Carbachol promotes Na+ entry and augments Na/Ca exchange current in guinea pig ventricular myocytes

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Carbachol promotes Na⁺ entry and augments Na/Ca exchange current in guinea pig ventricular myocytes

Tomoaki Saeki, Jian-Bing Shen, and Achilles J. Pappano

Department of Pharmacology, University of Connecticut Health Center, Farmington, Connecticut 06030

ABSTRACT

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Abstract
Introduction
Methods
Results
Discussion
References

The effect of carbachol (CCh) on the Na/Ca exchange current (I_Na/Ca) was studied in voltage-clamped ventricular myocytes isolatedfrom guinea pig hearts and superfused with Tyrode solution at35°C. CCh (100 µM) increased outward current during depolarizations(10-200 ms) from $-$ 45 mV and tail current amplitude on repolarization;CCh had no effect on the L-type Ca²⁺ current. Amplitudes of the outward and tail currents declinedwith increasing duration of the depolarizing clamp pulse. Ouabainproduced similar current changes that are suppressed by intrapipetteethylene glycol-bis( $beta$ -aminoethyl ether)-N,N,N',N'-tetraaceticacid and are characteristic of I_Na/Ca. Depolarization from $-$ 80to $-$ 30 mV elicited the rapid Na⁺ current followed by a slowly decaying inward I_Na/Ca (J. C. Gilbert,T. Shirayama, and A. J. Pappano. Circ. Res. 69: 1632-1639, 1991.)that was reversibly increased by CCh. Atropine (1-3 µM) preventedthe CCh effect. All procedures that suppressed I_Na/Ca also suppressedthe CCh effect. Sarcoplasmic reticulum (SR) Ca²⁺ release participated in generating I_Na/Ca because 10 mM caffeineor 1 µM ryanodine blocked I_Na/Ca and the effect of CCh. Rapidsuperfusion of 10 mM caffeine induced inward I_Na/Ca at $-$ 75 mV;a caffeine-induced charge transfer gives an SR Ca²⁺ content of 67 µM. CCh increased caffeine-induced current; SRCa²⁺ content rose to 98 µM. CCh also augmented the amplitude of steady-stateintracellular Ca²⁺ transients and contractions during a train of voltage-clamp pulses( $-$ 75 to 30 mV for 200 ms) at 1 Hz. CCh elevated intracellularNa⁺ (M. Korth and V. Kühlkamp. Pflügers Arch. 403: 266-272, 1985)by inducing a background Na⁺ current [K. Matsumoto and A. J. Pappano. J. Physiol. (Lond.)415: 487-502, 1989]. Together with these data, the present resultsare consistent with the hypothesis that CCh, via muscarinic receptors,eventually promotes I_Na/Ca at the sarcolemma through a mechanismthat requires the SR and that this action accounts for the increasedcontractions.

caffeine-induced current; muscarinic agonist; ouabain; sarcoplasmic reticulum

	INTRODUCTION

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MUSCARINIC-RECEPTOR (mAChR) agonists inhibit the heart via a signal transduction mechanism that requires pertussis toxin (PTX)-sensitiveG proteins (reviewed in Ref. 21). In the presence of PTX, agonistoccupancy of the mAChR stimulates the rate and force of heartcontractions when applied at concentrations greater than thosethat cause inhibition (21). However, PTX treatment is not essentialto reveal stimulant effects. In guinea pig ventricular muscle,choline ester muscarinic agonists exert a positive inotropic effectin the absence of PTX treatment (10). In single guinea pig ventricularmyocytes, carbachol (CCh) induces a tetrodotoxin (TTX)-resistantNa⁺ current (I_Na) (15) and increases the extent of cell contractions(22). These effects of muscarinic agonist on membrane currentand cell contraction in ventricular myocytes also do not requirePTX treatment.

Muscarinic agonists per se do not increase the L-type Ca²⁺ current [I_Ca(L)] that initiates excitation-contraction coupling inheart cells (reviewed in Ref. 17). In the absence of PTX, CChincreased phasic contractions without increasing I_Ca(L) in electricallystimulated guinea pig ventricular myocytes (22). Therefore,the increase in contractions by muscarinic agonists is achievedby another mechanism. In guinea pig ventricular myocytes, muscarinicagonists increased the intracellular activity of Na⁺ (aⁱ_Na) (10). This effect, attributed toNa⁺ influx through TTX-resistant Na⁺ channels (15), could increase the subsarcolemmal Na⁺ concentration and promote reverse-mode Na/Ca exchange. In quiescentrat ventricular myocytes, CCh increased intracellular Ca²⁺ activity secondary to the increase in aⁱ_Na(11). Although the Na/Ca exchanger has been suggested to participatein the ionic changes caused by CCh (11), there is no directevidence for this mechanism in stimulated myocytes. If the CCheffect in stimulated myocytes also includes an action throughthe Na/Ca exchange, it should be possible to detect this by measurementof the exchange current (I_Na/Ca).

