Involvement of adrenergic pathways in activation of catalase by myocardial ischemia-reperfusion

doi:10.1152/ajpregu.00278.2001

Involvement of adrenergic pathways in activation of catalase by myocardial ischemia-reperfusion

Young-Hoon Kim¹, Yang-Sook Chun², Jong-Wan Park², Chan-Hyung Kim², and Myung-Suk Kim²

¹ Department of Pharmacology, College of Medicine, University of Ulsan, Seoul 138-736; and ² Department of Pharmacology and Heart Research Institute, College of Medicine, Seoul National University, Seoul 110-799, Korea

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In situ rabbit hearts were subjected to 15 min of regional myocardial ischemia, and at various time points of reperfusion,antioxidant enzyme activity and mRNA expression were measuredin ischemic and nonischemic myocardium. Catalase activity increasedsignificantly in both ischemic and nonischemic myocardium, peakingat 1 h after reperfusion and then gradually returning to the controllevel. Northern blot analysis showed enhanced expression of catalasemRNA in both areas. There were no changes in redox status, becauseglutathione levels were not altered by ischemia-reperfusion (I/R).We also tested whether catalase activation in the heart resultsfrom signaling pathways that might influence not only the heartbut also other organs. We found that catalase activity in thebrain was increased after myocardial I/R and ischemic stress tothe intestine was equipotent to myocardial I/R in catalase activation.We next sought to elucidate the possible involvement of the adrenergicsystem in catalase stimulation induced by ischemic stimuli. Afterpretreatment with the $alpha$ -adrenergic receptor antagonist prazosin,I/R failed to increase catalase activity in the heart and brain.Intravenous norepinephrine increased catalase activity in theheart, brain, and liver. This study shows that brief I/R activatesa signaling mechanism to induce catalase activation in multipleorgans and the $alpha$ -adrenergic system is involved as an intermediatepathway in this signaltransmission.

antioxidant; adrenergic system

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

REACTIVE OXYGEN METABOLITES, including superoxide anion, hydrogen peroxide, and hydroxyl radical, are continuously producedduring metabolic processes of aerobic organisms, and sometimesthe generation of reactive oxygen metabolites is accelerated bycertain exogenous energy or chemicals, including radiation energyand some anticancer drugs. Reactive oxygen metabolites are highlyreactive electrophiles, which may attack cellular constituentslike protein, lipid, or nucleic acid, resulting in various abnormalitiesof structures and functions. In normal conditions, the small amountof reactive oxygen metabolites produced in metabolic processesis neutralized by the endogenous antioxidant defense system. Theantioxidant system consists of antioxidant enzymes, includingsuperoxide dismutase (SOD) and catalase, and nonenzymatic antioxidants,including glutathione, vitamin C, and vitamin E. However, whenthe balance between the production and the neutralization of reactiveoxygen metabolites is deterred by certain causes, various patternsof oxidative cell injuries occur. It is generally accepted thatthese oxidative damages play an important role in some major pathophysiologicalsituations, including inflammatory diseases, ischemia-reperfusioninjury, aging, and cancer (13, 26).

Therefore, it is presumed possible to develop practical measures to prevent or control those diseases through inhibition ofoxidative cell damages. In this regard, many investigators havetried experimental approaches to reduce the oxidative damages(14, 25). Some of these studies (14) adopted methods tosuppress the generation of reactive oxygen metabolites or scavengethem by administration of exogenous antioxidant agents like SOD,catalase, or vitamin E. However, in many conditions, these exogenousagents hardly reach the target in active and stable forms, sothat most of these studies have been far fromsatisfactory.

There have been some attempts (29) to enhance endogenous antioxidant system to prevent oxidative damage. It has been reported(22, 25) that antioxidant enzymes can be stimulated by variousmodalities of cellular stress. For example, mild ischemia-reperfusion(7), heat stress (6), inflammatory mediators (3), andhyperbaric oxygenation (21) were reported to increase antioxidantenzyme activity in experimental animals. Among these, mild ischemicstress was shown to enhance mRNA expression of several genes,including the catalase gene, which was significantly increasedas early as 30 min after the ischemic stress (7). On the otherhand, in some of these experiments (2, 16), it was also observedthat the activation of antioxidant enzymes is accompanied by thesuppression of ischemia-reperfusion injuries, showing that theincreased antioxidant enzyme capacity actually induces the toleranceto oxidative insults. Therefore, defining the physiological conditionsand underlying mechanism of antioxidant activation would leadto the development of effective measures to minimize oxidativeinjuries.

