Hemoglobin Toxicity in Experimental Bacterial Peritonitis Is Due to Production of Reactive Oxygen Species

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Clinical and Diagnostic Laboratory Immunology, November 1999, p. 938-945, Vol. 6, No. 6
1071-412X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Hemoglobin Toxicity in Experimental Bacterial Peritonitis Is Due to Production of Reactive Oxygen Species

Yeong-Min Yoo,¹^,² Ki-Mo Kim,¹ Sung-Soo Kim,³ Jeong-A Han,¹ Ho-Zoo Lea,² and Young-Myeong Kim¹^,^*

Departments of Molecular and Cellular Biochemistry¹ and Pharmacology,³ College of Medicine, and Department of Biology, College of Natural Science,² Kangwon National University, Chunchon, Kangwon-do, Korea

Received 9 December 1998/Returned for modification 31 March 1999/Accepted 12 July 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Hemoglobin (Hb) is a toxic molecule responsible for the extreme lethality associated with experimental Escherichia coli peritonitis,but the mechanism has yet to be elucidated. Hb, but not globin,showed toxic effects in a live E. coli model but not in a modelusing killed E. coli. Methemoglobin, hematin, and the well-knownFenton reagents iron and iron-EDTA demonstrated the same lethaleffect in E. coli peritonitis as Hb, while the addition of theFenton inhibitors desferrioxamine (DF) and diethylenetriaminepentaacetate removed most of the cytotoxic activity of iron. Administrationof a combined dose of superoxide dismutase and catalase minimizedthe action of Hb and iron-EDTA, suggesting that both O₂^· and H₂O₂ are involved in the toxic action of Hb in this rat model.The combination of the antioxidative enzymes and DF further suppressediron-mediated lethality. An electron spin resonance techniquewith the spin-trapping reagent 5,5-dimethyl-1-pyroline-N-oxide(DMPO) showed O₂^· generation in the peritoneal fluid of rats injected with E. colialone or E. coli plus iron-DF, and ^·OH generation was detected in the peritoneal fluid of the ratsinjected with iron-EDTA. Hb did not show any spin adduct of oxygenradicals, suggesting that Hb produces non-spin-trapping radicalferryl ion, which decayed the spin adduct of DMPO. In the presenceof Hb or iron-EDTA, O₂-generating activity and viability of phagocytes decreased, whereaslipid peroxidation of peritoneal phagocytes increased. Generationof oxygen radicals and lipid peroxidation did not differ in thelive and dead bacterial models. Bacterial numbers in the peritonealcavity and blood were markedly increased in the live bacterialmodel with Hb and iron-EDTA. The Fenton inhibitor iron-DF preventedthe loss of phagocyte function, lipid peroxidation, and bacterialproliferation. These results led us to conclude that the lethaltoxicity of Hb in bacterial peritonitis is associated with a Fenton-typereaction, the products of which decrease phagocyte viability,through the induction of lipid peroxidation, allowing bacterialproliferation and resulting inmortality.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Phagocytes (macrophages and neutrophils) are primary host defense systems against peritoneal infection. They induce an importantbiochemical pathway, a respiratory burst, which results in generationof O₂^· and H₂O₂, followed by the formation of more-toxic secondary oxidantssuch as hydroxyl radical (^·OH) and HOCl. These oxidizing species are responsible for pathologicalevents (29) such as destruction of biomolecules, killing ofinfected microorganisms, and autokilling of phagocytes. The hydroxylradical is generated by transition metals, particularly iron,via the Fenton reaction in an O₂^·-generating environment. This radical is thought to be a majorspecies for oxygen toxicity in biological systems. Yamazaki andPiette (31) have stoichiometrically measured the formation of^·OH and confirmed the formation of not only ^·OH but also ferryl ion from the Fenton reaction by using a spin-trappingtechnique.

Hemoglobin (Hb) may also act as a Fenton reagent in biological systems (22, 24). This possibility has been supported bymany lines of evidences that show that Hb causes the oxidationof several organic molecules by producing ^·OH and/or ferryl ion [Fe(IV)==O] in the presence of H₂O₂ (9,23). Free Hb causes injury to the central nervous system throughperoxidation of membrane lipid (26). We confirmed that neutrophilswere inactivated by the oxidizing species, ferryl ion, producedfrom Hb in O₂^·-generating systems (17).

Hb has been known as a potent toxic molecule responsible for the high lethality associated with experimental Escherichia coliperitonitis since the early 1960s, when Davis and Yull (3,4) discovered a synergistic effect on mortality between bacteriaand erythrocytes in the peritoneums of rats. This synergisticaction is a perplexing problem caused by the combination of bloodand bacteria during surgery. Recently, Kim et al. reported thaterythrocytes scavenge both O₂^· and nitric oxide and then inhibit the formation of the bactericidalmolecule peroxynitrite (14). Although the lethal toxicity ofpurified Hb has been thought to be associated with various biochemicalevents in the peritoneal cavity (1, 7), the lethal effectof Hb in the animal model is not fullyunderstood.

We have therefore examined the possibilities that Hb produces strong oxidizing species by reacting with O₂^· and H₂O₂ generated by recruited neutrophils in the peritonealcavity and that these oxidizing species cause deleterious effectson the host defense system. By comparing Hb toxicity with theeffects of well-known Fenton reagents and inhibitors on the mortalityof rats, reactive oxygen production, and the pathobiochemicalchanges in this animal model, we demonstrated that a Fenton-typereaction producing reactive oxygen species may be involved inthe lethality of Hb in experimental E. coliperitonitis.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials. Catalase (CAT) (from bovine liver), superoxide dismutase (SOD) (from bovine erythrocytes), phorbal myristate acetate, cytochromec (from horse heart), phosphate-buffered saline (PBS) (pH 7.4),5,5-dimethyl-1-pyroline-N-oxide (DMPO), globin, and hemin wereobtained from Sigma. DMPO was used after redistillation. DesferrioxamineB (deferoxamine) (DF) was from CIBA Pharmaceutical Co. Hematinsolutions were prepared by dissolving hemin in a small volumeof weak alkaline solution and diluting with PBS within 1 h ofexperiments. Hb was prepared from bovine erythrocytes by a one-stepprocedure with a DEAE-Sephadex A-50 column (30). Methemoglobin(MetHb) was prepared by oxidizing Hb with a slight excess of potassiumferricyanide and separated from the added components through aSephadex G-25 column. Hb and MetHb were concentrated with a Centriconapparatus (Amicon). The Hb concentration was calculated as a hemeconcentration byspectrophotometry.

