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Biophys J, May 2001, p. 2167-2175, Vol. 80, No. 5
Department of Physiology, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104 USA
Based on the structure of the KcsA potassium channel, the
Shaker K+ channel is thought to have, near
the middle of the membrane, a cavity that can be occupied by a permeant
or a blocking cation. We have studied the interaction between cations
in the cavity and the activation gate of the channel, using a set of
monovalent cations together with Shaker mutants that
modify the structure of the cavity. Our results show that reducing the
size of the side chain at position 470 makes it possible for the mutant
channel, unlike native Shaker, to close with
tetraethylammonium (TEA+) or the long-chain TEA-derivative
C10+ trapped inside the channel. Neither I470 mutants nor
Shaker can close when N-methyl-glucamine
(NMG+) is in the channel, even though this ion is smaller
than C10+. Apparently, the carbohydrate side chain of
NMG+ prevents gate closing. Gating currents recorded from
Shaker and I470C were measured in the presence of
different intracellular cations to further analyze the interaction of
cations with the gate. Our results suggest that the cavity in
Shaker is so small that even permeant cations like
Rb+ or Cs+ must leave the cavity before the
channel gate can close.
Biophys J, May 2001, p. 2167-2175, Vol. 80, No. 5
© 2001 by the Biophysical Society 0006-3495/01/05/2167/09 $2.00
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