Receptor-Mediated Effects of Endothelin on the L-Type Ca++ Current in Ventricular Cardiomyocytes

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Vol. 286, Issue 2, 662-669, August 1998

Receptor-Mediated Effects of Endothelin on the L-Type Ca⁺⁺ Current in Ventricular Cardiomyocytes

Elizabeth J. Kelso, J. Paul Spiers, Barbara J. McDermott, C. Norman Scholfield and Bernard Silke

Department of Therapeutics and Pharmacology (E.J.K., B.J.McD., B.S.), and School of Biomedical Sciences (J.P.S., C.N.S.), The Queen's University of Belfast, Belfast, Northern Ireland

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The purpose of this study was to establish whether specific receptor subtypes are responsible for mediating the effects ofendothelin-1 (ET-1) and endothelin-3 (ET-3) on the L-type calciumcurrent (I_Ca) using a number of receptor-selective antagonists,including PD155080 (ET_A), BQ-788, RES-701 and IRL-1038 (ET_B) andthe ET_A/ET_B receptor-non-selective antagonist PD145065. Ventricularcardiomyocytes were isolated from adult New Zealand White rabbitsusing Langendorff perfusion with collagenase. I_Ca was recordedusing a whole-cell patch-clamp technique. ET-1 decreased, whereasET-3 increased, I_Ca at equimolar concentrations of 10 nM. Thedecrease in I_Ca produced by ET-1 was completely blocked by PD155080and PD145065 (1 and 10 µM); however, I_Ca was increased upon washoutof PD155080. Although the decrease in I_Ca produced by ET-1 waspartially blocked by BQ-788 (1 and 10 µM), ET-1 in combinationwith either RES-701 (1 and 10 µM) or IRL-1038 (1 µM) produceda decrease in I_Ca similar to that produced by ET-1 alone. Theincrease in I_Ca by ET-3 was completely abolished by either BQ-788or IRL-1038 (1 µM). These data indicate that the decrease in I_Caproduced by ET-1 in rabbit ventricular cardiomyocytes is mediatedby the ET_A receptor subtype, because PD155080 completely inhibitedthis response. The ET_B receptor-selective antagonists RES-701and IRL-1038 did not alter the decrease in current produced byET-1, although the response was partially sensitive to BQ-788,which may lack receptor-subtype selectivity in these cells. Incontrast, the increase in I_Ca produced by ET-3 was mediated bythe ET_B receptor subtype, because BQ-788 and IRL-1038 abolishedthis response.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Endothelin is a 21-amino-acid polypeptide that was originally isolated from the culture medium of porcine aortic endothelialcells (Yanagisawa et al., 1988). Three structurally and pharmacologicallydistinct isoforms of endothelin have been identified: ET-1, ET-2,ET-3 (Haynes and Webb, 1993). Although initially identified asa potent vasoconstrictor peptide, ET-1 mediates a wide varietyof pharmacological activities in various tissues (Rubanyi andPolokoff, 1994). Many reports have described the positive inotropic,positive chronotropic and hypertrophic effects of ET-1 on themyocardium (Ishikawa et al., 1988a,b; Moravec et al., 1989; Takanashiand Endoh, 1991). The cellular basis for the actions of ET-1 ishighly complex; however, alterations in Ca⁺⁺ homeostasis appear to be central to the cardiac actions of thisisopeptide. Although it is not clear whether ET-1 plays a physiologicalrole, the isopeptide is implicated in many cardiovascular pathophysiologicaldisorders, including hypertension, atherosclerosis, cardiogenicshock and myocardial infarction (Cavero et al., 1990; Kohno etal., 1990; McMurray et al., 1992; Huggins et al., 1993). Elevatedplasma levels of ET-1 after myocardial infarction are likely toaccompany much higher local concentrations of the peptide in themyocardium.

Two distinct subtypes of endothelin receptor, ET_A and ET_B, have been pharmacologically distinguished by the different potenciesof the endothelin isopeptides toward the receptors. ET-1 has ahigher affinity for the ET_A receptor subtype than do ET-2 andET-3, whereas the isopeptides have a similar affinity for theET_B receptor subtype (Rubanyi and Polokoff, 1994). Recently, thedevelopment and subsequent use of receptor-selective compoundshave made receptor classification more complex (Sudjawaro et al.,1994; Warner, 1994). An increasing number of atypical ET responseshave been identified that point to populations of receptors characterizedas partially atypical or subtypes of ET_A and ET_B (Bax and Saxena,1994). ET_A receptors have been subdivided, on the basis of theirdifferential selectivities to the ET_A receptor-selective antagonistBQ-123, into ET_A1 (BQ-123-sensitive) and ET_A2 (BQ-123-insensitive)receptors (Sudjawara et al., 1994). In addition, the ET_B receptorsubtypes located on vascular endothelium (ET_B1) and those locatedon smooth muscle (ET_B2) differ in antagonist selectivity (Douglaset al., 1994).