In the present study, we tried to characterize the changes in antioxidant enzyme activity after ischemic stress. In the ischemicand the nonischemic myocardium of rabbit hearts subjected to abrief regional ischemia, the activity and mRNA expression of catalaseincreased not only in the affected ischemic myocardium but alsoin the virgin nonischemic myocardium. Increased catalase activitywas evident in the brain as well, indicating that a certain multiorgansignal transmission mechanism is involved. Moreover, ischemicstress to the intestine also evoked catalase activation in theheart and brain. We next sought to find the transmitter of thissignaling pathway. Because it is well known that the sympatheticnervous system is activated by stress, including myocardial ischemia,and induces some physiological responses to compensate the stress,we speculated that this system may play a role in the defensiveantioxidant activation and tested whether the sympathetic nervoussystem isinvolved.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Experimental Protocol and Sample Collection

Rabbits (New Zealand White, male, 1.5-2.5 kg) were used for all procedures. Each experimental group included sixanimals.

Experiment 1: changes in SOD, glutathione peroxidase, and catalase activity in ischemic and nonischemic myocardium after regional myocardial ischemia. Rabbits were subjected to 15 min of regional myocardial ischemia. Tissue samples from ischemic and nonischemic myocardiumwere taken 0, 1, 3, and 8 h after the onset of reperfusion forassays of SOD, glutathione peroxidase, andcatalase.

Experiment 2: changes in catalase activity in heart, brain, and liver after regional myocardial ischemia. Rabbits were subjected to 15 min of regional myocardial ischemia. Tissue samples from the heart, brain, and liver were takenafter reperfusion for 1 h. Catalase activity in each organ wasmeasured and compared with the values of the sham-operatedgroup.

Experiment 3: changes in catalase activity in heart, brain, and liver after regional intestinal ischemia. Rabbits were subjected to 15 min of regional intestinal ischemia. Tissue samples from the heart, brain, and liver were takenafter reperfusion for 1 h. Catalase activity in each organ wasmeasured and compared with the values of sham-operatedgroup.

Experiment 4: effect of adrenergic antagonists on catalase activation by regional myocardial ischemia. As a fundamental procedure to test the hypothesis that the adrenergic nervous system might act as a mediator in catalase stimulation,we studied whether catalase stimulation could be inhibited byblockade of the adrenergic receptors before ischemia and reperfusion.Prazosin ( $alpha$ -adrenergic receptor antagonist) or propranolol ( $beta$ -adrenergicreceptor antagonist) was administered before the myocardial ischemia,and catalase activity was measured in the heart, brain, and liverafter 1 h reperfusion following 15 min ofischemia.

Experiment 5: effect of adrenergic agonist on catalase activity in heart, brain, and liver. To test whether an adrenergic agonist can exert an effect on catalase activity similar to that of regional ischemia, norepinephrinewas administered intravenously for 10 min. Organ samples weretaken 1 h after the infusion wasfinished.

Operative Procedures

For regional myocardial ischemia, rabbits were anesthetized with pentobarbital sodium (30 mg/kg, iv). After tracheotomy, rabbitswere intubated and ventilated with room air. The hearts were exposedby a left thoracotomy through the fourth intercostal space. Asilk snare was placed around the large marginal branch of thecircumflex artery 2 cm from the atrioventricular groove. The arterywas occluded for 15 min by pulling the snare and then reperfusedby removing the snare. For intestinal ischemia, anesthetized rabbitswere subjected to laparotomy and the superior mesenteric arterywas occluded for 15 min. For the sham-operation groups, all operativeprocedures were performed identically, except for the occlusionof the coronaryartery.