Preparation of bacterial solution. E. coli (ATCC 25922) was incubated on a blood agar plate at 37°C for 17 h, and a single colony was cultured in tryptic soybroth for an additional 18 h to produce a suspension of approximately10⁹ cells/ml. The bacteria were harvested by centrifugation, washedthree times with saline, and resuspended in saline. The cell concentrationwas measured by spectrophotometry at 550 nm. The bacterial solution(absorbance was ~1.0 at 550 nm) was diluted in PBS by 10⁶- and 10⁷-fold, inoculated on agar plates, and incubated at 37°C for 18h (17). The number of viable bacteria was measured by countingdeveloped colonies. Killed E. coli was prepared by treatment withformalin (5).

Animal mortality. Male Sprague-Dawley rats (180 to 200 g) were given standard rat pellets and water ad libitum. Experimental peritonitis wasinduced in rats by intraperitoneal (i.p.) injection of E. coli(4 × 10⁹ CFU/kg of body weight) with or without iron complexes (12.4 µmolof iron/kg of body weight). The injection mixtures were preparedimmediately before injection, and the injection volume was 5 ml/kgof body weight. Mortality of rats was determined at 24 h afteradministration. The effects of SOD and CAT were examined by twoi.p. injections of 2,600 and 11,000 U/kg of body weight, respectively,at 0 and 8 h following injection ofbacteria.

Measurement of O₂^· production in the peritoneal fluid. The rats injected i.p. with viable E. coli with or without an iron complex were anesthetized with an intramuscular injectionof Ketamine (44 mg/kg) at various time points. The rats were i.p.injected with 1 ml of saline and then physically shaken for 1min to ensure adequate mixing of peritoneal contents. A midlinelaparotomy was performed, and the fluid was obtained from allregions of the peritoneal cavity. O₂^· generation in an ex vivo system was measured by SOD (100 U/ml)-inhibitablecytochrome c reduction, monitored at 550 nm ( $Delta$ $varepsilon$ ₅₅₀ = 21 mM¹ cm¹ for reduced oxidized cytochrome c), in PBS (1 ml) containingcytochrome c (100 µM), peritoneal fluid (250 µl), and CAT (100U).

Isolation, quantitation, and viability of peritoneal phagocytes. All peritoneal fluid was obtained from the rats injected i.p. with viable E. coli with or without an iron complex. Peritonealphagocytes were prepared by centrifugation at 300 × g for 8 minand washed twice with ice-cold PBS. The cell pellets were resuspendedin PBS. Total phagocytes (macrophages and neutrophils) were countedby light microscopy with trypan blue staining. For counting themacrophage population, a cell suspension was plated on 24-wellplates and incubated for 2 h at 37°C in a CO₂ incubator. The plateswere washed three times with PBS, and the adhering cells werecounted by light microscopy. Cell viability was determined bytrypan blue dyeexclusion.

Bacterial counts in peritoneal fluid and blood. Blood was collected by heart puncture and collected in a Vacutainer (Becton Dickinson; 7-ml capacity) containing 10.5 mg ofEDTA. Peritoneal fluid and blood samples were diluted with ice-coldsterile water. The number of viable bacteria was measured as describedabove.

Lipid peroxidation. Peritoneal exudate cells were prepared by centrifugation at 500 × g for 10 min and suspended in a small volume of PBS. Lipidperoxidation was assayed by measuring thiobarbituric acid (TBA)-reactivesubstance (TBARS) at 532 nm (2). A sample (0.25 ml) was mixedwith 0.5 ml of trichloroacetic acid-TBA-HCl (15%, 0.375%, and0.25 N, respectively) containing 0.05% butylated hydroxytoluene.The mixture was heated in a boiling water bath for 20 min. Afterbeing cooled with tap water, the mixture was centrifuged at 2,200× g and 4°C for 20 min. The absorbance of the supernatant wasmeasured at 532 nm. TBARS as a lipid peroxide level was calculatedby using an extinction coefficient of 1.56 × 10⁵ M¹ cm¹.

ESR spectroscopy of DMPO spin adducts. Peritoneal fluid was collected from the rats 4 h after the i.p. injection of E. coli with or without iron complexes. The fluid(460 µl) was mixed with 40 µl of 1 M DMPO and incubated at 37°Cfor 8 min. The mixture was immediately transferred into an electronspin resonance (ESR) flat cell, and ESR spectra were recordedwith a Varian E-109 spectrometer. Spectrometer settings were asfollows: microwave power, 20 mW; modulation frequency, 100 kHz;modulation amplitude, 1.0 G; time constant, 0.25 s; receiver gain,1.25 × 10⁴. For decay of DMPO-OH by ferryl ion, DMPO-OH was formed by incubationof DMPO (10 mM), 100 µM Fe²⁺-EDTA, and 200 µM H₂O₂ for 1 min and then addition of CAT (100U/ml) to remove excessive H₂O₂. The reaction mixture was incubatedwith or without ferryl ion, which is generated by mixing Hb (0.4mM) with H₂O₂ (0.4 mM) for 4 min and then incubating with 100U of CAT/ml for 1 min. After 8 min, ESR spectra were recordedwith a Varian E-109 spectrometer with a receiver gain of 2 × 10².

