Inflammatory Neurodegeneration Mediated by Nitric Oxide from Activated Glia-Inhibiting Neuronal Respiration, Causing Glutamate Release and Excitotoxicity

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GLUTAMIC ACID HYDROCHLORIDE
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The Journal of Neuroscience, September 1, 2001, 21(17):6480-6491

Inflammatory Neurodegeneration Mediated by Nitric Oxide from Activated Glia-Inhibiting Neuronal Respiration, Causing Glutamate Release and Excitotoxicity
Anna Bal-Price and Guy C. Brown
Department of Biochemistry, University of Cambridge, Cambridge, CB2 1QW, United Kingdom

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glia undergo inflammatory activation in most CNS pathologies and are capable of killing cocultured neurons. We investigatedthe mechanisms of this inflammatory neurodegeneration using amixed culture of neurons, microglia, and astrocytes, either whenthe astrocytes were activated directly with lipopolysaccharide(LPS) and interferon- $gamma$ (IFN- $gamma$ ) or LPS/IFN- $gamma$ -activated microgliawere added to mixed neuronal cultures. In either case, activatedglia caused 75-100% necrotic cell death within 48 hr, which wascompletely prevented by inhibitors of inducible nitric oxide synthase(iNOS) (aminoguanidine or 1400W). Activated astrocytes or microgliaproduced nitric oxide (NO) (steady-state level ~0.5 µM), whichimmediately inhibited the cellular respiration of cocultured neurons,as did authentic NO. NO donors also decreased ATP levels and stimulatedlactate production by neurons, consistent with NO-induced respiratoryinhibition. NO donors or a specific respiratory inhibitor causedrapid (<1 min) release of glutamate from neuronal and neuronal-astrocyticcultures and subsequent neuronal death that was blocked by anantagonist of NMDA receptor (MK-801). MK-801 also blocked neuronaldeath induced by activated glia. High oxygen also prevented NO-inducedneuronal death, consistent with death being induced by NO inhibitionof cytochrome c oxidation in competition with oxygen. Thus activatedglia kill neurons via NO from iNOS, which inhibits neuronal respirationresulting in glutamate release and subsequent excitotoxicity.This may contribute to neuronal cell death in inflammatory, infectious,ischemic, and neurodegenerativediseases.

Key words: nitric oxide; mitochondria; astrocytes; microglia; neurons; inflammation

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Astrocytes and/or microglia become "activated" by inflammatory mediators in a wide range of CNS pathologies, including braininflammation, trauma, ischemia, and stroke; brain infections suchas AIDS dementia, meningitis, and malaria; neurodegenerative diseasessuch as Alzheimer's, Parkinson's, Huntington's, multiple sclerosis,amyotrophic lateral sclerosis; and normal aging (Eddleston andMucke, 1993; Kreutzberg, 1996). Glial activation involves changesin cell phenotype and gene expression, including the de novo expressionof major histocompatibility complex class I and II antigens, celladhesion molecules, cytokines such as tumor necrosis factor $alpha$ (TNF $alpha$ ) and interleukin-1 $beta$ (IL-1 $beta$ ), and the inducible isoform ofnitric oxide synthase(iNOS).

Glial activation is thought to be protective via destruction of pathogens, removal of debris, and promotion of tissue repair;however, excess activation can be deleterious (Banati et al.,1993; Hewett et al., 1994; Bolanos et al., 1997). Activated gliacan kill neurons in coculture (Chao, 1996; Hu et al., 1997; Kinghamet al., 1999; Tanabe et al., 1999), and this may occur in vivoduring brain trauma, inflammation, post-ischemia, and infection,and in neurodegenerative diseases (Loihl and Murphy, 1998; Bolanosand Almeida, 1999; Liberatore et al., 1999). The mechanisms bywhich activated glia kill neurons in culture have been suggestedto include the release of nitric oxide (Chao, 1996; Bolanos etal., 1997; Hu et al., 1997; Loihl and Murphy, 1998), reactiveoxygen species (Beckman et al., 1994; Chao et al., 1995b), glutamate(Barger and Basile, 2001), TNF $alpha$ , and IL-1 $beta$ (Chao et al., 1995a;Viviani et al., 1998). NO is released from activated astrocytesand microglia (Brown et al., 1995; Chao, 1996; Murphy, 2000),and neurons are remarkably sensitive to NO-induced cell death(Leist et al., 1997a; Wei et al., 2000). The mechanisms of NOneurotoxicity are still unclear, but have been proposed to includethe following: (1) activation of poly (ADP ribose) polymerasefollowed by NAD⁺ and ATP depletion (Zhang et al., 1994), (2) induction of apoptosisby poorly defined mechanisms (Leist et al., 1997b; Tamatani etal., 1998; Uehara et al., 1999), and (3) glutamate release (Meffertet al., 1994; Trabace and Kendrick, 2000) and excitotoxicity (Hewettet al., 1994; Leist et al., 1997a) and inhibition of mitochondrialrespiration (Heals et al., 1999).

NO can potently, acutely, and reversibly inhibit mitochondrial respiration at cytochrome c oxidase in competition with oxygen(Brown and Cooper, 1994; Brown, 1999). We have shown previouslythat NO from activated astrocytes reversibly inhibits the cellularrespiration of those astrocytes (Brown et al., 1995) and thatNO reversibly inhibits the respiration of isolated nerve terminals(synaptosomes) at nanomolar concentrations (Brown and Cooper,1994), causing acute glutamate release from the nerve terminalscaused by the inhibition of cytochrome c oxidase (McNaught andBrown, 1998). Thus a possible mechanism of glial-induced neuronaldeath is NO from activated glia causing inhibition of neuronalrespiration, leading to release of glutamate, which subsequentlycauses excitotoxic death of the neurons. We set out to test thisand related hypotheseshere.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuronal cell culture. Cerebellar granule cells (CGCs) were prepared from 7-d-postnatal Wistar rats as described previouslyby Cambray-Deakin (1995) with some modifications. In brief, thecerebella were dissociated in Versene solution (1:5000; Life Technologies,Paisley, UK) and plated at 0.25 × 10⁶ cells/cm² in 24-well plates (in 500 µl of DMEM) coated with poly-L-ornithinehydrochloride (15 µg/ml; Sigma, Paisley, UK). Cultures were maintainedin DMEM (Life Technologies) supplemented with heat-inactivatedhorse serum (5%, Life Technologies) and fetal calf serum (5%;Sigma), 2 mM L-glutamine, 25 mM KCl, and 10 µg/ml gentamicin.Cytosine-D-arabinoside (10 µM; ara-C, Sigma) was added to somecultures 24 hr after plating to inhibit non-neuronal cell proliferation,which are called "neuronal cultures" here (0.5 ± 0.1% of astrocytesand 0.4 ± 0.2% of microglia). Cultures of CGCs untreated withara-C (called "neuronal-astrocytic cultures") contained 12.2 ±2.8% of astrocytes and 3.1 ± 0.7% of microglia as assessed immunocytochemicallyusing antibodies against glial fibrillary acidic protein (GFAP;marker of astrocytes) and OX-42 (marker of microglia). Cells weremaintained at 37°C in a humidified atmosphere of 5% CO₂/95% air.Neurons were routinely used at 9 d in vitro (DIV) because formationof synapses and response to NMDA receptor stimulation in the cultureof CGCs are high after 8 DIV (Leist et al., 1997a).