Drug Treatments

Prazosin was dissolved in saline at a concentration of 0.5 mg/ml, and 2 mg/kg were intraperitoneally injected 10 min beforethe onset of ischemia. Propranolol was also dissolved in salineat a concentration of 0.5 mg/ml, and 2 mg/kg were continuouslyinjected via the ear vein for 10 min before the onset of ischemia.Norepinephrine was dissolved in normal saline at a concentrationof 2.5 µg/ml, and 10 µg/kg were infused continuously for 10 min.The doses of antagonists or agonists were selected on the basisof previous experiments using rabbits (1, 27). All stocksolutions were freshly prepared to avoiddegradation.

Preparation of Tissue Samples

In experiment 1, hearts were removed and washed by perfusion with cold saline. Myocardial samples (1-2 g) were taken fromthe ischemic area and the normally perfused, nonischemic areaof the left ventricle. To estimate the ischemic area, we performedseparate preliminary experiments using Langendorff-perfused, isolatedhearts. Isolated hearts were perfused and stained with Evans blue(0.1%) during occlusion of the coronary artery to demarcate theischemic risk area and the normally perfused area. In in situexperimental hearts, the region of pallor and akinesia duringthe coronary occlusion was visually inspected to confirm the demarcationestimated in the isolated Langendorff-perfused hearts. The myocardialsamples were taken from the central zone of the estimated areas,frozen quickly in liquid nitrogen, and stored at $-$ 70°C until theenzymeassays.

In subsequent experiments, whole left ventricles were used for myocardial samples, and at the same time, samples were takenalso from liver and brain. Liver samples were taken from the inferiormedial portion of the left lobe, and the cerebrum was used forbrainsamples.

Measurement of Antioxidant Enzyme Activity and Other Biochemical Assays

Myocardial samples were homogenized in 4 vol of homogenation buffer (30 mM KCl, 1 mM EDTA, and 10 mM KH₂PO₄, pH 7.4) usinga Polytron tissue disintegrator (Brinkman Instruments) and anultrasonicator (Heat Systems, Ultrasonics). The homogenate wascentrifuged at 10,000 g for 20 min, and the supernatant was takenfor the enzyme assay. The protein concentration was measured bythe bicinchoninic acid method (Bio-Rad) with BSA as astandard.

SOD activity was determined by the epinephrine autoxidation method according to Misra and Fridovich (18). The prepared samplewas added to 3 ml of 50 mM carbonate buffer (pH 10.2, 30°C) containing0.1 mM EDTA and 0.13 mM epinephrine. The absorbance change wasmonitored at 325 nm by ultraviolet spectrophotometer (Hewlett-Packard).One unit of SOD was defined as the enzyme amount that reducesthe rate of epinephrine autoxidation by 50%.

Glutathione peroxidase activity was assayed according to the method described by Delmaestro and McDonald (8). The sample(20 µl) was added to 0.98 ml of 50 mM phosphate buffer (pH 7.0)containing 1 mM EDTA, 0.24 U/ml glutathione reductase, 1 mM GSH,0.15 mM reduced NADP (NADPH), and 1.2 mM t-butyl hydroperoxide.The absorbance change was monitored at 37°C and 340 nm by ultravioletspectrophotometer. One unit of glutathione peroxidase was definedas the enzyme amount to consume 0.5 µmol of NADPH for 1min.

Catalase activity was measured by monitoring the rate of O₂ generation resulting from the decomposition of H₂O₂ (16). H₂O₂(final, 4.6 mM) was added to 5 ml of reaction buffer (0.1% EDTAand 10 mM potassium phosphate, pH 7.4) containing an aliquot ofthe tissue sample. The rate of O₂ generation was measured witha Clark-type oxygen electrode at 30°C. Enzyme activity was calculatedfrom the standard curve of purified catalase(Sigma).

