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Vol. 280, Issue 1, 483-491, 1997
The University Department of Pharmacology, Mansfield Road, Oxford,
OX1 3QT, U.K.
The effects of nicorandil on ionic currents recorded from single smooth
muscle cells of pig proximal urethra were investigated using
patch-clamp techniques. Tension measurement was also performed to study
the effects of nicorandil on the resting tone of pig urethra.
Nicorandil produced a concentration-dependent sustained outward current
that was suppressed by glibenclamide at
50 mV and was carried
selectively by K+. In cell-attached configuration,
nicorandil activated a 43-pS K+ channel that was reversibly
inhibited by 10 µM glibenclamide. This glibenclamide-sensitive 43-pS
K+ channel (KGS) "ran down" after excision
of the membrane patch. In inside-out configuration, the application of
either 1 mM Mg-ATP or 1 mM nucleotide diphosphate reactivated the
KGS. In symmetrical 140 mM K+ conditions, 300 µM nicorandil and 300 µM levcromakalim activated a 2.14-pA
K+ channel that exhibited the same amplitude and similar
channel-opening kinetics. Methylene blue (10-100 µM), a soluble
guanylate cyclase inhibitor, did not inhibit the opening of the
nicorandil-induced KGS. The KGS was not
activated by either sodium nitroprusside (10-100 µM) or 8-bromo
guanosine 3
:5
-cyclic monophosphate (1 mM). Nicorandil caused a
concentration-dependent relaxation of the urethral resting tone but was
less potent than levcromakalim. The relaxation induced by 10 µM
nicorandil was partially inhibited by glibenclamide (1-10 µM) and
also by methylene blue (10-100 µM). These results indicate that two
independent nicorandil-induced relaxation mechanisms may be present
in pig urethra.
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