Antagonism by Class I Antiarrhythmic Drugs of Levcromakalim-Induced Relaxation in Isolated Rat Aorta

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Vol. 287, Issue 1, 81-86, October 1998

Antagonism by Class I Antiarrhythmic Drugs of Levcromakalim-Induced Relaxation in Isolated Rat Aorta¹

Angel L. Cogolludo, Francisco Perez-Vizcaino and Juan Tamargo

Department of Pharmacology, Institute of Pharmacology and Toxicology (CSIC/UCM), School of Medicine, University Complutense of Madrid, 28040 Madrid, Spain

	Abstract

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We have analyzed the effects of several class I antiarrhythmic drugs (propafenone, quinidine, its enantiomer quinine, disopyramide,flecainide and mexiletine), tetraethylammonium (TEA) and glibenclamideon the vasodilator effects of the adenosine 5'-triphosphate-dependentK⁺ channels channel opener levcromakalim in isolated rat aorta precontractedby 30 mM KCl. TEA (>1 mM) and disopyramide ( $>=$ 10 µM), induced asustained contraction in resting aortic rings. Propafenone ( $>=$ 3µM), quinidine ( $>=$ 30 µM), disopyramide ( $>=$ 100 µM) and flecainide( $>=$ 100 µM) but not the other drugs decreased the contraction inducedby 30 mM KCl in a concentration-dependent manner. Propafenone( $>=$ 1 µM), quinidine ( $>=$ 10 µM), quinine ( $>=$ 1 µM), disopyramide ( $>=$ 3µM), flecainide ( $>=$ 100 µM), mexiletine ( $>=$ 3 µM), TEA ( $>=$ 0.3 mM) andglibenclamide ( $>=$ 0.1 µM) caused a concentration-dependent inhibitionof the vasodilation induced by levcromakalim in rat aortic rings.The order of potency of the drugs, expressed as pD₂ values, toinhibit the vasodilation induced by 0.3 µM levcromakalim was thefollowing: glibenclamide (6.84) > quinine (6.14) > propafenone(5.27) > disopyramide (5.03) > quinidine (4.80) > mexiletine (4.68)> flecainide (3.37) > TEA (3.20). With the exception of flecainideand mexiletine, the slopes of the Schild plots were similar tounity. Based on the mode of antagonism these drugs could be classifiedin four groups: 1) glibenclamide which only shifted the curvesto the right, 2) quinidine and disopyramide that, at low concentrations,shifted the curve to the right but, at higher concentrations,it also reduced the maximal relaxant effect, 3) propafenone, quinineand TEA that shifted the curve rightwards and reduced the maximalrelaxation at all concentrations and 4) flecainide and mexiletinewhose Schild slopes were clearly different from unity. In conclusion,class I antiarrhythmic drugs inhibited levcromakalim-induced relaxationin isolated rat aorta. The concentrations at which these effectswere observed were within the therapeutic range (except for flecainide)and similar to those reported to inhibit adenosine 5'-triphosphate-dependentK⁺ channel currents. Analysis of the concentration-response curvesrevealed that these drugs produced a noncompetitive antagonismof levcromakalim-induced relaxations.

	Introduction

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K_ATP are expressed in a wide variety of cell types and regulate important cellular activities such as insulin secretion inpancreatic $beta$ cells, smooth muscle tone and repolarization of thecardiac action potential (Ashcroft and Ashcroft, 1990). Thesechannels are specifically inhibited by physiological cytosolicATP concentrations or by sulphonylurea drugs such as glibenclamideand are activated by K_ATP channel openers (Edwards and Weston,1993). In vascular smooth muscle cells, activation of K_ATP channelshyperpolarize the cell membrane and reduce Ca⁺⁺ channel activity decreasing vascular tone (Quast, 1993; Edwardsand Weston, 1995). Therefore, K_ATP channel openers are powerfulvasodilators, levcromakalim being the most representative agentof this group.

