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(American Journal of Pathology. 2003;163:779-787.)
© 2003 American Society for Investigative Pathology

Animal Models

Translocation of Glutamate Transporter Subtype Excitatory Amino Acid Carrier 1 Protein in Kainic Acid-Induced Rat Epilepsy

Akiko Furuta^*, Mami Noda, Satoshi O. Suzuki^*, Yoshinobu Goto, Yoshiko Kanahori, Jeffrey D. Rothstein and Toru Iwaki^*

From the Departments of Neuropathology^* and Clinical Neurophysiology, Neurological Institute, Graduate School of Medical Sciences, and the Laboratory of Pathophysiology, Graduate School of Pharmaceutical Sciences, Kyushu University, Fukuoka, Japan; and the Departments of Neurology and Neuroscience, The Johns Hopkins University School of Medicine, Baltimore, Maryland

Abstract

Glutamate excitotoxicity has been implicated in the pathophysiology of epilepsy. Systemic injection of kainic acid (KA) in the rat produces an animal model of human temporal lobe epilepsy. We examined the temporal expression of the sodium-dependent neuronal glutamate transporter, excitatory amino acid carrier 1 (EAAC1), in KA-induced rat epilepsy. As an early alteration, perinuclear deposits of EAAC1 protein were found mainly in the large pyramidal neurons at the hippocampus, neocortex, piriform cortex, and amygdala with the reduction of neuropil staining 6 hours after KA injection. Immunoelectron microscopic study revealed that the perinuclear EAAC1 immunoreactivity corresponded to the translocation to the Golgi complex. At this time point, EAAC1 mRNA was down-regulated. The intracellular aggregation of EAAC1 primarily disappeared by 24 hours. In vitro studies indicated that internalization of EAAC1 from the plasma membrane to the intracellular compartment by KA treatment was associated with the reduction of electrogenic transporter currents. Our results suggest that the transient EAAC1 internalization participates in the modulation of the transporter function preventing excessive glutamate uptake to pyramidal neurons during the early stage of epilepsy.

Systemic or intracerebral injection of KA, a rigid analogue of glutamate, in the rat is frequently used to produce an animal model of human temporal lobe epilepsy. Since the description by Olney and colleagues,¹⁷ the neurotoxicity of KA has been extensively studied neuropathologically and electrophysiologically.¹⁸ In the present study, we found transient translocation of EAAC1 protein to the Golgi complex with the reduction of neuropil staining in the pyramidal neurons 6 hours after KA injection. To test the hypothesis that the EAAC1 internalization by KA treatment is associated with functional impairment, in vitro studies were also performed with C6 glioma cells. We used the C6 glioma cell line because it endogenously expresses only EAAC1 among sodium-dependent glutamate transporter subtypes⁷ and it has been used to investigate the membrane trafficking of the EAAC1 through protein kinase C and phosphatidylinositol 3-kinase.^19-21 Moreover, cultured hippocampal neurons express not only EAAC1 but also GLT-1.²² In our result, the reduction of the reversed transporter current with the change of subcellular localization was observed by KA treatment. The intracellular trafficking and functional role of EAAC1 in epilepsy have been discussed.