Both ET_A and ET_B receptor subtypes have been identified, using radioligand binding assays, in cardiac tissues isolated fromhuman (Molenaar et al., 1993), rabbit (Takanashi and Endoh, 1991),guinea pig (Ono et al., 1994) and rat (Koseki et al., 1989). Bothreceptor subtypes coexist in cardiomyocytes, as has been demonstratedusing in situ hybridization techniques (Hori et al., 1992). Manyof the intracellular actions of ET-1 in cardiac tissues are mediatedthrough the ET_A receptor subtype. For example, ET-1 inhibits aprotein kinase-A-dependent chloride current via the ET_A receptorsubtype in guinea pig ventricular cardiomyocytes (James et al.,1994). Moreover, BQ-123 abolished the decrease, produced by ET-1,in the accumulation of cyclic AMP and I_Ca in atrial cells (Onoet al., 1994). It is speculated that stimulation of the ET_B receptorsubtype is likely to produce electrophysiological effects verydifferent from those described for the ET_A receptor subtype. ET-1has been reported both to increase (Lauer et al., 1992; Bkailyet al., 1995; Tong et al., 1995) and to decrease (Tohse et al.,1990; Ono et al., 1994; Cheng et al., 1995) the I_Ca in cardiomyocytes,depending on the concentration and experimental conditions (Laueret al., 1992; Kelso et al., 1996). The purpose of the currentstudy was to establish, using a number of recently developed receptor-selectiveand receptor-non-selective antagonists, whether specific receptorsubtypes are responsible for mediating the effects of ET-1 onI_Ca. An integral part of this investigation was to examine alsothe effects of ET-3, which has an equal affinity for the ET_A andET_B receptor subtypes.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Isolation of cardiomyocytes. Ventricular cardiomyocytes were obtained from male New Zealand White rabbits (2.5-3 kg) after enzymatic dissociation usingcollagenase (Kelso et al., 1995a). All procedures were undertakenin accordance with Guidance on the Operations of the Animals (ScientificProcedures) Act 1986. Rabbits were anesthetized using sodium pentabarbitone(50 mg/kg i.v.) after heparinization (400 I.U./kg i.v.), and thechest was opened and the heart quickly removed and cannulated,through the ascending aorta, on a modified Langendorff perfusionapparatus. Blood was flushed from the coronary vasculature witha Ca⁺⁺-free modified Krebs Ringer buffer (KRB) containing 110 mM NaCl,2.6 mM KCl, 25 mM NaHCO₃, 1.2 mM MgSO₄, 1.2 mM KH₂PO₄ and 11 mMglucose (pH 7.4, 37°C), which had just previously been aeratedwith 95%O₂/5%CO₂. The perfusate was subsequently supplementedwith 0.12% (w/v) collagenase and recirculated for approximately15 min while maintained at 37°C and continuously aerated with95%O₂/5%CO₂. After enzymatic digestion, the hearts were cut atthe atrioventricular junction, sliced vertically toward the apexand chopped into cubes of 0.7 mm³ using a mechanical tissue chopper (McIlwain Chopper, Mickle LaboratoryEngineering Co. Ltd., Surrey, U.K.). The minced tissue was placedin the collagenase-containing perfusate that had been supplementedwith 0.2% (w/v) BSA, and the mixture was triturated using a 10-mlserological pipette for approximately 5 min. The loosened cellswere filtered through a nylon mesh gauze of pore size 200 µm andwashed twice. Ca⁺⁺ was restored by means of centrifugation at 25 × g twice, andthe cells were resuspended in modified KRB solutions containing250 µM and 500 µM CaCl₂, respectively. Finally, the cells werelayered onto a solution of 4% (w/v) BSA containing 1 mM CaCl₂and were left to settle by gravity at 37°C. After approximately5 min the supernatant was aspirated and the resulting cell materialresuspended at a density of 1 to 2 mg protein/ml in a storagemedium (M199 with Earle's salts, containing 5 mM creatine, 5 mMtaurine, 2 mM carnitine, 100 I.U./ml streptomycin, 100 µg/ml penicillin,pH 7.4) at 37°C. Suspensions of cardiomyocytes were more than70% viable as estimated by their elongated rod-shaped morphology.

