Thiol Regulation of Pro-Inflammatory Cytokines Reveals a Novel Immunopharmacological Potential of Glutathione in the Alveolar Epithelium

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Vol. 296, Issue 3, 996-1005, March 2001

Thiol Regulation of Pro-Inflammatory Cytokines Reveals a Novel Immunopharmacological Potential of Glutathione in the Alveolar Epithelium

John J. E. Haddad, Bared Safieh-Garabedian, Nayef E. Saadé and Stephen C. Land

Oxygen Signaling Group, Center for Research into Human Development, Tayside Institute of Child Health, Faculty of Medicine, Ninewells Hospital and Medical School, University of Dundee, Dundee, Scotland, United Kingdom (J.J.H., S.C.L.); and the Departments of Biology (B.S.-G.), Faculty of Arts and Sciences, Human Morphology and Physiology (N.E.S.), Faculty of Medicine, American University of Beirut, Beirut, Lebanon

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The therapeutic immunopharmacological potential of glutathione in the alveolar epithelium is not well characterized. We developedan in vitro model of fetal alveolar type II epithelial cells toinvestigate the effect of redox disequilibrium on chemioxyexcitation( $Delta$ pO₂/ROS) induced up-regulation of pro-inflammatory cytokines.Buthionine sulfoximine, an irreversible inhibitor of $gamma$ -glutamylcysteinesynthetase, the rate-limiting enzyme in glutathione (GSH) biosynthesis,induced intracellular reactive oxygen species (ROS) and the releaseof interleukin-1 $beta$ (IL-1 $beta$ ), IL-6, and tumor necrosis factor- $alpha$ .Chloroethyl nitrosourea, which blocks the NADPH-dependent recyclingof oxidized glutathione (GSSG), reduced ROS-induced cytokine production,similar to pyrrolidine dithiocarbamate, an antioxidant/pro-oxidantthiuram, which elevates GSSG. The antioxidant and GSH precursor,acetylcysteine, abrogated cytokine release concomitant with suppressionof ROS, an effect mimicked by $gamma$ -glutamylcysteinyl-ethyl ester,a cell permeant GSH. Cysteine, the rate-limiting amino acid inthe de novo synthesis of GSH, administered as oxothiazolidinecarboxylate and adenosylmethionine, mitigated the chemioxyexcitation-dependentcytokine release. Ebselen, an anti-inflammatory antioxidant, whichmimics the effect of glutathione peroxidase, neutralized ROS bythe GSH-peroxidase-coupled reaction, thereby blocking the pathwayto cytokine enhancement. Our results indicate that modulatingredox equilibrium by pharmacological thiols exhibits differentialregulation on pro-inflammatory cytokines, thus bearing clinicalconsequences for the therapeutic treatment of pediatric distressesinpathophysiology.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

The tripeptide L- $gamma$ -glutamyl-L-cysteinyl-glycine, or glutathione (GSH), a ubiquitous thiol, plays a major role in maintainingintracellular redox balance and regulating pathways augmentedby oxidative stress (Meister, 1988; Haddad and Land, 2000a; Haddadet al., 2000a). The cysteinyl moiety of GSH provides the reactivethiol as a functional element responsible for the diverse propertiesof glutathione, whose participation in the physiology of metabolismreflects its importance in intracellular functions. These include:1) an antioxidant potential mediated by the peroxidase-coupledreaction; 2) regulation of cellular sulfhydryl status and redoxequilibrium; 3) governing pathways in neuro-immune-endocrine interactionsas a neurotransmitter and an immunopharmacological thiol; and4) regulation of the expression/activation of redox-sensitivetranscription factors induced by stress-evoked responses (Drögeet al., 1994; Hayes and McLellan, 1999; Haddad et al., 2000a).The pivotal role of redox cycle in maintaining the integrity ofthe biological system in the face of oxidative stress is, therefore,of particular clinicalrelevance.

The "biomarkers" of oxidative stress, such as antioxidant inefficiency, redox disequilibrium, and derivation of oxidant radicals,for instance, may arise from conditions other than hyperoxia (oxidizingsignals) per se, such as hypoxia/reoxygenation and cytokine-dependentprocesses (Thom et al., 1997; Haddad and Land, 2000a). In physiologicalconditions, the intracellular redox status of thiols is highlyreductive. GSH, for example, is present in high concentrationsin lung epithelial lining fluid (Cantin et al., 1989) and hasbeen reported to maintain the integrity of the airspace epitheliumin vitro and in vivo (Li et al., 1997). In contrast, GSH depletionhas been linked to the pathophysiology of idiopathic pulmonaryfibrosis (Cantin et al., 1989), adult respiratory distress syndrome(Bunnell and Pacht, 1993), bronchopulmonary dysplasia (Saugstad,1997), and cystic fibrosis (Roum et al., 1993), thus highlightingits central role in maintaining the functional integrity of aphysiologically competent epithelium. There is growing evidence,moreover, supporting the notion that oxidative conditions modulateredox-linked pathways by altering the dynamic equilibrium of glutathionehomeostasis (Haddad et al., 2000a). Exogenous/endogenous agents,which induce the formation of ROS, for example, can affect redoxhomeostasis by up-regulating antioxidant enzymes, particularlyglutathione peroxidase and enzymes involved in glutathione recyclingand biosynthesis (Douglas, 1987; Goss et al., 1997; Li et al.,1997; Haddad and Land, 2000a). Furthermore, ROS signaling couldbe mediated by cytokines, peptide hormones, and immunoregulators,whose participation in cellular pathways is modulated by redoxstatus (Rovin et al., 1997; Pena et al., 1999; Yamashita et al.,1999; Haddad et al., 2001). Conversely, cytokines, which themselvesare mediators of oxidative stress (Nussler et al., 1992; Desmarquestet al., 1998; Yamashita et al., 1999), have the potential to alterredox equilibrium, thereby affecting GSH/oxidized glutathionedisulfide (GSSG) shuttling and recycling (Chen et al., 1998).How chemioxyexcitation [ $Delta$ pO₂/reactive oxygen species (ROS)] inductionof cytokines modulate signaling pathways in oxidative stress throughredox equilibrium in the fetal alveolar epithelium has yet tobe ascertained. Furthermore, pharmacological manipulation of glutathionehomeostasis in perinatal epithelia and its effects on cytokine-mediatedresponses are not known; subsequently, unraveling the biochemistryof redox-linked pathways bears a typical clinical approach fordiagnosing pathophysiological conditions in the developinglung.

