Distinct Role for Microglia in Rotenone-Induced Degeneration of Dopaminergic Neurons

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (120)

Citing Articles via Google Scholar

Google Scholar

Articles by Gao, H.-M.

Articles by Liu, B.

Search for Related Content

PubMed

PubMed Citation

Articles by Gao, H.-M.

Articles by Liu, B.

Previous Article  |  Next Article

The Journal of Neuroscience, February 1, 2002, 22(3):782-790

Distinct Role for Microglia in Rotenone-Induced Degeneration of Dopaminergic Neurons
Hui-Ming Gao¹^,², Jau-Shyong Hong¹, Wanqin Zhang², and Bin Liu¹
¹ Neuropharmacology Section, Laboratory of Pharmacology and Chemistry, National Institute of Environmental Health Sciences, National Institutes of Health, Research Triangle Park, North Carolina 27709, and ² Department of Physiology, Dalian Medical University, Dalian, 116027, China

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Increasing evidence has suggested an important role for environmental factors such as exposure to pesticides in the pathogenesisof Parkinson's disease. In experimental animals the exposure toa common herbicide, rotenone, induces features of parkinsonism;mechanistically, rotenone-induced destruction of dopaminergicneurons has been attributed to its inhibition of the activityof neuronal mitochondrial complex I. However, the role of microglia,the resident brain immune cells in rotenone-induced neurodegeneration,has not been reported. Using primary neuron-enriched and neuron/gliacultures from the rat mesencephalon, we discovered an extraordinaryfeature for rotenone-induced degeneration of cultured dopaminergicneurons. Although little neurotoxicity was detected in neuron-enrichedcultures after treatment for 8 d with up to 20 nM rotenone, significantand selective dopaminergic neurodegeneration was observed in neuron/gliacultures 2 d after treatment with 20 nM rotenone or 8 d aftertreatment with 1 nM rotenone. The greatly enhanced neurodegenerativeability of rotenone was attributed to the presence of glia, especiallymicroglia, because the addition of microglia to neuron-enrichedcultures markedly increased their susceptibility to rotenone.Mechanistically, rotenone stimulated the release of superoxidefrom microglia that was attenuated by inhibitors of NADPH oxidase.Furthermore, inhibition of NADPH oxidase or scavenging of superoxidesignificantly reduced the rotenone-induced neurotoxicity. Thisis the first report demonstrating that microglia play a pivotalrole in rotenone-induced degeneration of dopaminergic neurons.The results of this study should advance our understanding ofthe mechanism of action for pesticides in the pathogenesis ofParkinson'sdisease.

Key words: pesticides; microglia; superoxide; dopamine; Parkinson's disease; neurotoxicity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Parkinson's disease (PD) is characterized by a progressive and selective loss of dopaminergic neurons in the substantia nigra(SN), resulting in movement disorders (Olanow and Tatton, 1999).Sporadic PD accounts for >90% of the incidence of the disease,with the remaining fraction of mostly familial PD suspected tobe linked to mutations in several recently identified genes, including $alpha$ -synuclein and parkin (Langston, 1998; Polymeropoulos, 1998;de Silva et al., 2000). Unlike its familial counterpart, idiopathicPD usually begins in the fifth decade of life and progresses overa period of 10-20 years. Although the etiology of idiopathic PDremains unknown, epidemiological and case control studies haveimplicated rural living, well water consumption, and pesticideexposure as potential risk factors for PD (Priyadarshi et al.,2001). Among these factors, exposure to pesticides and insecticidesappears to have one of the strongest correlations with an increasedincidence of PD (Gorell et al., 1998; Ritz and Yu, 2000; Herishanuet al., 2001).

Recent success in demonstrating the degenerative effect of several pesticides on the nigrostriatal dopaminergic system inexperimental animals has revitalized interest in identifying specificagents as possible causes of PD (Betarbet et al., 2000; Thiruchelvamet al., 2000). For example, Betarbet et al. (2000) reported thatchronic administration of a common herbicide, rotenone, resultedin a selective destruction of the nigrostriatal dopaminergic system,formation of cytoplasmic inclusions in nigral neurons, and inductionof hypokinesia and rigidity in rats, reproducing the key featuresof human PD. The selective toxicity for dopaminergic neurons inthe SN bestowed on rotenone has been attributed to its inhibitionof the activity of complex I of the mitochondrial respiratorychain and the unique vulnerability of dopaminergic neurons tooxidative damage as a result of mitochondrial complex I inhibition(Greenamyre et al., 1999; Jenner, 2001).

Microglia are the resident immune cells in the brain (Kreutzberg, 1996; Gonzalez-Scarano and Baltuch, 1999). Under normalconditions the microglia play a role in immune surveillance. Microglialactivation has been associated with neurodegeneration via theproduction of a variety of proinflammatory and neurotoxic factors,including tumor necrosis factor- $alpha$ (TNF $alpha$ ), interleukin-1 $beta$ (IL-1 $beta$ ),eicosanoids, nitric oxide (NO), and superoxide (Chao et al., 1992;Cassarino et al., 1997; Liu et al., 2000, 2001a; McGuire et al.,2001). Of the various factors released by activated microglia,reactive oxygen species such as superoxide free radical appearto play a key role in the inflammation-mediated oxidative damageto neurons. One of the major sources of superoxide is the activity-dependent,multi-component, and plasma membrane-associated NADPH oxidase(Babior, 1999). Because the midbrain area that encompasses theSN has the highest density of microglia in the brain (Lawson etal., 1990; Kim et al., 2000), microglial activation may be anearly event contributing to the degeneration of SN dopaminergicneurons as a consequence of a variety of oxidative insults. However,the role of microglia in rotenone-induced neurotoxicity has notbeenreported.

Using mesencephalic cultures, we report in this study that rotenone, at concentrations that were nontoxic to dopaminergicneurons in neuron-enriched cultures, induced selective degenerationof dopaminergic neurons in neuron/glia cultures. The rotenone-induceddopaminergic neurodegeneration was at least partially mediatedby the activation of microglia and the NADPH oxidase-mediatedrelease of superoxide freeradical.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. Cell culture ingredients were obtained from Invitrogen (San Diego, CA). [³H]dopamine (DA; 30 Ci/mmol) and GABA (90 Ci/mmol) were from NEN(Boston, MA). Monoclonal antibodies against the CR3 complementreceptor (OX-42) and microtubule-associated protein-2 (MAP-2)were from BD PharMingen (San Diego, CA) and Roche (Indianapolis,IN), respectively. The polyclonal anti-glial fibrillary acidicprotein (GFAP) antiserum and antibody diluent were from Dako (Carpinteria,CA). The polyclonal anti-tyrosine hydroxylase (TH) antiserum wasa gift from GlaxoWellcome (Research Triangle Park, NC). The monoclonalanti-neuron-specific nuclear protein (Neu-N) antibody was fromChemicon (Temecula, CA). The ED1 antibody and biotinylated isolectinwere from Serotec (Raleigh, NC) and Sigma (St. Louis, MO), respectively.The Vectastain avidin-biotin complex (ABC) kit and biotinylatedsecondary antibodies were from Vector Laboratories (Burlingame,CA). Dextran and Ficoll-Hypaque were from Amersham Pharmacia (Piscataway,NJ). Apocynin (Fluka, Milwaukee, WI) and diphenylene iodonium(DPI; Molecular Probes, Eugene, OR) were dissolved in ethanol(200 mM) or dimethylsulfoxide (20 mM) as stock solutions, respectively.Rotenone was purchased from Calbiochem (San Diego, CA). For eachexperiment a fresh stock solution of rotenone (10 mM) was preparedin dimethylsulfoxide, which was diluted further to desired finalconcentrations in treatment medium before use. All other reagentswere fromSigma.

