beta -Adrenergic stimulation causes cardiocyte apoptosis: influence of tachycardia and hypertrophy

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$beta$ -Adrenergic stimulation causes cardiocyte apoptosis: influence of tachycardia and hypertrophy

Yukitaka Shizukuda¹, Peter M. Buttrick¹, David L. Geenen¹, Alain C. Borczuk², Richard N. Kitsis¹^,³, and Edmund H. Sonnenblick¹

¹ Division of Cardiology and Departments of ² Pathology and ³ Cell Biology, Albert Einstein College of Medicine, Bronx, New York 10461

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

To establish whether catecholamines per se in the absence of significant increases in systolic load induce myocardial damagevia apoptosis, rats were treated with vehicle or isoproterenol(400 µg · kg¹ · h¹). Apoptotic cardiocytes (Apo) were identified in paraffin-embeddedsections using terminal deoxynucleotide transferase-mediated dUTPnick end labeling. Results were confirmed using an independentligase assay. Systolic blood pressures were comparable in isoproterenol-treatedand control rats. Twenty-four hours of treatment with isoproterenolresulted in significant numbers of Apo compared with control [7.9± 2.5 vs. 0.3 ± 0.3 (SE) cm², P < 0.05]. A cohort of animals was subjected to ventricularpacing to induce a tachycardia equivalent to that induced by isoproterenol,and these animals did not show an increase in Apo. The left ventricularhypertrophy induced by 2 wk of abdominal aortic banding also increasedApo (~7.2-fold); however, 24 h of isoproterenol infusion did notinduce additional Apo in these rats. Thus catecholamines, in theabsence of altered systolic load, induce Apo which is not mediatedsolely by tachycardia. Left ventricular hypertrophy secondaryto abdominal aortic banding is associated with Apo, but this doesnot increase sensitivity to isoproterenol-induced Apo.

catecholamines; myocardial cell death; cardiac pacing; ligase reaction; rats

	INTRODUCTION

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APOPTOSIS, OR PROGRAMMED cell death, is observed in experimental heart failure due to multiple intracoronary embolization(26), tachycardia (18), postmyocardial infarction (22),or left ventricular hypertrophy (1, 10, 17) and is seenin human hearts with myocardial infarction (13, 24), ischemiccardiomyopathy (20, 21), and idiopathic dilated cardiomyopathy(20, 21). These findings support a role for apoptosis in thepathogenesis of heart failure.

Heightened adrenergic drive, as well as activation of the renin-angiotensin system, is the hallmark of the neurohumoral changesin heart failure, and the extent of elevation of plasma norepinephrinecorrelates with the severity of the left ventricular dysfunction(28) and with mortality (4). In addition, chronic adrenergicactivation is considered to be deleterious in heart failure becauseof its hemodynamic consequences and direct cardiocyte toxicity.

The purpose of this study was to determine whether continuous $beta$ -adrenergic stimulation alone can induce apoptosis in rat myocardiumin vivo without other intercurrent alterations in systolic stressand, if so, whether pathologically hypertrophied cardiocytes havea greater susceptibility to catecholamine-induced apoptosis.

	METHODS

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Animals. Male Wistar rats weighing 250-330 g were used for this study. The animals were maintained in accordance with the guidelinesof the National Research Council and the standing committee onAnimal Care of the Albert Einstein College of Medicine. Catecholaminewas infused continuously, as previously reported (2, 11).Briefly, Alzet minipumps (model 2001, Alza Pharmaceutical, PaloAlto, CA) were implanted subcutaneously in the neck, under methoxyfluraneanesthesia. The minipump was filled with l-isoproterenol HCl dissolvedin acidified isotonic saline (0.001 N HCl) or acidified isotonicsaline alone (vehicle). The pump rate was 1 µl/h, and the drugwas delivered at 40 or 400 µg · kg¹ · h¹. The higher dose has been previously shown to significantly increaseheart rate without any change in systolic blood pressure and tocause significant desensitization to catecholamines after 2 hof infusion (2, 11). In initial studies, control and isoproterenoltreatment was for 12 h, 24 h, or 7 days. On the basis of the resultsof this time-course study, the 24-h infusion was chosen for thesubsequent pacing and hypertrophy protocols. Heart rate and systolicblood pressure were measured by the tail-cuff technique underlight methoxyflurane anesthesia before implantation, 24 h, 4 days,and 7 days after implantation, and at the time the animals werekilled.

