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Previous Article | Next Article
The Journal of Neuroscience, May 1, 2003, 23(9):3623
Scaffolding of Fyn Kinase to the NMDA Receptor Determines Brain Region Sensitivity to Ethanol
Rami Yaka, Khanhky Phamluong, and Dorit Ron Ernest Gallo Research Center and the Department of Neurology, University of California San Francisco, Emeryville, California 94608
ABSTRACT
TOP
ABSTRACT
Introduction
Alcohol (ethanol) abuse is a major societal problem. Although ethanol is a structurally simple, diffusible molecule, its sites of action are surprisingly selective, and the molecular mechanisms underlying specificity in ethanol actions are not understood. The NMDA receptor channel is one of the main targets for ethanol in the brain. We report here that the brain region-specific compartmentalization of Fyn kinase determines NMDA receptor sensitivity to ethanol. We demonstrate that, in the hippocampus but not in the cerebral cortex, Fyn is targeted to the NR2B subunit of the NMDA receptor by the scaffolding protein RACK1. During acute exposure to ethanol, RACK1 is dissociated from the complex, thereby facilitating Fyn-mediated phosphorylation of NR2B, which enhances channel activity, counteracting the inhibitory actions of ethanol. In this way, the selective scaffolding can account for the ethanol-induced acute tolerance of NMDA receptor activity that is detected in the hippocampus but not in the cerebral cortex. The phosphorylation-dependent, region-specific activities of ethanol on the NMDA receptor provide a compelling molecular explanation that accounts for the selective activities of ethanol and may have important implications for elucidating pathways leading to alcohol addiction.
Key words: ethanol; NMDA; RACK1; Fyn; tyrosine phosphorylation; scaffolding proteins
Introduction
The major excitatory neurotransmitter in the brain, glutamate, binds to the ligand-gated ion receptor channel NMDA (Sucher et al., 1996
). The NMDA receptor (NMDAR) is a major target of ethanol. The activities of ethanol on the NMDAR are important contributors to the development of disease states associated with alcohol abuse such as tolerance, dependence, withdrawal, craving, and relapse (for review, see Chandler et al., 1998
NMDARs are heteromers composed of an obligatory NR1 subunit and combinations of different NR2 (A-D) subunits (Sucher et al., 1996
/
Important regulators of the phosphorylation state of NMDAR subunits are scaffolding proteins. Scaffolding proteins provide both spatial organization and specificity of signaling cascades (Pawson and Scott, 1997
Materials and Methods
Reagents. The polyclonal anti-NR2B, anti-NR2A, anti-actin, and anti-Fyn antibodies and Fyn blocking peptide were purchased from Santa Cruz Biotechnologies (Santa Cruz, CA). The monoclonal anti-phosphotyrosine, anti-RACK1, anti-PSD95, and anti-NR2B antibodies were purchased from Transduction Laboratories (Lexington, KY). The monoclonal anti-hemagglutinin (HA) antibodies were purchased from Roche (Nutley, NJ). The monoclonal anti-NR1 antibodies were purchased from Zymed (South San Francisco, CA). The monoclonal anti-MAP2 (microtubule associated protein-2) and polyclonal anti-NR2B antibodies were purchase from Chemicon (Temecula, CA). The polyclonal anti-(pY1336)NR2B, anti-(pY1252)NR2B, and anti-(pY1472)NR2B antibodies were described previously (Takasu et al., 2002
Recombinant proteins. RACK1 was subcloned into pTAT-HA and expressed in Escherichia coli as described previously (He et al., 2002
Preparation of slice and brain homogenates. Experimental protocols involving the use of vertebrate animals were approved by the Gallo Research Center subcommittee on Research Animal Care and met National Institutes of Health guidelines.
