Intravasal Peroxynitrite Generation Causes Dysfunction in the Isolated Perfused Rat Lung via Endothelin

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Vol. 297, Issue 1, 128-132, April 2001

Intravasal Peroxynitrite Generation Causes Dysfunction in the Isolated Perfused Rat Lung via Endothelin

Katja Eichert, Jürg Hamacher, Michael Andreas Wunder and Albrecht Wendel

Biochemical Pharmacology, Department of Biology, University of Konstanz, Konstanz, Germany

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

In septic shock excessive nitric oxide and superoxide are produced, thus generating peroxynitrite. This study investigateswhether and how intravasal peroxynitrite causes lung dysfunction.To generate peroxynitrite, isolated and ventilated rat lungs wereperfused blood-free in a pressure-constant, recirculating modewith hypoxanthine/xanthine oxidase plus sodium nitroprusside.Airway and vascular resistance, and release of thromboxane A₂,prostacyclin, and endothelin-1 were assessed over 200 min. Peroxynitritegeneration, as demonstrated by oxidation of the marker 2',7'-dichlorodihydrofluoresceindiacetate, caused broncho- and vasoconstriction starting after100 min. Both reactants alone, i.e., NO^· or O &cjs1138; ₂, had no effect. The thromboxane A₂/prostaglandin H₂ receptorantagonist BM13.177 did not affect peroxynitrite-induced broncho-and vasoconstriction. Combined endothelin_A/B (ET_A/B) receptorantagonism (BQ123 plus BQ788) prevented broncho- and vasoconstrictionmore effectively than the ET_A receptor antagonist BQ123 alone.In tissue from lungs exposed to peroxynitrite, significantly increasedamounts of endothelin-1 were detected. This study identifies endothelin-1rather than prostanoids as a distal mediator induced by the reactionproduct of superoxide and nitric oxide, i.e., peroxynitrite. Itis concluded that 1) endothelin-1 is a causal mediator of peroxynitrite-inducedacute rat lung injury, and 2) peroxynitrite-induced broncho- andvasoconstriction are mediated by both ET_A and ET_Breceptors.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Oxidant-mediated tissue injury and impaired vascular and bronchial function play a prominent role in pulmonary dysfunctionassociated with syndromes such as acute respiratory distress syndrome(ARDS) (Haddad et al., 1994; Kooy et al., 1995; Lamb et al., 1999)and ischemia-reperfusion injury (Eckenhoff et al., 1992). Underthese conditions, the rates of superoxide (O &cjs1138; ₂) and nitric oxide(NO^·) released from activated inflammatory cells such as macrophagesand neutrophils as well as from enzymes such as inducible NO synthaseare increased, and thus, the potent oxidant peroxynitrite maybe formed. There is widespread evidence that reactive oxygen speciescause direct cellular damage in different models of acute lunginjury. However, sparse information is available on the endogenousmetabolites of such radical-mediated tissue injury. The toxicityof peroxynitrite is attributed to the rapid reaction of NO^· with O &cjs1138; ₂ (k = 2 × 10¹⁰ M¹ s¹) (Kissner et al., 1997). This kinetics implies that NO^· is capable of outcompeting the O₂ removal via superoxide dismutase,which has a second order rate constant of k = 2 × 10⁹ M¹ s¹ (Royall et al., 1995). On the other hand, this kinetics impliesthat every 10-fold increase in O &cjs1138; ₂ and NO^· formation will cause a hundredfold increase in peroxynitritegeneration. Peroxynitrite has strong oxidizing properties towarda large variety of biological molecules. These reactions includeon the one hand killing of pathogenic microorganisms as a partof the innate host defense (Darrah et al., 2000). On the otherhand peroxynitrite can nitrate free or protein-associated tyrosineresidues and other phenolics (Ducrocq et al., 1999). The detectionof tissue nitrotyrosine residues by specific antibodies is usedas a marker for peroxynitrite action (Crow and Ischiropoulos,1996). Peroxynitrite eventually also leads to sulfhydryl oxidation(Radi et al., 1991a), lipid peroxidation (Radi et al., 1991b),as well as structural and functional alterations of surfactantproteins (Haddad et al., 1993), i.e., to adverse effects on lungfunction. Vasoconstriction is either indirectly initiated viaa diminished release of prostacyclin (PGI₂) or NO^·, or directly via receptor-dependent vasoconstrictors such as,among others, thromboxane and endothelins (ETs). In particular,the extremely potent vasoconstrictor ET-1 and its receptors, whichare abundant in mammalian lung, cause vaso- and bronchoconstrictionand increase vascular permeability (Hay, 1997). Since ET-1 actsvia the two different receptors ET_A and ET_B, we used the selectiveET_A receptor antagonist BQ123 (Ihara et al., 1992) and ET_B receptorantagonist BQ788 (Ishikawa et al., 1994) to discern which receptormediates the ET-1 signal in this model. The roles of thromboxaneA₂/prostaglandin H₂ (TXA₂/PGH₂) and PGI₂ release were also investigated.With peroxynitrite generated intravasally from chemically releasedNO^· and enzymatically formed O &cjs1138; ₂ from hypoxanthine/xanthine oxidase,we investigated the consequences of exposure of the isolated ratlung to peroxynitrite on its functional integrity. Our aims were1) to define the mode and time course of the action of peroxynitriteon lung physiology, and 2) to identify the mediator(s) that causepulmonary dysfunction and corroborate these findings by pharmacologicalinhibitors.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. Pentobarbital sodium (Narcoren) was from Merial GmbH, Hallbermoos, Germany; glucose was from Riedel-de Haën AG, Seelze, Germany;and HEPES was from ICN Biomedicals Inc., Cleveland, OH. DL-Lysine-mono-acetylsalicylicacid (Aspisol) was purchased from Bayer, Leverkusen, Germany.Hypoxanthine (6-hydroxypurine) and xanthine oxidase (XO) [in asuspension of 2.4 M (NH₄)₂SO₄, 1 mM sodium phosphate buffer, 1mM EDTA, and 1 mM sodium salicylic acid, pH 7.8], 2',7'-dichlorodihydrofluoresceindiacetate (DCHF), aprotinin, leupeptin, pepstatin, cycloheximide,and actinomycin D were from Sigma, Deisenhofen, Germany. Sulotroban(BM13.177) was a gift from Roche Diagnostics Inc., Mannheim, Germany.The NO donor sodium nitroprusside (SNP) was purchased from ResearchBiochemicals International, Natick, MA. The ET_A and ET_B receptorantagonists BQ123 and BQ788 were from Alexis Inc., Grünberg,Germany. ET-1 and PGI₂ EIA detection kit were purchased from Biotrend,Köln, Germany. The thromboxane B₂ EIA detection kit, which measuresthe stable secondary product of thromboxane A₂, was obtained fromCayman distributor in Massy Cedex,France.