The I_Na/Ca has been measured under voltage-clamp conditions in which it has been related to contractions (reviewed in Ref.20). In our laboratory, I_Na/Ca was identified in guinea pigventricular myocytes in several ways (4). Depolarization to $-$ 40 mV from a more negative holding potential evokes an earlyinward tail current evident after I_Na decay. The early inwardtail current was not a slowly inactivating component of I_Na. Repolarizationto $-$ 40 mV from more positive potentials evokes a late inward tailcurrent. The early and late inward tail currents require externalNa⁺ and internal Ca²⁺ as expected for I_Na/Ca. Furthermore, the early and late tailcurrents are suppressed by agents (ryanodine, caffeine) that interferewith sarcoplasmic reticulum (SR) Ca²⁺ content and are augmented by inositol 1,4,5-trisphosphate [Ins(1,4,5)P₃],a Ca²⁺-mobilizing messenger (4). Altogether, the results are consistentwith a model in which entering Na⁺ that presumably accumulates in a subsarcolemmal space (2,14, 32) is exchanged with extracellular Ca²⁺ that enters the SR and thereby increases its content. The importanceof subsarcolemmal Na⁺ for the regulation of SR function via Na/Ca exchange has beendescribed (12, 19). In view of the results obtained by others(10, 11) and Matsumoto and Pappano (15), one might expectthat the muscarinic agonist increases I_Na/Ca in heart cells. Furthermore,there is reason to suppose that the depolarization-induced changesin I_Na/Ca involve an interaction between the plasma membrane andthe SR membrane. The present experiments were carried out to testthe hypotheses that CCh augments the I_Na/Ca in guinea pig ventricularmyocytes and that this involves the SR. A preliminary accountof some of these data has been presented in abstract form (22).

	METHODS

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Cell isolation. Hearts were rapidly excised from adult guinea pigs of either sex (300-500 g) that had been anticoagulatedwith heparin (1,000 U) and anesthetized with pentobarbital sodium(30 mg/kg) administered intraperitoneally. The heart was perfusedwith oxygenated Tyrode solution (37°C) for 5-10 min at a rateof 8-10 ml/min through the aorta in a Langendorff apparatus. Thecomposition of Tyrode solution was (in mM) 135 NaCl, 5.4 KCl,1.8 CaCl₂, 1.0 MgCl₂, 0.33 NaH₂PO₄, 10 N-2-hydroxyethylpiperazine-N'-2-ethanesulfonicacid (HEPES), and 20 dextrose (pH 7.4 adjusted with NaOH). Theenzymatic dissociation procedure was essentially the same as reportedpreviously (25). Enzyme-containing solution was washed out witha recovery solution composed of (in mM) 130 K aspartate, 5 K₂ATP,5 HEPES, and 20 dextrose (pH 7.4 adjusted with KOH). After theperfusion was completed and the ventricles were removed, the cellswere isolated by gentle mechanical agitation and kept in the recoverysolution at 4°C for at least 1 h. An aliquot of the cell suspensionwas placed in a 500-µl chamber mounted on the stage of an invertedmicroscope. After a 5- to 10-min settling period, the cells weresuperfused with Tyrode solution (dextrose was reduced to 10 mM)at 2-4 ml/min. All the experiments were done at 35 ± 1°C.

Electrophysiological techniques. The whole cell patch-clamp technique was used for the experiments. Electrodes, prepared fromborosilicate glass capillaries, had resistances of 1-3 M $Omega$ whenfilled with a pipette solution composed of (in mM) 120 K aspartate,30 KCl, 5 Na₂ATP, 5 HEPES, and 1 MgCl₂ (pH 7.3 adjusted with KOH).The pipette was connected through an Ag-AgCl wire to the headstage of a List EPC-7 amplifier (Medical Systems, Greenvale, NY).After a gigaohm seal between the membrane and the pipette tipwas formed, the cell membrane was ruptured by additional negativepressure. Voltage-clamp protocols were generated by pClamp software(Axon Instruments, Foster City, CA), and membrane currents werestored for later analysis. The protocols are described in RESULTS.

The amplitudes of the early and late inward tail currents were obtained by subtracting the steady current at the end (200ms) of the test potential (I_control) from that detected at 20ms after the inactivation of the rapid I_Na or the deactivationof the I_Ca(L), respectively. In some illustrations, the changein the tail current produced by CCh (I_CCh) or other agents isshown by the difference current (I_diff = I_CCh $-$ I_control).

Cell contraction. Contractions of single myocytes were evoked by a train of voltage-clamp pulses ( $-$ 75 to 30 mV for 200 ms)at 1 Hz. Because the cell shortens along its long axis, the displacementof one or both ends of the cell edge is an indicator of the extentof cell contraction. A video edge-detector system (Crescent Electronics,Sandy, UT) tracked cell edge movement. The cell image (magnified×400) was continuously observed on a high-resolution black-and-whitetelevision monitor via a sequential scanning video camera attachedto a side port of the microscope. The camera position can be rotatedto bring the video monitor raster lines parallel with the longaxis of the cell. The temporal resolution of this detector is16.7 ms, and motion as little as 0.1 µm can be detected. The signalfrom the detector is sent to a strip-chart recorder (Gould 2000)and to a videocassette recorder for storage and analysis.

Intracellular Ca²⁺ transients. The apparatus for measuring intracellular Ca²⁺ (Ca²⁺_i) is built around a Zeiss inverted microscope with a PTIDeltascan system. For this, ultraviolet light at 340 and 380 nmfrom a 75-W xenon arc lamp is selected by monochromators and alternatelypassed via a quartz fiber-optic bundle to the epifluorescenceport of the microscope. Excitation light is transmitted througha dichroic mirror (410 nm) and ×40 fluor objective (Nikon) ontoa myocyte in the test chamber loaded with fura 2 (50 µM, pentapotassiumsalt) for 5-10 min by dialysis from the patch pipette. Fluorescenceemitted from a cell region passes through the objective and a510-nm filter to a photomultiplier tube. Signals from the photomultipliertube are digitized and stored for later analysis. Ca²⁺_iis derived from the ratio of the fluorescence signals at the twoexcitation wavelengths, and its concentration is estimated froman in vitro calibration of a thin film of buffered Ca²⁺ solutions. The fluorescence ratio is corrected for backgroundautofluorescence, which is recorded with the patch pipette sealedto the membrane but before patch rupture.