Astrocyte and microglial cultures. Primary, mixed glial cell cultures were prepared from the cerebral cortex of 7-d-old rats(Wistar) as described previously (Bal et al., 1994). The samerat brains were used for isolation of CGCs. Briefly, cells isolatedfrom cerebral hemispheres were dissociated in HBSS containing0.25% trypsin (Sigma) and 0.02 mg/ml deoxyribonuclease I (Sigma-Aldrich,Steinheim, Germany) and plated at a density of 0.1 × 10⁶ cells/cm² in 75 cm² culture flasks (Falcon) in DMEM with 10% fetal calf serum. Atconfluency (12-14 DIV), primary glial cultures were used to isolatemicroglial cells as described previously (Taupenot et al., 1996).Briefly, mixed glial cultures were shaken to dislodge microgliathat were loosely attached to the astrocytes. Microglia were purifiedby preplating for 30 min into culture flasks (75 cm²) at a density of 0.1 × 10⁶ cells/cm², and then the contaminating cells were removed by changing themedium. Microglia were maintained in astrocyte-conditioned medium(medium collected from astrocytic cultures after 2 d and spundown) mixed 1:1 v/v with fresh DMEM (containing 10% fetal calfserum). Microglial cultures were used 24 hr after plating. Thepurity of the microglial and astrocyte culture (after isolationof microglia) was determined immunocytochemically with OX-42 (microgliamarker, an anti-CR3 complement receptor antibody; Serotec, Oxford,UK) and anti-GFAP antibody (an astrocytic marker; AutogenBioclear,Calne, UK). The cells were fixed in 4% paraformaldehyde (Sigma)and then incubated with OX-42 or anti-GFAP (all at 1:200 dilutions)and visualized using biotinylated anti-mouse IgG antibodies (1:200dilution), avidin-biotin-horseradish peroxidase complex, and diaminobenzidinetetrahydrochloride (ABC staining System; Santa Cruz Biotechnology,Santa Cruz, CA). Of the cells in microglial cultures, 99.5 ± 0.3%were positive for OX-42, the marker for macrophage/microglialcell types (GFAP-positive cells were not present). In astrocyteculture, 97-98% cells were anti-GFAP positive and only 2-3% cellswere OX-42 positive(microglia).

Activation of microglia and astrocytes in culture. Cultures of astrocytes (12-14 DIV, confluent, 75 cm² culture flasks, after shaking off microglia) or microglia (24hr after isolation from mixed glial cultures) were activated byexposure to lipopolysaccharide (LPS) from Salmonella typhimurium(10 µg/ml, Sigma, St. Louis, MO) and interferon- $gamma$ (IFN- $gamma$ , 100U/ml; Sigma) in the presence of arginase (0.2 U/ml) for 16-18hr. After the activation time, the microglia or astrocytes weregently trypsinized (0.1%) for 2-3 min (at 37°C), and the cellswere spun down and resuspended in DMEM or Krebs-HEPES buffer consistingof (in mM): 1.5 CaCl₂, 5.6 glucose, 10 HEPES, 4.7 KCl, 1.2 KH₂PO4,1.1 MgSO_4, 118 NaCl, pH 7.4.

Assessment of cell viability and morphology. The viability of CGCs was estimated by propidium iodide (20 µg/ml) (Sigma) andHoechst 33342 (10 µg/ml) (Sigma) staining using a fluorescencemicroscope (Leica). Propidium iodide stained only the cells withdisrupted plasma membrane integrity, so these cells were consideredto be necrotic. The nuclear morphology of the cell (chromatincondensation and fragmentation) was studied using the cell-permeableDNA dye Hoechst 33342 to assess whether apoptotic cells were present.Cells with homogeneously stained nuclei were considered to beviable. Additionally, to distinguish between necrosis and apoptosisat the single-cell level, annexin-V (Roche Diagnostics GmbH, Mannheim,Germany) and propidium iodide staining were performed simultaneously.Cells positive for both annexin-V and propidium iodide were consideredto be necrotic, and cells that were annexin-V positive only (propidiumiodide negative) were considered to beapoptotic.

Necrotic and apoptotic neurons were counted in three microscopic fields in each well (three wells per treatment) and expressedas a percentage of the total number of neurons. Each exposurewas repeated at least three times. To estimate the number of deadcells that disappeared in cocultures of CGCs with activated microglia,the total number of dead and live cells was quantified and comparedwith the total number of cells in sister (nontreated, control)cultures.

Measurement of NO generation and oxygen consumption. Measurement of NO production and oxygen consumption of cells was performedusing a Clark-type NO electrode (World Precision Instruments)inserted through the top of a thermostated, stirred, and sealedvessel with a Clark-type oxygen electrode in the base (Rank Brothers),permitting simultaneous measurement of NO and O₂ levels (Brownand Cooper, 1994). The NO electrode was calibrated with aliquotsof NO-saturated water, assumed to contain 2 mM NO. After gentlescraping, CGCs (9 DIV), in sheets from 25 cm² culture flasks (~4.0 × 10⁶ cells), were transferred into the above-described vessel maintainedat 37°C in 0.5 ml of Krebs-HEPES buffer, pH 7.4, additionallysupplemented with 2 mM glutamine and 25 mM KCl. After a few minutes(~5 min), the activated astrocytes or microglia (~0.5 × 10⁶ of cells) were added to the vessel followed by the addition ofarginine (200 µM; NOS substrate). At the end of the experiment,10 µM hemoglobin (NO scavenger) was added to verify whether inhibitionof neuronal respiration isreversible.

Measurement of intracellular ATP levels in neuronal and astrocyte cultures. ATP was determined luminometrically (Jade luminometer,Labtech International) using ATP Bioluminescence Assay Kit (BoehringerMannheim) according to the provided protocol. Briefly, after theexposure of astrocyte culture (12-14 DIV, confluent, 24-well plate)or CGCs (in neuronal or neuronal-astrocytic cultures, 9 DIV, 0.25× 10⁶/cm², cultured in 24-well plates) to NO donor, NOC-18 (500 µM), forvarious intervals of time (5, 10, or 20 min or 4 and 24 hr), themedium was withdrawn (stored for measurements of the lactate level)and the cells were exposed to lysed buffer mixed with dilutionbuffer for 5 min and than harvested by scraping. The aliquotsof cellular extract were assayed for ATP content using the ATPdependency of the light-emitting luciferase-catalyzed oxidationof luciferin. ATP concentrations were expressed as percentageofcontrol.

Determination of lactate accumulation. Aliquots of deproteinized culture medium were assayed for lactate using a L-lacticacid kit (Boehringer Mannheim) according to the provided protocol.The amount of lactate was measured by monitoring the oxidationof L-lactic acid to pyruvate by NAD in the presence of L-lactatedehydrogenase. The equilibrium of the reaction was displaced infavor of pyruvate and NADH formation by glutamate-pyruvate transaminasein the presence of glutamate. NADH formation was monitored at340 nm and was proportional to lactateconcentration.

