Effects of ACE inhibition and beta -receptor blockade on energy metabolism in rats postmyocardial infarction

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Effects of ACE inhibition and $beta$ -receptor blockade on energy metabolism in rats postmyocardial infarction

Stephanie Hügel, Michael Horn, Mark de Groot, Helga Remkes, Charlotte Dienesch, Kai Hu, Georg Ertl, and Stefan Neubauer

Medizinische Universitätsklinik, 97080 Würzburg, Germany

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Chronic treatment with $beta$ -receptor blockers or angiotensin-converting enzyme (ACE) inhibitors in heart failure can reduce mortalityand improve left ventricular function, but the mechanisms involvedin their beneficial action remain to be fully defined. Our hypothesiswas that these agents prevent the derangement of cardiac energymetabolism. Rats were subjected to myocardial infarction (MI)or sham operation. Thereafter, animals were treated with bisoprolol,captopril, or remained untreated. Two months later, cardiac functionwas measured in the isolated heart by a left ventricular balloon(pressure-volume curves), and energy metabolism of residual intactmyocardium was analyzed in terms of total and isoenzyme creatinekinase (CK) activity, steady-state levels (ATP, phosphocreatine),and turnover rates (CK reaction velocity) of high-energy phosphates(³¹P nuclear magnetic resonance) and total creatine content (HPLC).Bisoprolol and partially captopril prevented post-MI hypertrophyand partially prevented left ventricular contractile dysfunction.Residual intact failing myocardium in untreated, infarcted heartsshowed a 25% decrease of the total, a 26% decrease of MM-, anda 37% decrease of the mitochondrial CK activity. Total creatinewas reduced by 15%, phosphocreatine by 21%, and CK reaction velocityby 41%. Treatment with bisoprolol or captopril largely preventedall of these changes in infarcted hearts. Thus the favorable functionaleffects of $beta$ -receptor blockers and ACE inhibitors post-MI areaccompanied by substantial beneficial effects on cardiac energymetabolism.

adrenergic antagonist; angiotensin-converting enzyme inhibitors; infarction; remodeling; energy metabolism

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

THE PROGNOSIS of patients with heart failure remains poor, although chronic treatment with angiotensin-converting enzyme (ACE)inhibitors (8, 37, 42) and, more recently, $beta$ -receptor blockers(4, 6, 44) may reduce mortality. The mechanisms of theprotective effects of ACE inhibitors and $beta$ -receptor blockers areonly partially understood and are, almost certainly, complex andmultifactorial. One attractive hypothesis is that the failingheart is energy depleted (16, 19, 20, 30), and that thebeneficial functional effects of ACE inhibitors and $beta$ -receptorblockers are accompanied and possibly accounted for, by a preservationof energy metabolism. Although a large number of experimentalstudies have demonstrated the protective functional effects ofACE inhibitors and, to a lesser extent, of $beta$ -receptor blockersin heart failure models, only sporadic evidence exists on theenergetic effects of these compounds in heart failure (24, 36,45). The poor prognosis of patients with heart failure necessitatesthe search for novel therapeutic approaches, and the demonstrationof a protective effect of established heart failure drugs suchas ACE inhibitors or $beta$ -receptor blockers on energy metabolismmay fuel the search for therapies targeted more specifically tocellular systems involved in the regulation of energymetabolism.

The purpose of this study was thus to define the geometric, functional, and energetic cardiac effects of chronic treatmentwith the $beta$ -receptor blocker bisoprolol and the ACE inhibitor captoprilin a clinically highly relevant model of cardiac dysfunction,occurring postmyocardial infarction (MI) in the rat. Using a combinationof nuclear magnetic resonance (NMR) spectroscopy, high-performanceliquid chromatography (HPLC), and enzyme analysis, we define steady-statelevels, turnover rates, and free energy change of high-energyphosphates as well as tissue activities (V_max) of creatine kinase(CK)isoenzymes.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Animals and experimental MI. Infarcts or sham operations were performed in 12-wk-old Wistar rats kept in a 12:12-h light-darkcycle. Left coronary artery ligation (MI) was induced by a previouslydescribed technique (11, 35). A left thoracotomy was performedunder ether anesthesia and positive pressure ventilation. Theheart was rapidly exteriorized by applying gentle pressure onboth sides of the thorax. The left coronary artery was ligatedbetween the pulmonary outflow tract and the left atrium. The heartwas then replaced into the thorax, lungs were inflated by increasingpositive end-expiratory pressure, and the wound was closed immediately.Sham operation was performed using an identical procedure exceptthat the suture was passed under the coronary artery without ligation.Mortality rate of infarcted rats for the first 24 h after theoperation was 40-50%. Surviving rats were kept on commercial ratchow and water ad libitum. The investigation conformed with the"Guiding Principles for Research Involving Animals and HumanBeings."

