Role of intracellular Ca2+ and pH in positive inotropic response of cardiomyocytes to diacylglycerol

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Role of intracellular Ca²⁺ and pH in positive inotropic response of cardiomyocytes to diacylglycerol

Yeqing Pi and Jeffery W. Walker

Department of Physiology, University of Wisconsin, Madison, Wisconsin 53706

ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Diacylglycerol has been hypothesized to mediate the positive inotropic response of myocardium to the $alpha$ -adrenergic agonistsangiotensin II and endothelin. The mechanism of action of diacylglycerolwas examined here in adult rat ventricular myocytes by releasingdioctanoylglycerol (diC₈) intracellularly from a caged compoundwhile monitoring Ca²⁺ transients and pH with fluorescent indicators. DiC₈ caused athree- to fourfold increase in twitch amplitude and a twofoldincrease in the systolic Ca²⁺ transient. No other parameter was consistently influenced bydiC₈, including the kinetics of Ca²⁺ cycling, the Ca²⁺ content of the sarcoplasmic reticulum, or the myofilament Ca²⁺ sensitivity. DiC₈ also had no detectable effect on intracellularpH or Na⁺/H⁺ antiport activity. Consistent with this finding, the Na⁺/H⁺ exchange inhibitor N-ethylisopropyl amiloride was without effecton the positive inotropic response to diC₈. The marked enhancementof systolic Ca²⁺ by diC₈ suggests that the process of excitation-contraction couplingis an important and possibly preferred target of diacylglycerol-proteinkinase C signaling in myocardium.

excitation-contraction coupling; fluorescent indicators; ventricular cells; sodium/hydrogen antiport

	INTRODUCTION

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ACTIVATION OF protein kinase C (PKC) by diacylglycerol has been hypothesized to mediate the positive inotropic response ofmyocardium to the $alpha$ -adrenergic agonists angiotensin II and endothelin(28, 35). Phorbol esters have been useful in implicating PKCin the regulation of cardiac function (28, 35), but a clearpicture of the role of PKC has not emerged, in part, because thereare conflicting reports in the literature concerning the effectsof phorbol esters on ventricular tissues. Positive (24), negative(5, 15, 21, 42), and both positive and negative inotropy(38) have been described, and these differences cannot be attributedto age or species differences. Moreover, a number of investigatorshave suggested that the negative inotropic effects of phorbolesters are independent of PKC (38, 39). In an attempt to clarifythe role of PKC in ventricular muscle, we developed a method forcontrolled elevation of diacylglycerols within living cells usinglight activation of caged diacylglycerol (14). We observed forthe first time that the widely used short-chain analog dioctanoylglycerol(diC₈) is capable of initiating a strong positive inotropic effectin ventricular myocytes that is dose dependent, stereospecific,and blocked by PKC antagonists (26).

The magnitude of the response to photoreleased diC₈ rivaled the magnitude of the myocyte response to the $beta$ -agonist isoproterenol(26). The intracellular mechanisms underlying the $beta$ -adrenergicresponse have been well characterized and involve stimulationof Ca²⁺ influx via phosphorylation of the L-type Ca²⁺ channel (10, 13), stimulation of the sarcoplasmic reticulum(SR) Ca²⁺ pump via phosphorylation of phospholamban (17, 40), and desensitizationof the myofilaments to Ca²⁺ as a result of phosphorylation of troponin I (19). Thus regulationof excitation-contraction coupling, SR Ca²⁺ content, and myofilament properties all contribute to the cardiomyocyteresponse to $beta$ -stimulation. These changes can be mimicked by elevationof cAMP and stimulation of intracellular protein kinase A (PKA)(10, 13, 17, 40).

Diacylglycerol acting through PKC has been hypothesized to regulate some of these same processes such as L-type Ca²⁺ channel activity (8, 21), Ca²⁺ pumping (17, 31), and myofilament Ca²⁺ sensitivity (6, 12, 36). In contrast to the consensusthat exists for the mechanisms of the positive inotropic and lusitropicaction of PKA, regulation of contractile function by PKC is muchless clearly defined. In the present study, we took advantageof the robust positive inotropic response produced by photogenerationof diacylglycerol to characterize PKC-dependent mechanisms withgood signal-to-noise ratio in living cardiomyocytes. Reportedhere are results of measurements of intracellular Ca²⁺ and intracellular pH during this large enhancement of contractility.We found that the vast majority of the positive inotropic responseto diacylglycerol is attributable to enhancement of systolic Ca²⁺ as a result of stimulation of the process of excitation-contractioncoupling. Some of this work was presented in preliminary formto the Biophysical Society (27).