Measurement of glutamate content in neuronal conditioned medium. CGCs for measurements of glutamate release were culturedin 25 cm² culture flasks at high density (0.6-1.0 × 10⁶ of trypan blue-excluding cells per square centimeter) for 9 din the presence or absence of 10 µM ara-C (neuronal and neuronal-astrocyticcultures, respectively). The volume of the medium in the cultureflasks with CGCs was reduced to 2.5 ml just before exposure toNOC-18 (500 µM) or myxothiazol (2 µM) for various intervals oftime (5, 10, or 20 min or 24 hr). After this time the deproteinizedmedium of cultured CGCs was assessed for levels of glutamate bya colorimetric method coupled to glutamate dehydrogenase and aformazan end product using a commercially available kit (BoehringerMannheim). In brief, diaphorase, iodonitrotetrazolium chloride,and conditioned culture medium (after deproteinization) were combined(according to the provided protocol) and incubated for 2 min.Then 3.0 U of glutamate dehydrogenase solution was added, andthe absorbability was measured at 492 nm after 15 min and thenevery 3 min until the reaction reached steady state. A standardcurve was constructed by adding known concentrations of glutamateto culturemedium.

Statistical analysis. Data are expressed as mean ± SD and were analyzed for significance usingANOVA.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nitric oxide produced by activated microglia and astrocytes induces excitotoxic cell death of CGCs in culture

To determine whether activated microglia could kill neurons, we activated microglia with LPS/IFN- $gamma$ for 16-18 hr, washed them,then cocultured them with CGCs (85% neuronal/12% astrocytic cultures,9 DIV, 0.25 × 10⁶ cells/cm² in 500 µl of DMEM, 24-well plate) at three different densities(0.1, 0.2, and 0.3 × 10⁶ cells of activated microglia per square centimeter) for 24 hr.After 24 hr the cell death of CGCs was assessed by propidium iodideand Hoechst 33342 staining and compared with a control culture(not exposed to activated microglia). Control cultures of CGCs(neuronal-astrocytic, 9 DIV) showed well differentiated neuronswith an extensive neuritic network (Fig. 1A) and very low necroticcell death (Fig. 2). After addition of activated microglia (atany density), the first morphological change, evident after 3-4hr, was retraction of all neurites (data not shown). After 24hr of coculture of CGCs with activated microglia at the lowestdensity (0.1 × 10⁶ of cells per square centimeter), only 20 ± 5.0% of neurons wereviable, and the rest were necrotic (propidium iodide-positivecells, 34.8 ± 5.4%), had condensed DNA (Hoechst-positive cells,12.7 ± 2.4%), or had disappeared (32.5 ± 3.8%, as compared withthe number of neurons in control cultures), presumably becauseof phagocytosis by activated microglia. Hoechst-positive cellsdisplayed highly fluorescent nuclei with condensed chromatin,but mostly without fragmentation, a phenotype not present in controlcultures. When CGCs where cocultured with activated microgliaat the higher density (0.2 or 0.3 × 10⁶cells/cm²), none of the neurons survived. At the density of 0.2 × 10⁶cells/cm² (Fig. 1B), both necrotic and Hoechst-positive cells were observed,and some of the neurons disappeared (Fig. 2). At the highest density(0.3 × 10⁶cells/cm²) of activated microglia, only necrotic cell death was observed(14.8 ± 3.8%), and the rest of the neurons disappeared (85.2 ±10.8%), presumably because of phagocytosis by activated microglia.

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Figure 1. Cell death of CGCs (neuronal-astrocytic cultures, 9 DIV) induced by coculture with activated microglia or by direct exposure to proinflammatory cytokines or NOC-18 (NO donor). A, In the control culture of CGCs, note the phase-bright normal cell bodies and dense neuritic network. B, Coculture of CGCs (9 DIV, 0.25 × 10⁶cells/cm²) with LPS/IFN- $gamma$ -activated microglia (0.2 × 10⁶ cells/cm²) for 24 hr induced cell death of all neurons. Note shrunken cell bodies and nuclei and loss of all neurites (phase-contrast photographs). C, Addition of LPS (4 ng/ml) and IFN- $gamma$ (100 U/ml) simultaneously for 48 hr to the CGCs, cultured in the presence of glial cells (9 DIV, nontreated with ara-C), caused severe neuronal cell death, but dead cells were not phagocytosed. D, Morphological analysis of nuclear chromatin in CGC culture (neuronal-astrocytic, 9 DIV) exposed to 500 µM NOC-18 for 4 hr using DNA-binding fluorochrome Hoechst 33342 (fluorescence microscope). Viable cells showed round nuclei with weak fluorescence, but some nuclei had strongly condensed chromatin (bright fluorescence), predominantly without fragmentation. However, a few nuclei with fragmented chromatin were also present. Particular cell or nuclear types are indicated by the following abbreviations (placed to the right of the cell): n, healthy neurons; a, astrocyte; am, activated microglia; dn, dead neurons; cc, condensed chromatin; fn, fragmented chromatin; ncc, non-condensed chromatin. Scale bar (shown in C): A-C, 40 µm; D, 20 µm.

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Figure 2. Cell death of CGCs (neuronal-astrocytic cultures, 9 DIV) induced by addition of LPS/IFN- $gamma$ -activated microglia (0.2 × 10⁶ cells/cm²) for 24 hr. The presence of activated microglia caused predominantly necrotic cell death (PI-positive cells); however, Hoechst 33342-stained (HS) neurons (with condensed chromatin, occasionally with fragmentation) were also present. Also, some CGCs disappeared completely (presumably because of phagocytosis by activated microglia). Values represent the means ± SD of three or more separate cultures. In each experiment, three wells per treatment were analyzed, and the cells in three fields per well were counted (~80 ± 25 cells per field). **p < 0.01, ***p < 0.001 from control groups.

The neuronal death observed in the presence of activated microglia was mediated by nitric oxide because the presence of Hoechst-positiveor propidium iodide-positive neurons was almost entirely blockedby the iNOS inhibitors, 200 µM aminoguanidine (Sigma) or 25 µM1400W (Alexis Biochemicals, Lausanne, Switzerland) (Fig. 3A).The production of NO in the cocultures of CGCs with activatedmicroglia was confirmed by the presence of nitrite in the medium(19.5 ± 0.6, 22.3 ± 1.2, and 27.8 ± 0.9 µM in the presence of0.1, 0.2, and 0.3 × 10⁶ activated microglia per square centimeter, respectively) as measuredby the Griess reaction (Schmidt and Kelm, 1996). After additionof activated microglia (0.1 × 10⁶cells/cm²) in the presence of iNOS inhibitors, 200 µM aminoguanidine or25 µM 1400W, the level of nitrite in the medium was significantlydecreased (5.6 ± 0.4 and 4.4 ± 0.3 µM, respectively; control level,without added microglia, 3.8 ± 0.4 µM). The death of CGCs wasalso prevented by the NMDA noncompetitive receptor antagonist,10 µM MK-801 (dizocilpine maleate, Calbiochem), added 30 min beforeactivated microglia (Fig. 3A), suggesting that microglial NO-inducedneuronal death was mediated by glutamate.