Isolated Perfused Rat Lung. The lungs of female Wistar rats (weight 200-250 g; Harlan-Winkelmann, Borchen, Germany) were prepared after terminal i.p.anesthesia by 160 mg/kg pentobarbital sodium (Merial GmbH) andperfused as formerly described (Uhlig and Wollin, 1994a). Allequipment was obtained from Hugo Sachs Electronics (March-Hugstetten,Germany). Lungs were perfused at constant hydrostatic pressure(12 cm of H₂O) through the pulmonary artery, which resulted ina flow rate of approximately 35 ml/min. As perfusion medium aKrebs-Henseleit buffer (38°C) containing 2% bovine serum albumin(fraction V; Serva, Heidelberg, Germany), 0.1% glucose (Riedel-deHaën Inc., Seelze, Germany), and 0.3% HEPES (ICN BiomedicalsInc.) was used. The total amount of recirculating buffer was 100ml. The lungs were suspended by the trachea and ventilated bynegative pressure ventilation (inspiratory pressure, $-$ 7 cm ofH₂O; expiratory pressure, $-$ 2 cm of H₂O) with 80 breaths/min, resultingin a tidal volume of approximately 2 ml. Every 5 min a deep inspiratorybreath ( $-$ 20 cm of H₂O) was performed. Artificial thorax chamberpressure was measured with a differential pressure transducer(Validyne DP 45-14), and air flow velocity with a pneumotachographtube (Fleisch type 0000) connected to a differential pressuretransducer (Validyne DP 45-15). The perfusate flow (NarcomaticRT-500) and the arterial and venous pressure (Statham P23BB) werecontinuously monitored. The pH of the perfusate before enteringthe lung was kept at 7.25 to 7.35 by automatic bubbling of thebuffer with CO₂ as soon as the pH exceeded this range. A weighttransducer was integrated into the chamber lid and allowed continuousassessment of lung weight. Data were recorded on a Pentium IIcomputer using the Matlab Software package (MathWorks, Inc., Natick,MA). For lung mechanics, the data were analyzed by applying thefollowing formula:

