Developmental Changes in Synaptic AMPA and NMDA Receptor Distribution and AMPA Receptor Subunit Composition in Living Hippocampal Neurons

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The Journal of Neuroscience, November 1, 2000, 20(21):7922-7931

Developmental Changes in Synaptic AMPA and NMDA Receptor Distribution and AMPA Receptor Subunit Composition in Living Hippocampal Neurons
Lisa Pickard, Jacques Noël, Jeremy M. Henley, Graham L. Collingridge, and Elek Molnar
Medical Research Council Centre for Synaptic Plasticity, Department of Anatomy, University of Bristol, School of Medical Sciences, University Walk, Bristol BS8 1TD, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

AMPA and NMDA receptors mediate most excitatory synaptic transmission in the CNS. We have developed antibodies that recognizeall AMPA or all NMDA receptor variants on the surface of livingneurons. AMPA receptor variants were identified with a polyclonalantibody recognizing the conserved extracellular loop region ofall four AMPA receptor subunits (GluR1-4, both flip and flop),whereas NMDA receptors were immunolabeled with a polyclonal antibodythat binds to an extracellular N-terminal epitope of the NR1 subunit,common to all splice variants. In non-fixed brain sections theseantibodies gave labeling patterns similar to autoradiographicdistributions with particularly high levels in the hippocampus.Using these antibodies, in conjunction with GluR2-specific andsynaptophysin antibodies, we have directly localized and quantifiedsurface-expressed native AMPA and NMDA receptors on cultured livinghippocampal neurons during development. Using a quantitative cellELISA, a dramatic increase was observed in the surface expressionof AMPA receptors, but not NMDA receptors, between 3 and 10 din culture. Immunocytochemical analysis of hippocampal neuronsbetween 3 and 20 d in vitro shows no change in the proportionof synapses expressing NMDA receptors (~60%) but a dramatic increase(~50%) in the proportion of them that also express AMPA receptors.Furthermore, over this period the proportion of AMPA receptor-positivesynapses expressing the GluR2 subunit increased from ~67 to ~96%.These changes will dramatically alter the functional propertiesof hippocampalsynapses.

Key words: glutamate; AMPA; NMDA; GluR; development; synapse; antibody; histoblot; hippocampal neurons; immunofluorescence; cellular ELISA

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ionotropic glutamate receptors (iGluRs) are the principal excitatory neurotransmitter receptors in the CNS. On the basis oftheir pharmacology and electrophysiology, iGluRs are classifiedas AMPA, kainate, and NMDA subtypes (Dingledine et al., 1999).AMPA and NMDA receptors participate in plastic changes in theefficacy of synaptic transmission, such as long-term potentiation(LTP; Bliss and Collingridge, 1993) and long-term depression (LTD;Bear and Abraham, 1996) and in the formation of neural networksduring development (Durand et al., 1996). AMPA receptors are composedof four subunits, GluR1-4. NMDA receptors comprise the essentialNR1 subunit and one or more of the modulatory NR2 subunits, NR2A-D(Hollmann and Heinemann 1994).

At developmentally early time points many excitatory synapses are thought to be postsynaptically "silent", possessing functionalNMDA but lacking functional AMPA receptors (Isaac et al., 1995,1997; Liao et al., 1995; Durand et al., 1996; Wu et al., 1996;Li and Zhuo, 1998). Such synapses have been termed "silent synapses"because the NMDA pore is largely blocked at resting membrane potentials(Mayer et al., 1984: Nowak et al., 1984). Following protocolsthat induce LTP, however, these functionally silent synapses rapidlybecome AMPA receptor-responsive (Isaac et al., 1995; Liao et al.,1995). One possible mechanism to explain this observation is thata pool of pre-assembled AMPA receptors can be moved from an intracellularcompartment to the postsynapticmembrane.

