Pyruvate Released by Astrocytes Protects Neurons from Copper-Catalyzed Cysteine Neurotoxicity

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The Journal of Neuroscience, May 15, 2001, 21(10):3322-3331

Pyruvate Released by Astrocytes Protects Neurons from Copper-Catalyzed Cysteine Neurotoxicity
Xue Feng Wang and Max S. Cynader
Brain Research Centre and Department of Ophthalmology, University of British Columbia and Vancouver Hospital & Health Sciences Centre, Vancouver, British Columbia, Canada V5Z 3N9

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have found previously that astrocytes can provide cysteine to neurons. However, cysteine has been reported to be neurotoxicalthough it plays a pivotal role in regulating intracellular levelsof glutathione, the major cellular antioxidant. Here, we showthat cysteine toxicity is a result of hydroxyl radicals generatedduring cysteine autoxidation. Transition metal ions are candidatesto catalyze this process. Copper substantially accelerates theautoxidation rate of cysteine even at submicromolar levels, whereasiron and other transition metal ions, including manganese, chromium,and zinc, are less efficient. The autoxidation rate of cysteinein rat CSF is equal to that observed in the presence of ~0.2 µMcopper. In tissue culture tests, we found that cysteine toxicitydepends highly on its autoxidation rate and on the total amountof cysteine being oxidized, suggesting that the toxicity can beattributed to the free radicals produced from cysteine autoxidation,but not to cysteineitself.
We have also explored the in vivo mechanisms that protect against cysteine toxicity. Catalase and pyruvate were each foundto inhibit the production of hydroxyl radicals generated by cysteineautoxidation. In tissue culture, they both protected primary neuronsagainst cysteine toxicity catalyzed by copper. This protectionis attributed to their ability to react with hydrogen peroxide,preventing the formation of hydroxyl radicals. Pyruvate, but notcatalase or glutathione peroxidase, was detected in astrocyte-conditionedmedium and CSF. Our data therefore suggest that astrocytes canprevent cysteine toxicity by releasingpyruvate.

Key words: glia; glutathione; toxicity; oxidative stress; transition metal; autoxidation; conditioned medium

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutathione is the major cellular antioxidant and thiol compound, and it plays a central role in cellular antioxidative defense.It is synthesized from glutamate, cysteine, and glycine. Cysteineis the rate-limiting precursor of glutathione synthesis (Beutler,1989). Neurons prefer to take up cysteine, rather than cystine,to synthesize glutathione (Kranich et al., 1996). Our recent datahave shown that astrocytes can provide cysteine to neurons indirectlyby releasing glutathione, and that cysteine is maintained at astable level in CSF and astrocyte-conditioned medium (ACM) (Wangand Cynader, 2000). However, cytotoxic effects of cysteine havealso been noted, particularly in neurons. Extensive degenerativechanges in the CNS are induced after subcutaneous injection ofcysteine in newborn mice (Olney et al., 1972) and rats (Karlsenet al., 1981). Cysteine is also toxic to cultured neurons (Puka-Sundvallet al., 1995), hepatocytes (Saez et al., 1982), and kidney celllines (Nath and Salahudeen, 1993). The underlying mechanisms ofcysteine toxicity have been studied, and there are several theories.(1) Olney et al. (1990) found that NMDA antagonists can preventcysteine toxicity and that cysteine is a bicarbonate-sensitiveexcitotoxin. They suggest a direct toxicity of cysteine. (2) Someresearchers reported that glutathione potentiates glutamate toxicityby modulating the redox site of the NMDA receptor-channel complex(Sucher and Lipton, 1991; Janaky et al., 1993; Regan and Guo,1999). Like glutathione, cysteine can also regulate redox statusby participating in the thiol/disulfide exchange reaction, thusexerting an indirect toxic effect. (3) Cysteine autoxidation cangenerate free radicals, which are cytotoxic (Saez et al., 1982;Nath and Salahudeen, 1993). This last mechanism has not been studiedin neurons. Because neurons are vulnerable to oxidative stress,attributable to the high oxygen consumption of the brain, theirhigh proportion of membrane polyunsaturated fatty acids, and theweak activities of their antioxidative enzymes (Makar et al.,1994), free radicals may play an important role in cysteine neurotoxicityin brain. In the experiments reported here, we explore the freeradical mechanisms of cysteine toxicity. We investigate the influenceof cysteine autoxidation, the generation of free radicals fromcysteine autoxidation, and its neurotoxicity to culturedneurons.

Another aim of our experiments is to identify possible protective mechanisms against cysteine toxicity. The data to be reportedindicate that cysteine in the extracellular fluid of the CNS willconstantly generate reactive oxygen intermediates via an autoxidationprocess. The organism must have developed certain mechanisms toremove the free radicals produced. In this paper, we have exploredthe possible protective effects of catalase and pyruvate on cysteinetoxicity. Pyruvate, as well as other $alpha$ -ketoacids, can react withhydrogen peroxide (H₂O₂) nonenzymatically, being converted tocarbon dioxide and the carboxylic acid with one less carbon: R-COCOOH+ H₂O₂ $right-arrow$ R-COOH + H₂O + CO₂ (Holleman, 1904; Bunton, 1949). RemovingH₂O₂ will prevent the formation of the hydroxyl radical (·OH),which is the major damaging radical. The protective effects ofpyruvate against oxidative stress in biological systems have beenreported (O'Donnell-Tormey et al., 1987; Desagher et al., 1997;Giandomenico et al., 1997). The enzymatic activities of glutathioneperoxidase (GPx), catalase, and pyruvate were examined in ACMand theCSF.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. Long-Evans pregnant rats were obtained from Charles River (Laval, Quebec, Canada). Coumarin-3-carboxylic acid (CCA)was obtained from Aldrich (Milwaukee, WI). 7-Hydroxycoumarin-3-carboxylicacid (7-OHCCA) was obtained from Molecular Probes (Eugene, OR).Fetal bovine serum (FBS), trypsin, and 10 mM Dulbecco's PBS wereobtained from Life Technologies (Grand Island, NY), and DNaseI was obtained from Boehringer Mannheim (Mannheim, Germany). Cysteine,glutathione, sodium pyruvate, sodium lactate, cupric sulfate,cuprous chloride, ferric chloride, ferrous sulfate, manganesesulfate, chromium chloride, zinc chloride, hemin, 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazoliumbromide (MTT), iodoacetic acid, 1-fluoro-2,4-dinitrobenzene (FDNB),5,5'-dithiobis(2-nitrobenzoic acid) (DTNB), isopropanol, dithiothreitol,2-mercaptoethanol, tert-butyl hydroperoxide (t-BuOOH), H₂O₂, catalase,glutathione peroxidase, glutathione reductase, lactic dehydrogenase(LDH), $beta$ -nicotinamide adenine dinucleotide reduced form ( $beta$ -NADH), $beta$ -nicotinamide adenine dinucleotide phosphate reduced form ( $beta$ -NADPH),Earle's balanced salt solution (EBSS), Eagle's MEM, cystine-freeEagle's MEM (M-2289), phenol red-free Eagle's MEM (M-4144), insulin,transferrin, selenium, and poly-L-lysine were obtained from Sigma(St. Louis, MO). The Angiocath catheter was obtained from BectonDickinson (Sandy, UT). Centricon-3 was obtained from Amicon (Beverly,MA). HPLC was performed using the 712 Gilson gradient system fromGilson Medical Electronics (Middleton, WI). The 3-amino propylion-exchange column, with a particle size of 5 µm and dimensionsof 4.6 × 200 mm, was obtained from CEL Associates (Houston, TX).Fluorescent measurement was accomplished using the luminescencespectrometer model LS 50B from Perkin-Elmer (Buckinghamshire,UK).

