Abstract
The cause of Parkinson's disease (PD) is unknown, but epidemiological studies suggest an association with pesticides and other environmental toxins, and biochemical studies implicate a systemic defect in mitochondrial complex I. We report that chronic, systemic inhibition of complex I by the lipophilic pesticide, rotenone, causes highly selective nigrostriatal dopaminergic degeneration that is associated behaviorally with hypokinesia and rigidity. Nigral neurons in rotenone-treated rats accumulate fibrillar cytoplasmic inclusions that contain ubiquitin and α-synuclein. These results indicate that chronic exposure to a common pesticide can reproduce the anatomical, neurochemical, behavioral and neuropathological features of PD.
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Parkinson's disease is a late-onset, progressive motor disease marked by selective degeneration of dopaminergic neurons of the substantia nigra and formation of fibrillar cytoplasmic inclusions, known as Lewy bodies, which contain ubiquitin and α-synuclein1. Rare cases of familial PD have been linked to mutations in α-synuclein or parkin2,3,4, but the cause of the more commonly encountered sporadic disease is unknown, and the role of genetics in these cases is uncertain5. Post mortem studies strongly implicate oxidative damage and mitochondrial impairment in the pathogenesis of PD6. Epidemiological studies have suggested that pesticide exposure is associated with an increased risk of developing PD7,8,9.
After the pro-toxin N-methyl-4-phenyl-1,2,3,6-tetrahydropyridine (MPTP) was reported to produce in humans an acute parkinsonian syndrome that is virtually indistinguishable from idiopathic PD10, its metabolite, 1-methyl-4-pyridinium (MPP+), was found to be a mitochondrial poison that inhibits mitochondrial respiration at complex I of the electron transport chain11,12. The selectivity of MPP+ for dopaminergic neurons is due to the fact that it is an excellent substrate for the dopamine transporter, and is thereby accumulated preferentially in cells that transport dopamine13. Following recognition of MPTP's toxicity and its mechanism of action, several laboratories reported a selective defect in complex I of the electron transport chain in PD14,15,16,17,18,19,20,21,22. This defect seems to be systemic, affecting not only the brain, but also peripheral tissues such as platelets.
An accurate in vivo experimental model of PD should reproduce the progressive, selective nigrostriatal dopaminergic degeneration and Lewy body formation seen in PD, test the relevance of the systemic complex I defect, and explain the potential involvement of pesticide exposure in development of parkinsonism. Unfortunately, no current animal model incorporates all of these features. The MPTP model causes selective nigrostriatal degeneration by inhibiting complex I, but, unlike PD, MPTP does not cause a systemic complex I defect. Instead, the inhibition is highly selective for dopaminergic neurons. Moreover, MPTP does not typically produce cytoplasmic inclusions that closely resemble Lewy bodies23. Transgenic mice expressing the pathogenic human α-synuclein mutation develop modest dopaminergic pathology (although the specificity of this degeneration is not detailed), and many neurons contain small cytoplasmic inclusions that are granular rather than fibrillar24.
To develop a more accurate in vivo model of PD, we exposed rats chronically, continuously and systemically to the common pesticide, rotenone. A naturally occurring compound derived from the roots of certain plant species, rotenone is commonly used as an insecticide in vegetable gardens, and is also used to kill or sample fish populations in lakes and reservoirs. It is widely believed to be a safe, natural alternative to synthetic pesticides. Rotenone is also a well characterized, high-affinity, specific inhibitor of complex I, one of the five enzyme complexes of the inner mitochondrial membrane involved in oxidative phosphorylation. Because it is extremely hydrophobic, rotenone crosses biological membranes easily, and it does not depend on the dopamine transporter for access to the cytoplasm. Therefore, rotenone—unlike MPTP—is well-suited to produce a systemic inhibition of complex I.