Pacing protocol. To determine whether the effects of isoproterenol on cardiac apoptosis were related to elevated heart rate alone, a separatecohort of rats was subjected to cardiac pacing. Rats were anesthetizedwith chloral hydrate (400 mg/kg ip) and ventilated with positivepressure. A left thoracotomy was performed, and Biomed wires (CoonerWire, Chatsworth, CA) were sutured on the epicardial surface ofthe apex and base of the heart with 9-0 sutures (Ethicon, Somerville,NJ). Wires were connected to a stimulator (model SD9, Grass MedicalInstruments, Quincy, MA), and the heart was paced at 500 beats/min.This heart rate was chosen to approximate the mean of isoproterenol-inducedheart rates [517 ± 21 (SE) beats/min, n = 4]. The pacing was confirmedby visual inspection of the heart in the open chest when the stimulatorwas turned on. The chest was closed, and wires were passed throughthe skin, tunneled to the neck, and exteriorized. The wires wereprotected by a custom-made rat vest jacket and a flexible coiledmetal spring tube. Rats were able to freely ambulate in the cageand were paced continuously for 24 h.

Aortic banding. Descending aortic coarctation was created using techniques that are standard in our laboratory. Briefly, animals were anesthetizedwith methoxyflurane, the abdominal aorta just above the renalartery bifurcation was isolated, and a 20-gauge needle was placedalong the side of the abdominal aorta and tied with a 5-0 silkthread. After the suture was secured, the needle was removed,creating partial banding of the abdominal aorta. Rats were cageconfined for 2 wk to allow ventricular hypertrophy to develop,then they were treated with vehicle or with 400 µg · kg¹ · h¹ isoproterenol for 24 h via Alzet pump, as described above. Additionalage- and weight-matched sham-operated rats were treated for 24h with vehicle only or 400 µg · kg¹ · h¹ isoproterenol and served as controls.

Staining and morphometric analysis. Hearts were excised quickly after animals were anesthetized with methoxyflurane. The aorta was cannulated and perfused with10 ml of chilled normal saline, then with 10 ml of chilled 10%neutral buffered Formalin. The heart without atria was weighedand then sliced into three sections perpendicular to the longaxis of the ventricle. Sections were stored in 10% neutral bufferedFormalin for 24 h and then embedded in paraffin. Slide sections(5 µm) from midventricular level were stained by in situ terminaldeoxynucleotide transferase-mediated dUTP nick end labeling (TUNEL)using an in situ apoptosis detection kit [TACS 2TdT (TBL), Trevigen,Gaithersburg, MD]. The details of TUNEL assay have been describedelsewhere (7). Positive-stained controls were prepared by incubatingserial sections of each paraffin block with 10 U/ml DNase I for20 min at 37°C before treatment with terminal transferase. Negativecontrols were prepared by staining serial slides without terminaldeoxynucleotide transferase. Red counterstain C (Trevigen) wasused to stain cytoplasm. TUNEL-positive nuclei stained blue inthis assay. Serial sections were also used for hematoxylin-eosinstaining for standard histological evaluation. The entire stainedsection was scanned at ×100 under light microscopy. When TUNEL-positivecells were detected, magnification was changed to ×400 to assesswhether staining occurred in cardiocytes or noncardiocytes. OnlyTUNEL-positive cardiocytes were counted in each slide. We classifiedcells as TUNEL-positive cardiocytes according to the followingcriterion: nuclei were inside cardiocyte contour. Any nuclei thatwere ambiguous were not counted. Round homogenous dark dots (consideredto be artifact) and stained cell debris were carefully eliminatedfrom counting. Brownish nuclei-like deposits, considered to beFormalin crystals, were not counted. To assess whether tissuedamage was present in locations of TUNEL-positive cardiocytes,the corresponding hematoxylin-eosin-stained serial sections wereexamined. The area of the heart in the slide preparation was measuredby a modified cut-and-weigh technique (23). Briefly, the areaof the heart slice was enlarged to ×64 by a photo enlarger. Thecontour of the heart section was traced on high-quality paper.The paper was cut as traced and weighed. Areas were computed asthe ratio of the weight of the paper to the weight of a unit ofknown area. The numbers of apoptotic cardiocytes were normalizedto areas of tissue (cm²) and per 10,000 cardiocyte nuclei estimated by the morphometricmethod. From the positive control of each section, 12 light-microscopicfields (×400) were chosen to count the number of cardiocyte nuclei.Endocardial, midmyocardial, and epicardial areas were chosen fromseptum and lateral, anterior, and posterior walls of the leftventricle. The number of cardiocyte nuclei in each microscopicfield was counted under a grid covering a total area of 0.0625mm². Only nuclei that were completely contained within cardiocytecontours were counted. The number of cardiocyte nuclei in 12 fieldswas averaged. Estimated total cardiocyte nuclei per slide werecalculated as the area of tissue of each slide (mm²) × [the average number of cardiocyte nuclei in 12 light-microscopicfields/0.0625 (mm²)]. The number of TUNEL-positive cells per 10,000 cardiocyte nucleiin each slide was calculated as total positive cells in each slidedivided by estimated total cardiocyte nuclei in each slide multipliedby 10,000. The morphometry results of two sections from each heartthat were >3 mm apart were averaged for statistical comparisons.

