Evidence against a Cytochrome P450-Derived Reactive Oxygen Species as the Mediator of the Nitric Oxide-Independent Vasodilator Effect of Bradykinin in the Perfused Heart of the Rat

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Vol. 280, Issue 2, 702-709, 1997

Evidence against a Cytochrome P450-Derived Reactive Oxygen Species as the Mediator of the Nitric Oxide-Independent Vasodilator Effect of Bradykinin in the Perfused Heart of the Rat¹

D. Fulton, J. C. McGiff, M. S. Wolin, P. Kaminski and J. Quilley

Departments of Pharmacology (D.F., J.C.M., J.Q.) and Physiology (M.S.W., P.K.), New York Medical College, Valhalla, New York

	Abstract

Top Abstract Introduction Methods Results Discussion References

The coronary vasodilator effect of bradykinin (BK) in the rat is independent of NO but dependent on activation of phospholipaseswith involvement of cytochrome P450 mono-oxygenase (P450) andstimulation of Ca⁺⁺-activated K⁺ channels, implicating an unidentified hyperpolarizing factorgenerated via P450 metabolism of arachidonic acid (AA). BecauseP450 activity also generates free radicals, such as superoxide,which can lead to the formation of hydrogen peroxide and hydroxylradicals, which are vasoactive, we addressed the contributionof superoxide to the vasodilator effect of BK in the rat heart.Using rat renal microsomes as a source of P450, we verified thatP450-dependent metabolism of AA generated superoxide, as detectedby chemiluminescence with lucigenin. The signal was almost abolishedby inhibition of P450 with clotrimazole and the superoxide scavenger4,5-dihydroxy-1,3-benzene sulfonic acid. However, base-line superoxideformation, detected by chemiluminescence, in cardiac slices andperfused hearts was unchanged in response to BK or AA. Furthermore,in perfused hearts treated with nitroarginine and indomethacinto eliminate NO and prostaglandins and elevate perfusion pressure,dose-dependent vasodilator responses to BK were unaffected bysuperoxide dismutase plus catalase, a combination that abolisheddilator responses to hydrogen peroxide. Similarly, the superoxidescavengers 4,5-dihydroxy-1,3-benzene sulfonic acid and 4-hydroxy-2,2,6,6-tetramethylpiperidine-noxylwere without effect on vasodilator responses to BK. Thus, thecoronary vasodilator action of BK is independent of superoxideor its derivatives, which can be excluded as hyperpolarizing factorsmediating NO-independent vasodilation in the rat.