Bisoprolol and captopril treatment and experimental groups. Rats were randomly assigned to one of six groups: untreated sham(sham, n = 9), untreated MI (MI, n = 8), bisoprolol-treated sham(sham-Biso, n = 13), bisoprolol-treated MI (MI-Biso, n = 6), captopril-treatedsham (sham-Capto, n = 11), and captopril-treated MI (MI-Capto,n = 6). After surgery, bisoprolol-treated groups received 60 mg· kg¹ · day¹ bisoprolol with the drinking water. Captopril was added to thedrinking water at 2 g/l. These concentrations were chosen becausethey were shown to exert a small but significant hemodynamic effect[10% reduction of blood pressure (captopril) or heart rate (bisoprolol)(3, 24)]. Because bisoprolol has a slightly bitter taste,5% glucose was added to the drinking water of all groups. Drinkingwater was freshly prepared every other day. Therapy was continuedfor 8 wk and was stopped 1 day before the isolated heartexperiment.

Isolated rat heart preparation. Eight weeks after the left coronary artery ligation or sham operation, rats were anesthetizedwith the injection of 50 mg pentobarbital sodium intraperitoneally.A transverse laparotomy and left and right anterolateral thoracotomywere performed, and the heart was rapidly excised and immersedin ice-cold buffer. The aorta was dissected free and mounted ontoa cannula attached to a perfusion apparatus, as previously described(2). Retrograde perfusion of the heart was begun in the Langendorffmode at a constant temperature of 37°C and at a constant coronaryperfusion pressure of 100 mmHg. A small vent made out of polyethylenetubing was pierced through the apex of the left ventricle to allowdrainage of flow from Thebesian veins. For control perfusion,phosphate-free Krebs-Henseleit buffer was used containing (mM)118 NaCl, 4.7 KCl, 1.75 CaCl₂, 1.2 MgSO₄, 0.5 ethylenediaminetetraacetatetetrasodium, 25.0 NaHCO₃, and 11.0 glucose. Equilibrating thebuffer with 95% O₂-5% CO₂ yielded a pH of 7.4. Coronary flow wascontinuously measured by an ultrasonic flow probe (Transonic Systems,Ithaca, NY) built into the perfusate inflow tubing. As previouslyshown (2), the perfusion system allowed maintenance of heartsin a steady state for at least 90 min with changes of <5% forall mechanical and metabolicparameters.

Cardiac performance measurements. A water-filled latex balloon was inserted into the left ventricle through an incision inthe left atrial appendage, via the mitral valve, and secured bya ligature. The balloon was connected to a Statham P23 Db pressuretransducer (Gould Instruments, Glen Burnie, MD) via a small-borepolyethylene tubing for continuous measurement of left ventricularpressure and heart rate on a four-channel recorder (Graphtec,Tokyo, Japan). Performance was estimated as the product of heartrate and left ventricular developed pressure (LVDP, mmHg/min).Frank-Starling curves were obtained by increasing the volume ofthe intraventricular balloon by 0.05-ml increments until LVDPreached amaximum.

