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Previous Article | Next Article
The Journal of Neuroscience, March 1, 2003, 23(5):1688
Impaired Spinal Cord Glutamate Transport Capacity and Reduced Sensitivity to Riluzole in a Transgenic Superoxide Dismutase Mutant Rat Model of Amyotrophic Lateral Sclerosis
John Dunlop1, H. Beal McIlvain1, Yijin She2, and David S. Howland2 1 Neuroscience and 2 Molecular Genetics, Wyeth Research, Princeton, New Jersey 08543-8000
ABSTRACT
TOP
ABSTRACT
Introduction
We characterized synaptosomal glutamate transport activity in a recently developed transgenic rat model of amyotrophic lateral sclerosis (ALS) overexpressing the G93A Cu2+/Zn2+ superoxide dismutase (SOD1) mutation. Using spinal cord synaptosomes, a significant reduction (43%) in the maximal velocity for high-affinity, Na+-dependent glutamate uptake was observed at disease end stage in G93A rats compared with age-matched controls. Similarly, a 27% reduction in maximum velocity (Vmax) was measured at disease onset, but no difference in spinal cord Vmax values were observed with presymptomatic animals compared with controls. In comparison, we observed no differences in the Vmax for glutamate clearance at disease end stage with synaptosomes from cortex, hippocampus, striatum, cerebellum, and brainstem, indicating a specific deficit in the spinal cord. The pharmacological sensitivity of spinal cord uptake to dihydrokainate suggests that the GLT-1 (glutamate transporter-1) subtype primarily mediates the transport activity. Expression analysis revealed a loss of GLT-1 as well as qualitative changes in GLAST (glutamate/aspartate transporter) but no measurable changes in EAAC1 (excitatory amino acid carrier 1) in spinal cord of end-stage G93A rats, indicating that deficits in glutamate transporters in this rat model may be glial specific. Riluzole, a neuroprotective agent used clinically to slow the progression of ALS, produced an enhancement of spinal cord synaptosomal glutamate uptake in control animals and early-stage disease G93A rats, but this effect was lost in end-stage animals. Altered expression of astroglial glutamate transporters accompanied by reduced capacity for spinal cord clearance of extracellular glutamate in the G93A SOD1 transgenic rat may account for a dampened effect of riluzole to enhance glutamate uptake at end-stage disease.
Key words: Cu2+/Zn2+ superoxide dismutase; ALS; GLT-1; GLAST; glutamate; riluzole
Introduction
Amyotrophic lateral sclerosis (ALS) is a late-onset neurodegenerative disease involving progressive motor neuron degeneration, paralysis, and death (Brown, 2001
; Cleveland and Rothstein, 2001
Transgenic mice harboring a human Cu2+/Zn2+ superoxide dismutase 1 (SOD1) transgene containing the G93A mutation (Gurney et al., 1994
Recently, transgenic rats expressing human SOD1 G93A have been generated (Howland et al., 2002
Materials and Methods
Materials. Transgenic G93A rats (Howland et al., 2002
Preparation of synaptosomes. Specific regions of the nervous system, including spinal cord, cortex, hippocampus, striatum, cerebellum, and brainstem, were dissected, collected in ice-cold isolation medium (310 mM sucrose and 10 mM HEPES, pH 7.4), and homogenized with a Teflon-glass homogenizer, followed by centrifugation at 1000 × g for 5 min. The resulting supernatant was collected and centrifuged at 20,000 × g for 20 min to obtain the crude synaptosomal P2 pellet which was used at a protein concentration of 0.75 mg/ml in HEPES-buffered saline (HBS) (in mM: 10 HEPES, 5 Tris base, 140 NaCl, 2.5 KCl, 1.2 CaCl2, 1.2 MgCl2, 1.2 K2HPO4, and 10 glucose, pH 7.4). Protein concentration was determined by a modified Bradford method using the commercially available Bio-Rad protein assay kit. Synaptosomal pellets were kept on ice under isolation medium and were resuspended in HBS at room temperature 15-30 min before the assay of L-[3H]glutamate uptake.