	Introduction

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Endothelium-dependent vasodilation is generally attributed to the release of NO (Furchgott and Zawadski, 1980; Ignarro etal., 1987; Palmer et al., 1987). However, depending on the species,vascular tissue and agonist, endothelium-dependent, but NO-independent,vasodilation can be observed, an effect attributed to the releaseof a hyperpolarizing factor (Chen et al., 1988; Komori et al.,1988; Pacicca et al., 1992), the identity of which remains tobe elucidated. Our studies using the perfused heart and kidneyof the rat provide evidence for a P450-derived product of AA asthe mediator of BK-induced vasodilation that is independent ofNO and prostaglandins (Fulton et al., 1992, 1995). Thus, responsesto BK, which is a recognized stimulus for phospholipases, areattenuated by inhibitors of P450 and abolished by inhibitors ofboth phospholipase A₂ and phospholipase C (Fulton et al., 1996).Of the P450 metabolites, an epoxide (EET) is considered the mostlikely candidate for a hyperpolarizing factor, an idea supportedby several recent reports (Bauersachs et al., 1994; Campbell etal., 1996; Hecker et al., 1994). Epoxides are vasodilators thatare synthesized by the endothelium and act via Ca⁺⁺-activated K⁺ channels (Hu and Kim, 1993; Rosolowsky et al., 1991; Zou et al.,1994). Furthermore, in the coronary perfusate, we detected EETsby gas chromatography-mass spectometry, whereas products of theother pathway of P450-dependent AA metabolism, the HETEs, couldnot be detected under basal or stimulated conditions (Fulton etal., 1995). Nevertheless, the vasodilator potency of EETs in thekidney and heart is less than would be anticipated for a putativemediator of the vasodilator effect of BK; microgram quantitiesare required (Fulton et al., 1996), whereas nanogram quantitiesof BK elicit maximal dilation (Fulton et al., 1992). Therefore,we also considered the possibility that a by-product of P450-dependentmetabolism of AA (i.e., a free radical) could contribute to thevascular action of BK because it exhibits absolute dependencyon phospholipases and also involves mono-oxygenase activity (Fultonet al., 1995,1996). BK has been shown to stimulate the releaseof superoxide from endothelial cells and feline and murine cerebralarterioles (Holland et al., 1990; Kontos et al., 1990; Rosenblum,1987; Shimizu et al., 1994). Several sources of superoxide generationwithin endothelial cells have been identified and encompass NAD(P)H-dependentelectron transport chains, mitochondria, xanthine oxidase andAA oxygenases, including cyclo-oxygenase and lipoxygenase (Wolin,1996). Similarly, reactions involving P450 generate superoxide(Bondy and Naderi, 1994), although this has not been establishedfor isozymes that metabolize AA. The promiscuous reactivity ofsuperoxide results in the genesis of other reactive oxygen species(Kukreja and Hess, 1992). Products of superoxide (i.e., hydrogenperoxide and hydroxyl radicals) induce vasodilation in a varietyof vessels, and hydrogen peroxide hyperpolarizes endothelium-denudedporcine coronary arteries (Beny and von der Weid, 1991). Consequently,we investigated whether free radicals generated via P450-dependentmetabolism of AA could fulfill the requirements as a mediatorof endothelium-dependent, but NO-independent, vasodilation toBK in the rat heart. Thus, in this preparation, vasodilator responsesto BK are independent of NO but susceptible to inhibitors of P450and K⁺ channels (Fulton et al., 1995, 1994). We first established thatP450-dependent metabolism of AA could generate superoxide andthen addressed the release of superoxide from the perfused heartin response to BK. Finally, we determined the effects of intracellularand extracellular free radical scavengers on vasodilator responsesto BK in the perfused rat heart in which NO and prostaglandinsynthesis was inhibited to isolate the P450-dependent componentof the response. The results provide evidence against an oxygen-derivedfree radical as the mediator of the coronary vasodilator effectof BK.

	Methods

Top Abstract Introduction Methods Results Discussion References

Renal cortical microsomes were used as a source of P450 to examine whether P450-dependent metabolism of AA generates superoxide.Male Wistar rats (300-400 g) were anesthetized with pentobarbital(65 mg/kg), and after a midline laparotomy, the aorta was cannulatedbelow the renal arteries and ligated above the renal arteries.The kidneys were flushed free of blood with 0.9% saline and excised,and the cortex was separated and homogenized in Tris/sucrose buffer.The suspension was centrifuged at 10,000 × g for 15 min, and theresultant supernate was centrifuged at 100,000 × g for 60 min.The resulting pellet was washed twice and resuspended in potassiumphosphate buffer (0.1 M), and the protein concentration was determinedusing the BioRad (Hercules, CA) method.

