Abstract

Although considerable primary sequence data have been developed for voltage-dependent sodium channels by this laboratory and others, and a number of detailed models have been proposed for channel tertiary structure, experimental data have been reported that relates directly to the three-dimensional conformation of the channel in the membrane. Given the difficulties encountered in obtaining x-ray crystallographic information for membrane proteins such as the sodium channel, it is likely that high-resolution structural data will still be some years in coming. In the meantime, studies relating structure to function require the best possible analysis of channel three-dimensional structure in order to proceed. Because of the indirect nature of most structural approaches short of crystallography, a number of different techniques will have to be brought to bear. Building on our recent biochemical studies of the skeletal muscle sodium channel, and our cloning of the primary sequence for the rat TTX-sensitive and TTX-resistant isoforms of the sodium channel and their human homologs, we propose here to continue a multidisciplinary approach to muscle sodium channel structure, and to begin an analysis of the relationship between this structure and its function. We will probe the organization of the sodium channel in the membrane with studies that focus on the membrane topography of specific segments of the primary sequence, on the organization of the large extramembrane regions in the channel structure, and on the structure of the compactly folded internal repeat domains. Specifically, we will complete our analysis of the location of sites of post-translational modification in the channel primary sequence. We will extend our detailed analysis of the location and kinetics of protease-sensitive regions in the channel structure to include a topographical analysis of these regions, and an analysis of their response to alterations in membrane potential or toxin binding. We will extend our use of monoclonal antibodies to probe the interaction and location of the extramembranous domains. We will use antibodies to interhelical loops or to foreign epitopes inserted into interhelical loops to begin an analysis of the folding pattern within the repeat domains. Finally, in collaboration with Dr. Richard Horn, we will begin an analysis of structure function relationships in the muscle channel that takes advantage of the characteristic differences in toxin binding, single channel conductance, and kinetics between the muscle TTX-sensitive and TTX-resistant channels. This analysis will take specific advantage of the availability of expressible full-length clones for the two rat skeletal muscle sodium channel isoforms. Chimeras will be constructed between the two clones and the partitioning of characteristic properties investigated. Initial leads will be pursued with site-directed mutagenesis. Special attention will be paid to the S5-S6 interhelical loop regions in light of their potential role in toxin binding, and their markedly different treatment in key models of channel structure.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
2R01NS018013-11
Application #
3398027
Study Section
Physiology Study Section (PHY)
Project Start
1981-12-01
Project End
1995-11-30
Budget Start
1991-12-01
Budget End
1992-11-30
Support Year
11
Fiscal Year
1992
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

Filatov, G N; Nguyen, T P; Kraner, S D et al. (1998) Inactivation and secondary structure in the D4/S4-5 region of the SkM1 sodium channel. J Gen Physiol 111:703-15
Ji, S; George Jr, A L; Horn, R et al. (1996) Paramyotonia congenita mutations reveal different roles for segments S3 and S4 of domain D4 in hSkM1 sodium channel gating. J Gen Physiol 107:183-94
Sun, W; Cohen, S A; Barchi, R L (1995) Localization of epitopes for monoclonal antibodies directed against the adult rat skeletal muscle sodium channel (rSkM1) using polymerase chain reaction, fusion proteins, and western blotting. Anal Biochem 226:188-91
Chahine, M; George Jr, A L; Zhou, M et al. (1994) Sodium channel mutations in paramyotonia congenita uncouple inactivation from activation. Neuron 12:281-94
Yang, N; Ji, S; Zhou, M et al. (1994) Sodium channel mutations in paramyotonia congenita exhibit similar biophysical phenotypes in vitro. Proc Natl Acad Sci U S A 91:12785-9
Ji, S; Sun, W; George Jr, A L et al. (1994) Voltage-dependent regulation of modal gating in the rat SkM1 sodium channel expressed in Xenopus oocytes. J Gen Physiol 104:625-43
Ptacek, L J; Gouw, L; Kwiecinski, H et al. (1993) Sodium channel mutations in paramyotonia congenita and hyperkalemic periodic paralysis. Ann Neurol 33:300-7
Yang, J S; Bennett, P B; Makita, N et al. (1993) Expression of the sodium channel beta 1 subunit in rat skeletal muscle is selectively associated with the tetrodotoxin-sensitive alpha subunit isoform. Neuron 11:915-22
Chen, L Q; Chahine, M; Kallen, R G et al. (1992) Chimeric study of sodium channels from rat skeletal and cardiac muscle. FEBS Lett 309:253-7
Ptacek, L J; George Jr, A L; Barchi, R L et al. (1992) Mutations in an S4 segment of the adult skeletal muscle sodium channel cause paramyotonia congenita. Neuron 8:891-7

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