Class I antiarrhythmic drugs include those agents that block cardiac Na⁺ channels, decreasing the rate of depolarization of cardiac cells(Tamargo et al., 1992). According to the rate of binding-dissociationfrom Na⁺ channels, class I drugs have been further classified into threesubgroups: Ia, Ib and Ic (Vaughan Williams, 1984). However, mostof the currently available class I drugs exhibit multiple actions,so that they can inhibit several other cardiac Ca⁺⁺ and K⁺ channels, thus, exerting also class III and class IV antiarrhythmicactions (Salata and Wasserstrom, 1988; Kotake et al., 1988; Scampset al., 1989; Tamargo et al., 1992; Delgado et al., 1993; Slawskyand Castle, 1994; Delpón et al., 1995). In vascular smooth muscle,these drugs also inhibit Ca⁺⁺ entry through L-type Ca⁺⁺ channels leading to vascular smooth muscle relaxation (Carrónet al., 1991; Pérez-Vizcaíno et al., 1991, 1994; Fernándezdel Pozo et al., 1996, 1997).

A wide range of antiarrhythmic drugs has been reported to inhibit glibenclamide-sensitive currents activated by K_ATP channelopeners in Xenopus oocytes (Sakuta et al., 1992). In addition,an inhibitory effect of some class I antiarrhythmic drugs (disopyramide,quinidine and its enantiomer quinine) on K_ATP channels has alsobeen reported in isolated mammalian cells (Bovkist et al., 1990;De Lorenzi et al., 1995; Moser et al., 1995). However, the relationshipbetween the inhibitory actions on K⁺ efflux and relaxation induced by K_ATP channel openers is unclear(e.g., the K⁺ channel blocker tedisamil inhibited cromakalim-induced ⁸⁶Rb⁺ efflux approximately 30 times more potently than cromakalim-inducedrelaxation in the rat aorta; Bray and Quast, 1991). Unfortunately,the effects of class I antiarrhythmics on vascular smooth musclerelaxation induced by K_ATP channel openers are unknown.

Therefore, we have analyzed the effects of several class I antiarrhythmic drugs (class Ia: quinidine, its enantiomer quinineand disopyramide; class Ib: mexiletine; and class Ic: propafenoneand flecainide) on the vasodilator effects of the K_ATP channelopener levcromakalim in isolated rat aorta.

	Materials and Methods

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Tissue preparation. Male Wistar rats (300-350 g), were killed by a blow on the head and then exsanguinated. The descending thoracic aorta wasrapidly dissected and placed in Krebs solution of the followingcomposition (in mM): NaCl 118, KCl 5, NaHCO₃ 25, MgSO₄ 1.2, CaCl₂2, KH₂PO₄ 1.2 and glucose 11 at pH 7.4. After excess of fat andconnective tissue had been removed, the aorta was cut into rings(2-3 mm) and endothelium was mechanically removed by gently rubbingthe intimal surface of the rings with a metal rod. The rings weresuspended horizontally by means of two parallel L-shaped stainlesssteel holders inserted into the lumen in 5-ml organ baths filledwith Krebs and bubbled with a 95% O₂-5% CO₂ gas mixture and maintainedat 37°C. One holder served as anchor and the other was attachedto an isometric force-displacement transducer coupled to a signalamplifier (Model PRE 206-4, Cibertec, Madrid, Spain) and connectedto a computer via an A/D interface. Contractile tension was recordedby a REGXPC computer program (Cibertec) as previously described(Pérez-Vizcaíno et al., 1997). Each ring was stretched to aresting tension of 2 × g and allowed to equilibrate for 60 to90 min. During this period tissues were restretched and washedevery 30 min with warm Krebs solution. The procedure of endotheliumremoval was tested by the lack of relaxant effects of 10⁶ M acetylcholine in rings precontracted with 10⁶ M noradrenaline.