Results
Sprague-Dawley and Lewis rats were infused continuously with rotenone by a jugular vein cannula attached to a subcutaneous osmotic minipump. Lewis rats showed less variability and more consistent lesions than Sprague-Dawley rats25 and were used exclusively after completion of pilot studies. Initially, rotenone was infused at doses ranging from 1 to 12 mg/kg per day for various lengths of time. High doses of rotenone for short periods of time produced systemic (cardiovascular) toxicity and non-specific brain lesions, as reported by others26 (M.F. Beal and J. Shulz, personal communication). Downward titration of rotenone dosing resulted in less systemic illness and highly specific dopaminergic degeneration. The optimal dose for inducing the pathology of PD was determined to be 2–3 mg/kg per day in Lewis rats, and animals were euthanized after 7 days to more than 5 weeks of continuous treatment. In the study presented here, 25 rats were infused with rotenone in this dose range, and 12 demonstrated clear nigrostriatal dopaminergic lesions; no vehicle-treated rats had lesions.
Rotenone infusion affected complex I selectively. Enzymatic activities of succinate dehydrogenase (complex II) and cytochrome oxidase (complex IV), analyzed histochemically27, were not affected by rotenone infusion. In animals treated systemically with rotenone, [3H]dihydrorotenone binding to complex I in brain28 was reduced by about 75% (Fig. 1a). Systemically administered rotenone acted on complex I uniformly throughout the brain, consistent with its ability to cross biological membranes easily. Based on the affinities of rotenone and dihydrorotenone for complex I, a 75% inhibition of specific binding translates to a free rotenone concentration of 20–30 nM in the brain28. This concentration is known to partially inhibit complex I activity29. However, oximetry analysis indicated that in brain mitochondria—but not liver mitochondria—this level of complex I inhibition was insufficient to inhibit glutamate-supported respiration (Fig. 1b).
Selective nigrostriatal dopaminergic degeneration
Systemic partial inhibition of complex I resulted in progressive nigrostriatal dopaminergic degeneration. Immunocytochemistry of phenotypic markers for dopaminergic neurons (tyrosine hydroxylase, TH; dopamine transporter, DAT; vesicular monoamine transporter type 2, VMAT2) all gave identical results, indicating dopaminergic degeneration. Depending on the dose and duration of rotenone exposure, animals demonstrated varying degrees of striatal dopaminergic denervation (Fig. 2b–d). Lesions typically began focally in the central or dorsolateral portion of the anterior striatum, as evidenced by a complete loss of phenotypic markers, and spread to involve most of the motor striatum. Even when striatal TH depletion was almost complete, there was relative sparing of dopaminergic fibers in medial aspects of striatum, nucleus accumbens and olfactory tubercle (Fig. 2d), areas that are relatively spared in idiopathic PD30.
There was also evidence of dopaminergic lesions in the cell bodies of the substantia nigra pars compacta. Animals with partial reductions in TH staining in striatum had dopaminergic neurons in substantia nigra that looked relatively normal (Fig. 2f and g); however, in animals with near complete striatal denervation, there were obvious reductions in TH-stained cells in substantia nigra (Fig. 2h). These results suggest that striatal nerve terminals were affected earlier and more severely by rotenone than nigral cell bodies. Similarly, in brains of dying patients with PD, there is a more profound loss of dopamine in striatum compared to substantia nigra31. Neurons in the lateral portion and ventral tier of the substantia nigra pars compacta were most vulnerable to systemic rotenone infusion (Fig. 2h). This pattern of vulnerability matches the pattern in idiopathic PD. Despite the loss of TH staining in substantia nigra, dopaminergic neurons of the ventral tegmental area (VTA) were relatively spared, as they are in PD. Moreover, just as in idiopathic PD, noradrenergic neurons of the locus ceruleus were mildly to moderately affected (data not shown).