Ligase reaction. To verify the results of TUNEL assay, midventricular sections from 9 rats (3 from 12-h vehicle-treated rats, 4 from 12-h isoproterenol-treatedrats, 2 from aortic-banded rats) were subjected to this in situapoptosis staining. We used the technique published by Didenkoand Hornby (5) with minor modifications. Probes for this reactionwere prepared by the following methods. Briefly, a 168-bp double-strandedDNA fragment was prepared using primers 5'-AATTAACCCTCACTAAAGGG-3'and 5'-GCAATTAACCCTCACTAAAG-3' complementary to plasmid pBluescriptII KS (Stratagene, La Jolla, CA). To prepare fragments by PCR,the following reaction mix was set up: 100 µl of 10 mM Tris ·HCl, pH 8.3, 50 mM KCl, 1.5 mM MgCl₂, 70 µM digoxigenin-11-dUTP(Boehringer Mannheim, Indianapolis, IN), 130 µM dTTP, 200 µM dATP,200 µM dGTP, 200 µM dCTP (other nucleotides from Sigma Chemical,St. Louis, MO), 200 nM each primer, and 10 ng of plasmid. Taqpolymerase (5 U; PE Applied Biosystems, Foster City, CA) was added.After the mixture was heated to 94°C for 5 min, PCR was performedwith 35 cycles of 1 min at 94°C, 1 min at 50°C, and 2 min at 74°C,with the final cycle having an extension time of 4 min. The resultantprobe was purified by spin columns using high pure PCR productspurification kit (Boehringer Mannheim) according to the company'sinstruction. The Formalin-embedded sections were deparaffinized,rehydrated, and treated with proteinase K, as previously described(5). Sections were incubated with a mixture of 50 mM Tris ·HCl, pH 7.8, 10 mM MgCl₂, 10 mM dithiothreitol, 1 mM ATP, and50 µg/ml BSA, with digoxigenin-DNA fragment at 3 µg/ml and DNAT4 ligase (New England BioLabs, Beverly, MA) at 32 U/ml in a humidifiedbox for 1 h. Then sections were preblocked and incubated withsheep anti-digoxigenin Fab fragment-alkaline phosphatase conjugatein blocking buffer (Boehringer Mannheim), as previously described(5). For color development, sections were then placed in thesolution recommended by the manufacturer (0.1 M Tris, pH 9.5,50 mM MgSO₄, 0.4 mg/ml nitro blue tetrazolium, 0.19 mg/ml 5-bromo-4-chloro-3-indolylphosphate), and color development was monitored under the microscope.Positive and negative controls were stained simultaneously. Thepositive controls were treated with DNase I as described above,and negative controls were stained without DNA T4 ligase. Thereaction was terminated by washing sections in water when colorof nuclei of positive controls developed. The wet sections weremounted by Fluoromount-G (Southern Biotechnology Associates, Birmingham,AL) and covered by cover glasses without counterstain. Morphometricanalyses were performed on these slides as described above.

Statistics. Values are means ± SE. The statistical significance of normalized positive cells, body weight, heart weight, and hemodynamicvariables between the control and isoproterenol-treated groupwas evaluated using Student's nonpaired t-test. The statisticaldifferences of apoptotic cardiocyte numbers, body weight, heartweight, and hemodynamic variables between the different time periodsin the same group and between more than three groups were testedby ANOVA with Bonferroni's post hoc test. P < 0.05 was consideredto be significant.

	RESULTS

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General characteristics of animal models. All the control animals survived the vehicle treatment. However, two of the six animals in the 24-h isoproterenol-treatedgroup and two of the six animals in the 7-day isoproterenol-treatedgroup died before the animals were to be killed.

Table 1 shows hemodynamic parameters in control and isoproterenol-treated rats. Systolic blood pressure was comparable betweenthe groups. Heart rates in isoproterenol-treated rats during thetreatment period were significantly higher than in controls (Table1). In rats treated with 40 µg · kg¹ · h¹ isoproterenol (n = 5), systolic blood pressure was comparable(84 ± 7 vs. 89 ± 5 mmHg) and a significant increase in heart ratewas observed compared with control rats (497 ± 8 vs. 424 ± 16beats/min, P < 0.05). However, this increase was equivalent tothat seen in the group treated with 400 µg · kg¹ · h¹ isoproterenol. In paced rats (n = 5), systolic blood pressureand heart weight-to-body weight ratio were comparable to the controls.A comparable increase in heart rate was seen after 24 h of pacingvs. rats treated with 400 µg · kg¹ · h¹ isoproterenol (509 ± 6 vs. 517 ± 21 beats/min).