For slice homogenates preparation, transverse hippocampal or coronal cerebral cortical slices (350-400 µm) were prepared from 3- to 4-week-old male Sprague Dawley rats (Simonsen Laboratories, Gilroy, CA). Slices were maintained for 2 hr in artificial CSF (aCSF) that contained the following (in mM): 126 NaCl, 1.2 KCl, 1.2 NaH2PO4, 0.01 MgCl2, 2.4 CaCl2, 18 NaHCO3, and 11 glucose (saturated with 95%O2-5%CO2) at 25°C. After recovery, slices were treated and homogenized in homogenization buffer (HB) [320 mM sucrose, 10 mM Tris-HCl, pH 7.4, 10 mM EDTA, 10 mM EGTA, protease inhibitor mixture (Roche), and phosphatase inhibitor mixture (Sigma)]. Homogenates were centrifuged at 5000 × g. The pellet was resuspended in solubilization buffer (10 mM Tris-HCl, pH 7.4, 10 mM EDTA, 10 mM EGTA, and protease and phosphatase inhibitor mixtures) that includes 1% Triton X-100 for phosphorylation assays or 1% deoxycholate for association assays. The suspension was then centrifuged at 60,000 × g to yield supernatant (soluble material) and pellet (insoluble material).
For brain homogenates preparation (in vivo), 3- to 4-week-old SVJ/129 male mice (Charles River Laboratories, Wilmington, MA) were intraperitoneally injected with saline or ethanol (3.5 gm/kg) for the time indicated in the figure legends. The cerebral cortex and hippocampus were dissected immediately and frozen in liquid nitrogen. Samples were homogenized and solubilized as described above.
Subcellular fractionation. Tissue from 3- to 4-week-old male rats was homogenized as described previously (Huttner et al., 1983
Immunoprecipitation. The supernatant soluble material from slice or brain homogenates were precleared by incubation with protein G agarose. The samples were centrifuged, and protein quantity was determined using BCA reagent. Immunoprecipitation was performed with 5 µg of the appropriate antibody, with ~0.5 mg of protein diluted in 1× immunoprecipitation buffer [1% Triton X-100, 150 mM NaCl, 10 mM Tris HCl, pH 7.4, 1 mM EDTA, 1 mM EGTA, 0.2 mM sodium orthovanadate, protease inhibitor mixture (Roche), and phosphatase inhibitor mixture (Sigma)]. After overnight incubation at 4°C, protein G agarose was added, and the mixture was incubated at 4°C for 2 hr. The protein G was washed extensively, and pellets were resolved on a 10% SDS-PAGE.
Western blot analysis. Fifty micrograms of protein were resolved on a 10% SDS-PAGE and transferred to a nitrocellulose membrane. Membranes were probed with the appropriate antibodies, and immunoreactivity was detected with enhanced chemiluminescence and processed using the STORM system. Digitized images of the bands corresponding to NMDAR subunits were quantitatively analyzed by densitometry, with NIH Image version 1.61 providing peak areas, and values were expressed as a ratio of phosphorylated to total amount of immunoprecipitated NMDAR subunits or actin as indicated in the figure legends. Statistical analysis was performed using Student's t test for significant differences.
In vitro translation assay. [35S]methionine-labeled proteins were generated in rabbit reticulocyte lysates (TNT kit; Promega, Madison, WI) programmed with cDNAs encoding the cytoplasmic tail of NR2B (amino acids 839-1482), Fyn, and RACK1 as described previously (Yaka et al., 2002
In vitro kinase assay. Fyn (10 U, 0.32 pmol · min
[32P]ATP, and 125 µM cold ATP) at room temperature for 20 min. Aliquots of the reaction were spotted onto P81 paper, Fyn activity was measured using scintillation counting, and specific activity was expressed as pmol of phosphorylation per minute per units of Fyn.