Primary cultures of cortical neurons and astrocytes. Primary cultures of cortical neurons were prepared in serum-free medium.Cerebral cortices of 18-d-old rat embryos were taken, and meningeswere removed. The tissue was dissected and enzymatically digestedwith 0.25% trypsin and 0.1 mg/ml DNase. The dissociated cellswere suspended in the serum-free medium and plated onto glasscoverslips (28 mm in diameter) at a density of 1 × 10⁵ cells/cm². The coverslips were coated with poly-L-lysine and dried. Beforethe dissociated cells were plated, the coverslips were brieflycoated with 10% FBS-supplemented MEM for 5 min and rinsed twicewith Hank's solution. The latter procedure helps cell attachmentin serum-free medium (Wang and Cynader, 1999). The culture mediumwas serum-free Eagle's MEM, supplemented with glucose (33 mM),glutamine (2 mM), NaHCO₃ (26 mM), and a mixture of insulin (10mg/l), transferrin (5.5 mg/l), and sodium selenite (5 µg/l). Cellswere cultured at 37°C in a humidified atmosphere of 5% CO₂ and95% air. After 24 hr in culture, the cells were used for neurotoxicityassays.

To prepare neuron-conditioned medium (NCM), the primary neurons were cocultured with a confluent astrocyte feeder layer inserum-free MEM using a noncontact method, which we have describedin detail previously (Wang and Cynader, 1999). At 7 d in vitro(DIV), the astrocyte feeder layer was removed. The serum-freemedium was added to the neuronal cultures at a concentration of1.33 ml per 1 × 10⁶ cells. The NCM was collected 24 hrlater.

Astrocyte cultures were prepared by a method modified from that described by McCarthy and de Vellis (1980). Cerebral corticesof 2-d-old newborn rats were used. The tissue was enzymaticallydigested as described above. The dissociated cells were platedin poly-L-lysine-precoated 75 cm² plastic flasks at a high density of 2 × 10⁵ cells/cm². The culture medium was Eagle's MEM, supplemented with glucose(33 mM), glutamine (2 mM), NaHCO₃ (26 mM), and 10% FBS. The mediumwas changed twice a week. The cultures were grown to confluencein 2 weeks. At 14 DIV, the flasks were tightly sealed and shakenat 260 rpm for 18 hr. Suspended cells in the flasks were discardedafter shaking, and the adherent cells were flat, polygonal astrocytes,which were identified by morphology and glial fibrillary acidicprotein immunostaining. The density of confluent astrocytes was~1 × 10⁵ cells/cm². Astrocyte-enriched cultures that were 2- to 6-week-old in flaskswere used to makeACM.

To prepare ACM, serum-free MEM was added to the confluent astrocyte cultures at a concentration of 1.33 ml per 1 × 10⁶ cells (10 ml per flask). The ACM was collected 24 hrlater.

MTT colorimetric assay of neuronal viability. Neuronal survival was determined by the MTT method, modified from Denizot andLang (1986). The tetrazolium salt MTT is reduced into a blue formazanby the mitochondrial enzyme succinate-dehydrogenase (Slater etal., 1963), and the amount of formazan produced is proportionalto the number of living cells. The cultured neurons were incubatedwith 0.5 mg/ml of MTT in phenol red-free MEM. After a 3 hr incubationat 37°C in a humidified atmosphere of 5% CO₂, the medium was removed,and 1 ml of propanol was added to each dish to solubilize theformazan. The optical density was measured at 560 nm with 690nm as a reference (OD_560-690). The cell viability was normalizedas a percentage ofcontrol.

HPLC analysis of cysteine, cystine, and related compounds. The HPLC analysis of cysteine, cystine, and related compounds,including glutathione and cysteine-glutathione disulfide, hasbeen described in detail elsewhere (Wang and Cynader, 2000), withmodifications from Reed et al. (1980). Briefly, a 100 µl samplewas first reacted with 12.5 µl of 100 mM iodoacetic acid in 0.2mM m-cresol purple and 12.5 µl of NaHCO₃ (0.24 M)/NaOH (0.12 M)buffer for 30 min. Then, 112.5 µl of 1% (v/v) FDNB in ethanolwas added, and the mixture was stored at 4°C overnight. Finally,12.5 µl of 1 M lysine was added to eliminate the unreacted FDNB,and the sample was then ready for analysis. HPLC solvent A was80% methanol in water. Solvent B was 0.8 M sodium acetate in 64%methanol. A 100 µl sample was injected into the HPLC column. Themobile phase was maintained at 80% A/20% B for 5 min, followedby a gradient elution to 1% A/99% B over 10 min, and held for5 min. The flow rate was 1.5 ml/min. The concentrations of cysteineand related compounds in the samples were calculated from thepeak areas. The minimal detectable concentrations in this experimentwere 0.1 µM for thiols and 0.05 µM fordisulfides.