The immunopharmacological potential assigned to glutathione (Thompson et al., 1985) stems from established observations. Interleukin-1(IL-1)-induced responses, for instance, occur through modulatingredox equilibrium (Rovin et al., 1997). In addition, ROS signalingregulating the transcription of IL-4 (Jeannin et al., 1995), IL-6,IL-8 (Gosset et al., 1999), and tumor necrosis factor- $alpha$ (TNF- $alpha$ )(Neuschwander-Tetri et al., 1996; Gosset et al., 1999) occursthrough a thiol-dependent mechanism. Interestingly, antioxidants(Reimund et al., 1998; Barrett et al., 1999) and glutathione precursors(Jeannin et al., 1995; Pena et al., 1999) have been shown to down-regulatecytokine synthesis, activation, and downstream processes. Amongseveral agents that were used for repletion and depletion of GSH,N-acetyl-L-cysteine (NAC) and L-buthionine-(S,R)-sulfoximine (BSO)are, respectively, of particular importance as they exhibit antagonisticeffects on a pro-inflammatory signal. NAC, an antioxidant anda GSH precursor (Bernard, 1991; Haddad et al., 2000a), amelioratescytokine production (Tsuji et al., 1999) and ROS-mediated lunginjury (Bernard, 1991). In contrast, BSO, which depletes GSH byirreversibly inhibiting $gamma$ -glutamyl-L-cysteinyl-ethyl ester ( $gamma$ -GCS),the rate-limiting enzyme in the biosynthesis of glutathione (Griffithand Meister, 1979; Haddad and Land, 2000a), has the potentialto enhance cytokine secretion by up-regulating ROS (Gosset etal., 1999). We reasoned that a differential manipulation of glutathionehomeostasis and shuttling may antagonistically affect a pro-inflammatorysignal, thus bearing potential consequences for the treatmentof respiratory distresses, where cytokines are recognized as majorparticipants in their pathophysiology (Saugstad, 1997).

This study elaborates in vitro an immunopharmacological potential of glutathione in the perinatal epithelium. Accordingly,we derive the hypotheses that 1) chemioxyexcitation ( $Delta$ pO₂/ROS)regulation of intracellular redox homeostasis is dependent onthe flux kinetics and duration of ROS exposure, and 2) glutathionedepletion and repletion differentially manipulate pro-inflammatorycytokines, an effect antagonistically reversed by restoring redoxequilibrium. The mechanisms implicated in redox-associated cytokinepathways are thereafter developed in the light of the novel roleof glutathione as an immunopharmacological regulatorythiol.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

All experimental procedures involving the use of live animals were approved under the Animals Act legislation, 1986 (UK).Chemicals/reagents were obtained from Sigma Chemical Co. (St.Louis, MO) and Calbiochem (La Jolla,CA).

Primary Cultures of Alveolar Epithelia. Fetal alveolar type II (fATII) epithelial cells were isolated from lungs of rat fetuses on gestation day 19, essentially asdescribed elsewhere (Haddad and Land, 2000a,b). Briefly, fetalrats were removed from pregnant Sprague-Dawley rats by cesareansection at day 19 of gestation (term = 22 days), and the lungswere excised, teased free from heart and upper airway tissue,and finely minced then washed free of erythrocytes using sterile,chilled Mg²⁺- and Ca²⁺-free Hanks' balanced salt solution. The cleaned lung tissue wasresuspended in 1 ml/fetus Hanks' balanced salt solution containingtrypsin (0.1 mg/ml), collagenase (0.06 mg/ml), and DNase I (0.012%w/v), and was agitated at 37°C for 20 min. The solution was thencentrifuged at 100g for 2 min to remove undispersed tissue, thesupernatant was saved to a fresh sterile tube, and an equal volumeof Dulbecco's modified Eagle's medium (DMEM) with 10% (v/v) fetalcalf serum (FCS) was added to the supernatant. After passing thesupernatant through a 120-µm pore sterile mesh, the filtrate wascentrifuged at 420g for 5 min, the pellet was resuspended in 20ml of DMEM/FCS, and the cells were placed into a T-150 cultureflask for 1 h at 37°C to enable fibroblasts and nonepithelialcells to adhere. Unattached cells were washed three times by centrifugationat 420g for 5 min each and then seeded onto 24-mm diameter Transwell-clearpermeable supports (0.4-µm pore size, Costar, Cambridge, MA) ata density of 5 × 10⁶ cells per filter and were allowed to adhere overnight at fetaldistal lung pO₂ (23 torr $approx$ 3% O₂/5% CO₂). DMEM/FCS was exchangedfor 4 ml of serum-free PC-1 media (BioWhittaker, Walkersville,MD) pre-equilibrated to pO₂ = 23 torr and 37°C 24 h later, andcells were maintained at this pO₂ until theexperiment.