	MATERIALS AND METHODS

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All reagents were purchased from Sigma Chemical (St. Louis, MO) unless otherwise noted. Endothelin-1, ryanodine, 2,3-butanedionemonoxime (BDM), and NH₄Cl were prepared fresh in distilled water.Caffeine was prepared fresh in 1 mM Ca²⁺ Ringer buffer (see below). Caged diC₈ was the $alpha$ -carboxyl-2-nitrobenzylform synthesized and purified as previously described (14).Fura 2, fluo 3, and 2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluorescein(BCECF) were obtained in their acetoxymethyl ester (AM) formsfrom Molecular Probes (Eugene, OR). Ventricular myocytes wereenzymatically dissociated from adult male rats as previously described(26). The yield was ~1-3 × 10⁶ cells per heart, and >80% were rod-shaped and Ca²⁺ tolerant. CaCl₂ was added to Ca²⁺-free Ringer to achieve the indicated Ca²⁺ concentration. Ca²⁺-free Ringer buffer had the following composition (in mM): 125NaCl, 2 NaH₂PO₄, 5 KCl, 1.2 MgSO₄, 25 HEPES, 5 pyruvate, 11 glucose,and 0.001 insulin, and pH was adjusted to 7.4 with NaOH at roomtemperature.

Fluorescence measurements. Cells were loaded with fluorescent indicators in their AM forms. Fura 2-AM, fluo 3-AM, or BCECF-AM were separately added toa suspension of 2-3 × 10⁴ cells/ml to a final concentration of 2 µM and then incubatedfor 1 h at room temperature. Myocytes were then pelleted, washedtwice with 0.5 mM Ca²⁺ Ringer solution, and resuspended in the same solution at thesame cell density. Cells were then loaded with 700 µM caged diC₈for 30 min at room temperature as previously described (26)and then transferred to a chamber connected to a perfusion system.All measurements were performed with a DeltaScan D-140 MicroscopicPhotometer system (Photon Technology, Jersey City, NJ). Fura 2was excited at 340 and 380 nm, and fluorescence emission was monitoredat 510 nm. Fluo 3 was excited at 495 nm with emission at 525 nm.BCECF was excited at 499 and 441 nm with emission at 536 nm. Thedata sampling rate was 1,200 Hz for fura 2 and fluo 3 and 300Hz for BCECF. Data were collected, saved, and analyzed with aPentium personal computer using Felix software (Photon Technology).

Calibration of Ca²⁺ indicators in myocytes. Calibration of signals for conversion of fluorescence to free Ca²⁺ was carried out according to the methods described by Borzaket al. (3). Adult myocytes were individually calibrated insitu by sequential exposure to fura 2 or fluo 3 solutions. Fura2 solutions were as follows: solution I, 3 mM Ca²⁺ Ringer solution; solution II, solution I with 25 µM ionomycin;and solution III, solution II with 10 mM EGTA replacing CaCl₂.The ratio of 340/380 fluorescence (R) detected at 510 nm was convertedto free intracellular Ca²⁺ concentration ([Ca²⁺]_i) using the formula [Ca²⁺]_i = K_d(R $-$ R_min)/(R_max $-$ R), where K_d is the dissociation constant(224 nM), R_min is R in absence of Ca²⁺, and R_max is R at saturating Ca²⁺. Fluo 3 solutions were as follows: solution A, 1 mM Ca²⁺ Ringer solution plus 12.5 µM ionomycin; solution B, solutionA with 3 mM ZnCl₂ replacing 1 mM CaCl₂; and solution C, solutionB with 10 µM digitonin replacing ZnCl₂. The fluorescence (F) wasconverted to [Ca²⁺]_i using the formula [Ca²⁺]_i = K_d(F $-$ F_min)/(F_max $-$ F), where K_d = 400 nM and F_min and F_maxare minimum and maximum fluorescence, respectively.