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Figure 3. Necrotic cell death of CGCs (0.25 × 10⁶cells/cm²) induced by activated microglia (A) or LPS/IFN- $gamma$ (B). Addition of 0.2 - 10⁶cells/cm² of LPS/IFN- $gamma$ -activated microglia for 24 hr (A) or LPS/IFN- $gamma$ for 48 hr (B) to the culture of CGCs (neuronal-astrocytic) caused necrosis (PI-positive cells). The necrotic neuronal cell death was completely prevented by iNOS inhibitors aminoguanidine (200 µM) or 1400W (25 µM), was wholly or partially blocked by an NMDA receptor antagonist (10 µM MK-801), and in the case of (B) was completely prevented by pretreatment with ara-C (to eliminate glial cells). Percentages of necrotic neurons (PI-positive cells) were calculated, and the values represent the means ± SD of at least three independent experiments. ***p < 0.001 from control groups and ⁺⁺⁺p < 0.001 from activated microglia (A) or ⁺⁺p < 0.01, ⁺⁺⁺p < 0.001 from LPS/IFN- $gamma$ treatment (B).

To test whether activated astrocytes could kill neurons by similar mechanisms, neuronal-astrocytic cultures (9 DIV), untreatedwith ara-C (12.2 ± 2.8% of astrocytes and 3.1 ± 0.7% of microglia),were incubated with LPS (4 ng/ml) and IFN- $gamma$ (100 U/ml) for 48hr (Fig. 1C). After that time only necrotic neuronal death wasobserved (propidium iodide-positive cells) and it was mediatedby NO because the cell death was completely blocked by iNOS inhibitors(200 µM aminoguanidine or 25 µM 1400W) (Fig. 3B). The death ofCGCs was also prevented by MK-801 (10 µM) (Fig. 3B), suggestingagain that glial NO-induced neurotoxicity was mediated by glutamate.When neuronal cultures (CGCs, 9 DIV, pretreated with ara-C toblock the proliferation of glia; 0.5 ± 0.1% of astrocytes and0.4 ± 0.2% of microglia as assessed immunocytochemically) wereexposed to LPS/IFN- $gamma$ , no significant cell death was observed (Fig.3B). This suggests that LPS/IFN- $gamma$ is not directly toxic to neurons,but rather toxicity is mediated by glia. The death of CGCs culturedin the presence of glia and LPS/IFN- $gamma$ was caused by NO releasedfrom activated glia cells because it could be prevented by iNOSinhibitors (Fig. 3B). In this case, activated astrocytes are themain source of NO because 9-d-old culture of CGCs contained 12.2± 2.8% of astrocytes and only 3.1 ± 0.7% of microglia. LPS orIFN- $gamma$ added to neuronal-astrocytic cultures separately did notcause any significant celldeath.

NO-induced death of CGCs is prevented by MK-801

To test whether nitric oxide released from NO donors could reproduce cell death of neurons observed in the cocultures of CGCswith activated glia, CGCs (neuronal-astrocytic cultures) wereexposed to either a "pure" NO donor NOC-18 (diethylenetriamine-nitricoxide adduct), also known as DETA-NONOate (RBI, Natick, MA; Sigma),or one capable of transnitrosylation S-nitroso-N-acetyl-DL-penicillamine(SNAP; Alexis) at different concentrations (50, 100, and 500 µM)for various intervals of time (4, 16, or 24 hr). The level ofNO was measured using a NO-sensitive electrode. In the case of0.5 mM SNAP, the release of NO was variable, but in most casesthe steady-state level of NO measured by electrode was 0.5-0.75µM in DMEM after 10-15 min. In the case of 0.5 mM NOC-18, therelease of NO was less variable, and the steady-state level wasbetween 0.4 and 0.6 µM in DMEM after 15-25min.

Short incubations (4 hr) with either NO donor (NOC-18 or SNAP) at any concentration (50, 100, or 500 µM) caused little orno necrosis, as indicated by staining with propidium iodide. However,most of the cells at this time had strong chromatin condensationbut mostly without nuclear fragmentation, as assessed by Hoechst33342 staining (Fig. 1D). Additionally, only a small percentageof neurons (4-5%) bound annexin-V after the exposure to 500 µMNOC-18 or SNAP. These results suggest that NO-induced cell deathhad some apoptotic characteristic but without the classical morphologicalfeatures (apoptotic-like cells). The presence of these apoptotic-likecells could not be prevented by a cell-permeable nonspecific caspaseinhibitor, benzyloxycarbonyl-Val-Ala-Asp-fluoromethyl ketone (z-VAD-fmk;Alexis) at the concentration of 50 or 75 µM (100 µM was foundto be toxic to the neurons), suggesting that these NO-inducedchanges may not be mediated by caspases. At this time (4 hr incubation),the presence of Hoechst-positive cells could be completely preventedby 10 µM MK-801 (noncompetitive inhibitor of NMDA receptor, added30 min before NO donor), suggesting that NO-induced cell deathof CGCs was mediated by glutamate (Fig. 4A). After 16 hr of incubationwith NO donors (SNAP or NOC-18), the number of Hoechst-positivecells was very low (between 3 and 5%; results not shown), butthe presence of necrotic cells was significantly increased andalmost completely prevented by MK-801 (10 µM) (Fig. 4B). After24 hr of incubation with NO donors (NOC-18 or SNAP), only necrosis(presence of propidium iodide-positive cells) was observed. Atthat time, MK-801 (10 µM) could only partially prevent the presenceof necrotic cells (Fig. 4C). Because the presence of Hoechst-positiveand propidium iodide-positive cells was almost completely preventedby MK-801 (after 4 and 16 hr of incubation), this suggests thatexcitotoxicity was the main mechanism of granule cell death inducedby nitric oxide.

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Figure 4. Induction of neuronal death in CGC cultures (neuronal-astrocytic, 9 DIV) by NO donors (NOC-18 or SNAP) after 4 hr (A), 16 hr (B), and 24 hr (C). After 4 hr of incubation with either NO donor (SNAP or NOC-18), Hoechst-positive neurons were observed (condensed chromatin, rarely with fragmentation) (Fig. 1D), but no propidium iodide-staining cells were seen. After 16 or 24 hr of incubation, neurons died mainly by necrosis (PI-positive cells). Neuronal cell death induced by both NO donors (SNAP or NOC-18) was prevented by MK-801 (NMDA receptor antagonist) after 4 and 16 hr (but not 24 hr) of incubation. Values represent means ± SD (bars) of determinations made in three separate cultures. *p < 0.05, **p < 0.01, ***p < 0.001 from control groups and ⁺p < 0.05, ⁺⁺p < 0.01, ⁺⁺⁺p < 0.001 from SNAP or NOC-18 treatment.

The neuronal death of CGCs was also observed 24 hr after the addition of very low concentrations of NO-saturated water (1or 2 µM NO) (Fig. 5A). The presence of necrotic cells after theexposure of CGCs to NO-saturated water or NOC-18 was blocked bytwo different NO scavengers: 25 µM 2-phenyl-4,4,5,5-tetramethyl-imidazoline-1-oxyl3-oxide (PTIO; Sigma) (Fig. 5A) and 50 µM hemoglobin (Sigma) (Fig.5B). After the exposure of CGCs (24 hr) to SNAP, necrotic neuronaldeath (25 ± 3, 28.9 ± 4.2, and 66.9 ± 11.5% after 50, 100, or500 µM SNAP, respectively) was also significantly blocked by bothNO scavengers: 50 µM hemoglobin (14.3 ± 2.3, 15.6 ± 2.1, and 25.4± 4.3%) and 25 µM PTIO (18.4 ± 4.6, 19.0 ± 4.2, and 36.2 ± 6.3%).