P=1/C×V<SUB><UP>t</UP></SUB>+R<SUB><UP>L</UP></SUB><UP>d</UP>V/<UP>d</UP>T

where P is chamber pressure, C pulmonary compliance, V_T tidal volume, and R_L airway resistance. All lung physiology parameterswere normalized to time point 0, i.e., after the end of the preconditioningperfusion of 40min.

Measurement of Perfusate Samples. Samples taken from the perfusate were stored at $-$ 20°C. Rat ET-1 was assessed by human endothelin-1 EIA detection kit detectingan amino acid sequence common to bovine, rat, canine, murine,and porcine ET-1. The relative cross reactivity of the detectingantibody to ET-1 was indicated as 100%, to ET-2 3%, to ET-3 <0.1%, and to big ET-1(-2, -3) < 0.1%. Recovery was 99.5% (manufacturer'sinformation). TXB₂ and PGI₂ were measured in perfusate samplesaccording to manufacturer'sinstructions.

Experimental Design. To obtain a stable baseline, all lungs were perfused for 10 min before any substance was added to the recirculating buffer.To obtain formation of peroxynitrite, 1 mU/ml xanthine oxidaseand 0.34 mM SNP were infused together at 0 min, whereas hypoxanthine,the substrate of the xanthine oxidase reaction, was already givenat $-$ 30 min. The inhibitors were usually injected before peroxynitriteformation: 190 µM TXA₂/PGH₂ receptor antagonist BM13.177 was givenat $-$ 36 min, 8 µM ET_A/ET_B receptor antagonists BQ123/BQ788, 10µM 2',7'-dichlorofluorescein diacetate, and 640 nM actinomycinD were given at $-$ 10 min. Cycloheximide in a final concentrationof 177 µM was applied either at $-$ 10 or 80 min. None of these substancesalone led to any measurable changes of the parameters investigatedin the concentrations used. Perfusion and ventilation were continuedfor another 160 min. Hypoxanthine, sodium nitroprusside, and BQ123/BQ788were each dissolved in PBS/MilliQ. Xanthine oxidase was purchasedin liquid form. The TXA₂/PGH₂ receptor antagonist BM13.177 wasdissolved in 30 µl dimethyl sulfoxide and then in 5 ml of perfusionbuffer. 2',7'-Dichlorodihydrofluorescein diacetate was dissolvedin ethanol and stored as 10-mg/ml stock solution at $-$ 20°C.

Preparation of Lung Tissue Homogenates. At the time point 120 min the buffer was replaced by PBS/MilliQ for another 2-min perfusion to remove the albumin-containingbuffer from the lung. Lung tissue was shock frozen in nitrogen.Corresponding to the lung tissue weight, 10 volumes of PBS containingantiproteases (5 µg/ml each of aprotinin, leupeptin, and pepstatin)were added. After homogenization on ice the tissue samples werecentrifuged (15 min, 17,900g at 4°C). The supernatant was usedfor ET-1 measurement. The ET-1 amount present in untreated lungswas subtracted from the treated lungs. The results were calculatedas $Delta$ ET-1 (pg/ml).