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Table 1. Hemodynamic parameters of control and isoproterenol-treated rats

Table 2 represents the body weights and heart weights in the control and isoproterenol-treated groups. Body weight tendedto increase over the study period in both groups; however, thedifferences between groups and between preimplantation and treatmentperiods in both groups did not reach statistical significance.At day 7 the isoproterenol-treated group showed significantlyhigher heart weight-to-body weight ratios than the control group(P < 0.05). In rats treated with 40 µg · kg¹ · h¹ isoproterenol, the heart weight-to-body weight ratio was similarto the controls (3.4 ± 0.2 vs. 3.4 ± 0.3 mg/g).

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Table 2. Effect of isoproterenol on body weight and heart weight

Table 3 shows hemodynamic variables and normalized heart weight data from the aortic-banded rats. A significant increasein heart weight-to-body weight ratio was noted in banded ratsirrespective of isoproterenol treatment compared with nonbandedcontrol rats. Heart rate but not blood pressure was significantlyhigher in isoproterenol-treated rats than in matched controls.

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Table 3. Hemodynamic parameters of control and aortic-banded rats with and without isoproterenol treatment

Histology of the heart. Hearts from rats treated with 400 µg · kg¹ · h¹ isoproterenol showed diffuse interstitial edema that was more prominent in theendocardial layer at 12 h and interstitial edema with infiltrationof inflammatory cells including mast cells in the perivascularareas and occasionally at cardiocyte layers at 24 h of treatment.At 7 days, focal fibrosis associated with cell necrosis was seenpredominantly in endocardial layers but was also scattered throughoutthe midmyocardial and epicardial layers with significant thickeningof the arterial walls. No remarkable histological changes wereseen in hearts treated with 40 µg · kg¹ · h¹ isoproterenol and in paced hearts. No qualitative increase infibrosis was seen in control or aortic-banded control groups.

Apoptotic cardiocytes. Figure 1 illustrates TUNEL staining of apoptotic cells. Positive control staining is shown in Fig. 1A, in which almost allcell nuclei were stained. Negative control staining is shown inFig. 1B. Apoptotic cardiocytes were delineated well under microscopicobservation (Fig. 1C). Cardiocyte apoptosis is unusual in controlhearts (Fig. 1D).

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Fig. 1. Staining of myocardial sections by terminal deoxynucleotide transferase-mediated dUTP nick end labeling (TUNEL). A: positive control staining from 12-h vehicle-treated animal. B: negative control staining from 12-h vehicle-treated animal. C: typical TUNEL-positive cardiocyte (arrow) in 12-h isoproterenol-treated heart. D: typical control heart. No cardiocyte apoptosis is seen. Original magnification ×400.

Figure 2 indicates the number of apoptotic cardiocytes per unit area (Fig. 2A) and per 10,000 cardiocyte nuclei (Fig. 2B)at different time points. Apoptotic cardiocytes were rarely seenin the control group. Throughout the study period, isoproterenol-treatedhearts manifested consistently higher numbers of apoptotic cardiocytesthan controls normalized to surface areas (Fig. 2A; 12.6 ± 2.3vs. 2.0 ± 1.2 at 12 h, 7.9 ± 2.5 vs. 0.3 ± 0.3 at 24 h, 5.9 ±1.5 vs. 0.9 ± 0.4 at 7 days, all P < 0.05) and also normalizedto 10,000 cardiocyte nuclei (Fig. 2B; 1.78 ± 0.36 vs. 0.30 ± 0.19at 12 h, 1.26 ± 0.39 vs. 0.04 ± 0.04 at 24 h, 1.02 ± 0.18 vs.0.13 ± 0.06 at 7 days, all P < 0.05). In 15 sections where histologicalcharacteristics were examined in detail, at 12 h of treatment,66.6% of cardiocyte apoptosis was located in areas with some evidenceof structural damage (such as areas with early damage of cardiocyte,mild inflammatory infiltration, interstitial edema); at 24 h oftreatment, 60% of positively stained cardiocytes were seen indamaged areas; at 7 days, 87.5% of cardiocyte apoptosis was seenin histologically abnormal areas (Fig. 3). In 43 sections, theanatomic locations of which were defined, 6% of the total numberof TUNEL-positive cardiocytes were observed in the right ventriclesin isoproterenol-treated rats and no cardiac apoptosis was seenin the right ventricles of controls.

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Fig. 2. Apoptotic cardiocytes in experimental animals normalized to areas (per cm², A) and cardiocyte nuclei estimated from positive control slides of serial sections (per 10,000 cardiocyte nuclei, B). * P < 0.05; ** P < 0.01 vs. control.