The change in O₂ equilibrium from fetal to postnatal environments constitutes a potential signaling mechanism in the perinatallung. The choice of this form of oxidative stress was based onits clinical relevance of the situation resembling the birth transitionperiod and beyond (Haddad and Land, 2000a

; Haddad et al., 2000a

).Consequently, shifts in pO₂ were recreated where cells were culturedat fetal pO₂ (23 torr), followed by control period at the samepO₂ or re-equilibrated to early postnatal pO₂ (100 torr), mild(152 torr), and severe hyperoxia (722 torr). In each case, andunder conditions of independent pretreatments, the adenylate energycharge, an index of cell viability and competence, remained at $>=$ 0.7, and transepithelial monolayer resistance was maintainedconstant at $>=$ 250 to 350 $Omega$ cm² (Haddad and Land, 2000a

). The static cellular energy charge ofcell cultures pretreated with various drugs rules out any nonspecificcytotoxicity. To further confirm this fact, the total proteincontent of pretreated cells was determined to be insignificantlydifferent (P > 0.05) from control cultures (data not shown). Inaddition, alveolar pretreatment has been shown to intervene specificallyat the level of the cell cycle events (such as with p53), andat the level of factors that are key components of the signalingpathways governing apoptosis (such as with Bax and Bcl-2 proto-oncogenes),suggesting specificity rather than necrotic toxicity (Haddad andLand, 2000b

). We have also shown that these drugs selectivelyinterfere with the stabilization, nuclear translocation, and consensusDNA binding activity of the redox-sensitive transcription factors,hypoxia-inducible factor 1 $alpha$ (HIF-1 $alpha$ ) and nuclear factor- $kappa$ B (NF- $kappa$ B),implicating specific intervention in signaling transduction pathways(J. J. E. Haddad, B. Safieh-Garabedian, N. E. Saadé, and S. C.Land, unpublishedobservations).

Enzyme-Linked Immunosorbent Assay Assessment of the Cytokine Profile. Cytokines in cell-free supernatants were measured by sandwich enzyme-linked immunosorbent assay. Polyclonal antibodies (2µg/ml) were used to coat high binding microtiter plates (Safieh-Garabedianet al., 1997). Recombinant and biotinylated immunoglobulins (agenerous gift from Dr. Stephen Poole, National Institute for BiologicalStandards and Control, UK) were used for capturing, followed bycolor development with streptavidin-poly-horseradish peroxidaseand tetramethylbenzidine dihydrochloride. Inter- and intra-assaycoefficients of variations at 450 nm were $<=$ 10%, and the minimumdetectable sensitivity was $<=$ 2 pg/ml.

Thiol Regulation of Intracellular ROS with Ascending $Delta$ pO₂ Regimen (Oxyexcitation). To determine H₂O₂ production, cells were coated in microtiter plates (10⁵/well) and incubated overnight at either 23 or 152 torr, followedby pretreatment (24 h) with BSO (50 µM), 1,3-bis-(2-chloroethyl)-1-nitrosourea(BCNU; 100 µM), pyrrolidine dithiocarbamate (PDTC; 100 µM), NAC(50 mM), $gamma$ -GCE (100 µM), or ebselen (100 µM). Phenolsulfonphthaleincontaining horseradish peroxidase (20 U/ml) was added followedby shifting to ascending $Delta$ pO₂. The reaction was terminated with1 M NaOH and measured at 600 nm (Pick and Mizel, 1981). A standardcurve (0-100 µM H₂O₂) was developed, and results were convertedto nmol · mg¹ of protein. To determine O 2− production, cellsfollowing pretreatments were covered with 80 µM ferricytochromec suspended in phenol red solution. The amount of Oreleased was measured at 550 nm against blanks containing ferricytochromec and superoxide oxidoreductase dismutase (300 U/ml) (Pick andMizel, 1981). Experiments were performed in duplicates, and dataare presented as O 2− released based on nanomolesof reduced cytochrome · mg¹ of protein. The hydroxyl radical reacts with dihydrorhodamine(DHR) to yield water and a tertiary free radical, which is ratherstable. This radical undergoes rearrangement of the $pi$ electrons,leading to formation of fluorescent rhodamine (Weiss et al., 1978).To determine ^·OH production, cells were pretreated before oxyexcitation in thepresence of 50 µM DHR. Fluorescence was measured at 485/535 nmexcitation and emission wavelengths, respectively. The ^·OH level measured under hypoxia was calibrated to 100%, and variableswere plotted against this baseline as logarithmic fluorescenceunits.