Northern Blot Analysis

Total RNA was extracted by the acid-guanidinium thiocyanate-phenol-chloroform method (5). Human catalase (American TypeCulture Collection) and human $beta$ -actin (Clontech) cDNAs were usedas probes. Fifteen micrograms of total RNA were applied to elecrophoresisand transferred to a nitrocellulose filter. Probes were labeledby using a random-primed DNA labeling kit (Life Technologies).Filters were prehybridized at 42°C in a solution containing 50%formamide, 5× SSPE (NaCl, NaH₂PO₄, and EDTA), 0.1% SDS, 2× Denhardt'ssolution, 100 g/ml denatured salmon sperm DNA, and 2% dextransulfate and then incubated with the cDNA probes overnight at 42°C.Filters were washed at 60°C successively in 3× SSC (NaCl and sodiumcitrate) for 1 h, 1× SSC for 1 h, and 0.2× SSC plus 0.1% SDS for30 min and exposed to X-ray film at $-$ 70°C using intensifying screens.The intensity of blots was analyzed by densitometricscanning.

Measurement of Glutathione Contents

Cellular redox state was evaluated by measuring the glutathione contents. Total glutathione (GSH + GSSG) and GSSG contentswere analyzed according to the method of Griffith (12). Themyocardial samples were homogenized in 5 vol of 6% perchloricacid. The homogenates were centrifuged at 10,000 g for 2 min,and the supernatant was neutralized with 5 M K₂CO₃. The supernatantwas buffered by 2 vol of NaHCO₃ (100 mM, pH 6.5). 2-Vinylpyridine(6 µl) was added to a 0.3-ml aliquot of the mixture and incubatedfor 1 h to inactivate GSH. The mixtures with and without 2-vinylpyridinewere used for measurement of GSSG and total glutathione, respectively.Samples were added to the reaction mixture containing 1.8 ml KH₂PO₄(120 mM, pH 7.5), 20 µl NADPH (17 mM), 100 µl DTNB (12 mM), and10 µl glutathione reductase (200 U/ml). Changes in absorbanceat 412 nm and 30°C were monitored and compared with the valuesof standards. The GSH level was calculated by subtracting theGSSG level from the total glutathionelevel.

Statistical Analysis

Results are expressed as means ± SE. Differences were compared by unpaired two-tailed t-test, with P < 0.05 consideredsignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Responses to Regional Myocardial Ischemia

The area supplied by the large marginal branch of the left circumflex coronary artery was ~40-50% of the total left ventricle,including about one-third of the apical portion, a part of theanterior wall, and the papillary muscles; this demarcation wasof little variance among animals. We tried to ligate only theartery excluding vein branches, except for cases in which thetwo vessels were too close to isolate. The ST segment elevationon the electrocardiogram monitor was apparent right after theligation.

In preliminary experiments, we compared the effect of 15-min ischemia and 30-min ischemia. By 30-min ischemia, ~40% of therisk area showed irreversible injury, which was indicated by triphenyltetrazoliumchloride nonstaining. In addition, 30-min ischemia resulted inhemorrhagic lesions in most cases (data not shown). However, noneof these signs were observed in hearts subjected to 15-min ischemia.Therefore, we speculated that ischemia of more than 15 min induration is unsuitable for observing responses of viable cellsto stressfulstimulation.

Changes in Antioxidant Enzyme Activity After Ischemia-Reperfusion

Fifteen minutes of regional ischemia followed by reperfusion for 1-8 h failed to induce any significant changes in SOD andglutathione peroxidase activity in both ischemic and nonischemicmyocardium (Fig. 1).

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Fig. 1. Superoxide dismutase (SOD; A) and glutathione peroxidase activity (B) in nonischemic and ischemic myocardium of rabbit hearts. Rabbits were subjected to 15 min of regional myocardial ischemia. Tissue samples from ischemic and nonischemic myocardium were taken 0, 1, 3, and 8 h after the onset of reperfusion for assays of SOD and glutathione peroxidase. For the sham-operation group, all operative procedures were performed identically, except for the occlusion of the coronary artery.

However, catalase activity was significantly changed by this stimulus. Although the catalase activity in ischemic and nonischemicmyocardium was not altered immediately after the ischemia, reperfusionevoked an increased catalase activity in both ischemic and nonischemicregions, with a peak observed at 1 h after reperfusion and a gradualreturn to the control level at 8 h. Compared with the controlheart, the enzyme activity in the ischemic myocardium increasedby 79.5% and 62.3% at 1 and 3 h after reperfusion, respectively.The extent of the increase in the nonischemic myocardium at eachtime point was comparable to that in the ischemic myocardium,and there were no statistical differences between them. The catalaseactivity of the sham-operated heart was not different from thecontrol level (Fig. 2).