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Fig. 3. Percentages of apoptotic cardiocytes in histologically intact areas and damaged areas from 12 h to 7 days of treatment.

Effects of heart rate on cardiocyte apoptosis. Because isoproterenol increases heart rate, the increase in apoptosis might have been due to this effect rather than a directeffect of $beta$ -adrenergic stimulation on cardiocytes. To differentiatethese possibilities, we studied a cohort of rats subjected tocardiac pacing or to the lower isoproterenol infusion rate (40µg · kg¹ · h¹). Although 40 µg · kg¹ · h¹ isoproterenol elicited an increase in heart rate similar to thatelicited by 400 µg · kg¹ · h¹ [497 ± 8 (n = 5) vs. 517 ± 21 (n = 4) beats/min, P > 0.05], cardiocyteapoptosis detected by TUNEL assay in the group treated with thelower dose was not significantly different from that in the controlgroup. Furthermore, pacing at a rate analogous to that seen withisoproterenol (at either dose) did not increase cardiocyte apoptosisrelative to nonpaced control animals (Fig. 4).

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Fig. 4. Relationship between heart rate and extent of cardiocyte apoptosis. Cardiocyte apoptosis is significantly greater in rats treated with 400 µg · kg¹ · h¹ isoproterenol than in rats treated with 40 µg · kg¹ · h¹ isoproterenol (P < 0.05), although heart rate is not significantly different between groups. Mechanical pacing at 500 beats/min also does not increase cardiocyte apoptosis with increase in heart rate similar to that in rats treated with 400 µg · kg¹ · h¹ isoproterenol. * P < 0.05 vs. cardiocyte apoptosis of control (cont); ^# P < 0.05 vs. heart rate of control.

Effects of left ventricular hypertrophy on cardiocyte apoptosis. Because the transition from left ventricular hypertrophy to heart failure may be partially mediated by apoptotic cell loss,we evaluated rats with left ventricular hypertrophy secondaryto abdominal aortic banding to establish whether hypertrophiedhearts manifest cardiocyte apoptosis and whether they are susceptibleto additional damage by $beta$ -adrenergic stimulation. Aortic-bandedrats without isoproterenol treatment showed a significant increasein cardiocyte apoptosis compared with nonbanded age- and weight-matchedcontrol rats [7.9 ± 1.5 vs. 1.1 ± 0.5 cm² (P < 0.05) and 1.08 ± 0.23 vs. 0.14 ± 0.07 per 10,000 cardiocytes(P < 0.05)]. In these rats, most of cardiocyte apoptosis was seenin the left ventricle; however, 11% of cardiocyte apoptosis wasobserved in the right ventricle. When isoproterenol was superimposedon established ventricular hypertrophy, the extent of cardiocyteapoptosis was not significantly different from that seen withhypertrophy alone (Fig. 5). Isoproterenol induced a degree ofcardiocyte apoptosis in control, non-aortic-banded rats similarto that induced in the slightly younger rats used for time-coursestudy (Fig. 5).

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Fig. 5. Effects of isoproterenol (400 µg · kg¹ · h¹) on cardiocyte apoptosis in hypertrophied hearts induced by suprarenal abdominal aortic banding. Left ventricular hypertrophy per se increases cardiocyte apoptosis. Isoproterenol does not increase cardiocyte apoptosis of hypertrophied hearts further. * P < 0.05; ** P < 0.01 vs. non-aortic-banded control rats.

Ligase reaction. Single-base 3' overhangs have been reported to be highly specific for the DNA damage associated with apoptosis as opposedto a variety of nonapoptotic processes (5). The ligase reactioncan stain single 3' overhangs in situ. Thus we used this assayto verify the results of our TUNEL staining. As seen in Fig. 6,most nuclei were stained in a positive control (Fig. 6A), andno stained nuclei were seen in a negative control (Fig. 6B). Ligasereaction-positive cardiocyte nuclei were seen in isoproterenol-treatedhearts (Fig. 6C) and aortic-banded animals (Fig. 6D). Cardiocyteapoptosis was seen at 17.5 ± 1.2 cm² and 2.32 ± 0.08 per 10,000 cardiocyte nuclei in 12-h isoproterenol-treatedrats (n = 4), 2.4 ± 1.2 cm² and 0.38 ± 0.19 per 10,000 cardiocyte nuclei in control ratstreated with vehicle for 12 h (n = 3), and 13.7 ± 2.7 cm² and 1.53 ± 0.19 per 10,000 cardiocyte nuclei in aortic-bandedrats (n = 2), which were comparable to the results seen in ourTUNEL assay.