Mesencephalic mixed neuron/glia cultures. Primary rat ventral mesencephalic neuron/glia cultures were prepared by followingour previously published protocol with modifications (Liu et al.,2000). Briefly, ventral mesencephalic tissues were dissected fromembryonic day 13/14 Fischer 344 rats and dissociated with a mildmechanical trituration. Cells were seeded to 24-well (5 × 10⁵/well) culture plates precoated with poly-D-lysine (20 µg/ml)and maintained in 0.5 ml/well of MEM supplemented with 10% heat-inactivatedfetal bovine serum (FBS) and 10% heat-inactivated horse serum(HS), 1 gm/l glucose, 2 mM L-glutamine, 1 mM sodium pyruvate,100 µM nonessential amino acids, 50 U/ml penicillin, and 50 µg/mlstreptomycin. Cultures were maintained at 37°C in a humidifiedatmosphere of 5% CO₂/95% air. Cultures were replenished with 0.5ml/well fresh medium 3 d later and were used for treatment 7 dlater. For treatment the cultures were maintained in 1 ml/wellof MEM containing 2% FBS, 2% HS, 2 mM L-glutamine, 1 mM sodiumpyruvate, 50 U/ml penicillin, and 50 µg/ml streptomycin. Immunocytochemicalanalysis indicated that, at the time of treatment, the cultureswere made up of ~12% OX-42-immunoreactive (IR) microglia, 48%GFAP-IR astrocytes, and 40% Neu-N-IR neurons of which 2.8-3.8%were TH-IRneurons.

Mesencephalic neuron-enriched cultures. Dissociated rat ventral mesencephalic cells were seeded first at 5 × 10⁵ cells/well into poly-D-lysine-coated 24-well culture plates asdescribed above. Then 2 d after initial seeding, cytosine $beta$ -D-arabinofuranoside(5-10 µM) was added to suppress the proliferation of glial cells.At 2-3 d later the cultures were changed back to fresh medium.Those 7-d-old cultures that contained <0.1% OX-42-IR microgliaand 8% GFAP-IR astrocytes were used for treatment. Of the Neu-N-IRneurons, 2.7-3.9% were TH-IR neurons. Alternatively, cells wereplated at 5 × 10⁵ cells/well into 24-well culture plates and maintained in DMEM/F12supplemented with 10% FBS, 6 gm/l glucose, 1× B27, 50 U/ml penicillin,and 50 µg/ml streptomycin (Lotharius et al., 1999). Then 2 d laterthe cultures were changed to serum-free Neurobasal medium containing1× B27, 0.5 mM L-glutamine, 0.01 µg/ml streptomycin, and 100 U/mlpenicillin. At 7 d after the initial plating the cultures consistedof 3% GFAP-IR astrocytes, <0.1% OX-42-IR microglia, and 96% Neu-N-IRneurons of which 2.9-3.8% were TH-IR neurons. Initial comparisonof the two aforementioned neuron-enriched cultures for responseto rotenone-induced neurotoxicity yielded identical results. Therefore,the neuron-enriched cultures prepared with the use of cytosine $beta$ -D-arabinofuranoside were used in subsequentexperiments.

Microglia-enriched cultures. Microglia were prepared from whole brains of 1-d-old Fischer 344 rats as described previously(Liu et al., 2001b). Briefly, brain tissues, devoid of meningesand blood vessels, were dissociated by a mild mechanical trituration.The isolated cells (5 × 10⁷) were seeded in 150 cm² culture flasks in DMEM/F12 containing 10% FBS, 2 mM L-glutamine,1 mM sodium pyruvate, 100 µM nonessential amino acids, 50 U/mlpenicillin, and 50 µg/ml streptomycin. The cultures were maintainedat 37°C in a humidified atmosphere of 5% CO₂/95% air, and themedium was changed 4 d later. On reaching confluence (12-14 d),the microglia were separated from astrocytes by shaking the flasksfor 5 hr at 180 rpm. The enriched microglia were >98% pure asdetermined by OX-42-IR and GFAP-IR.

Cell lines. The human monocytic U937 cells were obtained from American Type Culture Collection (Manassas, VA) and maintainedat 37°C in RPMI 1640 supplemented with 10% FBS, 50 U/ml penicillin,and 50 µg/ml streptomycin in a humidified incubator with 5% CO₂/95%air.

Preparation of rat neutrophils. Fresh blood was collected from the abdominal aorta of adult Fischer 344 male rats, and neutrophilswere purified by following the modified protocol of Wang et al.(1995). Briefly, heparinized blood was sedimented with dextran,and the neutrophils were isolated by centrifugation through theFicoll-Hypaque density gradient, followed by a hypotonic lysisto remove residual erythrocytes. Purified neutrophils (>95% viablecells, trypan blue exclusion) were resuspended in phenol red-freeHBSS and kept on ice untiluse.

Immunocytochemistry. Immunostaining was performed essentially as described previously (Kim et al., 2000; Liu et al., 2000).Neurons were stained with the anti-MAP-2 antibody to detect bothperikarya and neurites or the anti-Neu-N antibody to detect perikaryaonly. Dopaminergic neurons were detected with the anti-TH antibody.Astrocytes were recognized with the anti-GFAP antibody. Microgliawere detected with an anti-complement type 3 receptor antibody(OX-42), an anti-macrophage-specific glycoprotein antibody (ED1),or the biotinylated isolectin. Briefly, after blocking, formaldehyde-fixedcells were incubated overnight at 4°C with primary antibodiesdiluted in antibody diluent (anti-MAP-2, 1:400; anti-Neu-N, 1:2000;anti-TH, 1:20,000; OX-42, 5 µg/ml; ED-1, 1:250; biotinylated isolectin,13 µg/ml; or anti-GFAP, 1:1000). Except for biotinylated biotin,the bound primary antibody was visualized by incubation with anappropriate biotinylated secondary antibody, followed by the VectastainABC reagents and color development with 3,3'-diaminobenzidine.For double immunostaining, cultures were first stained with theanti-TH antibody and then with the anti-neu-N antibody followedby intensification using nickel sulfate. Images were recordedwith a CCD camera and the MetaMorph software (Universal ImagingSystems, West Chester, PA). For visual enumeration of the immunostainedcells in cultures, 10 representative areas per well were counted.For dopaminergic neurons the overall dendrite length for individualTH-IR neurons was measured by following our previously publishedprotocol (Liu et al., 2001c). Two to four wells of identical treatmentfrom each experiment and 50 TH-IR neurons per well were selectedfor measurement. Results were obtained from two separate experimentsand were expressed as a percentage of the controlcultures.