Experimental procedures. After equilibration, aortic rings were initially contracted by 30 mM KCl and when the tonic contractile response was stable,they were washed with Krebs solution to recover the basal tone.Rings were then exposed for 30 min to vehicle or the followingdrugs: propafenone (1, 3 and 10 µM), quinidine (3, 10, 30 and100 µM), quinine (0.3, 1, 3 and 30 µM), disopyramide (3, 10, 30and 100 µM), flecainide (10, 30 and 100 µM), mexiletine (1, 3,10, 30 and 100 µM), TEA (0.1, 0.3, 1 and 3 mM) and glibenclamide(0.1, 0.3 and 1 µM). Thereafter, a second contraction was inducedby 30 mM KCl and a concentration-response relaxation curve wasobtained by cumulative addition of levcromakalim (0.01-10 µM)in the continuous presence of the drugs. The relaxant responseto levcromakalim in treated arteries was expressed as a percentageof the maximal response to levcromakalim in control arteries obtainedin parallel experiments for each drug.

Drugs. The following drugs were used: quinidine sulfate, quinine hydrochloride, disopyramide phosphate, glibenclamide, tetraethylammoniumchloride, acetylcholine chloride, noradrenaline (Sigma Chemical,Madrid, Spain), flecainide acetate (Laboratorios Dr. Esteve S.A.Barcelona, Spain), propafenone hydrochloride (Knoll AG Ludwigshafen,Germany), mexiletine (Boheringer Ingelheim) and levcromakalim(Smith Kline Beecham Pharmaceuticals Betchworth, U.K.). All drugswere dissolved in distilled deionized water to prepare a 10² or 10³ M stock solution (except glibenclamide that was dissolved inDMSO) and further dilutions were made in Krebs solution. The finalconcentration of DMSO used ( $<=$ 0.01%) had no effect on the assaysperformed. Quinidine sulfate contains 2 mol of quinidine baseper mol but the concentrations were expressed as final quinidinebase concentrations.

Analysis of the results. Results are expressed as means ± S.E. of measurements in arteries from n different animals. Contractile responses are expressedas a percentage of the initial response to 30 mM KCl. Individualcumulative concentration-response curves were fitted to a logisticequation. The drug concentration exhibiting 50% of the maximaleffect (E_max) was calculated from the fitted concentration-responsecurves for each ring and expressed as negative log molar (pD₂).The concentration-response curves to levcromakalim in the presenceand absence of the drugs were analyzed by plotting the negativelogarithm of the ratio of concentrations of the agonist that producedthe same effect (50% relaxation) in the presence and absence ofthe antagonist minus 1 [log (concentration ratio $-$ 1)] againstthe negative logarithm of the concentration of antagonist (i.e.,Schild-plot analysis, Arunlakshana and Schild, 1959). The intercepton the abcissa yields the pA₂ value (negative logarithm of theconcentration of antagonist which induces a 2-fold rightward ofthe concentration-response to the agonist) which is an indicatorof the affinity of the antagonist. The slope of this plot is anindicator of the type of antagonism, i.e., a slope similar to1 is considered to be competitive antagonism. Statistically significantdifferences were calculated by a two-way analysis of varianceanalysis. P < .05 was considered statistically significant.

	Results

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Effects on basal tension. At the range of concentrations tested, propafenone, quinine, flecainide, mexiletine and glibenclamide did not produce anysignificant change in basal tension. A transient contraction wasoccasionally observed with 100 µM quinidine or 1 mM TEA but thefinal tone after 30 min of exposure to the drug was not significantlydifferent from the basal value. TEA (3 mM) and disopyramide ( $>=$ 10µM) induced a sustained contraction representing 66 ± 18% (n =7) and 48 ± 4% (n = 6) of the contraction induced by 30 mM KCl,for 3 mM TEA and 100 µM disopyramide, respectively.

Effects on KCl-induced contraction. Rings were initially contracted by 30 mM KCl (1052 ± 33 mg, n = 219), then washed in normal Krebs solution, exposed to vehicleor different concentrations of class I drugs, TEA or glibenclamidefor 30 min and again exposed to 30 mM KCl. The contractile responseto 30 mM KCl after exposure to vehicle in control rings averaged107 ± 2% of the initial contraction (n = 43). Propafenone ( $>=$ 3µM), quinidine ( $>=$ 30 µM), disopyramide ( $>=$ 100 µM) and flecainide( $>=$ 100 µM) significantly decreased the degree of contraction inducedby 30 mM KCl in a concentration-dependent manner as compared tocontrols (76 ± 6 and 44 ± 3% at 3 and 10 µM propafenone, respectively;84 ± 2 and 46 ± 2% at 30 and 100 µM quinidine, respectively; 85± 3% at 100 µM disopyramide and 44 ± 5% at 100 µM flecainide,P < .05, n = 5-8). In contrast, at the range of concentrationstested, quinine, mexiletine, TEA and glibenclamide had no effecton the 30 mM KCl-induced contraction.