Intracellular Redox Homeostasis on Exposure to ROS (Chemiexcitation). To evaluate whether chemioxyexcitation exposure (X/XO, 100 µM/2 mU/ml; H₂O₂, 250 µM) modulates redox potential, we determinedthe equilibrium ratio GSH/GSSG. Following incubations, filterswere treated with 7% perchloric acid, then centrifuged at 10,000gfor 5 min. Glutathione concentration (24 h) after neutralizationwith 3 M KHCO₃ was spectrophotometrically determined (Haddad andLand, 2000a). The assay conditions for determining the activitiesof enzymes involved in glutathione homeostasis are detailed elsewhere(Haddad and Land, 2000a). Specific activities of glutathione peroxidase(GSH-PX), glutathione reductase (GSSG-RD), $gamma$ -GCS, and glutathionesynthase (GS) determined in cytosolic extracts of cells treatedwith X/XO and H₂O₂ are expressed as units · mg¹ of protein, where 1 unit (U) of enzyme activity is the amountthat catalyzes the formation of 1 µmol of product/min. All assayswere conducted at 30°C. To determine GSH-PX activity, cytosolicextracts were incubated in PBS buffer containing 5 mM EDTA, 10mM NAD(P)H, GSSG-RD (100 U/ml), 1.125 M NaN₃ (a catalase inhibitor),and 150 mM GSH in a final volume of 1 ml. The enzymatic reactionwas initiated by addition of 100 µl of 2 mM H₂O₂ (30%; 10.15 M),and the linear rate of conversion of NADPH/H⁺ to NADP⁺ at 340 nm between 0 and 5 min after initiation of the reaction,was followed. The rate of oxidation of NAD(P)H by GSSG at 30°Cwas used as a standard measure of the enzymatic activity of GSSG-RD,by monitoring the rate of formation of NADP⁺ at 340 nm between 0 and 5 min after addition of the sample. Theenzyme activity of $gamma$ -GCS was determined in a reaction mixture(1 ml) containing Tris-HCl (100 mM, pH 8.2), sodium L-glutamate(10 mM), Na₂-ATP (5 mM), sodium phosphoenol pyruvate (2 mM), KCl(150 mM), NADH (0.2 mM), pyruvate kinase (5 U; bovine heart typeIII), and lactate dehydrogenase (10 U; rabbit heart type II).The reaction was initiated by adding the sample, and the rateof NAD⁺ formation was followed at 340 nm. GS activity was assayed ina reaction mixture containing Tris-HCl (100 mM; pH 8.2 at 30°C),KCl (50 mM), L- $gamma$ -glutamyl-L- $alpha$ -aminobutyric acid (5 mM), ATP (10mM), glycine (5 mM), MgCl₂ (20 mM), EDTA (2 mM), and sample (addedlast) in a final volume of 0.1 ml. Added to this was 0.02 ml of10% sulfosalicylic acid and 0.9 ml of a buffer containing phosphoenolpyruvate(0.5 mM), NADH (0.2 mM), pyruvate kinase (1 U), MgCl₂ (40 mM),KCl (50 mM), and K₂HPO₄ (250 mM; pH 7.0). The reaction was initiatedwith 1 unit of lactate dehydrogenase, and the rate of NAD⁺ formation was followed as above. Regression analysis was performedto determine the degree of correlation between enzyme activities(units · mg¹ of protein) andchemioxyexcitation.

Redox Homeostasis and Chemioxyexcitation-Induced Cytokine Secretion. To determine the effect of redox disequilibrium on cytokine release, cells were pretreated (24 h) with: 1) BSO, a specificand irreversible inhibitor of $gamma$ -GCS (Griffith and Meister, 1979);2) BCNU, a specific inhibitor of GSSG-RD (Hardwick et al., 1990);and 3) PDTC, an antioxidant/pro-oxidant, which elevates GSSG (Schrecket al., 1992; Haddad et al., 2000a). Cells were exposed to chemioxyexcitation,and supernatants were collected 24 h later and assessed forcytokines.

The hypothesis that replenishing GSH would interfere with the capacity to produce cytokines has been investigated with exogenousprecursors. Cells were pretreated (24 h) with: 1) $gamma$ -GCE, a membrane-permeatingprecursor (Okamota et al., 1999

); 2) NAC, an antioxidant and GSHprecursor (Bernard, 1991

; Haddad et al., 2000a

); 3) 2-oxothiazolidine-4-carboxylate(OTC; 100 µM), a cysteine pro-drug (Anderson and Luo, 1998

); and4) S-adenosyl-L-methionine (SAM; 100 µM), an antioxidant and aprecursor of GSH (Evans et al., 1997

). Following pretreatments,cells were challenged and supernatants were collected for cytokineassessment.

Selective Modulation of Redox-Sensitive Enzymes and Regulation of Cytokines. Glutathione is postulated as a negative modulator of cytokine release, but whether this effect represents an antioxidant propertyhas to be determined in the alveolar epithelium. Cells were pretreatedwith BSO for 24 h, before simultaneous incubation with NAC andchemioxyexcitation, followed by analysis of cytokines. Separately,we tested the effect of ebselen, a membrane permeant GSH-PX mimeticand an antioxidant (Schewe, 1995), on chemioxyexcitation-inducedcytokinerelease.

Statistical Analysis and Data Presentation. Data are the means and the error bars the S.E.M. of at least three independent cell cultures. Statistical evaluation was performedby one-way analysis of variance (ANOVA), followed by post hocTukey's test, and the a priori level of significance at 95% confidencelevel was considered at P < 0.05.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Thiol Regulation of H₂O₂ Production. The profile of H₂O₂ formation in response to oxyexcitation is differentially regulated by glutathione-modulating agents (Fig.1). The level of H₂O₂ is increased with ascending $Delta$ pO₂ regimenat 24 h. Although BSO potentiated oxyexcitation-dependent H₂O₂production, BCNU, PDTC, NAC, $gamma$ -GCE, and ebselen abrogated thiseffect.

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Fig. 1. Thiol regulation of intracellular H₂O₂ in response to oxyexcitation. A through E, the formation of H₂O₂ at 24 h is enhanced with ascending pO₂ (P < 0.05, P < 0.01, P < 0.001, as compared with pO₂ = 23 torr). BSO synergistically potentiated oxyexcitation-induced H₂O₂ production (⁺P < 0.05, as compared with control). BCNU and PDTC, as agents that elevate GSSG, abrogated the induced production of H₂O₂. NAC and $gamma$ -GCE, as precursors of GSH, substantially blocked H₂O₂ formation, an effect mimicked by ebselen (*P < 0.05, **P < 0.01, ***P < 0.001, as compared with control).

Thiol Regulation of O Production. The variation in O 2− production with thiol-modulating agents is shown in Fig. 2. The level of Ois increased with ascending $Delta$ pO₂ regimen at 24 h. BSO increasedthe release of O at 23, 23 $right-arrow$ 100, and 23 $right-arrow$ 722torr (24 h), whereas BCNU, PDTC, NAC, $gamma$ -GCE, and ebselen abrogatedits formation.