To confirm that the loss of staining of dopaminergic neurons and nerve terminals was due to degeneration rather than reduced expression of phenotypic markers by surviving cells, silver staining was done alone and in combination with TH immunostaining. In the striatum, regions of degeneration densely stained with silver corresponded to areas where there was loss of TH staining (Fig. 3a and b). In the substantia nigra, there was also clear degeneration. Although animals treated with vehicle never showed nigral degeneration (Fig. 3c), animals with partial loss of striatal dopamine terminals had many nigral neurons with silver deposits in their cell bodies or dendrites, interspersed with neurons that looked normal (Fig. 3d and e). Thus, although nigral TH staining was relatively normal in animals with partial denervation of striatum, silver staining revealed degenerative changes. Animals with severe dopaminergic denervation of striatum had extensive silver deposition in substantia nigra corresponding to the loss of phenotypic markers in this region (Fig. 3f). Silver staining also confirmed the progressive, retrograde nature of dopaminergic degeneration in the rotenone model. In an animal that survived for two weeks beyond the end of rotenone infusion, there was no longer silver staining in the region of striatum depleted of dopaminergic markers. Presumably, this was due to previous phagocytosis of degenerating neuronal elements. However, in this animal, there was massive silver deposition in substantia nigra (data not shown). Silver staining also showed that there was no consistent neuronal degeneration elsewhere in the brains of rotenone-treated animals. For example, there was no silver staining in the cortex in Fig. 3b. Although we never saw silver staining in control animals, there was the possibility that silver deposition could reflect protein aggregation in the absence of frank degeneration. Therefore, the neuronal degeneration was confirmed in rotenone-infused animals with Fluoro-Jade B histochemistry. Fluoro-Jade B is a fluorescein derivative that selectively stains neurons undergoing degeneration32. Vehicle-infused animals had no Fluoro-Jade B-positive neurons in substantia nigra (Fig. 3g); however, there were numerous Fluoro-Jade B-positive neurons in substantia nigra of rotenone-infused animals (Fig. 3h). Together, silver staining and Fluoro-Jade B histochemistry conclusively demonstrated selective degeneration of nigrostriatal dopamine neurons in rotenone-infused animals.
Despite the profound loss of presynaptic dopaminergic nerve terminals in striatum, postsynaptic neuronal elements in striatum remained intact. Nissl staining, though relatively insensitive in striatum, did not show obvious lesions of striatal neurons (data not shown). More than 90% of striatal neurons use γ-aminobutyric acid as their transmitter, and they can be identified with immunocytochemistry for glutamic acid decarboxylase (GAD). In striatal regions lacking dopaminergic terminals, there was no loss of GAD immunoreactivity (Fig. 4a–d). Thus, the predominant cell type in striatum seemed to be intact in rotenone-treated animals. This is in direct contrast to what occurs when complex II—rather than complex I—is inhibited systemically. Animals treated systemically with the complex II inhibitor, 3-nitropropionic acid, display selective degeneration of striatal neurons with relative sparing of the nigrostriatal dopamine system33. An additional smaller population of striatal neurons is cholinergic, and can be assessed with acetylcholinesterase (AChE) staining34. Striatal AChE staining was similar in vehicle- and rotenone-treated animals (Fig. 4e and f). These results further support the nigrostriatal dopaminergic selectivity of rotenone-induced neurodegeneration.
Cytoplasmic inclusions reminiscent of Lewy bodies
Rats with dopaminergic degeneration had cytoplasmic inclusions in nigral neurons. These inclusions shared some features of the Lewy bodies associated with PD1. With hematoxylin and eosin staining, pale eosinophilic inclusions were seen that resembled the 'pale body' precursors to Lewy bodies (Fig. 5a and b). With light microscopy, we saw some nigral neurons that also showed aggregates (usually 1–4 μm in diameter) containing ubiquitin (Fig. 5c) and α-synuclein (Fig. 5d and e). Electron microscopy showed electron-dense cytoplasmic inclusions (1–2 μm in diameter) in the cytoplasm of nigral neurons (Fig. 5f); such inclusions were frequently clustered in the cytoplasm. Ultrastructural features included a homogeneous dense core surrounded by fibrillar elements similar to those seen in Lewy bodies. Some of the inclusions had a more granular appearance, like those described in α-synuclein transgenic mice24. By immuno-electron microscopy, we saw that these inclusions contained α-synuclein immunoreactivity (Fig. 5f, inset). We did not find neuronal inclusions in rotenone-treated animals that did not have dopaminergic lesions as assessed by TH staining.