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Figure 5. Necrotic cell death of CGCs (PI-positive cells) induced by NO-saturated water or NO donor (NOC-18) after 24 hr of exposure was prevented by NO scavengers PTIO (A) or hemoglobin (B) or by high oxygen (95% O₂/5% CO₂) (C). The data present the mean ± SD of three independent experiments. *p < 0.05, **p < 0.01 from control groups and ⁺p < 0.05, ⁺⁺p < 0.01 from NO or NOC-18 treatment.

The applied concentrations of NOC-18 or SNAP caused cell death of neurons only, without affecting the viability of glial cells.The fact that a single addition of 1 or 2 µM of authentic NO causedsignificant cell death (18-22%) after 24 hr indicates that theseneurons are very sensitive to NO-induced cell death and that becausethe NO breaks down rapidly (Fig. 6A), the NO needs to be presentfor only a few minutes to initiate cell death. Interestingly,NO-induced necrosis of CGCs (after addition of NO-saturated water)was prevented when the medium was transiently oxygenated with95% O₂ and 5% CO₂ before NO exposure (Fig. 5C). However, thishigh oxygen level on its own induced some apoptotic-like (Hoechst-positive)CGCs (Fig. 5C). We have shown previously that oxygen antagonizesthe NO-induced inhibition of respiration and glutamate releasein synaptosomes, because nitric oxide binds competitively withoxygen to the same binding site on cytochrome oxidase (Brown andCooper, 1994; McNaught and Brown,1998). Thus these results suggestthat neuronal cell death could be mediated by NO-induced inhibitionof mitochondrial respiration at cytochrome oxidase.

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Figure 6. Rapid inhibition of mitochondrial respiration of CGCs by addition of 2 µM NO-saturated water (A) or NO produced by activated microglia (B) or activated astrocytes (C). A, Oxygen consumption (top trace) of CGCs (~4.0 × 10⁶ of cells) before addition of NO-saturated water was 3.9 natom of O/min/10⁶ cells; after addition of NO-saturated water (2.0 µM NO), oxygen consumption was completely and immediately inhibited for the first few minutes, but the rate recovered as the NO level declined (3.1 natom of O/min/10⁶ cells). B, Addition of activated microglia (~0.5 × 10⁶cells; NO level 0.62 µM) and arginine (200 µM; NOS substrate) caused rapid and strong inhibition of neuronal respiration (~4.2 × 10⁶cells; oxygen consumption, 4.2 natom of O/min/10⁶ cells and 0.81 natom of O/min/10⁶ cells before and after addition of activated microglia, respectively). The inhibition of neuronal respiration was reversible, because the addition of 10 µM hemoglobin (HbO₂, NO scavenger) resulted in full activation of mitochondrial respiration (4.16 natom of O/min/10⁶ cells). C, Addition of activated astrocytes (~0.75 × 10⁶ cells; NO level 0.56 µM) and arginine (200 µM) induced significant inhibition of oxygen consumption of CGCs (~4.2 × 10⁶ cells; oxygen consumption, 6.0 and 1.4 natom of O/min/10⁶ cells before and after addition of activated astrocytes, respectively), which was reversed by hemoglobin (HbO₂) (7.3 natom of O/min/10⁶ cells). Values placed next to the oxygen traces express oxygen consumption in natom of oxygen per minute per 10⁶ cells.

Nitric oxide produced by activated microglia or astrocytes rapidly and reversibly inhibits mitochondrial respiration of surrounding neurons

We have shown previously that nanomolar concentrations of NO cause a rapid and reversible inhibition of mitochondrial respirationin brain synaptosomes (Brown and Cooper 1994) and astrocytes (Brownet al., 1995) caused by inhibition of cytochrome oxidase. We testedhere whether NO could inhibit neuronal respiration in a similarway.

Oxygen consumption of CGCs alone (~4.0 × 10⁶ cells) was 3.9 natom of O/min/10⁶ cells, but the addition of NO-saturated water (2 µM NO) causedimmediate and complete inhibition of neuronal respiration (Fig.6A). However, it recovered once the NO levels in the medium wereclose to 0.0 µM (3.1 natom of O/min/10⁶ cells) (Fig. 6A). Dramatic inhibition of neuronal respirationwas also observed after addition of activated microglia (~0.5× 10⁶ microglia added to 4.2 × 10⁶ neurons), producing 0.55 ± 0.1 µM NO after addition of 200 µMarginine. Oxygen consumption was inhibited from 4.3 ± 0.4 in theabsence of microglia to 0.75 ± 0.2 natom of O/min/10⁶ in the presence of activated microglia, i.e., 82.0 ± 4.0% inhibition.This inhibition of respiration was reversible, because the additionof hemoglobin (NO scavenger) resulted in full activation of neuronalrespiration (4.2 ± 0.2 nmol of O/min/10⁶ cells) (means ± SD from nine independent experiments) (Fig. 6B,sample trace). Similar results were also observed when CGCs wereincubated with activated astrocytes (Fig. 6C). Addition of activatedastrocytes (~0.75 × 10⁶ cells of astrocytes added to 4.2 × 10⁶ neurons) producing 0.52 ± 0.16 µM NO caused strong and rapidinhibition of neuronal respiration (oxygen consumption beforeand after addition of activated astrocytes was 5.8 ± 0.26 and1.2 ± 0.3 natom of O/min/10⁶ cells, respectively, i.e., 79.0 ± 5.0% of inhibition), and theinhibition of respiration was completely reversed by hemoglobin(6.5 ± 0.8 natom of O/min/10⁶ cells) (means ± SD from three independent experiments) (Fig.6C, sample trace).

To test what levels of NO were produced by activated glial cells alone, activated microglia or astrocytes were incubated bythemselves (~1.0 × 10⁶ cells), and the level of NO was measured using a NO electrode.They produced NO continuously to reach a steady-state level after10-15 min of 1.1 ± 0.23 and 0.76 ± 0.35 µM (activated microgliaand astrocytes, respectively) (data from three independentexperiments).

Because NO produced by activated astrocytes or microglia inhibits neuronal respiration, this respiratory inhibition mightcontribute to neuronal celldeath.