Photolysis of caged diC₈ was initiated by a separate xenon arc lamp reflected off a DM-400 dichroic mirror and passed throughthe same epifluorescence light path as the fluorescence excitationbeam. Both beams were guided onto a dual-pass dichroic mirrorthat reflected 300- to 385-nm light and 480- to 500-nm light througha Nikon Fluor ×40 1.3 NA objective and onto the cell chamber.To evaluate bleaching of fura 2 fluorescence by the photolysisbeam, the individual signals arising from 340- and 380-nm excitationwere monitored before and immediately after 20 s of irradiationof fura 2-loaded cells by the photolysis beam. The standard 20-sphotolysis protocol had no detectable effect on 340- or 380-nmfura 2 fluorescence. To minimize the effects of fura 2 excitationon caged diC₈ photolysis, we limited fura 2 excitation to a maximumof 20 s for any given fluorescence measurement. In four cellsloaded with fura 2 and caged diC₈ and then exposed to the fura2 excitation protocol for 40 s, inotropic responses were minimal(<20% increase in twitch amplitude). Thus, with due care, fura2 can be used in conjunction with ultraviolet photolysis of cagedcompounds.

Calibration of BCECF in myocytes. BCECF calibration was carried out as described previously (3, 4) using the K⁺/H⁺ exchange activator nigericin to equilibrate intracellular andextracellular pH. At the end of each experiment, 1 mM Ca²⁺ Ringer solution was changed to calibration solution and signalswere recorded for three pH standards. Calibration buffers contained4 mM HEPES-KOH, 120 mM KCl, 0.5 mM EGTA, 5 mM pyruvate, 5.6 mMglucose, 10 mM K-ATP, and the ionophores nigericin (20 µM), ionomycin(4 µM), and carbonyl cyanide m-chlorophenylhydrazone (0.2 µM).pH was adjusted at room temperature with KOH or HCl to standardthe pH values 7.42, 6.62, and 7.23.

Twitch shortening. Electrical field stimulation was carried out in a custom-designed 200 µl Plexiglas chamber with a glass floor and two platinumelectrodes. The standard stimulation protocol was 0.4 Hz, 1 msduration, and 40 V with the use of a Grass SD9 stimulator (Quincy,MA) at 20-22°C. The chamber was mounted on a Nikon Diaphot invertedmicroscope. The myocyte image was created with transmitted lightfiltered to pass red light. A DM-600 dichroic mirror reflectedthe red light emerging from the output port up onto a Panasoniccharge-coupled device video camera. Individual cell length wasmonitored with a model VED 104 video edge detector and plottedon an X-Y plotter.

Statistics. Data are expressed as means ± SE. Statistical significance was tested with a Student's paired or unpaired t-test, and P <0.05was taken as significant.

	RESULTS

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Ca²⁺ transients. Figure 1 summarizes the effects of controlled release of diacylglycerol on electrically paced twitch amplitude and the correspondingintracellular Ca²⁺ transients measured with fluo 3. Release of sufficient diC₈ toincrease twitch amplitude by fourfold increased the Ca²⁺ transient amplitude by about twofold (Fig. 1A). The increaseof systolic Ca²⁺ developed in parallel with the increase in twitch amplitude (Fig.1B). Fluo 3 was chosen for these studies because it is excitedwith visible light, so its use eliminates potential cross talkbetween fluorophore excitation and photolysis of the caged compound.However, fluo 3 is not a ratiometric indicator, so it is susceptibleto artifacts that alter the effective dye concentration, suchas dye leakage or cell motion. To control for the effects of cellmotion, myocytes were incubated with 20 mM BDM after photoreleaseof diC₈. This treatment greatly reduced the extent of twitch shortening(by inhibiting actomyosin interactions), but the twofold increasein systolic Ca²⁺ was still observed (Fig. 1C).

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Fig. 1. Effects of dioctanoylglycerol (diC₈) on intracellular Ca²⁺ transients. A: representative traces from a single myocyte. Top traces: 3 control twitches are compared with 3 twitches 5 min after a 20-s pulse of diC₈ (inset shows time course of a representative twitch before and after diC₈ normalized to same amplitude). Bottom traces: corresponding fluo 3 fluorescence measurements in same cell (inset shows normalized Ca²⁺ transient time courses before and after diC₈). [Ca²⁺]_i, intracellular Ca²⁺ concentration. B: summary of changes in systolic and diastolic [Ca²⁺]_i caused by diC₈ pulses in 15 separate myocytes. Systolic Ca²⁺ increased on average from 300 to 600 nM (P < 0.01), but diastolic Ca²⁺ was not significantly elevated in this group of cells. Changes in twitch amplitude for same 15 cells are shown for comparison. Cell shortening averaged 6 µm in control and 19 µm in diC₈-treated cells, and average resting cell length was 110 µm. C: effects of cell movement on increase in systolic Ca²⁺ measured with fluo 3. BDM (20 mM) was used to reduce myocyte twitch amplitude by >80% (top traces), but effect of diC₈ to increase systolic Ca²⁺ was unchanged by BDM (bottom traces).