Microsomes (150 µg), suspended in Krebs-Henseleit buffer, pH 7.4, containing 10 mM HEPES, 2.8 µM indomethacin, 250 µM lucigeninand 250 µM NADPH, were incubated with and without AA (10 µg),clotrimazole (10 µM) as an inhibitor of P450 or its vehicle (ethanol,1%), and scavengers of superoxide, Tiron (10 mM) and SOD (400U/ml). The concentration of clotrimazole was 10-fold that previouslyshown to attenuate renal and coronary vasodilator responses toBK (Fulton et al., 1992, 1995) and was used in excess to ensureinhibition of both epoxygenase and $omega$ -hydroxylase (Harder et al.,1995). At 2 min before the reaction, microsomes were resuspendedin 0.885 ml of Krebs' buffer, and inhibitors or respective vehicles(10 µl) were added, followed by NADPH (5 µl) and lucigenin (100µl). The reaction was initiated by the addition of AA, and superoxideproduction was estimated by quantification of lucigenin chemiluminescence(Paky et al., 1993), measured as cpm (0.1-min interval) with aPackard Tricarb 1900TR liquid scintillation analyzer at 2 minafter initiation of the reaction. A positive control was alsoused to address any nonspecific actions of the inhibitors. Thus,0.1 U of xanthine oxidase, suspended in Krebs' buffer, pH 7.4,containing 10 mM HEPES and 250 µM lucigenin, was combined withits substrate, xanthine (100 µM), and tested against the inhibitors.

Cardiac slices were used initially to examine the effects of BK and AA on superoxide production, detected by chemiluminescenceas described above. After anesthesia with pentobarbital (65 mg/kg)and intravenous heparin (1000 U/kg), a thoracotomy was performed,and the heart with attached aorta was excised, flushed free ofblood and immersed in cold saline. The apex, aorta and the topof the atria were removed, and the heart was bisected. Transversesections of cardiac tissue (~150 mg wet weight and ~2 mm thick)were obtained using a tissue slicer. Slices were placed in 7-mlglass scintillation vials containing 1 ml of Krebs' buffer with50 µM nitroarginine, 50 µM NADPH, 10 mM HEPES and 250 µM lucigenin.To increase superoxide release, slices were preincubated for 30min with diethyldithiocarbamate (1 mM) to inhibit endogenous Cu⁺⁺/Zn⁺⁺ superoxide dismutase. Thus, in preliminary studies, slices incubatedin the absence of NADPH and diethyldithiocarbamate did not producea detectable increase in superoxide after stimulation with BKor AA. Lucigenin-enhanced chemiluminescence, an index of superoxideproduction, was monitored as described 2 min after the stimulationof cardiac slices with BK (1 µg) or AA (5 µg).

Perfused heart. Male Wistar rats (weight, 350-400 g) were anesthetized with pentobarbital (65 mg/kg intraperitoneally) and given heparin (1000U/kg). After thoracotomy, the heart was excised and perfused,via an aortic cannula, at constant flow with oxygenated (95% O₂/5%CO₂) Krebs' buffer at 37°C according to the method of Langendorffas modified by Broadley (1979). Flow was adjusted to 9-10 ml/min,which resulted in a basal perfusion pressure of 25-40 mm Hg, whichincreased to ~130-140 mm Hg as a result of nitroarginine (50 µM)in the buffer to which indomethacin (2.8 µM) had also been added.Nitroarginine and indomethacin were included in the perfusateto inhibit NO and prostanoid synthesis, respectively, and isolatethe P450-dependent vasodilator response to BK. The contributionof free radicals to the coronary vasodilator effect of BK wasexamined using various inhibitors of intracellular and extracellularfree radicals. Thus, vasodilator responses to BK (10-1000 ng)were assessed in the absence and presence of SOD (100 U/ml) toscavenge extracellular superoxide and Tiron (3 mM) or TEMPO (0.3mM), superoxide scavengers that gain access to the intracellularmilieu. The concentrations of Tiron and TEMPO that were chosenfor these experiments were determined in preliminary studies tobe devoid of nonspecific effects on vasodilator responses (seebelow). However, to verify that the concentrations of Tiron andTEMPO as well as SOD were effective in scavenging superoxide,we used cardiac slices as described. Basal superoxide production,determined by lucigenin-enhanced chemiluminescence, was abolishedby 3 mM Tiron and reduced by 95% and 72% by 0.3 mM TEMPO and 100U/ml SOD, respectively (n = 2). In experiments using SOD, catalase(400 U/ml) was also included to scavenge hydrogen peroxide. Vasodilatorresponses to cromakalim (5 µg), an ATP-sensitive K⁺ channel opener, or SCA40 (1 µg) or NS1619 (15 µg), agents reportedto stimulate Ca⁺⁺-activated K⁺ channels, and in some cases hydrogen peroxide (60 µg), were alsoexamined to assess any effects of the inhibitors unrelated toinhibition of free radicals as well as to assess the effectivenessof the various interventions.