³¹P NMR spectroscopy. The perfused hearts were placed into a 20-mm NMR sample tube and inserted into a probe seated in the bore of a superconductingsuperwide bore (150 mm), 7.05-Tesla magnet (Bruker, Rheinstetten,Germany) as previously described (30). Hearts were bathed intheir own perfusate, which was pumped from the NMR tube at a levelimmediately above the heart. An Aspect 3000 computer (Bruker)was used in the pulsed Fourier transform mode to generate ³¹P NMR spectra at 121.50 MHz. A 14-channel Shim Unit served tohomogenize the magnetic field. Single ("one pulse") spectra wereaccumulated over 5-min periods, and averaging data from 152 freeinduction decays were obtained using a pulse time of 37.6 µs,a pulse angle of 45°, and an interpulse delay of 1.93 s. The resonanceareas corresponding to ATP, phosphocreatine (PCr), and P_i, whichare proportional to the number of phosphorus atoms of the respectivecompound, were measured by integration using the NMR1 software(TRIPOS, Munich, Germany). Relative saturation factors for eachresonance were determined by comparing spectra to fully relaxedspectra obtained using a pulse angle of 45° and an interpulsedelay of 15 s; correction factors were 1.12 ± 0.03 for PCr and1.08 ± 0.05 for P_i (n = 15); spectra were corrected accordingly.Myocardial ATP content was found to be 28.3 ± 5.6 nmol/mg proteinin sham and 28.0 ± 3.0 nmol/mg protein in MI hearts by HPLC (30);the myocardial contents of the other metabolites were calculatedby multiplying the ratio of resonance area of metabolite to the[ $gamma$ -P]ATP area by 28.3 nmol/mg protein for sham and by 28.0 nmol/mgprotein for MI hearts. This assumes that neither bisoprolol norcaptopril affected normal ATP content, demonstrated before forsham-operated and infarcted hearts (30), which is most likelythe case. ATP could not be determined by HPLC in this study, becauseleft ventricles were fixed in Formalin for infarct size measurements,and right ventricles were cut off and frozen allowing determinationof total creatine and CK activity. ATP levels were not determinedin the right ventricle because we cut off the right ventriclefrom the beating heart and froze it after several seconds, becausefreeze-clamping the beating heart was impossible when we wantedto determine infarct size. In our experience, ATP levels cannotreliably be determined when tissue is not directly freeze-clamped.Intracellular pH (pH_i) was measured by comparing the chemicalshift between P_i and creatine phosphate with values obtained froma standard curve. The free cytosolic ADP concentration was calculatedby using [ATP], [PCr], and [H⁺] measured in the intact beating heart by ³¹P-NMR spectroscopy, and total creatine was measured chemicallyin the right ventricular homogenates by assuming that CK is inequilibrium and by using a CK equilibrium constant of 1.66 × 10⁹ M¹ (25, 43)

[ADP] = ([ATP][Cr]free)/([PCr][H+]1.66 × 109)

The free energy change of ATP hydrolysis ( $Delta$ G) was calculated as

&Dgr;<IT>G</IT> (kJ/mol) = &Dgr;<IT>G</IT>° + <IT>RT</IT> ln ([ADP][Pi]/[ATP])

where $Delta$ G° ( $-$ 30.5 kJ/mol) is the value of $Delta$ G under standard conditions of molarity, temperature, pH, and [Mg²⁺] (14); R is the gas constant (8.3 J/mol K); and T is the temperaturein Kelvin(K).

³¹P-NMR magnetization transfer measurements of CK kinetics. For magnetization transfer experiments, each broad-band pulse was preceded by a low-power, narrow-band pulse at the resonancefrequency of [ $gamma$ -P]ATP for 0, 0.3, 0.6, 1.2, 2.4, or 3.6 s as previouslydescribed (29, 30). Separate studies showed that the narrow-bandpulse directly attenuated the PCr magnetization by <5% when thecarrier frequency was placed 2.5 ppm downfield from the resonanceof PCr. For each of the six saturation transfer spectra, 64 scanswere accumulated by repetitively cycling through the six differenttimes of presaturation. Thus any metabolic deterioration occurringduring the saturation transfer measurement was equally distributedamong the spectra. A complete saturation transfer experiment wasacquired in 32 min. Stability of the preparation was assessedby comparing one-pulse spectra obtained before and after eachmagnetization transfer experiment. Magnetization transfer measurementsof the forward CK reaction phosphocreatine $right-arrow$ [ $gamma$ -P]ATP were analyzedaccording to the two-site chemical exchange model of Forsen andHoffman (9), providing estimates of the pseudo first-orderrate constant (k_for) and the intrinsic longitudinal relaxationtime for PCr (T₁). Briefly, as the time of saturation at [ $gamma$ -P]ATP,t, is increased from 0 to 3.6 s, the integrated signal intensityof the PCr resonance peak (M_t) decays from M₀ to M (definedas magnetization at zero and infinite saturation times, respectively)with a time constant $tau$ ₁ as

<IT>M</IT>t = <IT>M</IT>∞ + (<IT>M</IT>0 − <IT>M</IT>∞)<IT>e</IT>−<IT>t</IT>/&tgr;1

where

1/&tgr;1 = 1/<IT>T</IT>1 + <IT>k</IT>for

Nonlinear regression of PCr magnetization at different saturation times of [ $gamma$ -P]ATP was used to determine M₀, M, and $tau$ ₁. T₁ and k_for were then calculated by solving the equations

<IT>k</IT>for = (<IT>M</IT>0 − <IT>M</IT>∞)/(<IT>M</IT>0&tgr;1)

and

<IT>T</IT>1 = (<IT>M</IT>0 /<IT>M</IT>∞)&tgr;1

Multiplying the rate constant by substrate concentration yielded reaction velocity (2).