Uptake assays for tritiated DA or GABA. Cultures were washed two times with Krebs-Ringer buffer [containing (in mM) 16 sodiumphosphate, 119 NaCl, 4.7 KCl, 1.8 CaCl₂, 1.2 MgSO₄, 1.3 EDTA,and 5.6 glucose; pH 7.4]. For DA and GABA uptake the cultureswere incubated for 15 min at 37°C with 1 µM [³H]DA and 5 µM [³H]GABA in Krebs-Ringer buffer, respectively. After being washed(three times) with ice-cold Krebs-Ringer buffer, the cells werecollected in 1N NaOH, and radioactivity was counted with a liquidscintillation counter (Liu et al., 2000). Nonspecific uptake wasdetermined in parallel wells that received both the tritiatedtracer and 10 µM mazindol for DA uptake or 10 µM NO-711 for GABAuptake (Suzdak et al., 1992). In addition, for GABA uptake, comparableresults were obtained with the inclusion of $beta$ -alanine (1 mM),which preferentially affects glial GABA uptake (Mabjeesh et al.,1992).

Nitrite, TNF $alpha$ , and IL-1 $beta$ assays. The production of NO was determined by measuring the accumulated level of its stable metabolite,nitrite, in the supernatant with the Griess reagent (Green etal., 1982). The assay had a detection limit of ~0.5 µM. TNF $alpha$ orIL-1 $beta$ released into the culture medium was measured with respectiverat enzyme-linked immunosorbent assay kits from R&D Systems (Minneapolis,MN), with detection limits of 5 pg/ml, as described previously(Liu et al., 2000).

Measurement of superoxide production. The release of superoxide was determined by measuring the superoxide dismutase (SOD)-inhibitablereduction of cytochrome c as described previously (Chao et al.,1992; Liu et al., 2000). Primary microglia (0.5-1 × 10⁵/well) were grown overnight in 96-well plates in DMEM containing10% FBS. For superoxide assay the cultures were washed twice withHBSS and then maintained in 100 µl/well of phenol red-free HBSS.U937 monocytes or neutrophils were washed twice with HBSS andseeded (0.5-1 × 10⁵/well) in 100 µl/well in 96-well plates. Added to each well was50 µl of HBSS containing desired concentrations of drugs and withor without 800 U/ml SOD, immediately followed by 50 µl of 160µM ferricytochrome c in HBSS. The cultures were incubated for30 min at 37°C; the absorbance at 550 nm was read with a SpectraMaxPlus microplate spectrophotometer equipped with a solid-stateheated (37°C) chamber (Molecular Devices, Sunnyvale, CA). To determinethe effect of NADPH oxidase inhibitors on superoxide release,we preincubated the cells for 5 min with the vehicle or the inhibitorsbefore the addition of rotenone. The amount of SOD-inhibitablesuperoxide was calculated by using a molar extinction coefficientof 2.11 × 10⁴/M/cm for cytochrome c at 550 nm (Massy, 1959).

Statistical analysis. Statistical significance was assessed with an ANOVA, followed by the Bonferroni's t test via the StatViewprogram (Abacus Concepts, Berkeley, CA). A value of p < 0.05 wasconsidered statisticallysignificant.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The presence of glia dramatically increases the sensitivity of dopaminergic neurons to rotenone-induced neurodegeneration

Primary mixed neuron/glia or neuron-enriched cultures were treated for 8 d with the vehicle control (control group) or 0.5-30nM rotenone. [³H]DA uptake was measured to assess neurotoxicity to dopaminergicneurons. The treatment of neuron-enriched cultures with up to20 nM rotenone did not have any significant effect on [³H]DA uptake (Fig. 1A). Treatment of neuron-enriched cultures withhigher concentrations of rotenone resulted in a sudden drop in[³H]DA uptake, and a near-complete loss of DA uptake was seen incultures treated with 30 nM rotenone (Fig. 1A). In contrast, inmixed neuron/glia cultures a significant reduction in [³H]DA uptake was observed after treatment with 1 nM rotenone (Fig.1A). The decrease in DA uptake became more prominent with increasingconcentrations of rotenone, and a 50% reduction was seen in culturestreated with 10 nM rotenone (Fig. 1A). Counts of TH-IR neuronsindicated that no significant reduction in the number of TH-IRneurons was observed in neuron-enriched cultures after treatmentfor 8 d with up to 10 nM rotenone. However, a concentration-dependentdecrease in the number of TH-IR neurons was seen in neuron/gliacultures, with a 50% decrease in the cultures treated for 8 dwith 10 nM rotenone (Fig. 1B). Analysis of the time dependenceof rotenone-induced degeneration of dopaminergic neurons in neuron/gliacultures treated with 1-20 nM rotenone for 2-8 d demonstrateda time-dependent neurodegeneration (Fig. 1C). Although the reductionin DA uptake in cultures treated with 1 nM rotenone was only significant8 d later, a significant reduction was seen in cultures treatedwith $>=$ 20 nM rotenone as early as 2 d after treatment (Fig. 1C).The rapid onset of the rotenone-induced decrease in DA uptakeat the higher concentrations (20 and 25 nM) was likely attributableto its direct neurotoxicity as a consequence of the inhibitionof mitochondrial function.

View larger version (20K):
[in this window]
[in a new window]
Figure 1. Differential sensitivity of dopaminergic neurons in neuron-enriched and mixed neuron/glia mesencephalic cultures to rotenone-induced degeneration. A, B, Primary neuron-enriched or neuron/glia cultures were treated for 8 d with the vehicle (control group) or 1-30 nM rotenone; degeneration of dopaminergic neurons was evaluated with the [³H]DA uptake assay (A) or quantification of TH-IR neurons in the cultures (B). C, Mixed neuron/glia cultures were treated for 2-8 d with the vehicle or 1-25 nM rotenone; the [³H]DA uptake was determined at the desired time points. The amount of DA uptake for the vehicle-treated neuron/glia cultures at the time of treatment and 8 d after treatment was 0.77 ± 0.04 and 0.65 ± 0.06 and for vehicle-treated neuron-enriched cultures was 0.81 ± 0.07 and 0.77 ± 0.08 pmol/min per well, respectively. The results for DA uptake (A, C) and cell counts (B) are expressed as a percentage of the control cultures and are the mean ± SEM of four experiments performed in triplicate. *p < 0.01, compared with the control.