Materials and Methods

Animal Procedures and Tissue Preparation

This study was approved by the Animal Committee of Kyushu University. Male Wistar rats weighing 180 to 200 g (8-weeks-old; Kyudo, Japan) were divided into seven groups of five rats each. Rats were injected intraperitoneally with 10 mg/kg KA (Sigma, St. Louis, MO or Ocean Produce Int., Nova Scotia, Canada). After being deeply anesthetized with ether, rats were intra-aortically perfused with 4% paraformaldehyde and brain tissue samples were obtained at 2 hours, 6 hours, 24 hours, 1 week, and 4 weeks after the KA injection. In the two control groups, the rats were injected intraperitoneally with 0.1 mol/L of phosphate-buffered saline (200 µl) and killed at 6 hours and 4 weeks after the injection. After the KA injection, behavioral changes were observed to determine the seizure stages according to the criteria of Racine.²³ Intraperitoneal KA injection (10 mg/kg) produced the following acute-stage behavioral changes in each Wistar rat: within 2 hours, the rats developed masticatory movements, head nodding, and wet dog shakes (class 1 and 2 by Racine²³ ), followed by forelimb clonus and rearing (class 3 and 4); between 2 and 4 hours after KA injection, the rats exhibited severe, repeated status epilepticus with rearing and falling and reached class 5 motor seizures; the seizures declined and rats appeared exhausted between 4 and 6 hours; spontaneous motor seizures were occasionally observed in the late stage 1 week after KA injection.

Western Blotting

Fresh-frozen samples from the hippocampus of the control and KA-treated rats killed at 6 hours and 4 weeks were used. Western blotting was performed as described previously.²⁴ Samples were homogenized in protein lysis buffer. Each sample (10 µg/lane) was separated by 7.5% sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis and transferred to a polyvinylidene difluoride membrane (Millipore, Bedford, MA). The membranes were incubated overnight with EAAC1 antibody (1:1000)⁴ in blocking buffer at 4°C, then washed and incubated with peroxidase-conjugated secondary antibody (1:20,000; Chemicon, Temecula, CA) for 1 hour. The immunoreactive proteins were visualized with enhanced chemiluminescence (Amersham, Buckinghamshire, UK). Then, the membrane was washed and incubated with actin antibody (1:5000, Amersham) and developed with enhanced chemiluminescence as a loading control.

Northern Blotting

Total RNA was isolated by the guanidine isothiocyanate method²⁵ from each hippocampus from which a contralateral sample was used for Western blotting. RNA (10 µg/lane) was diluted in loading buffer (0.5x 3-(N-morpholino)propanesulfonic acid (MOPS), 50% formamide, 6.7% formaldehyde, 10 µg/ml ethidium bromide), electrophoresed in 1% denaturing agarose gel containing 1x MOPS and 6.7% formaldehyde, and transferred onto nylon membrane (Roche, Mannheim, Germany). The membrane was hybridized with ³²P-labeled EAAC1 cDNA probes overnight at 65°C. After washing twice in 6x standard saline citrate (SSC) at room temperature for 10 minutes, once in 2x SSC/0.1% SDS and 0.2x SSC/0.1% SDS at 65°C for 20 minutes, the membrane was exposed to X-ray film (Eastman-Kodak, Rochester, NY) overnight at -80°C. After stripping the EAAC1 probe in 2x SSC/50% formamide at 65°C overnight, the membrane was reprobed with glyceraldehyde phosphate dehydrogenase (GAPDH) cDNA as a loading control as described above.

Immunohistochemistry and Immunoelectron Microscopy

Immunohistochemistry and immunoelectron microscopy were performed as described previously.²⁴ For histopathological examination, the coronal sections at the level of the dorsal hippocampi and the sagittal sections of the cerebellum were stained with hematoxylin and eosin (H&E). For immunohistochemistry, paraffin-embedded 5-µm-thick sections were deparaffinized and incubated with 0.3% hydrogen peroxide in absolute methanol for 30 minutes. Sections were autoclaved in 0.01 mol/L of citrate buffer, pH 6.0, to enhance the immunoreactivity. After washing with Tris-HCl buffer (50 mmol/L Tris-HCl, pH 7.6), the sections were incubated at 4°C overnight with primary antibodies diluted 1:100 for EAAC1⁴ (rabbit, polyclonal), N-methyl-D-aspartate receptor (NR) 1 (rabbit, polyclonal; Chemicon) and glutamate receptor (GluR) 2/3 (rabbit, polyclonal; Chemicon). The sections were then washed and incubated with biotinylated rabbit antibodies diluted 1:200 and peroxidase-conjugated streptavidin-biotin complex or fluorescein isothiocyanate-conjugated streptavidin (Amersham) diluted 1:100 sequentially. The colored reaction product was developed with 3,3'-diaminobenzidine tetrahydrochloride solution. The sections for immunofluorescence were counterstained with propidium iodide and were observed under a confocal laser microscope (LSM-GB200; Olympus, Tokyo, Japan). For immunoelectron microscopy, rats were perfused with 2% paraformaldehyde/2% glutaraldehyde in 0.1 mol/L of phosphate buffer. Vibratome sections (40 µm) were pretreated by 1% sodium borohydride for 10 minutes, then immunohistochemistry was performed using the labeled biotin-streptavidin method with 3,3'-diaminobenzidine tetrahydrochloride reaction the same as with paraffin sections. Ultrathin sections without lead staining were observed under an electron microscope (JEM-100CX; JEOL, Japan).