To address release of free radicals in response to BK, the procedure was slightly modified to include a single-photon-countingapparatus constructed in a light-tight sealed box (Mohazzab-Het al., 1996

). After cannulation of the aorta, the heart (fromrats of weight 200 g) was placed in a cuvette (1 cm² spectrophotometer cuvette; Fisher, Springfield, NJ) and mountedin a thermostat-controlled (37°C) cell holder on the surface ofLucite light guide (with a shutter cover), directed into a cooled( $-$ 12°C) Thorn EMI photomultiplier tube (model 9235B). The heartwas positioned such that the left ventricle was facing the photomultiplier.A Thorn EMI amplifier-discriminator (model C604) and photon counter(model C660) were used to quantify chemiluminescence. Counts wereintegrated over 5-sec periods by the photon counter, and an analogsignal of the integrated counts was continuously recorded on apolygraph recorder (Grass, model 7) together with coronary perfusionpressure. Suction and gas lines were placed in the cuvette tocontrol the level of perfusate (4 ml) and manipulate the oxygentension. Once a stable perfusion pressure was obtained, the perfusateof oxygenated (5% CO₂/balance air) Krebs' buffer was switchedto Krebs' buffer containing lucigenin (250 µM) and and recirculated.After several minutes of recirculation, the shutter on the photonmultiplier was opened, and chemiluminescence was measured. Vascularresponses to BK (1 µg), cromakalim (5 µg) and AA (5 µg) were thendetermined. As a positive control for the detection of endogenoussuperoxide formation, the heart was subjected to a 15-min periodof hypoxia (cessation of flow and gassing with nitrogen) followedby reoxygenation (return of flow and oxygen).

Materials. The following reagents, which were obtained from the Sigma Chemical (St. Louis, MO), were dissolved in deionized water beforeuse: Tiron, TEMPO, SOD, catalase, xanthine, xanthine oxidase,lucigenin (bis-N-methylacridinium nitrate), 1,3-dimethyl-2-thiourea,BK, sodium nitroprusside and nitroarginine. Clotrimazole, cromakalimand indomethacin were also obtained from Sigma and were dissolvedin ethanol, acetone and 4.2% NaHCO₃, respectively. Clotrimazolewas subsequently diluted with water. SCA 40, a gift from Dr. Cervoni(American Home Products, Pearl River, NY), was dissolved in 10%ethanol, and NS1619, obtained from Research Biochemicals International(Natick, MA), was dissolved in ethanol and diluted with water.Sodium arachidonate from NuChek (Elysian, MN) was dissolved inwater, divided into aliquots, sealed under nitrogen, and storedat $-$ 70°C.

Data analysis. Results are presented as mean ± S.E.M. Data were compared by analysis of variance, and individual values were compared byNeuman-Keuls test. A value of P < .05 was considered statisticallysignificant.

	Results

Top Abstract Introduction Methods Results Discussion References

P450. The addition of AA to indomethacin-pretreated renal cortical microsomes, a rich source of P450 mono-oxygenases, produced a5-fold increase in lucigenin-enhanced chemiluminescence (an indexof superoxide production) over the control value (vehicle-treatedmicrosomes). The increase in chemiluminescence was abolished bythe P450 inhibitor clotrimazole (fig. 1). The scavengers of superoxide,SOD (extracellular) and Tiron (intracellular and extracellular),significantly reduced lucigenin-enhanced chemiluminescence, withTiron being the most effective (fig. 1). The effects of theseagents were also tested on a known superoxide-generating system,xanthine and xanthine oxidase, which significantly increased chemiluminescence.The increase was inhibited by both SOD and Tiron but was not affectedby clotrimazole (fig. 1).