Recording techniques. An aliquot of cell suspension was placed in a transparent recording chamber and allowed to settle for 10 min before bathingwith a modified Tyrode's solution containing 137 mM NaCl, 5.4mM KCl, 3 mM CaCl₂, 1.2 mM MgCl₂, 5 mM HEPES and 10 mM glucose(pH 7.4). The I_Ca was recorded in voltage-clamp mode using anAxopatch 1D patch-clamp amplifier, and electrodes were filledwith 110 mM K-gluconate, 20 mM KCl, 2 mM MgCl₂, 10 mM HEPES, 11mM EGTA, 1 mM CaCl₂, 0.1 mM Na₂GTP and 2.5 mM creatine phosphate(pH 7.2). Patch electrodes were fabricated from thin-walled borosilicatecapillaries with a filament (1.5 mm in outside diameter, ClarkeElectrochemical) by means of a horizontal lazer puller (SutterInstruments, Model P2000) and had tip resistances of 1 to 3 M $Omega$ when filled with the electrode solution. Access to the cell interiorwas achieved by applying a brief pulse of negative pressure tothe electrode after a gigaseal was formed. After stabilization,Ca⁺⁺ currents were elicited by stepping the membrane voltage for 200ms from a holding potential of $-$ 40 mV to test potentials of $-$ 30to +60 mV at 5-s intervals and 10-mV increments; recordings weremade at 90-s and 180-s intervals before and after the applicationof each drug combination. Current "rundown" was not significantover the time course of the experiments $---$ that is, over a 10-minperiod. All currents were stored on computer for subsequent analysisusing customized software. Drugs were applied locally to the cellusing a gravity-fed microperfusion system at approximately 150µl/min, which allowed the solution bathing the cell to be changedin approximately 2 s.

Data analysis. The I_Ca was measured, using standard methodology, as the difference between the peak of the inward current and the steady-statecurrent level at the end of the voltage pulse (Varro et al., 1991).Current-voltage relationships were constructed, and peak I_Ca valueswere compared at +10 mV. I_Ca values were expressed as mean ± S.E.and data were analyzed, by comparing before and after drug applications,using analysis of variance followed by a Dunnett's multiple comparisontest (n > 2) or Student's t test (n = 2); P values less than .05were taken as indicating statistical significance.

Materials. ET-1 was purchased from Bachem Inc. (Torrance, CA). RES-701 and IRL-1038 were obtained from the American Peptide Co. (Sunnyvale,CA), and BQ-788 PD155080 and PD145065 were gifts from Parke-DavisPharmaceutical Co., Ann Arbor, MI. All antagonists were dissolvedin DMSO and stored in aliquots of 10⁴ M at $-$ 20°C; the final concentration of DMSO was <0.01%. ET-1was dissolved in dilute acetic acid (0.01%) and stored in aliquotsof 10⁵ M at $-$ 20°C. Collagenase (type I) was purchased from Serva Feinbiochemica(Heidelberg, Germany). Medium 199 was obtained from Gibco Ltd.(Paisley, U.K.). All other chemicals were of analytical grade(U.K.); twice-distilled water that had been deionized througha Millipore-Q system (Millipore, Harrow) was used in all experiments.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Effects of ET-1 and ET-3 on the I_Ca. Figure 1A shows original current traces at test potentials between $-$ 30 mV and +50 mV, in the absence and presence of ET-1(1 and 10 nM). At the end of each experiment, the current wascompletely abolished using nifedipine (5 µM), which substantiatesthat the current measured was indeed that of the I_Ca (resultsnot shown). Contamination of the I_Ca was minimized by inducingvoltage pulses from $-$ 40 mV, which inactivates the Na⁺ current. The influence of K⁺ currents was minimized by subtracting the current at the endof the test pulse from the peak inward current (Varro et al.,1991). ET-1 (10 nM) decreased (P < .05) the I_Ca to $-$ 1.86 ± 0.18nA from a control value of $-$ 2.90 ± 0.16 nA (n = 6); this inhibitoryeffect was maximum after 90 s, remained stable at 180 s and waspartially reversed to $-$ 2.46 ± 0.30 nA (fig. 1, B and C) aftera 180-s washout of the peptide. ET-1, at a concentration of 1nM, did not significantly alter the I_Ca from control. The correspondingcurrent-voltage relationships, shown in figure 1B, revealed thatthe effects of ET-1 were not associated with a shift along thevoltage axis but decreased the I_Ca at all potentials. ET-1 hadno effect on the background holding current.