Procedure. After membrane rupture, the voltage-clamp protocol to be used was applied at the indicated frequencies for at least5 min (control period). Thereafter, a CCh-containing solutionwas introduced for 3-5 min; a washout period of 5-15 min followedto test recovery. Cells that exhibited oscillations of membranecurrent (e.g., transient inward currents) or did not contractwere excluded. In some experiments with caffeine, the alkaloidwas applied to the myocyte by rapid superfusion from a reservoirvia solenoid-controlled delivery (27). The time for completesolution change, estimated from the membrane current responseto doubling the extracellular K⁺ concentration, was <1 s, with a half-time of ~120 ms. All drugsused in this study were obtained from Sigma Chemical (St. Louis,MO).

Data analysis. Experimental results are expressed as means ± SE. Student's paired t-test was used to evaluate the statisticalsignificance of the difference between means, with P < 0.05 takenas statistically significant.

	RESULTS

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Effects of CCh on plateau currents. In this series of experiments (n = 4), the membrane was clamped at a holding potentialof $-$ 45 mV that inactivated I_Na and the T-type Ca²⁺ current. The membrane was depolarized to +20 mV for various durationsat 0.1 Hz; records of a representative experiment in the absenceand presence of CCh are shown in Fig. 1A, top and middle, respectively.Although CCh had no effect on the peak inward current throughL-type Ca²⁺ channels, current during the pulse shifted in an outward direction,and the tail current on repolarization to $-$ 45 mV increased. TheCCh-induced current, obtained by digital subtraction, is a decliningoutward current during the voltage jump to +20 mV followed byan increased inward tail current elicited on repolarization to $-$ 45 mV (Fig. 1A, bottom). This pattern of currents is very similarto that described for I_Na/Ca by others (8). The results indicatethat 100 µM CCh promotes both the forward and reverse modes ofI_Na/Ca in guinea pig ventricular myocytes. In this regard, ouabainwas also tested because its inhibition of the Na-K pump raisessubsarcolemmal Na⁺ and increases I_Na/Ca. Results typical of four experiments withouabain are shown in Fig. 1B. Compared with control experiment(Fig. 1B, top), ouabain (Fig. 1B, middle) induced an outward currentduring depolarization and increased the amplitude of the inwardtail current on repolarization to $-$ 45 mV. The difference currentsfor ouabain (Fig. 1B, bottom) and CCh (Fig. 1A, bottom) are quitesimilar.

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Fig. 1. Time dependence of carbachol (CCh)-induced current (A) compared with that of ouabain-induced current (B) recorded in another cell. CCh (100 µM) or ouabain (1 µM) increased amplitude of late inward tail current. Test pulses to +20 mV from a holding potential of $-$ 45 mV were applied at durations of 10, 50, 90, 130, and 170 ms (A) and 15, 50, 85, 120, and 155 ms (B). Inset: protocol for clamp pulses ( $Delta$ t) that were applied every 10 s. A: top, control; middle, after 2 min in CCh; bottom, difference current (middle $-$ top). B: top, control; middle, after 3 min in ouabain; bottom, difference current (middle $-$ top). Short horizontal lines at left, zero-current level.

The voltage dependences of the plateau current in the absence and presence of CCh are shown in Fig. 2. The membrane was depolarizedto various potentials ranging from $-$ 40 to +50 mV in 10-mV stepsfor 25 ms at 0.2 Hz in the absence and presence of 100 µM CCh(Fig. 2A). The CCh-induced difference currect was obtained bydigital subtraction (Fig. 2A'). CCh (100 µM) reversibly increasedboth the outward current during the depolarizing pulse and theinward tail current elicited on repolarization to $-$ 45 mV. Similarresults were obtained with 1 µM ouabain (Fig. 2, B and B'). Inspectionof the current-voltage relationships (n = 4 cells) for the currentduring the depolarizing test pulse (Fig. 2C,a) and after repolarization(Fig. 2C,b) indicated that their voltage dependence was similarto that of I_Na/Ca (5, 8). The voltage dependence of theCCh-induced difference current during and after the depolarizingpulses is given in Fig. 2C,c. These results were not obtainedwhen the pipette solution contained 10 mM ethylene glycol-bis( $beta$ -aminoethylether)-N,N,N',N'-tetraacetic acid (EGTA) because I_Na/Ca was absentunder this condition (n = 3 experiments; data not shown).

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Fig. 2. Voltage dependence of CCh-induced current (A) compared with ouabain-induced current (B) from superimposed records of membrane currents elicited by a 25-ms depolarization to +50 mV from a holding potential of $-$ 45 mV in absence and presence of 100 µM CCh and 1 µM ouabain. Inset: pulse protocol that was applied every 5 s. A' and B': difference currents obtained from each experiment. C: voltage dependence of membrane current at end of depolarizing pulse (a), tail current on repolarization to $-$ 45 mV (b), and difference current (c) obtained by subtraction of control current ( $open circle$ ) from CCh current ( $bullet$ ). Amplitude of outward current was measured at end of pulse, and that of inward tail current was obtained by subtraction of current value at 200 ms after repolarization to $-$ 45 mV from that at 20 ms. Values are means ± SE; n = 4 experiments.