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Fig. 1. Lucigenin-enhanced chemiluminescence as an index of superoxide production by (A) rat renal cortical microsomes in the presenceof AA (10 µg; n = 15) and (B) xanthine oxidase (XO) in the presenceof xanthine (X; 100 µM; n = 8). Effects of clotrimazole (CTZ;10 µM, n = 6), SOD (400 U/ml; n = 7 for microsomes and n = 5 forXO) and Tiron (10 mM; n = 7 for microsomes and n = 5 for XO).Results are expressed as the increase in chemiluminescence fromthe respective controls without AA or xanthine. P < .01 relativeto vehicle-treated microsomes (A) or vehicle-treated xanthineoxidase (B).

Cardiac slices. Superoxide production, estimated by lucigenin-enhanced chemiluminescence, was subsequently investigated in cardiac slicesstimulated with BK and AA. The addition of either agent was withouta significant effect in stimulating superoxide production. Thus,chemiluminescence was 31 ± 4 × 10⁴ cpm for the control vs. 25 ± 5 × 10⁴ cpm and 26 ± 4 × 10⁴ cpm for slices stimulated with AA and BK, respectively. In theabsence of NADPH, chemiluminescence was 11 ± 2 × 10⁴ cpm for the control compared with 12 ± 2 × 10⁴ cpm for the corresponding slices treated with BK.

Perfused heart. Figure 2 is a representative tracing from six experiments of the simultaneous recording of perfusion pressure and lucigenin-enhancedchemiluminescence. Administration of BK, AA and cromakalim produceddilation of the coronary circulation but failed to increase theamount of lucigenin chemiluminescence detected. Consequently,we tested the effects of hypoxia and reoxygenation on the productionof superoxide to validate this method of detection using an isolatedheart. Interruption of coronary flow and reduced O₂ tension resultedin a rapid decline in both the perfusion pressure and the chemiluminescencesignal. Reperfusion and reoxygenation elicited a rapid rise inperfusion pressure and a dramatic increase in luminescence (fig.2).

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Fig. 2. Representative tracing from six experiments of simultaneous recordings of perfusion pressure- and lucigenin-enhanced chemiluminescencefrom the isolated, perfused heart of the rat showing the effectsof BK (1 µg), AA (5 µg), cromakalim (CK; 5 µg) and hypoxia (stopflow) followed by reperfusion (start flow). The perfusate containednitroarginine (50 µM) to inhibit NO synthesis and elevate perfusionpressure from 30 to 40 mm Hg to 130-140 mm Hg.

Perfused heart and radical scavengers. Vasodilator responses to BK, SCA40 and hydrogen peroxide were determined in nitroarginine- and indomethacin-treated hearts,and the effects of free radical scavengers were assessed. In someexperiments, responses to NS 1619, an opener of Ca⁺⁺-activated K⁺ channels, were also assessed. This agent was included becauseit, unlike SCA40, has been shown to directly activate these channels(Macmillan et al., 1995).

Inclusion of SOD and catalase in the coronary perfusate did not affect vasodilator responses to BK or SCA40, whereas responsesto hydrogen peroxide were abolished (fig. 3). Similarly, vasodilatorresponses to BK were unaffected by Tiron or TEMPO, scavengersof superoxide that penetrate to intracellular sites (fig. 4A).Neither of these agents affected vasodilator responses to theK⁺ channel openers SCA40, cromakalim or NS 1619 (fig. 4B).

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Fig. 3. Effect of SOD (400 U/ml) plus catalase (400 U/ml), denoted by open bars (n = 6), and vehicle (solid bars; n = 6) on vasodilatorresponses to BK, SCA40 and hydrogen peroxide (H₂O₂) in isolated,perfused hearts treated with indomethacin (2.8 µM) and nitroarginine(50 µM) to elevate perfusion pressure (PP) from ~40 mm Hg to 140mm Hg. ** P < .01 vs. control.