Immunohistochemistry. Three- to 4-week-old male rats were anesthetized and perfused with 4% paraformaldehyde. Brains were removed and sectioned on a vibratome (VT1000S; Leica, Nussloch, Germany). Slices (35 µm) that contained the hippocampus and cerebral cortex were blocked in PBS containing 0.1% Triton X-100 and 10% normal goat serum for 1 hr at room temperature. Blocking solution was aspirated, and sections were then double stained with anti-RACK (1:500) and anti-MAP2 (1:250) antibodies, anti-RACK1 (1:500) and anti-Fyn (1:250) antibodies, and anti-RACK1 (1:500) and anti-NR2B (1:250) antibodies overnight at 4°C. Antibodies were then aspirated, and sections were washed three times in PBS containing 0.1% Triton X-100. Sections were incubated for 2 hr at room temperature with the following secondary antibodies: Texas Red-conjugated antibody (goat anti-mouse IgM for RACK1; 1:250) and FITC-conjugated antibody (goat anti-mouse IgG for MAP2 and goat anti-rabbit IgG for Fyn and NR2B; 1:250). Sections were then washed and mounted on Fisher Superfrost glass slides. Slides were mounted using Vectashield and viewed with a Zeiss (Oberkochen, Germany) LSM-1024 laser-scanning microscope. The confocal images were processed using Adobe Photoshop (Adobe Systems, San Jose, CA). Specificity of RACK1 staining was confirmed by preabsorbing anti-RACK1 antibodies with recombinant RACK1 as described previously (Ron et al., 2000
Blood ethanol determination. Blood samples of ~50 µl were obtained from the tail vein of SVJ/129 male mice 15 min after intraperitoneal injection of 3.5 gm/kg ethanol. Blood ethanol concentration was determined using the Sigma Alcohol Diagnostic kit 332.
Electrophysiology. Transverse hippocampal or coronal cerebral cortical slices (350-400 µm) were prepared from 3- to 4-week-old male Sprague Dawley rats (Simonsen Laboratories). Slices were maintained for at least 2 hr in aCSF that contained the following (in mM): 126 NaCl, 1.2 KCl, 1.2 NaH2PO4, and 0.01 for fEPSPs) or 1.2 (for EPSCs) MgCl2, 2.4 CaCl2, 18 NaHCO3, and 11 glucose (saturated with 95%O2-5%CO2 at 25°C). After recovery, slices were submerged and continuously superfused with aCSF at 25°C.
Field recording-field EPSPs (fEPSPs) were recorded from stratum radiatum of CA1 region or layers II-III of the prefrontal cortex with glass microelectrodes filled with 2 M NaCl. To obtain NMDAR-mediated fEPSPs, picrotoxin (100 µM) and NBQX (10 µM) were added to the bath solution. To evoke fEPSPs, Schaffer collateral/commissural (hippocampus) or horizontal (cortex) afferents were stimulated with 0.1 Hz pulses using steel bipolar microelectrodes at intensities adjusted to produce an evoked response that was 50% of the maximum recorded fEPSP for each recording. The maximal rate of change in fEPSP within a time window selected around the rising phase was calculated.
Whole-cell recording-somatic whole-cell voltage-clamp recordings were made from CA1 pyramidal cells using 3-6 M
electrodes. The whole-cell solution contained the following (in mM): 117 cesium methansulfonic acid, 2.8 NaCl, 20 HEPES, 0.4 EGTA, 5 TEA-Cl, 2.5 MgATP, and 0.25 MgGTP, pH 7.2-7.4 (285-295 mOsm). To obtain NMDAR-mediated EPSCs, picrotoxin (100 µM) and NBQX (10 µM) were added to the bath solution. Cells were held at +40 mV, and series and input resistances were monitored continuously with a 4 mV depolarizing step, given with every afferent stimulus. The amplitudes of EPSCs were measured using a window at the peak of the event, relative to the baseline taken immediately before the stimulus artifact.
Data were collected using an Axopatch-1D amplifier (Axon Instruments, Foster city, CA), filtered at 2 kHz, and digitized at 5-10 kHz. Bath application of ifenprodil (25 µM) in hippocampal or cortical slices inhibited NMDAR-mediated fEPSPs by nearly 90%, confirming high levels of NR2B-containing NMDARs (data not shown).