Spectrophotometric assay of cysteine with Ellman's reagent (DTNB). This is an alternative method for quantitating cysteine.It is based on the thiol/disulfide reaction of thiol and DTNB,a disulfide, liberating the chromophore 5-mercapto-2-nitrobenzoicacid (Ellman, 1959; Hu, 1994). The advantage of this reagent isthat its reaction with thiols is faster (in seconds) than iodoaceticacid (in minutes), which is used in our HPLC analysis. Althoughit cannot detect multiple components of thiols and disulfides,it is suitable for simple systems, such as the study of cysteineautoxidation in pure solutions. DTNB stock solution (10 mM) wasprepared in methanol. Hemin stock solution (10 mM) was preparedin 50 mM NaOH. The stock solutions of other transition metal ions(100 µM to 10 mM), including FeSO₄, FeCl₃, CuCl, CuSO₄, MnSO₄,CrCl₃, and ZnCl₂, were prepared in dH₂O. These stock solutionswere freshly prepared. The reaction mixture included transitionmetal ions and cysteine in PBS. After the reaction, 0.1 ml ofDTNB was added to 0.9 ml of the reaction mixture. It was measuredagainst a reference of 1 mM of DTNB in PBS. An additional blankcontrol containing all components except cysteine was evaluatedto correct the absorption of transition metal ions. Cysteine concentrationswere measured from absorbance at 412 nm and calculated on thebasis of cysteinestandards.

Procedures for obtaining CSF. CSF was obtained from the rat cerebellomedullary cistern. Three-month-old male Long-Evans ratswere anesthetized with a mixture of ketamine (80 mg/kg) and xylazine(5 mg/kg). The rat was placed in a stereotaxic frame. The skinwas incised along the midline over the occipital crest, and themuscles were separated. A puncture through occipital foramen magnumwas made with an Angiocath catheter. Approximately 100 µl of CSFwas slowly drawn over 2 min. The CSF was centrifuged at 300 ×g for 2 min to remove the tiny amount of contaminating blood cells.To examine the cysteine autoxidation rate in CSF, 10 µl of 1 mMcysteine solution was added to 90 µl of CSF, to reach a finalconcentration of 100 µM. The original cysteine concentration inthe CSF (~1.12 µM) (Wang and Cynader, 2000) can be ignored. TheCSF was incubated at 37°C in a humidified atmosphere of 5% CO₂.

Fluorimetric assay of hydroxyl radicals. Production of ·OH was estimated by using CCA. Nonfluorescent CCA was converted by·OH to highly fluorescent 7-OHCCA (Collins et al., 1994). Formeasuring ·OH produced during autoxidation of 100 µM cysteinein the presence of 0.2 µM Cu²⁺, the reaction mixture was prepared as follows in sequence: 0.885ml of PBS, 0.1 ml of 10 mM CCA (final concentration: 1 mM), 10µl of 10 mM cysteine, and 5 µl of 40 µM Cu²⁺. The solution was left at 37°C and 100% air to finish the reactioncompletely. After 4 hr incubation, the samples were measured usinga fluorescence spectrometer, with excitation wavelength of 400nm and emission of 450 nm. CCA (1 mM) in PBS was used as the reference.A standard curve was calculated by measuring the fluorescenceintensities of a series of concentrations of 7-OHCCA. The produced·OH from cysteine autoxidation was represented by the corresponding7-OHCCAconcentrations.

Pyruvate assay. Pyruvate in ACM, NCM, and the CSF was measured using an enzymatic method described by Von Korff (1969). LDHcatalyzes the conversion of pyruvate to lactate with NADH: pyruvate+ NADH $left-right-arrows$ lactate + NAD⁺. The reaction mixture was prepared as follows: 198 µl of PBS,100 µl of 1 mM NADH, 100 µl of the sample, and 2 µl of 0.4 U/µlLDH. The decrease of NADH was monitored at 340 nm with a spectrophotometerfor 300 sec until a constant value was obtained. Pyruvate concentrationwas calculated from the oxidized NADH ( $epsilon$ _NADH = 6290 M¹ cm¹ at 340nm).

Determination of enzyme activities. GPx activity was determined using a method modified from Takahashi et al. (1987). GPxactivity was assessed from the oxidation of NADPH in the presenceof glutathione reductase and oxidized glutathione formed by GPx.The reaction mixture included Tris-HCl (0.1 M, pH 8.0), NADPH(0.2 mM), EDTA (0.5 mM), glutathione (2 mM), glutathione reductase(1 U/ml), sample (100 µl), and t-BuOOH (100 µM). The total volumewas 1 ml, and t-BuOOH was added last. The oxidation of NADPH wasmonitored against a reference mixture without sample and t-BuOOH.A negative control containing all components except the samplewas used to correct the oxidation of glutathione and NADPH byt-BuOOH. The samples were adult rat CSF and ACM. The latter was10× concentrated ACM prepared by filtering ACM in a centriconwith a 3 kDa molecular weight cutoff. Calculation of GPx activitywas based on the consumption of NADPH at A₃₄₀ ( $epsilon$ _NADPH = 6220 M¹ cm¹ at 340nm).

Catalase activity was measured by monitoring the absorbance change of H₂O₂ (Duffy et al., 1998). The reaction mixture includedPBS, EDTA (0.5 mM), H₂O₂ (10 mM), and 100 µl of sample. The totalvolume was 1 ml. The reference contained all components exceptthe sample. The samples were adult rat CSF and the concentratedACM, as above. Absorbance was monitored at 240 nm from 300 to600 sec. The minimal detectable enzyme activity of this test was5 mU/ml. One unit of enzyme activity was defined as the amountof the enzyme that decomposes 1 µmol of H₂O₂ perminute.