In Situ Hybridization

Nonradioisotopic in situ hybridization was performed as described previously.²⁶ To detect the EAAC1 transcripts, a 149-bp cDNA fragment of rat EAAC1 (GenBank accession number U21107; position 504 to 652) was amplified by polymerase chain reaction from rat cerebral cDNA and was cloned in TA-cloning vector (Invitrogen Corp., Carlsbad, CA). Digoxigenin-labeled anti-sense and sense cRNA probes were generated using a DIG RNA Labeling Kit (SP6/T7) (Roche). Paraffin-embedded sections were deparaffinized, digested with 20 µg/ml of proteinase K for 15 minutes at room temperature, acetylated with 0.25% acetic anhydride/0.1 mol/L triethanolamine (TEA), pH 8.0, for 10 minutes, and treated with 0.2 N HCl for 10 minutes. Then, sections were hybridized with the probes overnight at 50°C. After being rinsed in 2x SSC/50% formamide at 65°C for 30 minutes, sections were treated with 50 µg/ml of RNase A in 10 mmol/L of Tris-HCl, pH 7.6/500 mmol/L NaCl/1 mmol/L ethylenediaminetetraacetic acid at 37°C for 30 minutes, and washed once in 2x SSC/0.1% SDS at 65°C for 20 minutes and twice in 0.2x SSC/0.1% SDS at 65°C for 20 minutes. Sections were then incubated with alkaline phosphatase-conjugated anti-digoxigenin monoclonal antibody (1:500) overnight at 4°C (DIG Nucleic Acid Detection kit, Roche). Sections were developed in 350 µg/ml nitro blue tetrazolium, 175 µg/ml 5-bromo-4-chloro-3-indolyl phosphate/100 mmol/L Tris-HCl, pH 9.5, 100 mmol/L NaCl, and 50 mmol/L MgCl for 16 to 24 hours in the dark. To determine the specificity of the digoxigenin-labeled EAAC1 anti-sense probe, hybridization with an EAAC1 sense probe as well as competitive hybridization with digoxigenin-labeled and nonlabeled probes was performed at the same time.

Densitometric Analysis

Image analysis of immunohistochemistry and in situ hybridization for EAAC1 was performed on a Macintosh computer using the public domain NIH Image program 1.62 (National Technical Information Service, Springfield, VA) as described previously.²⁷ The optical densities at large neurons were obtained from five fields (0.025 inches) of each section of CA3 at the hippocampus, layer 5 at the neocortex, and mediodorsal nuclei at the thalamus, and then averaged for three rats. Statistical analysis for the differences of regional changes between control and KA-treated rats was performed with a Kruskal-Wallis test as well as a Mann-Whitney U-test using a StatView J4.5 program (Abacus Concepts, Berkeley, CA).