Effects of CCh on early and late tail currents. We used another protocol to study the Na/Ca exchanger; the procedures areessentially the same as reported previously by others (1, 12)and Gilbert et al. (4). Eight conditioning pulses ( $-$ 80 mV to+30 mV for 200 ms) were applied at 1 Hz to provide a constantSR Ca²⁺ load before each test pulse (Fig. 3A). The test pulse, delivered1 s after the conditioning pulse train, consisted of a 200-msstep to $-$ 30 mV from a holding potential of $-$ 80 mV, a second stepto +20 mV for 25 ms and sequential repolarizing steps to $-$ 30 and $-$ 80 mV. The sequence of conditioning plus test pulses was repeatedevery 10 s. The control responses of a myocyte to test pulsesafter the first and sixth conditioning trains are depicted inFig. 3B (trace 1). An early inward tail current of ~280 pA (openarrow) is evident after the decay of I_Na when a myocyte was depolarizedfrom $-$ 80 to $-$ 30 mV; this current decreased slowly over the next80-100 ms. A late inward tail current of ~280 pA (solid arrow)occurred on repolarization from +20 to $-$ 30 mV. After the sixthconditioning train, the amplitude of the early and late tail currentsincreased to ~470 pA. CCh (100 µM) increased the early inwardtail current after the first and sixth conditioning trains to~420 and 1,000 pA, respectively (Fig. 3B, trace 2). The I_Ca(L)did not change substantially in the presence of CCh, whereas therewas a tendency toward a small increase in the late inward tailcurrent (Fig. 3, B and C). Ten minutes after the washout of CCh,the amplitude of the early inward tail current returned to thecontrol value (Fig. 3, trace 3). The digitally subtracted differencecurrents (Fig. 3C) show that the increments of the early and latetail currents caused by CCh are greater after the sixth (right)than after the first conditioning train (left).

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Fig. 3. Effect of CCh on early (open arrows) and late (solid arrows) inward tail currents. A: voltage-clamp protocol consisting of a conditioning pulse train ( $-$ 80 to +30 mV for 200 ms at 1 Hz for 8 s) followed by test pulses that started from a holding potential of $-$ 80 mV, a 200-ms step to $-$ 30 mV, a second depolarization jump to +20 mV for 25 ms, and sequential repolarization jumps to $-$ 30 and $-$ 80 mV. B: representative records of transmembrane currents elicited by test voltage-clamp pulse protocol after 1st and 6th conditioning trains. Traces are control (1), after 2-min exposure to 100 µM CCh (2), and 5 min after washout of CCh (3). C: difference current obtained by digital subtraction (trace 2 $-$ trace 1). Short horizontal line at left, zero-current level.

In a series of five experiments, the amplitude of the early inward tail current in the control period increased progressivelyfrom the first (188 ± 35 pA) through the fifth train (344 ± 40pA) where it reached maximum. The late inward tail current alsoincreased with conditioning; it averaged 381 ± 30 and 453 ± 37pA after the first and sixth conditioning periods, respectively.In CCh, the early inward tail current increased to 443 ± 76 pAat the first test pulse and to 662 ± 102 pA at the sixth conditioningtrain; the difference (I_CCh $-$ I_control) was maximal after thesecond train. The CCh-induced increase in the early inward tailcurrent was significant (P $<=$ 0.02) at each test pulse number.In CCh, the late inward tail current averaged 475 ± 31 pA afterthe first and 486 ± 49 pA after the sixth conditioning periods;the small increase was not statistically significant. The I_Ca(L)during the test pulse after the first conditioning period (2.3± 0.37 nA) was not appreciably changed by the sixth conditioningtrain (2.3 ± 0.36 nA). There was no significant change in I_Ca(L)by CCh because I_Ca(L) averaged 2.3 ± 0.27 and 2.3 ± 0.26 nA afterthe first and sixth conditioning trains, respectively. In lightof previous reports (1, 4, 12), the early and late inwardtail currents are I_Na/Ca operating in the forward mode and dependenton release of Ca²⁺ from the SR (see below). The extra Na⁺ influx caused by CCh secondarily increases intracellular Ca²⁺ concentration ([Ca²⁺]_i) via Na/Ca exchange and eventually increases SR Ca²⁺ content. In this regard, the late inward tail current was notsignificantly increased by CCh, presumably because the Ca²⁺ store of the SR was not fully reprimed after discharge of theearly tail current.

The inward tail currents, as expected for I_Na/Ca, depended on [Ca²⁺]_i because neither was observed when 10 mM EGTA was present inthe pipette solution (5). Addition of CCh had no effect onthe tail currents under this condition (n = 3 experiments; datanot shown). We also confirmed that the inward tail current, likeI_Na/Ca, depended on the extracellular Na⁺ concentration with experiments in which Li⁺ was substituted for the extracellular Na⁺ (n = 4 experiments; data not shown). Li⁺ permeates voltage-gated Na⁺ channels but is unable to substitute for Na⁺ in the Na/Ca exchanger (1, 4, 5).