Glutamate uptake assays. Uptake studies in synaptosomes were performed with synaptosomal P2 fractions isolated from cervical spinal cord or the specified brain regions. L-[3H]Glutamate uptake was assayed in a final volume of 250 µl of HBS containing 75 µg of synaptosomal protein, 1 µM L-glutamate, and 0.25 µCi/assay L-[3H]glutamate in the absence and presence of inhibitors for the determination of IC50 values. Kinetic experiments were undertaken in the presence of 1-30 µM L-glutamate in the presence of 0.25 µCi/assay L-[3H]glutamate as tracer. The effect of riluzole was evaluated by preincubating synaptosomes with the indicated concentrations for 10 min, followed by measurement of L-[3H]glutamate uptake, as described above for the inhibitors, in the continued presence of riluzole. Reactions were incubated for 4 min at room temperature and then terminated by filtration using a Packard Filtermate 96-well harvester, followed by rapid washing with ice-cold Na+-free HBS (prepared by equimolar replacement with choline). Radioactivity retained on the filters was determined by scintillation counting. In all uptake experiments, the radioactivity retained after incubation in Na+-free HBS was used to correct all data to represent Na+-dependent uptake.
Histochemical analysis. Animals were anesthetized using approved animal welfare protocols and perfused by cardiac puncture with 4% paraformaldehyde-PBS. Brain and spinal cord were removed, followed by regional dissection. Tissue blocks were embedded in paraffin for sectioning (7 µm). Hematoxylin and eosin stains of brain and spinal cord were performed on paraffin sections. Immunostaining was performed with antibody to glial fibrillary acidic protein, GFAP (1:50; Dako, Copenhagen, Denmark).
Immunoblot analysis of glutamate transporters. The expression of GLT-1, GLAST, and EAAC1 in whole spinal cord and brainstem homogenates was examined by immunoblot. Whole cervical spinal cord or brainstem (~0.2 gm) was homogenized in 2 ml of 50 mM Tris-HCl, 150 mM NaCl, 5 mM EDTA, 1% Nonidet P-40, and 1% SDS, pH 7.4, with protease inhibitors (Complete; Roche, Indianapolis, IN) and centrifuged at 14,000 × g. Five to 25 µg of total extract protein was electrophoresed on 7.5% SDS-polyacrylamide gels. Immunoblots were probed with anti-GLT-1 (1:5000), anti-GLAST (1:2000), anti-EAAC1 (1:500), anti-GFAP (1:5000), anti-actin (C4; 1:5000), or anti-synaptophysin (1:5000) antibodies. Secondary antibodies conjugated to HRP used at 1:2000 were followed by signal detection using ECL (Amersham Biosciences, Piscataway NJ).
Data analysis. All data for uptake assays were corrected to represent Na+-dependent uptake by subtraction of the uptake observed in the absence of extracellular Na+. Kinetic data were determined by nonlinear regression analysis of the saturation curves using the following Michaelis-Menten equation: velocity = Vmax × [S]/Km + [S], where [S] is substrate concentration, using Origin 6.0 software (Microcal Software, Northampton, MA). In the pharmacological experiments, control uptake was calculated as the total Na+-dependent uptake measured over 4 min, and drug effects were expressed as a percentage of the control response. Log concentration-response curves were constructed for the determination of IC50 values using the following four-parameter logistic function: y = (Top
Bottom/1 + (x/IC50)p)) + Bottom, where p represents the Hill coefficient.
Quantitation of immunoblots was done using Scion Image software. Statistical analyses were performed using between-groups ANOVA, followed by Dunnett's t test.