Glia-enhanced neurodegeneration is selective for dopaminergic neurons

One of the hallmarks of Parkinson's disease is the selective loss of dopaminergic neurons in the SN. Therefore, it is of particularinterest to determine whether the glia-enhanced neurodegenerationwas selective for dopaminergic neurons among the various neuronalpopulations in the mixed neuron/glia culture. First, the cultureswere treated with 1-25 nM rotenone for 8 d and then analyzed forthe uptake of [³H]DA or [³H]GABA. As shown in Figure 2A, although rotenone decreased [³H]DA uptake in a dose-dependent manner, [³H]GABA uptake in the cultures treated with up to 20 nM rotenonewas not affected significantly. The difference in neurotransmitteruptake was reduced markedly in cultures treated with 25 nM rotenone(Fig. 2A). Consistent with the effect observed with the uptakeassays, a quantification of immunostained neurons demonstratedthat rotenone dose-dependently reduced the number of TH-IR neuronsthat accounted for ~3.3% of the total neuronal population (Fig.2B). In contrast, no significant reduction in Neu-N-IR or MAP-2-IRneurons, which represented the majority if not all of the neurons,was observed in cultures treated with 20 nM rotenone for 8 d (Fig.2B). Again, a significant loss in Neu-N-IR or MAP-2-IR neuronswas seen in cultures treated with 25 nM rotenone for 8 d (Fig.2B). In addition to a reduction in cell numbers, TH-IR neuronsin rotenone-treated cultures displayed a less extensive dendriticnetwork compared with those in control cultures, whereas the dendriticnetwork of MAP-2-IR neurons, in general, was not affected significantly(Fig. 2C). Quantitation of the overall dendrite length of TH-IRneurons in the neuron/glia cultures demonstrated that, after treatmentfor 8 d with 10 and 20 nM rotenone, the average dendrite lengthreduced to 56.2 ± 6.6 and 30.0 ± 4.5% of that of the control cultures,respectively (p < 0.01 compared with control). In addition, double-labelimmunostaining for TH-IR and Neu-N-IR neurons further demonstratedthe selective destruction of dopaminergic neurons in rotenone-treatedneuron/glia cultures (Fig. 2C).

View larger version (45K):
[in this window]
[in a new window]
Figure 2. Selectivity of rotenone-induced neurodegeneration in mixed neuron/glia cultures. A, B, Mixed neuron/glia cultures were treated for 8 d with the vehicle or 5-25 nM rotenone. Afterward the cultures were assayed for uptake of [³H]DA or [³H]GABA (A) or were immunostained with anti-TH, Neu-N, or MAP-2 antibodies, followed by quantification of the positively stained cells (B). The amount of GABA uptake at the time of treatment and 8 d after treatment for the vehicle-treated neuron/glia cultures was 39.4 ± 4.2 and 35.2 ± 3.2 pmol/min per well, respectively. The number of Neu-N-IR, MAP-2-IR, and TH-IR neurons in the control cultures was ~490, 460, and 14/mm². The results are expressed as a percentage of the control cultures and are the mean ± SEM of three experiments performed in triplicate. *p < 0.01, compared with the control. C, Immunocytochemical analysis. Mixed neuron/glia cultures were treated for 8 d with the vehicle or 10 or 20 nM rotenone. Cultures then were immunostained for TH-IR, Neu-N-IR, or MAP-2-IR neurons or were double stained for TH-IR and Neu-N-IR neurons. Scale bars: TH-IR and Neu-N-IR neurons, 50 µm; MAP-IR neurons, 100 µm; neurons in the TH and Neu-N double-immunostained cultures, 75 µm.

The addition of microglia to neuron-enriched cultures significantly increases the sensitivity of dopaminergic neurons to rotenone-induced neurotoxicity

The vast difference in sensitivity of dopaminergic neurons to rotenone neurotoxicity between the mixed neuron/glia and neuron-enrichedcultures prompted us to speculate that the neurotoxicity of rotenonewas dependent on the presence of glia, especially that of microglia.To test this hypothesis directly, we added cells from primarymicroglia-enriched cultures to mesencephalic neuron-enriched cultures;DA uptake of neuronal cultures and microglia-supplemented neuronalcultures was compared after treatment with 10 nM rotenone for8 d. As shown in Figure 3, whereas the DA uptake of the neuron-enrichedcultures was not affected by the addition of microglia (2.5-7.5× 10⁴/well), the addition of microglia significantly increased thesensitivity of dopaminergic neurons to rotenone-induced neurotoxicity.The increase in sensitivity to rotenone neurotoxicity positivelycorrelated with the number of microglia added to the neuron-enrichedcultures (Fig. 3). For example, the addition of 5 × 10⁴ microglia/well to neuron-enriched cultures, a level comparablewith that observed in mixed neuron/glia cultures, reduced theirDA uptake to 46% of the control cultures (Fig. 3), close to thedegree of reduction observed in mixed neuron/glia cultures treatedwith 10 nM rotenone for 8 d (Fig. 1A). In contrast, after treatmentfor 8 d with 10 nM rotenone, no significant difference was detectedin GABA uptake between the neuron-enriched cultures (96 ± 2% ofcontrol) and those with 7.5 × 10⁴ microglia added per well (93% ± 4% of control, from two experimentsperformed in triplicate). These data further strengthen the notionthat microglia play a pivotal role in dictating the sensitivityand selectivity of dopaminergic neurons to rotenone-induced degeneration.

View larger version (36K):
[in this window]
[in a new window]
Figure 3. Effect of the addition of microglia to neuron-enriched cultures on rotenone-induced degeneration of dopaminergic neurons. Neuron-enriched mesencephalic cultures were supplemented with 2.5-7.5 × 10⁴ microglia/well. At 24 hr later the cultures were treated with the vehicle or 10 nM rotenone, and DA uptake was determined 8 d after the treatment. The results are expressed as a percentage of the control cultures and are the mean ± SEM of three experiments performed in triplicate. *p < 0.01, compared with the control.

Rotenone-induced microglial activation precedes neurodegeneration

To study further the role of microglia in the rotenone-induced preferential and enhanced degeneration of dopaminergic neurons,we first examined whether rotenone could activate microglia inthe mixed neuron/glia cultures. Microglial activation is characterizedby dramatic changes in morphology and increased expression ofsurface antigens such as the complement type 3 receptor (Kreutzberg,1996). Cultures were treated for 1 d with 10 nM rotenone, andmicroglia were detected with the antibody OX-42 that recognizesthe complement receptor. Compared with control cultures, a significantportion of the OX-IR microglia in rotenone-treated cultures waslarger in size than those in control cultures (Fig. 4A). Moreprominently, the number of immunoreactive microglia in the rotenone-treated(1-10 nM) cultures increased significantly over that in the controlcultures (Fig. 4B). A significant increase in OX-IR cells wasseen in cultures that were treated for 1 d with 1 nM rotenone,and a 67% increase over the control cultures was observed with10 nM rotenone (Fig. 4B). Similar results were obtained when thecultures were immunostained for other specific markers of microgliawith isolectin and the antibody ED-1 (Fig. 4B). These resultsdemonstrated that rotenone was capable of inducing microglialactivation, which preceded the degeneration of dopaminergic neuronsin the mixed neuron/glia cultures.