Na⁺ influx through fast Na⁺ channels is linked by Na/Ca exchange to SR Ca²⁺ content (27) and/or release (12, 14). Accordingly, theincreased Na⁺ entry by CCh through TTX-resistant channels (10, 15, 16)should also share this mechanism. We tested this hypothesis inexperiments with ryanodine, which interferes with the SR Ca²⁺-release channel. With the use of the same protocol as in Fig.3, the initial early I_Na/Ca (Fig. 4, trace 1) increased in thepresence of 100 µM CCh (trace 2). Five minutes after the additionof 1 µM ryanodine to the CCh-containing solution (Fig. 4, trace3), the early I_Na/Ca was less than the initial I_Na/Ca, indicatingthat not only the CCh effect but also the basal I_Na/Ca had beenaffected. Similar results were obtained in five other cells. Caffeine,which releases Ca²⁺ from the SR, reversibly eliminated the increases in the earlyand late I_Na/Ca induced by 100 µM CCh as well as those portionsof the currents present before CCh (n = 4 experiments; data notshown). Inhibition of the tail currents by caffeine or ryanodineis consistent with the hypothesis that these tail currents arisefrom Na⁺ influx through the Na/Ca exchanger and are secondary to releaseof Ca²⁺ from the SR.

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Fig. 4. Effect of ryanodine (1 µM) on tail currents from conditioning/test voltage-clamp protocol in Fig. 3. Trace 1: control membrane currents in response to clamp protocol illustrating early inward tail current (open arrow) of ~1 nA. Trace 2: after 2 min in 100 µM CCh, early tail current is increased to ~1.4 nA and late tail current (solid arrow) is essentially unchanged. Trace 3: addition of ryanodine on top of CCh reduces early tail current to ~0.4 nA, and late tail current is also decreased.

Concentration dependence and effect of atropine. In the concentration range from 10 to 100 µM, CCh increased the early tailcurrent amplitude by 43 ± 11, 134 ± 17, and 236 ± 32 pA at 10,30, and 100 µM, respectively (n = 5 cells at each concentration).The pharmacological nature of the CCh effect was evaluated inexperiments with atropine. The early inward tail current on thesixth test pulse (Fig. 5A) was increased in the presence of 100µM CCh (Fig. 5B). The change induced by CCh is shown by the differencecurrent (Fig. 5, B-A) which also indicates an declining outwardcurrent during the voltage step to +20 mV and a slightly increasedlate inward tail current on repolarization. After washout of CCh,3 µM atropine was applied; the early inward tail current or I_Na/Cawas unaffected by atropine (Fig. 5C). CCh had no effect on eitherthe early or late inward tail current or on the current at +20mV in the presence of atropine (Fig. 5, D and D-C). Similar resultswere obtained in five other experiments done with 1-3 µM atropine.

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Fig. 5. Atropine prevents CCh effect on tail current. Voltage-clamp protocol in Fig. 3 was used; all records were taken from 1 cell. A: control; early (open arrow) and late (solid arrow) tail currents are ~0.5 nA in amplitude. B: CCh (100 µM) increases amplitude of early and late tail currents to ~0.8 and 0.6 nA, respectively. Difference current (B $-$ A) shows magnitude of current changes induced by CCh. C: in presence of 3 µM atropine after washout of CCh, tail currents are at initial control values as in A. D: CCh was added on top of atropine; there is no change produced by CCh as indicated by difference current (D $-$ C).

Effect of CCh on caffeine-induced current. The evidence indicates that Ca²⁺ released from the SR participates in the I_Na/Ca and in the effectof CCh on it. If the action of CCh includes an eventual increaseof SR Ca²⁺ stores, the activation of I_Na/Ca would generate a larger current.We tested this hypothesis in experiments with caffeine. Rapidapplication of this alkaloid with the membrane voltage clampedat the resting potential releases Ca²⁺ from the SR and produces an inward current due to forward-modeNa/Ca exchange (18). The results of an experiment with caffeineare shown in Fig 6. A train of 20 conditioning depolarizing pulses( $-$ 75 mV holding potential to +30 mV for 200 ms at 1 Hz) was appliedevery 60 s. One second after the end of the conditioning pulsetrain, 10 mM caffeine was applied for 1 s. Caffeine induced aninward current of ~500 pA in the absence of CCh (Fig. 6A); thiscurrent developed more rapidly and increased to ~740 pA in thepresence of CCh (Fig. 6B). Ten minutes after the removal of CCh,the caffeine-induced current returned toward its initial value(Fig. 6C). In eight experiments of this type, the caffeine-inducedcurrent averaged 2.5 ± 0.56 pA/pF in control experiments, 3.2± 0.65 pA/pF in CCh experiments, and 2.5 ± 0.54 pA/pF after washout.The increase in the caffeine-induced current by CCh was statisticallysignificant (P < 0.01). Integration of the caffeine-induced currentgave estimated charge movements of 1.3 ± 0.16 pC/pF in the absenceof CCh. The charge movement increased significantly to 1.8 ± 0.24pC/pF in the presence of CCh (n = 8 experiments; P < 0.01).

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Fig. 6. CCh increases amplitude of caffeine-induced current. Protocol consisted of a train of 20 depolarizing voltage-clamp pulses at 1 Hz and a 1-s superfusion with 10 mM caffeine 1 s after last pulse of train (top). A: membrane current during last conditioning pulse followed by caffeine-induced inward current at $-$ 75 mV. B: in 100 µM CCh for 2 min. C: 10 min after washout of CCh. Calibrations are 400 pA for caffeine-induced currents and 1 nA for clamp currents.