Statistical analysis. Data were analyzed by the chi-square test for animal mortality and by the Student t test. Statistical significance was establishedat a P value of <0.05.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

As shown by Simmons' group (5, 6, 10, 11, 19, 22), purified Hb administered simultaneously with E. coli intothe peritoneal cavity results in a potentiated lethal effect (Fig.1). Viable E. coli at 8 × 10⁸ bacteria/200 g of body weight, which is a nonlethal dose, resultedin more than 80% mortality when Hb was administered within 24h of injection (Fig. 1A). However, formalin-killed E. coli, showinga similar dose-response mortality curve at a concentration about100 times higher than that for live bacteria, did not show a synergisticeffect on mortality at 5 × 10¹⁰ bacteria/200 g of body weight when concomitantly injected withHb (Fig. 1B), indicating that the viability of E. coli is an importantfactor in the toxic effect of Hb in experimental peritonitis.

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FIG. 1. Effect of Hb on mortality in experimental E. coli peritonitis. Six or seven animals were studied in each group. Mortality was measured at 24 h after i.p. injection of live E. coli (A) or formalin-killed E. coli (B) with or without Hb (12.4 mmol/kg of body weight [BW]). The total volume of the injection was 5 ml/kg of body weight.

It is well known that iron from a variety of sources, including Hb, can enter into Fenton-type chemistry (25) and that neutrophilsinfiltrating the infectious site produce O₂^· (13). It is therefore possible that Hb as a Fenton reagentproduces a highly toxic oxidant in the peritoneal cavity duringbacterial peritonitis. To test the hypothesis that a Fenton-typereaction is responsible for the lethal effect of Hb in bacterialperitonitis, we investigated the effects of globin, hematin, andseveral iron(II) chelates on mortality in the rat peritonitismodel (Fig. 2). Hematin, iron itself, and iron-EDTA showed effectson mortality similar to those of Hb, whereas globin did not showa toxic effect. The initial valence state of iron, either ferrousor ferric, did not change the mortality (data not shown). UnlikeEDTA, DF and diethylenetriamine pentaacetate (DTPA) significantlyreduced the toxic effect of iron itself in experimental peritonitis.These data suggest that a Fenton-type reaction may be involvedin the toxic effect of Hb in this animal model.

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FIG. 2. Effects of Hb, globin, hematin, and iron chelates on mortality in experimental E. coli peritonitis. Rats were injected i.p. with E. coli (4 × 10⁹ cells/kg of body weight) and iron complex or globin (12.4 mmol/kg of body weight), and mortality was determined at 24 h after injection. The injection mixtures were prepared immediately before injection. The total volume injected was 5 ml/kg of body weight. The molar ratio of iron(II) to chelator was 1:2. The ratio of dead rats to treated rats is indicated above each bar. Statistically significant mortality reductions (asterisks) with chelators, DF, and DTPA versus iron ion itself (P < 0.001) were determined by the chi-square test. MetHb and iron(III) ion had the same adjuvant effects as Hb and Fe(II) ion, respectively.

To test whether iron complexes play a role as a Fenton reagent in the rat peritonitis model, the effects of SOD and CAT onmortality and on generation of O₂^· and H₂O₂ in the peritoneal cavity (since these oxygen metabolitesare important reagents in Fenton chemistry) were investigated.A mixture of SOD and CAT was injected twice i.p. with E. coliand Hb or iron-EDTA into rats, simultaneously and 8 h after injectionof bacteria. The toxic effect of the iron complexes on mortalitywas examined at 24 h after treatment. Administration of an SOD-CATmixture reduced the toxic action of Hb (P < 0.01) and iron-EDTA(P < 0.01), though not completely (Fig. 3). Furthermore, the combinationof the antioxidative enzymes and DF strongly suppressed iron-mediatedlethality. The results suggest that phagocytes (resident macrophagesand recruited neutrophils) produced activated oxygen species (O₂^· and H₂O₂), which react with Hb and iron-EDTA to generate more-toxicspecies such as ferryl ion and ^·OH.

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FIG. 3. Effect of both SOD and CAT on the adjuvant effect of Hb or iron-EDTA in experimental E. coli peritonitis. Experimental conditions were as described in the legend to Fig. 2, except that SOD and CAT were injected i.p. twice, at 2,600 and 11,000 U/kg, respectively, at 0 and 8 h after i.p. injection of E. coli and adjuvant. The ratio of dead rats to treated rats is indicated above each bar. Statistically significant mortality reductions versus each control were determined by the chi-square test (*, P < 0.01; **, P < 0.05).

To establish definitively the generation of reactive oxygen species in our experimental model, we used ESR spectroscopy todetect spin adducts of DMPO with oxygen radicals which were generatedin the peritoneal fluid collected from rats at 4 h after injectionwith bacteria alone or bacteria plus iron chelates. As shown inFig. 4A, DMPO spin adducts were not found in the peritoneal fluidof rats which received saline as a control. The mixtures of DMPOspin adducts of O₂^· (DMPO-OOH) and ^·OH (DMPO-OH), but mostly DMPO-OH, were detected directly in theperitoneal fluid of rats injected with bacteria alone (Fig. 4B).The spectrum obtained for the system of bacteria plus iron-DFwas not different from that obtained for rats injected with bacteriaalone (Fig. 4E). Under the same experimental conditions, the spectrumof DMPO-OH disappeared with the addition of SOD (data not shown),indicating that DMPO-OH was generated by decay of DMPO-OOH, aspreviously reported (20). However, the spectrum of only DMPO-OHwas identified in the peritoneal fluid of rats injected with bacteriaplus iron-EDTA (Fig. 4D), but no spin adduct was found in ratsinjected with bacteria plus Hb (Fig. 4C). Since DMPO spin adductscan be rapidly decayed by the reaction product of Hb and H₂O₂,the disappearance of the DMPO adduct of ^·OH was examined. An ESR spectrum of DMPO-OH was detected in themixture of iron-EDTA and H₂O₂ (Fig. 4F), and this spectrum disappearedwith the addition of ferryl ion generated from the reaction ofHb with H₂O₂ (Fig. 4G).