View larger version (63K):
[in this window]
[in a new window]
Figure 4. Effect of rotenone on microglial activation. Mixed neuron/glia cultures were treated for 1 d with the vehicle or 1-10 nM rotenone and then were immunostained with antibodies against specific markers of microglia. A, Immunocytochemical analysis with the OX-42 antibody of cultures treated for 1 d with the vehicle or 10 nM rotenone. In control cultures a significant portion of the OX-IR resting microglia was small and round (open arrowheads). After treatment with 10 nM rotenone, OX-42-IR microglia were enlarged significantly and were irregularly shaped (filled arrowheads), indicative of activation. Part of the images of OX-42-IR microglia (in closed boxes, a and b) presented in A was cut out and presented in B for better representation of the differences. C, Quantification of microglial activation. Vehicle or rotenone-treated cultures were immunostained with OX-42, ED-1, or isolectin; positively stained microglia were counted. The number of OX-42-IR microglia in the control cultures was ~120/mm². The results are expressed as a percentage of the control cultures and are the mean ± SEM of three experiments performed in triplicate. *p < 0.01, compared with the control. Scale bar, 50 µm.

Rotenone induces NADPH oxidase-mediated release of superoxide from activated microglia

Activated microglia secrete a variety of proinflammatory and cytotoxic factors such as the cytokines TNF $alpha$ and IL-1 $beta$ and freeradical NO and the reactive oxygen species (ROS), which work inconcert to induce neurodegeneration. We first measured the accumulationof nitrite (an indicator of NO production), TNF $alpha$ , or IL-1 $beta$ inmedia from neuron/glia cultures after treatment with the vehicleor 1-20 nM rotenone for 1-8 d. However, the quantities of thesefactors in either vehicle- or rotenone-treated cultures were ator below the detection limits for the assays that were used (TNF $alpha$ ,5 pg/ml; IL-1 $beta$ , 5 pg/ml; NO, 0.5 µM).

Next, we examined the release of superoxide free radical from microglia by measuring the SOD-inhibitable reduction of cytochromec. After incubation of microglia for 30 min with vehicle or 1-10nM rotenone, a dose-dependent release of superoxide was observed(Fig. 5A). Significant release of superoxide was detected in microgliatreated with 5 or 10 nM rotenone. Similar profiles for superoxiderelease were observed in the human monocytic U937 cells that areof close lineage to macrophage and microglia (Fig. 5A). Becausethe main source of superoxide released is dependent on the activityof the membrane-associated NADPH oxidase that is expressed mostabundantly in neutrophils (Griendling et al., 2000), we next testedthe effect of rotenone on the release of superoxide from rat neutrophils.Indeed, significant release of superoxide was detected in neutrophilsafter treatment with concentrations of rotenone as low as 1 nM(Fig. 5A). The involvement of the activity of NADPH oxidase inrotenone-induced release of superoxide was determined by examiningthe effects of two mechanistically dissimilar inhibitors of NADPHoxidase, DPI and apocynin, with the former directly inhibitingthe catalytic activity of the enzyme (Irani et al., 1997) andthe latter preventing the assembly of the multi-subunit enzymecomplex (Stolk et al., 1994). As shown in Figure 5B, both DPI(2.5-5 µM) and apocynin (0.25-0.5 mM) significantly inhibitedthe rotenone-induced release of superoxide from neutrophils. Theseresults demonstrated that the rotenone-induced release of superoxidefree radical involved the activity of NADPH oxidase.

View larger version (25K):
[in this window]
[in a new window]
Figure 5. Rotenone stimulated the release of superoxide. A, Rat primary microglia, human monocytic U937 cells, or rat neutrophils were seeded to 96-well plates. Cells were treated with the vehicle or 1-10 nM rotenone. Superoxide production, measured as SOD-inhibitable cytochrome c reduction, was determined as described in Materials and Methods. The results are a percentage of the control cultures and are expressed as the mean ± SEM of three experiments performed in triplicate. *p < 0.01, compared with the control. B, Effect of NADPH oxidase inhibitors on rotenone-induced release of superoxide from neutrophils. Neutrophils were pretreated for 5 min with the vehicle or indicated concentrations of DPI or apocynin before treatment with 10 nM rotenone. Then the amount of superoxide released was determined as described in Materials and Methods. The results are a percentage of the control cultures and are expressed as the mean ± SEM of three experiments performed in triplicate. *p < 0.01, compared with rotenone-treated cells. C, Control; Rot, rotenone; APO, apocynin.

The relevance of rotenone-stimulated superoxide release in mediating microglia-induced facilitation of dopaminergic neurodegenerationwas established by the observation that neutralization of thereactivity of superoxide or inhibition of NADPH oxidase affordedneuroprotection. As shown in Figure 6, the addition of a combinationof SOD (50 U/ml) and catalase (50 U/ml) to the neuron/glia culturesright before and 24 hr after the addition of rotenone significantlyreduced rotenone-induced damage to dopaminergic neurons. Neutralizationof superoxide by SOD/catalase increased the DA uptake of culturestreated with 5 and 10 nM rotenone from 76 and 53% of the controlcultures to 93 and 74% of the control cultures, respectively (Fig.6). Pretreatment of neuron/glia cultures with 1 mM NG-nitro-L-argininemethyl ester, an inhibitor of nitric oxide synthase, did not affordany significant neuroprotection (data not shown). However, pretreatmentof neuron/glia cultures with an inhibitor of NADPH oxidase, apocynin,before treatment with rotenone significantly attenuated the rotenone-induceddegeneration of dopaminergic neurons measured either by [³H]DA uptake (Fig. 7A) or counts of TH-IR neurons (Fig. 7B). Theneuroprotective effect of apocynin was concentration-dependentover a range of 0.1-0.5 mM (Fig. 7C). Unexpectedly, treatmentof cultures for 8 d with DPI (0.1-5 µM) resulted in significantdamage to neurons in the culture (data not shown). Despite this,the results obtained with SOD/catalase and apocynin strongly suggestedthat NADPH oxidase-mediated production of superoxide in microgliaunderlies microglial facilitation of the rotenone-induced dopaminergicneurodegeneration.

View larger version (18K):
[in this window]
[in a new window]
Figure 6. Effect of SOD/catalase on rotenone-induced degeneration of dopaminergic neurons. SOD/catalase (50 U/ml each) were added to neuron/glia cultures right before and 24 hr after the addition of the indicated concentrations of rotenone. The cultures were assayed for [³H]DA uptake 8 d later. The results are the mean ± SEM of three experiments performed in triplicate. *p < 0.01, compared with the control.