Biochemical measurements. Because biochemical measurements cannot be made in Formalin-pretreated hearts (necessary for histologicaldetermination of infarct size), right ventricles were separatedafter the NMR experiment and frozen in liquid nitrogen. We havepreviously shown that changes of total creatine and CK isoenzymeactivities in chronically infarcted hearts are similar for leftand right ventricles (23).

HPLC measurements. A piece of tissue (~10 mg) was separated with a Minimot 40/E drill (Proxxon, Niersbach, Germany) underliquid nitrogen and was analyzed for total creatine and totaladenine nucleotide (TAN) content as previously described (22,32). Briefly, the powder was homogenized in 0.42 N perchloricacid at 0°C, and an aliquot of the homogenate was removed forprotein determination. The homogenate was neutralized and centrifugedfor 5 min. The supernatant was used for measuring total creatineand TAN by HPLC as previously described. Noncollagen protein wasmeasured by the method of Lowry et al. (26). Metabolite concentrationswere expressed in millimoles perliter.

Enzyme analysis. From each sample, 5-10 mg of tissue were homogenized in 0.1 M K₂HPO₄ buffer, pH 7.4, containing 1 mM EGTA,1 mM $beta$ -mercaptoethanol, and 0.1% Triton X-100 at 4°C (final tissueconcentration 5 mg/ml). Before the addition of Triton, aliquotsfor measurements of protein and creatine content were taken. Allsamples were kept on ice. CK (39), citrate synthase (38),and lactate dehydrogenase (1) enzyme activities were measuredusing an Ultraspec III spectrophotometer (Pharmacia Biosystems,Freiburg, FRG). To measure the CK isoenzyme distribution the RapidElectrophoresis System (REP, Helena Diagnostika) as a separationunit and the REP CK Isoforms Kit (Helena Diagnostika) for agarosegel and incubation solution were used. The agarose gel containsa Tris-barbital buffer with sodium azide as a preservative. TheElectrophoresis Data Center (EDC, Helena Diagnostika) automaticallyquantified the separated isoenzymebands.

Experimental protocols. All hearts were given 10-15 min for stabilization where left ventricular end-diastolic pressure wasset to 10 mmHg by adjusting the balloon volume in the left ventricle.After baseline left ventricular pressures (mmHg), heart rate (beats/min),and coronary flow (ml/min) were recorded, and the balloon wasemptied. A left ventricular pressure-volume curve was performedby stepwise inflation of the balloon by 0.05 ml until maximumLVDP was obtained or until the end-diastolic pressure exceeded50 mmHg. Recordings of all parameters were made at each step whena new steady state was reached, which occurred within 2 min. Afteranother 15-min stabilization period (end-diastolic pressure setto 10 mmHg), a 5-min one-pulse spectrum was recorded. Thereafter,a set of six ³¹P NMR magnetization transfer spectra was recorded in 32 min. Aftera final one-pulse ³¹P NMR spectrum was obtained, the right ventricle was separatedand rapidly frozen in liquid nitrogen for HPLC and enzyme measurements,and the left ventricle was fixed in Formalin for determinationof infarctsize.

Determination of infarct size. The left ventricle was embedded in paraffin, and 20-µm sections were cut serially from theapex to the base of the heart. Sections were stained for collagenusing Picrosirius red stain. A sustained increase in collagencontent, measured as the Sirius red-positive area on each section,determines the infarct area. Slices were digitized by using theNIH Image 1.59/ppc scanner software (National Institute of Health,Bethesda, MD), and lengths of scar and noninfarcted muscle forboth endocardial and epicardial surfaces were determined by cursormeasurements for every section using the above software. The ratioof the lengths of scar and surface circumferences defined theinfarct size for endo- and epicardial surfaces, respectively.Final infarct size was determined as the average of endo- andepicardial surfaces and is given in percentage. Average infarctsize including all hearts was 29 ± 3% in the untreated, 27 ± 3%in the bisoprolol-treated, and 27 ± 4% in the captopril-treatedgroup. To test whether treatment with bisoprolol or captoprilaffects the remodeling process post-MI, all hearts with an infarctsize <30% were excluded from the analysis (untreated n = 12, bisoprololn = 11, and captopril n = 12) to ensure comparability of the infarctedgroups and to only include hearts where impairment of left ventricularmechanical functionoccurs.