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Fig. 1. Effects of ET-1 on I_Ca in ventricular cardiomyocytes isolated from rabbit myocardium (N = 5). a) Representative tracings recorded from a single cell showing the I_Ca before and 180 s after the application of ET-1 (10 nM), from a holding potential of $-$ 40 mV to test potentials between $-$ 30 mV and +50 mV. b) Current-voltage relationships constructed as the difference between the peak of the inward current and the steady-state current level at the end of the voltage pulse (n = 6). Recordings were made after a 180-s exposure to each concentration of the drug, and washout was assessed after perfusion in control solution, in the absence of ET-1, for a further 180 s. c) The concentration-dependent effects of ET-1 on peak I_Ca, at +10 mV, were illustrated as percent change relative to control. Vertical lines are S.E.M. *P < .005 represents a difference from control peak I_Ca. $dagger$ P < .01 represents a difference compared with peak I_Ca in the presence of ET-1 (10 nM). N represents number of animals; n represents number of cells.

ET-3, at concentrations of 1 and 10 nM, increased (P < .05) the amplitude of peak I_Ca to $-$ 3.05 ± 0.27 nA (fig. 2A, and B)and $-$ 2.77 ± 0.21 nA (fig. 2C), respectively, from control valuesof $-$ 2.49 ± 0.16 nA and $-$ 2.10 ± 0.13 nA, respectively. This increasewas time-dependent over a period of 270 s (fig. 2B). The peakI_Ca continued to increase to $-$ 3.10 ± 0.26 nA (fig. 2B) and $-$ 2.84± 0.22 nA (graph not shown) for a further 90 s in the absenceof ET-3. The current then declined in amplitude to $-$ 2.87 ± 0.25nA and $-$ 2.32 ± 0.19 nA, respectively, after a 270-s washout ofET-3. Because the effect of this isopeptide on I_Ca was slower,requiring a longer experiment time than ET-1, we recorded theeffects of ET-3 at concentrations of 1 and 10 nM separately indifferent experiments (fig. 2, A and C). The current-voltage relationshipsin the presence of ET-3 were not associated with a shift alongthe voltage axis, and ET-3 had no effect on the background holdingcurrent. The effect of ET-3 was partially reversed (P < .01) uponwashout of the drug (fig. 2D).

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Fig. 2. Effects of ET-3 on the I_Ca (N = 6). Because the effect of ET-3 on I_Ca was slow, it was necessary to examine the concentration effects of ET-3 in separate experiments. a) Current-voltage relationships constructed as the difference between the peak of the inward current and the steady-state current level at the end of the voltage pulse (n = 9). Recordings were plotted after a 270-s exposure to ET-3 (1 nM), and washout was assessed after perfusion in control solution, in the absence of ET-3, after a further 270 s. b) The time course of changes in peak I_Ca amplitude at +10 mV in response to ET-3 (1 nM). An initial recording was taken at time 0 in the absence of ET-3; three further recordings were taken in the presence of ET-3 at 90-s intervals, followed by three recordings after removal of the drug and perfusion in control solution (n = 9). Control readings were also obtained in the absence of drug (n = 6). c) Current-voltage relationships in the absence and presence of ET-3 (10 nM) (n = 12). d) The concentration-dependent effects of ET-3 on peak I_Ca were illustrated as percent change relative to control. Vertical lines are S.E.M. *P < .01 represents a difference from control peak I_Ca. $dagger$ P < .005 represents a difference compared with peak I_Ca in the presence of ET-3. N represents number of animals; n represents number of cells.

Influence of the ET_A receptor subtype on the ET-1-induced decrease in I_Ca. PD155080, at concentrations of 1 and 10 µM, had no effect on the I_Ca (n = 6) (peak I_Ca values of $-$ 2.72 ± 0.26 nA and $-$ 2.76± 0.28 nA, respectively, compared with a control value of $-$ 2.90± 0.33 nA) (graph not shown). In order to minimize current rundown,the effects of ET-1 in combination with PD155080 were examinedin a separate group of cells from those in which the effects ofthe antagonist alone were examined, or from those where the effectsof ET-1 alone were examined. ET-1 (10 nM) in the presence of PD155080(1 and 10 µM) did not alter the peak I_Ca amplitude, as observedfrom the original current trace in figure 3A, or over the voltagerange of $-$ 30 to +60 mV (fig. 3B). The peak I_Ca amplitudes recordedin the presence of ET-1 in combination with PD155080 (1 and 10µM) were $-$ 2.53 ± 0.13 nA and $-$ 2.58 ± 0.14 nA, respectively, whichwas not different from the control value of $-$ 2.65 ± 0.15 nA (n= 6). Washout of ET-1 in combination with PD155080 resulted ina small but significant increase in the peak I_Ca amplitude (fig.3C) to $-$ 2.88 ± 0.13 nA. However ET-1 in combination with PD155080did not affect the voltage dependence of activation on I_Ca.