Results
Spinal cord synaptosomal uptake of glutamate
High-affinity Na+-dependent glutamate uptake was examined in spinal cord synaptosomes prepared from presymptomatic (8-10 weeks), disease onset (13-15 weeks), and end-stage (15-17 weeks) G93A rats and compared with the activity measured in age-matched control (nontransgenic) animals. Onset of the disease was typified by the appearance of hindlimb abnormal gait, followed by a rapid progression (<2 weeks) to complete hindlimb paralysis, with end-stage animals characterized with a loss of righting reflex concomitant with paralysis extending to at least one forepaw (Table 1). No difference in the Vmax of glutamate transport in spinal cord synaptosomes was observed with presymptomatic animals compared with controls; however, a reduction in the Vmax was observed coincident with disease onset and was more dramatic at end stage (Fig. 1). Vmax values were 161 ± 16 and 92 ± 17 pmol · min
1 · mg
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Table 1. Clinical classification of G93A SOD1 transgene-induced disease progression
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Figure 1. Saturation isotherm for the high-affinity Na+-dependent transport of glutamate in spinal cord synaptosomes prepared from disease end-stage G93A transgenic rats and age-matched controls (a) and effect on Vmax relative to control as a function of disease progression (b). Glutamate uptake into P2 synaptosomal fractions prepared from presymptomatic, disease onset, and end-stage G93A rats, together with age-matched controls, was measured as described in Materials and Methods for the estimation of the kinetic parameters Km and Vmax. Solid line in a depicts data from control animals, and the dashed line represents the G93A data. Initial rates of Na+-dependent glutamate uptake were expressed as picomoles per minute per milligram of synaptosomal protein after subtraction of the uptake observed in the absence of extracellular Na+ (equimolar replacement of NaCl with choline chloride). Kinetic constants Km and Vmax were estimated from the saturation isotherm using the Michaelis-Menten equation, and data in b represent the percentage control Vmax values for the G93A animals at each stage of the disease evaluated. Data represent mean ± SEM values from three to four independent experiments. * indicates statistically significant difference from presymptomatic, by ANOVA with Dunnett's test for multiple comparisons at the 5% significance level.
With each preparation of synaptosomes, we also examined the sensitivity of the transport process to the nonselective glutamate uptake blocker trans-PDC and the selective GLT-1/EAAT2 inhibitor DHK. Inhibitor sensitivity, in combination with Na+ dependency of uptake, was evaluated as an index of the integrity of the synaptosomal preparations, and the analysis was also performed to determine any changes in pharmacological sensitivity. Glutamate uptake activity in spinal cord synaptosomes from presymptomatic G93A and age-matched control rats was blocked in a concentration-dependent manner by both trans-PDC and DHK, with equivalent IC50 values between G93A animals and controls (Fig. 2a, Table 2). No changes in the inhibitor sensitivity were observed with spinal cord synaptosomes prepared from disease onset or end-stage G93A rats compared with either their corresponding age-matched controls (Fig. 2b,c) or the results obtained for presymptomatic animals. A summary of the pharmacological comparison for spinal cord synaptosomes is provided in Table 2.
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Figure 2. Log concentration-response curves for the inhibition of glutamate uptake into spinal cord synaptosomes prepared from G93A transgenic rats and age-matched controls. Glutamate uptake into P2 synaptosomal fractions prepared from presymptomatic (a), disease onset (b), and end-stage (c) G93A rats, together with age-matched controls, was measured in the absence and presence of the nonselective transport inhibitor trans-PDC or the selective GLT-1/EAAT2 inhibitor DHK. Solid lines depict data from control animals, and dashed lines rep resent the G93A data. The net Na+-dependent glutamate uptake values were expressed as a percentage of the activity observed in the absence of drug, and IC50 values were determined from the log concentration-response curves by nonlinear regression analysis using the four-parameter logistic function. Averaging the percentage control values obtained from three independent experiments generated each curve shown, and the IC50 values are summarized in Table 2.
