Regulation of glibenclamide-sensitive K+ current by nucleotide phosphates in isolated rabbit pulmonary myocytes

doi:10.1016/S0008-6363(95)00067-4

Cardiovascular Research 1995 30(3):460-468; doi:10.1016/S0008-6363(95)00067-4
© 1995 by European Society of Cardiology

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Regulation of glibenclamide-sensitive K⁺ current by nucleotide phosphates in isolated rabbit pulmonary myocytes

Lucie H. Clapp^*

Cardiovascular Research, The Rayne Institute, St Thomas's Hospital, Lambeth Palace Road, London SE1 7EH, UK

Objective: Although the existence of ATP-sensitive K⁺ (K_ATP)channels in vascular muscle is widely accepted, there appearsto be little consensus as to what the primary regulator of thesechannels is under physiological or pathophysiological conditions.Recent evidence has suggested that nucleotide diphosphates (NDPs)may play a more important role than ATP. However, since theproperties of vascular K_ATP channels are quite diverse, andthe effects of these nucleotides are poorly understood, theaim of this study was to test the hypothesis that intracellularATP can regulate whole-cell K_ATP current (I_kATP) in the absenceof NDPs. Methods: Single cells were isolated from rabbit mainpulmonary artery by enzymatic treatment with papain. Whole-cellpatch clamp experiments were performed in cells dialysed withdifferent nucleotides. The effect of the K_ATP channel activator,levcromakalim (10 µM), was investigated at a holding potentialof –60 mV. The contribution of I_K,ATP to the holding currentwas defined as the current which was blocked by glibenclamidefollowing washout of levcromakalim. Results: Lowering the intracellularATP concentration ([ATP]_i) from 1 to 0.1 mM, in the presenceor absence of GTP, enhanced the levcromakalim-induced current(I_lev) by ~2.5 fold and increased a glibenclamide-sensitivebackground K⁺ current (I_glib). However, I_glib was larger withGTP and the total glibenclamide-sensitive current (I_lev + I_glib)increased with time. Significant activation of I_glib failedto occur when the pipette contained no nucleotides and the responsesto levcromakalim were generally much smaller than seen withATP. GDP (0.5 mM), in the absence of pipette ATP, activateda large background K⁺ current which had similar properties toI_lev. Consistent with this was the observation that I_lev becamesubstantially reduced in the presence of GDP, presumably becausea significant amount of I_K,ATP was already activated. Conclusions:The response to levcromakalim in isolated cells from pulmonaryartery was, as expected for an agent activating K_ATP channels,modulated by changes in the pipette [ATP]. This effect was notdependent on the presence of other pipette nucleotides, althoughthe possibility cannot be excluded that metabolites from thecellular breakdown of ATP are essential for normal channel regulation.GDP could also activate I_K,ATP under conditions where the channelis probably in a low phosphorylation state. The time-dependenteffects of GTP require further work to determine the precisemechanism, but may suggest that GTP and/or G-proteins are involvedin the regulation of K_ATP channels.

KEYWORDS Potassium channel, ATP sensitive; Potassium channel openers; Sulphonylureas; Nucleotide phosphates; Rabbit, vascular myocytes

^* Tel. 928-9292 ext. 3373; Fax (+44-71) 928-0658.

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