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Fig. 3. Influence of the ET_A receptor-selective antagonist PD155080 on the ET-1-induced decrease of I_Ca (N = 5) a) Representative tracings showing the inhibitory effect of the ET-1 (10 nM)-induced decrease in peak I_Ca at +10 mV, by PD155080 (1 µM), in a single cell. b) Current-voltage relationships in the absence and presence of ET-1 (10 nM) in combination with PD155080 (1-10 µM). Recordings were obtained at 180-s intervals before and after exposure to ET-1 (10 nM) in combination with PD155080 (1 and 10 µM) and after washout of drug in control solution. c) Comparison of percent changes, relative to the control, in peak I_Ca by ET-1, in the absence and presence of PD155080. The blank bar is included for comparative purposes (fig. 1), whereas the shaded bars represent the change in peak I_Ca values from another group of cells (n = 6). Vertical lines are S.E.M. *P < .005 compared with peak I_Ca in the absence of drugs. PD155 represents PD155080.

Influence of the ET_B receptor subtype on the ET-1-induced decrease in I_Ca. At concentrations of 1 and 10 µM, neither RES-701 ( $-$ 2.50 ± 0.23 nA and $-$ 2.53 ± 0.29 nA, respectively, compared with a controlvalue of $-$ 2.64 ± 0.24 nA) nor BQ-788 ( $-$ 2.20 ± 0.23 nA and $-$ 2.28± 0.27 nA, respectively, compared with a control value of $-$ 2.35± 0.22 nA) alone had any effect on the I_Ca (n = 6-8) (graphs notshown). ET-1 (10 nM) in combination with RES-701 (1 and 10 µM)decreased (P < .05) the peak I_Ca amplitude (n = 10) to $-$ 1.63 ±0.13 nA and $-$ 1.59 ± 0.23 nA, respectively, from a control valueof $-$ 2.65 ± 0.24 nA. This effect was partially reversed upon washoutof the peptides to a peak I_Ca amplitude of $-$ 2.26 ± 0.24 nA (fig.4A). However, the decrease in current amplitude seen at all potentialswas not associated with a shift along the voltage axis (fig. 4B).The magnitude of the decrease in peak I_Ca amplitude produced byET-1 in combination with RES-701 (34 ± 4% to 36 ± 4%) was similarto the decrease produced by ET-1 alone (34 ± 4%; fig. 4C). Moreover,ET-1 (10 nM) in combination with IRL-1038 (1 µM) decreased (P< .05) the peak I_Ca amplitude (n = 4) to $-$ 1.77 ± 0.46 nA froma control value of $-$ 2.37 ± 0.50 nA (graphs not shown).

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Fig. 4. Influence of the ET_B receptor-selective antagonist RES-701 on the ET-1-induced decrease in I_Ca (N = 5). a) Representative tracings of peak I_Ca, at +10 mV, obtained in a single cell before and after the application of ET-1 (10 nM) in combination with RES-701 (1 µM) and after washout of the drugs. b) Current-voltage relationships in the absence and presence of ET-1 (10 nM) in combination with RES-701 (1 µM). Recordings were obtained at 180-s intervals. c) Comparison of percent changes, relative to the control, in peak I_Ca, for ET-1 in the absence and presence of RES-701 (1 and 10 µM). The blank bar is included for comparative purposes (fig. 1), whereas the shaded bars represent the change in peak I_Ca values from another group of cells (n = 10). Vertical lines are S.E.M. *P < .005 compared with peak I_Ca in the absence of drugs. RES represents RES-701.

ET-1 (10 nM) in combination with BQ-788 (1 and 10 µM) decreased (P < .05) the peak I_Ca amplitude (n = 6) to $-$ 2.13 ± 0.20 nAand $-$ 2.28 ± 0.2 nA, respectively, from a control value of $-$ 2.57± 0.27 nA (fig. 5, A and B). This decrease in current amplitudewas completely reversed upon washout ( $-$ 2.56 ± 0.23 nA). In comparisonwith the decrease in peak I_Ca amplitude produced by ET-1 alone,BQ-788 produced a concentration-dependent antagonism of the ET-1-induceddecrease in I_Ca (fig. 5C). BQ-788 at concentrations of 1 and 10µM, in combination with ET-1, decreased the peak I_Ca amplitudeby 17 ± 3% and 11 ± 3%, respectively, compared with the 34 ± 4%decrease produced by ET-1 alone.