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Fig. 4. Effect of Tiron (3 mM; hatched bars; n = 4) and TEMPO (0.3 mM; open bars; n = 4) on (A) BK-induced vasodilation and (B) vasodilationin response to NS1619, SCA40 and cromakalim in the isolated, perfusedrat heart treated with indomethacin (2.8 µM) and nitroarginine(50 µM) to elevate perfusion pressure from ~40 mm Hg to 140 mmHg. * P < .05 compared with control (solid bars; n = 4).

To examine a role of hydroxyl radicals in the action of BK, the scavenger, dimethylthiourea was used. This agent did not affectvasodilator responses to BK (e.g., in the presence of DMTU, 100ng BK reduced perfusion pressure by 67 ± 9 mm Hg compared with57 ± 5 mm Hg in the control group).

	Discussion

Top Abstract Introduction Methods Results Discussion References

We have thus far shown that BK-induced vasodilation in the isolated perfused heart of the rat is independent of NO but susceptibleto inhibitors of P450 (Fulton et al., 1995) and phospholipases(Fulton et al., 1996) and is mediated via activation of a charybdotoxin-sensitiveK⁺ channel (Fulton et al., 1994), results that are consistent witha P450-dependent metabolite of AA as an endothelium-derived hyperpolarizingfactor. Indeed, a series of recent reports support this interpretation,providing evidence for an EET as a hyperpolarizing factor (Bauersachset al., 1994; Campbell et al., 1996; Hecker et al., 1994). EETshave been shown to be vasorelaxant and to increase the open probabilityof Ca⁺⁺-activated K⁺ channels (Rosolowsky et al., 1991; Hu and Kim, 1993; Zou et al.,1994). However, the relative lack of vasodilator potency of EETsin isolated preparations prompted us to examine other productsof P450-dependent metabolism of AA as putative mediators of NO-independentvasodilation to BK.

It is well established that P450-dependent mechanisms generate free radicals as by-products and that free radicals or theirderivatives exhibit vasoactivity (Bondy and Naderi, 1994; Rosenblum,1987). For example, superoxide can result in the formation ofhydrogen peroxide, which is a vasodilator and stimulates K⁺ channels (Beny and von der Weid, 1991). Furthermore, the dilatoreffect of BK in cat cerebral arterioles has been attributed tofree radicals generated via cyclo-oxygenase metabolism of AA (Kontoset al., 1990), which is released consequent to phospholipase stimulationby the peptide. Therefore, in this study, we examined the potentialcontribution of free radicals, generated by P450-dependent conversionof AA, to the coronary vasodilator effect of BK in the rat heart.Our approach was to first establish that P450-dependent metabolismof AA resulted in the formation of free radicals and, subsequently,to determine whether BK stimulated the release of superoxide inthe heart and whether free radical scavengers modified the P450-dependentvasodilator effect of the peptide.

Using rat renal cortical microsomes as a source of P450, we verified, using lucigenin-enhanced chemiluminescence, that metabolismof AA by P450, like other P450-dependent reactions, resulted inthe formation of superoxide. The addition of AA to microsomespretreated with indomethacin to eliminate cyclo-oxygenase activitystimulated an increase in chemiluminescence that was inhibitedby clotrimazole and scavengers of superoxide, confirming boththe source and identity of superoxide. Although both scavengersof superoxide, Tiron and SOD, were equally efficacious in reducingsuperoxide generated by xanthine oxidase, Tiron was much moreeffective against superoxide produced by renal microsomes. Thispresumably relates to the ability of Tiron, but not SOD, to penetratelipid membranes and therefore scavenge intravesicular superoxide(Ledenev et al., 1986).