Statistical analysis. All data are presented as means ± SE. With six experimental groups, 15 statistical comparisons are conceivable.Testing for this high number of comparisons with multifactorialANOVA would overcorrect significance levels. We therefore limitedthe statistical analysis by seven "biologically meaningful" comparisons:sham vs. MI, sham-Biso vs. MI-Biso, sham-Capto vs. MI-Capto, shamvs. sham-Biso, sham vs. sham-Capto, MI vs. MI-Biso, and MI vs.MI-Capto. Comparisons of variables between two groups were madeby using an unpaired Student's t-test. Bonferroni's correctionfor multiple comparisons was applied to yield a significance levelof 0.05:7 = 0.007. Calculations were performed by a commerciallyavailable program, StatView SE-Graphics (Brainpower, Calabasas,CA).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Heart weight, body weight, and infarct size. Table 1 shows infarct size, body weight, heart weight, heart-to-body weightratios, and left and right ventricular weight of the six groupsstudied. In the three infarcted groups, infarct size was ~40%of the left ventricular circumference and was not significantlydifferent. There was a tendency for body weight reduction in captopril-treated,sham-operated rats and in the bisoprolol-treated MI group. Withbisoprolol the increase in heart weight and left ventricular weight,which occurs in infarcted hearts, was no longer significant. Heartweight was substantially reduced in both sham-operated and infarctedcaptopril-treated rats. Infarction led to an increase in rightventricular weights, which was prevented by captopril (P < 0.007)but not significantly by bisoprolol.

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Table 1. Infarct size, body weight, heart weight, left and right ventricular weight, and their ratios for all experimental groups

Cardiac performance and pressure-volume relations. Table 2 shows heart rate, coronary flow, and LVDP of the six experimentalgroups, all recorded at an end-diastolic pressure of 10 mmHg.On average, heart rate was 273 ± 3 beats/min and was not significantlydifferent among groups. In contrast, LVDP was significantly reducedin chronically infarcted hearts (85 ± 11 vs. 135 ± 9 mmHg in sham,P < 0.007). Although treatment did not affect LVDP in sham-operatedhearts, bisoprolol completely and captopril treatment partiallyprevented the decrease of LVDP in infarcted hearts. Coronary flowwas 23 ± 1 ml/min on average and was not significantly differentamong groups.

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Table 2. Cardiac mechanical function and coronary flow for all experimental groups

Figure 1 shows pressure-volume relations for LVDP (Fig. 1A) and left ventricular end-diastolic pressure (Fig. 1B) in the sixgroups. The LVDP curve for the infarcted untreated group was shiftedto the right with a significantly reduced maximum developed pressure(Table 2) compared with LVDP curve for the sham-operated untreatedgroup. In infarcted hearts, the shift of developed pressure-volumecurves was partially prevented by bisoprolol and captopril treatment.Similarly, the reduction of maximum LVDP was completely preventedby bisoprolol, whereas captopril showed only a trend to increasemaximum LVDP (Table 2). Bisoprolol shifted the developed pressure-volumecurves of sham-operated hearts somewhat upward. The end-diastolicpressure-volume curves for the infarcted groups were also shiftedrightward and downward and were not significantly affected bytreatment. However, the shift between captopril-treated, sham-operatedand infarcted hearts did not reach significance, an indicationthat structural dilation was less than in untreated or bisoprolol-treatedinfarcted hearts.

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Fig. 1. A: pressure-volume curves for left ventricular developed pressure (LVDP) of all experimental groups. B: pressure-volume curves for left ventricular end-diastolic pressure (EDP) of all experimental groups. MI, myocardial infarction; Capto, captopril; Biso, bisoprolol. * P < 0.007 sham vs. MI, $dagger$ P < 0.007 Biso- or Capto-treated vs. untreated.