Results
Region-specific compartmentalization of Fyn determines the activity of ethanol
We recently found that in the hippocampus, the scaffolding protein RACK1 interacts with the tyrosine kinase Fyn and its substrate, the NR2B subunit of the NMDAR, and prevents Fyn phosphorylation of NR2B. During release of RACK1 from the complex, Fyn phosphorylates the channel, and, as a consequence of the phosphorylation, the activity of the channel is enhanced (Yaka et al., 2002
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Figure 1. A-C, In the hippocampus, Fyn is compartmentalized to NR2B via RACK1, and ethanol induced the dissociation of the tri-molecular complex. A, Rat hippocampal slices were treated without (control) or with 25 and 100 mM ethanol for 30 min. Immunoprecipitations (IPs) were performed with anti-RACK1 and anti-mouse IgM antibodies as control. Membranes were probed with anti-NR2B, anti-Fyn, and anti-RACK1 antibodies. Histogram depicts the mean ± SD level of Fyn and NR2B dissociation normalized to immunoprecipitated RACK1 (n = 4). B, Rat hippocampal slices were treated as in A, and samples were resolved on SDS-PAGE. Membranes were probed with anti-NR2B and anti-Fyn antibodies (n = 4). C, Three- to 4-week-old SVJ/129 male mice were injected intraperitoneally (IP) with saline or 3.5 gm/kg ethanol. Fifteen minutes later, the hippocampus was dissected, and immunoprecipitation was performed with anti-RACK1 antibodies and probed with anti-NR2B, anti-Fyn, and anti-RACK1 antibodies (n = 3). D, E, In the cerebral cortex, Fyn associated with RACK1 but not with NR2B, and ethanol did not affect the association. D, Rat cortical slices were treated with 100 mM ethanol for 30 min, immunoprecipitated, and probed as in A (n = 3). E, Mice were injected intraperitoneally with saline, and cortical tissues were harvested and analyzed as in C (n = 3).
Next, we determined whether acute administration of ethanol in vivo would induce the dissociation of RACK1 from NR2B and Fyn. To do so, mice were systemically treated with 3.5 gm/kg ethanol by intraperitoneal injection, and, 15 min after injection, blood alcohol concentration was measured, the hippocampus was dissected, and the presence of the complex was assessed. We found that intraperitoneal injection of 3.5 gm/kg ethanol produced blood alcohol concentration of 72 ± 3.3 mM (n = 5), and, at this concentration of ethanol, dissociation of the complex was observed (Fig. 1C).
Unexpectedly, we found that the NR2B-RACK1-Fyn tri-molecular complex did not exist in the cerebral cortex, in slices or in vivo (Fig. 1D,E). RACK1 associated only with Fyn in the cortex, and their interaction was not affected by ethanol (Fig. 1D). In summary, in the hippocampus, where RACK1 scaffolds Fyn to the NMDAR, ethanol exposure induced the dissociation of the tri-molecular complex.
RACK1 is compartmentalized to the dendrites in the hippocampus but not in the cortex, and ethanol-induced dissociation of RACK1 from NMDAR complex is mediated via protein kinase A signaling
We hypothesized that the NR2B-RACK1-Fyn complex does not exist in the cortex because of differences in RACK1 compartmentalization in the two brain regions. To test the hypothesis, the localization of RACK1 in hippocampal and cortical slices was determined by immunohistochemistry and confocal microscopy. Double labeling of anti-RACK1 antibodies and the antibodies for the dendritic marker MAP2 revealed that RACK1 is localized to dendrites of CA1 pyramidal neurons as seen by the orange color that resulted from the merged staining of RACK1 (red) and MAP2 (green) (Fig. 2A, top panel, left).
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Figure 2. A, B, RACK1 is compartmentalized differently in hippocampus and cerebral cortex. A, Representative sections of rat hippocampal and cortical slices (35 µM) double stained with anti-RACK1 and anti-MAP2 (top panels), anti-NR2B (middle panels), and anti-Fyn (bottom panels) antibodies as described in Materials and Methods. Slices were visualized with laser-scanning confocal microscope at 63× magnification and presented as merged images. Images were taken from the CA1 region of the hippocampus, including the stratum radiatum (SR) and layers II-III of cerebral cortex. B, Subcellular fractionation of rat hippocampal and cortical tissue was performed as described in Materials and Methods. Crude synaptosomal fraction (P2) and cytosolic and light membranes fraction (S2) were resolved on 10% SDS-PAGE, and membranes were probed with anti-RACK1 antibodies. To ensure the integrity of fractionation, membranes were probed with anti-PSD95 antibodies. C, D, Ethanol activities on the NR2B-RACK1-Fyn complex are not direct. C, [35S]Methionine-labeled proteins were generated in rabbit reticulocyte lysates. Translated proteins were incubated in the absence or presence of 100 mM ethanol for 30 min at room temperature. Interaction of the proteins was determined by coimmunoprecipitation from the lysates with anti-RACK1 antibodies. Control immunoprecipitation with anti-IgM and an aliquot of the triple translation reaction ( of reaction volume; Input) are also included; n = 3. D, Fyn kinase (10 U; 0.32 pmol/min/U) was incubated with Src/Fyn substrate peptide (150 µM) and increasing concentration of ethanol (25-100 mM) for 20 min at 20°C. Histogram depicts mean ± SD of Fyn-specific activity of three experiments. E, Ethanol-induced dissociation of RACK1 from NMDA receptor complex is mediated via PKA signaling. Rat hippocampal slices were preincubated with vehicle or with H89 (10 µM) for 30 min at room temperature. Slices were then treated with ethanol (100 mM) for an additional 30 min and homogenized, and immunoprecipitation (IP) was performed with anti-RACK1 antibodies and anti-mouse IgM antibodies as control. Membranes were probed with anti-NR2B, anti-Fyn, and anti-RACK1 antibodies. Histogram depicts the mean ± SD level of Fyn and NR2B dissociation normalized to immunoprecipitated RACK1 (n = 3). **p < 0.01 indicates significantly lower than EtOH plus H89; t test.
