Dynamic Interaction of S5 and S6 during Voltage-Controlled Gating in a Potassium Channel

doi:10.1085/jgp.118.2.157

Published 1 August 2001. doi:10.1085/jgp.118.2.157

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Original Article

Dynamic Interaction of S5 and S6 during Voltage-Controlled Gating in a Potassium Channel

Felipe Espinosa^a, Richard Fleischhauer^a, Anne McMahon^a, and Rolf H. Joho^a

^a Center for Basic Neuroscience, The University of Texas Southwestern Medical Center, Dallas, TX 75390
Center for Basic Neuroscience, The University of Texas Southwestern Medical Center, Dallas, TX 75390-9111.(214) 648-1801

rolf.joho{at}utsouthwestern.edu

A gain-of-function mutation in the Caenorhabditis elegans exp-2K⁺-channel gene is caused by a cysteine-to-tyrosine change (C480Y)in the sixth transmembrane segment of the channel (Davis, M.W.,R. Fleischhauer, J.A. Dent, R.H. Joho, and L. Avery. 1999. Science.286:2501–2504). In contrast to wild-type EXP-2 channels,homotetrameric C480Y mutant channels are open even at –160mV, explaining the lethality of the homozygous mutant. We modeledthe structure of EXP-2 on the 3-D scaffold of the K⁺ channelKcsA. In the C480Y mutant, tyrosine 480 protrudes from S6 tonear S5, suggesting that the bulky side chain may provide sterichindrance to the rotation of S6 that has been proposed to accompanythe open-closed state transitions (Perozo, E., D.M. Cortes,and L.G. Cuello. 1999. Science. 285:73–78). We testedthe hypothesis that only small side chains at position 480 allowthe channel to close, but that bulky side chains trap the channelin the open state. Mutants with small side chain substitutions(Gly and Ser) behave like wild type; in contrast, bulky sidechain substitutions (Trp, Phe, Leu, Ile, Val, and His) generatechannels that conduct K⁺ ions at potentials as negative as –120mV. The side chain at position 480 in S6 in the pore model isclose to and may interact with a conserved glycine (G421) inS5. Replacement of G421 with bulky side chains also leads tochannels that are trapped in an active state, suggesting thatS5 and S6 interact with each other during voltage-dependentopen-closed state transitions, and that bulky side chains preventthe dynamic changes necessary for permanent channel closing.Single-channel recordings show that mutant channels open frequentlyat negative membrane potentials indicating that they fail toreach long-lasting, i.e., stable, closed states. Our data supporta "two-gate model" with a pore gate responsible for the brief,voltage-independent openings and a separately located, voltage-activatedgate (Liu, Y., and R.H. Joho. 1998. Pflügers Arch. 435:654–661).

Key Words: inward-rectifier • oocyte expression • mutant channels • two-gate hypothesis

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