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Fig. 2. Thiol regulation of intracellular O 2−

in response to oxyexcitation. A through E, the formation of O 2−

at 24 h is enhanced with ascending pO₂ (P < 0.05, P < 0.01, as compared with pO₂ = 23 torr). BSO synergistically potentiated oxyexcitation-induced O 2−

production (⁺P < 0.05, as compared with control). BCNU and PDTC, as agents that elevate GSSG, abrogated the induced production of O 2−

. NAC and $gamma$ -GCE, as precursors of GSH, substantially blocked the formation of O 2−

, an effect mimicked by ebselen (*P < 0.05, **P < 0.01, ***P < 0.001, as compared with control).

Thiol Regulation of ^·OH Production. The conversion of DHR to fluorescent rhodamine in the presence of ^·OH is shown in Fig. 3. The profile of ^·OH release in response to thiol-modulating agents is determinedwith selective inhibitors of enzymes involved in glutathione homeostasis.BSO induced accumulation of ^·OH, an effect potentiated by oxyexcitation. Conversely, BCNU,PDTC, NAC, $gamma$ -GCE, and ebselen mediated suppression of ^·OH with ascending $Delta$ pO₂ regimen.

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Fig. 3. Thiol regulation of intracellular ^·OH in response to oxyexcitation. The reference value obtained at static 23 torr was set to 100%, and as such the corresponding variations are set against this baseline (dotted line). A through E, ^·OH kinetics following 24-h exposure to oxyexcitation (P < 0.05, P < 0.01, as compared with pO₂ = 23 torr). BSO synergistically potentiated oxyexcitation-induced ^·OH production (⁺P < 0.05, as compared with control). BCNU and PDTC abrogated the induced production of ^·OH. NAC and $gamma$ -GCE substantially blocked the formation of ^·OH, an effect mimicked by ebselen (*P < 0.05, **P < 0.01, ***P < 0.001, as compared with control).

Redox Equilibrium and Chemioxyexcitation. We investigated the hypothesis that chemiexcitation synergistically act with oxyexcitation to alter the redox state in favorof a reduction equilibrium. Exposure to H₂O₂ (Fig. 4A) and X/XO(Fig. 4B) elevated [GSH] with ascending $Delta$ pO₂ regimen. [GSSG] wasmarkedly depressed with either treatment, such that the ratioGSH/GSSG is increased 4- to 15-fold (H₂O₂) and 5- to 7-fold (X/XO)relative to controls without ROS exposure.

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Fig. 4. Reduction-oxidation (redox) potential in fATII cells exposed to oxyexcitation. A, reduced (GSH) and oxidized (GSSG) glutathione variations (24 h) are shown for cells exposed to ^·OH-generating system (⁺P < 0.05, ⁺⁺P < 0.01, ⁺⁺⁺P < 0.001, as compared with [GSH]_Control or [GSH]_H2O2). H₂O₂ induced the elevation of [GSH] as compared with control cultures at pO₂ = 23 or 152 torr (*P < 0.05, **P < 0.01). B, glutathione homeostasis (24 h) in the presence of an O 2−

-generating system. The concentration of GSH is increased in the presence of X/XO (*P < 0.05, **P < 0.01, ***P < 0.001). The levels of GSSG are markedly depressed, as compared with [GSH] (⁺P < 0.05, ⁺⁺P < 0.01, ⁺⁺⁺P < 0.001, as compared with [GSH]_Control or [GSH]_X/XO).

ROS Effect on Redox-Sensitive Enzymes. The transition from fetal to neonatal pO₂ attenuates the activity of enzymes involved in maintaining homeostatic levels ofintracellular glutathione (Haddad and Land, 2000a). To determinewhether exposure to ROS modulates their activities, we evaluatedthe role of O 2− and ^·OH on GSH-PX, GSSG-RD, $gamma$ -GCS, and GS. The dose-dependent analysisof enzyme activities (EU) is shown in Fig. 5. X/XO exposure inducedthe activity of GSH-PX (Fig. 5A), $gamma$ -GCS (Fig. 5E), and GS (Fig.5G), but not that of GSSG-RD (Fig. 5C). Inductive effects areevident at 23 $right-arrow$ 100, 23 $right-arrow$ 152, and 23 $right-arrow$ 722 $Delta$ pO₂ torr, where the linearregression analysis shows significant correlation between EU and[XO]. Exposure to the ^·OH-generating system significantly induced the activities of GSH-PX(Fig. 5B), $gamma$ -GCS (Fig. 5F), and GS (Fig. 5H) but marginally GSSG-RD(Fig. 5D). The effect of H₂O₂ is more prominent on enzyme activitiesthan that of X/XO. Linear regression analysis reveals significantcorrelation between EU and H₂O₂.

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Fig. 5. Kinetics of ROS-mediated effects on redox enzymes involved in maintaining homeostatic levels of glutathione. Dose-dependent analysis of the potential activity of GSH-PX (A, B), GSSG-RD (C, D), $gamma$ -GCS (E, F), and GS (G, H) in the presence of X/XO or H₂O₂ at various $Delta$ pO₂ regimens. Linear regression analysis of fitting curves reveals significant correlation within the range 0.75 $<=$ r $<=$ 0.85 (P < 0.05, as compared with enzyme activity of control).

GSH Depletion and Chemioxyexcitation-Induced Cytokine Secretion. As shown in Table 1, BSO up-regulated the release of IL-1 $beta$ , IL-6, and TNF- $alpha$ , an effect synergistically enhanced in responseto chemiexcitation (23 $right-arrow$ 152 torr). BCNU down-regulated the cytokineprofile in a manner similar to PDTC and ebselen. Similar resultswere reported at other pO₂ tensions (data not shown).

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TABLE 1
The effect of glutathione-modulating agents (depletion/recycling) on cytokines (ng/mg of protein)
Data are presented as means ± S.E.M. (n = 4, each).