However, in cortical neurons, RACK1 was mainly localized to the cell soma (Fig. 2A, top panel, right). Similar results were obtained when RACK1 distribution was compared in primary hippocampal and cortical cultures (data not shown). Double staining of anti-RACK1 and anti-NR2B antibodies revealed colocalization of the two proteins in CA1 hippocampal dendrites, as seen by the orange color that resulted from the merged staining of RACK1 (red) and NR2B (green) (Fig. 2A, middle panel, left). Colocalization between RACK1 and NR2B was not observed in cortical neurons (Fig. 2A, middle panels). When staining anti-RACK1 together with anti-Fyn antibodies, we found that RACK1 is partly colocalized with Fyn in the cell soma in both hippocampus and cortex; however, dendritic colocalization was observed only in the hippocampus (Fig. 2A, bottom panels). In addition, we performed subcellular fractionation and compared the levels of RACK1 in the crude synaptosomal fraction from hippocampus and cortex. As shown in Figure 2B, RACK1 levels in the crude synaptosomal fraction (P2) was higher in the hippocampus compared with cortex. Together, these results therefore suggest that, in the cortex, RACK1 is not localized in close proximity to NR2B and therefore is not capable of localizing Fyn to the NMDAR.
Next, we set out to identify a possible mechanism by which ethanol induces the dissociation of RACK1 from the NMDAR complex in the hippocampus. First, we determined whether ethanol affects the binding of RACK1 to NR2B and Fyn using an in vitro translation assay. As shown in Figure 2C, and as reported previously (Yaka et al., 2002
We found previously that ethanol induces the movement of RACK1 to the nucleus, and ethanol-induced RACK1 nuclear translocation was mediated through a mechanism that requires cAMP-dependent protein kinase (PKA) (Ron et al., 2000
Ethanol induces phosphorylation of NR2B but not NR2A in the hippocampus but not in the cortex
Previously, we found that the release of RACK1 from Fyn and NR2B enables Fyn to phosphorylate the subunit (Yaka et al., 2002
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Figure 3. Acute exposure to ethanol increased tyrosine phosphorylation of the NR2B but not NR2A in the hippocampus. A, Rat hippocampal slices were homogenized and solubilized as described in Materials and Methods, and immunoprecipitations (IPs) were performed with anti-NR2A, anti-NR2B, and anti-NR1 antibodies. Membranes were probed with anti-NR2A, anti-NR2B, and anti-NR1 antibodies. Control hippocampal homogenate was also included (n = 3). B, Rat hippocampal slices were treated with vehicle (DMSO, 1:20,000) or ethanol (100 mM) with or without PP2 (50 nM) for 30 min. Immunoprecipitations were performed with anti-NR2B or anti-NR2A antibodies and probed with anti-NR2B, anti-NR2A, and anti-phosphotyrosine (pY) antibodies. Histogram depicts quantification of the level of tyrosine phosphorylation of NR2B and NR2A. Data are presented as mean ± SD percentage of control (n = 3). **p < 0.01; t test. C, Mice were injected intraperitoneally with saline or 3.5 gm/kg ethanol. The hippocampus was dissected, homogenized, and resolved by SDS-PAGE. Membranes were probed with the anti-phoshpo-NR2B-specific antibodies (pTyr1252)NR2B, anti-(pTyr1336)NR2B, and anti-(pTyr1472)NR2B and anti-actin antibodies. Histogram depicts quantification of the levels of NR2B phosphorylation normalized to actin and presented as mean ± SD percentage of control (n = 3). D, Rat hippocampal slices were preincubated with PBS or with Tat-RACK1 (1 µM) for 2 hr. Slices were then treated with vehicle or ethanol (100 mM) for 30 min, homogenized, and resolved by SDS-PAGE. To ensure transduction of the Tat-fusion protein, membranes were probed with anti-RACK1 (middle panel) and anti-HA (bottom panel) antibodies. Membranes were probed with anti-(pTyr1252)NR2B and anti-actin antibodies. Histogram depicts quantification of the levels of phosphorylation normalized to actin and presented as mean ± SD percentage of control (n = 3). **p < 0.01; t test.
