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The Journal of Neurophysiology Vol. 83 No. 1 January 2000, pp. 418-430
Copyright ©2000 by the American Physiological Society
1Department of Ophthalmology, John A. Moran Eye Center, University of Utah Health Sciences Center, Salt Lake City, Utah 84132; 2Department of Cell and Molecular Biology, Tulane University, New Orleans, Louisiana 70118; and 3Bruce Rappaport Faculty of Medicine, Technion and Rappaport Institute, Haifa 31096, Israel
Solessio, Eduardo,
David M. Linn,
Ido Perlman, and
Eric M. Lasater.
Characterization With Barium of Potassium Currents in Turtle
Retinal Müller Cells. J. Neurophysiol. 83: 418-430, 2000. Müller cells are highly permeable to
potassium ions and play a crucial role in maintaining potassium
homeostasis in the vertebrate retina. The potassium current found in
turtle Müller cells consists of two components: an inwardly
rectifying component and a linear, passive component. These currents
are insensitive to broadband potassium channel blockers,
tetraethylammonium (TEA) and 4-aminopyridine (4-AP) and well blocked by
barium. Differential block by the polyamine spermine suggests that
these currents flow through different channels. In this study, we used
barium ions as a probe to investigate the properties of these currents
by whole cell, voltage-clamp recordings from isolated cells.
Current-voltage (I-V) relationships generated from
current responses to short (35 ms) and long (3.5 s) voltage pulses were
fit with the Hill equation. With extracellular barium, the time course
of block and unblock was voltage and concentration dependent and could
be fit with single exponential functions and time constants larger than
100 ms. Blocking effects by extracellular barium on the two types of
currents were indistinguishable. The decrease of the outward current
originates in part due to charge effects. We also found that
intracellular barium was an effective blocker of the potassium
currents. The relative block of the inward rectifier by intracellular
barium suggests the existence of two "apparent" binding sites
available for barium within the channel. Under depolarizing conditions
favoring the block by internal polyamines, the Hill coefficient for
barium binding was 1, indicating a single apparent binding site for
barium within the pore of the passive linear conductance. The
difference in the steepness of the blocking functions suggests that the
potassium currents flow through two different types of channels, an
inward rectifier and a linear passive conductance. Last, we consider
the use of barium as an intracellular K+ channel blocker
for voltage-clamp experiments.
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