In other experiments the ratiometric indicator fura 2 was used. Results were similar to those obtained with fluo 3 (Fig. 2),further ruling out a significant influence of dye leakage andcell shortening on the fluorescence records. The extent to whichthe fura 2 excitation source photolyzed the caged compound aswell as the degree of bleaching of fura 2 by the photolysis beamwas also evaluated (see MATERIALS AND METHODS). We found suchcross talk to be minimal with the specific protocols used.

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Fig. 2. Effect of diC₈ on Ca²⁺ content of sarcoplasmic reticulum (SR). Measurements were performed on myocytes loaded with fura 2 and caged diC₈. Top: 2 basal Ca²⁺ transients were measured, and then electrical stimulation was halted for 20 s. A rapid brief pulse of 20 mM caffeine was applied onto cell surface to induce SR Ca²⁺ release. Bottom: same protocol was repeated after a 20-s pulse of diC₈ from caged diC₈. Top inset: superimposed caffeine transients before and after diC₈. Bottom inset: summary of SR Ca²⁺ content before and after diC₈ in 12 myocytes. Mean area under caffeine Ca²⁺-response curve was similarly unchanged by diC₈. Data are means ± SE.

In contrast to the consistent enhancement of systolic Ca²⁺ by diC₈, it was more difficult to characterize changes in diastolicCa²⁺ because there was considerable variability from cell to cell.Approximately one-half of the cells examined showed a significantincrease in diastolic Ca²⁺ and a corresponding decrease in resting cell length (e.g., Figs.1A and 4C), whereas the other one-half showed no change in eitherparameter (e.g., Fig. 1C). This variability appears to be intrinsicto the cell population because it was observed on each experimentalday and did not correlate with temperature, dye loading conditions,or time after myocyte isolation. It was also independent of theCa²⁺ indicator used. Cells derived from the left versus right ventricleor from different transmural regions of the heart may show a differentdiastolic response to diC₈.

One possible explanation for dramatic changes in systolic Ca²⁺ after diC₈ might be that the SR Ca²⁺ content increases (2). This occurs, for example, during $beta$ -adrenergicstimulation as a result of a dramatic enhancement of the rateof Ca²⁺ pumping (17). Figure 1A, inset, shows the time course of Ca²⁺ transients measured in the same cell before and after diC₈. Therewas no significant change in the overall duration of the transientsand no change in the rate of decay to baseline, suggesting thatCa²⁺ pumping is unaltered by diC₈ under these experimental conditions.Figure 2 shows the results of an experiment in which the caffeine-releasableCa²⁺ content of the SR was compared before and after diC₈. There wasno significant difference in the total fura 2 fluorescence signalproduced by rapid caffeine application between control cells andcells exposed to a level of diC₈ that increased the Ca²⁺ transient by more than twofold (Fig. 2).

Further information about SR Ca²⁺ content and Ca²⁺-handling kinetics was obtained by investigating the phenomenon of postrestpotentiation. Figure 3 shows a typical negative staircase in thetwitch and Ca²⁺ transient responses of a rat myocyte after a 2-min rest period.The first twitch is very large, and then subsequent twitches decreasein amplitude to a steady-state level that depends on the stimulationfrequency. Again, changes in systolic Ca²⁺ paralleled the twitch changes. This phenomenon is thought tobe due to a balance of Ca²⁺ leak and Ca²⁺ pump fluxes that causes the SR to be loaded during periods ofrest. Photorelease of diC₈ did not alter the maximum Ca²⁺ release or twitch response after the rest period, and diC₈ didnot alter the nature or kinetics of the negative staircase phenomenon(Fig. 3B). Thus there is no indication that Ca²⁺ pumping or SR Ca²⁺ content was changed significantly by this inotropic stimulus.

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Fig. 3. Simultaneous measurements of twitch contractions and fluo 3 fluorescence during postrest potentiation. A: original records of twitch contractions (top) and fluo 3 fluorescence (bottom) showing 2 steady-state twitches followed by a 2-min rest period (break), and then stimulation was resumed until steady state was reestablished. Left: control records. Right: records 5 min after a 20-s diC₈ pulse. B: time courses of recovery of twitch amplitude (top) or Ca²⁺ transient amplitude (bottom) during postrest potentiation before (control) and after diC₈. Each data point represents mean ± SE for at least 8 cells. Curves show fits to a monoexponential function as previously described (41), which gave apparent rate constants of 2.2 s¹ (control twitch amplitude), 1.8 s¹ (diC₈ twitch amplitude), 1.9 s¹ (control Ca²⁺ amplitude), and 2.0 s¹ (diC₈ Ca²⁺ amplitude). Errors in these values are estimated to be ±15%.