Effects on levcromakalim-induced relaxation. Levcromakalim (0.01-10 µM) induced a concentration-dependent relaxation in control arteries precontracted by 30 mM KCl (pD₂= 7.04 ± 0.02, E_max = 85 ± 2%, n = 43). Propafenone (1, 3 and10 µM), quinidine (3, 10, 30 and 100 µM), quinine (0.3, 1, 3,10 and 30 µM), disopyramide (3, 10, 30 and 100 µM), flecainide(10, 30 and 100 µM), mexiletine (1, 3, 10, 30 and 100 µM), TEA(0.1, 0.3, 1 and 3 mM) and glibenclamide (0.1, 0.3 and 1 µM) causeda concentration-dependent inhibition of the vasodilation inducedby levcromakalim in rat aortic rings (fig. 1). All these agentsshifted the concentration-response curve to the right, decreasingthe pD₂ value for levcromakalim-induced relaxation. This effectreached statistical significance for all concentrations testedof propafenone, disopyramide and glibenclamide, and for concentrations $>=$ 10 µM quinidine, $>=$ 1 µM quinine, $>=$ 100 µM flecainide, $>=$ 3 µM mexiletineand $>=$ 0.3 mM TEA. The E_max for levcromakalim was not significantlydifferent in aortic rings treated with glibenclamide, flecainideor with the low concentrations of quinidine (3, 10 and 30 µM),disopyramide (3 and 10 µM), mexiletine (1 µM) or TEA (0.1 mM)as compared to controls, whereas propafenone, quinine and higherconcentrations of quinidine, disopyramide, mexiletine and TEAsignificantly decreased the E_max. The E_max reduction induced bythese drugs was concentration-dependent except for mexiletinewhich induced a similar reduction at concentrations between 3and 100 µM.

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Fig. 1. Antagonism by class I antiarrhythmic drugs (A-F), TEA (G) and glibenclamide (H) of the relaxant response to levcromakalim. Concentration-response curves to levcromakalim were carried out in arteries pre-contracted by 30 mM KCl in the absence (controls

) or in the presence of propafenone, quinidine, quinine, disopyramide, flecainide, mexiletine, TEA or glibenclamide. Each symbol represents the mean ± S.E. of five to nine experiments. Results are expressed as a percent of the maximal relaxation in control experiments.

The inhibitory effect of these drugs on the relaxation induced by 0.3 µM levcromakalim (a submaximally effective concentration)is plotted in figure 2. The order of potency of the drugs forthis inhibitory action expressed as pD₂ values was the following:glibenclamide (6.84), quinine (6.14), propafenone (5.27), disopyramide(5.03), quinidine (4.80), mexiletine (4.51), flecainide (3.37)and TEA (3.20). Therefore, quinidine was about 20 times less potentthan its enantiomer quinine.

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Fig. 2. Inhibitory effects of propafenone (

), quinidine ( $open circle$ ), quinine ( $bullet$ ), disopyramide ( $black-triangle$ ), flecainide ( $triangle$ ), mexiletine ( $diamond$ ), TEA (

) and glibenclamide ( $black-lozenge$ ) on the levcromakalim-induced relaxation. The results (% inhibition of the relaxation induced by 0.3 µM levcromakalim) are plotted from the data in figure 1.

The Schild plot for the inhibitory action on levcromakalim-induced relaxation is shown in figure 3. The slopes of these plotsyielded values of 1.06 for propafenone, 0.96 for quinidine, 0.82for quinine, 0.89 for disopyramide, 0.51 for flecainide, 0.41for mexiletine, 0.84 for TEA and 1.06 for glibenclamide. Therefore,with the exception of flecainide and mexiletine, these slopeswere similar to unity. The pA₂ values calculated from the Schildplot were 5.58 for propafenone, 5.20 for quinidine, 6.21 for quinine,5.64 for disopyramide, 4.05 for flecainide, 4.93 for mexiletine,3.54 for TEA and 7.06 for glibenclamide.