Antibodies that recognize extracellular epitopes and can thus label iGluRs on living neurons are important tools for the studyof receptor localization and dynamics. The first such antibody(Molnar et al., 1993) was used to compare the cell surface andintracellular distributions of GluR1 in cultured hippocampal neurons(Richmond et al., 1996) and provided anatomical evidence in supportof the "silent synapse" hypothesis. Antibodies against the sameregion of GluR1 and the N-terminal portion of GluR2 were usedto further investigate AMPA receptor localization and dynamics(Mammen et al., 1997; O'Brien et al., 1998b; Carroll et al., 1999;Liao et al., 1999; Lüscher et al., 1999). Using subunit-specificantibodies, however, it is not possible to distinguish betweenthe absence of AMPA receptors and the lack of a particular subuniton the cell surface. For this reason we have used an antibodythat recognizes all AMPA receptor subtypes on living neurons.Probes for studying NMDA receptors on living neurons are evenmore limited. Until now only fluorescently tagged conantokin-Ghas been used to observe NMDA receptor clusters (Benke et al.,1993; Durand et al., 2000). We have therefore developed an antibodythat labels NMDA receptors on livingneurons.

Here we describe the characterization and application of these antibodies to study the developmental profile of AMPA and NMDAreceptor surface expression. Our results support the view thatearly in development there are a large proportion of NMDA receptor-onlysynapses that subsequently acquire AMPA receptors. In addition,we have found a developmental increase in the relative ratio ofGluR2 compared to other AMPA receptor subunits on the neuronalsurface.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pfu DNA polymerase, BamHI, and HindIII were obtained from Stratagene (La Jolla, CA). All oligonucleotides were synthesizedby Cruachem (Glasgow, UK). Tissue-culture materials were purchasedfrom Life Technologies (Paisley, Strathclyde, UK). For solid phasepeptide synthesis, all reagents were purchased from Novabiochem(Nottingham, UK). All other reagents were from Sigma (Poole,UK).

Selection of sequences for antibody production. For production of pan-AMPA antibodies we used 25, 58, and 92 amino acid longsegments of the GluR1_flop sequence (residues 757-781, 724-781,and 690-781, respectively) preceding the last transmembrane domain(Hollmann et al., 1989). This region shows ~90% sequence homologywith all other AMPA receptor subunits (GluR2-4) and is thoughtto be extracellular (Cockcroft et al., 1993; Hollmann et al.,1994; Bennett and Dingledine, 1995). In the extracellular N-terminaldomain of the NR1 NMDA receptor subunit, a short unique regionwas identified (residues 436-450 in NR1a). This segment is believedto form a hydrophilic, surface-exposed, and flexible loop linkingconserved secondarystructures.

Expression and purification of glutathione S-transferase-GluR1flop fusion proteins. Three glutathione S-transferase (GST)fusion proteins containing 25, 58 and 92 amino acid residues precedingthe last membrane-spanning segment of GluR1_flop (Hollmann et al.,1989) were produced (Fig. 1A). DNA fragments encoding amino acidresidues 757-781, 724-781, and 690-781 of GluR1_flop were synthesizedby PCR. The sequences of the forward primers were: (S1) 5'-GCGGGATCCAAAACAAAAGGCAAATACGCC-3',(S2) 5'-GCGGGATCCGATTCC-AAAGGCTATGGC-3', (S3) 5'-GCGGGATCCCAGGGGCTTTTGGAC-3'.A common reverse primer was used for all these PCR reactions (AS5'-GCGCAAGCTTCAGCTGGTC-TTGTCCTT-GGA-3'). The primers containedsites for BamHI and HindIII (as indicated by the underlined sequences).The reverse primer also incorporated a stop codon at the 3'-endof the amplified sequence. PCR products were purified on a 10%acrylamide gel, digested with BamHI and HindIII, than purifiedagain on a 10% acrylamide gel, and ligated into a BamHI and HindIII-digestedpGEX-2TH bacterial expression vector (Pharmacia, Piscataway, NJ).GST fusion proteins were expressed in Escherichia coli strainHB101 competent cells (Promega, Madison, WI). After inductionand lysis, GST fusion proteins were purified on a glutathioneagarose column and analyzed by SDS-PAGE (Fig. 1B). The purifiedfusion proteins were dialyzed against 20 mM Tris-HCl, pH 7.5,2 mM MgCl₂, and 1 mM DTT and protein concentration was measuredwith the Lowry et al. (1951) assay. From selected clones, plasmidDNA was prepared, and the DNA sequence was confirmed by di-deoxyDNA sequencing using the Sequenase Quick-Denature plasmid-sequencingkit (United States Biochemical, Cleveland, OH) with a 5' pGEXsequencing primer (5'-GGGCTGGCAAGCCACGTTTGGTG-3'; Pharmacia).