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FIG. 4. ESR spectrum of DMPO spin adducts of oxygen radical generated in peritoneal fluid. DMPO spin adducts in peritoneal fluids collected from rats injected with saline (A), E. coli (B), E. coli plus Hb (C), E. coli plus iron-EDTA (D), or E. coli plus iron-DF (E) were measured. In vitro formation of DMPO-OH was detected in the reaction mixture of Fe²⁺-EDTA and H₂O₂ (F) in the presence of ferryl ion (G), which is formed by incubation of Hb and H₂O₂, by ESR spectroscopy. Spectrometer settings are described in Materials and Methods. The spectra were from one of three experiments, which showed similar results.

Our previous data showed that neutrophils are inactivated by toxic oxidants generated from Fenton-type reagents, includingHb in an O₂^·-generating system (17). To test if peritoneal phagocytes areinactivated by iron complexes in experimental bacterial peritonitis,we examined the phagocyte population and its O₂^·-generating activity in the peritoneal cavity (Fig. 5). The numbersof peritoneal macrophages were nearly unchanged, while the neutrophilpopulation was significantly increased after 4 h of bacterialinjection (Fig. 5A). The O₂^·-generating activity of the peritoneal phagocytes isolated fromrats injected with E. coli alone or E. coli plus iron-DF increasedafter 2 h and reached maximum levels after 7 h (P < 0.01) (Fig.5B). Under the same conditions, however, treatment with iron-EDTAor Hb attenuated the O₂^·-generating activity of peritoneal phagocytes.

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FIG. 5. Quantitation of peritoneal phagocytes and their O₂^·-generating activity in experimental E. coli peritonitis. Numbers of total peritoneal phagocytes were determined by light spectroscopy with the trypan blue staining method. Macrophages were counted from adhered cells on culture plates. Subpopulations of neutrophils and macrophages (A) were calculated by the subtraction method. O₂^· production (B) was measured by SOD-inhibitable cytochrome c reduction in peritoneal phagocytes obtained from the rats injected with bacteria in the absence of iron complex and in the presence of Hb, iron-EDTA, or iron-DF. Each point represents the mean ± standard deviation for three individual rats.

Toxic oxidants produced from a Fenton-type reaction cause oxidative injury through lipid peroxidation (28), resulting incell death and inactivation of neutrophil function (17). Toaddress this concern, lipid peroxidation and phagocyte viabilitywere measured in the peritoneal phagocytes of rats injected withE. coli and iron complexes. Figure 6A shows that injection ofE. coli alone into the peritoneal cavity did not significantlyincrease lipid peroxidation in peritoneal phagocytes, but itsinjection with Hb or iron-EDTA markedly increased lipid peroxidationin peritoneal phagocytes (P < 0.02 at 15 h). Iron-DF had no effecton lipid peroxidation. Phagocyte viability in the peritoneal cavitydecreased (P < 0.01 at 15 h) following injection with Hb or iron-EDTAbut did not decrease significantly (P > 0.1 at 15 h) when bacteriawere injected alone or with iron-DF (Fig. 6B). Furthermore, weexamined the effects of live and dead E. coli on reactive oxygengeneration and lipid peroxidation in the peritoneal cavity. Theformation of DMPO spin adducts and lipid peroxidation in the peritonealcavity were not significantly different between these peritonitismodels with or without Hb (Table 1). These results suggest thatbacterial proliferation through phagocyte inactivation is a criticalfactor for Hb toxicity in E. coli peritonitis.

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FIG. 6. Effects of Hb and iron chelates on lipid peroxidation (A) and viability (B) of peritoneal phagocytes during E. coli peritonitis. Peritoneal phagocytes were prepared by centrifugation immediately after collection of the peritoneal fluids and washed with PBS. Data represent the means ± standard deviations for three individual rats, with results obtained in duplicate for each experiment.

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TABLE 1. Effects of live and dead E. coli on reactive oxygen generation and lipid peroxidation in bacterial peritonitis

From work performed by Dunn et al. (5) and O'Brien (21), one might conclude that an important role for Hb or any ironsource in experimental peritonitis is to cause uncontrolled bacterialproliferation in the peritoneal cavity. Although for E. coli alonethe number of cells in the peritoneal cavity began to decreaseafter an initial weak increase, the number of E. coli cells injectedwith Fenton-type reagents, Hb, or iron-EDTA rapidly increasedin the peritoneal cavity, by about 10³-fold within 15 h (P < 0.01) (Fig. 7A). The number of viable bacteriain blood was lower than that in the peritoneal cavity but itstime dependence was identical to that in the peritoneal cavity(Fig. 7B). When Fe-DF (ratio of 1 to 2) was injected, the numbersof viable bacteria in the peritonal cavity and blood were similarto those in animals injected with bacteria alone until 10 h andthereafter were a little higher (P < 0.05 at 15 h), probably dueto the suppression of phagocyte-dependent bacterial killing bythe excessive amount of DF (27).