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Fig. 6. Staining of myocardial sections by ligase reaction. A: positive control treated with DNase I. B: negative control. Ligase-positive cardiocyte nuclei are seen in isoproterenol (400 µg · kg¹ · h¹)-treated hearts (C) and hearts of aortic-banded rats (D). Original magnification ×400.

	DISCUSSION

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In this study we demonstrate that 1) continuous $beta$ -adrenergic stimulation by isoproterenol induces consistent apoptosis ofcardiocytes throughout a study period of 7 days in rat myocardium,2) cardiocyte apopotosis induced by $beta$ -adrenergic stimulation isnot mediated solely by increased heart rate, 3) cardiac hypertrophyby abdominal aortic banding leads to an increase in cardiocyteapoptosis, and 4) no synergistic effect on cardiocyte apoptosisis seen when hypertrophy and $beta$ -adrenergic stimulation are superimposed.

Apoptosis is a type of cell death associated with chromatin condensation, endonuclease digestion of internucleosomal DNA into180- to 200-bp segments, and cell fragmentation into small membrane-boundvesicles (6, 16). An apoptotic body is a rounded, eosinophilicbody with highly condensed nuclear chromatin, broken into an aggregateof small dense fragments seen in routine histology (12). Inthe present study we did not use routine histological analysisalone to assess apoptosis, since previous reports suggest thattypical apoptotic bodies are rarely seen in myocardium, even instudies of myocardial ischemia and reperfusion (8) and myocardialinfarction (24). The amount of apoptosis was insufficient forquantitation by DNA ladder assay, which is a highly specific markerof apoptosis, although this would not distinguish the particularcell type involved. We therefore employed the TUNEL method, whichis a sensitive assay that also allows morphological assessmentof cell types to detect apoptotic cell bodies in the myocardium.The specificity of the TUNEL method has been questioned, and thetechnique may well overestimate the number of apoptotic cells(25). We have addressed this in two ways. First, we used verystrict histological criteria to eliminate noncardiocytes and contaminationwith nonspecific staining from analysis and, as a result, we observedrelatively small numbers of apoptotic cells. Second, we employedan independent method (the ligase reaction) to define apoptoticnuclei. Didenko and Hornby (5) recently reported that the ligasereaction is more specific to apoptotic cell death than blunt-endedDNA damage detected by TUNEL, which can be seen in a variety ofcases of nonapoptotic cell death in a low level. In our studythe amount of cardiocyte apoptosis in control, isoproterenol-treated,and aortic-banded hearts seen with the ligase reaction was quitesimilar to that seen using the TUNEL assay, which provides independentconfirmation that the extent of apoptosis is accurately reflectedin our data.

Few TUNEL-positive cells were observed in control hearts, which is consistent with previous studies (6, 17, 18, 21,24). Although the number of TUNEL-positive cells was significantlygreater in the hearts infused with isoproterenol than in controlhearts, we still observed relatively small numbers of cardiocytesundergoing apoptosis at 12 h, 24 h, and 7 days of $beta$ -adrenergicstimulation. Because apoptosis occurs over a very short time inmany types of cells (16), the accumulating cardiocyte loss dueto apoptosis in the in vivo setting may be much more substantial.For example, in neonatal rat hearts during adaptation, 10.4, 6.1,and 2.5 cardiocyte nuclei per 10,000 cardiocyte nuclei undergoapoptotic changes on the day of birth in right ventricle, interventricularseptum, and left ventricle, respectively (15). Correspondingvalues at 5 days after birth are 3.7, 3.5, and 2.0 cardiocytenuclei per 10,000 cardiocyte nuclei. These numbers are qualitativelysimilar to those we observed in $beta$ -adrenergic-induced apoptosis.Because significant anatomic changes occur in neonatal heartsas they adjust from the fetal circulation to the adult circulation,the apoptotic cardiocyte loss in our model may represent substantialdamage to the heart even in the short time period. In clinicalautopsy study, as many as 0.8% of cells have been identified asapoptotic in the border zones of acute myocardial infarction (24).This may reflect the relative severity and transient nature ofthe stimulus that differs from our model, in which the damageand apoptotic cardiocyte loss occur less acutely. In pacing-inducedheart failure in dogs, 37 cardiocytes per 10,000 total nucleiundergo apoptotic changes (18).

Direct toxic effects of catecholamines on the myocardium have been known for many years since Ziegler (29) reported thatcatecholamines induced myocardial damage. High doses of catecholaminesalso cause diffuse necrotic lesions in the myocardium with accompanyinginflammation and subsequent fibrous scarring (9). Recently,Matsui et al. (19) reported induction of apoptosis of culturedneonatal rat cardiocytes by norepinephrine and suggested thatcatecholamines may trigger cardiocyte apoptosis in hearts in vivo.Our report extends the observation of Matsui et al. in culturedneonatal rat cardiocytes and implies that a part of catecholamine-inducedmyocardial injury in vivo may be mediated by cell loss due toapoptosis. We chose isoproterenol, because it lacks a hypertensiveeffect that might contribute to cardiocyte apoptosis due to increasedsystolic wall stress (3).