Detection of Peroxynitrite by 2',7'-Dichlorodihydrofluorescein Diacetate. Ten minutes before peroxynitrite generation by xanthine oxidase and SNP, the fluorescent dye DCHF (10 µM) was added to thehypoxanthine-containing buffer. At the end of perfusion, the lungtissue was homogenized as described above. The fluorescence intensityin the supernatant was measured with a fluorescence spectrometer(excitation at 485 nm and emission at 535 nm). The results werecalculated as fluorescence counts per milligram of totalprotein.

Statistics. Data are given as mean ± S.E.M. Due to normal distribution of the variables, ANOVA was performed. P $<=$ 0.05 is considered tobesignificant.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Peroxynitrite-Induced Bronchoconstriction and Vasoconstriction. About 100 min after infusion of the peroxynitrite-generating agents into rat lungs, airway (p = 0.93) and vascular (p < 0.001)resistance started to increase (Fig. 1, A and B), whereas pulmonarycompliance and tidal volume decreased from 0.36 ± 0.03 to 0.16± 0.03 ml/cm H₂O and 1.85 ± 0.09 to 1.00 ± 0.21 ml, respectively,after 160 min. Infusion of either reactant alone did not leadto any measurable changes (Fig. 1, A and B) in comparison to controlperfusions. This demonstrates that none of the agents alone islikely to be responsible for the observed changes in lung physiologyinitiated by peroxynitrite. Within 160 min of perfusion of theperoxynitrite-generating agents, the lung weight was increasedcompared with controls (HX/XO: 0.45 ± 0.20-0.77 ± 0.14 g; SNP:0.37 ± 0.35-0.48 ± 0.43 g; HX/XO plus SNP: 0.68 ± 0.17-1.14 ±0.24 g) without statistical significance. Therefore, this parameterwas not investigated further.

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Fig. 1. A and B, peroxynitrite generation induced broncho- and vasoconstriction. Time course of peroxynitrite (HX/XO plus SNP)-induced changes in airway (A) and vascular (B) resistance. XO (1 mU/ml) and 0.34 mM SNP were added to the perfusate at 0 min (arrow). The substrate HX (1 mM) was infused at $-$ 30 min. Airway R_L/R_{L 0 min} and vascular R_V/R_{V 0 min} resistance are normalized to 0 min. Data are means ± S.E.M, n = 3 (p = 0.93 and ***p < 0.001, respectively).

Chemical Evidence for Peroxynitrite Formation. To verify that peroxynitrite was actually generated in the perfusate by hypoxanthine/xanthine oxidase plus SNP, the followingcontrols were carried out. 1) Oxidation of DCHF to the fluorescentdye 2'7'-dichlorofluorescein was increased after 120 min of infusionin the simultaneous presence of SNP and hypoxanthine/xanthineoxidase from 42,000 in untreated control lungs, or 46,000 and39,000 in HX/XO and SNP-treated lungs, respectively, to 76,000counts of 2'7'-dichlorofluorescein/mg of protein in the homogenateof peroxynitrite-treated lungs. 2) After perfusion with DCHF inthe presence of peroxynitrite-generating agents, no significantchange compared with controls in the lung parameters investigatedwas observed (data not shown). This indicates that peroxynitritewas chemically reduced by DCHF to a form that is biologicallyinactive.