Parkinsonian behavior
Initial characterization of this model focused on delineating the biochemical, molecular and anatomical pathology of rotenone-induced degeneration. However, rotenone-treated animals developed motor and postural deficits characteristic of PD, the severity of which depended on the extent of lesions. All animals with a dopaminergic lesion became hypokinetic and had unsteady movement and hunched posture, even after termination of the rotenone infusion. Seven animals developed severe rigidity, and three animals had shaking of one or more paws that was reminiscent of rest tremor. Preliminary experiments in two animals indicate that the motor deficits were ameliorated by the dopamine agonist, apomorphine (data not shown).
Discussion
Taken together, our results indicate that a systemic partial defect in complex I is enough to reproduce the behavioral, anatomical, neurochemical and neuropathological features of PD. The finding that rotenone affected complex I uniformly throughout the brain (Fig. 1a), coupled with the resultant highly selective neurodegeneration of the nigrostriatal dopaminergic system, suggested that this population of neurons had an intrinsic sensitivity to complex I defects. Because the brain rotenone concentration (20–30 nM) was enough to partially inhibit complex I, but too low to significantly impair respiration of brain mitochondria, it seemed that a bioenergetic defect with ATP depletion could not explain the neurodegneration. Instead, oxidative damage might have been involved. Inhibition of complex I by rotenone stimulates production of reactive oxygen species35,36. Moreover, we have found that culture of neural cells with 5 nM rotenone induces, over a period of weeks, progressive oxidative damage to proteins and DNA, and sensitizes cells to subsequent oxidative stressors; eventually, it also begins to induce release of cytochrome c from mitochondria to the cytoplasm (Sherer et al., Soc. Neurosci. Abstr. 26, 280.21, 2000). This mechanism could also explain the cytoplasmic inclusions found in nigral neurons of rotenone-treated rats, because both oxidative damage and cytochrome c enhance α-synuclein aggregation37,38.
Rotenone seems to have little toxicity when administered orally (T. B. S. and J. T. G., unpublished results); however, our results highlight the possibility that environmental toxins, including pesticides that inhibit mitochondrial function, may contribute to the pathogenesis of PD. Many other naturally occurring compounds and synthetic pesticides are potent inhibitors of complex I39. Individuals are likely to be variably exposed to numerous natural or synthetic complex I inhibitors through diet, drinking water or other environmental factors. Such exposures, combined with genetic differences in complex I function14,15,16,17,18,19,20,21,22, or inter-individual differences in the ability to metabolize xenobiotics7, may underlie most cases of typical idiopathic PD.
Methods
Animal surgery.
We used male Sprague Dawley and Lewis rats (300–350 g; approximately 2 months old) for this study. Alzet osmotic mini pumps (models 2ML4 or 2ML1) were filled with rotenone, dissolved in equal volumes of dimethylsulfoxide (DMSO) and polyethylene glycol (PEG). Pumps were attached to Tygon microbore (0.58 mm i.d.) tubing (Fisher Scientific, Pittsburgh, Pennsylvania) and placed in sterile 0.9% saline at 37°C for at least 4 h. Ketamine (75 mg/kg) and Rompum (10 mg/kg) were injected intramuscularly for anesthetic. Alzet osmotic mini pumps were implanted under the skin on the back of each animal, and the right jugular vein was cannulated. Pumps were exchanged after 28 days. Control rats received DMSO:PEG (1:1) only. Following surgery, rats were monitored for behavior, weight loss and overall health. In the instances when rotenone-treated rats began to lose weight, diet was supplemented with oral administration of Nutrical (Evsco Pharmaceuticals, Buena, New Jersey). Subcutaneous lactated Ringer's injection USP solution (Baxter Healthcare Corporation, Deerfield, Illinois) was given when rats showed signs of dehydration.
Mitochondrial respiration.
Oxygen consumption by rat brain and liver mitochondria was measured polargraphically as described40 using an Instech minichamber (Instech Laboratories, Plymouth Meeting, Pennsylvania) equipped with a magnetic stirrer and oxygen electrode (Yellow Spring Instrument Company, Yellow Springs, Ohio) connected to a chart recorder. For maximum State 3 respiration activity, the following medium was used: 125 mM KCl, 10 mM MOPS, 2 mM MgCl2, 2 mM KH2PO4, 1 mM EGTA, 0.7 mM CaCl2, 20 mM glucose, 8 units of hexokinase, and 20 mM glutamate plus 2 mM malate. Brain mitochondria were isolated by the method of Sims41 without BSA, because BSA binds rotenone nonspecifically.