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Table 2. Pharmacological characterization of glutamate uptake into spinal cord synaptosomes prepared from transgenic G93A rats and age-matched controls Loss of glutamate uptake enhancement by riluzole in end-stage spinal cord from G93A rats
Riluzole, a neuroprotective agent used clinically to slow the progression of ALS, has been reported to increase the glutamate transport capacity in spinal cord synaptosomes (Azbill et al., 2000
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Figure 3. Effect of riluzole on the high-affinity Na+-dependent uptake of glutamate in spinal cord synaptosomes prepared from G93A transgenics and age-matched controls. Glutamate uptake into P2 synaptosomal fractions prepared from disease onset (a) and end-stage (b) G93A rats, together with age-matched controls, was measured in the absence or presence of riluzole (0.1-300 µM) after a 10 min pretreatment with the drug. The net Na+-dependent glutamate uptake data were expressed as a percentage of the activity observed in the absence of drug. A significant enhancement of glutamate uptake by riluzole was measured for control tissue (a, b) and G93A transgenic tissue at disease onset (a) (ANOVA; p < 0.05) but not for G93A transgenic tissue at end-stage disease (b).
Disease changes and synaptosomal glutamate uptake in various brain regions
Spinal cord from end-stage G93A transgenic rats shows a complete loss of ventral large motor neuron cell bodies (Fig. 4A) as well as dramatic increases in gliosis (Fig. 4A,B) but only few vacuoles. Vacuoles appear in higher abundance in earlier stages of disease in these rats (Howland et al., 2002
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Figure 4. Histochemical analysis of pathology in end-stage G93A transgenic rat spinal cord and brain regions. Cervical spinal cord (A) or brain areas including brainstem (C), neocortex (D), and hippocampus (E) were stained with hematoxylin and eosin to show extent of neuronal loss, degenerative structures (vacuoles), as well as gliosis in end-stage G93A rats compared with age-matched control rats (Con). Arrows in A and C denote the presence of large motor neuron cell bodies, rarely found in end-stage diseased spinal cord. Representative spinal cord sections from control and end-stage G93A rats are also shown stained with anti-GFAP antibody (B). Arrows in B highlight a hypertrophic astrocyte, frequently found in end-stage diseased spinal cord.
High-affinity Na+-dependent glutamate uptake was examined in synaptosomes prepared from cortex, hippocampus, striatum, cerebellum, and brainstem using end-stage G93A rats and compared with the activity measured in the same tissues from age-matched control animals. In contrast to what we observed in G93A rat spinal cord, there was no difference in either the Vmax or Km values for glutamate uptake in cortical, hippocampal, striatal (Fig. 5), cerebellar, or brainstem (Fig. 6) synaptosomes between end-stage disease G93A and age-matched control animals. Similarly, we observed no difference in the pharmacological sensitivity to either trans-PDC or DHK using synaptosomes prepared from these same brain regions when comparing G93A rats with control animals (Table 3). Both trans-PDC and DHK were effective blockers of glutamate uptake in all regions examined, with the exception of DHK in cerebellar synaptosomes in which 50% inhibition of uptake was not achieved, even at 1 mM.
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Figure 5. Saturation isotherms for the high-affinity Na+-dependent transport of glutamate in cortical (a), hippocampal (b), and striatal (c) synaptosomes prepared from end-stage G93A transgenic rats and age-matched controls. Glutamate uptake into P2 synaptosomal fractions was measured as described in Materials and Methods for the estimation of the kinetic parameters Km and Vmax. Initial rates of Na+-dependent glutamate uptake were expressed as picomoles per minute per milligram of synaptosomal protein after subtraction of the uptake observed in the absence of extracellular Na+ (equimolar replacement of NaCl with choline chloride). Kinetic constants Km and Vmax were estimated from the saturation isotherm using the Michaelis-Menten equation and are presented in Table 3. Data represent mean ± SEM values from three independent experiments.
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Figure 6. Saturation isotherms for the high-affinity Na+-dependent transport of glutamate in cerebellar (a) and brainstem (b) synaptosomes prepared from end-stage G93A transgenic rats and age-matched controls. Note that the scale of the y-axis in this figure is lower than tissue analyzed in Figure 5. Brainstem and cerebellum typically exhibited lower overall glutamate uptake capacity. Glutamate uptake measurements and calculations of Vmax and Km were identical to that as described in Figure 5. Kinetic constants Km and Vmax were estimated from the saturation isotherm using the Michaelis-Menten equation and are presented in Table 3. Data represent mean ± SEM values from three independent experiments.
