Abstract

Two forms of voltage-sensitive sodium channels (NaChs) exist in rat and human striated muscles, SkM1 (skeletal muscle subtype 1) and H1 (heart subtype 1). These NaChs have a common structural motif, four internal highly homologous repeat domains (D) separated by one homologous and two quite divergent interdomain segments. The isotypes differ in their electrophysiological and pharmacological characteristics, notably, in activation and inactivation kinetics, single channel conductance and sensitivity to block by various divalent metal ions or toxins. The expression of the subtypes also differs in their tissue distribution, time of occurrence during development and response to denervation. Our goal is to help understand which of the distinct electrophysiological or structural features of a channel subtype are responsible for a cell choosing to express a given NaCh subtype. First, we will study chimeric channels comprised of domains and interdomain segments obtained from hSkM1, hH1, rSkM1, rH1 (hereafter called rSkM2/rH1). Three of these channels have been shown to be electrophysiologically and pharmacologically distinguishable by our collaborators (mainly Dr. R. Horn) and the one most recently discovered, hSkM1, is currently being characterized. Based on these results, we will extend the studies to higher resolution with clustered (block) and site-specific point mutations. The goal is to define the parts of the channel protein which form the extracellular mouth of the ion permeation pathway by determining toxin and divalent ion binding sites. We will then proceed to analyze by similar mutational strategies: (1) inactivation, (2) the effects of compounds that block open channels from the inside of the cell, and (3) interactions of these blockers with the inactivation gate. Third, we will create and study autologous and heterologous complementary hemichannels (D1-D2 & D3-D4) and partial channels (e.g. D1-D2-D3 & D4). Successful combinations, those which support voltage-dependent Na ion conductance, will facilitate the mutagenesis process and help to delineate interdomain interactions by the characterization of these NaChs electrophysiologically and pharmacologically. Fourth, we will attempt to determine the functions of individual segments of channels by deletional, insertional and hybrid mutagenesis experiments. The creation and analysis of hybrid channels formed from NaCh and KCh elements electrophysiologically and pharmacologically is designed to define interdomain interaction surfaces, the inactivation gate and the ion selectivity region. Such experimental data may help to define the three-dimensional structure of the channel.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Arthritis and Musculoskeletal and Skin Diseases (NIAMS)
Type
Research Project (R01)
Project #
5R01AR041762-02
Application #
3162192
Study Section
Physiology Study Section (PHY)
Project Start
1992-09-01
Project End
1996-08-31
Budget Start
1993-09-01
Budget End
1994-08-31
Support Year
2
Fiscal Year
1993
Total Cost
Indirect Cost

  Institution

Name
University of Pennsylvania
Department
Type
Schools of Medicine
DUNS #
042250712
City
Philadelphia
State
PA
Country
United States
Zip Code
19104

  Publications

Ma, Zhongming; Kong, Jun; Kallen, Roland G (2009) Studies of alpha-helicity and intersegmental interactions in voltage-gated Na+ channels: S2D4. PLoS One 4:e7674
Zhang, H; Kolibal, S; Vanderkooi, J M et al. (2000) A carboxy-terminal alpha-helical segment in the rat skeletal muscle voltage-dependent Na+ channel is responsible for its interaction with the amino-terminus. Biochim Biophys Acta 1467:406-18
O'Reilly, J P; Wang, S Y; Kallen, R G et al. (1999) Comparison of slow inactivation in human heart and rat skeletal muscle Na+ channel chimaeras. J Physiol 515 ( Pt 1):61-73
Chahine, M; Sirois, J; Marcotte, P et al. (1998) Extrapore residues of the S5-S6 loop of domain 2 of the voltage-gated skeletal muscle sodium channel (rSkM1) contribute to the mu-conotoxin GIIIA binding site. Biophys J 75:236-46
Tang, L; Chehab, N; Wieland, S J et al. (1998) Glutamine substitution at alanine1649 in the S4-S5 cytoplasmic loop of domain 4 removes the voltage sensitivity of fast inactivation in the human heart sodium channel. J Gen Physiol 111:639-52
Wolska, B M; Averyhart-Fullard, V; Omachi, A et al. (1997) Changes in thyroid state affect pHi and Nai+ homeostasis in rat ventricular myocytes. J Mol Cell Cardiol 29:2653-63
Frohnwieser, B; Chen, L Q; Schreibmayer, W et al. (1997) Modulation of the human cardiac sodium channel alpha-subunit by cAMP-dependent protein kinase and the responsible sequence domain. J Physiol 498 ( Pt 2):309-18
Chahine, M; Deschenes, I; Trottier, E et al. (1997) Restoration of fast inactivation in an inactivation-defective human heart sodium channel by the cysteine modifying reagent benzyl-MTS: analysis of IFM-ICM mutation. Biochem Biophys Res Commun 233:606-10
Benzinger, G R; Drum, C L; Chen, L Q et al. (1997) Differences in the binding sites of two site-3 sodium channel toxins. Pflugers Arch 434:742-9
Marcotte, P; Chen, L Q; Kallen, R G et al. (1997) Effects of Tityus serrulatus scorpion toxin gamma on voltage-gated Na+ channels. Circ Res 80:363-9

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