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FIG. 7. Effects of Hb and iron chelates on bacterial proliferation in the peritoneal cavity (A) and blood (B) during E. coli peritonitis. Experimental conditions were the same as described in the legend to Fig. 5. Each point represents the mean ± standard deviation of CFU from two individual rats, with results obtained in triplicate, at each indicated time point after i.p. inoculation with E. coli.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

As reported previously (6, 18), Hb increased lethality in experimental bacterial peritonitis. The most prominent characteristicreported so far regarding the toxic effect of Hb in experimentalperitonitis seems to be the significantly increased rate of bacterialproliferation in vivo (7, 11). Hb did not increase the lethalityin a peritonitis model of killed E. coli, supporting a role forHb in increasing bacterial growth. We previously reported thatHb diminished the microbicidal activity of neutrophils in an O₂^·-generating system (17), and we postulated that a Fenton reactionproducing toxic radicals played an important role in neutrophilinactivation. We here report that Hb and the Fenton reagent iron-EDTA,but not the Fenton inhibitor iron-DF, increased lethal toxicityby decreasing phagocyte viability and increasing bacterial growthin experimental bacterialperitonitis.

Peritoneal phagocytes such as resident macrophages and infiltrating neutrophils are the first line of defense against bacterialperitonitis. They produce O₂^· and H₂O₂, which are implicated in bacterial killing. O₂^· supplied by phagocytes interacts with oxidized iron to generatethe reduced form of iron. The reduced forms of iron ion and itschelate complexes are well-known Fenton reagents that react withH₂O₂ to produce strong oxidizing species such as ^·OH and Fe(IV)==O, which oxidize several cellular components (17,24).

Many investigators (9, 23, 25, 26, 30) have reported that Hb produces oxidizing species, ^·OH and/or Fe(IV)==O, in the presence of H₂O₂ through a Fenton-typereaction. It has been suggested that these oxidizing species areresponsible for oxygen toxicity, including neutrophil inactivation(17) and protein degradation (16), in various biological systems.Although iron(II)-DF and iron(II)-DTPA produce ^·OH in the presence of H₂O₂, DF and DTPA, probably because of theslow oxidation-reduction cycle of these iron chelates, are knowninhibitors of the Fenton reaction. Here, we will first focus ourdiscussion on the possibility that the lethal effects of Hb andiron-EDTA in our peritonitis model are associated with the productionof oxidizing species through a Fenton-type reaction (Fig. 2).Dead bacteria or lipopolysaccharide can also stimulate phagocytesand produce reactive oxygen species (12). The oxygen radicalsinactivate the O₂^·-generating activity of neutrophils through lipid peroxidationin the presence of a Fenton reagent in vitro (17). AlthoughHb also increases peroxidation through oxygen radical generationin dead E. coli peritonitis to a level similar to that in liveE. coli peritonitis (Table 1), Hb did not enhance the lethaleffect (Fig. 1B). These results suggest that bacterial proliferationthrough decreased phagocyte function in the peritoneal cavityis one critical factor for Hb-mediated adjuvant mortality in bacterialperitonitis.

SOD and CAT are powerful scavengers of O₂^· and H₂O₂. Therefore, they are effective in inhibiting a Fenton reaction (18) andneutralizing neutrophil-mediated tissue damage (8). In ourperitonitis model, administration of SOD and CAT reduced the lethaleffect of Hb and iron-EDTA (Fig. 3), and the Fenton inhibitorsDF and DTPA also suppressed the lethal effect of iron (Fig. 2).Furthermore, the combination of SOD, CAT, and DF strongly inhibitediron-mediated mortality in our peritonitis model. These resultssuggest that O₂^· and H₂O₂ are involved in the production of oxidizing speciesfrom the Fenton reaction of Hb and cause the toxic effect of Hbin our peritonitismodel.

Phagocytes, i.e., macrophages and neutrophils, are known to produce O₂^· and H₂O₂, which normally are involved in the killing of infectiousbacteria, and such was the case when E. coli alone was injected.These oxygen species can interact with Fenton reagents such asiron-EDTA and Hb and produce stronger oxidants such as ^·OH and ferryl ion, which are involved in tissue injury throughlipid peroxidation (17). ESR spectroscopy showed direct evidencethat peritoneal phagocytes produce reactive oxygen species duringbacterial peritonitis, followed by the formation of more-autotoxicsecondary oxidants such as ^·OH or ferryl ion in the presence of Fenton reagents. Neither O₂^· nor ^·OH was detected in the peritoneal cavities of the rats injectedwith bacteria plus Hb. A major reactive species produced by thereaction of Hb with H₂O₂ is thought to be ferryl ion (17), whichis not directly trapped by DMPO (31). The ferryl species rapidlydecayed DMPO spin adducts to other products that were not detectedby ESR spectroscopy (15). This evidence may explain why no ESRspectrum was detected when Hb was injected into the peritonealcavity. These results indicate that the large number of neutrophilswhich migrated into the peritoneal cavity 4 h after bacterialinjection appear to be the major source of O₂^· and H₂O₂, participating in lipid peroxidation, inactivation ofphagocytic function, and bacterial proliferation via a Fentonreaction.

^·OH and ferryl ion are highly reactive species and react with a variety of biological molecules such as protein, membrane lipid,and nucleic acids. Peroxidation of membrane lipid is a major cellularinjury caused by these oxidizing species. This markedly decreasedthe O₂^· production in the peritoneal cavity in the presence of Hb oriron-EDTA (Fig. 5), probably because of the decreased phagocyteviability through Fenton-type reactions (Fig. 6B). Inactivationof phagocyte function allowed increased bacterial proliferation(Fig. 7). The protective effect of DF on O₂^· production suggests that the Fenton-type reaction causes inactivationof the peritoneal phagocytes. The results are in accordance within vitro neutrophil inactivation by Fenton-type iron complexesin the O₂^·-generating system (17).

