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The Journal of Neurophysiology Vol. 83 No. 6 June 2000, pp. 3453-3461
Copyright ©2000 by the American Physiological Society
Departments of Pediatrics and Neuroscience, Case Western Reserve University, Cleveland, Ohio 44106
Aoki, Takuya and
Scott C. Baraban.
Properties of a Calcium-Activated K+ Current on
Interneurons in the Developing Rat Hippocampus. J. Neurophysiol. 83: 3453-3461, 2000. Calcium-activated potassium currents have an essential role in
regulating excitability in a variety of neurons. Although it is well
established that mature CA1 pyramidal neurons possess a
Ca2+-activated K+ conductance
(IK(Ca)) with early and late components,
modulation by various endogenous neurotransmitters, and sensitivity to
K+ channel toxins, the properties of
IK(Ca) on hippocampal interneurons (or
immature CA1 pyramidal neurons) are relatively unknown. To address this
problem, whole-cell voltage-clamp recordings were made from visually
identified interneurons in stratum lacunosum-moleculare (L-M) and CA1
pyramidal cells in hippocampal slices from immature rats (P3-P25). A
biphasic calcium-activated K+ tail current was elicited
following a brief depolarization from the holding potential (
50 mV).
Analysis of the kinetic properties of IK(Ca)
suggests that an early current component differs between these two cell
types. An early IK(Ca) with a large peak
current amplitude (200.8 ± 13.2 pA, mean ± SE), slow time
constant of decay (70.9 ± 3.3 ms), and relatively rapid time to
peak (within 15 ms) was observed on L-M interneurons
(n = 88), whereas an early IK(Ca) with a small peak current amplitude
(112.5 ± 7.3 pA), a fast time constant of decay (39.4 ± 1.6 ms), and a slower time-to-peak (within 26 ms) was observed on CA1
pyramidal neurons (n = 85). Removal of
extracellular calcium or addition of inorganic Ca2+ channel
blockers (cadmium, nickel, or cobalt) was used to demonstrate the
calcium dependence of these currents. Addition of norepinephrine, carbachol, and a variety of channel toxins (apamin, iberiotoxin, verruculogen, paxilline, penitrem A, and charybdotoxin) were used to
further distinguish between IK(Ca) on these
two hippocampal cell types. Verruculogen (100 nM), carbachol (100 µM), apamin (100 nM), TEA (1 mM), and iberiotoxin (50 nM)
significantly reduced early IK(Ca) on CA1
pyramidal neurons; early IK(Ca) on L-M
interneurons was inhibited by apamin and TEA. Combined with previous
work showing that the firing properties of hippocampal interneurons and
pyramidal cells differ, our kinetic and pharmacological data provide
strong support for the hypothesis that different types of
Ca2+-activated K+ current are present on these
two cell types.
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