Cell Culture

C6 rat glioma cells (CL 107, American Type Culture Collection, Rockville, MD) that endogenously express EAAC1⁷ were cultured in Dulbecco’s modified Eagle’s medium supplemented with 10% heat-inactivated calf serum. For electrophysiology, cells were plated in 35-mm dishes and incubated with 500 nmol/L of phorbol 12-myristate 13-acetate (PMA) for 3 hours. Then, KA (10 µmol/L) was applied for 1.5 hours before use. For immunocytochemistry, culture cells were plated in Lab-Tek chamber slides (Nunc Inc., Naperville, IL), and fixed with 4% paraformaldehyde, pretreated with 1% Nonidet P-40 for 10 minutes, and incubated overnight with EAAC1 antibody diluted 1:10. Then cells were incubated with fluorescein isothiocyanate-conjugated anti-rabbit IgG (Amersham) and propidium iodide (Sigma). The slides were observed under a laser scan confocal microscopy (LSM-GB200; Olympus, Japan).

Electrophysiological Measurements

Patch-clamp recordings were made as reported previously.^28,29 C6 glioma cells were whole cell-clamped using a patch pipette containing 90 mmol/L NaCl, 10 mmol/L L-glutamate, 3 mmol/L MgATP, 5 mmol/L HEPES, 1 mmol/L CaCl₂, 4 mmol/L MgCl₂, and 5 mmol/L EGTA. The pH of the solution was adjusted to 7.3 with N-methyl-D-glucamine. The pipette resistance was 6 to 9 M. The external solution contained 0 or 10 mmol/L KCl, 110 or 100 mmol/L choline chloride, 0.5 mmol/L MgCl₂, 3 mmol/L CaCl₂, 5 mmol/L HEPES, 15 mmol/L glucose, 6 mmol/L BaCl₂, and 0.1 mmol/L ouabain. The pH of the solution was adjusted to 7.4 with N-methyl-D-glucamine. The external potassium solution was applied rapidly using the Y-tube technique,³⁰ which allows the complete exchange of the external solution surrounding a cell within 20 ms. The temperature monitored in the recording dishes was 33 to 34°C.

Results

Western and Northern Blot Analysis of EAAC1

Western blotting of the hippocampal homogenates from control and KA-treated rats at 6 hours and 4 weeks demonstrated a single band that corresponded to EAAC1 protein using C-terminal EAAC1 antibody. Total expression level of EAAC1 protein was not altered 6 hours after KA treatment. Degradation products were not observed in the homogenates from KA-treated rats (Figure 1A) . Northern blotting of the hippocampal homogenates revealed a single band at 3.8 kb that corresponds to EAAC1 transcripts using ³²P-labeled EAAC1 cDNA probes (Figure 1B) . Neither the truncated nor aberrant form of EAAC1 mRNA was detected in KA-treated rats.

View larger version (58K): [in this window] [in a new window]   Figure 1. Western (A) and Northern (B) blot analysis for each EAAC1 protein and EAAC1 mRNA in the hippocampal tissue from control and KA-treated rats at 6 hours (6h) and 4 weeks (4w). A: Western blotting demonstrates the specificity of antibodies raised against the synthetic peptide corresponding to the C-terminus of EAAC1. Actin was used as a loading control. Each lane was loaded with 10 µg of protein. B: Northern blotting with 32P-labeled EAAC1 cDNA probes detects a single band at 3.8 kb that corresponds to EAAC1 transcripts. GAPDH was used as a loading control. Each lane was loaded with 10 µg of total RNA.