The data were analyzed by using ANOVA. The post hoc tests to determine significant differences between means of individualgroups were followed whennecessary.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cysteine autoxidation in the presence of transition metal ions and in CSF

To study the factors determining cysteine autoxidation, we first investigated the autoxidation rate of cysteine in the followingthree solutions: EBSS, cystine-free MEM (MEM-CSSC), and MEM-CSSC with cultured neurons. EBSS contains the basal salts of MEM.The medium of the primary cortical neurons was replaced by MEM-CSSC before testing. Only a small amount of cell debris was presentin the cell cultures. All of these solutions were incubated at37°C and pH 7.4 in a humidified atmosphere of 5% CO₂. Cysteinewas added to a final concentration of 100 µM. Cysteine and cystinewere measured by HPLC at 0, 5, 15, 30, 60, and 120 min after cysteinewas added to the three solutions. The results showed that cysteinewas gradually oxidized to cystine. Only a small proportion ofcysteine (~1-2%) was oxidized to cysteic acid (data not shown).Cysteine concentrations in MEM-CSSC and neuronal culture medium did not differ significantly fromthe corresponding values in EBSS (p > 0.05) (Fig. 1A). This resultdemonstrates that the components of culture medium and culturedcells have no obvious influence on cysteine autoxidation.

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Figure 1. The factors influencing cysteine (CSH) autoxidation. The reaction conditions to assess cysteine autoxidation were 37°C and pH 7.4 in a humidified atmosphere of 5% CO₂ and 95% air. The samples were taken at different time points for HPLC assays. A, Cysteine (100 µM) autoxidation in Earle's balanced salt solution (EBSS), cystine-free MEM (MEM-CSSC), and neuronal culture medium. The latter was made from MEM-CSSC, which replaced the original cystine-containing MEM in the neuronal cultures before testing. Cysteine was gradually oxidized to cystine. Cysteine concentrations in MEM-CSSC and culture medium were not significantly different from the corresponding values in EBSS (p > 0.05). B, The effects of iron on cysteine autoxidation. Ferric chloride (FeCl₃), at concentrations of 0.1, 1, and 10 µM, was incubated with 100 µM cysteine in EBSS. Cysteine concentrations in the three Fe³⁺ solutions were not significantly different from the corresponding values in EBSS (p > 0.05). C, The effects of copper on cysteine autoxidation. Cupric sulfate (CuSO₄), at concentrations of 0.1, 1, and 10 µM, was incubated with 100 µM cysteine in EBSS. Cysteine autoxidation was substantially accelerated in the presence of Cu²⁺ at all three concentrations. Results are normalized as the percentage of 100 µM total cysteine. Each column represents the average of three independent experiments performed in duplicate (mean ± SEM). *p < 0.01 versus corresponding values of cysteine autoxidation in EBSS.

Transition metal ions, such as Fe³⁺ and Cu²⁺, are believed to catalyze the oxidation of reducing agents, including thiol-containingcompounds (Halliwell and Gutteridge, 1985). The effects of Fe³⁺ and Cu²⁺ on cysteine autoxidation were measured under the same conditionsas described above. Fe³⁺, at concentrations of 0.1, 1.0, and 10 µM, had no obvious effectson the autoxidation rate of cysteine, as assessed by comparingcysteine concentrations with the corresponding value in EBSS (p> 0.05) (Fig. 1B). There were also no obvious differences amongthe three different concentrations (p > 0.05). Our results showedthat Cu²⁺ substantially accelerated the autoxidation rate of cysteine atconcentrations between 0.1 and 10 µM (Fig. 1C). The efficacy ofsubmicromolar levels of Cu²⁺ in catalyzing cysteine autoxidation has significant physiologicalmeaning because these are well within the physiological range.The concentrations of loosely bound copper in human CSF have beenreported to be in the range of 0.13-0.75 µM (Gutteridge, 1984).

We compared the effects of variable oxidation valences of iron (Fe²⁺ and Fe³⁺) and copper (Cu⁺ and Cu²⁺) on cysteine autoxidation. The effects of hemin, the low molecularweight complex of Fe³⁺, and some other biologically important transition metal ions,including Mn²⁺, Cr³⁺, and Zn²⁺, on cysteine autoxidation were also studied. As shown in Figure2, cysteine autoxidation with Fe²⁺ was faster than that with Fe³⁺ at concentrations of 100 and 200 µM but was not significantlydifferent at concentrations of 1 and 10 µM. The effects of Cu⁺ and Cu²⁺ on cysteine autoxidation were not significantly different atconcentrations of 0.01-1 µM. Hemin was more efficient in catalyzingcysteine autoxidation than Fe²⁺ and Fe³⁺, but still much less efficient than Cu⁺ and Cu²⁺. The concentration for hemin to catalyze the half oxidation of100 µM cysteine in 60 min was ~10 µM, whereas the concentrationfor Cu⁺ and Cu²⁺ was between 0.1 and 0.2 µM, a ~50- to 100-fold difference. Mn²⁺ was efficient at concentrations of 100 and 200 µM. No catalyzingeffects of Cr³⁺ and Zn²⁺ were observed at concentrations between 1 and 200 µM.

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Figure 2. Comparisons of cysteine autoxidation in the presence of several transition metal ions. A series of concentrations of FeSO₄, FeCl₃, hemin, MnSO₄, CrCl₃, ZnCl₂, CuCl, and CuSO₄ were reacted with 100 µM cysteine, respectively. The control was 100 µM cysteine without transition metal ions. The reaction mixtures were incubated in PBS at pH 7.4 and 37°C in a humidified 100% air. Cysteine concentrations were determined with Ellman's reagent after 60 min. A, Cysteine autoxidation with Fe²⁺, Fe³⁺ (1-200 µM), and hemin (1-100 µM). B, Cysteine autoxidation with Mn²⁺, Cr³⁺, and Zn²⁺ (1-200 µM). C, Cysteine autoxidation with Cu⁺ and Cu²⁺ (0.01-1 µM). Data are the mean ± SEM of three independent experiments in duplicate. *p < 0.01, significantly different from the control. ^a,
bp < 0.01 versus corresponding values of Fe³⁺ groups.