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Table 3. Kinetic parameters and inhibitor IC50 values for glutamate uptake in synaptosomes prepared from various brain regions of transgenic G93A rats and age-matched controls Expression analysis of GLT-1, GLAST, and EAAC1 in spinal cord and brainstem of G93A rats
Whole cervical spinal cord from end-stage G93A rats and nontransgenic age-matched controls (16-20 weeks) were analyzed for levels of glial glutamate transporters GLT-1 and GLAST, as well as the neuronal transporter EAAC1, by immunoblot analysis (Fig. 7A). In addition, immunoblots were probed with antibodies to GFAP to index the extent of gliosis, synaptophysin to index the degree of neuronal cell loss, and actin to control for protein loading. A significant decrease of GLT-1 of 45% was observed in end-stage cervical spinal cord of the G93A rats compared with controls (Fig. 7A). No consistent changes in gel migration of the 72 kDa GLT-1 monomeric species were observed between control and end-stage disease tissue, in contrast to that reported by Deitch et al. (2002)
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Figure 7. Immunoblot analysis of GLT-1, GLAST, and EAAC1 protein expression in whole cervical spinal cord (A) and brainstem (B) homogenates. Expression of glutamate transporters (GLT-1, GLAST, and EAAC1), as well as GFAP, actin, and synaptophysin is shown in nontransgenic animals (Con) and end-stage SOD G93A rats between 16 and 20 weeks of age and depict typical results obtained. Asterisks denote G93A rats that were scored as most severely affected in this group. Five micrograms of extract protein were immunoblotted for GLT-1, GFAP, synaptophysin (SYPH), and actin (ACT), and 25 µg of protein were immunoblotted for EAAC1 and GLAST.
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Figure 8. Immunoblot analysis of GLT-1 and GLAST, as well as GFAP, synaptophysin, and actin expression in whole cervical spinal cord through disease progression [nontransgenic (Con), presymptomatic G93A (8 weeks), onset G93A (16 weeks), and end-stage G93A (18 weeks) rats]. Five micrograms of extract protein were immunoblotted for GLT-1, GFAP, synaptophysin (SYPH), and actin, and 25 µg of protein were immunoblotted for GLAST.
In contrast to GLT-1 changes in spinal cord, we observed no consistent changes in GLT-1 immunoreactivity in brainstem of end-stage G93A rats (Fig. 7B). A slightly decreased mobility for the 65 kDa form of GLAST was evident in brainstem but was not as dramatic as that seen in spinal cord from end-stage diseased rats. No significant changes in EAAC1 immunoreactivity were noted in the brainstem of the G93A rats. As expected, GFAP immunoreactivity was significantly elevated in brainstem (twofold) of the G93A rats; however, no significant changes in synaptophysin immunoreactivity were noted, consistent with a lower degree of neuron cell loss in brainstem compared with spinal cord. Cortex of the G93A end-stage rats as well as controls were also analyzed in a similar manner as for spinal cord and brainstem; however, no changes in any of the transporters was noted in this brain region (data not shown).
