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The Journal of Neuroscience, August 15, 2001, 21(16):6069-6076
The Activation of Dopamine D4 Receptors Inhibits Oxidative Stress-Induced Nerve Cell Death
Kumiko Ishige, Qi Chen, Yutaka Sagara, and David Schubert Cellular Neurobiology Laboratory, The Salk Institute for Biological Studies, La Jolla, California 92037
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Oxidative stress is thought to be the cause of nerve cell death in many CNS pathologies, including ischemia, trauma, and neurodegenerative disease. Glutamate kills nerve cells that lack ionotropic glutamate receptors via the inhibition of the cystine-glutamate antiporter x
, resulting in the inhibition of cystine uptake, the loss of glutathione, and the initiation of an oxidative stress cell death pathway. A number of catecholamines were found to block this pathway. Specifically, dopamine and related ligands inhibit glutamate-induced cell death in both clonal nerve cell lines and rat cortical neurons. The protective effects of dopamine, apomorphine, and apocodeine, but not epinephrine and norepinephrine, are antagonized by dopamine D4 antagonists. A dopamine D4 agonist also protects, and this protective effect is inhibited by U101958, a dopamine D4 antagonist. Although the protective effects of some of the catecholamines are correlated with their antioxidant activities, there is no correlation between the protective and antioxidant activities of several other ligands. Normally, glutamate causes an increase in reactive oxygen species (ROS) and intracellular Ca2+. Apomorphine partially inhibits glutamate-induced ROS production and blocks the opening of cGMP-operated Ca2+ channels that lead to Ca2+ elevation in the late part of the cell death pathway. These data suggest that the protective effects of apomorphine on oxidative stress-induced cell death are, at least in part, mediated by dopamine D4 receptors via the regulation of cGMP-operated Ca2+ channels. Key words: HT22 cells; cell death; apomorphine; apocodeine; dopamine D4 receptors; glutamate; cGMP
INTRODUCTION
Dopamine and its five receptor subtypes play diverse roles in the CNS. Their activation is thought to adversely contribute to several neuropathological disorders, including Parkinson's disease and schizophrenia (Seeman and Van Tol, 1994
; Sokoloff and Schwartz, 1995
HT22 cells are immortalized mouse hippocampal cells and can be considered a model of oxidative toxicity on exposure to glutamate. HT22 cells have no ionotropic glutamate receptors (Maher and Davis, 1996
MATERIALS AND METHODS
Materials. The oligonucleotides were purchased from Sigma-Genosys (The Woodlands, TX). The chemicals used were: [3H]spiperone (specific activity 610.5 GBq/mmol; NEN, Boston, MA); dopamine receptor D4 affinity purified polyclonal antibody (Chemicon, Temecula, CA); 2',7'-dichlorofluorescein diacetate (DCF), indo-acetoxymethylester (Indo-1), pluronic F-127, and propidium iodode (all from Molecular Probes, Eugene, OR); haloperidol and L745870 (Tocris Cookson, Ballwin, MO); and 8-(4-clorophenylthio) cGMP (pCPT-cGMP), apomorphine, apocodeine, PD168077, U101958, dopamine, and spiperone (Sigma, St. Louis, MO).
Cell culture and 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide assay. The HT22 cells were propagated in DMEM that was supplemented with 10% fetal bovine serum (FBS). Cell survival was determined by the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay. MTT is taken up by recycling vesicles in which it is reduced and cycled to the extracellular space (Liu et al., 1997
Total antioxidant activity assay. Total antioxidant activity was measured using the procedure described by Miller et al., (1993)
GSH, ROS, and Ca2+ measurements. Total GSH was measured as described by Tan et al. (1998a)
Reverse transcription polymerase chain reaction. Total RNA was prepared from HT22 cells and various tissues of mice and then treated with DNase for 30 min at 15°C. Oligonucleotide primers used for the PCR amplification were: D4-1, 5'-CCTTACCCAGCCTCCGGACGA-3', which corresponds to nucleotides 764-784 of the mouse D4 receptor sequence; and D4-2, 5'-GACACGAAGCAAGCCGGACA-3', which is complementary to nucleotides 1018-1037 of the same sequence. PCR products were electrophoresed on 2% agarose gels and detected by ethidium bromide.