View larger version (21K):
[in this window]
[in a new window]
Figure 7. Effect of apocynin on rotenone-induced degeneration of dopaminergic neurons. A, B, Neuron/glia cultures were pretreated for 30 min with the vehicle or 0.25 mM apocynin before treatment with 5 or 10 nM rotenone. Then 8 d later the degeneration of dopaminergic neurons was assessed as [³H]DA uptake (A) and counts of TH-IR neurons (B). C, Neuron/glia cultures were pretreated for 30 min with the vehicle or the indicated concentration of apocynin before treatment with 10 nM rotenone. The cultures were assayed for [³H]DA uptake 8 d later. The results are the mean ± SEM of three experiments performed in triplicate. *p < 0.01 and ⁺p < 0.05, compared with the control.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Using primary rat mesencephalic mixed neuron/glia and neuron-enriched cultures, this study for the first time demonstratesthat microglia are actively involved in the rotenone-induced selectivedegeneration of dopaminergic neurons. At concentrations (1-15nM) that are nontoxic to dopaminergic neurons in the neuron-enrichedcultures, the presence of microglia in the mixed neuron/glia culturesenables rotenone to induce significant and selective degenerationof dopaminergic neurons. The dramatically enhanced dopaminergicneurodegeneration is primarily attributable to the rotenone-inducedactivation of microglia and their release of superoxide free radicalas demonstrated by the measured SOD-inhibitable reduction of cytochromec, the neuroprotective effect of SOD/catalase, and that of theNADPH oxidase inhibitorapocynin.

Microglia, the resident immune cells in the brain, play a pivotal role in the detection of invading pathogens, host defense,and tissue repair (Kreutzberg, 1996; Aloisi, 1999). In responseto injury or immunological challenges, microglia become readilyactivated and undergo dramatic changes in morphology, surfaceexpression of molecules such as major histocompatibility complex,and the complement type 3 receptor, recognizable by the antibodyOX-42 (Streit et al., 1988). Furthermore, activated microgliaproduce a wide array of immunomodulatory and cytotoxic factors,including TNF $alpha$ , IL-1 $beta$ , eicosanoids, NO, and superoxide free radical.Although a few of these factors are thought to contribute to tissuerepair (Streit et al., 1988), a majority are believed to workvia mechanisms not yet fully understood to induce neurodegeneration(McGeer et al., 1988; Chao et al., 1992; Jeohn et al., 1998; Minghettiand Levi, 1998; Liu et al., 2001a).

Numerous studies have suggested that, among the factors produced by activated microglia, oxygen free radicals play a prominentrole in the degeneration of dopaminergic neurons. For example,stimulation of mesencephalic neuron/glia cultures with the bacterialendotoxin activated microglia to produce TNF $alpha$ , IL-1 $beta$ , NO, andsuperoxide (Kim et al., 2000; Liu et al., 2000). However, inhibitionof microglial production of superoxide, but not the other factors,was most effective in protecting neurons, indicating that superoxidewas a dominant degenerative factor for the dopaminergic neuronsin the culture (Liu et al., 2000). In the current study the rotenone-induceddegeneration of dopaminergic neurons in neuron/glia cultures may,at least in part, be attributable to the activation of microgliaand NADPH oxidase-mediated release of superoxide free radical.This notion is supported by the following observations: (1) significantaccumulation of NO was not observed, and inhibition of NO productiondid not afford neuroprotection; (2) although their participationin neurotoxicity could not be ruled out completely, the accumulatedlevels of IL-1 $beta$ or TNF $alpha$ were very low, and studies have shownthat sufficient quantities of these factors, possibly even incombination with other factors (e.g., NO), are necessary to inducesignificant neurotoxicity (Jeohn et al., 1998); (3) significantrelease of superoxide, as measured by the SOD-inhibitable reductionof cytochrome c, was detected in rotenone-stimulated microgliaas well as monocytes and neutrophils (Fig. 5A); (4) the rotenone-inducedrelease of superoxide was sensitive to inhibitors of NADPH oxidaseDPI and apocynin (Fig. 5B); and (5) significant protection ofdopaminergic neurons in the mixed neuron/glia cultures againstrotenone-induced degeneration was achieved by the superoxide scavengersSOD and catalase and the NADPH oxidase inhibitor apocynin (Figs.6, 7). NADPH oxidase is expressed widely in cells of the mesodermallineage, including leukocytes and vascular cells (Babior, 1999).It is made up of at least seven subunits that are distributedbetween the cytosol and plasma membranes. In response to stimulithe cytosolic components, especially the p47 subunit, undergoextensive phosphorylation, and the entire group of cytosolic subunits(p40, p47, and p67) translocate to become associated with themembrane-bound heterodimeric cytochrome b₅₅₈, composed of gp91and p22. Two small G-proteins, Rac-1 and Rap1A, also are involvedin the activation process of NADPH oxidase. The assembly of afully functional NADPH oxidase catalyzes the transfer of electronsfrom NADPH to molecular oxygen, resulting in the generation ofsuperoxide. It is believed that neutrophils and other immune cellsgenerate superoxide as part of a repertoire to kill invading pathogens.In vascular and cardiac cells, NADPH oxidase-generated superoxidemay be involved in cell signaling pathways (Griendling et al.,2000). Excessive and/or unintended activation of NADPH oxidasemay result in tissue damage. It is, therefore, of tremendous significanceto decipher the precise interaction between rotenone and membersof the NADPH oxidase in relation to its stimulation of superoxiderelease frommicroglia.

It is worth noting that, although apocynin has been considered an effective inhibitor of the oxidative burst by blocking theassembly of the NADPH oxidase complex (Simons et al., 1990; Stolket al., 1994), the neuroprotective effect of apocynin observedin this study (Fig. 7) may not be attributed exclusively to theinhibition of NADPH oxidase-mediated superoxide generation. Theobservation that SOD and catalase afforded only a partial neuroprotectionalso lends support to this notion. In other words, rotenone maybe capable of inducing the release of additional neurotoxic factorsfor which the identities are not yetdisclosed.

Oxygen free radicals are highly reactive and can interact with proteins, DNA, or RNA to alter their functions or induce lipidperoxidation, leading to eventual cell death (Facchinetti et al.,1998). Among the various populations of neurons in the brain,dopaminergic neurons in the SN are uniquely vulnerable to oxidativestress (Jenner and Olanow, 1998; Greenamyre et al., 1999). Theelevated sensitivity of dopaminergic neurons to oxidative damageso far has been attributed in large part to their known reducedantioxidant capacity, increased accumulation of iron, and theconcentration of neurochemicals such as dopamine that are proneto oxidative modification. However, of particular relevance tothe current study are the reports that nonmitochondria-originatedfree radicals can, at least in vitro, impair complex I selectivelyand possibly trigger a self-amplifying cycle of additional freeradical generation (Turrens and Boveris, 1980; Hasegawa et al.,1990). In others words the mixed neuron/glia culture system ofthe current study may be a reflection of the microenvironmentin the brain: dopaminergic neurons may be under the dual assaultof oxygen free radicals generated by rotenone-activated microgliaand that generated as a consequence of the inhibition, by rotenone,of the mitochondrial complex I activity. Hence, it is plausibleto speculate the existence of a potential amplification mechanismfor superoxide generation in dopaminergic neurons as a consequenceof the exposure of both microglia and dopaminergic neurons torotenone. These observations, together with the fact that thenigral region has the highest concentration of microglia amongthe major brain regions that have been examined (Lawson et al.,1990; Kim et al., 2000), may be part of the mechanisms underlyingthe selective destruction of dopaminergic neurons in the SN afterrotenone treatment (Betarbet et al., 2000; Foley and Riederer,2000), although the exact mechanism remains to be understoodfully.