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Fig. 2. Catalase activity in nonischemic and ischemic myocardium of rabbit hearts. Rabbits were subjected to 15 min of regional myocardial ischemia. Tissue samples from ischemic and nonischemic myocardium were taken 0, 1, 3 and 8 h after the onset of reperfusion for assays of catalase. For the sham-operation group, all operative procedures were performed identically, except for the occlusion of the coronary artery. * P < 0.01 vs. control; # P < 0.05 vs. control.

Expression of Catalase mRNA

Northern blot analysis revealed an enhanced expression of catalase mRNA in both the ischemic and nonischemic myocardium onreperfusion after 15 min of regional ischemia. The enhancementof mRNA expression paralleled the increase in the enzyme activity,showing a peak at 1 h after reperfusion and a gradual decreasethereafter. As determined by densitometric analysis, the amountof mRNA expressed at 1 h after reperfusion was more than twofoldhigher in both the ischemic and the nonischemic myocardium thanin the sham-operated hearts (Fig. 3).

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Fig. 3. Northern blot analysis and densitometric analysis of catalase mRNA in nonischemic and ischemic myocardium. Tissue samples from ischemic and nonischemic myocardium were taken 0, 1, 3, and 8 h after the onset of reperfusion. A: total RNA (15 µg) was applied to elecrophoresis and transferred to nitrocellulose filters. Filters were incubated with the cDNA probes of catalase (C) or $beta$ -actin (A). B: the intensity of blots was analyzed by densitometric scanning, and the relative intensity of catalase signal normalized by $beta$ -actin signal was illustrated. S, sham-operation group.

Changes in Myocardial Glutathione Content

To investigate the involvement of oxidative stress mediated by reactive oxygen species in the stimulation of antioxidant enzymes,we evaluated cellular redox state by measuring myocardial glutathionecontents. As shown in Fig. 4, there was no apparent change ineither the GSH or GSSG content in both ischemic and nonischemicmyocardium after 15 min of ischemia and reperfusion of varyingduration.

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Fig. 4. Reduced (GSH; A) and oxidized glutathione (GSSG; B) content in ischemic and nonischemic regions of myocardium of rabbit hearts. Deproteinized myocardial samples incubated with or without 2-vinylpyridine were assayed for GSSG and total glutathione, respectively. The GSH level was calculated by subtracting the GSSG level from the total glutathione level.

Changes in Catalase Activity in Heart, Brain, and Liver After Regional Myocardial Ischemia

In subsequent experiments, it was confirmed that the catalase activity of the heart after 1 h of reperfusion following 15min of regional myocardial ischemia was significantly higher thanthat in the sham-operated animal. The catalase activity of thereperfused heart was 49 ± 8.54 U/mg protein, which was significantlyhigher than in the sham-operated animal (26.02 ± 1.23 U/mg protein).Measured in samples taken from the same animals, the catalaseactivity in the brain showed a similar pattern. Brain catalaseactivity increased to 7.61 ± 0.88 U/mg protein after myocardialischemia-reperfusion, whereas that of the sham-operated animalwas 4.84 ± 0.22 U/mg protein. On the other hand, the catalaseactivity in the liver was not altered by myocardial ischemia-reperfusion(Fig. 5).

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Fig. 5. Changes in catalase activity in the heart (A), brain (B), and liver (C) after regional myocardial ischemia. Rabbits were subjected to 15 min of regional myocardial ischemia. Tissue samples from the heart, brain, and liver were taken 1 h after the onset of reperfusion for assays of catalase. For the sham-operation group, all operative procedures were performed identically, except for the occlusion of coronary artery. I/R, ischemia-reperfusion. * P < 0.05.