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Figure 1. Antibodies raised against different segments of the GluR1_flop TM3-TM4 loop can be used to identify all known AMPA receptor subunit proteins. A, Site-directed antibodies were raised against three GST fusion proteins, containing amino acid residues 690-781 (I), 724-781 (II), and 757-781 (III) of GluR1_flop. The location of putative membrane-spanning domains [TM1-4 or A-C (Hollmann et al., 1994) are indicated in the figure]. B, The immunostaining of GST-GluR1_flop fusion proteins. GST fusion proteins (0.25 µg/lane), containing residues 757-781 (III), 724-781 (II), or 690-781 (I) of the GluR1_flop subunit, were either stained with Coomassie blue or immunostained with a polyclonal rabbit antibody raised against the GST-GluR1_757-781 fusion protein. C, Characterization of the subunit specificity of antibodies raised against residues 690-781, 724-781, and 757-781 of the GluR1_flop AMPA receptor subunit. Membrane proteins (30 µg/lane) from rat brain (RB) and transiently transfected COS-7 cells expressing either GluR1-4 (AMPA) or GluR5-7 (kainate) receptor subunits were immunostained with the indicated antibody (1 µg/ml). All four antibodies cross-react with all of the AMPA receptor subunit proteins (GluR1-4), and both flip and flop alternatively spliced isoforms of GluR1. The kainate receptor subunits (GluR5-7) were unlabeled.

Preparation of synthetic peptides and peptide-carrier protein conjugates for NR1 antibody production. Sequence correspondingto residues 436-450 of NR1a (Moriyoshi et al., 1991) was usedto prepare synthetic peptides. This sequence is identical in allknown NR1 splice variants (NR1a-g; Moriyoshi et al., 1991). TheN-terminal splice site (N1; 190-211) is far from the 436-450 segmentand therefore unlikely to interfere with antibody binding. TheNR1_436-450 peptide was coupled to mercaptosuccinylated ovalbumincarrier protein (Klotz and Heiney, 1962) via the N-terminal cysteineof the peptide, which was conjugated to 5-thio-2-nitrobenzoicacid beforecoupling.

Immunization and immunoaffinity purification of antibodies. Rabbits (two to four for each fusion protein) were injected subcutaneouslywith one of the purified GST fusion proteins (containing residues757-781, 724-781, or 690-781 of GluR1_flop), boosted every 4 weeks,and bled 10 d after each boost. Two guinea pigs were injectedsubcutaneously with the GST fusion proteins containing residues724-781 (0.1 mg), boosted every 2 weeks, and bled 7 d after eachboost. The antisera were preadsorbed using a Sepharose 4B columncoupled with the unfused GST protein. Subsequently, GluR1 portion-specificantibodies were affinity-purified with a Sepharose 4B column coupledwith the appropriate GST fusion protein containing residues 757-781,724-781, or 690-781 of GluR1_flop. The antibodies were eluted fromthe columns using a buffer containing 0.1 M glycine-HCl, pH 2.5.The elute was immediately neutralized by addition of 1/10 volumeof 1 M Tris-HCl, pH 8.0. The antibody solution was dialyzed againstPBS. All rabbits and guinea pigs immunized produced antibodiesrecognizing the fusion proteins and GluR1-4 subunit proteins intransfected COS-7 cells and rat brain membrane samples (Fig. 1B,C).