In another series of experiments, we evaluated the effect of different CCh concentrations on the magnitude of the caffeine-inducedcurrent. The increments in the caffeine-induced current averaged43 ± 11 (n = 5 cells), 125 ± 17 (n = 3 cells), 216 ± 32 (n = 4cells), and 249 pA (n = 2 cells) in 10, 30, 100, and 300 µM CCh,respectively. No more than two CCh concentrations were testedin one cell. The results illustrate that the effects of the muscarinicagonist on I_Na/Ca, whether induced by caffeine or by depolarizingvoltage jumps, occur over the same concentration range.

Effect of CCh on contractions and Ca²⁺_i transients. A train of 200-ms voltage-clamppulses ( $-$ 75 to +30 mV) was applied at 1 Hz, with a rest intervalof 1 min between trains. The protocol was essentially the sameas that used in the experiments with caffeine (see Effect of CChon caffeine-induced current). A representative experiment is shownin Fig. 7A. The first contraction after the rest period had anamplitude of 2.8 µm, and the succeeding contractions displayeda positive staircase such that the steady-state shortening of6.1 µm on the last contraction in the train was about twice aslarge as the initial one (Fig. 7A, control). After 5 min in 100µM CCh (Fig. 7A, CCh), the first contraction after the rest intervalwas 4.4 µm, which is 1.57 times the control value. A positivestaircase ensued, and the last contraction in the train had adisplacement of 8.1 µm. The steady-state contraction in CCh was1.33 times that in the control experiment. Washout of CCh for6 min was accompanied by a reduction in the contraction amplitudeof corresponding contractions to about initial levels (Fig. 7A,washout). In the five experiments in this series, the steady-statecontraction in CCh (4.3 ± 1.13 µm) averaged 1.55 ± 0.25 timesthe control value (P = 0.03). The initial postrest contractionin CCh (3.0 ± 0.77 µm) was 1.44 ± 0.10 times the control value,but the change was not quite statistically significant (0.06 >P > 0.05). Altogether, the results indicate that the positivestaircase seen at 1 Hz was preserved in CCh, albeit with a greatersteady-state contraction amplitude, as expected for an agonistthat increased SR Ca²⁺ content.

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Fig. 7. CCh increases contraction amplitude (A), plateau current (B), and intracelluar Ca²⁺ transient (C) in guinea pig ventricular myocytes. Voltage-clamp protocol was the same as in Fig. 6. A: records taken from 1 myocyte showing staircase response to 1-Hz stimulation in control, after 5 min in CCh, and 10 min after drug removal (washout). B: records taken from another cell. At steady state, membrane current at +30 mV shifts outward in 100 µM CCh ( $bullet$ ) relative to control (left; 200-pA current calibration). Difference current (right; 70-pA current calibration) shows that CCh induced a slowly declining outward current during 200-ms jump to +30 mV. C: intracellular Ca²⁺ transients recorded from the same cell at steady state in control, after 5 min in 100 µM CCh, and 5 min after washout of agonist.

CCh also increased Ca²⁺_i transients under conditions where contractions were augmented. An example is shownin Fig. 7, B and C, from a myocyte subjected to a train of 21depolarizations at 1 Hz. In the steady state, the membrane currentduring a 200-ms voltage jump to +30 mV from a holding potentialof $-$ 75 mV shifted in the outward direction in the presence ofCCh (Fig. 7B, left). The record in Fig. 7B (right) shows the differencecurrent and indicates that the outward current induced by CChdeclined during the voltage jump. The Ca²⁺_i transientsfrom this cell are shown in Fig. 7C. From a basal level of 0.11µM, the Ca²⁺ transient reached a peak of ~1 µM (Fig. 7C, control). After 5min in CCh, the Ca²⁺ transient rose to ~1.4 µM from an initial level of 0.13 µM (Fig.7C, CCh). The Ca²⁺_i transient returned to initiallevels 5 min after CCh was removed (Fig. 7C, washout). Similarmeasurements were made in six additional cells. Basal [Ca²⁺]_i averaged 89 ± 15 nM (n = 7 cells) in the absence and 122 ±33 nM in the presence of 100 µM CCh. The small increase of 33± 20 nM did not attain statistical significance (P = 0.16). However,the peak [Ca²⁺]_i increased significantly by 182 ± 65 nM (from the control levelof 591 ± 118 to 773 ± 157 nM in CCh; P = 0.03).

	DISCUSSION

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Carbachol augments I_Na/Ca by an indirect action. Matsumoto and Pappano (15, 16) previously reported that CCh induces a TTX-resistant I_Na in guinea pig ventricular myocytes.Induction of this current confirmed a hypothesis for the mechanismby which choline ester muscarinic agonists increased intracellularNa⁺ in guinea pig papillary muscle (10). In this report, we testedthe hypothesis that by virtue of the effect on Na⁺ entry and accumulation, CCh should augment I_Na/Ca and that theSR participates in this action. The hypothesis for CCh actionis derived from a general scheme advanced by others (12, 19,20) and that Gilbert et al. (4) confirmed in a study on I_Na/Ca.Entering Na⁺ accumulates in a restricted subsarcolemmal space and providessubstrate to drive reverse-mode Na/Ca exchange. Evidence for restricteddistribution of intracellular Na⁺ has come from measurements of Na⁺-pump current (2) and from electron probe microanalysis inguinea pig ventricular myocytes (32). Ca²⁺ entering through reverse-mode Na/Ca exchange or retained by thecell as Na⁺ is extruded is taken up by and increases the SR Ca²⁺ content, from which it is released by I_Ca(L). Our hypothesisneither requires nor excludes that Ca²⁺ entering during reverse-mode Na/Ca exchange triggers SR Ca²⁺ release but simply that it increases the Ca²⁺ content of the SR.