Western blotting. HT22 cells were collected by scraping in sample buffer. Mouse tissues were homogenized with a Polytron (Kinematica, Basel, Switzerland) for 20 sec in PBS supplemented with a mixture of protease inhibitors (Complete; Roche Molecular Biochemicals, Indianapolis, IN), and then centrifuged at 48,000 × g for 30 min at 4°C. The resulting pellets were resuspended in sample buffer (3% SDS, 1% glycerol, 0.5% 2-mercaptoethanol, 0.05% bromophenol blue, and 80 mM Tris-HCl buffer, pH 6.8, with Complete protease inhibitors). The samples were heated for 3 min in boiling water, fractionated on 12% polyacrylamide gels, and electroblotted onto membranes. Dopamine receptor D4 affinity purified polyclonal antibody was used as the primary antibody. Immunoreactive bands were detected with the ECL (Amersham Pharmacia Biotech, Arlington Heights, IL) Western blotting detection reagents.
Binding assays. HT22 cells were homogenized with a Polytron for 20 sec in 15 ml of 50 mM Tris-HCl buffer, pH 7.4, containing 1 mM EDTA, and then centrifuged at 48,000 × g for 30 min at 4°C. The resulting pellet, which constitutes the membrane fraction, was resuspended in 50 mM Tris-HCl buffer, pH 7.4. Binding assays were performed as described by Maroto et al. (1995)
Statistical analysis. The significance of differences between two groups was assessed by Student's t test. The significance of three or more groups was assessed by the Bonferroni test.
RESULTS
Effect of dopamine and related compounds on glutamate-induced cell death
Because there have been suggestions in the literature that catecholamines can protect nerve cells from oxidative stress (Noh et al., 1999
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Figure 1. Protective effects of apomorphine and related compounds on glutamate-induced cell death in HT22 cells and primary cortical cells. HT22 (A) and 1-d-old primary cortical (B) cells were incubated with various drugs and 2.5 mM or 5 mM glutamate, respectively, for 20 hr; then cell survival was measured by the MTT assay. The results are presented as the mean ± SEM relative percentage survival for three or four independent experiments each done in triplicate. AM, Apomorphine (1 µM). **p < 0.01 (vs no glutamate); ##p < 0.01 (vs glutamate alone).
To confirm the data with the MTT assay and to visually present the dramatic effects of the dopamine analogs on rescuing the cells from glutamate toxicity, some of the conditions in Figure 1 were repeated with the cell viability stain calcein AM. Calcein AM is a fluorogenic esterase substrate that passes through the cell membrane and is hydrolyzed inside the viable cell to the green fluorescent product calcein (Vaughan et al., 1995
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Figure 2. Viability assays using calcein AM. Cells were treated as described below, and viability was determined 20 hr later using calcein AM instead of MTT. A, Quantitation of viable cells. Twenty microscopic fields containing between 0 and 80 (control) cells each were scored for viable calcein-positive cells, and the average cells per field in the control (untreated) cultures was given as 100%. The data are presented as the mean cell number relative to control ± SEM. Cont., Control; Glu, 2.5 mM glutamate; AC, 10 µM apocodeine; PD, 50 µM PD168077; AM, 1 µM apomorphine; L74, 3 µM L745870; cGMP, 2.5 mM pCPT-cGMP. The last three columns were from a separate experiment than the first six. B, Photomicrographs of calcein-stained HT22 cell cultures after treatment with the reagents described in A and Figure 1. The conditions are those described in A. a, Control; b, glutamate; c, glutamate plus apocodeine; d, glutamate plus PD168077; e, glutamate plus apomorphine; f, glutamate plus apomorphine plus L745870; g, control; h, pCPT-cGMP; i, pCPT-cGMP plus apomorphine.
Because apomorphine and apocodeine are ligands for dopamine receptors (Van Tol et al., 1991
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Figure 3. Inhibitory effects of D4 antagonists on the neuroprotective effects by apomorphine and related compounds. A, HT22 cells were incubated with glutamate (2.5 mM) and apomorphine (AM; 1 µM), apocodeine (AC; 1 µM), dopamine (DA; 30 µM), epinephrine (EP; 100 µM), or norepinephrine (NE; 100 µM) in the presence or absence of the D4 antagonists, L745870 (3 µM) or U101958 (10 µM), for 20 hr; then cell survival was measured by the MTT assay. B, HT22 cells were incubated with 2.5 mM glutamate and 50 µM PD168077 in the presence or absence of 10 µM U101958 for 20 hr; then cell survival was measured by the MTT assay. The results are presented as the mean ± SEM relative percentage survival for three independent experiments. **p < 0.01 (vs control, no glutamate); ##p < 0.01 (vs glutamate alone); #p < 0.05 (vs glutamate alone); @p < 0.05 (vs glutamate in each group). The statistical analysis was performed with the Bonferroni test.