Changes in Catalase Activity in Heart, Brain, and Liver After Regional Intestinal Ischemia

In another series of experiments, intestinal ischemia by occlusion of the superior mesenteric artery was employed. Rabbitswere subjected to intestinal ischemia for 15 min followed by 1h of reperfusion. As with myocardial ischemia, intestinal ischemia-reperfusionevoked increased catalase activity in the heart and brain. Thedegree of catalase activation was comparable to that in the myocardialischemic stress group. Liver catalase activity was not affectedby intestinal ischemia (Fig. 6).

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Fig. 6. Changes in catalase activity in the heart (A), brain (B), and liver (C) after intestinal ischemia. Rabbits were subjected to 15 min of superior mesenteric artery (SMA) occlusion. Tissue samples from the heart, brain, and liver were taken 1 h after the onset of reperfusion for assays of catalase. For the sham-operation group, all operative procedures were performed identically, except for the occlusion of the artery. * P < 0.05.

Effect of Adrenergic Antagonists on Catalase Activation by Regional Myocardial Ischemia

It was tested whether stimulation of catalase in the heart and brain by myocardial ischemia could be inhibited by adrenergicreceptor blockade. After pretreatment with prazosin, an $alpha$ -adrenergicreceptor antagonist, ischemia-reperfusion failed to increase catalaseactivity in the heart and brain. However, propranolol, a $beta$ -adrenergicreceptor antagonist, did not exert any influence on catalase activity.The catalase activity in the liver was not altered by any intervention(Fig. 7).

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Fig. 7. Effect of adrenergic antagonists on the catalase activation by regional myocardial ischemia. Rabbits were subjected to 15 min of regional myocardial ischemia. Tissue samples from the heart (A), brain (B), and liver (C) were taken 1 h after the onset of reperfusion for assays of catalase. For the sham-operation group, all operative procedures were performed identically, except for the occlusion of the coronary artery. PN-I/R, treatment with prazosin (2 mg/kg) before I/R; PL-I/R, treatment with propranolol (2 mg/kg) before I/R. * P < 0.05.

Effect of Adrenergic Agonist on Catalase Activity in Heart, Brain, and Liver

Norepinephrine, administered for 10 min intravenously, increased catalase activity in the heart to 66.81 ± 16.69 U/mg proteinand the brain to 8.34 ± 0.77 U/mg protein. The degree of catalaseactivation was higher than that observed in animals subjectedto regional myocardial ischemia-reperfusion. Moreover, norepinephrinealso increased the catalase activity in the liver from 237.36± 12.74 to 305.03 ± 17.79 U/mg protein (Fig. 8).

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Fig. 8. Effect of adrenergic agonist on catalase activity in the heart (A), brain (B), and liver (C). Norepinephrine (NE) was dissolved in normal saline at a concentration of 2.5 µg/ml, and 10 µg/kg were infused continuously for 10 min. Tissue samples from the heart, brain, and liver were taken in 1 h for assays of catalase. Con, control. * P < 0.05 vs. control.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The antioxidant enzyme-mediated defense mechanism against reactive oxygen metabolites is essential to all cells under oxygenatedenvironments. The regulatory machinery of the antioxidant systemin prokaryotes is well documented (9, 10). Although the knowledgeabout the responsive regulation of mammalian antioxidant enzymesis limited, it has been reported (3, 6, 7, 21, 24)that the endogenous antioxidant defense system could be activatedby various modalities of sublethal stresses. In the present study,we observed increased catalase activity and mRNA expression after1-h reperfusion following brief ischemia, which is similar tothe results of some previous reports (4, 7). Surprisingly,however, catalase activity and mRNA expression were increasednot only in affected ischemic myocardium but also in nonischemicmyocardium and were comparable indegree.

The simultaneous activation of catalase in the nonischemic and ischemic regions of the heart implies that a certain signalgenerated by regional ischemia and/or reperfusion influences notonly the affected ischemic-reperfused part of the myocardium butalso the adjacent normally perfused myocardium to stimulate catalase.An increased oxidative stress could trigger the antioxidant defensesystem to be induced in tissues. We thus hypothesized that myocardialcatalase activity would increase in association with an increasedoxidative stress mediated by increased production of reactiveoxygen species during ischemia and reperfusion. However, we failedto detect any evidence of altered redox state as there were nochanges in the GSH and GSSG contents in either the ischemic orthe nonischemic myocardium. It was, therefore, suggested thatsome factor(s) other than the oxidative stress incurred by theischemia-reperfusion might be involved in the activation of catalasein both areas. Involvement of systemic stress caused by operativeprocedures other than the coronary artery occlusion was excludedas there were no changes in either the enzyme activity or mRNAexpression in the sham-operatedanimals.