Role of Cyclooxygenase Products. Since there is in vitro evidence that peroxynitrite induces cyclooxygenase 2 and thus stimulates prostanoid production (Goodwinet al., 1999), we examined whether prostanoids were involved inthe pulmonary dysfunction by pharmacological means. Neither nonspecificinhibition of cyclooxygenases (COX 1/2) by 500 µM acetylsalicylicacid, which inhibits prostanoid formation (Uhlig et al., 1994b),nor TXA₂/PGH₂ receptor antagonism with BM13.177 had any significanteffect on the peroxynitrite-induced increase in airway and vascularresistance in peroxynitrite-treated lungs (data not shown). Moreover,no significant differences in the rates of TXB₂ or PGI₂ synthesiswere found in lungs exposed to peroxynitrite (1.2 ± 0.3 pg/mlmin TXB₂ and 12 ± 4 pg/ml min PGI₂) compared with lungs treatedonly with hypoxanthine/xanthine oxidase (1.0 ± 0.3 pg/ml min TXB₂and 14.2 ± 4 pg/ml min PGI₂). This finding makes it unlikely thatprostanoids are causal mediators of the peroxynitrite-inducedlunginjury.

Formation and Action of Endothelins. ET-1 concentrations were determined in the supernatant of lung homogenates 120 min after infusion of hypoxanthine/xanthineoxidase and/or SNP. The data in Fig. 2 show that the ET-1 concentrationin lung homogenate supernatants from hypoxanthine/xanthine oxidaseand SNP-treated lungs was significantly increased compared withtreatment with either agent alone (p < 0.01). This finding demonstratesincreased ET-1 production in the lung after peroxynitrite exposure.

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Fig. 2. Endothelin-1 release after peroxynitrite generation. ET-1 concentrations in tissue homogenate from controls and lungs exposed for 120 min to peroxynitrite. ET-1 was measured in the supernatant of lung homogenates by EIA. XO (1 mU/ml) was infused together with 0.34 mM SNP at 0 min. The substrate HX (1 mM) was infused at time $-$ 30 min. The increase in ET-1 is expressed as $Delta$ ET-1 (pg/ml) over untreated control lungs. Data are means ± S.E.M, n = 3 (**p < 0.01).

To find out whether ET-1 release is causal in the lung injury and by which ET receptor this effect is mediated, we used theselective ET_A receptor antagonist BQ123 (Ihara et al., 1992

) andthe ET_B receptor antagonist BQ788 (Ishikawa et al., 1994

). Asshown in Fig. 3, A and B, antagonism of the ET_A receptor by BQ123attenuated peroxynitrite-induced broncho- and vasoconstriction.The combination of BQ123 and BQ788 inhibited pulmonary broncho-and vasoconstriction completely and more effectively than BQ123alone. In contrast, a block of the ET_B receptor only by BQ788did not significantly affect peroxynitrite-induced bronchial constrictionand had no significant effect on vasoconstriction.

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Fig. 3. A and B, endothelin antagonism abolished effects of peroxynitrite generation. Time course of peroxynitrite (HX/XO plus SNP)-induced changes in airway (A) and vascular (B) resistance in lungs pretreated with either 8 µM BQ123 alone, 8 µM BQ788 alone, or 8 µM BQ123 in combination with 8 µM BQ788 10 min before generation of peroxynitrite by 1 mU/ml XO, plus 0.34 mM SNP at 0 min (arrow). HX (1 mM) was infused at $-$ 30 min. Airway R_L/R_{L 0 min} and vascular R_V/R_{V 0 min} resistance are normalized to 0 min. Data are means ± S.E.M, n = 3 (p = 0.38 and p = 0.06, respectively).

Dependence of Peroxynitrite-Induced Endothelin Action on Protein Synthesis. Since endothelins are not stored in cells, we checked the influence of transcriptional or translational arrest on peroxynitrite-inducedalterations of lung physiology. Inhibition of transcription byactinomycin D and of translation by cycloheximide before peroxynitritegeneration completely prevented peroxynitrite-induced bronchoconstriction(p = 0.02) as well as vasoconstriction (p < 0.001; data not shown).These findings indicate that de novo peptide/protein synthesisis required for the manifestation of pulmonary peroxynitrite-inducedalterations. Remarkably, infusion of cycloheximide protected againstpulmonary dysfunction as late as 80 min after peroxynitrite generation,i.e., about 20 min before injury could be detected. This indicatesthat the peptide that is causal to lung injury is released andacts very soon after translation, as is known forendothelins.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