Previously, selective desensitization of cardiac $beta$ -adrenoceptors in rats by prolonged infusion of isoproterenol at the sameinfusion rate that we used has been reported (2, 11). Inthose studies, desensitization occurs as early as 2 h after infusionstarts and lasts for at least 7 days. This degree of $beta$ -adrenergicdesensitization, which is considered to be an adaptive mechanismto $beta$ -adrenergic stimulation, is probably not sufficient to protecthearts from $beta$ -adrenergic stimulation-induced apoptosis in ourmodel, inasmuch as the extent of cell death was similar and sustainedthroughout the time course of our analysis.

The mechanism(s) by which $beta$ -adrenergic simulation induces cardiocyte apoptosis is unclear. Tachycardia is a hemodynamic consequencesecondary to $beta$ -adrenergic simulation. As previously reported,apoptosis is seen in pacing-induced heart failure (18). In ourmodel, heart rates increased by 20-33% from baseline with isoproterenoltreatment, which is less than that seen in the pacing-inducedcanine heart failure model (73%) (18). We tested rats pacedfor 24 h to assess whether an increase in heart rate alone caninduce cardiocyte apoptosis. In this protocol the increase inthe heart rate by pacing is not sufficient to induce cardiocyteapoptosis. We also observed that low-dose isoproterenol-treatedrats failed to show an increase in cardiocyte apoptosis, eventhough an increase in heart rate similar to that seen in ratstreated with 400 µg · kg¹ · h¹ isoproterenol is observed.

Cardiac muscle stretch has been associated with myocyte apoptosis (3), but no significant changes in systolic blood pressurewere seen in our model, which suggests that major changes in systolicload did not occur. This makes stretch per se unlikely to playa major role in catecholamine-induced apoptosis. Myocardial ischemiahas also been reported to cause apoptosis (7, 8, 14). $beta$ -Adrenergic stimulation increases cardiac contractility and oxygenconsumption and is known to cause vascular damage, which can contributeto myocardial ischemia.

Recently, it was reported that cardiocytes undergoing necrosis also manifest the typical DNA fragmentation that is usuallyseen in apoptosis (13). We have observed that some TUNEL-positivecardiocytes are located in the layers of normal-appearing cardiocyteswithout vascular injury and cardiocyte necrosis by light-microscopicobservation (Fig. 3). Although it would seem likely that theseapoptotic cardiocytes are nonischemic and not vulnerable to secondarynecrosis, this is unproven. The results in neonatal cardiocyteculture suggest that a direct effect of catecholamines not mediatedby ischemia can induce cardiocyte apoptosis (19).

In our study we show that left ventricular hypertrophy by abdominal aortic banding increases cardiocyte apoptosis. Previousreports suggest that cardiocyte apoptosis is increased by cardiachypertrophy (1, 10, 17, 27). Teiger et al. (27) reportedthat apoptotic activity peaks at 4 days and lasts for >30 daysafter the ascending thoracic aorta is banded in a rat model. Theyobserved a 50% increase in left ventricular weight by day 4 ofascending aortic banding, which is correlated with peak apoptoticactivity (27). On the other hand, using TUNEL assay, Li et al.(17) reported 3.89 ± 1.28 apoptotic cells per 10,000 nucleiin spontaneous hypertensive rats between 18 and 24 mo of age (17).

In our study, abdominal aortic banding was used to induce cardiac hypertrophy, and the number of apoptotic cardiocytes wasnormalized to the area and the total cardiocyte nuclei. We observeda relative increase of 22% in the heart weight-to-body weightratio over 2 wk of abdominal aortic banding with increased apoptoticcardiocytes. The extent of left ventricular hypertrophy was milderin our model than in the study by Teiger et al. (27). Our resultssuggest that milder and chronic hypertrophy is associated withcardiocyte apopotosis in rat hearts.

We also observed no synergistic effect on cardiocyte apoptosis between hypertrophy and $beta$ -adrenergic stimulation in our experimentalsetting. Whether this result is due to the true adaptive mechanismor selection process, namely, elimination of susceptible cardiocyteto catecholamine-induced cardiac hypertrophy during developmentof hypertrophy, is unclear. Also, it is possible that the effectsof $beta$ -adrenergic stimulation and hypertrophy overlap, so no synergyis seen.