High-energy phosphate metabolism. Representative ³¹P NMR spectra from the various groups of hearts are shown in Fig. 2. Meanvalues for high- and low-energy phosphates and pH_i are given inTable 3. P_i resonances were comparable in sham and chronicallyinfarcted hearts, but there was a significant reduction of thePCr resonance in untreated chronically infarcted hearts (10.6± 0.6 vs. 13.5 ± 0.7 mM in untreated sham-operated hearts, P <0.007). With bisoprolol treatment, PCr remained almost unchangedand also captopril could limit the extent of the PCr reduction.There was no effect of treatment on ³¹P metabolites in the sham-operated groups. The total creatinepool tended to be reduced by chronic infarction (19.7 ± 1.2 vs.23.0 ± 1.0 mM in sham-operated rats). Treatment with bisoprololprevented this reduction, whereas captopril did not. Free creatinewas, on average, 9.4 ± 0.5 mM and tended to reduce in infarctedhearts but not in treated hearts. Intracellular pH was 7.15 ±0.00, and the values were comparable among sham and infarcted,treated and untreated, hearts. Free cytosolic ADP concentrationswere, on average, 89 ± 5 µM, and $Delta$ G values were $-$ 59.5 ± 0.4 kJ/mol.TANs measured in the right ventricle were 32.1 ± 1.0 nmol/mg proteinon average. There were no significant differences among groups(Table 3).

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Fig. 2. Representative ³¹P nuclear magnetic spectroscopy (NMR) spectra of all experimental groups. PCr, phosphocreatine.

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Table 3. High-energy phosphate metabolism for all experimental groups

CK reaction velocity. Figure 3 depicts stacked plots of ³¹P NMR spectra obtained from saturation transfer experiments for sham-operateduntreated, infarcted untreated, infarcted bisoprolol-treated,and infarcted captopril-treated hearts. The spectra show thatthe extent of saturation transfer from the PCr to [ $gamma$ -P]ATP resonanceis reduced in infarcted hearts and that this reduction is partiallyprevented by treatment either with bisoprolol or captopril.

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Fig. 3. Stacked plots of ³¹P-NMR spectra from saturation transfer experiments of an untreated sham-operated (A) and infarcted heart (B), and a Biso (C)- and Capto (D)-treated infarcted heart. For reasons of clarity, only PCr and $gamma$ -ATP resonances are shown.

Mean data from saturation transfer experiments are shown in Table 3 and in Fig. 4. On average, the T₁ of PCr was 3.49 ± 0.14s and was not different among groups (Table 3). There was a trendfor a decrease of the CK rate constant in all infarcted groups.CK reaction velocity was reduced in all infarcted hearts but significantlyless so in hearts treated with either bisoprolol or captopril(Fig. 4). However, the reduction post-MI did not reach significancein the bisoprolol-treated group. Thus energy reserve via CK remainedat higher levels when infarcted hearts were treated with eitherthe $beta$ -blocker bisoprolol or the ACE inhibitor captopril.

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Fig. 4. Mean creatine kinase reaction velocity (CK flux) of all experimental groups. * P < 0.007 sham vs. MI; $dagger$ P < 0.007 Biso- or Capto-treated vs. untreated.

Biochemical analysis. Table 4 summarizes the results of enzyme analysis of right ventricular homogenates. Total CK activityshowed a trend for reduction after MI from 8.1 ± 0.5 to 6.0 ±0.7 IU/mg protein in untreated but not in hearts treated withbisoprolol or captopril. CK isoenzyme distribution showed a trendfor the changes characteristic of failing myocardium: a decreaseof the absolute MM-CK and mitochondrial CK activities and an increaseof the relative activities of fetal $beta$ -containing isoenzymes. Treatmentwith bisoprolol or captopril completely prevented all changesin total CK and isoenzyme activities after MI both in absoluteand relative terms. Activities of the mitochondrial enzyme citratesynthase and of the glycolytic enzyme lactate dehydrogenase didnot change in any experimental group.

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Table 4. Enzyme activities in right ventricle for all experimental groups

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Definition of model. The present study defines cardiac function and energy metabolism under various forms of treatment ina clinically highly relevant model of heart failure, occurringpost-MI. For untreated groups, changes of cardiac geometry andfunction were as previously reported (23, 30). End-diastolicand systolic pressure-volume relations were shifted to the rightin infarcted hearts, indicating structural dilatation (40).At the same time, maximum LVDP was substantially reduced, attestingto contractile dysfunction. This model is well suited to studybeneficial or adverse effects of various forms of pharmacologicaltreatment (10, 17).