The principle change then appears to occur at the level of coupling electrical excitation to contraction. To test whetherthe enhancement of systolic Ca²⁺ after diC₈ was due to stimulation of the normal excitation-contractionmechanism or to mobilization of Ca²⁺ via a distinct pathway, we treated myocytes with the Ca²⁺ release channel blocker ryanodine. At 2 µM, ryanodine inhibitedboth basal systolic Ca²⁺ and the diC₈-stimulated systolic Ca²⁺ by 50%. At 6 µM, ryanodine inhibited both types of Ca²⁺ transients by 80%. Thus diC₈ appears to stimulate a ryanodine-inhibitableprocess consistent with diC₈ regulating the traditional excitation-contractioncoupling mechanism.

Ca²⁺ sensitivity of myofilaments. Another possible contributor to the positive inotropic action of diC₈ is an increase in the Ca²⁺ responsiveness of the myofilaments. The fact that the twitchamplitude increased by three- to fourfold, whereas the Ca²⁺ transient only increased by twofold, opens the possibility thatthe Ca²⁺ regulatory system is also more sensitive to Ca²⁺ after diC₈. However, it is also possible that changes in twitchshortening and free Ca²⁺ are not strictly proportional. To investigate Ca²⁺ sensitivity in living myocytes, we first examined the relationshipbetween free Ca²⁺ and twitch shortening during the large swings in these two parametersobserved during postrest potentiation. A comparison was then madebetween control and diC₈ treated cells using this relationship.In most myocytes (13 of 22), there was no detectable differencein the ratio of cell shortening to Ca²⁺ transient amplitude before and after diC₈ (Fig. 4A). In ~40%of myocytes (9 of 22), there was a small leftward shift in thisrelationship after diC₈ treatment (not shown). The direction ofthis shift was the same as that observed after treatment withendothelin (Fig. 4B). However, unlike the diC₈ response, the endothelinresponse was observed in all eight cells tested. The magnitudeof this effect was also at least twofold greater in response toendothelin than to diC₈.

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Fig. 4. Effects of diC₈ on myofilament responsiveness to Ca²⁺. A: relationship between cell twitch amplitude and intracellular Ca²⁺ amplitude in a control cell derived by plotting values obtained during postrest potentiation experiments as in Fig. 3. Twitch and Ca²⁺ transient amplitudes were normalized to their respective maxima. The cell was then exposed to a 20-s pulse of diC₈, and the new relationship between twitch amplitude and Ca²⁺ transient amplitude was derived in the same manner. B: relationships between twitch amplitudes and intracellular Ca²⁺ amplitude before (control) and after 10 nM endothelin (ET). Lines in A and B represent linear regressions. C: plane loops for cell length versus free Ca²⁺ phase in a myocyte before diC₈ (control) and at various times after exposure to diC₈. Dotted line is shown to help visualize relengthening trajectory.

It has been argued that a plot of peak shortening versus peak Ca²⁺ transient is an imperfect measure of myofilament Ca²⁺ dynamics because Ca²⁺ binding does not reach an equilibrium at this point in the twitch(34). A better assessment of myofilament Ca²⁺ responsiveness may be obtained by examining the relengtheninglimb of cell length versus free Ca²⁺ phase in a plane diagram. It is during the relengthening (relaxation)phase of the twitch that Ca²⁺ binding to the myofilaments may achieve a quasi-equilibrium (34).A plot of cell length versus intracellular free Ca²⁺ shows characteristic phase-plane loops in which the relengtheninglimb of the loops occurred along a common trajectory. The positionof this relengthening trajectory is a measure of responsivenessof the myofilaments to Ca²⁺ (34), and this trajectory did not change in response to diC₈(Fig. 4C). For the cell shown in Fig. 4C, a significant increasein diastolic Ca²⁺ was observed after exposure to diC₈. Interestingly, the new startingposition at the lower left of each loop (representing diastolicCa²⁺ and diastolic cell length) also moved along this common trajectory.Thus there was little evidence for a consistent increase or decreaseof the myofilament responsiveness to Ca²⁺ after exposure of these intact, electrically stimulated myocytesto diC₈.