Oxidant-mediated tissue injury as well as vascular and bronchial dysfunction play a prominent role in various lung diseases.Our study provides a new link between biologically relevant reactiveoxygen reaction products and endothelin-induced lung dysfunction.Our experiments confirmed in an organ system that simultaneousgeneration of O &cjs1138; ₂ and NO^· yield the reactive oxidant peroxynitrite (Beckman et al., 1990).It is shown that increased amounts of ET-1 are found in lung tissueexposed to the peroxynitrite-generating agents. Finally, the studydemonstrates that peroxynitrite caused broncho- and vasoconstrictionby a process with a lag phase of about 100 min requiring intactprotein synthesis and engagement of both the ET_A and ET_Breceptor.

Evidence for Exogenous Peroxynitrite Generation. As a methodological prerequisite, any detectable influence of the separate components of the exogenous peroxynitrite-generatingagents on lung physiology needed to be excluded. SNP potentiatesmyocardial ischemia-reperfusion injury independent of peroxynitritegeneration (Cope et al., 1997), and is reductively metabolizedto cyanide and nitric oxide (Ivankovich et al., 1978). This vasodilatoralso interferes with hypoxic pulmonary vasoconstriction and thereforepromotes mismatching of ventilation with perfusion (Oates, 1996).It has to be recalled that in our isolated perfused rat lungs,neither infusion of SNP alone nor of the nonspecific competitiveNO synthase inhibitor L-N^G-monomethyl-L-arginine monoacetate affect bronchial tone comparedwith untreated lungs (K. Eichert, unpublished results). This suggeststhat in the not innervated isolated organ, spontaneous, endogenousNO formation plays a minor role. The negative controls of eithercomponent of the peroxynitrite-generating agents alone indicatethat the pulmonary dysfunction we observed was in fact initiatedonly by the reaction product of NO^· and O &cjs1138; ₂, i.e., peroxynitrite. Any alternative combination productof these agents is consideredunlikely.

The known ability of peroxynitrite to diffuse into tissue is confirmed by our finding that oxidized DCHF was found in peroxynitrite-perfusedlung tissue compared with lungs treated only with SNP or HX/XO,or control lungs. Only peroxynitrite but neither O &cjs1138;

₂, nor hydrogenperoxide without cofactors such as horseradish peroxidase, norphysiological concentrations of NO^· are capable of oxidizing DCHF (Possel et al., 1997

). A recentarticle reports that uric acid, formed from hypoxanthine/xanthineoxidase, effectively inhibits tyrosine nitration (Sawa et al.,2000

). Therefore, we made no attempt in our experimental settingto detect protein-bound 3-nitrotyrosine, which is considered a"footprint" of in vivo peroxynitrite formation in lungs of ARDSpatients (Haddad et al., 1994

; Kooy et al., 1995

), or in bronchoalveolarlavage from ARDS patients inhaling NO^· (Lamb et al., 1999

Peroxynitrite-Induced Broncho- and Vasoconstriction. Because COX 1/2 inhibition and TXA₂/PGH₂ receptor antagonism had no effect on peroxynitrite-induced vasoconstriction, COX-derivedprostanoids are unlikely to be chief mediators in this acute lunginjury model. Because PGI₂ synthesis was not impaired under ourconditions, an inhibition of prostacyclin synthase by nitrationvia peroxynitrite detected in bovine artery strips described recentlydoes not seem to be the mechanism leading to the increased resistancethat we observed (Zou and Ullrich, 1996). An alternative explanation,i.e., that peroxynitrite-induced activation of COX 1/2 with ensuingenhanced prostaglandin synthesis is involved (Goodwin et al.,1999), also seems unlikely in perfused rat lung, since peroxynitritetreatment did not lead to a further increase in the rates of TXA₂/PGH₂and PGI₂ release compared with lungs exposed to HX/XO, i.e., superoxidegeneration alone, and because the inhibition of COX 1/2 by acetylsalicylicacid did not prevent lunginjury.