Cysteine autoxidation in CSF was examined. As described in the Materials and Methods, cysteine was added to rat CSF to a concentrationof 100 µM. The samples were taken for test at 15, 30, 60, and120 min after this addition. The results showed that cysteinewas oxidized at a moderate rate in the CSF (Fig. 3A). Most ofthe cysteine was converted to cystine (~80%). The other smallportion of cysteine participated in the thiol/disulfide exchangereaction and formed mixed disulfides, such as cysteine-glutathionedisulfide and cysteine-protein disulfides. We compared cysteineautoxidation in CSF and in Cu²⁺-supplemented solutions (Fig. 3B). The autoxidation rate of cysteinein CSF was roughly equal to that observed in solutions of 0.2-0.3µM Cu²⁺. In Discussion, we propose that copper is likely the major catalystin CSF for cysteine autoxidation. We chose 0.2 µM Cu²⁺ to mimic the cysteine autoxidation in CSF in the following toxicityexperiments.

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Figure 3. Cysteine autoxidation rates in CSF and comparisons with those in Cu²⁺-supplemented solutions. CSF was taken from 3-month-old rats as described in Materials and Methods. Cysteine was added to the CSF with a final concentration of 100 µM. The CSF was incubated under conditions of pH 7.4 and 37°C in a humidified atmosphere of 5% CO₂ and 95% air. Samples were taken at several time points for HPLC assays. A, Time course of the concentrations of cysteine and related compounds in the CSF during cysteine autoxidation. B, Comparison of cysteine autoxidation in CSF and in Cu²⁺-supplemented solutions. Cu²⁺ was prepared in EBSS at concentrations of 0.1, 0.2, and 0.3 µM and incubated under the same conditions as the CSF. Data are the mean ± SEM of three independent experiments in duplicate. CSSC, Cystine; CSSG, cysteine-glutathione disulfide; GSH, glutathione.

Neurotoxic effects of cysteine

Cysteine neurotoxicity was investigated in our cell culture system. We observed the effects of the autoxidation rate of cysteineand the amount of cysteine being oxidized, as well as the effectsof cysteine concentrations, on cysteine neurotoxicity. In Figure4, primary neurons were cultured in the presence of a series ofconcentrations of cysteine (0, 10, 20, 50, 100, 200, 500, 1000,and 2000 µM) and in the absence or presence of copper (0, 0.2,and 1.0 µM) in 2 ml culture medium (MEM). Neurotoxicity was estimated24 hr later by the MTT assay. The role of copper in this experimentwas to modulate the autoxidation rate of cysteine. Without additionof cysteine, copper itself had no visible effect on neuronal survival.The neuronal survivals in the presence of copper and absence ofcysteine were 99.6 ± 11.3% (mean ± SEM; Cu²⁺ = 0.2 µM) and 105 ± 5% (Cu²⁺ = 1.0 µM); there were no significant differences from the control100 ± 1.5% (Cu²⁺ = 0) (p > 0.05). Without Cu²⁺, cysteine was toxic only at relatively high concentrations (EC₅₀~600 µM). With the addition of Cu²⁺, the toxic concentrations of cysteine decreased (EC₅₀ ~30 µMat 0.2 µM Cu²⁺ and EC₅₀ ~12 µM at 1.0 µM Cu²⁺). This result demonstrates that cysteine toxicity is closelyrelated to its autoxidation rate.

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Figure 4. Neurotoxic effects of cysteine in the presence of copper. Primary cortical neurons were cultured in serum-free MEM. Cysteine was added at concentrations as indicated in the presence of 0, 0.2, and 1.0 µM Cu²⁺. Neuronal viability was estimated 24 hr later using the MTT assay. Results are expressed as the percentage of surviving neurons compared with control cultures (without the addition of cysteine and Cu²⁺). Data represent the mean ± SEM of three independent experiments in triplicate.

The effect on its toxicity of the total amounts of cysteine being oxidized was investigated further. Cu²⁺ (0.2 µM) was added for the purpose of catalyzing cysteine autoxidation.Cysteine (10 µM) was added to the culture medium either 1, 5,or 10 times at a rate of once every 5 min, respectively. Cysteine(10 µM) was completely oxidized in 5 min (Fig. 5). Although asingle dose of cysteine showed no obvious toxicity (91 ± 5.1%of viability), multiple additions of cysteine substantially increasedcysteine toxicity. Neuronal survival was 91.5 ± 5.1% (mean ± SEM;p > 0.05 vs control) with the addition of 10 µM cysteine one timeand decreased to 28.9 ± 4.4% (p < 0.01 vs control) with five additionsof 10 µM cysteine and to 12.6 ± 1.5% (p < 0.01 vs control) with10 applications. Note that the repeated addition increased thetotal amounts of cysteine being oxidized, whereas the maximalconcentration of cysteine never exceeded 10 µM at any one time.These results demonstrate that cysteine toxicity is closely relatedto the total amount of cysteine being oxidized.

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Figure 5. Effect of total amount of cysteine being oxidized on neuronal survival. Primary cortical neurons were cultured in serum-free MEM. The concentration of Cu²⁺ was 0.2 µM. Cysteine (10 µM) was added each time and once or repetitively every 5 min for a total of 5 and 10 times. Cysteine (10 µM) was completely oxidized within 5 min in the presence of 0.2 µM Cu²⁺ (inset, top right). Neuronal viability was estimated 24 hr later using the MTT assay. Results are expressed as the percentage of surviving neurons compared with control cultures (without addition of cysteine). Data represent the mean ± SEM of three independent experiments in triplicate. *p < 0.01, significantly different from the control.

Taken together, these data suggest that cysteine autoxidation, rather than cysteine itself, is responsible for cysteine toxicity.Using CCA as a probe, we measured the production of ·OH generatedfrom cysteine autoxidation. The hydroxyl radical reacts with CCAto generate 7-OHCCA. Cysteine in PBS was incubated at 37°C andpH 7.4 for 4 hr. As shown in Figure 6A, little ·OH was producedfrom cysteine autoxidation without the presence of Cu²⁺. In the presence of 0.2 µM Cu²⁺, hydroxyl radicals were generated in substantial amounts duringcysteine autoxidation, and the amount of ·OH increased with cysteineconcentration. We also compared the generation of ·OH with someother thiols. Glutathione, N-acetyl-cysteine, homocysteine, dithiothreitol,and 2-mercaptoethanol can all generate ·OH with Cu²⁺ as a catalyst to variable degrees (Fig. 6B). Disulfides (cystineand glutathione disulfide) and sulfur-containing amino acid (cysteicacid) did not generate ·OH.