Similarly, changes in cardiac energy metabolism in untreated infarcted hearts were as previously reported: steady-state TANlevels are unaltered, whereas PCr is reduced by 22% and totalcreatine content by 14% (20, 21, 30). On the basis of CKequilibrium assumptions, we calculated unchanged free ADP and $Delta$ G levels at least for the baseline performance conditions studiedhere. CK reaction velocity, a measure of ATP transfer from mitochondriumto myofibrils (21), was reduced by 41%. Also, changes in totalCK and CK isoenzyme distribution, measured in the right ventricle,were as previously described (23, 30), indicating that thechronically failing heart is characterized by reduced MM-CK andmitochondrial CK activity. The alterations of energy metabolismfound here are characteristic of many models of cardiac hypertrophyand failure, i.e., they occur independent of the etiology of heartfailure (5, 20, 21, 28).

Effects of $beta$ -receptor blockade and ACE inhibition on cardiac geometry and function. In untreated infarcted hearts, substantialleft and right ventricular hypertrophy occurred, as indicatedby increased left and right ventricular weights occurring despitethe loss of ~40% of left ventricular tissue due to infarction.The increase in heart weight was reduced by both captopril andbisoprolol treatment, most effectively in the right ventricle,indicating that both forms of treatment blunted the hypertrophicresponse post-MI. However, even under captopril treatment, therewas still significant hypertrophy after MI. This is in agreementwith previous findings on $beta$ -blockers (13, 24) and ACE inhibitors(17, 46). Aside from a small increase in maximum LVDP by bisoprolol,both forms of treatment did not affect function and geometry insham-operated hearts, as assessed by pressure-volume curves. Incontrast, in infarcted groups, ACE inhibition with captopril partiallyprevented the rightward and downward shift of the systolic anddiastolic pressure-volume curves, a well-characterized effect(12, 33, 46). Data are controversial on the functional effectsof chronic $beta$ -receptor blockade in the post-MI rat model. Severalstudies suggested that $beta$ -blockers promote left ventricular dilation(13, 18). In contrast, our present work showed unchanged end-diastolicpressure to end-diastolic volume relations with bisoprolol treatment.In addition, bisoprolol improved LVDP (end-diastolic pressure= 10 mmHg) and maximum LVDP in infarcted hearts studied underthe same loading conditions as sham-operated hearts. The presentstudy clearly demonstrates that chronic bisoprolol treatment partiallyprevented the decrease of LVDP at various loading conditions butdid not change end-diastolic pressure-volume relations. For thedosages used, the extent of the beneficial effect was similarto that exerted bycaptopril.

In the isolated isovolumic heart preparations used in this study, global coronary flow was not significantly different amongthe six groups of hearts. Therefore, the beneficial effects ofchronic $beta$ -blocker or ACE inhibitor treatment on function and energymetabolism may be due at most in part to improved global perfusionand microcirculation after MI. Because isolated hearts were notperfused with bisoprolol or captopril, these changes reflect chronicalterations of myocardial perfusion rather than acute coronaryvascular effects of thesedrugs.