Glutamate transporter levels were also assessed in the G93A rat spinal cord at different stages of disease (nontransgenic, presymptomatic, onset, and end stage) (Fig. 8). Reduced levels of GLT-1 were evident as well as GLAST, showing altered gel migration in all G93A rats at end stage. GLT-1 changes, however, were not typically evident in G93A rats at disease onset or in presymptomatic rats when analyzing whole spinal cord tissue. However, we showed previously that, when rat spinal cord is microdissected into ventral and dorsal horns, decreased levels of GLT-1 are evident as early as 100 d old (late presymptomatic) (Howland et al., 2002
Discussion
We describe a kinetic and pharmacological characterization of synaptosomal glutamate transport capacity in multiple regions of the nervous system using a recently developed transgenic rat model of ALS overexpressing the human G93A mutant Cu2+/Zn2+ superoxide dismutase 1 gene (Howland et al., 2002
We examined glutamate uptake in tissue known to contain ALS-like lesions in the G93A transgenic rats (spinal cord and brainstem) as well as regions devoid of pathology (cortex, hippocampus, striatum, and cerebellum). Functional glutamate transport is only deficient in spinal cord of the G93A rats, is evident as early as disease onset, and becomes more severe by end stage. Our results in end-stage diseased spinal cord are similar to those described previously for transgenic mice harboring the same G93A mutant form of SOD1 (Canton et al., 1998
Studies with synaptosomal preparations prepared from postmortem human ALS tissue have described a marked reduction in the maximal velocity of glutamate transport in spinal cord (
A molecular mechanism for the deficits in glutamate clearance capacity was initially suggested in the human study with the demonstration that expression levels of the glial-specific glutamate transporter EAAT2 (GLT-1) were dramatically reduced in both spinal cord and motor cortex (Rothstein et al., 1995
Immunohistochemical methods were also used to demonstrate reductions of GLT-1 in G93A transgenic mouse spinal cords at 14-18 weeks in age, a time when motor impairments is evident (Bendotti et al., 2001
Our results with the G93A transgenic rats support a model of dysfunction of astroglial glutamate transporter expression represented by loss of total GLT-1 protein, accompanied by the appearance of GLAST at an intermediate molecular weight, possibly reflecting a posttranslational modification. These changes in glutamate transporters in end-stage diseased spinal cord from the G93A rats were accompanied by decreased synaptophysin immunoreactivity and markedly reduced numbers of large motor neurons in spinal cord (Howland et al., 2002
Pharmacological sensitivity of spinal cord glutamate transport to both the nonselective glutamate uptake blocker trans-PDC and the selective GLT-1/EAAT2 inhibitor DHK was observed in our study at all developmental time points evaluated, with no changes in inhibitor IC50 observed as the disease progressed. Sensitivity to DHK in the spinal cord preparation suggests that the GLT-1 subtype of glutamate transporter predominantly mediates the measured transport activity. This conclusion is consistent with the reported high expression of GLT-1 in spinal cord homogenates by immunoblot analysis and the relatively low expression of GLAST or EAAC1 immunoreactivity. The loss of glutamate transport capacity observed in the spinal cord of G93A rats together with the pharmacological identification of GLT-1 as the predominant subtype provides indirect evidence for the loss of GLT-1 in this model as a contributing factor to the deficit. More directly, the 45% loss of GLT-1 protein correlates well with the 43% reduction in net glutamate uptake capacity.
Additional characterization of the pharmacological properties of spinal cord glutamate transport was explored in this study by examining the facilitatory effect of riluzole on the uptake mechanism. Riluzole is used clinically in delaying the progression of ALS (Desai and Swash, 1997
In summary, we demonstrated marked deficits in glutamate uptake in spinal cord, but not brainstem and other brain areas not affected by disease, in the G93A transgenic rat. Reductions in spinal cord glutamate transport capacity are accompanied by altered expression of astroglial glutamate transporters GLT-1 and GLAST. Significant deficits in glutamate uptake mediated by glial cells is likely to be the cause for loss of efficacy of riluzole to potentiate glutamate uptake in end-stage G93A spinal cord compared with rats at earlier stages of disease. On the basis of these data, it is possible that the effectiveness of riluzole in ALS patients in latter stages of disease may be dampened compared with patients at earlier stages of disease on this drug therapy.
FOOTNOTES Received Oct. 4, 2002; revised Dec. 3, 2002; accepted Dec. 16, 2002.
We are grateful to John Kulik, George Psaltis, and Lisa DeVito for assistance with the transgenic rat colony. We thank Drs. Seung Kwak and Erika Holzbaur for technical assistance and advice.
Correspondence should be addressed to Dr. David Howland, Wyeth Research, Neuroscience, CN8000, Princeton, NJ 08543. E-mail: howland{at}wyeth.com.
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