Respiratory inhibitors cause extensive neuronal cell death

To determine whether inhibition of mitochondrial respiration causes neuronal cell death, CGCs (neuronal-astrocytic cultures,9 DIV) were exposed to specific respiratory inhibitors (myxothiazol,KCN, or azide) for various periods of time (4, 16, or 24 hr),and then the cell death was assessed by propidium iodide, Hoechst33342, and annexin-V staining. After 4 hr of incubation with 2µM myxothiazol (specific inhibitor of respiratory complex III)(Fig. 7A), some necrotic cells were present (propidium iodidepositive), but mainly Hoechst-positive neurons were observed (withbright and condensed chromatin, without fragmentation). The presenceof Hoechst-positive cells could not be blocked by z-VAD-fmk. Onlya very small percentage of cells was stained with annexin-V (between1.0 and 2.0%). At this time of incubation, the presence of Hoechst-positiveas well as propidium iodide-positive cells was almost completelyprevented by MK-801 (NMDA receptor antagonist added 30 min beforemitochondrial inhibitor) (Fig. 7A). After 16 hr of incubation,the number of necrotic cells increased, but MK-801 was less effectiveat blocking cell death (Fig. 7B). After 24 hr of incubation, almostall dead CGCs were necrotic (propidium iodide positive), and MK-801was not effective at all in preventing cell death (Fig. 7C). Similarresults were obtained after the exposure of CGCs to 2 mM azideor 2.5 mM KCN (inhibitors of cytochrome c oxidase). In the caseof azide, the percentage of Hoechst-positive cells was 64.5 ±8.6, 32.9 ± 11.0, and 4.8 ± 1.5% in the absence of MK-801 and0.5 ± 0.5, 29.0 ± 8.2, and 3.2 ± 1.8% in the presence of 10 µMMK-801 (after 4, 16, or 24 hr of incubation, respectively). Azidealso caused necrotic cell death (propidium-positive cells): 8.9± 1.2, 52.1 ± 8.5, and 95.2 ± 2.3% in the absence of MK-801 and2.8 ± 0.3, 54.4 ± 9.8, and 96.8 ± 3.4% of necrotic cells in thepresence of MK-801 after 4, 16, or 24 hr of incubation, respectively.After exposure of CGCs to 2.5 mM KCN, Hoechst-positive cells werealso present (54.0 ± 10.3, 26.4 ± 5.6, and 15.0 ± 3.8%, in theabsence of MK-801), and these was partially blocked by 10 µM MK-801(0.4 ± 0.3, 18.5 ± 4.9, and 14.8 ± 3.6% after 4, 16, and 24 hrof incubation, respectively). KCN also induced necrosis (12.1± 3.5, 73.6 ± 8.4, and 85.0 ± 9.8 in the absence of MK-801 and2.3 ± 0.9, 45.2 ± 6.5, and 86.0 ± 8.4% in the presence of 10 µMMK-801 after 4, 16, and 24 hr of exposure, respectively).

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Figure 7. Induction of neuronal death in CGCs (neuronal-astrocytic cultures) by a specific mitochondrial inhibitor (2 µM myxothiazol) for 4 hr (A), 16 hr (B), and 24 hr (C) in the presence and absence of the noncompetitive NMDA receptor antagonist MK-801 (10 µM). A, After 4 hr of incubation with 2 µM myxothiazol (Myxo) mainly Hoechst-positive (HS) cells were observed (with condensed chromatin, without fragmentation). MK-801 prevented the neuronal death induced by myxothiazol after 4 hr (A) and partially after 16 hr of incubation (B) but not after 24 hr (C). Values represent means ± SD (bars) of determinations made in three separate cultures. **p < 0.01, ***p < 0.001 from control groups and ⁺p < 0.05, ⁺⁺p < 0.01 from myxothiazol treatment.

In general, the pattern of mitochondrial inhibitor- and NO donor-induced neuronal cell death was similar. Mitochondrial inhibitor-or NO donor-induced early condensation of DNA (4 hr incubation)was prevented by MK-801, but the later necrosis was only partiallyblocked by this NMDA receptor antagonist. In the case of respiratoryinhibitors, MK-801 was generally less effective at blocking necrosisthan in the case of NO donors. This might be because the respiratoryinhibitor irreversibly inhibited neuronal respiration, whereasrespiratory inhibition by NOC-18 was partially reversible withtime.

Because NO inhibits respiration and specific respiratory inhibitors cause neuronal death of a similar type and time course(but with some differences), these results suggest that NO inhibitionof mitochondrial respiration could be the main mechanism involvedin triggering NO-induced neuronaldeath.

Nitric oxide rapidly depletes neuronal but not astrocytic ATP

Because NO-induced mitochondrial inhibition might result in energy depletion, ATP levels were studied in neuronal and neuronal-astrocyticcultures (CGCs, 9 DIV, treated or untreated with ara-C, respectively)and astrocytic cultures (12-14 DIV, confluent) exposed to NOC-18(500 µM) for various intervals of time (5, 10, or 20 min or 4and 24 hr). Severe and rapid ATP depletion (38.0 ± 7.0% in 20min and 91.0 ± 1.0% after 24 hr) was observed in neuronal cultures(depleted of glial cells) (Fig. 8A). In neuronal-astrocytic cultures,the decrease in ATP levels after exposure to NOC-18 (500 µM) wasless dramatic but still significant (48.7 ± 1.8% after 24 hr)(Fig. 8B). In contrast to neurons, astrocytes were much less sensitiveto NO-induced ATP depletion. Indeed, short-time exposure to NOC-18(500 µM) did not cause any ATP depletion (Fig. 8C), and 24 hrincubation caused only 10.0 ± 5.0% of ATP decrease when comparedwith the control culture (Fig. 8C). Even after 72 hr exposureto NOC-18 the ATP level had decreased by only 36.0 ± 4.0% (datanot shown). However, astrocytes and neurons appeared to be equallysensitive to NO-induced inhibition of mitochondrial respiration(Brown et al., 1995) (Fig. 6A). These results are consistent withneurons being particularly dependent on mitochondrial energy productionin contrast to astrocytes, which after NO-induced mitochondrialinhibition may be able to maintain ATP levels by glycolysis.

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Figure 8. Depletion of ATP caused by 500 µM NOC-18 in neuronal cultures (CGCs treated with ara-C) (A), in neuronal-astrocytic cultures (CGCs cultured in the absence of ara-C) (B), and in pure astrocytic cultures (C). The data are expressed as percentage of the control (untreated) ATP levels, which were 1.51 ± 0.13 nmol of ATP/10⁶cells in the neuronal cultures (A), 1.75 ± 0.1 nmol of ATP/10⁶ cells in the neuronal-astrocytic cultures (B), and 7.1 ± 0.5 nmol of ATP/10⁶ cells in the astrocytic cultures (C). Values represent means ± SD (bars) of determinations made in three separate cultures. *p < 0.05, **p < 0.01, ***p < 0.001 from control groups.

NO donors increase the level of L-lactic acid in neuronal and astrocytic cultures after prolonged exposure

To test whether NO-induced mitochondrial inhibition and subsequent ATP depletion in neuronal and astrocytic cultures wouldstimulate glycolysis, the level of L-lactic acid was measuredin the medium of CGCs (9 DIV, 24-well plates) or astrocyte culture(12-14 DIV, confluent, 75 cm² flasks) exposed to a NO donor (500 µM NOC-18) or a specific mitochondrialinhibitor (2 µM myxothiazol) for various intervals of time (5min, 30 min, 4 hr, or 24 hr). Surprisingly, a short time incubation(5 or 30 min) with NOC-18 (but not with myxothiazol) caused aslight decrease in L-lactic acid levels, but longer exposure times(4 or 24 hr) significantly increased the level of L-lactic acidin both types of cultures, neuronal (Fig. 9A) and astrocytic (Fig.9B). However, in neuronal cultures (depleted of glia), the increasedlevels of L-lactic acid after the exposure to NOC-18 was only28.3 ± 0.4% in contrast to astrocyte culture in which the levelof lactate was increased 68.2 ± 0.8% when compared with the controlculture.