Next, we predicted that, if ethanol-induced NR2B phosphorylation is mediated via the release of RACK1 from the NMDAR complex, then the transduction of recombinant RACK1 into hippocampal slices would reverse the activities of ethanol by binding to Fyn and/or NR2B and blocking the phosphorylation of NR2B by Fyn. To test this hypothesis, we used the Tat-protein transduction method (Nagahara et al., 1998
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Figure 5. The PTK inhibitor PP2 increases ethanol-induced inhibition of NMDAR-mediated fEPSPs-EPSCs and inhibits ethanol-induced rebound potentiation in hippocampal slices. A, NMDAR-mediated fEPSP slopes were plotted for recordings made from the stratum radiatum in the CA1 region. fEPSPs were measured in the presence of PP2 (25 nM, ; n = 6 slices), ethanol (100 mM,
; n = 10) or ethanol plus PP2 (
; n = 6), as indicated by the horizontal bar. Data are presented as the mean ± SEM percentage of baseline. The traces in the inset represent NMDA receptor fEPSPs in the CA1 field (average of 12 single sweeps) obtained from the following: left, a slice recorded before (baseline) and during application of ethanol; right, a slice recorded before (baseline) and during coapplication of ethanol and PP2. Histogram on the right shows comparison of fEPSPs at 20 min (peak inhibition) and 30 min (10 min after ethanol washout). Two-way repeated-measures ANOVA showed overall significant interactions between treatments and time points (F(4,16) [infi] = 5.87; p < 0.006). Post hoc analysis showed significant effects of PP2 on ethanol inhibition (20 vs 30 min; *p < 0.02; Student-Newman-Keuls test) and on ethanol-induced rebound potentiation (20 vs 30 min; *p < 0.019; Student-Newman-Keuls test). B, NMDAR-mediated fEPSPs were measured in the CA1 region in the presence of ethanol (100 mM), followed by washout and a subsequent second application of ethanol and washout with PP2 (25 nM), as indicated by the horizontal bars. Data are presented as the mean ± SEM percentage of baseline from six slices. The traces in the inset represent NMDA receptor fEPSPs in the CA1 field (average of 12 single sweeps) obtained from the follow ing: a, a slice recorded before application of ethanol; b, during application of ethanol; c, after ethanol washout. Histogram shows the mean ± SEM fEPSPs slope recorded at 26 min (peak rebound potentiation, 6 min after ethanol washout) or 51 min (6 min after the start of washout with PP2). **p < 0.01; paired t test. C, Time course of NR2B phosphorylation correlates with recordings. Rat hippocampal slices were incubated without (control) or with (100 mM) ethanol for 10, 20, and 30 min. Slices were homogenized and resolved by SDS-PAGE. Membranes were probed with anti-(pTyr1336)NR2B and anti-NR2B antibodies. Histogram depicts quantification of the levels of phosphorylation normalized to NR2B and are presented as mean ± SD percentage of control (n = 3). D, NMDAR-mediated EPSCs were plotted for recordings made using standard whole-cell voltage clamp from CA1 pyramidal neurons (n = 5). EPSCs were measured in the presence of ethanol (100 mM), followed by washout, as indicated by the horizontal bars. The traces in the inset represent NMDA receptor EPSCs in the CA1 field (average of 12 single sweeps) obtained from the following: a, a neuron recorded before application of ethanol; b, during application of ethanol; c, after ethanol washout. D, NMDAR-mediated EPSCs were recorded in the presence of PP2 (25 nM) in the recording pipette. Ethanol (100 mM) was bath applied as indicated by the horizontal bar, followed by washout (n = 5). The traces in the inset represent NMDA receptor EPSCs in the CA1 field (average of 12 single sweeps) obtained from the following: a, a neuron recorded before application of ethanol; b, during application of ethanol.