The ovalbumin-coupled NR1 peptide was coadsorbed with an adjuvant peptide (N-acetylmuramyl-L-alanyl-D-isoglutamine) to colloidalgold particles before immunization of New Zealand white rabbitsfollowing previously published protocols (Pow and Crook, 1993).The anti-NR1 antibody was immunoaffinity-purified using the cysteinecontaining synthetic peptide (5 mg) coupled to activated thiopropylSepharose 6B (Pharmacia). Other steps of the purification procedurewere performed as described above. Serum antibody titers and thebinding activity of the purified antibodies were analyzed usingELISA, as described previously (Molnar et al., 1993).

Dot-blot assay. The subunit specificity of the antibodies raised against the NR1_436-450 segment was tested using syntheticpeptides representing corresponding residues of NR2A, NR2B, NR2C,and NR2D (residues 439-453, 436-449, 450-464, and 465-477, respectively;Monyer et al., 1992; Cockcroft et al., 1993; Ishii et al., 1993).Nonconjugated synthetic peptides were dissolved in 13 mM sodiumcarbonate, 35 mM sodium bicarbonate, pH 9.6, and 0.1 µg/dot ofeach peptide was used to prepare nitrocellulose membranes forimmunoreaction. After drying, membranes were immersed in blockingsolution (5% nonfat dry milk and 1:50 dilution of normal swineserum in PBS) for 1 hr at 4°C. The membranes were then incubatedfor 2 hr with 1:200 dilution of the various antisera at room temperature.The bound antibodies were visualized by the enzymatic reactionof the alkaline phosphatase-conjugated anti-rabbit secondary antibody,as described previously (Molnar et al., 1993).

Preparation of membrane fractions from rat brain samples and transfected COS-7 cells. Membrane fractions were prepared fromdissected cortical, hippocampal, and cerebellar areas of maleWistar rats. Tissue samples were homogenized in 25 ml of 0.3 Msucrose and 20 mM Tris-HCl, pH 7.4, containing the following proteaseinhibitors: 2 mM DL-dithiothreitol (DTT), 1 µM pepstatin A, 1mM iodoacetamide, 1 mM phenylmethylsulfonyl fluoride (PMSF), 1mM 1,10-phenanthroline, 2 mM EDTA, and 2 mM EGTA at 2°C with aglass-Teflon homogenizer. The homogenate was centrifuged at 10,000× g for 15 min, and the microsomal fraction was collected by centrifugingthe first supernatant at 200,000 × g for 30 min. All pellets wereresuspended in the previously described buffer, snap-frozen inliquid nitrogen, and stored at $-$ 70°C untiluse.

The culturing of COS-7 cells, the transient transfection with cDNA coding for different ionotropic subunits, and the membranepreparation from transfected cells were performed as describedpreviously (McIlhinney and Molnar, 1996). All plasmids were preparedfor transfection studies using the Wizard Maxiprep plasmid kit(Promega). Protein concentrations in various membrane fractionswere estimated by the procedure of Lowry et al. (1951), usingBSA asstandard.

SDS-PAGE, electrophoretic transfer of proteins and immunoblot analysis. SDS-PAGE was performed on 7.5 or 10% gels (Laemmli,1970). Proteins were transferred electrophoretically onto polyvinylidenedifluoride microporous membrane (Immobilon; Millipore, Bedford,MA) using an Atto HorizBlot Electrophoretic Transfer Unit witha discontinuous buffer system for 1.5 hr at room temperature,as recommended by the manufacturer (Atto, Tokyo, Japan). Beforeimmunostaining, the Immobilon sheets were blocked overnight at4°C with 5% nonfat dry milk and 1:50 dilution of normal swineserum in PBS (blocking solution). The proteins on Immobilon sheetswere reacted with different affinity-purified antibodies (0.5-1µg/ml) in blocking solution for 12-16 hr at 4°C. The bound antibodieswere detected with either alkaline phosphatase- or horseradishperoxidase-conjugated anti-rabbit or anti-guinea pig IgG secondaryantibody, as described previously (Molnar et al., 1993; McIlhinneyand Molnar, 1996).

