and a co-culture of SCG neurons and mouse cardiomyocytes.
In specific aim #1, we will study the biochemical and molecular interactions between PIP2, calmodulin and their binding domains on KCNQ channels using inside-out macropatches, surface plasmon resonance spectroscopy and isothermal calorimetry. We hypothesize PIP2 and CaM to act on overlapping domains on the channels, providing for allosteric """"""""cross-talk."""""""" In specific aim #2, we will probe the mechanism of receptor-mediated stimulation of phosphatidylinositol 4- and 5-kinases that we hypothesize to underlie the receptor specificity in modulation of M channels. We will also probe the underlying mechanism of receptor-specificity in Ca2+i signaling, focusing on the proteins IRBIT, DAG- kinase, and small GTPases of the Rho family.
In specific aim #3, we investigate the functional role of M-channel regulation in control over NT release, using two innovative approaches. The first is a co- culture in which SCG neurons make adrenergic synapses on spontaneously-beating cardiomyocytes cultured in a dish, using cells taken from wild-type or receptor knock-out mice. The second uses isolated hippocampal neurons which form autapses, allowing the input/output relation between action potential and NT release to be directly determined. The molecules and signaling pathways that we study have broad relevance to human health and disease, as these channels play a dominant role in regulating excitability of neurons, and their regulation likely underlies changes in emotional state, memory and regulation of body organs. Thus, our research should provide the basis for the development of novel modes of therapeutic intervention for a variety of nervous diseases.

Public Health Relevance

K+ and Ca2+ ion channels underlie critical activities in the brain and peripheral nervous system, and their modulation is involved in many diseases, and in many therapeutic interventions. We study regulation of these channels by lipid signaling molecules, and by Ca2+-binding proteins, using primary nerve cells, molecular biology, and biochemical/biophysical techniques allowing study of signaling pathways at the single-cell and molecular levels.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS043394-12
Application #
8462002
Study Section
Biophysics of Neural Systems Study Section (BPNS)
Program Officer
Stewart, Randall R
Project Start
2002-06-01
Project End
2015-05-31
Budget Start
2013-06-01
Budget End
2014-05-31
Support Year
12
Fiscal Year
2013
Total Cost
$426,951
Indirect Cost
$139,448

  Institution

Name
University of Texas Health Science Center San Antonio
Department
Physiology
Type
Schools of Medicine
DUNS #
800772162
City
San Antonio
State
TX
Country
United States
Zip Code
78229

  Publications

Zhang, Jie; Shapiro, Mark S (2016) Mechanisms and dynamics of AKAP79/150-orchestrated multi-protein signalling complexes in brain and peripheral nerve. J Physiol 594:31-7
Zhang, Jie; Carver, Chase M; Choveau, Frank S et al. (2016) Clustering and Functional Coupling of Diverse Ion Channels and Signaling Proteins Revealed by Super-resolution STORM Microscopy in Neurons. Neuron 92:461-478
Bierbower, Sonya M; Choveau, Frank S; Lechleiter, James D et al. (2015) Augmentation of M-type (KCNQ) potassium channels as a novel strategy to reduce stroke-induced brain injury. J Neurosci 35:2101-11
Evseev, Alexey I; Semenov, Iurii; Archer, Crystal R et al. (2013) Functional effects of KCNQ K(+) channels in airway smooth muscle. Front Physiol 4:277
Ferrer, Tania; Aréchiga-Figueroa, Ivan Arael; Shapiro, Mark S et al. (2013) Tamoxifen inhibition of kv7.2/kv7.3 channels. PLoS One 8:e76085
Bierbower, Sonya M; Shapiro, Mark S (2013) Förster resonance energy transfer-based imaging at the cell surface of live cells. Methods Mol Biol 998:209-16
Zhang, Jie; Shapiro, Mark S (2012) Activity-dependent transcriptional regulation of M-Type (Kv7) K(+) channels by AKAP79/150-mediated NFAT actions. Neuron 76:1133-46
Choveau, Frank S; Hernandez, Ciria C; Bierbower, Sonya M et al. (2012) Pore determinants of KCNQ3 K+ current expression. Biophys J 102:2489-98
Choveau, Frank S; Bierbower, Sonya M; Shapiro, Mark S (2012) Pore helix-S6 interactions are critical in governing current amplitudes of KCNQ3 K+ channels. Biophys J 102:2499-509
Choveau, Frank S; Shapiro, Mark S (2012) Regions of KCNQ K(+) channels controlling functional expression. Front Physiol 3:397

Showing the most recent 10 out of 43 publications