The signal transmission responsible for the stimulation of catalase in the nonischemic and ischemic myocardium would involvea local myocardial pathway or systemic pathway. For the localpathway, we proposed several hypotheses. First, a kind of chemicalmediator produced in the ischemic area might diffuse to the nonischemicarea through interstitial space or gap junctions to stimulatecatalase simultaneously in both areas. In another possibility,alterations in myocardial contractility by ischemia-reperfusionmight stimulate both areas mechanically to result in some changesin enzyme activity. However, these hypotheses were presumed lessprobable as the observed catalase stimulation was uniform whilethe effects of diffusing chemical mediators or mechanical stimuliwere not presumed to be uniform in two distantareas.

Therefore, we supposed that the catalase activation in the nonischemic region of the heart is probably the result of a certainsignal originating from the systemic pathways. To test this hypothesis,we observed whether catalase activity in other organs is alsoinfluenced by this signal in the same manner as the nonischemicmyocardium. Catalase activity in the brain as well as in the heartwas found to be increased, indicating that the signaling pathwayinvolves a systemictransmission.

Moreover, ischemic stress to the intestine was equipotent to myocardial ischemia-reperfusion in catalase activation, showingthat the hypothesized signaling pathway triggered by ischemicstimulus is not confined to the myocardium. Gho et al. (11)have quantitated the ischemic stress-induced protective effectagainst cardiac ischemia-reperfusion injury, in which they comparedthe ischemic stresses to the heart, intestine, and kidney in rabbits.It was reported (11) that 15-min coronary artery occlusion and15-min mesenteric artery occlusion were equally effective to limitthe infarct size after lethal myocardial ischemia-reperfusion.

For the next step, we sought to find the transmitter of this signaling pathway. Systemic catalase activation by ischemia ispresumed to be a kind of stress adaptation mechanism. As the primarysystems activated in response to stressful stimuli, sympatheticnervous system and several stress hormones are well known. Amongthese, we tested whether the adrenergic nervous system is involved.We found that pretreating animals with prazosin abolished thecatalase activation, suggesting that the $alpha$ -adrenergic receptorpathway is involved. In addition, intravenous norepinephrine administrationinstead of ischemia-reperfusion induced catalase activation inthe heart, brain, and liver. Transient hypertension induced bynorepinephrine might have exerted mechanical stimuli on the myocardium,but this presumably did not contribute to the effect on catalaseactivity, as the simultaneous catalase activation in the brainand liver was not attributable to hemodynamic alterations. Fromthese results, we concluded that the $alpha$ -adrenergic receptor isa part of the signaltransmission.

However, we couldn't clarify whether the $alpha$ -adrenergic agonist itself induces catalase activation of the target cells or playsa role in transmitting the signal to another signaling system.The assumption that the $alpha$ -adrenergic system is not the final effectoris supported by the pharmacological properties of norepinephrine.Because of the low permeability to the blood-brain barrier, intravenousnorepinephrine cannot reach the brain parenchymal cells in aneffective concentration. Therefore, it is hardly possible thatintravenous norepinephrine directly acts on the brain cells toinduce catalaseactivation.

Catalase and other antioxidant enzymes are fundamental proteins expressed in all aerobic organisms, including prokaryotesand plants. However, the regulation mechanism of these enzymesin animals is mostly unknown, whereas that of prokaryotes is relativelywell known. The results of the present study could shed lighton the physiological regulation mechanism of catalase activity.For example, the catalase activity of the liver showed a responsepattern different from that of the heart and brain. Although thecatalase activity of the heart and brain was responsive to theendogenous signal originating from myocardial ischemia-reperfusion,the catalase activity of the liver was not increased under thesame conditions. However, the catalase activity of the liver wasresponsive to intravenous norepinephrine as was that of the heartand brain. These results imply that the regulation machinery ofdifferent organs might differ in sensitivity to the endogenouscatalase-activatingsignal.