Histoblotting. The distribution of AMPA receptor subunits was analyzed in rat brain, using an in situ blotting technique (histoblot;Tönnes et al., 1999). In brief, horizontal cryostat sections(10 µm) from rat brain were apposed to nitrocellulose membranesmoistened with 48 mM Tris-base, 39 mM glycine, 2% SDS, and 20%methanol for 15 min at room temperature. After blocking in 3%fish skin gelatin, nitrocellulose membranes were DNase I-treated(5 U/ml), washed, and incubated in 2% SDS, 100 mM $beta$ -mercaptoethanolin 100 mM Tris-HCl, pH 7.0, for 60 min at 45°C to remove adheringtissue residues. After extensive washing, the blots were processedfor immunostaining as described forimmunoblotting.

Hippocampal cell cultures. Hippocampal cultures were prepared from 3- to 5-d-old rats as previously described (Richmond etal., 1996; Noel et al., 1999). Neurons were used for experiments3-5, 7-10, and 14-20 d afterplating.

Quantification of total and surface-expressed AMPA and NMDA receptor proteins in neuronal cultures using an ELISA-based assay(cell-ELISA). Hippocampal cells were grown on 6-well plates asdescribed above. Cells were fixed using 4% paraformaldehyde in50 mM phosphate buffer, pH 7.2, for 20 min at room temperature,and then washed three times with PBS. Cells were incubated with3% H₂O₂ in PBS for 5 min to minimize endogenous peroxidase activity.Cultures were incubated with blocking solution (5% fetal bovineserum and 1% BSA in PBS) in the presence and absence of 1% TritonX-100 for 30 min, and then with primary antibodies against GluR1-4or NR1 (1 µg/ml in blocking solution) for 1 hr at room temperature.The addition of 1% Triton X-100 was omitted for detection of surface-expressedproteins. Cells were washed three times with blocking solution,incubated with anti-rabbit peroxidase-conjugated secondary antibody(1:3000 dilution in blocking solution) for 1 hr at 25°C, and washedfour times in PBS. Samples in each well were incubated with 0.8ml of K-Blue substrate (Neogen) for 10 min, after which the coloredreaction end product was transferred from the plates into microfugetubes containing 0.2 ml 1 M HCl to stop the reaction. The opticaldensity of samples was determined at 450 nm. Control experimentswith preimmune serum, or plates without hippocampal cells, wereincluded routinely to determine background value, which was subtractedfrom the OD₄₅₀ readings. After the incubation with K-Blue substrate,cells were washed four times in PBS and solubilized in 0.2 ml0.5% SDS. Protein concentration was determined with the Pierce(Rockford, IL) BCA protein assay kit using BSA as standard. EachOD₄₅₀ value of the ELISA reaction was normalized to protein levels.For each experiment four parallel samples were used. The cellELISA approach was not possible with the anti-GluR2 monoclonalantibody (MAB397; Chemicon, Temecula, CA), because it did notwork on paraformaldehyde-fixedcells.

Immunofluorescence staining. The specificity of the purified anti-GluR1-4 antibodies was analyzed using transiently transfectedCOS-7 cells expressing AMPA receptor subunits. The anti-NR1 antibodywas tested using immunohistochemistry on human embryonic kidney(HEK) 293 cells transiently cotransfected with NR1 and NR2A subunits.The transfection and immunostaining procedure was performed asdescribed previously (McIlhinney and Molnar, 1996; McIlhinneyet al., 1996, 1998). Whereas untransfected COS-7 or HEK 293 cellsshowed no staining, transiently transfected COS-7 and HEK 293cells showed specific surface staining with the anti-GluR1-4 orNR1 antibodies,respectively.