It should be pointed out that, in this study, in neuron-enriched cultures treated with 20-30 nM rotenone a sudden drop inthe viability of dopaminergic neurons was observed (Fig. 1A).This reflects an important characteristic of rotenone workingas a mitochondrial complex I inhibitor. Studies have shown thatrotenone at between 25 and 30 nM will inhibit complex I activitysignificantly, which, in turn, will lead to a decrease in themitochondrial membrane potential that is lethal to dopaminergicneurons (Greenamyre et al., 1999). Therefore, at these concentrationsof rotenone, direct inhibition of neuronal mitochondrial complexI activity and the resultant decrease in mitochondrial membranepotential may have become the predominant force in determiningthe fate of dopaminergic neurons. However, exposure to concentrationsof rotenone as low as 1 nM, which is at least 20 times lower thanthe critical concentration(s) needed to impair mitochondrial complexI activity directly, may be more relevant, at least in vitro,to the degeneration of dopaminergicneurons.

The present study using in vitro mesencephalic cultures provides important clues to our understanding of the rotenone-induceddopaminergic neurodegeneration. Continuing exploration of therole of microglia should further our quest to identify the environmentalfactors such as pesticides as potential factors involved in thepathogenesis of Parkinson'sdisease.

  FOOTNOTES

Received Oct. 1, 2001; revised Oct. 30, 2001; accepted Nov. 7, 2001.

We thank Dr. Jerome L. Maderdrut for reading thismanuscript.
Correspondence should be addressed to Bin Liu, F1-01, National Institute of Environmental Health Sciences, P.O. Box 12233,Research Triangle Park, NC 27709. E-mail: liu3{at}niehs.nih.gov.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aloisi F (1999) The role of microglia and astrocytes in CNS immune surveillance and immunopathology. Adv Exp Med Biol 468:123-133[ISI][Medline].
Babior BM (1999) NADPH oxidase: an update. Blood 93:1464-1476[Free Full Text].
Betarbet R, Sherer TB, MacKenzie G, Garcia-Osuna M, Panov AV, Greenamyre JT (2000) Chronic systemic pesticide exposure reproduces features of Parkinson's disease. Nat Neurosci 3:1301-1306[ISI][Medline].
Cassarino DS, Fall CP, Swerdlow RH, Smith TS, Halvorsen EM, Miller SW, Parks JP, Parker Jr WD, Bennett Jr JP (1997) Elevated reactive oxygen species and antioxidant enzyme activities in animal and cellular models of Parkinson's disease. Biochim Biophys Acta 1362:77-86[Medline].
Chao CC, Hu S, Molitor TW, Shaskan EG, Peterson PK (1992) Activated microglia mediate neuronal cell injury via a nitric oxide mechanism. J Immunol 149:2736-2741[Abstract].
de Silva HR, Khan NL, Wood NW (2000) The genetics of Parkinson's disease. Curr Opin Genet Dev 10:292-298[Medline].
Facchinetti F, Dawson VL, Dawson TM (1998) Free radicals as mediators of neuronal injury. Cell Mol Neurobiol 18:667-682[ISI][Medline].
Foley P, Riederer P (2000) Influence of neurotoxins and oxidative stress on the onset and progression of Parkinson's disease. J Neurol 247[Suppl 2]:II82-II94.
Gonzalez-Scarano F, Baltuch G (1999) Microglia as mediators of inflammatory and degenerative diseases. Annu Rev Neurosci 22:219-240[ISI][Medline].
Gorell JM, Johnson CC, Rybicki BA, Peterson EL, Richardson RJ (1998) The risk of Parkinson's disease with exposure to pesticides, farming, well water, and rural living. Neurology 50:1346-1350[Abstract/Free Full Text].
Green LC, Wagner DA, Glogowski J, Skipper PL, Wishnok JS, Tannenbaum SR (1982) Analysis of nitrate, nitrite, and [¹⁵N]nitrate in biological fluids. Anal Biochem 126:131-138[ISI][Medline].
Greenamyre JT, MacKenzie GM, Peng T-I, Stephans SE (1999) Mitochondrial dysfunction in Parkinson's disease. Biochem Soc Symp 66:85-97[Medline].
Griendling KK, Sorescu D, Ushio-Fukai M (2000) NAD(P)H oxidase: role in cardiovascular biology and disease. Circ Res 86:494-501[Abstract/Free Full Text].
Hasegawa E, Takasgige K, Oishi T, Murai Y, Minikami S (1990) 1-Methyl-4-phenylpyridinium (MPP+) induces NADH-dependent superoxide formation and enhances NADH-dependent lipid peroxidation in bovine heart submitochondrial particles. Biochem Biophys Res Commun 170:1049-1055[ISI][Medline].
Herishanu YO, Medvedovski M, Goldsmith JR, Kordysh E (2001) A case-control study of Parkinson's disease in an urban population of southern Israel. Can J Neurol Sci 28:144-147[ISI][Medline].
Irani K, Xia Y, Zweier JL, Sollott SJ, Der CJ, Fearon ER, Sundaresan M, Finkel T, Goldschmidt-Clermont PJ (1997) Mitogenic signaling mediated by oxidants in Ras-transformed fibroblasts. Science 275:1649-1652[Abstract/Free Full Text].
Jenner P (2001) Parkinson's disease, pesticides, mitochondrial dysfunction. Trends Neurosci 24:245-247[ISI][Medline].
Jenner P, Olanow CW (1998) Understanding cell death in Parkinson's disease. Ann Neurol 44:S72-S84[ISI][Medline].
Jeohn GH, Kong LY, Wilson B, Hudson P, Hong JS (1998) Synergistic neurotoxic effects of combined treatments with cytokines in murine primary mixed neuron/glia cultures. J Neuroimmunol 85:1-10[ISI][Medline].
Kim WG, Mohney RP, Wilson B, Jeohn GH, Liu B, Hong JS (2000) Regional difference in susceptibility to lipopolysaccharide-induced neurotoxicity in the rat brain: role of microglia. J Neurosci 20:6309-6316[Abstract/Free Full Text].
Kreutzberg GW (1996) Microglia: a sensor for pathological events in the CNS. Trends Neurosci 19:312-318[ISI][Medline].
Langston JW (1998) Epidemiology versus genetics in Parkinson's disease: progress in resolving an age-old debate. Ann Neurol 44:S45-S52[ISI][Medline].
Lawson LJ, Perry VH, Dri P, Gordon S (1990) Heterogeneity in the distribution and morphology of microglia in the normal adult mouse brain. Neuroscience 39:151-170[ISI][Medline].
Liu B, Du L, Hong JS (2000) Naloxone protects rat dopaminergic neurons against inflammatory damage through inhibition of microglia activation and superoxide generation. J Pharmacol Exp Ther 293:607-617[Abstract/Free Full Text].
Liu B, Gao HM, Wang J-Y, Jeohn G-H, Cooper CL, Hong JS (2001a) Role of nitric oxide in inflammation-mediated neurodegeneration. Ann NY Acad Sci, in press.
Liu B, Wang K, Gao HM, Mandavilli B, Wang JY, Hong JS (2001b) Molecular consequences of activated microglia in the brain: overactivation induces apoptosis. J Neurochem 77:182-189[ISI][Medline].
Liu B, Qin L, Yang SN, Wilson BC, Liu Y, Hong JS (2001c) Femtomolar concentrations of dynorphins protect rat mesencephalic dopaminergic neurons against inflammatory damage. J Pharmacol Exp Ther 298:1133-1141[Abstract/Free Full Text].
Lotharius J, Dugan LL, O'Malley KL (1999) Distinct mechanisms underlie neurotoxin-mediated cell death in cultured dopaminergic neurons. J Neurosci 19:1284-1993[Abstract/Free Full Text].
Mabjeesh NJ, Frese M, Rauen T, Jeserich G, Kanner BI (1992) Neuronal and glial $gamma$ -aminobutyric acid⁺ transporters are distinct proteins. FEBS Lett 299:99-102[ISI][Medline].
Massy V (1959) The microestimation of succinate and the extinction coefficient of cytochrome c. Biochim Biophys Acta 24:255-265.
McGeer PL, Itagaki S, Boyes BE, McGeer EG (1988) Reactive microglia are positive for HLA-DR in the substantia nigra of Parkinson's and Alzheimer's disease brains. Neurology 38:1285-1291[Abstract/Free Full Text].
McGuire SO, Ling ZD, Lipton JW, Sortwell CE, Collier TJ, Carvey PM (2001) Tumor necrosis factor alpha is toxic to embryonic mesencephalic dopamine neurons. Exp Neurol 169:219-230[ISI][Medline].
Minghetti L, Levi G (1998) Microglia as effector cells in brain damage and repair: focus on prostanoids and nitric oxide. Prog Neurobiol 54:99-125[ISI][Medline].
Olanow CW, Tatton WG (1999) Etiology and pathogenesis of Parkinson's disease. Annu Rev Neurosci 22:123-144[ISI][Medline].
Polymeropoulos MH (1998) Autosomal dominant Parkinson's disease. J Neurol 245[Suppl 3]:P1-P3[ISI][Medline].
Priyadarshi A, Khuder SA, Schaub EA, Priyadarshi SS (2001) Environmental risk factors and Parkinson's disease: a metaanalysis. Environ Res 86:122-127[Medline].
Ritz B, Yu F (2000) Parkinson's disease mortality and pesticide exposure in California, 1984-1994. Int J Epidemiol 29:323-329[Abstract/Free Full Text].
Simons JM, Hart BA, Ip Vai Ching TR, Van Dijk H, Labadie RP (1990) Metabolic activation of natural phenols into selective oxidative burst agonists by activated human neutrophils. Free Radic Biol Med 8:251-258[ISI][Medline].
Stolk J, Hiltermann TJ, Dijkman JH, Verhoeven AJ (1994) Characteristics of the inhibition of NADPH oxidase activation in neutrophils by apocynin, a methoxy-substituted catechol. Am J Respir Cell Mol Biol 11:95-102[Abstract].
Streit WJ, Graeber MB, Kreutzberg GW (1988) Functional plasticity of microglia: a review. Glia 1:301-307[ISI][Medline].
Suzdak PD, Frederiksen K, Andersen KE, Sorensen PO, Knutsen LJ, Nielsen EB (1992) NNC-711, a novel potent and selective $gamma$ -aminobutyric acid uptake inhibitor: pharmacological characterization. Eur J Pharmacol 224:189-198[ISI][Medline].
Thiruchelvam M, Richfield EK, Baggs RB, Tank AW, Cory-Slechta DA (2000) The nigrostriatal dopaminergic system as a preferential target of repeated exposures to combined paraquat and maneb: implications for Parkinson's disease. J Neurosci 20:9207-9214[Abstract/Free Full Text].
Turrens JF, Boveris A (1980) Generation of superoxide anion by the NADH dehydrogenase of bovine heart mitochondria. Biochem J 191:421-427[ISI][Medline].
Wang JP, Raung SL, Kuo YH, Teng CM (1995) Daphnoretin-induced respiratory burst in rat neutrophils is, probably, mainly through protein kinase C activation. Eur J Pharmacol 288:341-348[ISI][Medline].