Several lines of evidence from voltage-clamp experiments are consistent with the hypothesis for CCh action. The pattern ofCCh-induced "creep" current during depolarizing steps from $-$ 45mV is consistent with increased reverse-mode Na/Ca exchange. CChincreased not only the membrane currents during depolarizationfrom $-$ 45 mV but also the magnitude of the tail currents on repolarization.The voltage and time dependences of the CCh-induced current arecharacteristic of I_Na/Ca (6; reviewed in Ref. 20). Ouabain,an inhibitor of the Na-K pump, also induced the same pattern ofcreep and tail currents as CCh. Shen and Pappano (25) previouslyfound that ouabain increases both forward- and reverse-mode I_Na/Ca,an effect consistent with subsarcolemmal Na⁺ accumulation during Na-K pump inhibition (2). We assume thatCCh also raises subsarcolemmal Na⁺ when it increases intracellular Na⁺, although CCh does so by increasing a background I_Na (15) ratherthan by inhibiting the Na-K pump. The voltage dependence of theCCh-induced difference currents during depolarization and on repolarizationresembles that reported for the Na⁺ ionophore monensin, which increased I_Na/Ca in frog atrial myocytes(8), and that attributed to I_Na/Ca in rabbit ventricular myocytes(5).

Voltage-clamp test pulses elicited an early inward tail current after I_Na at $-$ 30 mV and a late inward tail current after I_Ca(L)(4). The early and late inward tail currents are sensitiveto procedures that modify I_Na/Ca and are increased by the agonistCCh. All of the procedures that interfered with the generationof I_Na/Ca in the absence of CCh also interfered with the stimulanteffect of CCh on this current. By interfering with SR Ca²⁺ storage and/or release (caffeine, ryanodine), the reaction isinterrupted and the subsequent inward tail current due to forward-modeNa/Ca exchange is prevented (Fig. 5). By chelating Ca²⁺, EGTA would suppress I_Na/Ca, whereas the reduction in I_Na/Cain Li⁺-rich bath solution is consistent with the failure of enteringLi⁺ to allow exchange with Ca²⁺ (1, 4). We propose that all the steps involved in regulatingNa/Ca exchanger activity operate at a greater subsarcolemmal Na⁺ because CCh initially promotes Na⁺ entry.

Participation of SR in CCh effect on I_Na/Ca. There are several reasons to implicate SR Ca²⁺ stores in the reaction mechanism that is influenced by CCh in addition to theevidence obtained with ryanodine or caffeine. The effect of conditioningwith depolarizing voltage-clamp pulses also agrees with the capacityof the SR to increase its store (4, 6, 12). Rapid applicationof 10 mM caffeine induced an inward current at a holding potentialof $-$ 75 mV. This current is attributed to forward-mode I_Na/Ca byvirtue of Ca²⁺ release from the SR (18). The size of the SR Ca²⁺ store can be estimated from the caffeine-induced charge movement(28). In the absence of CCh, the caffeine-induced charge movementamounted to 1.3 ± 0.16 pC/pF in cells in which the average capacitancewas 180 pF (n = 8). If a specific cell capacitance of 10⁶ F/cm² and a surface-to-volume ratio of 5 × 10³ cm¹ are assumed (9), the charge transported by the Na/Ca exchangerinvolves a Ca²⁺-release flux from the SR of 67 µM. In the presence of CCh, thecaffeine-induced charge movement rose to 1.8 ± 0.24 pC/pF, givingan estimated Ca²⁺ flux of 98 µM (an increase of 31 ± 7 µM; P < 0.01). These areunderestimates of SR Ca²⁺ content because the calculations neglect contributions of thesarcolemmal Ca²⁺ pump to Ca²⁺ extrusion. The caffeine-induced current of 2.5 ± 0.56 pA/pF is~36% greater than that reported in guinea pig ventricular myocytesby others (23). The experimental conditions are rather different(pipette Na⁺, temperature, bath composition) so that a strict comparison isnot warranted.

Earlier work by others helped to develop the hypothesis that implicated the Na/Ca exchange in the response to CCh. The initialaccumulation of intracellular Na⁺ (10) was succeeded by an increase in Ca²⁺_iin myocytes that were not electrically stimulated (11). In thelatter experiments, the increase in Ca²⁺_i didnot involve the SR because neither ryanodine nor caffeine interferedwith this action of CCh. Our experiments were done with myocytesstimulated by depolarizing voltage-clamp pulses. Under this condition,the relationship between the plasma membrane and the SR membranebecomes evident because the ability of depolarizing clamp stepsto elicit forward-mode I_Na/Ca requires a functional SR (6).In the absence of repetitive membrane depolarization, SR storesare not stimulated to release Ca²⁺ because the usual trigger via L-type Ca²⁺ channels is not activated.