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Figure 6. Generation of hydroxyl radical (·OH) by the autoxidation of cysteine and other thiols. Cysteine and related compounds were incubated in PBS under the conditions of pH 7.4 and 37°C in a humidified atmosphere of 100% air. CCA (1 mM) was added to react with the generated ·OH, producing 7-OHCCA. Fluorescence was measured 4 hr after the reaction began. A, Cysteine, at concentrations of 0-200 µM, was incubated in the presence or absence of 0.2 µM Cu²⁺. B, Generation of ·OH from the autoxidation of thiols. Thiols, disulfides, and sulfur-containing amino acid (100 µM of each) were incubated with 0.2 µM Cu²⁺. The thiols include cysteine (CSH), glutathione (GSH), N-acetyl-cysteine (NAC), homocysteine (HSH), dithiothreitol (DTT), and 2-mercaptoethanol (2-ME). The disulfides include cystine (CSSC) and glutathione disulfide (GSSG). The sulfur-containing amino acid is cysteic acid (CA). Data represent the mean ± SEM of three independent experiments in duplicate.

The effects of catalase and pyruvate on the cysteine toxicity and the generation of hydroxyl radicals

When cysteine is oxidized, O₂ accepts electrons one by one, and reactive oxygen intermediates are produced. The hydroxyl radicalis the major reactive oxygen species to cause tissue damage andis generated from H₂O₂. Therefore it is reasonable to expect thatcatalase, which decomposes H₂O₂, could prevent ·OH generationfrom cysteine autoxidation and thus reduce cysteine toxicity.Likewise, pyruvate would also be expected to have the same effectbecause of its reactivity with H₂O₂. The effects of catalase andpyruvate on cysteine neurotoxicity were tested in our primaryneuronal cultures. In the presence of Cu²⁺ (0.2 µM), cysteine (100 µM) was toxic to neurons (16.8 ± 2.8%of viability) (Fig. 7A). Addition of catalase (10 U/ml) or pyruvate(1 mM) completely prevented cysteine toxicity, with 101 ± 4 and104 ± 5% of viability, respectively. Pyruvate and lactate areboth glucose metabolites and important energy suppliers to neurons(Selak et al., 1985; Pellerin and Magistretti, 1994; Tsacopoulosand Magistretti, 1996). To demonstrate that the preventive effectof pyruvate against cysteine toxicity is caused by its specificreactivity with H₂O₂, other than its energy supplying effect,sodium lactate was used as control. The results showed that lactatecould not prevent cysteine neurotoxicity (Fig. 7A). The protectivecapacity of pyruvate was dose dependent. In the presence of 0.2µM Cu²⁺ and 50 or 100 µM cysteine, increasing concentrations of pyruvate(up to 1 mM) produced a progressive enhancement of neuronal protection(Fig. 7B).

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Figure 7. The protective effects of catalase and pyruvate on cysteine neurotoxicity. Primary cortical neurons were cultured in serum-free MEM. Cysteine toxicity was induced by addition of 100 µM cysteine and 0.2 µM Cu²⁺. Neuronal viability was estimated 24 hr later using the MTT assay. Results are expressed as the percentage of surviving neurons compared with control cultures (without addition of cysteine). A, Catalase (10 U/ml), pyruvate (1 mM), and lactate (1 mM) were added immediately before addition of cysteine and Cu²⁺. Data represent the mean ± SEM of three independent experiments in triplicate. B, Dose-response curve illustrating the neuroprotective effect of pyruvate. Cysteine concentrations were 0, 50, and 100 µM, respectively. Data represent the mean ± SEM of three independent experiments in duplicate. *p < 0.01, significantly different from the control.

Because of their ability to remove H₂O₂, catalase and pyruvate are expected to prevent the formation of ·OH generated fromcysteine autoxidation. In the presence of 0.2 µM Cu²⁺ and 100 µM cysteine, the generation of ·OH was measured in PBSat 37°C and pH 7.4. Catalase and pyruvate substantially decreased·OH production, whereas lactate did not (Fig. 8A). Lactate evenincreased the ·OH production, and the reason for this is unknown.The inhibitory effect of pyruvate on ·OH production from cysteineautoxidation was dose dependent (Fig. 8B).

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Figure 8. Effects of catalase and pyruvate on the generation of ·OH from cysteine autoxidation. Cysteine (100 µM) and Cu²⁺ (0.2 µM) were incubated in PBS under the conditions of pH 7.4 and 37°C in a humidified atmosphere of 100% air. CCA (1 mM) was added to react with the generated ·OH, producing 7-OHCCA. The fluorescence was measured 4 hr after the reaction. Data represent the mean ± SEM of three independent experiments in duplicate. A, Catalase (10 U/ml), pyruvate (1 mM), and lactate (1 mM) were added immediately before addition of cysteine and Cu²⁺. B, Pyruvate, at concentrations of 0, 0.1, 1, and 10 mM, was added immediately before addition of cysteine and Cu²⁺. *, **p < 0.01, significantly different from the control (cysteine only).

Pyruvate released by astrocytes

We explored two potential extracellular antioxidative mechanisms, which may prevent the toxic effects of cysteine autoxidation:(1) enzymatic mechanisms and (2) small molecule antioxidant mechanisms.For the former, we tested the activities of GPx and catalase inACM and CSF. The concentrated ACM prepared from primary confluentastrocyte cultures was used as described in Materials and Methods.CSF was taken from 3-month-old rats. The results showed that theactivities of the two enzymes were not detected in ACM and CSF.GPx activity of ACM was 1.6 ± 0.2 mU/ml (mean ± SEM, n = 6), whichwas not significantly different from the negative control (1.9± 0.4 mU/ml; n = 6; p > 0.05). GPx activity of CSF was 2.2 ± 0.2mU/ml (n = 6), which was not significantly different from thenegative control (1.7 ± 0.2 mU/ml; n = 6; p > 0.05). Catalaseactivity was not detected in ACM and CSF (<5 mU/ml, n = 6,respectively).