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Fig. 5. Influence of the ET_B receptor-selective antagonist BQ-788 on the ET-1-induced decrease in I_Ca (N = 6) a) Representative tracings of peak I_Ca, at +10 mV, obtained in a single cell before and after the application of ET-1 (10 nM) in combination with BQ-788 at a concentration of 1 µM and after washout of the drugs. b) Current-voltage relationships in the absence and presence of ET-1 (10 nM) in combination with BQ-788 (1 and 10 µM). Recordings were obtained at 180-s intervals. c) Comparison of percent changes, relative to the control, in peak I_Ca, for ET-1 (10 nM) in the absence and presence of BQ-788 (1 and 10 µM). The blank bar is included for comparative purposes (fig. 1), whereas the shaded bars represent the change in peak I_Ca values from another group of cells (n = 8). Vertical lines are S.E.M. *P < .05 compared with peak I_Ca in the absence of drugs. $dagger$ P < .005 compared with peak I_Ca in the presence of ET-1.

ET_A/B receptor-non-selective antagonist in the presence of ET-1. ET-1 (10 nM), in combination with the ET_A/B receptor-non-selective antagonist PD145065 (1 and 10 µM), had no effect on theI_Ca (n = 8). Values of peak current amplitude in the presenceof ET-1, in combination with PD145065, were $-$ 1.98 ± 0.26 nA and $-$ 2.05 ± 0.30 nA at concentrations of 1 and 10 µM, respectively(fig. 6A) and were not changed from a control value of $-$ 2.11 ±0.29 nA. Hence, PD145065 completely inhibited the effect of ET-1alone on the I_Ca (fig. 6B).

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Fig. 6. The inhibitory effect of the ET_A/B receptor-non-selective compound PD145065 on the negative I_Ca response of ET-1 (N = 5) a) Current-voltage relationships in the absence and presence of PD145065 (1 and 10 µM) in combination with ET-1 (10 nM). Recordings were obtained at 180-s intervals. b) Comparison of percent changes, relative to the control, in peak I_Ca, for ET-1 (10 nM) in the absence and presence of PD145065 (1 and 10 µM). The blank bar is included for comparative purposes (fig. 1), whereas the shaded bars represent the change in peak I_Ca values from another group of cells (n = 8). Vertical lines are S.E.M. *P < .005 compared with peak I_Ca in the absence of drugs. PD145 represents PD145080.

Influence of the ET_B receptor subtype on the ET-3-induced increase in I_Ca. ET-3 (1 nM) in the presence of either BQ-788 or IRL-1038 (1 µM) did not alter the I_Ca from control values of $-$ 2.07 ± 0.11nA and $-$ 2.11 ± 0.15 nA, respectively (fig. 7). Both ET_B receptor-selectiveantagonists abolished the increase (26 ± 7%) produced by ET-3(1 nM) (fig. 2D). The combination of ET-1 and ET-3, at equimolarconcentrations of 10 nM, did not alter the I_Ca from a controlvalue of $-$ 2.20 ± 0.18 nA; that is, both the decrease producedby ET-1 (fig. 1) and the increase produced by ET-3 (fig. 2) werecompletely abolished.

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Fig. 7. Effects of ET-1 (10 nM), BQ-788 (1 µM) and IRL-1038 (1 µM) on the increase in peak I_Ca amplitude produced by ET-3 (10 nM). Peak I_Ca values at +10 mV were recorded before and after a 270-s exposure of the cells to ET-3, in combination with ET-1 (n = 10), BQ-788 (n = 5) or IRL-1038 (n = 8). Vertical lines are S.E.M. *P < .005 is the difference from control peak I_Ca. IRL-10 represents IRL-1038.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Both ET-1 and ET-3 have potent positive inotropic effects on cardiac tissues (Rubanyi and Polokoff, 1994). Although Ishikawaet al. (1988b) originally speculated that the positive inotropiceffect of ET-1 could be attributed to an increase in the I_Ca,subsequent studies have yielded conflicting findings. ET-1 hasbeen reported to increase (Lauer et al., 1992; Tong et al., 1995;Bkaily et al., 1995), to decrease (Tohse et al., 1990; Ono etal., 1994; Cheng et al., 1995) and even to have no effect on theI_Ca (Furukawa et al., 1992; Habuchi et al., 1992) in cardiac tissues.The decrease in I_Ca produced by ET-1 could be reversed by alteringthe experimental conditions to maintain elevated intracellularGTP (Lauer et al., 1992). Other investigators, however, foundthat ET-1 decreased the I_Ca even when GTP was added to the dialyzingpipette solution (Cheng et al., 1995). Recently, using the perforatedwhole-cell patch-clamp technique, we demonstrated that ET-1 increasesthe I_Ca at a concentration of 1 nM (Kelso et al., 1996). Thiseffect was reversed, in the same cells, at greater than nanomolarconcentrations, producing a decrease in current amplitude at concentrationsof 10 to 100 nM. This finding prompted us to investigate whethermultiple endothelin receptor subtypes were responsible for theeffects of ET isopeptides on the I_Ca.