For immunofluorescence experiments with living hippocampal neurons, the cells were washed twice with a HEPES-buffered saline(HBS; 119 mM NaCl, 5 mM KCl, 2 mM CaCl₂, 2 mM MgCl₂, 25 mM HEPES,30 mM glucose, and 0.5 µM TTX) heated to 37°C. The cells werelabeled with the following antibodies at 20°C in 5% dialyzed BSAin HBS: (1) rabbit or guinea pig polyclonal antibody to the conservedextracellular loop regions of all four GluR1-4 subunits (100 µg/ml),(2) rabbit polyclonal antibody directed against the N-terminalextracellular domain of NR1 (100 µg/ml), or (3) mouse monoclonalantibody to the N-terminal domain (amino acid residues 175-430)of GluR2 (100 µg/ml; MAB397, Chemicon; Vissavajjhala et al., 1996).We have verified that this antibody remains specific for GluR2during the immunofluorescence staining procedure (at 100 µg/mlconcentration) using HEK 293 cells transiently transfected witheither GluR2 or the closely related GluR1 AMPA receptor subunit(data notshown).

Incubation with the primary antibody lasted 1.5 hr at room temperature. After washing for at least 1 hr, the cells were fixedwith methanol ( $-$ 20°C for 1-2 min). For the localization of synapses,immunostained cells were first fixed and permeabilized with methanolfollowed by a second immunostaining with a mouse monoclonal antibody(Boehringer Mannheim, Mannheim, Germany; 2 µg/ml) or rabbit polyclonalantibody (Biogenesis; 57 µg/ml) to synaptophysin. The primaryantibodies against GluR1-4, GluR2, NR1, and synaptophysin werevisualized using the appropriate fluorochrome-conjugated secondaryantibody (Oregon green 488 goat anti-rabbit IgG antibody, 2-20µg/ml, Molecular Probes, Eugene, OR; Texas Red goat anti-mouseIgG antibody, 10 µg/ml, Jackson ImmunoResearch, West Grove, PA;Texas Red goat anti-guinea pig IgG antibody, 10 µg/ml, Rockland,Gilbertsville, PA) in HBS with 5% BSA, and 0.2% goat serum wasthen applied for 1.5 hr at 4°C. Coverslips were mounted in Vectashieldmounting medium (Vector Laboratories, Peterborough,UK).

Images were captured on a Leica (Heidelberg, Germany) TCS-NT confocal laser-scanning microscope attached to a DM RBE epifluorescencemicroscope using a 63× lens, (NA 1.32; Leica, Heidelberg, Germany).The 488 and 568 nm laser bands of a Kr-Ar laser were used fordual dye excitation and fluorescein isothiocyanate/tetramethylrhodamineisothiocyanate filters for fluorescence emission. With the imagingconditions used, there was no detectable bleedthrough of fluorescencefrom one channel to the other when we studied single-labeled specimens.Microscope settings were adjusted so that imaging conditions forboth red and green channels were kept constant. For quantitativeanalysis, confocal images from the red (488 nm) and green (568nm) channels were merged using Adobe Photoshop software (AdobeSystems, San Jose, CA). Twice the level of background was thensubtracted from the merged image to define the receptor clusters.Therefore clusters (or puncta) were designated as discrete regionswith more than twice the fluorescence intensity of background.Clusters were ~1-2.5 µm in size. Only puncta lying along processesinterpreted as dendrites were counted. We have excluded regionsfrom quantification where the clear identification of neuronalprocesses was ambiguous. Synapses (defined as synaptophysin-positivepuncta) on dendritic processes were considered glutamate receptor-positiveif they were directly apposed (or within 2 pixels) of GluR1-4,GluR2, or NR1 puncta. Similarly, if NR1-positive puncta were directlyapposed or within 2 pixels of GluR1-4 or GluR2-positive puncta,they were taken to be colocalized. GluR2 or GluR1-4 puncta werethen expressed as a ratio of synaptophysin or NR1 puncta in thesame neurons. For statistical analysis, independent group t testswereused.