GSH Repletion and Chemioxyexcitation-Induced Cytokine Secretion. As shown in Table 2, pretreatment with cysteine precursors NAC, OTC, and SAM down-regulated chemioxyexcitation-induced IL-1 $beta$ ,IL-6, and TNF- $alpha$ release (23 $right-arrow$ 152 torr). The esterified glutathione-permeatingprecursor $gamma$ -GCE mimicked the effects of cysteine precursors byinhibiting the release of cytokines. Similar results were reportedat other pO₂ tensions (data not shown).

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TABLE 2
The effect of glutathione modulating agents (repletion/biosynthesis) on cytokines (ng/mg of protein)
Data are presented as means ± S.E.M. (n = 4, each).

Selective Modulation of Redox-Sensitive Enzymes and Cytokines. The effect of BSO on NAC-induced down-regulation of cytokine release is shown in Fig. 6 (23 $right-arrow$ 152 torr). NAC significantly reducedBSO/chemiexcitation-induced IL-1 $beta$ (Fig. 6A), IL-6 (Fig. 6B), andTNF- $alpha$ (Fig. 6C) release. Similar results were reported at otherpO₂ tensions (data not shown).

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Fig. 6. Effect of BSO on NAC-induced down-regulation of chemioxyexcitation-induced cytokine release at 23 $right-arrow$ 152 torr. NAC reduced BSO-induced up-regulation of IL-1 $beta$ (A), IL-6 (B), and TNF- $alpha$ (C), suggesting that its effects are independent of GSH biosynthesis (*P < 0.05, **P < 0.01, as compared with control; ⁺P < 0.05; P < 0.05, as compared with BSO).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The present report investigated in vitro regulatory mechanisms of pharmacological thiols on pro-inflammatory cytokines inthe perinatal epithelium. This approach bears clinical relevanceto the pediatric treatment of respiratory distresses, where cytokinesare crucial elements in their pathophysiology. Growing evidenceimplicates an association between oxidative stress and up-regulationof a pro-inflammatory state, thereby placing more demand on theutilization of intracellular glutathione (Sen, 1998; Alder etal., 1999). As such, the respiratory epithelium becomes more engagedin regulating enzymes involved in maintaining redox homeostasis.Although the glutathione biosynthetic machinery is overwhelmedin disease, an up-regulation of cytokines may contribute to acuteexacerbation of the clinical symptoms. Although cytokine participationin the pathogenesis of respiratory distress has been considerablyrecognized, the mechanisms involved have not been clearly defined.The development of an in vitro model enabled us to investigatethe immunopharmacological potential of glutathione, whereby thealveolar epithelium is recognized as a major participant in afront-line defense strategy to oxidants and subsequent lunginjury.

The rate-limiting substrate for GSH biosynthesis is glutamate-cysteine (K_m glutamate = 1.6 $-$ 2 mM; K_m cysteine= 0.3 mM). This pathway is selectively blocked by BSO, a specificand irreversible inhibitor of $gamma$ -GCS (Griffith and Meister, 1979).Consequently, the capacity of the epithelium to replenish intracellularstores of GSH is dramatically affected, thereby modulating theoptimum equilibrium necessary to evoke a defense strategy in oxidativestress (Haddad and Land, 2000a; Haddad et al., 2000a). This subsequentlyleads to ROS up-regulation, the inappropriate disposition, accumulation,and intracellular localization of which augment a pro-inflammatorysignal through activation of redox-sensitive transcription factors(Schreck et al., 1992; Luster and Simeonova, 1998). This is consistentwith the observation that the expression of $gamma$ -GCS was shown tosuppress TNF- $alpha$ -induced activation of NF- $kappa$ B (Manna et al., 1999).We believe that the pathway mediating BSO-induced up-regulationof cytokines in the alveolar epithelium involves a secondary mediator,the most likely candidate being the hydroxyl radical. This conformsto the evidence that GSH is involved in H₂O₂ reduction, a majorsource of ^·OH, through the GSH-PX-coupled reaction, suggesting that, in thecase of BSO preincubation, GSH depletion seems involved in itseffect. It is possible that GSH depletion by blocking its biosynthesisreduces the capacity of the epithelium to dispose accumulatingH₂O₂, with the resulting increase in ^·OH production. The likely occurrence of this biochemical conversionis extended by others (Yamauchi et al., 1990; Manna et al., 1999)and supported by corollary experiments with diethyl maleate, adepletor of glutathione, thereby leading to ^·OH/O 2− induction and cytokine release (J. J.E. Haddad, B. Safieh-Garabedian, N. E. Saadé, S. A. Kanaan, andS. C. Land, unpublished observations). It remains to be defined,however, whether GSH depletion is implicated in up-regulatingcytokines in association with lung disease, since the degree ofdepletion necessary to evoke cytokines in vitro is higher thanthat observed in pathophysiology in vivo (Sen, 1998; Alder etal., 1999; Gosset et al., 1999).

The ability of NAC to provide cysteine for GSH biosynthesis (Bernard, 1991), along with that of BSO to block de novo synthesis(Haddad and Land, 2000a), provided the criteria to establish whetherNAC inhibitory effects on chemioxyexcitation-induced cytokinerelease is rate-limited by glutathione biosynthesis. Interestingly,BSO did not affect NAC-mediated down-regulation of cytokine secretion,suggesting that its inhibitory effect is independent of its roleas a GSH precursor. Since the cysteine provided by NAC eventuallycannot feed into the biosynthetic pathway because of irreversibleinhibition of $gamma$ -GCS (Griffith and Meister, 1979), it's very likelythat NAC is acting either on components of the chemioxyexcitationsignaling transduction pathway or through an alternative metabolicmachinery. In this respect, the antioxidant, scavenging actionagainst ROS-induced cytokine release is a possible mechanism (Aruomaet al., 1989; Eugui et al., 1994).