Hb can interact with NO, synthesized from L-arginine by any of the three isotypes of NO synthase and oxidized to nitrate,which is a nontoxic stable product. Hb is known to be a biologicalscavenger of NO. NO interacts with O₂^· and then produces highly toxic peroxynitite, which reacts againstbacteria and host cells. Recent studies have reported that erythrocytesinhibit the formation of peroxynitrite and allow bacteria to proliferatein the peritoneal cavity, resulting in increased mortality (14).Purified Hb is very much different from erythrocytes, becauseerythrocytes contain many different types of antioxidative enzymesand antioxidants. The toxic mechanism of purified Hb may be differentfrom that of Hb in erythrocytes. Like Hb, the Fenton inhibitorFe-DTPA can interact with NO and neutralize the biological andpathological functions of NO (13). However, Fe-DTPA did notshow a synergistic effect on mortality with bacteria in our animalmodel. The production of reactive oxygen species, but not NO,in the peritoneal cavity was detected by ESR 4 h after bacterialinjection, because NO is produced in vivo by the induction ofinducibe NO synthase 8 to 10 h after injection of lipopolysaccharideor bacteria. These results suggest that inactivation of phagocytefunction may be due to a reactive oxygen-dependent Fentonreaction.

The products formed by the Fenton reaction, ferryl ion and ^·OH, may indiscriminately destroy biomolecules to kill not onlyhost cells but also microorganisms in the infectious site. Inour peritonitis model, however, apparently the host cells aredestroyed and the numbers of viable bacteria in the peritonealcavity and blood increase (Fig. 6). This finding could be explainedby assuming that the phagocytes are more susceptible to the oxidizingspecies than the bacteria because of differences in the cell wallstructures or proximity of the oxidant formation, resulting inbacterial proliferation. These phenomena are enhanced by the additionof Hb or iron-EDTA but not iron-DF, supporting the hypothesisthat Hb in this rat model produces oxidizing species which decreasephagocyte viability in the peritoneal cavity to allow bacterialproliferation, resulting inlethality.

	ACKNOWLEDGMENT

This work was supported by Korea Science and Engineering Foundation grant 981-0714-100-2 and Korea Research Foundation grant1998-021-F00050.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular and Cellular Biochemistry, College of Medicine, Kangwon NationalUniversity, Chunchon, Kangwon-do, Korea. Phone: 82-361-250-8831.Fax: 82-361-242-7571. E-mail: ymkim{at}cc.kangwon.ac.kr.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bornside, G. H., P. J. Bouis, Jr., and I. Cohn, Jr. 1970. Enhancement of Escherichia coli infection and endotoxic activity by hemoglobin and ferric ammonium citrate. Surgery 68:350-355[Medline].

2. Buege, J. A., and S. D. Aust. 1978. Microsomal lipid peroxidation. Methods Enzymol. 52:302-310[Medline].

3. Davis, J. H., and A. B. Yull. 1962. A possible toxic factor in abdominal injury. J. Trauma 2:291-300.

4. Davis, J. H., and A. B. Yull. 1964. A toxic factor in abdominal injury. II. The role of the red cell component. J. Trauma 4:84-90.

5. Dunn, D. L., R. A. Barke, J. T. Lee, Jr., R. M. Condie, E. W. Humphrey, and R. L. Simmons. 1983. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. VII. Hemoglobin does not inhibit clearance of Escherichia coli from the peritoneal cavity. Surgery 94:487-493[Medline].

6. Dunn, D. L., R. D. Nelson, R. M. Condie, and R. L. Simmons. 1983. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. VI. Effects of stroma-free hemoglobin and red blood cell stroma on mortality and neutrophil function. Surgery 93:653-659[Medline].

7. Filler, R. M., and H. K. Sleeman. 1967. Pathogenesis of peritonitis. I. The effect of Escherichia coli and hemoglobin on peritoneal absorption. Surgery 61:385-392[Medline].

8. Grisham, M. B., and D. N. Granger. 1988. Neutrophil-mediated mucosal injury. Dig. Dis. Sci. 33(Suppl.):6S-15S[Medline].

9. Gutteridge, J. M. C. 1986. Iron promoters of the Fenton reaction and lipid peroxidation can be released from haemoglobin by peroxides. FEBS Lett. 201:291-295[Medline].

10. Hau, T., R. D. Nelson, V. D. Fiegel, R. Levenson, and R. L. Simmons. 1977. Mechanisms of the adjuvant action of hemoglobin in experimental peritonitis. 2. Influence of hemoglobin on human leukocyte chemotaxis in vitro. J. Surg. Res. 22:174-180[Medline].

11. Hau, T., R. Hoffman, and R. L. Simmons. 1978. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. I. In vivo inhibition of peritoneal lekocytosis. Surgery 83:223-229[Medline].

12. Jersmann, H. P., D. A. Rathjen, and A. Ferrante. 1998. Enhancement of lipopolysaccharide-induced neutrophil oxygen radical production by tumor necrosis factor alpha. Infect. Immun. 66:1744-1747[Abstract/Free Full Text].

13. Kazmierski, W. M., G. Wolberg, J. G. Wilson, S. R. Smith, D. S. Williams, H. H. Thorp, and L. Molina. 1996. Iron chelates bind nitric oxide and decrease mortality in an experimental model of septic shock. Proc. Natl. Acad. Sci. USA 93:9138-9141[Abstract/Free Full Text].

14. Kim, Y. M., S. J. Hong, T. R. Billiar, and R. L. Simmons. 1996. Counterprotective effect of erythrocytes in experimental bacterial peritonitis is due to scavenging of nitric oxide and reactive oxygen intermediates. Infect. Immun. 64:3074-3080[Abstract].

15. Kim, Y. M., S. H. Jeong, I. Yamazaki, L. H. Piette, S. Han, and S. J. Hong. 1995. Decay studies of DMPO-spin adducts of free radicals produced by reactions of metmyoglobin and methemoglobin with hydrogen peroxide. Free Radic. Res. 22:11-21[Medline].

