K+-induced dilation of a small renal artery: no role for inward rectifier K+ channels

doi:10.1016/S0008-6363(97)00237-X

Cardiovascular Research 1998 37(3):780-790; doi:10.1016/S0008-6363(97)00237-X
© 1998 by European Society of Cardiology

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K⁺-induced dilation of a small renal artery: no role for inward rectifier K⁺ channels

H.M Prior, N Webster, K Quinn, D.J Beech^* and M.S Yates

Department of Pharmacology, University of Leeds, Leeds, LS2 9JT, UK

^* Corresponding author. Tel.: (+44-113) 2334310; Fax: (+44-113) 2334331; E-mail: d.j.beech@leeds.ac.uk

Objective: To investigate the mechanism of K⁺-induced vasodilationin a small artery from the kidney, with a particular emphasison the role of inward rectifier K⁺ channels. Methods: Lumendiameter and isometric tension recordings have been made fromrabbit renal arcuate artery using pressurised- and wire-myographyrespectively. In addition, conventional whole-cell and amphotericin-perforatedpatch whole-cell recordings have been made from single smoothmuscle cells isolated from the vessel. Results: Arcuate arteriesdilated when the extracellular K⁺ concentration was raised to8–10 mM from either zero or a normal physiological levelof about 6 mM. The effect was not endothelium-dependent. Applicationof 0.01–1 mM Ba²⁺ to block inward rectifier K⁺ channelshad no significant effect on K⁺-induced vasodilation in thearcuate artery, but under the same experimental conditions K⁺-induceddilation of the rat posterior cerebral artery was abolishedby Ba²⁺. In the presence of 60 mM extracellular K⁺, inward rectifierK⁺-current was detectable in some single smooth muscle cellsisolated from arcuate arteries but on average the current densitywas low (–1.44 pA pF^–1 at –60 mV). K⁺-inducedvasodilation of the arcuate artery was abolished by 10 µMouabain and the half-effective concentration of K⁺ which inducedvasodilation was 0.9–1.5 mM. Conclusions: The observationssuggest that an increase in the extracellular K⁺ concentration(up to about 10 mM) dilates the rabbit renal arcuate arteryand that the primary mechanism underlying the effect may bestimulation of Na⁺–K⁺ ATPase in the smooth muscle cellmembrane. Inward rectifier K⁺ channels have a low average densityin smooth muscle cells isolated from arcuate arteries and playno significant role in K⁺-induced vasodilation.

KEYWORDS Vasodilation; Arcuate artery; Rabbit; Kidney; K⁺ channel; Na⁺–K⁺ ATPase

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