As predicted, in the cerebral cortex where Fyn was not localized to the NMDAR (Fig. 1D,E), no change in the phosphorylation state of the NR2B subunit was detected after ethanol treatment (Fig. 4, top panels). In summary, our results suggest that, in the hippocampus, ethanol releases RACK1 from Fyn and NR2B and enables Fyn to phosphorylate the subunit. Importantly, ethanol-induced phosphorylation of the NR2B subunit is brain region specific and is observed in the hippocampus but not in the cortex where RACK1 localized to the NMDAR and presumably is not localizing Fyn near its substrate.
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Figure 4. Acute exposure to ethanol does not affect the phosphorylation state of either NR2B and NR2A in the cortex. Rat cortical slices were treated as in Figure 1A and homogenized, and immunoprecipitation (IP) was performed using anti-NR2B or anti-NR2A antibodies. Membranes were probed with anti-NR2B, anti-NR2A, and anti-phosphotyrosine (pY) antibodies. Histogram depicts quantification of the level of phosphorylation. Data are presented as mean ± SD percentage of control (n = 3).
Another NMDAR subunit that is phosphorylated on tyrosine residues is NR2A (Lau and Huganir, 1995
In the hippocampus, ethanol increases NMDAR channel activity and produces a rebound potentiation when ethanol is no longer present
Next, we assessed the physiological consequences of ethanol-induced NR2B tyrosine phosphorylation. Previous studies have shown that acute exposure to ethanol inhibits the activity of the NMDAR channel in hippocampal slice preparation (Lovinger et al., 1989
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Figure 6. In the cortex, PP2 is inactive, ethanol inhibition is greater compared with the hippocampus, and acute tolerance to ethanol inhibition does not develop. A, NMDAR-mediated fEPSP slopes were plotted for recordings made from layers II-III in the medial prefrontal cortex. fEPSPs were measured in the presence of ethanol (100 mM), followed by washout and subsequent application of ethanol plus PP2, as indicated by the horizontal bar. Data are presented as the mean ± SEM percentage of baseline from seven slices. The traces in the inset represent NMDA receptor fEPSPs in the CA1 field (average of 12 single sweeps) obtained from the following: a, a slice recorded before application of ethanol; b, during application of ethanol; c, during coapplication of ethanol and PP2. B, Histogram depicting the mean ± SEM ratio of fEPSP slopes recorded from hippocampal or cortical slices at the time of maximal effect of ethanol treatment (10 and 15 min, respectively). **p < 0.01; t test. C, NMDAR-mediated fEPSP slopes were measured in the CA1 region in the presence of 100 mM ethanol and in the absence ( ; n = 6) or after 2 hr preincubation of hippocampal slices with Tat-RACK1 (1 µM) in the bath solution (
; n = 5). Horizontal line depicts the period of ethanol application. Data are presented as the mean ± SEM percentage of baseline.
In the cortex, ethanol exposure does not result in enhancement of NMDAR channel activity, and rebound potentiation is not observed
Next, we tested the activities of ethanol on NMDAR function in the cortex, where RACK1 was not associated with the channel (Figs. 1D,E, 2A,B), and ethanol did not induce the phosphorylation of NMDAR subunits (Fig. 4). In the cortex, like the hippocampus, ethanol inhibited NMDAR-mediated fEPSP (Fig. 6A). However, unlike in the hippocampus, PP2 had no effect on fEPSPs in the presence of ethanol, and potentiation of NMDAR-mediated fEPSPs after ethanol washout was not observed (Fig. 6A). Furthermore, we observed that the peak inhibition of NMDAR-mediated fEPSPs in the presence of ethanol was significantly greater in cortical slices compared with hippocampal slices (Fig. 6B) (47.9 ± 6.4 vs 30.3 ± 2.6%; p < 0.01; t test). Together, these results suggest that the sensitivity of NMDARs to ethanol varies across brain regions and is determined, at least in part, by the scaffolding of Fyn to the NMDAR via RACK1 and the resulting phosphorylation state of the channel.