16. Kim, Y. M., S. S. Kim, G. Kang, Y. M. Yoo, K. M. Kim, M. E. Lee, J. A. Han, and S. J. Hong. 1998. Comparative studies of protein modification mediated by Fenton-like reaction of iron, hematin, and hemoglobin: generation of different reactive oxidizing species. J. Biochem. Mol. Biol. 31:161-169.

17. Kim, Y. M., I. Yamazaki, and L. H. Piette. 1994. The effect of hemoglobin, hematin, and iron on neutrophil inactivation in superoxide generating system. Arch. Biochem. Biophys. 309:308-314[Medline].

18. Kuppusamy, P., and J. L. Zweier. 1989. Characterization of free radical generation by xanthine oxidase. Evidence for hydroxyl radical generation. J. Biol. Chem. 264:9880-9884[Abstract/Free Full Text].

19. Lee, J. T., Jr., D. H. Ahrenholz, R. D. Nelson, and R. L. Simmons. 1979. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. V. The significance of the coordinated iron component. Surgery 86:41-48[Medline].

20. Lioyd, R. V., and R. P. Mason. 1990. Evidence against transition metal-independent hydroxyl radical generation by xanthine oxidase. J. Biol. Chem. 265:16733-16736[Abstract/Free Full Text].

21. O'Brien, A. D. 1982. Innate resistance of mice to Salmonella typhi infection. Infect. Immun. 38:948-952[Abstract/Free Full Text].

22. Pruett, T. L., O. D. Rotstein, V. D. Fiegel, J. J. Sorenson, R. D. Nelson, and R. L. Simmons. 1984. Mechanism of the adjuvant effect of hemoglobin in experimental peritonitis. VIII. A leukotoxin is produced by Escherichia coli metabolism in hemoglobin. Surgery 96:375-383[Medline].

23. Puppo, A., and B. Halliwell. 1988. Formation of hydroxyl radicals from hydrogen peroxide in the presence of iron. Is haemoglobin a biological Fenton reagent? Biochem. J. 249:185-190[Medline].

24. Rush, J. D., and W. H. Koppenol. 1986. Oxidizing intermediates in the reaction of ferrous EDTA with hydrogen peroxide. Reactions with organic molecules and ferrocytochrome c. J. Biol. Chem. 261:6730-6733[Abstract/Free Full Text].

25. Sadrzadeh, S. M. H., E. Graf, S. S. Panter, P. E. Hallaway, and J. W. Eaton. 1984. Hemoglobin. A biologic Fenton reagent. J. Biol. Chem. 259:14354-14356[Abstract/Free Full Text].

26. Sadrzadeh, S. M. H., and J. W. Eaton. 1988. Hemoglobin-mediated oxidant damage to the central nervous system requires endogenous ascorbate. J. Clin. Investig. 82:1510-1515.

27. Sane, A., S. Manzi, J. Perfect, A. J. Herzberg, and J. O. Moore. 1989. Desferoxamine treatment as a risk factor for zygomycete infection. J. Infect. Dis. 159:151-152[Medline].

28. van-Bebber, I. P., W. K. Boekholz, R. J. Goris, P. H. Schillings, H. P. Dinges, S. Bahrami, H. Redl, and G. Schlag. 1989. Neutrophil fuction and lipid peroxidation in a rat model of multiple organ failure. J. Surg. Res. 47:471-475[Medline].

29. Weiss, S. J., and A. F. LoBuglio. 1982. Biology of disease. Phagocyte-generated oxygen metabolites and cellular injury. Lab. Investig. 47:5-18[Medline].

30. Winterbourn, C. C. 1985. Reaction with superoxide with hemoglobin, p. 137-141. In R. A. Greenwald (ed.), CRC handbook of methods for oxygen radical research. CRC Press Inc., Boca Raton, Fla

31. Yamazaki, I., and L. H. Piette. 1990. ESR spin-trapping studies on the reaction of Fe²⁺ ions with H₂O₂-reactive species in oxygen toxicity in biology. J. Biol. Chem. 265:13589-13594[Abstract/Free Full Text].