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Fig. 3. Schild plots of the antagonism of propafenone (

), quinidine ( $open circle$ ), quinine ( $bullet$ ), disopyramide ( $black-triangle$ ), flecainide ( $triangle$ ), mexiletine ( $diamond$ ), TEA (

) and glibenclamide ( $black-lozenge$ ) of levcromakalim-induced relaxation. The results are plotted from the data in figure 1.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

We have analyzed the antagonism of several class I antiarrhythmics on the relaxation induced by the K_ATP channel opener levcromakalimin the isolated rat aorta. The results were compared to thoseof the specific K_ATP inhibitor glibenclamide and the nonselectiveK⁺ channel blocker TEA. All the drugs tested (i.e., propafenone,quinidine, quinine, disopyramide, mexiletine and flecainide) inhibitedthe relaxations induced by levcromakalim in a concentration-dependentmanner. The order of potency for this inhibitory action was thefollowing: glibenclamide, quinine, propafenone, disopyramide,quinidine, mexiletine, flecainide and TEA. All drugs, produceda rightward shift of the concentration-response curve to levcromakalim,and with the exception of glibenclamide, they also reduced itsmaximal relaxant response.

TEA and disopyramide produced a sustained contraction under basal tension. This effect may be attributable to the blockadeof the K⁺ channels involved in the control of resting membrane potentialleading to depolarization of vascular smooth muscle cells which,in turn, opens L-type Ca⁺⁺ channels (Bolton, 1979). However, despite the contraction inducedby TEA and disopyramide the tone after the subsequent additionof KCl was not greater than that in the absence of these drugs,i.e., TEA- and disopyramide-induced contractions were not additiveto the KCl-induced contraction. Propafenone, quinidine, disopyramideand flecainide (but not the other drugs) decreased the contractionsinduced by 30 mM KCl. The order of potency for this effect wasthe following: propafenone, quinidine, flecainide and disopyramide.This inhibitory action on 30 mM KCl-induced contractions is consistentwith our previous reports showing that these drugs inhibit thecontractions and ⁴⁵Ca⁺⁺ entry induced by high (80 mM) KCl concentrations due to theirL-type Ca⁺⁺ channel blocking properties (Carrón et al., 1991; Pérez-Vizcaínoet al., 1991, 1994; Fernández del Pozo et al., 1996, 1997). Furthermore,they confirm the stereoselectivity of quinidine-induced inhibition(Fernández del Pozo et al., 1996). This inhibition of Ca⁺⁺ entry limited the use of higher concentrations of some drugssuch as flecainide, which at 100 µM inhibited the contractioninduced by 30 mM KCl by about 50% and only had a weak inhibitoryaction on levcromakalim-induced relaxation. However, the inhibitoryaction of levcromakalim-induced relaxation seems to be independenton the inhibition of KCl-induced contractions since the orderof potency of both effects was different (e.g., the stereoselectivityof quinidine-induced inhibition for both effects was opposite).