In the control rat brains, EAAC1 was enriched in the large pyramidal neurons and neuropil of the hippocampus, caudate putamen, amygdala, piriform cortex, olfactory bulb, and cerebellar cortex (Figure 2 ; A, C, and E). Early histopathological changes 2 hours after KA injection were characterized by edema in the neuropil throughout the forebrain. Despite the marked neuropil changes in H&E sections, EAAC1 protein expressions were generally retained even in the shrunken neurons until 2 hours after KA injection during status epilepticus. Expression of EAAC1 increased slightly at the piriform cortex at 2 hours. The most dramatic change was disclosed at 6 hours; ie, perinuclear deposition of EAAC1 immunoreactivity was found together with the reduction of neuropil staining mainly in the large pyramidal neurons of the neocortex (Figure 2B) , hippocampus (Figure 2D) , amygdala, and piriform cortex. These changes were partly seen in the putaminal neurons and small pyramidal neurons of the neocortex, but not observed in the cerebellar Purkinje cells (Figure 2F) , spinal motor neurons, or astrocytes. In the immunoelectron microscopy, EAAC1-immunoreactivity at 6 hours was associated mainly with the outer membrane of the Golgi complex, which was consistent with the perinuclear staining of the large pyramidal neurons at 6 hours (Figure 2G) . Less immunoreactivity for EAAC1 was found in the dendrites, axons, plasma membranes, and nucleus. This intracellular relocation of EAAC1 is specific, because other membrane proteins such as one of the N-methyl D-aspartate (NMDA) receptors, NR1, and one of the -amino-3-hydroxy-5-methyl-4-isoxazole propionic acid (AMPA) receptors, GluR 2/3, did not undergo the same spatial reorganization in the immediate postseizure period (Figure 3) . The intracellular aggregation of EAAC1 at 6 hours (Figure 4, B and F) was not observed at 24 hours (Figure 4, C and G) , 1 week, and 4 weeks (Figure 4, D and H) after KA injection. EAAC1 expression partly decreased at the piriform cortex, the lateral part of amygdala, and the medial part of the thalamic nuclei at 1 week and 4 weeks.

View larger version (117K): [in this window] [in a new window]   Figure 2. Immunohistochemistry (A–F) and immunoelectron microscopy (G) in layer 5 of neocortex (A, B, and G), CA3 pyramidal neurons at hippocampus (C, D), and cerebellar Purkinje cells (E, F). A–D: In the control rats, pyramidal neurons and neuropil are immunoreactive for EAAC1 (A, C). EAAC1 immunoreactivity is found as perinuclear deposits at pyramidal neurons with reduced neuropil staining 6 hours after the KA injection (B, D), whereas immunoreactivities for EAAC1 are not altered with KA treatment in the Purkinje cells (E, F). G: Ultrastructural localization of EAAC1 in cortical pyramidal neurons 6 hours after the KA injection. Electron micrographs show enrichment of EAAC1 immunoreactivity around the Golgi apparatus (arrows) compared to that at the plasma membranes (arrowheads). Scale bars: 20 µm (A–F); 1 µm (G).

View larger version (152K): [in this window] [in a new window]   Figure 3. Immunohistochemistry for EAAC1 (A and B, green), NR1 (C and D, green), and GluR2/3 (E and F, green) in the hippocampal CA3 in the control (A, C, E) and 6 hours after KA injection (B, D, F). Although perinuclear immunoreactivity for EAAC1 was found in the 6 hours after KA injection (B), immunoreactivities for the glutamate receptors NR1 and GluR2/3 were not altered in the large pyramidal neurons. Nuclear staining with propidium iodide (A–F, red). Scale bar, 20 µm.

View larger version (115K): [in this window] [in a new window]   Figure 4. Immunohistochemistry (A–H, EAAC1) and in situ hybridization with digoxigenin-labeled anti-sense probes (I–P, EAAC1-ISH) in the hippocampus (A–D, I–L) and the magnification of CA3 (E–H, M–P) at control (A, E, I, M), KA 6 hours (6h; B, F, J, N), KA 24 hours (24h; C, G, K, O), and KA 4 weeks (4w; D, H, L, P). A and E: Hippocampal pyramidal neurons and neuropil are immunoreactive for EAAC1 in the control. B and F: EAAC1 immunoreactivity is found as perinuclear deposits at pyramidal neurons (inset in F) 6 hours after the KA injection. C, D, G, and H: Distribution and immunoreactivity for EAAC1 at the hippocampus have almost recovered to the control level 24 hours as well as 4 weeks after the KA injection. I and M: EAAC1 transcripts are enriched in the pyramidal neurons of the control hippocampus. J and N: Expression of EAAC1 mRNA decreases 6 hours after the KA injection. K, L, O, and P: Expression of EAAC1 mRNA has recovered 24 hours as well as 4 weeks after the KA injection. Scale bars: 500 µm (A–D and I–L); 50 µm (E–H); 40 µm (M–P).