The cell-permeable glutathione pro-drug, $gamma$ -GCE, was shown to be likewise potently effective in down-regulating chemioxyexcitation-inducedcytokine release. $gamma$ -GCE is rapidly de-esterified by intracellularesterase, thereby serving as an effective delivery agent for glutathione,which is a peptide incapable of crossing membranes in its nativeform. Although a distinction between the biological effects of $gamma$ -GCE and GSH is indiscriminate, intracellular conversion of $gamma$ -GCEsuggests that its effects are mediated by GSH. Exogenous/endogenousglutathione, therefore, may feed into one of the well characterizedpathways of metabolism (Meister, 1988). For instance, GSH playsan important role in determining how readily pro-inflammatorygenes can be regulated, and GSH/GSSG equilibrium is a major determinantof the activation of redox-sensitive transcription factors (Drögeet al., 1994; Arrigo, 1999). Exposure to chemioxyexcitation constitutessuch a mechanism of modulating redox equilibrium in the alveolarepithelium. Since $gamma$ -GCE is able to suppress intracellular ROSformation, the antioxidant/scavenging effects of this moleculeare likely to inhibit the production ofcytokines.

Further support for the involvement of a glutathione pathway in suppressing pro-inflammatory cytokines was provided with exogenouscysteine, a rate-limiting substrate for GSH biosynthesis. ReplenishingGSH is accomplished by administering compounds that increase thelevel of this amino acid, or by promoting the activity of $gamma$ -GCS.NAC, a cysteine pro-drug, can suppress cytokine production (Peristeriset al., 1992; Jeannin et al., 1995; Gosset et al. 1999) and protectagainst lung injury (Bernard, 1991). In addition, OTC and SAMare incorporated in glutathione therapy, since they provide cysteinefor GSH synthesis (Evans et al., 1997; Anderson and Luo, 1998).Although these agents are effective in suppressing chemioxyexcitation-inducedcytokine release, whether they act as antioxidants and/or pro-drugshas yet to be defined. The pathway implicated with cysteine isto complement the biosynthesis process, where GSH can directlyscavenge ROS. This mechanism does not exclude the probable actionof NAC, OTC, and SAM as antioxidants, which were reported to neutralizeexcess ROS (Aruoma e al., 1989; Evans et al., 1997; Anderson andLuo, 1998). It is apparently evident, therefore, that either pathwayis effectively up-regulated in response to oxidative stress. However,the incapacity of BSO to block NAC-induced suppression of cytokinesallows us to discriminate between the antioxidant/GSH precursorproperties of NAC. These findings are supported by the unequivocalpotency of ebselen, an antioxidant peroxidase mimetic (Schewe,1995), in mitigating the induced release of cytokines. As such,selective modulation of redox pathways regulates the cytokinenetwork in the alveolar epithelium in response tochemioxyexcitation.

Although the involvement of GSSG in pathways governing the induction of cytokines in the alveolar epithelium is not well characterized,its role in determining redox equilibrium is established (Meister,1988; Schreck et al., 1992; Dröge et al., 1994; Haddad et al.,2000a). Replenishing GSH is not only $gamma$ -GCS rate-limited but alsodetermined by the degree of NADPH-dependent GSSG recycling. Thus,favoring an oxidation equilibrium by elevating GSSG has been reportedto activate signaling pathways that down-regulate the activationof transcription factors (Sen, 1998; Schreck et al., 1992; Haddadet al., 2000a). Inhibition of GSSG recycling by BCNU negativelyattenuates the activation of NF- $kappa$ B in vitro (J. J. E. Haddad,R. E. Olver, and S. C. Land, unpublished observations). Intriguingly,GSSG, like GSH, has the potential to down-regulate chemioxyexcitation-dependentcytokine release. It's likely, therefore, that BCNU mitigatesa pro-inflammatory signal by suppressing the activation of NF- $kappa$ B,through elevation of [GSSG] (Shakhov et al., 1990). To confirmthis hypothesis, we used PDTC, a dithiocarbamate that exerts antioxidant/pro-oxidanteffects (Schreck et al., 1992; Brennan and O'Neill, 1996; Wildand Mulcahy, 1999; Haddad et al., 2000a). Dithiocarbamates inhibitthe phosphorylation-dependent release of NF- $kappa$ B from its cytosolicinhibitory subunit, I $kappa$ B (Brennan and O'Neill, 1996), suggestingthat the mechanism of ROS-induced activation of this transcriptionfactor involves a redox-sensitive kinase (Kanakaraj et al., 1998;Li et al., 1999). However, GSSG also promotes the formation ofa NF- $kappa$ B/disulfide complex, directly inhibiting DNA binding (Schrecket al., 1992; Brennan and O'Neill, 1996; Haddad et al., 2000a).PDTC elevates [GSSG] at the expense of [GSH], suggesting thatGSSG contribution to suppression of chemioxyexcitation-inducedcytokine release occurs through NF- $kappa$ B, a transcription factoressentially involved in regulating pro-inflammatory genes (Haddadet al., 2000a). The mechanism involved is that BCNU (GSSG) hasthe potential to retard NF- $kappa$ B nuclear translocation and subsequentactivation, a pathway that in turn switches off the expressionof genes encoding pro-inflammatory cytokines (Pfeilschifter andMühl, 1999).