The intensity of background fluorescence was no more than 7-13% of the mean values for puncta, for all antibodies at all threedevelopmental ages. Changing the criterion of the quantificationin our double-immunolabeling experiments (e.g., using 1-3 timesthe background as threshold) did not alter the relative ratiosof immunopositive puncta between the green and red channels. Wehave previously compared quantitatively the distribution of GluR1-4and NR1 puncta on paraformaldehyde-fixed and living neurons (Noelet al., 1999), and we have also performed acid-stripping of antibody-labeledcells, as described by Carroll et al. (1999). These data demonstratethat neither antibody-induced aggregation nor internalizationof receptors are significant factors in our living cell-stainingprotocols. Comparison with the GluR2 antibody (Chemicon) havenot been made, because it did not work on paraformaldehyde-fixedneurons (Noel et al., 1999).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Development and characterization of antibodies against AMPA and NMDA receptor subunits

To investigate the distribution of AMPA receptor proteins in living cells, polyclonal antibodies were raised against threefusion proteins derived from the TM3-TM4 linker region of theGluR1_flop subunit (Fig. 1A,B). A small segment of this regiondiffers in two alternatively spliced versions of AMPA receptorsubunits termed flip and flop (Sommer et al., 1990). The aminoacid sequence of the TM3-TM4 regions used for immunization shows~90% similarity in all cloned AMPA receptor subunits (Cockcroftet al., 1993; Hollmann and Heinemann 1994). The affinity-purifiedpolyclonal antibodies detected all three GST fusion proteins incorporatingamino acid residues 757-781, 724-781, or 690-781 of GluR1_flopAMPA receptor subunit on immunoblots, whereas no cross-reactivitywas observed to GST (data not shown). In immunoblots of rat brainmembranes, each of the antibodies specifically recognized a singleband with an apparent size of 110 kDa (Fig. 1C), correspondingto the molecular weight of AMPA receptor subunit proteins takinginto account subunit glycosylation. COS-7 cells expressing individualsubunits showed that antibodies raised against the conserved TM3-TM4linker recognize all AMPA receptor subunits (GluR1-4 flip andflop), with no cross-reactivity with the related kainate receptorsubunits GluR5-7 (Fig. 1C). Furthermore, in vitro translated GluR1-4subunits were also recognized in both flip and flop variants (datanot shown). All immunoreactivity was blocked by preadsorbing theantibody with 100 µg/ml of the protein used for immunization,and no specific staining was detected by replacing the antibodywith the preimmune serum (data notshown).

To study the expression pattern of NMDA receptor proteins, antipeptide antibodies were raised against the NR1 subunit, whichis an essential component of all known NMDA receptor heterooligomers(Monyer et al., 1992; Hollmann and Heinemann, 1994). Antibodieswere produced against synthetic peptides representing N-terminalresidues 436-450 of the NR1a subunit, a region that is presentin all splice variants (NR1a-g). All of the immunized rabbitsresponded to the antigen after the first boosting injection, asdetermined by dot-blot assays with the nonconjugated peptide (Fig.2A), and ELISA with the BSA-conjugated peptide (data not shown).The immune sera selectively labeled the synthetic peptide usedfor immunization but did not recognize the corresponding peptidesequences of other NMDA receptor subunits (Fig. 2A). The specificityof antibodies was further tested on immunoblots of membranes preparedfrom different regions of the rat brain and NR1a cDNA-transfectedCOS-7 cells (Fig. 2B). Antibodies raised against residues 436-450of NR1 reacted with a major band on immunoblots of brain samplesand NR1a-expressing COS-7 cells with the molecular weight of 115kDa, which closely approximates that expected for this subuniton the basis of amino acid sequence taking into account subunitglycosylation. The antibodies did not label membranes from COS-7cells expressing either of the related NR2A-D NMDA receptor subunits(data not shown). Preincubation of the antipeptide antibodieswith the respective synthetic peptide (100 µg of peptide/ml) blockedthe specific labeling (Fig. 2B). The anti-NR1 antibodies stainedthe surface of intact HEK 293 cells expressing recombinant NR1aand NR2A subunit-containing receptors (Fig. 2C, left panel). Nosignal was obtained with nontransfected HEK 293 cells (Fig. 2C,right panel).