The increase in I_Na/Ca by CCh, associated with an increased SR Ca²⁺ store, is accompanied by increases in the Ca²⁺_itransient and isotonic shortening. Altogether, these results indicatethat the stimulant effect of CCh arises from an increase in activatorCa²⁺ rather than in trigger Ca²⁺ via L-type Ca²⁺ channels. We found that CCh did not change I_Ca(L), thus excludinga change in this trigger as a source for the increased SR Ca²⁺ load. The ability of CCh to augment I_Na/Ca, Ca²⁺_itransients, and contractions agrees with the central role of subsarcolemmalNa⁺ in regulating cell contractions (6).

Concentration dependence and receptor. The effects of CCh on I_Na/Ca seen during and after voltage jumps and in the presenceof caffeine had a similar concentration dependence. The resultsindicate that the CCh effect occurs through low-affinity receptors.In the presence of atropine, the usual modulation of I_Na/Ca bythe magnitude, duration, and frequency of depolarizing pulsesoccurs. Although atropine had no effect on basal I_Na/Ca per se,it antagonized the effect of CCh on I_Na/Ca, indicating the muscarinicnature of the receptor (Fig. 6). Agonist occupancy of low-affinitymAChR increases aⁱ_Na (10) by activatinga TTX-resistant I_Na (15, 16). Action through a low-affinitymAChR also underlies the effect of CCh on the stimulation of contractionsin guinea pig papillary muscle (10) and in myocytes (22).

Does Ins(1,4,5)P₃ participate in CCh action on I_Na/Ca? Muscarinic agonists increase the synthesis of Ins(1,4,5)P₃, which is able to release Ca²⁺ from the SR in heart cells (4, 29). Ca²⁺ entering through reverse-mode Na/Ca exchange is said to triggerSR Ca²⁺ release (5, 12, 13, 31). Our experiments were not designedto evaluate the function of either messenger, which might servean ancillary role in the positive inotropic action of CCh becauseof the interaction between Ins(1,4,5)P₃ and Ca²⁺_i(30). Ca²⁺ entering through reverse-mode Na/Ca exchange, alone or togetherwith Ins(1,4,5)P₃, could sensitize SR Ca²⁺ release and increase the amplitude of I_Na/Ca that occurs withconditioning. If the fraction of SR Ca²⁺ released by Ins(1,4,5)P₃ was smaller than the increment causedby CCh through reverse-mode Na/Ca exchange, SR Ca²⁺ content could still increase but to a lesser extent than expected.This possibility could be tested by including an Ins(1,4,5)P₃-receptorantagonist in the pipette solution. There is evidence againsta direct stimulant action of Ins(1,4,5)P₃ on I_Na/Ca. In giantexcised membrane patches from guinea pig ventricular myocytes,phosphatidylinositol-4,5-bisphosphate (PIP₂), the precursor ofIns(1,4,5)P₃, promoted I_Na/Ca (7). When PIP₂ was metabolizedby its specific phospholipase C to Ins(1,4,5)P₃ or when phospholipaseC was activated by elevation of myoplasmic Ca²⁺, I_Na/Ca diminished. Although this does not necessarily mean thatIns(1,4,5)P₃ inhibits I_Na/Ca, it indicates that the preservationof PIP₂ is associated with a larger exchange current.

Comparison with an alternative mechanism. Our experiments demonstrating increased I_Na/Ca by CCh were done in the absence ofPTX because such treatment is not required to detect stimulationof contractions and of background I_Na by CCh (see introduction).We also found that the CCh-induced I_Na is independent of guaninenucleotides (26) and is initiated by M₂ mAChR occupancy (16),as is the stimulation of myocyte contractions (22). An alternativepathway for muscarinic signaling has been proposed in which PTXtreatment is required. In PTX-treated ventricular myocytes, CChis reported to increase I_Ca(L) (3). CCh also increases basaland peak [Ca²⁺]_i in rat ventricular myocytes treated with PTX (24). The increasedCa²⁺_i transient by CCh was tentatively linkedto the increased I_Ca(L), presumably by Ca²⁺-induced Ca²⁺ release. Both studies (3, 24) concluded that the PTX-insensitiveeffects of CCh are mediated by M₁ mAChR. Our results do not readilyagree with the alternative mechanism because our ability to detectstimulation of I_Na/Ca occurred without PTX treatment and withno change in I_Ca(L). Furthermore, the M₂ mAChR is most likelyinvolved (22).

Summary and conclusions. CCh, acting through an mAChR in guinea pig ventricular myocytes, promotes Na⁺ entry and eventually increases I_Na/Ca. These processes at theplasma membrane are linked by the SR inasmuch as the Ca²⁺ content of this organelle is increased by reverse-mode Na/Caexchange initiated by Na⁺ entry. The increased Ca²⁺ content of the SR is reflected by the greater magnitude of I_Na/Cagenerated either by depolarization or by caffeine and the occurrenceof larger Ca²⁺_i transients and contractions. Theseresults provide an explanation for the increased contraction ofthe ventricle by muscarinic agonists in the absence of PTX treatmentand without changes in I_Ca(L).

	ACKNOWLEDGEMENTS

We thank Rene Bumbera for expert secretarial assistance.

	FOOTNOTES

This work was supported by National Heart, Lung, and Blood Institute Grant HL-13339.

Address for reprint requests: A. J. Pappano, Dept. of Pharmacology, MC-6125, Univ. of Connecticut Health Center, Farmington, CT 06030.

Received 25 November 1996; accepted in final form 25 June 1997.

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