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Department of Pharmacology, Columbia University, New York, New York 10032
Human
ether-à-go-go-related
gene (HERG) encodes
a K channel similar to the rapid delayed rectifier channel current
(IKr) in
cardiac myocytes. Modulation of
IKr by
extracellular acidosis under pathological conditions may impact on
cardiac electrical activity. Therefore, we studied the effects of
extracellular acidification on
IKr function and
the underlying mechanism, using HERG
expressed in Xenopus oocytes as a
model. Acidification [extracellular pH (pHo) 8.5-6.5] accelerated
HERG deactivation (at
80 mV, the time constant
of the major
component of deactivation was 253 ± 17, 158 ± 10, and 65 ± 5 ms at pHo 8.5, 7.5, and 6.5, respectively; n = 7-10 each),
with no effects on other gating kinetics except a modest acceleration
of recovery from inactivation (at
80 mV,
of recovery was 4.7 ± 0.3, 3.8 ± 0.3, and 1.3 ± 0.2 ms at
pHo 8.5, 7.5, and 6.5, respectively; n = 4-7
each). The following were ruled out as the underlying
mechanisms: 1) voltage shift in
channel activation, 2) pore blockade
by protons, 3) protonation of
histidines on the extracellular domain of HERG,
4) acceleration of recovery from
C-type inactivation, and 5)
interaction between an external H+
binding site and the cytoplasmic
NH2-terminal domain (a key
determinant of HERG deactivation rate). Extracellular application of
diethylpyrocarbonate caused an irreversible acceleration of HERG
deactivation and prevented further acceleration by external
acidification. Our data suggest that side chains accessible to the
extracellular solution mediated the effects of elevating extracellular
H+ concentration on channel deactivation.
rapid delayed rectifier channel; C-type inactivation; deactivation; mutagenesis
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