Copyright © 2002 Society for Neuroscience 0270-6474/02/223782-09$05.00/0

This article has been cited by other articles:

X. Hu, D. Zhang, H. Pang, W. M. Caudle, Y. Li, H. Gao, Y. Liu, L. Qian, B. Wilson, D. A. Di Monte, et al.
Macrophage Antigen Complex-1 Mediates Reactive Microgliosis and Progressive Dopaminergic Neurodegeneration in the MPTP Model of Parkinson's Disease
J. Immunol., November 15, 2008; 181(10): 7194 - 7204.
[Abstract] [Full Text] [PDF]

J. Z. Guan, T. Maeda, M. Sugano, J.-i. Oyama, Y. Higuchi, T. Suzuki, and N. Makino
A Percentage Analysis of the Telomere Length in Parkinson's Disease Patients
J. Gerontol. A Biol. Sci. Med. Sci., May 1, 2008; 63(5): 467 - 473.
[Abstract] [Full Text] [PDF]

M.-J. Wang, S.-Z. Lin, J.-S. Kuo, H.-Y. Huang, S.-F. Tzeng, C.-H. Liao, D.-C. Chen, and W.-F. Chen
Urocortin Modulates Inflammatory Response and Neurotoxicity Induced by Microglial Activation
J. Immunol., November 1, 2007; 179(9): 6204 - 6214.
[Abstract] [Full Text] [PDF]

H. Klintworth, K. Newhouse, T. Li, W.-S. Choi, R. Faigle, and Z. Xia
Activation of c-Jun N-Terminal Protein Kinase Is a Common Mechanism Underlying Paraquat- and Rotenone-Induced Dopaminergic Cell Apoptosis
Toxicol. Sci., May 1, 2007; 97(1): 149 - 162.
[Abstract] [Full Text] [PDF]

M. P. Mount, A. Lira, D. Grimes, P. D. Smith, S. Faucher, R. Slack, H. Anisman, S. Hayley, and D. S. Park
Involvement of Interferon-{gamma} in Microglial-Mediated Loss of Dopaminergic Neurons
J. Neurosci., March 21, 2007; 27(12): 3328 - 3337.
[Abstract] [Full Text] [PDF]

W. Zhang, E.-J. Shin, T. Wang, P. H. Lee, H. Pang, M.-B. Wie, W.-K. Kim, S.-J. Kim, W.-H. Huang, Y. Wang, et al.
3-Hydroxymorphinan, a metabolite of dextromethorphan, protects nigrostriatal pathway against MPTP-elicited damage both in vivo and in vitro
FASEB J, December 1, 2006; 20(14): 2496 - 2511.
[Abstract] [Full Text] [PDF]