Abstract

Specificity of neuronal function at the cellular level is dictated by the exact functional properties of channels and receptors and the precise spatial distribution of these molecules. This specificity is vital to systems-level function. For example, severe loss of motor ability occurs in response to disorganization of Na channel distributions in demyelinating diseases such as multiple sclerosis and as a result of mutated Na channel genes that perturb specific functional properties in hyperkalemic periodic paralysis and related myotonias. Other neuromuscular and central disorders are likely to involve related mechanisms, but the molecular and cell biological dynamics that control function and distribution of channels and receptors are not well understood. This is true even for the Na and K channels responsible for a fundamental function like action potential conduction, especially in light of the fact that both of these """"""""channels"""""""" represent multi-gene families. At least 7 Na channel mRNA species are expressed in skeletal muscle. Four distinct sub- families of K channel genes exist; at least 10 human members of just the Shaker-related subfamily 1 have been reported. Expression of cloned channels in heterologous systems reveal a broad array of functional differences, even between closely related subtypes. How much of this complexity exists in vivo at the level of a single neuron, and to what degree can we understand the complexity of a single cell given available technology? These fundamental questions demand answering. This proposal describes a systematic approach to this end by focusing on the Na and Shaker-like K channels responsible for impulse conduction in a single neuron, the squid giant axon and its cell bodies. Unique features of this system, coupled with the enormous data base on functional properties of squid Na and K channels, will lead to a deep understanding of the processes acting to control neuronal function in a biologically relevant context.
Specific aims will answer: What channel subtypes are expressed and how do their native functional properties compare to those for their cloned counterparts? What is the spatial distribution of each channel isotype? How do post-translational modifications and interactions with other proteins act to control these spatial distributions and functional attributes? Finally, how are these control processes involved in long-term modification of expression patterns for specific channel isotypes that occur during development or in acquisition of new firing patterns? Answers to these questions will significantly advance our understanding of maintenance and modulation of neuronal function in living systems.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS017510-13
Application #
2263215
Study Section
Physiology Study Section (PHY)
Project Start
1981-07-01
Project End
1997-06-30
Budget Start
1994-07-01
Budget End
1995-06-30
Support Year
13
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
Stanford University
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
800771545
City
Stanford
State
CA
Country
United States
Zip Code
94305

  Publications

Sack, Jon T; Aldrich, Richard W; Gilly, William F (2004) A gastropod toxin selectively slows early transitions in the Shaker K channel's activation pathway. J Gen Physiol 123:685-96
Kelley, Wayne P; Wolters, Andrew M; Sack, Jon T et al. (2003) Characterization of a novel gastropod toxin (6-bromo-2-mercaptotryptamine) that inhibits shaker K channel activity. J Biol Chem 278:34934-42
Jerng, Henry H; Gilly, William F (2002) Inactivation and pharmacological properties of sqKv1A homotetramers in Xenopus oocytes cannot account for behavior of the squid ""delayed rectifier"" K(+) conductance. Biophys J 82:3022-36
Marshall, Jennifer; Kelley, Wayne P; Rubakhin, Stanislav S et al. (2002) Anatomical correlates of venom production in Conus californicus. Biol Bull 203:27-41
Brock, M W; Lebaric, Z N; Neumeister, H et al. (2001) Temperature-dependent expression of a squid Kv1 channel in Sf9 cells and functional comparison with the native delayed rectifier. J Membr Biol 180:147-61
Liu, T I; Lebaric, Z N; Rosenthal, J J et al. (2001) Natural substitutions at highly conserved T1-domain residues perturb processing and functional expression of squid Kv1 channels. J Neurophysiol 85:61-71
Brock, M W; Mathes, C; Gilly, W F (2001) Selective open-channel block of Shaker (Kv1) potassium channels by s-nitrosodithiothreitol (SNDTT). J Gen Physiol 118:113-34
Ellis, K C; Tenenholz, T C; Jerng, H et al. (2001) Interaction of a toxin from the scorpion Tityus serrulatus with a cloned K+ channel from squid (sqKv1A). Biochemistry 40:5942-53
Sweedler, J V; Li, L; Floyd, P et al. (2000) Mass spectrometric survey of peptides in cephalopods with an emphasis on the FMRFamide-related peptides. J Exp Biol 203:3565-73
Preuss, T; Gilly, W F (2000) Role of prey-capture experience in the development of the escape response in the squid Loligo opalescens: a physiological correlate in an identified neuron. J Exp Biol 203:559-65

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