Antioxidant activity (TEAC)
It is possible that at least a part of the neuroprotection by apomorphine and related compounds is attributable to their antioxidant activity (Yoshikawa et al., 1994
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Table 1. TEAC values
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Figure 4. Relationship between the TEAC values and protective effects on glutamate-induced cell death in HT22 cells. TEAC values were obtained from Table 1. EC50 values for suppression of 2.5 mM glutamate-induced cell death in HT22 cells were calculated from each concentration-response curve and are presented as the mean of three or four independent experiments. AM, Apomorphine; AC, apocodeine; PD, PD168077; DA, dopamine; SKF, SKF38393; DP, 7-hydroxy-dipropylaminotetralin (7-OH-DPAT); N, norepinephrine; E, epinephrine; HT, serotonin.
Glutathione, ROS and Ca2+ levels
Oxidative glutamate toxicity is associated with the depletion of GSH and the elevation of intracellular ROS and Ca2+ (Tan et al., 1998a
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Figure 5. The effects of apomorphine, apocodeine, and dopamine on glutathione (GSH) depletion, reactive oxygen species (ROS) production, and Ca2+ influx by glutamate. Cells were incubated with 2.5 mM (GSH) or 5 mM (GSH, ROS, and Ca2+) glutamate and each drug for 8 hr; then GSH, ROS and Ca2+ were measured as described in Materials and Methods. GSH was calculated as nanomoles GSH per milligram of protein and presented as a percentage of the control value. ROS and Ca2+ were calculated as described in Materials and Methods and presented as a percentage of control. All results are presented as the mean ± SEM for four independent experiments. -, Control; AM, apomorphine; AC, apocodeine; DA, dopamine. **p < 0.01 (vs no glutamate); #p < 0.05 and ##p < 0.01 (vs 5 mM Glu).
cGMP induced Ca2+ influx
In HT22 cells and cortical neurons, cGMP-dependent Ca2+ channels are opened near the end of the glutamate-induced cell death pathway (Li et al., 1997b
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Figure 6. Effects of dopamine receptor ligands on cGMP-induced cell death in HT22 cells and primary cortical neurons. HT22 (A) or 1-d-old cultured cortical (B) cells were incubated with CoCl2 (50 µM), apomorphine (AM; 1 µM), apocodeine (AC; 1 µM), dopamine (DA; 30 µM), or PD168077 (PD; 50 µM), followed by the addition of 2.5 mM pCPT-cGMP. Cell survival was measured by the MTT assay 24 hr later. C, Glutamate was added to all samples at 0 time, and 20 µM CoCl2, 1 µM apocodeine, 50 µM PD168077, 1 µM apocodeine plus 3 mM L745870 or 0.1 µg/ml actinomycin D were added at 2 hr intervals up to 10 hr; cell viability was determined after 20 hr. The results are presented as the mean ± SEM relative percentage survival for three independent experiments. *p < 0.05 and **p < 0.01 (vs no glutamate); #p < 0.05 and ##p < 0.01 (vs 5 mM glutamate).
If dopamine and its analogs protect cells primarily via the inhibition of Ca2+ influx, then it would be predicted that they protect cells from glutamate toxicity when added very late in the cell death program in which the Ca2+ influx occurs (Li et al., 1997b
Dopamine receptors in HT22 cells
The above experiments suggest that HT22 cells have dopamine D4 receptors that mediate the protective response. Three sets of experiments were done to determine whether the HT22 cells express the D4 receptor. D4 receptor mRNA was assayed by reverse transcription polymerase chain reaction (RT-PCR), Western blot experiments were performed to examine protein levels, and ligand binding assays were performed to examine receptor function. In RT-PCR, amplification with D4-1 and D4-2 primers generated a 195 bp cDNA fragment from the HT22 cells, mouse hippocampal RNA, and mouse cortical neuron RNA (Fig. 7A). The corresponding band was not detected in mouse liver or kidney. Similarly, Western blots with an antibody specific to D4 receptors showed that HT22 cells, mouse hippocampal membranes, and mouse cortical neurons have dopamine D4 receptors (Fig. 7AII). In the liver and kidney, this band was not observed. The molecular weight of these proteins was estimated at 55 kDa. These data show that HT22 cells and the tissue from which they were derived, mouse hippocampus, both express D4 receptors.