Using the ruptured whole-cell patch-clamp technique, we found that ET-1, at a concentration of 10 nM, decreased the I_Ca by34 ± 4% from control values (fig. 1), which is in contrast toan increase of similar magnitude (32 ± 5%) produced by ET-3 (fig.2). Because ET-3 has been referred to as an ET_B receptor-selectiveagonist (Ono et al., 1994) it appeared that the ET_B receptor subtypemight be involved in the positive effect on the I_Ca (an increasein current amplitude), whereas the ET_A receptor subtype was likelyto be involved in the negative effect of ET-1 on the I_Ca (thedecrease in current amplitude).

PD155080 is a non-peptide receptor-selective antagonist that has high potency and selectivity similar to those of BQ-123 forthe ET_A receptor subtype (Doherty et al., 1995). Unlike BQ-123,the novel antagonist PD155080 has no effect on the I_Ca per se(Kelso et al., 1995b). PD155080 completely inhibited the decreasein I_Ca produced by ET-1 (fig. 3), which confirms that the ET_Areceptor subtype is involved in this response. Interestingly,washout of ET-1, in the presence of the antagonist, resulted ina consistent increase (~10%) in the I_Ca. Because the effects ofET-1 were only partially reversed, it is likely that the positiveeffect of the agonist, which is apparent at lower concentrations(Kelso et al., 1995b), is unmasked, possibly through its actionat a different receptor subtype. No such effect was observed usingthe ET_A/B receptor-non-selective antagonist PD145065. ET-1, incombination with PD145065, did not alter the I_Ca from controlvalues, nor was there any change in current amplitude after washoutof the compounds (fig. 6). Although these differences are inconclusive,it is possible that the peptide antagonist PD145065, like ET-1,is less readily removed from the receptors than PD155080 and that,therefore, incomplete washout of PD145065 would prevent the increasein current amplitude observed using PD155080.

The ET_B receptor-selective antagonist RES-701 (Tanaka et al., 1994) did not prevent the decrease in I_Ca produced by ET-1 (fig.4). However, the ET_B receptor-selective antagonist BQ-788 (Ishikawaet al., 1994) partially inhibited the ET-1-induced decrease inI_Ca in a concentration-dependent manner (fig. 5), which suggeststhat the agonist may be mediated, in part, through a BQ-788-sensitiveET_B receptor subtype insensitive to RES-701. Such a receptor subtypehas been described in vascular tissues (Sudjawaro et al., 1994).The ET_B receptor subtype that mediates vasorelaxation in vascularendothelium was observed to be pharmacologically different fromthe subtype that mediates vasoconstriction in smooth muscle, andthese subtypes have been tentatively termed ET_B1 and ET_B2, respectively(Douglas et al., 1994). Whereas BQ-788 appeared to inhibit bothET_B1 and ET_B2 with similar affinity, RES-701 inhibited only theET_B1 receptor-mediated response (Warner, 1994; Sudjawaro et al.,1994). It is possible that the I_Ca response in ventricular cardiomyocytesis mediated by a ET_B2 receptor subtype similar to that found insmooth muscle. However, it is more likely that BQ-788 partiallyinhibited the decrease in I_Ca produced by ET-1 as a result ofa lack of selectivity of the antagonist for the receptor subtypes.Although BQ-788 has been identified as a potent and selectiveET_B receptor antagonist (Ishikawa et al., 1994; Fukuroda et al.,1994), a recent report (Peter and Davenport, 1996) indicates thatBQ-788 has low affinity and little selectivity for the ET_B receptorsubtype in human ventricular tissue.