Effects of $beta$ -receptor blockade and ACE inhibition on cardiac energy metabolism. In clinical studies of heart failure, both $beta$ -receptor blockers (7, 44) and ACE inhibitors (34, 37)have been shown to chronically reduce mortality and improve leftventricular function. The exact mechanisms of these beneficialeffects remain to be determined. Energy metabolism is compromisedin heart failure (19), and these compounds may, at least inpart, act by maintaining normal energy metabolism. Previous studieson this subject are limited: Sanbe et al. (36) showed in a post-MIrat model that improvement of cardiac index and high-energy phosphatelevels by various ACE inhibitors after MI was associated withan increased mitochondrial oxidative function. A more recent studyby Nascimben et al. (27) using Syrian myopathic hamsters showedmaintenance of CK reaction velocity by treatment with enalapril.Waagstein et al. (45) showed that myocardial lactate productionturns to lactate extraction in dilated cardiomyopathy patientstreated chronically with metoprolol. Previous work by Laser etal. (24) showed that the changes in CK and lactate dehydrogenaseisoenzyme composition could be prevented by bisoprolol treatmentin the post-MI rat model. Also, in six patients with dilated cardiomyopathy,we showed that the myocardial PCr-to-ATP ratio, measured noninvasivelywith ³¹P NMR spectroscopy, increased during chronic drug therapy, including(in 4 of 6 cases) metoprolol (31). In the present work, we systematicallyanalyze the effects of $beta$ -receptor blockers and ACE inhibitorson the various components of cardiac energy metabolism in thepost-MI rat model. Unequivocally, we demonstrate that the beneficialfunctional effects of both bisoprolol and captopril treatmentare accompanied by beneficial effects on cardiac energy metabolism:increased PCr content and CK reaction velocity; increased MM andmitochondrial CK activities; and prevention of the fetal reprogrammingwith relative increase of the $beta$ -containing CK isoenzymes. Forthe dosages used, both compounds were similarly effective, oneexception being that bisoprolol also prevented the loss of totalcreatine whereas captopril did not. The reason for this discrepancywarrants further study. It is likely that $beta$ -receptor blockersand ACE inhibitors exert their beneficial effects mainly by chronicallyreducing the energetic needs of the heart, via reduction of heartrate and pre- and afterload, respectively. In addition, it ispossible that these agents interfere more directly with energymetabolism, one potential site of action being the sarcolemmalcreatine transporter (15). This remains to be furtherevaluated.

Are the observed beneficial effects on cardiac energy metabolism causally related to the improvement of left ventricular functionand geometry, or are they merely epiphenomena of the treatmentwith these compounds? Our data do not provide a final answer butallow us to speculate: In principle, energy metabolism could limitperformance in heart failure by three distinct mechanisms: 1)a reduction of ATP content, 2) decrease of ATP transfer and thusATP availability at the myofibrils, and 3) a reduction of thefree energy change of ATP hydrolysis. Because steady-state ATPlevels are unchanged in our model of heart failure, simply a preservationof ATP levels can be ruled out as a mechanism. In contrast, ATPtransfer (CK flux) is reduced substantially in post-MI rat hearts,and this reduction is almost completely prevented by bisoprololand, to a lesser extent, by captopril. Thus maintenance of ATPtransfer, i.e., energy reserve via CK, may be involved in theprotective effect of $beta$ -receptor blockers and ACE inhibitors. Finally, $Delta$ G values remained unchanged for the baseline performance conditionsstudied here. However, Tian et al. (40) and Tian and Ingwall(41) have demonstrated that hearts with a compromised CK systemshow reduced contractile reserve. It is thus conceivable thatthe effects of reduced CK flux and the inability to maintain high $Delta$ G combine to limit the contractile reserve of the failing heartduring inotropic stimulation, and $beta$ -receptor blockers and ACEinhibitors may be able to maintain energy metabolism under theseconditions. This remains to be studied. Therefore, our resultsdo not prove a causal relation between the observed beneficialfunctional and energetic effects, but our findings are consistentwith the view that preservation of energy metabolism explains,at least in part, the favorable effects of $beta$ -receptor blockersand ACE inhibitors in chronic heartfailure.

Study limitations. Enzyme and HPLC analyses were performed on intact residual right ventricular tissue, because the left ventriclewas Formalin pretreated for histological determination of infarctsize. However, Laser et al. (23) previously showed that changesin energy metabolism are very similar for the left and right ventricle.The present study involves 53 successful long-term experiments,yet only a single dose for each compound, one that showed a mildhemodynamic effect, was tested. Therefore, it is open whetherthe agents tested here exert dose-dependent effects on energymetabolism. Our study, however, shows that alterations in energymetabolism can be largely prevented when, post-MI, rats are chronicallytreated with $beta$ -receptor blockers or ACEinhibitors.

	ACKNOWLEDGEMENTS

We thank Bristol-Myers Squibb, Regensburg, Germany, for providingcaptopril.

	FOOTNOTES

This work was supported by a research grant from E. Merck, Darmstadt, Germany, and by Grant SFB 355/A3 and B1 from the DeutscheForschungsgemeinschaft.

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 thisfact.

Address for reprint requests and other correspondence: S. Hügel, Medizinische Universitätsklinik, Josef-Schneider-Str. 2, 97080 Würzburg, Germany (E-mail: huegel{at}mail.uni-wuerzburg.de).

Received 19 January 1999; accepted in final form 6 July 1999.

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Effects of ACE inhibition and $beta$ -receptor blockade on energy metabolism in rats postmyocardial infarction