The enhancement of contractility by diC₈ was also blocked by the actomyosin ATPase inhibitor BDM (Fig. 1C). The concentrationfor 50% inhibition was ~8 mM BDM in both control and diC₈-stimulatedmyocytes. This observation indicates that BDM inhibits controland diC₈-stimulated twitches proportionately and that diC₈ didnot alter how BDM interacts with the filaments. That myofilamentproperties were altered in at least subtle ways is suggested bythe observation that the time course of the twitch was abbreviatedafter diC₈ treatment (Fig. 1B, inset).

Intracellular pH. The positive inotropic actions of a number of agonists in the heart appear to be correlated with an intracellular alkalinization(11, 16, 18, 29). To assess the contribution of pH changesto the mechanism of diC₈ action, we measured intracellular pHwith the fluorescent indicator BCECF. Intracellular pH was typically~7.1-7.2 before photorelease of diC₈, and it did not change significantlyunder conditions in which diC₈ caused a fourfold increase in twitchamplitude (Fig. 5A). The primary mechanism underlying alkalinizationis thought to be an increase in activity of a sarcolemmal Na⁺/H⁺ exchanger (11, 16, 18, 24, 29, 32). We also measuredthis activity directly by determining the rate of recovery ofpH from an acid load (24). First, it was confirmed in theseexperiments that the pH recovery process was virtually completelyinhibited by the amiloride analog N-ethylisopropyl amiloride (EIPA)(not shown), consistent with this intracellular pH change beingmediated by the Na⁺/H⁺ exchanger. Figure 6A shows that diC₈ did not accelerate the recoveryfrom an acid load, indicating that diC₈ did not stimulate Na⁺/H⁺ exchange activity. The change in Na⁺/H⁺ exchange activity measured in this way averaged $-$ 12 ± 13% (n= 6) after diC₈. Further control experiments showed that regulationof the exchanger was normal in these cells because treatment withendothelin-1 resulted in a measurable alkalinization (Fig. 5B)that was blocked by EIPA (Fig. 5C). Endothelin-1 also stimulatedexchange activity by 125 ± 42% (n = 4) (Fig. 6B), consistent withprevious reports of stimulation of the Na⁺/H⁺ exchanger by agonists (11, 16, 18, 29).

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Fig. 5. Measurements of intracellular pH (pH_i) in electrically paced myocytes. A: a myocyte was stimulated by photorelease of diC₈ (arrow) during a continuous recording of 2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluorescein (BCECF) fluorescence. N-ethylisopropyl amiloride (EIPA; 5 µM) perfusion had no detectable effect on this response. Similar results were obtained in 7 cells. B: a myocyte was perfused with 10 nM ET (horizontal bar) with continuous recording of BCECF fluorescence. Average pH change was 0.21 ± 0.06 (n = 5). C: experiment in B was repeated but with 5 µM EIPA (lower horizontal bar) applied by perfusion. Upper horizontal bar represents perfusion with ET. Similar results were obtained in 5 cells.

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Fig. 6. Measurements of Na⁺/H⁺ antiport activity. pH_i was monitored by BCECF fluorescence. Bars indicate times of exposure of myocytes to 10 mM NH₄Cl to induce an acid load (downward pH deflection). Initial rate of recovery (solid line) was taken as a measure of Na⁺/H⁺ antiport activity. A: Na⁺/H⁺ antiport activity before and after diC₈ (arrow) treatment. Mean change in initial rate of recovery for 6 cells was a 12 ± 13% decrease. B: Na⁺/H⁺ antiport activity before and after 10 nM ET treatment (bar). Mean change in recovery rate for 5 cells was a 125 ± 42% increase.

To rule out the possibility that the effects of diC₈ on Na⁺/H⁺ exchange and intracellular alkalinization escaped detection byBCECF because changes were either too small or too localized,we carried out further experiments with the Na⁺/H⁺ antiport inhibitor EIPA. Blockade of Na⁺/H⁺ antiporter activity with EIPA was without effect on the positiveinotropic response to diC₈ (Fig. 7A). Therefore, the positiveinotropic response did not require Na⁺/H⁺ antiport activity. In contrast to the effects of EIPA on diC₈responses, the response to endothelin-1 was reduced by ~50% inthe presence of EIPA (Fig. 7B). Overall, both the exchanger andits inhibitor behaved as expected in control experiments. We concludethat under conditions in which diC₈ gave rise to a large positiveinotropic effect, diC₈ did not activate the Na⁺/H⁺ exchange mechanism and therefore did not cause intracellularalkalinization that could influence myofilament function.