Densitometric Analysis of EAAC1 Expressions

Densitometric analysis of EAAC1 immunohistochemistry and in situ hybridization was performed at early phase (Figure 5A , KA 6 hours and KA 24 hours) and late phase (Figure 5B , KA 4 weeks). Optical densities for EAAC1 immunohistochemistry demonstrated that perikaryal staining (P in Figure 5A ) was increased in hippocampus and neocortex, whereas increased perikaryal staining was not seen in the mediodorsal nuclei of thalamus. Optical densities for neuropil staining in the immunohistochemistry (N in Figure 5A ) and the in situ hybridization became reduced in the hippocampus, neocortex, and thalamus at 6 hours. Such changes recovered to the control level at 24 hours. Significant difference is shown among the control, 6 hours and 24 hours in the perikaryal staining for hippocampus, as well as the neuropil staining and in situ hybridization in all three regions (Kruskal-Wallis test). Densities for both EAAC1-immunohistochemistry and in situ hybridization at 4 weeks (12-week-old rats) were reduced compared to those at 6 hours (8-week-old rats) in the control cases. In the KA-treated cases at 4 weeks, only neuropil staining for EAAC1 immunohistochemistry at the thalamus showed significant statistical decrease (Figure 5B , Mann-Whitney U-test).

View larger version (46K): [in this window] [in a new window]   Figure 5. Densitometric analysis of EAAC1 immunohistochemistry and in situ hybridization at CA3 of the hippocampus, layer 5 of the neocortex, and mediodorsal nuclei of the thalamus in the early phase (A): control (C), 6 hours (6h) and 24 hours (24h) after KA treatment in 8-week-old rats; and the late phase (B): control (C) and 4 weeks (4w) after KA treatment in 12-week-old rats. Optical densities for perikaryal staining (P) and neuropil staining (N) of immunohistochemistry and neuronal staining for in situ hybridization using digoxigenin-labeled anti-sense probes (ISH) are compared using the Kruskal-Wallis test (for A) and the Mann-Whitney U-test (for B). At 6 hours, perikaryal staining has increased, whereas neuropil staining has decreased in the hippocampus and the neocortex. The EAAC1 mRNA expression is reduced in the all three regions. These changes recover to the control level at 24 hours. Significant difference of optical densities is shown among the control, 6 hours, and 24 hours in the perikaryal staining of hippocampus as well as the neuropil staining and in situ hybridization in the all three regions. At 4 weeks, neuropil staining has significantly decreased in the thalamus. *, P < 0.05; **, P < 0.01. y axis indicates an arbitrary index.

To see the effect of KA on subcellular localization and the accompanying functional changes, we conducted in vitro studies on C6 glioma cells. In the EAAC1 immunocytochemistry, diffuse cytoplasmic staining was seen in the untreated C6 glioma cells (Figure 6A) . After the incubation with 500 nmol/L of PMA, membranous staining was observed in the subsets of C6 glioma cells (Figure 6B) as reported previously.¹⁹ Then, the 10 µmol/L KA treatment showed EAAC1 immunoreactivity in the perinuclear vesicular structures (Figure 6C) .