The inhibitory effects on K_ATP channels have been reported for disopyramide in cat ventricular myocytes (De Lorenzi et al.,1995) and mouse skeletal muscle (Moser et al., 1995), for quinidinein cat ventricular myocytes (De Lorenzi et al., 1995) and forquinine in pancreatic $beta$ cells (Bovkist et al., 1990). The actionsof a wide range of antiarrhythmics (including propafenone, quinidine,disopyramide, flecainide and mexiletine) on the K⁺ current induced by K⁺ channel openers have also been studied in Xenopus oocytes (Sakutaet al., 1992). It has been reported that K_ATP channels in Xenopusfollicular cells and in vascular smooth muscle cells share commonbiophysical, pharmacological and regulation properties (Guillemareet al., 1995). The order of potency reported in Xenopus oocytes(calculated pD₂ values of 6.52 for glibenclamide, 4.75 for disopyramide,4.2 for propafenone, 3.82 for quinidine and 3.35 for flecainide,Sakuta et al., 1992) was very similar to that reported in ourstudy. In fact, although our pD₂ values were slightly greaterthan those reported by Sakuta et al. (1992), we found a very goodcorrelation between the pD₂ values of both studies (correlationcoefficient of 0.93 and a slope of 0.94, P < .05). Furthermore,our results indicate that the degree of inhibition by class Iantiarrhythmics is a function of the concentration of K_ATP channelopener used because they behave, at least over a certain rangeof concentrations, as apparent competitive antagonists. The resultsobtained with mexiletine are difficult to compare with other studies,because it has been reported to be both an inhibitor (pD₂ = 2.89in Xenopus oocytes; Sakuta et al., 1992) and an activator of K_ATPchannels (in guinea pig papillary muscles; Sato et al., 1995).The potency of quinine in our study was also consistent with thatreported by Bovkist et al. (1990) in pancreatic $beta$ cells. Therefore,the inhibitory effect of class I antiarrhythmic drugs observedin our study on levcromakalim-induced relaxation paralleled thatfound on K_ATP channel opener-induced K⁺ currents by other authors.

In our study, glibenclamide shifted the concentration-response curves to levcromakalim to the right without affecting themaximal relaxant response and the Schild plot analysis yieldedslope values similar to unity, indicating an apparent competitiveantagonism. Quinidine and disopyramide, at low concentrations,reduced the pD₂ value without affecting the E_max of levcromakalim,whereas at higher concentrations they reduced both parameters.Propafenone, quinine and TEA at concentrations that induced aweak reduction in the pD₂ value significantly decreased the E_max.Therefore, despite the fact that the slope of the Schild plotwas similar to unity, the antagonism induced by these drugs cannotbe considered as competitive. Flecainide produced a weak inhibitoryaction which was observed only at concentrations that produceda marked inhibition of KCl-induced contraction. Mexiletine reducedboth the pD₂ value and the E_max, however, its inhibitory actiondid not show a clear concentration dependency because it induceda similar reduction at concentrations between 3 and 100 µM. Thiseffect might be related to its dual action on K_ATP channels, becauseit has been reported to be an inhibitor in Xenopus oocytes (Sakutaet al., 1992) and an activator in guinea pig papillary muscles(Sato et al., 1995).

K_ATP channel is a multimeric complex of inwardly rectifying K⁺ channel subunits (Kir 6.1 or Kir 6.2) and the sulphonylurea receptor(SUR1 or SUR2) (Inagaki et al., 1995). Glibenclamide interactsat a specific binding site in SUR1 that is not located in thepore region of the channel. In functional studies, glibenclamidebehaves as an apparent competitive antagonist of levcromakalimand other related K_ATP channel openers (Pérez-Vizcaíno et al.,1993; Edwards and Weston, 1993) but as shown in binding studies,K_ATP channel openers (with the exception of diazoxide) do notcompete with glibenclamide for its binding site (Gopalakrishnanet al., 1991), indicating that the glibenclamide site is differentfrom, but negatively allosterically coupled to the binding sitefor the openers (Bray and Quast, 1992). In contrast, the nonselectiveK⁺ channel blockers TEA and antiarrhythmic drugs are thought toinhibit K⁺ currents by binding to the pore region of the channel (Yellenet al., 1991; Kirsch et al., 1991; Snyders and Yeola, 1995) andat the concentrations at which inhibit levcromakalim-induced relaxation,quinine, quinidine and TEA had no effect on [³H]-glibenclamide binding (Gopalakrishnan et al., 1991). However,it is not known whether these drugs can bind to the K_ATP channelopener site. Furthermore, the inhibitory action of antiarrhythmicdrugs on K_ATP currents has been correlated with their abilityto bind calmodulin, suggesting the existence of a calmodulin-likestructure associated with the K_ATP channel (Sakuta et al., 1992).Thus, several targets related to the K_ATP channel might be responsiblefor the inhibition of levcromakalim-induced relaxation. However,an interaction of class I drugs with other targets different fromthe K_ATP channel that may indirectly affect levcromakalim-inducedrelaxation cannot be completely ruled out from our experiments.The different interaction of glibenclamide, TEA and class I antiarrhythmicdrugs with these targets may explain their distinct mode of antagonismon levcromakalim-induced relaxation.