Evidence for ET-Mediated Broncho- and Vasoconstriction. Our differential pharmacological inhibition experiments identify endothelins as candidate pivotal mediators of broncho- andvasoconstriction in this model. The ET_A-selective antagonist BQ123predominantly blocked peroxynitrite-induced vasoconstriction.The observation that ET_B receptor antagonism was associated witha trend to further increase the vascular resistance might be explainedby an enhanced activation of the ET_A receptor by ET-1. Since thecombined inhibition of both receptors completely prevented thevasoconstriction, we conclude that both receptors play a rolein mediating the effects of ET-1 in this model, however, to adifferentextent.

In a way different from this inhibition pattern, however, ET_A receptor antagonism completely inhibited peroxynitrite-inducedbronchoconstriction, whereas ET_B receptor blockade alone had noeffect. ET-1 is not stored, but is de novo produced e.g., in responseto hypoxia (Smith et al., 1997

) or shear stress (Kuchan and Frangos,1993

), regulated on the level of preproendothelin translation(Hay, 1997

). The lag phase until broncho- and vasoconstrictionwe observed after infusion of peroxynitrite-generating agentsindicates that de novo protein synthesis is required for action.This is further supported by transcription or translation inhibitionexperiments and is fully consistent with findings from othersstudying hypoxia in an isolated rat lung model who observed increasedET-1 perfusate levels after 85 min of hypoxia (Smith et al., 1997

).Recently, the interesting finding was reported that neutral endopeptidase(EC 3.4.24.11), an enzyme implicated in the breakdown of bioactiveET-1, is inactivated by peroxynitrite (Kanazawa et al., 1999

).Taken together, this and our study indicate that both an inductionand a stabilization of bioactive ET-1 may be caused byperoxynitrite.

In conclusion, we tentatively propose the following sequence of events as a mechanistic explanation of our findings: 1) stoichiometricgeneration of O &cjs1138;

₂ and NO^· gives rise to generation of the reactive oxidant peroxynitrite;2) peroxynitrite causes broncho-and vasoconstriction by a processthat needs time for peptide synthesis; 3) thus, ET-1 is the mostlikely candidate for causing broncho- and vasoconstriction, ascorroborated by differential pharmacological inhibition of ET_Aand ET_B receptors. Our findings provide a new link between a secondaryproduct of two different extracellular reactive oxygen species,physiologically of different cellular origin, and the known potentmediator endothelin as a receptor-dependent initiator of pulmonarydysfunction.

	Acknowledgments

We gratefully acknowledge the help of Martin Mehl, Volker Ullrich, and Stefan-Lutz Wollin, University of Konstanz, Konstanz,Germany, and of Stefan Uhlig, Research Center Borstel, Germany,as well as the helpful comments of Joseph Beckman, Universityof Alabama, Birmingham,AL.

	Footnotes

Accepted for publication December 26, 2000.

Received for publication October 16, 2000.

The study was supported by Grant We 686/18 of the Deutsche Forschungsgemeinschaft to the research group "Endogenous tissueinjury: Mechanisms of autodestruction".

Send reprint requests to: Dr. Albrecht Wendel, Biochemical Pharmacology, University of Konstanz, D-78457 Konstanz, Box M668, Germany. E-mail: Albrecht.Wendel{at}uni-konstanz.de

	Abbreviations

ARDS, acute respiratory distress syndrome; NO, nitric oxide; O &cjs1138; ₂, superoxide anion; PGI₂, prostacyclin; ET, endothelin; ET_A/B, endothelin_A/B receptor; TXA₂, thromboxane A₂; PGH₂, prostaglandin H₂; XO, xanthine oxidase; DCHF, 2',7'-dichlorodihydrofluorescein diacetate; EIA, enzyme immunoassay; TXB₂, thromboxane B₂; R_L, airway resistance; R_V, vascular resistance; PBS, phosphate-buffered saline; SNP, sodium nitroprusside; HX, hypoxanthine; COX 1/2, cyclooxygenase 1/2.

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