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Figure 7. The expression of D4 receptors in HT22 cells. A, RT-PCR and Western blot analysis of dopamine D4 receptors in HT22, hippocampal, and cortical cells. DNase-treated total RNA with (+) or without (-) reverse transcription was amplified by PCR. The estimated size of the PCR products was 195 bp. II, Lanes of HT22 cell lysates contained 40 µg of protein, and the other lanes contained 20 µg of protein. The estimated molecular weight of the D4 receptor is 55 kDa in HT22 and hippocampal neurons and slightly larger in cortical neurons. B, Representative Scatchard plot of [3H]spiperone binding. The binding assay was performed as described in Materials and Methods by using concentrations of spiperone between 0.5 nM and 2.5 µM. C, Displacement curves for [3H]spiperone binding. The binding assay was performed as described in Materials and Methods. The results are presented as the mean ± SEM of three to five independent experiments. IC50 values are shown in Table 3.
To further characterize the dopamine D4 receptors in HT22 cells, we performed binding assays. Scatchard plots for the dopamine receptor antagonist [3H]spiperone binding to HT22 cells are curvilinear (Fig. 7C), fitting a two site binding model. As shown in Table 2, the Kd values for high- and low-affinity sites are 7.21 ± 0.56 nM and 466 ± 177 nM, respectively, and the Bmax values are 28.88 ± 13.08 pmol/mg protein and 174.02 ± 51.99 pmol/mg protein, respectively. Displacement experiments showed that various nonselective and D4-selective ligands inhibited [3H]spiperone binding (Fig. 7C, Table 3). The most effective displacing agent was spiperone, followed by haloperidol. The IC50 value for apomorphine was almost the same as that of apocodeine. The displacing potency of dopamine was the same or weaker than that of the D4 ligands, U101958, L745870, and PD168077.
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Table 2. Kd and Bmax values for [3H]spiperone binding
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Table 3. IC50 values for [3H]spiperone binding
DISCUSSION
The above data show that the activation of dopamine D4 receptors can play a role in the protection of nerve cells from oxidative stress-induced cell death. This conclusion is based on the following observations. (1) Apomorphine, apocodeine, and dopamine all protect the HT22 mouse hippocampal nerve cell line and rat cortical neurons from oxidative stress induced by oxidative glutamate toxicity (Figs. 1, 2). (2) This protective effect is reversed by D4 antagonists, but not by D1, D2, or D3 antagonists (Fig. 3). (3) A selective D4 agonist, PD168077, also protects neurons from oxidative stress (Figs. 1, 2). (4) The protective effects of the D4 agonists cannot be explained by their inherent antioxidant properties alone (Fig. 4, Table 1). (5) HT22 cells express the mRNA, protein, and physiological binding properties of D4 dopamine receptors (Fig. 7, Tables 2, 3).
It has been suggested that the neuroprotective effects of catecholamines, including dopamine, epinephrine, and norepinephrine are attributable to their antioxidant activities and are not receptor-mediated (Grünblatt et al., 1999
It is also known that exogenous dopamine can be neurotoxic. Dopamine is degraded to hydrogen peroxide and dihydroxyphenylacetaldehyde by monoamine oxidase or spontaneously oxidizes to form quinones, semiquinones, and again hydrogen peroxide. Several of these products can lead to the generation of reactive oxygen species such as hydroxyl radicals. Therefore, there has been considerable interest in the potential role of dopamine in CNS ischemia and trauma. Indeed it has been established in several in vivo models that dopamine is involved in the cell death pathway. For example, when brain lesions are caused by malonate or 3-nitropropionic acid, two reagents that inhibit energy metabolism, the experimental reduction of dopamine greatly diminishes the extent of damage (Reynolds et al., 1998
The mouse dopamine D4 receptor mRNA is found in the hippocampus and other brain regions, and also in some peripheral tissues such as the adrenal gland and the testes (Van Tol et al., 1991
Binding assays also show that dopamine D4 receptors are expressed in the HT22 cells and that apomorphine and apocodeine bind the receptors with higher affinities than dopamine. These data agree with those that show that although apomorphine is a nonselective dopamine receptor agonist, its affinity for D4 receptors is severalfold higher than that of dopamine (Seeman and Van Tol, 1994
A great deal is understood about the programmed cell death pathway initiated by glutamate in HT22 cells and primary cortical neurons (Maher and Davis, 1996
FOOTNOTES Received April 23, 2001; revised April 23, 2001; accepted May 31, 2001.
This work was supported by a Nihon University grant to K.I., the Bundy Foundation Fellowship to Q.C., and grants from the United States Department of Defense (DAMD 17-991-1-9562) and the National Institutes of Health to D.S. We thank Drs. Pamela Maher, Richard Dargusch, and Shirlee Tan for their comments on this manuscript.
Correspondence should be addressed to Dr. David Schubert, The Salk Institute for Biological Studies, 10010 North Torrey Pines Road, La Jolla, CA 92037. E-mail: schubert{at}salk.edu.
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