In contrast to ET-1, however, the positive effect of ET-3 appears to be mediated through the ET_B receptor subtype. BQ-788completely abolished the increase in I_Ca produced by ET-3, butthis response was also completely inhibited by IRL-1038 (fig.7). Although these opposing responses, produced by ET-1 and ET-3,are coupled to different receptor subtypes (ET_A and ET_B, respectively),it is clear that multiple mechanisms are involved in the actionsof the isopeptides on the I_Ca in ventricular cardiomyocytes. Itis interesting that the magnitude of the decrease and increasein I_Ca produced by ET-1 and ET-3, respectively, are similar. Cardiactissues have a dense population of endothelin receptors (Takaiet al., 1992); however, ventricular cardiomyocytes have a muchgreater proportion of ET_A receptor subtypes than ET_B receptorsubtypes.

The mechanisms responsible for these effects are unclear. Both ET_A and ET_B receptor subtypes can couple to phospholipase C(Vogelsang et al., 1994), resulting in the hydrolysis of phosphatidylinositolto produce inositol-1,4,5-triphosphate and 1,2-diacyl glycerol.The latter may play a role in activating voltage-dependent Ca⁺⁺ channels via activation of protein kinase C. However, inositol-1,4,5-triphosphatestimulates release of Ca⁺⁺ from the intracellular stores, resulting in an increase in intracellularCa⁺⁺. Elevated intracellular Ca⁺⁺ levels can inhibit ET-1-induced Ca⁺⁺ influx and therefore may explain the heterogeneity at differentconcentrations. ET-1 is also reported to inhibit the accumulationof cyclic AMP in adult cardiomyocytes (Jones, 1996), which woulddecrease the I_Ca as a consequence of reduced protein kinase A-dependentphosphorylation of sarcolemmal proteins. However, in other cellsystems ET-1 can stimulate cyclic AMP generation (Sokolovsky etal., 1994). ET-1 stimulates the formation of cyclic AMP in Chinesehamster ovary cells that express the ET_A receptor subtype alonebut decreases cyclic AMP levels in cells that express the ET_Breceptor subtype alone (Aramori and Nakanishi, 1992). It is possiblethat in cardiac cells, the negative effect on accumulation ofcyclic AMP is coupled to an ET_B2 receptor subtype, resulting ina decrease in the I_Ca. However, the positive effect on the I_Cais unlikely to be mediated by such a mechanism, because ET-1 hasbeen found to increase cyclic AMP levels only at picomolar concentrations(Sokolovsky et al., 1994).

In summary, the ET_A receptor subtype is coupled to a decrease in I_Ca, whereas the ET_B receptor subtype is responsible foran increase in I_Ca. A role for endothelin has been proposed ina variety of cardiovascular disorders, including myocardial infarctionand cardiac ischemia (Rubanyi and Polokoff, 1994; Warner, 1994).The ability to alter calcium homeostasis will influence such pathogenicstates. Indeed, suppression of the I_Ca because of elevated levelsof ET-1 is likely to be important in protecting against ventriculararrhythmias and myocardial Ca⁺⁺ overload. However, evidence for multiple receptor subtypes thathave opposing actions may have important implications for futuretherapeutic intervention.

	Acknowledgments

The authors thank the Medicinal Chemistry Department at Parke-Davis Pharmaceutical Division, Ann Arbor, Michigan, for thegenerous supply of compounds: BQ-788, PD155080 and PD145065.

	Footnotes

Accepted for publication April 8, 1998.

Received for publication January 26, 1998.

Send reprint requests to: Dr. E.J. Kelso, Department of Therapeutics and Pharmacology, The Queen's University of Belfast, Whitla Medical Building, 97 Lisburn Road, Belfast, BT9 7BL, Northern Ireland.

	Abbreviations

ET-1, endothelin-1; ET-3, endothelin-3; I_Ca, L-type calcium current; BQ-788, N-[cis-(2,6-dimethylpiperizinyl) carbonyl](4Me)LLeu-(1-methoxycarbonyl)DTrp-DNle; RES-701, Gly-Asn-Trp-His-Gly-Thr-Ala-Pro-Asp-Trp-Phe-Phe-Asn-Tyr-Tyr-Trp; PD155080, sodium 2-benzo[1,3] dioxol-5-yl-3-benzyl-4(4-methoxy-phenyl)-4-oxobut-2-enoate; PD145065, Ac(D-2-(10,11-dihydro-5H-dibenzo[a,d]cyclohepten-5-yl))Gly-LLeu-LAsp-LIle-LIle-LTrp.Na; IRL-1038, Cys-Val-Tyr-Phe-Cys-His-Leu-Asp-Ile-Ile-Trp; DMSO, dimethyl sulfoxide; EGTA, ethyleneglycol-bis(b-aminoethyl ether)-N,N,N',N'-tetraacetic acid.

	References

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