View larger version (31K): [in this window] [in a new window]   Figure 6. Translocation and functional changes of EAAC1 in vitro. A–C: EAAC1 immunocytochemistry in the C6 glioma cells that endogenously express EAAC1. Green, EAAC1 immunoreactivity; red, propidium iodide for nuclear staining. A: Untreated C6 glioma cells show diffuse EAAC1 immunoreactivity in the cytoplasm. B: After PMA treatment (500 nmol/L), membranous EAAC1 staining is found in C6 glioma cells. C: Then, perinuclear EAAC1 immunoreactivity is seen in the KA (10 µmol/L)-treated C6 glioma cells. D–F: Electrogenic glutamate transporter in C6 glioma cells and the effect of KA. D: The reversed mode of the glutamate transporter was measured using the whole-cell patch clamp method. The outward current reflecting glutamate release from the C6 glioma cells was smaller in 10 µmol/L KA-treated cells than in the nontreated cells. The holding potential was -40 mV and [K+]o was raised from 0 to 10 mmol/L (timing shown by black bar). The series of voltage pulses from -100 to +50 mV for 50 ms as shown below was applied at the time indicated (a to d). E: The voltage-dependence of K+-evoked current. The current-voltage relationship obtained at the time point of a and c in D was subtracted from the one at b and d, respectively. F: The amplitude of K+-evoked currents at -40 mV in control and KA-treated cells. The normalized amplitude was 0.62 ± 0.09 pA/pF (n = 6) in control and 0.33 ± 0.06 pA/pF (n = 8) in KA-treated cells. Mean ± SEM. *, P < 0.05). Scale bar, 20 µm (C).

Discussion

This study first demonstrated internalization of the neuronal glutamate transporter EAAC1 in vivo. We found that the EAAC1 protein in large pyramidal neurons was transiently translocated to the Golgi complex 6 hours after KA injection during a postictal state. Transporter current via EAAC1 was reduced in KA-treated cells in vitro.

EAAC1 in Large Pyramidal Neurons Is Transiently Translocated to the Golgi Complex 6 Hours after KA Injection in the KA-Treated Rat Epilepsy

Perinuclear deposits with reduction of neuropil staining for EAAC1 in KA-treated rats were preferentially observed in the large neurons at the hippocampus, neocortex, piriform cortex, and amygdala, but not seen in the Purkinje cells or spinal motor neurons. Thus, the EAAC1 internalization occurred mainly in the large neurons on the propagation pathway. This phenomenon is specific for the EAAC1 protein because other membrane proteins such as glutamate receptors did not alter the subcellular localization 6 hours after KA injection. We hypothesized that EAAC1 immunoreactivity located at the Golgi complex 6 hours after KA injection exhibited translocation from the plasma membrane rather than from the newly synthesized EAAC1 protein because of the following results: EAAC1 immunoreactivity in the perikarya increased significantly whereas that in the neuropil decreased in the hippocampus and neocortex of the densitometric analysis; however, as was shown by Western blotting, the total expression level of EAAC1 was not decreased and the aberrant or truncated form of EAAC1 mRNA was not found in the Northern blotting, which rules out the possibility that a newly synthesized truncated form of EAAC1 without signal peptides accumulated around the Golgi complex. Also, in vitro study showed a rapid change of localization from the plasma membrane to the perinuclear vesicles within 1 hour. Further studies such as pulse-chase or protein synthesis inhibitor experiments may support our hypothesis. Previous articles regarding KA-induced rat epilepsy have not addressed this phenomenon, presumably because it occurs at the restricted time point of 6 hours after KA injection. Immunoelectron microscopic study disclosed that perinuclear deposits of EAAC1 immunoreactivity were located at the Golgi complex. Although clathrin-mediated internalization of acetylcholine³² or a dopamine transporter³³ is suggested, EAAC1 trafficking from the cell surface to the Golgi complex has not been reported. It has been suggested that Golgi serves not only as a secretory traffic but also a signaling platform for membrane sorting.³⁴ Interaction between EAAC1 and a variety of Golgi-associated proteins should be explored.

In the KA-treated brain, the EAAC1 translocation to the Golgi complex was observed in a subset of neurons, especially large pyramidal neurons, and was not seen in the astrocytes. In the astrocytes and GABAergic interneurons, glutamate can be changed to glutamine or GABA by glutamine synthetase and glutamic acid decarboxylase, respectively. Alternatively, intracellular glutamate concentration may be regulated by the internalization of EAAC1 in the glutamatergic neurons, which are devoid of glutamine synthetase and glutamic acid decarboxylase (Figure 7) .