Immunocytochemistry.
We used paraformaldehyde-fixed brains. For single immunolabeling studies, 40-μm sections were incubated in primary antibody for 24 h, followed by 1 h incubation with biotinylated secondary antibody. The avidin-biotin complex method was used to detect the antigen signal (ABC elite kit, Vector laboratories, Burlingame, California) and 3,3′-diaminobenzidine tetrachloride (DAB) was used to visualize the final product. The primary antibodies used were monoclonal mouse antibody against TH (1:2000; Chemicon, Temecula, California), polyclonal rabbit antibody against ubiquitin (1:1000; Dako Corporation, Carpinteria, California) and polyclonal rabbit antibody against α-synuclein (1:400). Secondary antibodies used were biotinylated goat anti-mouse immunoglobulin G (IgG) or biotinylated goat anti-rabbit IgG (1:200; Jackson Immunoresearch Labs, West Grove, Pennsylvania). Double labeling for TH and GAD was performed by immunofluorescence. Sections were simultaneously incubated with antibodies against TH (1:2000; Chemicon) and GAD (1:2000; polyclonal rabbit antibody; Chemicon) for 24 h. Texas red-conjugated goat anti-mouse IgG was used to detect TH-positive cells and fluorescein isothiocyanate-conjugated goat anti-rabbit IgG was used to detect GAD- expressing cells (1:200; Jackson Immunoresearch Labs). For controls, one or both primary antibodies were omitted. We examined immunostained sections using bright-field microscopy or conventional fluorescence microscopy. We captured images on a Leitz microscope (Leica, Wetzlar, Germany) linked to an image analysis system (Imaging Research, St. Catharines, Ontario, Canada) with selective filter sets to visualize FITC and Texas red separately, as well as simultaneously. For final output, images were processed using Adobe Photoshop 5.0 software.
Detection of neuronal degeneration.
Both silver staining and Fluoro-Jade B histochemistry were used to detect degenerating neurons. The FD Neurosilver kit (FD NeuroTechnologies, Ellicott City, Maryland) stained degenerating neuronal elements in paraformaldehyde-fixed brain tissue from control and rotenone-infused rats. Silver staining was done according to the manufacturer's protocol. Following silver staining, sections were mounted on Superfrost plus slides (Fisher Scientific, Pittsburgh, Pennsylvania), air-dried, cleared with xylene, and coverslipped with Permount. Sections were examined using bright-field microscopy. TH-immunostained sections were also processed for silver staining to demonstrate selective neurodegeneration. Fluoro-Jade B histochemistry was done on paraformaldehyde-fixed brain sections from control and rotenone-infused rats according to the manufacturer's protocol (Histo-Chem, Jefferson, Arkansas).
Electron microscopy.
Paraformaldehyde-fixed brain sections from four rats were processed for standard electron microscopy. The tissue was post-fixed in osmium tetroxide and embedded in epon. Ultra-thin sections were stained with uranyl acetate and lead citrate and examined with a Hitachi (Mountain View, California) electron microscope. For immuno-electron microscopy, sections stained for α-synuclein using DAB as chromophore were fixed with 0.5% glutaraldehyde and processed for routine electron microscopy as described.
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Acknowledgements
We thank P. Piccardo and B. Ghetti for donation of the α-synuclein antibody, which was generated with support from the Indiana Alzheimer's Disease Center (P30AG10133). We also thank M. DeLong and A. Levey for reading this manuscript. This work was supported by NIH grants to JTG (NS38399, NS33779, and AG14648).
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Betarbet, R., Sherer, T., MacKenzie, G. et al. Chronic systemic pesticide exposure reproduces features of Parkinson's disease. Nat Neurosci 3, 1301–1306 (2000). https://doi.org/10.1038/81834
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DOI: https://doi.org/10.1038/81834