Because pyruvate can scavenge H₂O₂, it may act as an extracellular antioxidant in vivo. Pyruvate concentration was thereforeassayed in ACM, NCM, and CSF. Relatively high levels of pyruvatewere found in ACM (254 ± 15 µM) and in CSF (131 ± 9 µM). Pyruvatewas also detected in NCM at relatively low concentrations (45.6± 4.4 µM) (Table 1), suggesting that the pyruvate pool of theextracellular space and CSF was contributed mainly by astrocytes.The time course of pyruvate release by astrocytes was also measured(Fig. 9). In the ACM made from pyruvate-free medium, pyruvateconcentration increased rapidly within 12 hr and reached a peakat 24 hr.


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Table 1. Pyruvate contents in ACM, NCM, and CSF

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Figure 9. Time course of pyruvate release by astrocytes. Confluent astrocytes in flasks were rinsed with Hank's solution. The serum-free MEM was added at a concentration of 1.33 ml per 1 × 10⁶ cells. Samples of the ACM were taken at 0, 6, 12, 24, and 48 hr and used for pyruvate assays. Data represent the mean ± SEM of three independent experiments in triplicate.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The biological role of cysteine is double edged. It is a very important amino acid for the synthesis of glutathione, whichis the major cellular antioxidant. Neurons, in particular, preferto take up cysteine, rather than cystine, to synthesize glutathione(Kranich et al., 1996). On the other hand, cysteine has been foundto be cytotoxic. Subcutaneous injection of cysteine in newbornmice (1 mg/gm weight) (Olney et al., 1972) and rats (1.2 mg/gmweight) (Karlsen et al., 1981) caused extensive neuronal death.Cysteine was toxic to cultured hepatocytes (4 mM) (Saez et al.,1982), kidney cell lines (4 mM) (Nath and Salahudeen, 1993), andprimary neurons (1 mM) (Puka-Sundvall et al., 1995). In our neuronalcultures, 1 mM cysteine decreased neuronal survival to 30.5% (EC₅₀~600 µM) in the absence of copper (Fig. 4), similar to other findings(Puka-Sundvall et al., 1995). Importantly, our results showedthat cysteine toxicity was greatly increased in the presence ofeven submicromolar levels of copper, whereas copper itself wasnoncytotoxic without cysteine (Fig. 4). Copper appears to functionas a catalyst to accelerate cysteine autoxidation (Fig. 10).

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Figure 10. Diagram of the proposed mechanism of protection by astrocytes in preventing cysteine toxicity catalyzed by copper. Astrocytes release glutathione and indirectly produce cysteine in the extracellular fluid of the CNS. Cysteine, as well as glutathione or other thiols, will be oxidized to disulfide under the catalysis of protein-unbound or loosely bound copper. Molecular oxygen, as the oxidant, accepts electrons step by step to produce superoxide radicals, hydrogen peroxide, and hydroxyl radicals. The latter is the major damaging free radical to the cells. In parallel, astrocytes also release pyruvate, which can react with hydrogen peroxide, preventing the formation of hydroxyl radicals.

Iron is generally considered the major transition metal ion in mediating the production of free radicals. Our experimentsshow that copper is much more efficient in catalyzing cysteineautoxidation than iron and some other transition metal ions, suchas manganese, chromium, and zinc. Variable valences of copperdo not influence its catalyzing efficacy. For iron, the solublelow molecular weight Fe³⁺ complex, hemin, is more efficient in catalyzing cysteine autoxidationthan Fe²⁺ and Fe³⁺. Fe³⁺ is insoluble at neutral pH, whereas Fe²⁺ is relatively soluble. Fe²⁺, however, will be oxidized to Fe³⁺ under aerobic conditions and form deposits. Whether solubilityis the cause of these differences is unknown. Even the catalyzingefficacy of hemin is still much lower than that of copper. Ourfinding that copper is a more potent catalyst than iron is notunique. It has been reported that copper is more efficient thaniron in mediating paraquat toxicity (Chevion, 1988) and in catalyzingdialuric acid autoxidation (Munday, 1988).

Our data show that cysteine was oxidized at a moderate rate in CSF. The autoxidation rate of 100 µM cysteine in CSF is equivalentto that in the presence of ~0.2 µM Cu²⁺ (Fig. 3). According to different authors, total copper concentrationsin human CSF are in the range of 0.22-1.7 µM (14.2-109 µg/l) (Kapakiet al., 1997; Jimenez-Jimenez et al., 1998; Joergstuerenburg etal., 1999; Stuerenburg, 2000). CSF also contains some other physiologicallyimportant transition metal ions, such as iron, manganese, chromium,and zinc. Their concentrations in human CSF are 1.1-3.8 µM forFe (Jimenez-Jimenez et al., 1998; LeVine et al., 1998), 12-60nM for Mn (D'Amico and Klawans, 1976; Kapaki et al., 1997; Jimenez-Jimenezet al., 1998), 0.28 µM for Cr (Aguilar et al., 1998), and 0.16-2.6µM for Zn (Palm and Hallmans, 1982; Kapaki et al., 1997; Jimenez-Jimenezet al., 1998). The binding status of copper in CSF is of particularimportance with regard to its catalyzing effect, because onlyprotein-unbound or loosely bound copper, which can form a lowmolecular weight complex with cysteine, can catalyze cysteineautoxidation (Halliwell and Gutteridge, 1985). The concentrationof loosely bound copper detected in human CSF ranges from 0.13to 0.75 µM (Gutteridge, 1984). By comparing the efficient catalyzingconcentrations of these transition metal ions and their physiologicalranges, we suggest that copper is the major determinant influencingthe cysteine autoxidation rate inCSF.

The mechanism of copper-catalyzed cysteine autoxidation has been investigated extensively (Cavallini et al., 1969; Munday,1989; Kachur et al., 1999). It has been suggested that the intermediatecysteine-Cu complex is initially formed in a 2:1 ratio. Cysteine,as well as other low molecular weight thiol compounds, can donateelectrons via catalysts. O₂ generally acts as an oxidant, acceptingelectrons one by one to generate reactive oxygen species: ·O,H₂O₂, and ·OH. In CSF, cysteine (1.12 ± 0.14 µM) and glutathione(5.87 ± 0.29 µM) are the major low molecular weight thiols (Wangand Cynader, 2000). The constant autoxidation of these thiolswill place neurons in a situation of oxidative stress if no mechanismsexist to remove the generated oxygen radicals. The hydroxyl radical,which has an extremely short half-life of 10⁹ sec (Pryor, 1986), is the major damaging radical. Once ·OH isproduced, it rapidly attacks polyunsaturated fatty acids to initiatethe chain reaction of lipid peroxidation, as well as DNA, proteins,and carbohydrates. H₂O₂ itself is stable and nontoxic and is theone-step precursor of ·OH. Eliminating H₂O₂ can therefore blockthe formation of ·OH. Although cytoplasmic enzymes, such as GPxand catalase, can eliminate membrane-permeable H₂O₂ intracellularly,H₂O₂ permeating the cell membrane itself is risky for cells. Inaddition, extracellularly generated H₂O₂ will be reduced to ·OHif it is not scavenged immediately. Therefore, it will be moreefficient and beneficial if extracellularly derived H₂O₂ can beeliminated in situ in the extracellularspace.