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Figure 9. Levels of L-lactic acid in the medium of neuronal or neuronal-astrocytic (A) and astrocytic (B) cultures, exposed to NO donors (500 µM SNAP or NOC-18) or a specific mitochondrial inhibitor (2 µM myxothiazol). Neuronal cultures were cultured in the presence of ara-C (+ara-C), neuronal-astrocytic cultures in the absence of ara-C ( $-$ ara-C). C, Increased levels of L-lactic acid and acidic pH (measured with pH electrode) in the medium of astrocytic cultures, activated for 18 hr with LPS/IFN- $gamma$ . Note the decreased levels of L-lactic acid (and increased pH) in the presence of an iNOS inhibitor (25 µM 1400W), suggesting that activation of glycolysis was mediated by NO. Values represent means ± SD (bars) of determinations made in three separate cultures. Statistical significance of the difference between L-lactic acid levels after 24 hr of exposure to NOC-18 was *p < 0.05 from control (+ara-C) and **p < 0.01 from control ( $-$ ara-C), and after exposure to myxothiazol it was **p < 0.01 from control ( $-$ ara-C) in A and **p < 0.01 after exposure to myxothiazol from control in B.

An activation of glycolysis was also observed in the culture of astrocytes after 18 hr of activation with LPS/IFN- $gamma$ becausethe level of L-lactic acid was significantly increased (controllevel, 7.18 ± 1.2 mM; after activation, 13.3 ± 1.15 mM) (Fig.9C). This activation of glycolysis was probably mediated by NO-inducedinhibition of respiration, because in the presence of an iNOSinhibitor (25 µM 1400W), levels of lactate were similar to thecontrol levels (Fig. 9C). Forty-two hours after activation, thelevels of lactate were even higher (26.2 ± 0.6 mM, pH 5.9 ± 0.15;control, 12.24 ± 0.5 mM, pH 7.4 ± 0.1), but in the presence ofiNOS inhibitor (25 µM 1400W), the levels of lactate were onlyslightly higher (14.5 ± 1.2, pH 7.2) than in the control (Fig.9C).

Nitric oxide causes glutamate release from neurons

Because neuronal cell death observed in the culture of CGCs exposed to activated glial cells (astrocytes or microglia) orto NO donors (SNAP or NOC-18) was prevented by MK-801 (NMDA receptorantagonist), suggesting that glutamate was involved in NO-inducedcell death, we tested whether nitric oxide would cause glutamaterelease from cultured neurons. Indeed, NOC-18 (500 µM) causedimmediate (<1 min) release of glutamate from neuronal-astrocytic(Fig. 10B) and neuronal cultures (Fig. 10A). Glutamate was undetectablein neuronal-astrocytic cultures before the addition of NO donor,but rose immediately after exposure to NOC-18 (500 µM) and wasat the same level for the initial 30 min (8.2 ± 0.5 µM) and thendecreased after longer incubation times (4 or 24 hr) (Fig. 10B),possibly because of reuptake by astrocytes. These concentrationsof glutamate in the medium are sufficient to activate NMDA receptors(Patneau and Mayer, 1990). In the case of neuronal cultures (CGCscultures depleted of glial cells), NOC-18 also caused glutamaterelease, but the level increased with time (16.2 ± 2.4 µM after24 hr) (Fig. 10A), possibly because it could not be removed fromthe medium by astrocytes.

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Figure 10. Release of glutamate from CGCs induced by NOC-18 (500 µM) or a specific mitochondrial inhibitor (2 µM myxothiazol). NOC-18 (500 µM) induced rapid release of glutamate from neuronal (A) or neuronal-astrocytic cultures (B) (treated and untreated with ara-C, respectively). C, Myxothiazol (2 µM; a specific mitochondrial inhibitor) also induced rapid glutamate release from neuronal-astrocytic cultures. Values represent means ± SD (bars) of determinations made in three separate cultures. Statistical significance of the difference between glutamate levels at time 0 and 10 min after treatment with NOC-18 was as follows: p < 0.05 in A, p < 0.001 in B, and after myxothiazol treatment p < 0.01 in C.

To test whether NO-induced inhibition of mitochondrial respiration could be the cause of glutamate release from CGCs, we studiedthe release of glutamate in neuronal-astrocyte cultures exposedto a specific mitochondrial inhibitor (2 µM myxothiazol) for variousintervals of time (1, 5, 10, or 30 min and 4 or 24 hr). Similarlyto the NO donor, myxothiazol also induced glutamate release fromCGCs after a very short time of incubation (Fig. 10C). These resultssuggest that NO-induced inhibition of mitochondrial respirationcould be the mechanism responsible for NO-induced release of glutamatefromCGCs.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have shown here (consistent with previous findings by Chao, 1996; Hu et al., 1997; Kingham et al., 1999; Tanabe et al.,1999) that inflamed glia have a remarkable capacity to kill coculturedneurons, even when present at relatively low concentrations. Thishas important implications for pathology because astrocytes, microglia,and macrophages become activated in virtually all CNS pathologies,including inflammatory, infective, post-ischemic, and neurodegenerativediseases, as well as aging (Eddleston and Mucke, 1993; Beal, 1995;Murphy, 2000). Activated glia may be directly causing neuronaldeath in these pathologies, although glial activation may alsohave protective roles, and neuronal death may contribute to glialactivation. For example, in Alzheimer's disease, activated microgliaand astrocytes expressing iNOS are found in the amyloid plaquessurrounded by dead and dystrophic neurites (Wa et al., 1996; Wallaceet al., 1997; Lee et al., 1999), $beta$ -amyloid can induce culturedglia to express iNOS and kill cocultured neurons via NO (Goodwinet al., 1995; Wisniewski et al., 1998), and anti-inflammatorydrugs protect against Alzheimer's disease (McGeer and McGeer,1995; McGeer et al., 1996; Lim et al., 2000).

In this study, activated microglia or astrocytes induced cell death of cocultured CGCs. The neuronal cell death was entirelymediated by glial NO from iNOS because it was completely preventedby two structurally unrelated iNOS inhibitors. This conclusionis supported by the finding that NO donors NOC-18 and SNAP (orNO-saturated water) producing steady-state levels of NO (0.5-0.75µM) similar to those produced by activated glia (0.5-1 µM) (Fig.6B,C) caused a similar type of neuronal death, with a similartime course, that was similarly blocked by MK-801. Thus in ourmodel of inflammatory neurodegeneration, neuronal death inducedby activated glia was mediated by iNOS-derived NO alone, ratherthan other suggested mediators such as cytokines (Chao et al.,1995a; Viviani et al., 1998), proteases (Glockzin et al., 1999),or reactive oxygen species (Tanaka et al., 1994; Chao et al.,1995b).