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Fig. 7. Effects of Na⁺/H⁺ exchange inhibitor EIPA on positive inotropic responses to diC₈ and ET. A: summary of intracellular Ca²⁺ transients (systolic and diastolic [Ca²⁺]) measured with fluo 3 and twitch responses (cell shortening) to diC₈ showing effects of EIPA. EIPA (5 µM) was applied by perfusion at 5 min (horizontal bar). B: summary of twitch responses to 10 nM ET (lower horizontal bar) showing effects of EIPA. EIPA (5 µM) was applied by perfusion at 5 min (upper horizontal bar). Error bars represent SE for a minimum of 5 separate cells. * Significant difference (P < 0.05).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Two well-established mechanisms for increasing the contractility of cardiac muscle are an increase in systolic Ca²⁺ and an increase in responsiveness of the myofilaments to Ca²⁺ (9). Under the conditions of our experiments, the positiveinotropic response to diacylglycerol can be accounted for by anincrease in the magnitude of the systolic Ca²⁺ transient. Diacylglycerol did not consistently alter the myofilamentresponsiveness to Ca²⁺. The Ca²⁺ transient can be influenced by the degree of Ca²⁺ loading in the SR (2), but we found no evidence that the SRwas "superloaded" with Ca²⁺ as a result of diacylglycerol treatment. Another possibilityis that diacylglycerol/PKC stimulated L-type Ca²⁺ channel activity. This channel is a major player in cardiac excitation-contractioncoupling, and its activity has been shown to be stimulated byagonists that elevate diacylglycerol (8). Moreover, both the $alpha$ - and $beta$ ₂-subunits of the cardiac L-type channel have been shownto be good substrates for PKC in vitro (30). The effects ofPKC phosphorylation on this channel, however, have been difficultto pin down. Most investigators report inhibitory effects of phorbolesters and diacylglycerol analogs on cardiac L-type channel activity,but these may be PKC independent (7, 33). Other investigatorshave reported stimulatory or biphasic effects of PKC activatorson voltage-gated Ca²⁺ channel function in ventricular tissue (8, 21).

Another candidate protein that could be influenced by diC₈ is the SR Ca²⁺ release channel/ryanodine receptor. This channel has been shownto be regulated by phosphorylation (23), but evidence for regulationby PKC phosphorylation is sparse. Other possibilities includecardiac K channels, which have been shown to be regulated by PKCactivators under various conditions (1, 25). A likely candidateis the transient outward K channel, whose inhibition by PKC activatorsprolongs the action potential (1), which in turn increasesthe duration of transarcolemmal Ca²⁺ influx. This is typically associated with an increase in durationof the twitch and the Ca²⁺ transient, but we did not observe such increases after photoreleaseof diC₈. At present we cannot distinguish among these three moleculartargets (L-type Ca²⁺ channels, ryanodine receptors, or K channels) with any degreeof certainty, so we lump them together as changes in excitation-contractioncoupling.

Another major control mechanism shown to occur under both physiological and pathological conditions is alteration of myofilamentsensitivity to intracellular Ca²⁺ (9, 11, 12, 18, 29). We employed methods developedby Lakatta and co-workers (34) to assess dynamic interactionsbetween intracellular Ca²⁺ and shortening myofilaments, and we found that diC₈ caused nochange in this interaction. A similar lack of an effect of diC₈on myofilament Ca²⁺ sensitivity was reported in a study using force-pCa measurementsin skinned myocytes that had been treated with diC₈ before skinning(22). However, using similar approaches, other groups have detectedan increase (36) or a decrease (12) in Ca²⁺ sensitivity after treatment with PKC activators. In none of theseexperiments was the inotropic response to the activator measuredin parallel. In skinned cells or reconstituted myofilaments, treatmentwith exogenous PKC has consistently failed to enhance the myofilamentCa²⁺ sensitivity (37) unless myosin light chain kinase was alsopresent (6). In experiments analogous to ours in intact myocytes,Capogrossi et al. (5) reported a negative inotropic responseand either no change or an increase in myofilament Ca²⁺ responsiveness after diC₈. The cause of the variability was notidentified. Therefore, although we cannot completely rule outthe possibility that activation of PKC under some conditions increasesmyofilament Ca²⁺ sensitivity, in many cells we observed a very large positiveinotropic response without such a change in Ca²⁺ responsiveness.