The present study suggests the involvement of the adrenergic system, but we still do not know the signal transmission stepsbetween ischemia-reperfusion and adrenergic activation or betweenadrenergic activation and systemic catalase activation. For themechanism of adrenergic activation by ischemia-reperfusion, severalrelated phenomena have been reported. Numerous biological alterationsmight be induced by ischemia-reperfusion, but among these, theincreased production of adenosine is most conspicuous. Endogenousadenosine production is increased in response to a decrease inoxygen supply-to-demand ratio as ATP degradation is accelerated(19). Adenosine is known to possess various biological activitiesto reduce the deleterious effects of ischemia-reperfusion (17),and at the same time, stimulate sympathetic afferents to increasesystemic sympathetic activity. Therefore, it is probable thatadenosine mediates the sympathetic activation following catalaseactivation.

Further research is required to understand the signal transmission step(s) between adrenergic activation and catalase activation.A hormonal factor such as glucocorticoid could participate inthe enzyme activation. Glucocorticoid is known to be releasedin response to physiological stress or sympathetic stimulation,and it has also been known to induce antioxidant enzymes, includingcatalase (15).

Another facet of the phenomenon attracting interest is the relation with so-called "ischemic preconditioning." It has beenknown for a long time that brief ischemia renders the heart resistantto subsequent severe ischemia-reperfusion. This phenomenon, knownas ischemic preconditioning, is the most promising among the experimentalmethods currently known to reduce ischemia-reperfusion injury(20, 23, 24). However, many questions about the mechanismof ischemic preconditioning are still unknown. Although the protocolof the present experiment is different from that of conventionalischemic preconditioning, catalase activation is likely to contribute,at least in part, to cardioprotection against ischemia-reperfusion.However, in a study using an in situ regional ischemia model ofrabbit hearts, Turrens et al. (28) reported that the activityof the major myocardial antioxidant enzymes, including catalase,was not changed in either the ischemic or nonischemic regions.This result is not consistent with our findings. The apparentdiscrepancy may be explained by the different experimental protocols.Turrens et al. (28) measured the antioxidant enzyme activity5 min after reperfusion following 30 min of ischemia, whereaswe did so after 1-8 h of reperfusion following 15 min of ischemia.Immediately on reperfusion after ischemia, we did not observeany significant changes in the antioxidant enzyme activity either.Hence, more detailed studies are required to clarify theissue.

In conclusion, brief regional myocardial ischemia induced catalase activation in the nonischemic myocardium and brain as wellas the ischemic myocardium, and the $alpha$ -adrenergic system was involvedin the systemic signaltransmission.

Perspectives

Numerous reports have indicated that antioxidant enzymes, including catalase, can be enhanced by sublethal experimental stimuli(25). However, as far as we know, this is the first report demonstratingthat catalase activation can be achieved through endogenous systemicsignaling pathways. This finding implies the existence of an inherentregulatory mechanism that maximizes the antioxidant capacity ofmultiple remote organs in response to oxidativestimuli.

Further research on the signal transmission pathway of systemic catalase activation may lead to the development of usefulpharmacological methods to activate the endogenous antioxidantdefense system in target organs. Through these medical interventions,we may be able to pretreat patients, who are to be subjected toinevitable oxidative injury like open heart surgery, organ transplantation,radiation therapy, and Adriamycin therapy, to minimize the problemsof oxidativeinjury.

	ACKNOWLEDGEMENTS

This study was partly supported by grants from the Korean Science and Engineering Foundation (2000) and the Ministry of Scienceand Technology, Korea(2000).

	FOOTNOTES

Address for reprint requests and other correspondence: M.-S. Kim, Dept. of Pharmacology, College of Medicine, Seoul NationalUniv., 28 Yongon-dong, Chongno-gu, Seoul 110-799, Korea (E-mail:kimmsu{at}snu.ac.kr).

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.Section 1734 solely to indicate thisfact.

10.1152/ajpregu.00278.2001

Received 15 May 2001; accepted in final form 10 January 2002.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

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