We have explored two possible extracellular H₂O₂-eliminating mechanisms, including enzymatic mechanisms and small moleculeantioxidant mechanisms. The activities of the two most plausibleantioxidative enzymes, GPx and catalase, were not detected inACM or CSF. The trophic effect of pyruvate on neuronal survivalhas long been reported (Selak et al., 1985; Katoh-Semba et al.,1988; Izumi et al., 1994; Matsumoto et al., 1994). Recently, pyruvatewas found to protect neurons (Desagher et al., 1997) or cell lines(Giandomenico et al., 1997) from H₂O₂-induced toxicity. We showthat pyruvate, as well as catalase, can inhibit the productionof ·OH generated from cysteine autoxidation by removing H₂O₂.The neuroprotective effect of pyruvate cannot be attributed toits role in energy metabolism, because lactate, a metabolic substrate,did not prevent the cysteine neurotoxicity and ·OH productionfrom cysteineautoxidation.

The source of pyruvate in the extracellular fluid and CSF has not been studied extensively, as has lactate. The lactate poolis mainly contributed by astrocytes, and much evidence supportsan astrocyte-to-neuron lactate shuttle mechanism (Walz and Mukerji,1988; Dringen et al., 1993; Tsacopoulos and Magistretti, 1996;Schousboe et al., 1997). A specific monocarboxylate transporteris responsible for the transport of pyruvate and lactate acrossthe plasma membrane (Poole and Halestrap, 1993; Garcia et al.,1994). It is a facilitated transport, and the net flux is mainlydetermined by the concentration gradient of substrates acrossthe membrane. Our studies have examined pyruvate concentrationsin different compartments: ACM (254 ± 15 µM) > CSF (131 ± 9 µM)> NCM (45.6 ± 4.4 µM). The related data from other investigatorsare as follows: rat ACM, 320 µM (Selak et al., 1985); adult ratCSF, ~200 µM (Vannucci and Duffy, 1976); basal intracellular pyruvateconcentration of cultured striatal neurons, ~90 µM (Desagher etal., 1997). The concentration gradients among these differentcompartments suggest a net flux of pyruvate from astrocytes toextracellular pool, then to neurons. In agreement with this, otherreports show that astrocytes release pyruvate (Pellerin and Magistretti,1994) and that neurons can use pyruvate for their function recoveryor survival (Selak et al., 1985; Matsumoto et al., 1994; Yoshiokaet al., 2000). Given the evidence above, it is suggested thatthe extracellular pool of pyruvate is contributed mainly by astrocytesrather than neurons. It is still unknown whether other brain cellssuch as choroidal epithelial cells or ependymocytes contributeto the pyruvatepool.

Another possible source of pyruvate is from blood. Pyruvate can be transported through the blood-brain barrier by the monocarboxylatetransporter (Pardridge and Oldendorf, 1977; Miller and Oldendorf,1986). However, the arteriovenous difference of pyruvate acrossthe brain of adult fed rats was found to be negligible (arterialblood, 141 ± 14 µM; sinus blood, 138 ± 14 µM), whereas the arteriovenousdifference for glucose was substantial (510 ± 50 µM) (Hawkinset al., 1971). This suggests that although pyruvate is permeableacross the blood-brain barrier, the net transport from blood tobrain contributes little to the pyruvate pool of the CNS undernormal conditions. Instead, the brain uses glucose and producespyruvate on its own. Taken together, these findings lead to theset of mechanisms outlined in Figure 10 as those underlying theneurosupportive effect of astrocytes against cysteinetoxicity.

Our data clearly indicate the importance of copper in oxidative stress. Wilson's disease is an inherited disorder characterizedby hepatic cirrhosis and neuronal degeneration attributable toan impairment of copper excretion (Loudianos and Gitlin, 2000).The pathological changes in the CNS include copper deposition(10- to 15-fold over normal) in virtually all parts of brain withresulting extensive neuronal loss and gliosis in the gray matter(Scheinberg and Sternlieb, 1983). Plasma loosely bound copperand free radical production are markedly increased in Wilson'sdisease (Ogihara et al., 1995). However, the molecular mechanismof copper-induced oxidative stress and cytotoxicity is still uncertain.Our studies suggest that elevated free copper in the CNS acceleratesthe autoxidation of cysteine and other reducing agents, resultingin increased production of free radicals and subsequent cytotoxicityin Wilson's disease. Mutations of Cu/Zn superoxide dismutase havebeen identified in patients with familial amyotrophic lateralsclerosis (FALS) (Rosen et al., 1993). Further studies have foundthat oxidative stress caused by altered copper coordination isthe major pathogenic factor in this FALS model (Estevez et al.,1999; Gabbianelli et al., 1999). Copper has also been found tomediate the deposition of A $beta$ in Alzheimer's disease (Huang etal., 1999). It is predicted that copper will be found to be involvedin the pathogenesis of many neurodegenerative diseases and otheroxidative stress-relatedconditions.

  FOOTNOTES

Received Oct. 30, 2000; revised Jan. 26, 2001; accepted Feb. 27, 2001.

This work is supported by a Canadian Institutes of Health Research/Canadian Neuroscience Research Program grant to M.S.C.We thank Dr. John Philips, Joan Martin, and Ying Zhao for theuse of HPLC equipment and Virginia Booth for excellentassistance.
Correspondence should be addressed to Xue Feng Wang, 2550 Willow Street, Vancouver, British Columbia, Canada V5Z 3N9. E-mail:xuefeng{at}interchange.ubc.ca.

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