View larger version (39K): [in this window] [in a new window]   Figure 7. Glutamate metabolism in the environment of high extracellular glutamate. A: In the astrocytes, glutamate (Glu) through GLAST and GLT-1 is changed into glutamine (Gln) by glutamine synthetase (GS). B: In the GABAergic neurons, glutamate through EAAC1 is changed to GABA by glutamic acid decarboxylase. C: Glutamatergic neurons, which do not contain glutamine synthetase or glutamic acid decarboxylase, were observed mainly in the translocation of EAAC1 proteins. As a result, excessive glutamate uptake or reverse glutamate transport is attenuated in the neurons.

It has been suggested that membrane trafficking regulates the activity of the neurotransmitter-transporting proteins including dopamine^33,35,36 and acetylcholine.³² In vitro studies demonstrated that preincubation with PMA causes increase in EAAC1-mediated [³H] L-glutamate transport activity and cell surface expression of EAAC1 in C6 glioma cells.^19,20 Although C6 glioma cells are not a model for neurons, we used these cells as a model of EAAC1 trafficking in general because cultured hippocampal neurons express both EAAC1 and GLT-1,²² and only C6 glioma cells showed high glutamate uptake as well as selective expression of EAAC1 among the nonneuronal cell lines including HeLa, CHO, and others in the preliminary studies (Dr. Isao Nagano, personal communication). In our result, the transporter currents were recorded after treatment of the cells with PMA by the whole cell patch-clamp method, which were reduced by KA treatment in accordance with the internalization of EAAC1. These results indicated that the translocation of EAAC1 induced by KA treatment modulated the glutamate uptake via EAAC1 regardless of cell type.

Regulation of EAAC1 Protein during Epilepsy

There may be several pathways to negatively modulate EAAC1 protein function other than the down-regulation of EAAC1 mRNA. Recently, the EAAC1-associated protein, GTRAP3–18, which leads to decreased EAAC1 activity has been identified.³⁷ Because GTRAP3–18 modulates EAAC1 transporter activity by lowering substrate affinity without altered protein trafficking, translocation of EAAC1 is thought to be a different mechanism to regulate EAAC1 proteins. It is conceivable that EAAC1 internalization is important for the rapid regulation of high-affinity glutamate uptake after the propagation of seizures. Because EAAC1 runs in reverse in vitro when ionic gradients are disrupted by such as pathological conditions,³⁸ EAAC1 internalization may have a role at preventing the excessive uptake or reverse transport of glutamate. During the EAAC1 translocation, which helps to minimize epileptic injury in pyramidal neurons, the astrocytic glutamate transporters, GLT-1 and GLAST, may undergo enough total glutamate uptake from the synaptic cleft. This EAAC1 protein translocation may provide a novel mechanism for neuronal protection against excitotoxicity.

Acknowledgements

We thank Dr. Isao Nagano for helpful comments, Ms. Kazue Hatanaka and Ms. Mikiko Sato at the Department of Neuropathology and Mr. Takaaki Kanemaru at the Morphology Core of Kyushu University for their excellent technical assistance, and Mr. Robert Debold for editing our manuscript.

Footnotes

Address reprint requests to Akiko Furuta, M.D., Ph.D. (Current address of A.F.), Department of Degenerative Neurological Diseases, National Institute of Neuroscience, National Center of Neurology and Psychiatry, 4-1-1, Ogawahigashi, Kodaira, Tokyo 187-8502, Japan. E-mail: afuruta{at}ncnp.go.jp

Supported by the Ministry of Education, Culture, Sports, Science, and Technology [grant-in-aid for scientific research (C) no. 13680824] and the Clinical Research Foundation (1999) of Japan.

Accepted for publication May 4, 2003.

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