In conclusion, we have shown that continuous $beta$ -adrenergic stimulation induces significant cardiocyte apoptosis constantlyover 12 h to 7 days in rat myocardium. Given the high load ofcatecholamines in heart failure, this may be an important causefor the progression of heart failure. The exact mechanisms of $beta$ -adrenergic stimulation-induced apoptosis are still not known.Left ventricular hypertrophy per se increases apoptotic cardiocytes,and no synergistic effect on cardiocyte apoptosis was seen betweenventricular hypertrophy and $beta$ -adrenergic stimulation. The mechanismsto explain these observations need to be elucidated.

	ACKNOWLEDGEMENTS

The authors are grateful to Leslie Gunther and William Schubert (Anatomical Imaging Facility, Albert Einstein College of Medicine)for technical assistance and to Dr. Ryoji Yokota (Division ofCardiology, Albert Einstein College of Medicine) for helpful discussions.

	FOOTNOTES

This work was supported by National Heart, Lung, and Blood Institute Grants HL-15498 (P. M. Buttrick) and HL-02699 (R. N.Kitsis). Ongoing support for these studies has been provided byCharles and Tamara Krasne.

Address for reprint requests: P. M. Buttrick, Sect. of Cardiology, University of Illinois at Chicago, 840 South Wood St. (MC 787), Chicago, IL 60612-7323.

Received 10 September 1997; accepted in final form 5 May 1998.

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This Article

Abstract

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				S.-D. Lee, C.-H. Chu, E.-J. Huang, M.-C. Lu, J.-Y. Liu, C.-J. Liu, H.-H. Hsu, J. A. Lin, W.-W. Kuo, and C.-Y. Huang Roles of insulin-like growth factor II in cardiomyoblast apoptosis and in hypertensive rat heart with abdominal aorta ligation. Am J Physiol Endocrinol Metab, August 1, 2006; 291(2): E306 - E314. [Abstract] [Full Text] [PDF]

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				Y.-T. Tseng, N. Yano, A. Rojan, J. P. Stabila, B. G. McGonnigal, V. Ianus, R. Wadhawan, and J. F. Padbury Ontogeny of phosphoinositide 3-kinase signaling in developing heart: effect of acute {beta}-adrenergic stimulation Am J Physiol Heart Circ Physiol, November 1, 2005; 289(5): H1834 - H1842. [Abstract] [Full Text] [PDF]

				M. D. Faulx, P. Ernsberger, D. Vatner, R. D. Hoffman, W. Lewis, R. Strachan, and B. D. Hoit Strain-dependent {beta}-adrenergic receptor function influences myocardial responses to isoproterenol stimulation in mice Am J Physiol Heart Circ Physiol, July 1, 2005; 289(1): H30 - H36. [Abstract] [Full Text] [PDF]

				C. Nakajima-Takenaka, S. Sakata, S. Kato, Y. Ohga, K.-y. Murata, S. Taniguchi, and M. Takaki Detrimental effects after dobutamine infusion on rat left ventricular function: mechanical work and energetics Exp Physiol, July 1, 2005; 90(4): 635 - 644. [Abstract] [Full Text] [PDF]

				M. Pareja, O. Sanchez, J. Lorita, M. Soley, and I. Ramirez Activated epidermal growth factor receptor (ErbB1) protects the heart against stress-induced injury in mice Am J Physiol Regulatory Integrative Comp Physiol, August 1, 2003; 285(2): R455 - R462. [Abstract] [Full Text] [PDF]

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				P. K. Tithof, M. Elgayyar, H. M. Schuller, M. Barnhill, and R. Andrews 4-(Methylnitrosamino)-1-(3-pyridyl)-1-butanone, a nicotine derivative, induces apoptosis of endothelial cells Am J Physiol Heart Circ Physiol, November 1, 2001; 281(5): H1946 - H1954. [Abstract] [Full Text] [PDF]

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				O.-E. Brodde and M. C. Michel Adrenergic and Muscarinic Receptors in the Human Heart Pharmacol. Rev., December 1, 1999; 51(4): 651 - 690. [Abstract] [Full Text] [PDF]

				B.-S. Tea, T.-V. Dam, P. Moreau, P. Hamet, and D. deBlois Apoptosis During Regression of Cardiac Hypertrophy in Spontaneously Hypertensive Rats : Temporal Regulation and Spatial Heterogeneity Hypertension, August 1, 1999; 34(2): 229 - 235. [Abstract] [Full Text] [PDF]

				Y. Shizukuda, M. E. Reyland, and P. M. Buttrick Protein kinase C-delta modulates apoptosis induced by hyperglycemia in adult ventricular myocytes Am J Physiol Heart Circ Physiol, May 1, 2002; 282(5): H1625 - H1634. [Abstract] [Full Text] [PDF]