To further investigate this important issue, we examined the involvement of another possible target of PKC, namely the Na⁺/H⁺ exchanger. PKC regulation of Na⁺/H⁺ exchange is controversial. It has been demonstrated in many celltypes that the growth factor-regulated Na⁺/H⁺ exchanger (NHE-1) is activated by growth factors and phorbolesters in a PKC-dependent manner (32). Sequence analysis ofthe NHE1 gene however, has revealed no phosphorylation sites forPKC, although sites are present for other kinases. This has ledto the proposal that PKC activates the exchanger indirectly forexample by activating a kinase cascade. In ventricular tissue,several groups have provided evidence of activation of Na⁺/H⁺ antiport by phorbol esters (24, 28). Growth factor-stimulatedalkalinization in the heart has also been blocked by PKC inhibitors.However, these findings have not been confirmed in all cases (29).Our results do not resolve this controversy, but they do showthat, under conditions in which diacylglycerol produces a dramaticinotropic response, in some ways mimicking agonist responses (26),the Na⁺/H⁺ exchanger is not activated. It is possible that diC₈ is compartmentalizedunder our experimental conditions so that certain natural PKCtargets are not accessible to the signal. We consider this unlikelybecause the levels of caged compound in the cell are substantial,the levels of diC₈ produced are at the high end of the physiologicalrange (26), and diC₈ is known to readily diffuse in aqueousand membrane environments (14). Our results suggest that diC₈alone is not sufficient to stimulate the Na⁺/H⁺ exchanger in ventricular tissue.

Cardiac cross-bridge kinetics is another factor that has been reported to be regulated by PKC phosphorylation. These conclusionswere derived from measurements of myosin ATPase activity (37)or myocyte shortening velocity (22), two parameters that werenot evaluated here. We did not detect a significant change inthe time course of the cardiac twitch, which may be sensitiveto changes in cross-bridge kinetics, although this latter pointis still under debate. It is also not clear how changes in cross-bridgekinetics might contribute to inotropism in cardiac muscle, althoughit has been suggested that PKC-mediated inhibition of cross-bridgekinetics may underlie negative inotropic effects (37).

In view of the relatively large number of cardiac proteins suggested to be substrates for, or under the control of, PKC (28,35), our observation that diacylglycerol predominantly influencesone measurable parameter in intact myocytes is surprising. Reasonsfor the unusual selectivity afforded by this experimental approachare currently unknown. The ability to precisely control diacylglycerolconcentration may be one factor. This selectivity may also bedue to the species of diacylglycerol used, although there is noindication from in vitro studies that diC₈ is selective for onePKC isoform or directs PKC to a particular substrate or sequencemotif. The observed selectivity does indicate that certain PKCsubstrates are preferred over others; in this case, the preferredsubstrates appear to be proteins involved in excitation-contractioncoupling. The selective action of diacylglycerol on myocyte functioncontrasts with the pleiotropic effects of agonists that activatephospholipases C and/or D (8, 9, 16, 28, 35, 36).This is an indication that diacylglycerol/PKC signaling in cardiactissue represents only a part of the complex signaling that occursdownstream of receptor occupation by agonists.

In summary, many cellular processes have been hypothesized to be regulated by PKC in cardiac muscle, including Ca²⁺ channels, K channels, the SR Ca²⁺ pump, the Na⁺/H⁺ exchanger, and the myofilament Ca²⁺ regulatory system. Under conditions in which the diacylglycerolanalog diC₈ produced a large positive inotropic effect in isolatedrat ventricular myocytes, the only significant and consistentchange we detected was an increase in systolic Ca²⁺. Because the SR Ca²⁺ load did not change, these observations suggest that cardiacexcitation-contraction coupling is a major locus of regulationby PKC. Details of the molecular mechanism such as the isoformof PKC responsible and the target cardiac proteins involved remainto be determined.

	ACKNOWLEDGEMENTS

The authors thank Dr. R. Sreekumar for the synthesis and purification of caged diC₈ and Drs. Sreekumar, XuPei Huang, J. R.Patel, Marion Greaser, Hector Valdivia, and Richard Moss for helpfuldiscussions.

	FOOTNOTES

This work was supported by National Heart, Lung, and Blood Institute Grant P01-HL-47053 and National Institutes of HealthResearch Career Development Award KO4-HL-03119. Y.-Q. Pi is aVisiting Scholar from Hunan Medical University, People's Republicof China, supported by a postdoctoral fellowship (no. 9704656A)from the American Heart Association, Wisconsin Affiliate.

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate this fact.

Address for reprint requests: J. W. Walker, Dept. of Physiology, 1300 Univ. Ave., Madison, WI 53706.

Received 9 February 1998; accepted in final form 18 June 1998.

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