One of the mechanisms by which NO causes neuronal death could be inhibition of mitochondrial respiration. In this study wefound that NO from NO-saturated water or from activated astrocytesor microglia caused rapid, potent, and reversible inhibition ofneuronal respiration. We have shown previously that such NO inhibitionof respiration is caused by the reversible inhibition of cytochromeoxidase in competition with oxygen (Brown and Cooper, 1994; Brownet al., 1995; Brown, 1999). Others have shown similar inhibitionin isolated mitochondria (Cleeter et al., 1994; Schweizer andRichter, 1994) and inhibition of energy metabolism in neurons(Brorson et al., 1999). We found here that a specific respiratoryinhibitor (myxothiazol) replicated many of the effects of NO,including immediate respiratory inhibition, followed by rapidglutamate release, followed by neuronal cell death, blocked byMK-801 (at early incubation times). Moreover, preventing NO inhibitionof respiration by transiently incubating the neurons with highoxygen during the exposure to NO-saturated water prevented subsequentNO-induced necrosis. However, we cannot rule out that this protectionwas mediated by more rapid breakdown of NO to NO₂ or peroxynitriteat high oxygen levels, thus resulting in a shorter exposure timeto NO. On the other hand, the fact that such short-term exposureto NO (1-5 min in Fig. 5C) results in significant neuronal celldeath, which is blocked by high oxygen, indicates that NO₂ orperoxynitrite is unlikely to mediate the neurotoxicity, and thatwhatever does mediate the actions of NO must happen within 1-2min of NO exposure. Because NO caused inhibition of neuronal respirationwithin seconds, and NO or a specific respiratory inhibitor (myxothiazol)caused glutamate release within 1 min, and subsequent neuronaldeath is blocked by MK-801, NO-induced cell death is probablytriggered by respiratory inhibition, followed by glutamate releaseand excitotoxicity. That NO inhibited respiration in the cultureis supported by the finding that NO donors caused rapid ATP depletionin neuronal cultures (25% decrease within 5 min, 40% in 20 min,90% in 24 hr) followed by activation of glycolysis (measured bylactate release), and that LPS/IFN $gamma$ -induced activation of astrocytecultures caused increased lactate levels and acidification ofthe culture medium (Fig. 9C).

NO donors caused rapid (<1 min) glutamate release into the medium of mixed and pure neuronal cultures. A similar pattern ofglutamate release was also observed after the exposure of mixedcultures to myxothiazol. Although the pattern differs after long-termtreatment (4 and 24 hr), when the amount of NO released from NOC-18may not be sufficient to fully inhibit respiration, the rapidrelease of glutamate caused by both NOC-18 and myxothiazol suggeststhat inhibition of mitochondrial respiration could be the mechanismresponsible for glutamate release. We have shown previously thatNO causes rapid glutamate release from synaptosomes caused byinhibition of cytochrome oxidase and probable reversal of theglutamate uptake carrier (McNaught and Brown, 1998). Others haveshown NO-induced glutamate release in cultures and in vivo (Takitaet al., 1997; Kingham et al., 1999; Trabace and Kendrick, 2000).The level of glutamate released into the culture medium by NO(~8 µM glutamate) (Fig. 10A) has been shown to be sufficient toinduce excitotoxic death of neurons (Patneau and Mayer, 1990).However, the NO-induced respiratory inhibition may also greatlyincrease the sensitivity of neurons to glutamate toxicity (becauseof depolarization and removal of the Mg²⁺ block of the NMDA receptor) (Vornov and Coyle, 1991). An antagonistof the NMDA receptor (MK-801) blocked neuronal death induced byactivated astrocytes, microglia, NO donors, and myxothiazol (aftershort incubation time), suggesting that death was triggered atleast in part by activation of NMDA receptors. MK-801 completelyblocked DNA condensation at 4 hr (imaged by Hoescht staining),induced by NO donors and myxothiazol, and completely or partiallyblocked necrosis at 16 hr but was less effective at blocking necrosisat 24 hr. This may indicate either that 10 µM MK-801 was not completelyeffective at blocking NMDA receptors or that other mechanismsof NO-induced cell death become important after longer-term incubationswith NO donors. Note that neuronal ATP was almost completely depletedat 24 hr (at least in the absence of MK-801) (Fig. 8A), whichsuggests that necrosis might have resulted from ATP depletion.However, MK-801 completely prevented neuronal death induced byexposure to activated microglia for 24 hr and very largely preventedthat induced by activation of astrocytes in mixed culture for48 hr, suggesting that cell death in these models is caused almostexclusively byexcitotoxicity.

Death induced by activated astrocytes or microglia, NO, NO donors, or myxothiazol was confined exclusively to neurons; therewas no significant cell death seen in astrocytes or microglia.This is consistent with our findings that NO donors caused nosignificant change in ATP levels in pure astrocyte cultures forup to 24 hr. The ATP level that we measured in mixed culturesprobably had contributions from both neurons and glia. We haveshown previously that astrocytes are sensitive to NO-induced inhibitionof respiration (Brown et al., 1995), and we found here that glycolysisis activated in the astrocyte cultures by NO donors and LPS/IFN- $gamma$ ,consistent with inhibition of respiration. However, astrocytesare known to have a higher glycolytic capacity than neurons (Pauwelset al., 1985; Peuchen et al., 1997) and are insensitive to excitotoxicity(Weiss et al., 1993).

We found previously in PC12 cells that NO donors induced necrosis caused by respiratory inhibition and ATP depletion if glucosewas not present, but this was completely prevented by glucose,suggesting that cells with insufficient glycolytic capacity wouldbe sensitive to NO-induce necrosis via respiratory inhibition.However, in the presence of glucose, NO induced caspase- and cytochromec-mediated apoptosis (Bal-Price and Brown, 2000). The levels ofNO donors used in the present study did not induce any cell deathin the astrocytes. However, we found that higher levels of NOdonors (1-2 mM NOC-18 for 48 or 72 hr) do induce apoptosis inastrocytes (DNA condensation and fragmentation; data notshown).

The neuronal cell death induced by activated glia, NO donors, and myxothiazol had some characteristics of apoptosis, but itwas not classical apoptosis. Within 4 hr of NO donor treatment,most neurites were lost, the nuclei had shrunk, and the DNA wasstrongly condensed. However, the nuclear DNA was condensed butnot fragmented, there was relatively little annexin-V staining,and a caspase inhibitor (zVAD) did not prevent DNA condensationor cell death. It is probably best to avoid trying to classifysuch death as either apoptotic or necrotic without furtheranalysis.

In conclusion, we found that activated glia potently kill cocultured neurons via glial NO-inhibiting neuronal respiration,resulting in glutamate release causing excitotoxic death of neuronsvia NMDA receptors (Fig. 11). We have found recently that NO causesglutamate release from astrocytes (our unpublished data), andthis might also contribute to excitotoxicity. NO inhibition ofneuronal respiration might also activate NMDA receptors via plasmamembrane depolarization. Calcium entry via NMDA receptors mayinduce neuronal death (possibly via mitochondrial damage) andmight further increase NO production by activation of neuronalnitric oxide synthase.

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Figure 11. Proposed scheme of inflammatory neurodegeneration mediated by glial NO. NO produced by activated microglia or astrocytes inhibits mitochondrial (mito) respiration of surrounding neurons, causing glutamate release (through glutamate transporters; GluT) from neurons (and possibly from astrocytes) and then stimulation of NMDA receptors (NMDAR). Activation of NMDA receptors by glutamate (possibly aided by respiratory inhibition-induced depolarization) triggers massive influx of Ca²⁺ into neurons, leading to apoptotic or necrotic cell death.

  FOOTNOTES

Received March 22, 2001; revised May 29, 2001; accepted June 14, 2001.

This work was supported by the WellcomeTrust.
Correspondence should be addressed to Anna Bal-Price, Department of Biochemistry, University of Cambridge, Tennis Court Road,Cambridge, CB2 1QW, UK. E-mail: akp26{at}mole.bio.cam.ac.uk.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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