It is interesting to note that, with the exception of flecainide, the concentrations of class I antiarrhythmic drugs whichsignificantly inhibited levcromakalim-induced relaxation in ourstudy were within the therapeutic range used for the treatmentof cardiac arrhythmias (therapeutic range: 0.92-5 µM for propafenone,6-15 µM for quinidine, 8-22 µM for disopyramide, 0.5-2 µM forflecainide and 2.8-11 µM for mexiletine; Roden, 1996). Thus, itmay be possible that the inhibitory action on K_ATP channels isclinically relevant during the course of arrhythmia treatmentwith class I antiarrhythmic drugs. Under physiological conditions,K_ATP channels are not basally activated in most vascular bedsand, therefore, their inhibition does not result in vasoconstriction.In fact, glibenclamide has no effect on arterial blood pressure(Edwards and Weston, 1995). However, K_ATP channels regulate arterialtone in several vascular beds, namely the coronary circulationwhere their blockade results in significant vasoconstriction (Samahaet al., 1992). Moreover, hypoxic vasodilation in isolated perfusedhearts can be blocked by glibenclamide and mimicked by cromakalim(Daut et al., 1990). These results suggest that opening of K_ATPchannels appears to be a major physiological way of achievingcoronary vasodilation (Richer et al., 1990). In our study, wefound that class I antiarrhythmic drugs block K_ATP channel-mediatedvasorelaxation. So that it would be expected that any pathophysiologicalrole of K_ATP channels in vascular smooth muscle tone might beinhibited by these drugs. The routine use of class I antiarrhythmicdrugs after myocardial infarction is associated with increasedmortality (Teo et al., 1993). One working hypothesis to explainincreased mortality is that class I drugs exert a deleterous effecton ischaemic myocardium (Etch et al., 1991; Podrid and Fogel,1992). In fact, in animal models class I antiarrhythmics havea proarrhythmic potential when combined with acute ischaemia,a condition where K_ATP channels are maximally activated (Elharraret al., 1977; Nattel et al., 1981). From our data it could bespeculated that K_ATP channel blockade by class I antiarrhythmicsmight increase coronary tone and inhibit hypoxia-induced coronaryvasodilation, thus increasing myocardial ischemia. This effecttogether with the slowing of intracardiac conduction may converta stable myocardium into an unstable and arrhythmogenic one (Podridand Fogel, 1992). However, we must keep in mind that class I antiarrhythmicagents exert multiple effects including calcium channel blockingproperties that may partially counteract the effect of blockingK_ATP channels. Therefore, the net final effect would be differentdepending on the drug and the experimental conditions.

In conclusion, the class I antiarrhythmic drugs (propafenone, quinidine, quinine, disopyramide, flecainide and mexiletine)inhibited levcromakalim-induced relaxation in isolated rat aorta.The concentrations at which these effects were observed were withinthe therapeutic range and similar to those reported to inhibitK_ATP currents. Analysis of the concentration-response curves revealedthat these drugs produced a noncompetitive antagonism of levcromakalim-inducedrelaxations.

	Acknowledgment

The authors are grateful to C. Rivas and R. Vara for the excellent technical assistance.

	Footnotes

Accepted for publication May 26, 1998.

Received for publication September 23, 1997.

¹ This work was supported by CICYT SAF 96-0042 and FIS 95/0308 Grants. A.L.C. is a recipient of a Comunidad Autonoma de Madrid(CAM) Grant.

Send reprint requests to: Dr. Francisco Pérez-Vizcaíno, Department of Pharmacology, Institute of Pharmacology and Toxicology (CSIC/UCM), School of Medicine, University Complutense of Madrid, 28040 Madrid, Spain.

	Abbreviations

DMSO, dimethylsulfoxide; ATP, adenosine 5'-triphosphate; K_ATP, ATP-dependent K⁺ channels; TEA, tetraethylammonium.

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