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1.	Bornside, G. H., P. J. Bouis, Jr., and I. Cohn, Jr. 1970. Enhancement of Escherichia coli infection and endotoxic activity by hemoglobin and ferric ammonium citrate. Surgery 68:350-355[Medline].
2.	Buege, J. A., and S. D. Aust. 1978. Microsomal lipid peroxidation. Methods Enzymol. 52:302-310[Medline].
3.	Davis, J. H., and A. B. Yull. 1962. A possible toxic factor in abdominal injury. J. Trauma 2:291-300.
4.	Davis, J. H., and A. B. Yull. 1964. A toxic factor in abdominal injury. II. The role of the red cell component. J. Trauma 4:84-90.
5.	Dunn, D. L., R. A. Barke, J. T. Lee, Jr., R. M. Condie, E. W. Humphrey, and R. L. Simmons. 1983. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. VII. Hemoglobin does not inhibit clearance of Escherichia coli from the peritoneal cavity. Surgery 94:487-493[Medline].
6.	Dunn, D. L., R. D. Nelson, R. M. Condie, and R. L. Simmons. 1983. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. VI. Effects of stroma-free hemoglobin and red blood cell stroma on mortality and neutrophil function. Surgery 93:653-659[Medline].
7.	Filler, R. M., and H. K. Sleeman. 1967. Pathogenesis of peritonitis. I. The effect of Escherichia coli and hemoglobin on peritoneal absorption. Surgery 61:385-392[Medline].
8.	Grisham, M. B., and D. N. Granger. 1988. Neutrophil-mediated mucosal injury. Dig. Dis. Sci. 33(Suppl.):6S-15S[Medline].
9.	Gutteridge, J. M. C. 1986. Iron promoters of the Fenton reaction and lipid peroxidation can be released from haemoglobin by peroxides. FEBS Lett. 201:291-295[Medline].
10.	Hau, T., R. D. Nelson, V. D. Fiegel, R. Levenson, and R. L. Simmons. 1977. Mechanisms of the adjuvant action of hemoglobin in experimental peritonitis. 2. Influence of hemoglobin on human leukocyte chemotaxis in vitro. J. Surg. Res. 22:174-180[Medline].
11.	Hau, T., R. Hoffman, and R. L. Simmons. 1978. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. I. In vivo inhibition of peritoneal lekocytosis. Surgery 83:223-229[Medline].
12.	Jersmann, H. P., D. A. Rathjen, and A. Ferrante. 1998. Enhancement of lipopolysaccharide-induced neutrophil oxygen radical production by tumor necrosis factor alpha. Infect. Immun. 66:1744-1747[Abstract/Free Full Text].
13.	Kazmierski, W. M., G. Wolberg, J. G. Wilson, S. R. Smith, D. S. Williams, H. H. Thorp, and L. Molina. 1996. Iron chelates bind nitric oxide and decrease mortality in an experimental model of septic shock. Proc. Natl. Acad. Sci. USA 93:9138-9141[Abstract/Free Full Text].
14.	Kim, Y. M., S. J. Hong, T. R. Billiar, and R. L. Simmons. 1996. Counterprotective effect of erythrocytes in experimental bacterial peritonitis is due to scavenging of nitric oxide and reactive oxygen intermediates. Infect. Immun. 64:3074-3080[Abstract].
15.	Kim, Y. M., S. H. Jeong, I. Yamazaki, L. H. Piette, S. Han, and S. J. Hong. 1995. Decay studies of DMPO-spin adducts of free radicals produced by reactions of metmyoglobin and methemoglobin with hydrogen peroxide. Free Radic. Res. 22:11-21[Medline].
16.	Kim, Y. M., S. S. Kim, G. Kang, Y. M. Yoo, K. M. Kim, M. E. Lee, J. A. Han, and S. J. Hong. 1998. Comparative studies of protein modification mediated by Fenton-like reaction of iron, hematin, and hemoglobin: generation of different reactive oxidizing species. J. Biochem. Mol. Biol. 31:161-169.
17.	Kim, Y. M., I. Yamazaki, and L. H. Piette. 1994. The effect of hemoglobin, hematin, and iron on neutrophil inactivation in superoxide generating system. Arch. Biochem. Biophys. 309:308-314[Medline].
18.	Kuppusamy, P., and J. L. Zweier. 1989. Characterization of free radical generation by xanthine oxidase. Evidence for hydroxyl radical generation. J. Biol. Chem. 264:9880-9884[Abstract/Free Full Text].
19.	Lee, J. T., Jr., D. H. Ahrenholz, R. D. Nelson, and R. L. Simmons. 1979. Mechanisms of the adjuvant effect of hemoglobin in experimental peritonitis. V. The significance of the coordinated iron component. Surgery 86:41-48[Medline].
20.	Lioyd, R. V., and R. P. Mason. 1990. Evidence against transition metal-independent hydroxyl radical generation by xanthine oxidase. J. Biol. Chem. 265:16733-16736[Abstract/Free Full Text].
21.	O'Brien, A. D. 1982. Innate resistance of mice to Salmonella typhi infection. Infect. Immun. 38:948-952[Abstract/Free Full Text].
22.	Pruett, T. L., O. D. Rotstein, V. D. Fiegel, J. J. Sorenson, R. D. Nelson, and R. L. Simmons. 1984. Mechanism of the adjuvant effect of hemoglobin in experimental peritonitis. VIII. A leukotoxin is produced by Escherichia coli metabolism in hemoglobin. Surgery 96:375-383[Medline].
23.	Puppo, A., and B. Halliwell. 1988. Formation of hydroxyl radicals from hydrogen peroxide in the presence of iron. Is haemoglobin a biological Fenton reagent? Biochem. J. 249:185-190[Medline].
24.	Rush, J. D., and W. H. Koppenol. 1986. Oxidizing intermediates in the reaction of ferrous EDTA with hydrogen peroxide. Reactions with organic molecules and ferrocytochrome c. J. Biol. Chem. 261:6730-6733[Abstract/Free Full Text].
25.	Sadrzadeh, S. M. H., E. Graf, S. S. Panter, P. E. Hallaway, and J. W. Eaton. 1984. Hemoglobin. A biologic Fenton reagent. J. Biol. Chem. 259:14354-14356[Abstract/Free Full Text].
26.	Sadrzadeh, S. M. H., and J. W. Eaton. 1988. Hemoglobin-mediated oxidant damage to the central nervous system requires endogenous ascorbate. J. Clin. Investig. 82:1510-1515.
27.	Sane, A., S. Manzi, J. Perfect, A. J. Herzberg, and J. O. Moore. 1989. Desferoxamine treatment as a risk factor for zygomycete infection. J. Infect. Dis. 159:151-152[Medline].
28.	van-Bebber, I. P., W. K. Boekholz, R. J. Goris, P. H. Schillings, H. P. Dinges, S. Bahrami, H. Redl, and G. Schlag. 1989. Neutrophil fuction and lipid peroxidation in a rat model of multiple organ failure. J. Surg. Res. 47:471-475[Medline].
29.	Weiss, S. J., and A. F. LoBuglio. 1982. Biology of disease. Phagocyte-generated oxygen metabolites and cellular injury. Lab. Investig. 47:5-18[Medline].
30.	Winterbourn, C. C. 1985. Reaction with superoxide with hemoglobin, p. 137-141. In R. A. Greenwald (ed.), CRC handbook of methods for oxygen radical research. CRC Press Inc., Boca Raton, Fla
31.	Yamazaki, I., and L. H. Piette. 1990. ESR spin-trapping studies on the reaction of Fe²⁺ ions with H₂O₂-reactive species in oxygen toxicity in biology. J. Biol. Chem. 265:13589-13594[Abstract/Free Full Text].