Acute tolerance of NMDAR function is determined by Fyn compartmentalization
Previous studies have demonstrated that ethanol-induced inhibition of NMDAR function is gradually reduced during the period of ethanol exposure (acute tolerance) in the CA1 region of the hippocampus (Grover et al., 1994
We hypothesized that, in the cortex, where RACK1 does not scaffold the kinase to the NMDAR, acute tolerance would be absent. Indeed, in cortical slices, ethanol-induced inhibition of NMDAR-mediated fEPSPs was stable throughout the period of ethanol exposure (Fig. 6C, white diamonds). It is unlikely that presynaptic events are mediating the enhancement of NMDAR activities in the presence of ethanol. Ethanol and/or PP2 did not alter hippocampal AMPAR-mediated fEPSPs (data not shown), and PP2 have been shown to induce exocytosis in primary neurons, suggesting that Src PTKs are necessary for the inhibition of presynaptic exocytosis events (Ohnishi et al., 2001
Discussion
In the present study, we present evidence for the mechanism by which ethanol induces tyrosine phosphorylation of a specific NMDAR channel subunit, in a specific brain region, and we further show that these changes have important physiological consequences. In the hippocampus, RACK1 is localized in part to the dendrites where RACK1 scaffolds Fyn to the NMDAR at the plasma membrane. Ethanol releases RACK1 from the NMDAR complex, enabling Fyn to phosphorylate the NR2B subunit. These changes lead to phosphorylation-dependent enhancement of NMDAR channel activity during exposure to ethanol, to a rebound potentiation of the channel activity when ethanol is washed out, and to acute desensitization. However, in the cortex, where RACK1 is found mainly in the cell soma but not in the dendrites, Fyn is not associated with the NMDAR. In the cortex, ethanol exposure does not result in changes in the phosphorylation state of the NR2B subunit, and ethanol exposure leads only to the inhibition of the channel activity and not to acute desensitization or rebound potentiation after ethanol washout.
Since the first report by Lovinger et al. (1989)
Our results also suggest that the composition of PSD proteins is different in the cortex compared with the hippocampus. The differences in PSD protein composition between different brain regions may also result in different activities of the same neurotransmitter and receptor systems in different brain regions. Interestingly, several studies allude to such possibilities. For example, Mannaioni et al. (2001)
What could be the mechanism that accounts for RACK1 dissociation from the NMDAR complex during exposure to ethanol? We found previously that, in cultured cells and in vivo, ethanol induces RACK1 to translocate to the nucleus, via a mechanism that involves the activation of the cAMP-PKA pathway (Ron et al., 2000
Protein targeting and subcellular localization are very important for processes such as synaptic plasticity but may also contribute (as we show in this paper) to disease states such as alcohol addiction. It is well established that ethanol alters the function of certain kinases (Chandler et al., 1998
FOOTNOTES Received Nov. 19, 2002; revised Feb. 13, 2003; accepted Feb. 20, 2003.
This work was supported by the State of California for medical research on alcohol and substance abuse through the University of California, San Francisco (D.R.) and National Institute on Alcohol Abuse and Alcoholism Grant R01AA/MH13438-O1A1 (D.R.).We thank S. Dowdy for supplying the pTAT-HA plasmid and M. Greenberg for the phospho-NR2B antibodies. We thank A. Vagts and D. Nikanjam for the expression and purification of Tat-RACK1 and Viktor Kharazia for technical assistance. We thank our colleagues A. Bonci, M. Moore, F. Hopf, P. Janak, C. Thornton, M. Ungless, N. Vasquez, and J. Whistler for critical reading of this manuscript.
Correspondence should be addressed to Dorit Ron, 5858 Horton Street, Suite 200, Emeryville, CA 94608. E-mail: dorit{at}itsa.ucsf.edu.
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