These pathways, however, do not account for GSSG-induced suppression of cytokines in hypoxia, where NF- $kappa$ B activation stateis depressed in a reducing environment (Brennan and O'Neill, 1996;Haddad and Land, 2000a, Haddad et al., 2000a). Since the activationof hypoxia-inducible factor-1 $alpha$ (HIF-1 $alpha$ ) increases exponentiallyon lowering pO₂, it's possible that this factor is involved inregulating pro-inflammatory genes (Wenger et al., 1996; Hellwig-Bürgelet al., 1999; Yan et al., 1999). BCNU was shown to down-regulateHIF-1 $alpha$ activation in vitro by reducing GSH/GSSG, thereby favoringan oxidation equilibrium (J. J. E. Haddad, R. E. Olver, and S.C. Land, unpublished observations). We are currently extendingthese observations to investigate the kinetics of HIF-1 $alpha$ -mediatedregulation of cytokines in hypoxia. Taken together in hand withselective modulation of glutathione pathways as directly affectingthe cytokine profile, our results have demonstrated a novel mechanismof thiol regulation mediated by glutathione in the alveolar epithelium.Thiol-mediated pathways simulating functional mechanisms controllingpro-inflammatory cytokines are schematized in Fig. 7.

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Fig. 7. Schematic model of thiol regulation of chemioxyexcitation-induced cytokine secretion in the alveolar epithelium. The predominant form of intracellular glutathione is GSH, which is synthesized by $gamma$ -GCS. OTC, SAM, and NAC are major precursors of cysteine, the rate-limiting substrate in the biosynthesis of GSH, a pathway that is selectively blocked by BSO. BSO up-regulates the formation of intracellular ROS, which are major inducers of cytokine secretion. GSH is either rapidly exported, where the membrane-bound $gamma$ -glutamyl transpeptidase ( $gamma$ -GT) degrades it into its subcellular components to be used for resynthesis or is converted by GSSG by GSH-PX and its mimetic ebselen, at the expense of ROS, which are promptly detoxified (reduced) into ROOH, a hydroperoxide, according to the equation ROOH + 2GSH $right-arrow$ ROH + H2O + GSSG. The formation of GSSG and/or reduction of ROS down-regulate the chemioxyexcitation-dependent cytokine release. GSSG is rapidly recycled back into GSH by GSSG-RD, a pathway, which is selectively blocked by BCNU, leading to accumulation of GSSG, which along with pyrrolidine dithiocarbamate, a precursor of GSSG, down-regulates the formation of ROS and abrogates the cytokine-dependent sequelae. Cytokines act as major participants in the pathophysiology and aggravation of the clinical symptoms of respiratory distresses (RD).

This report has elaborated in vitro an immunopharmacological potential of glutathione and subsequent regulation of pro-inflammatorycytokines. These findings are highlighted as follows: 1) selectiveinhibition of $gamma$ -GCS up-regulates cytokines via the formation ofROS; 2) blockage of glutathione recycling uncouples the ROS/cytokinepathway, an effect closely mimicked by PDTC an antioxidant/pro-oxidantagent that elevates [GSSG]; 3) exogenous precursors of [GSH] andcysteine suppress ROS production and the down-stream cytokine-dependentpathway; and 4) shifting redox potential in favor of a reductionequilibrium negatively interferes with the capacity to up-regulatea pro-inflammatory signal. Our results indicate that modulatingredox status by pharmacological thiols has potential clinicalconsequences for the therapeutic treatment of pediatric distressesin which cytokines act as major participants in their pathophysiology.Thus, dynamic variation in pO₂ and redox disequilibrium antagonisticallyregulate chemioxyexcitation-induced cytokines, thereby bearingconsequences for determining the survivorship of epithelial cellsunder conditions mimicking clinical O₂ therapy (Haddad and Land,2000b).

	Acknowledgment

We thank Dr. Stephen Poole from the National Institute for Biological Standards and Control (NIBSC, England, UK) for providingenzyme-linked immunoassay reagents to J.J.H.

	Footnotes

Accepted for publication November 17, 2000.

Received for publication August 25, 2000.

This work was supported by grants from the Medical Research Council, Anonymous Trust and Tenovus-Scotland (S.C.L.). J.J.H.is a recipient of the George John Livanos prize (London). Partof this work was presented at Experimental Biology-2000, San Diego,CA (Haddad et al., 2000b).

Send reprint requests to: Dr. John J. E. Haddad, Oxygen Signaling Group, Center for Research into Human Development, Tayside Institute of Child Health, Faculty of Medicine, Ninewells Hospital and Medical School, University of Dundee, Dundee DD1 9SY, Scotland, UK. E-mail: j.j.haddad{at}dundee.ac.uk

	Abbreviations

GSH, L- $gamma$ -glutamyl-L-cysteinyl-glycine; NAC, N-acetyl-L-cysteine; SAM, S-adenosyl-L-methionine; BCNU, 1,3-bis-(2-chloroethyl)-1-nitrosourea; BSO, L-buthionine-(S,R)-sulfoximine; DHR, dihydrorhodamine; $gamma$ -GCE, $gamma$ -glutamyl-L-cysteinyl-ethyl ester; GSSG, glutathione disulfide oxidized; GSH-PX, glutathione peroxidase; GSSG-RD, glutathione reductase; $gamma$ -GCS, $gamma$ -glutamylcysteine synthetase; GS, glutathione synthase; IL, interleukin; OTC, 2-oxothiazolidine-4-carboxylate; ebselen, 2-phenyl-1,2-benzisoselenazol-3(2H)-one; PDTC, pyrrolidine dithiocarbamate; ROS, reactive oxygen species; redox, reduction-oxidation; TNF- $alpha$ , tumor necrosis factor- $alpha$ ; X/XO, xanthine/xanthine oxidase; DMEM, Dulbecco's modified Eagle's medium; FCS, fetal calf serum; EU, enzyme unit activity; HIF1- $alpha$ , hypoxia-inducible factor 1 $alpha$ ; NF- $kappa$ B, nuclear factor- $kappa$ B.

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