Cultured endothelial cells, which lose the ability to express P450, generate superoxide in response to BK as a result of cyclo-oxygenase-dependentmetabolism of AA (Holland et al., 1990; Shimizu et al., 1994).To evaluate a potential role of superoxide generated by P450,we obtained measurements of superoxide from freshly isolated tissuesstimulated with BK. However, we were unable to demonstrate increasesin superoxide release in cardiac slices pretreated with indomethacinand nitroarginine to inhibit cyclo-oxygenase and NO synthase andmimic the conditions under which we have demonstrated P450-dependentcoronary vasodilation to BK (Fulton et al., 1995). To improvethe sensitivity of superoxide measurements and to associate changesin perfusion pressure with superoxide levels, hearts were placedin a light-shielded box in close apposition to a photon multiplierso that simultaneous changes in perfusion pressure and superoxidecould be monitored (Mohazzab-H et al., 1996). However, the P450-dependentvasodilator action of BK was not associated with increases insuperoxide. Thus, BK elicited a vasodilator response in the perfusedheart that was not associated with a increase in lucigenin-enhancedchemiluminescence. Furthermore, metabolism of AA by cyclo-oxygenase,an established source of superoxide, also failed to increase thechemiluminescent signal. However, the method of detection doesnot appear to be a limitation in that reperfusion of the heartafter a period of hypoxia, a known stimulus for superoxide formation,resulted in a dramatic increase in superoxide, 5-fold base-line,demonstrating that endogenously produced superoxide can be detectedusing this method. Consequently, the results suggest that BK doesnot stimulate the formation of superoxide or its derived metabolitesfrom the heart in sufficient quantities to account for the vasculareffects. Nevertheless, to exclude the possibility that undetectedchanges in superoxide or its derivatives contribute to the coronaryvasodilator action of BK, we determined the effect of variousscavengers of superoxide on the dilator response in the perfusedheart. The combination of enzymes, SOD and catalase, scavengersof superoxide and hydrogen peroxide, respectively, were withouteffect on the vasodilator response to BK but abolished that tohydrogen peroxide, showing that effective concentrations wereused. These results, which tend to exclude superoxide and hydrogenperoxide as potential mediators of BK-induced dilation, shouldbe interpreted with the knowledge that SOD and catalase do notreadily cross cell membranes and may not access sites of intracellularsuperoxide production (Beckman et al., 1988). However, the lackof effect of these agents on BK-induced vasodilation is good evidenceagainst an endothelium-derived reactive oxygen species that isreleased to exert its effect on the underlying smooth muscle.Furthermore, free radical scavengers that do penetrate to intracellularsites, Tiron and TEMPO, were also without effect on the coronaryvasodilator action of BK. These results indicate that althoughP450-dependent metabolism of AA generates superoxide, it doesnot contribute to the vasodilator action of BK and is in agreementwith those of Beny and von der Weid (1991), who excluded hydrogenperoxide as the hyperpolarizing factor mediating the vasodilatoreffect of BK.

In conclusion, we have demonstrated that the P450-dependent coronary vasodilator response to BK that requires the activationof phospholipases and Ca⁺⁺-activated K⁺ channels is not associated with the release of superoxide andis not affected by scavengers of reactive O₂ species. By exclusion,these observations further support the role of a P450-derivedmetabolite of AA, most probably an EET, as the putative hyperpolarizingfactor that mediates the vasodilator effect of BK in the rat heart.

	Footnotes

Accepted for publication October 28, 1996.

Received for publication August 8, 1996.

¹ This work was supported by National Institutes of Health grants RO1-25394, RO1-49275 and PO1-43023 and AHA grant 940-318.

Send reprint requests to: Dr. J. Quilley, Department of Pharmacology, New York Medical College, Valhalla, NY 10595.

	Abbreviations

BK, bradykinin; P450, cytochrome P450; AA, arachidonic acid; SOD, superoxide dismutase; TEMPO, 4-hydroxy-2,2,6,6-tetramethylpiperidine-noxyl; NO, nitric oxide; EET, epoxyeicosatrienoic acid; Tiron, 4,5-dihydroxy-1,3-benzene sulfonic acid; HEPES, 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid.

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