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Figure 2. Characterization of the NR1 antibody using synthetic peptides, rat brain membrane fractions, and transiently transfected COS-7 and HEK 293 cells. A, Dot-blot assay of antipeptide NR1 antibody specificity using synthetic peptides corresponding to sequences of different NMDA receptor subunits. Immune sera from two rabbits (1:200 dilution) reacted only with the NR1 peptide, confirming the sequence specificity of these anti-NR1 antibodies. B, Immunoblot analysis of NR1 subunit proteins in rat brain and transiently transfected COS-7 cell membrane preparations. Aliquots of cerebral cortical (CTX), hippocampal (HIP), cerebellar (CER), spinal cord (SPC), and NR1a-transfected COS-7 cell membrane fractions (50 µg of protein/lane) were prepared, as described previously (Molnar et al., 1993; McIlhinney and Molnar, 1996). The bound antibodies were detected by reaction with alkaline phosphatase-conjugated anti-rabbit IgG. The preincubation of the antibody with the NR1 (436-450) peptide (1 µg/ml) blocked the labeling. C, Immunofluorescence staining of intact nonpermeabilized HEK 293 cells after transient transfection with NR1a and NR2A subunits. Transfected cells showed specific surface staining with the anti-NR1 antibody, whereas untransfected cells showed no immunostaining. Scale bars, 10 µm.

Immunochemical characterization of regional expression of AMPA and NMDA receptor proteins in unfixed rat brain

The regional distribution of GluR1-4 and NR1 immunoreactivity was analyzed on horizontal sections of whole unfixed adult ratbrains blotted onto nitrocellulose membranes for immunostaining,as described by Tönnes et al. (1999) (Fig. 3). The preparationof tissue samples for immunocytochemistry often requires fixationthat introduces covalent modification of the proteins, which couldalter the antibody-binding sites. The cross-linked molecules couldtherefore hinder the access of antibody to epitopes. Direct transferof proteins onto immobilizing membrane gives much improved accessibilityfor immunochemical analysis, and it is particularly useful forthe testing of antibodies, because it retains the anatomical localizationof different brain regions (Benke et al., 1995; Wenzel et al.,1997; Tönnes et al., 1999). Protein images on the nitrocellulosemembranes were immunostained with the purified GluR1-4 and NR1subunit-specific antibodies using conventional immunoblotting.Both GluR1-4 and NR1 immunoreactivities were predominant in thehippocampal formation (particularly in the CA1 region) and inthe neocortex. The strongest GluR1-4 staining was found in theneuropil layers of the hippocampal formation, in the superficiallayers of neocortex, and in the cerebellar molecular layer. Moderatelevels of labeling was found in deeper layers of the neocortex,in the striatum, and in the olfactory bulb (Fig. 3, left panel).The histoblot labeling pattern obtained with the NR1-specificantibody (Fig. 3, right panel) was in agreement with the immunoblotanalysis (Fig. 2B). The strongest labeling was in the hippocampalformation, where the highest reactivity was observed in the strataradiatum and oriens of CA1 and in the dentate molecular layer.Weaker reactivity was seen in the CA1 stratum pyramidale and inthe dentate granule cell layer and in the CA3 region. In the neocortexthe strongest NR1 staining was observed in the superficial layers.Cerebellar NR1 staining was relatively weak and was restrictedto the granule cell layer (Fig. 3, right panel).

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Figure 3. Regional distribution of AMPA and NMDA receptor proteins in rat brain. AMPA and NMDA receptor protein distribution was analyzed on adult rat brain histoblots using affinity-purified anti-GluR1-4 (0.5 µg/ml) and anti-NR1 (1 µg/ml) antibodies. The bound antibodies were visualized using an alkaline phosphatase-conjugated anti-rabbit antibody.

Quantification of developmental changes in total and surface-expressed AMPA and NMDA receptor proteins in CA3-CA1 primary neuronal cultures

Quantitative analysis of the surface expressed and total GluR1-4 and NR1 subunit proteins was performed by cell-ELISA on 3-,10-, and 17-d-old populations of cultured hippocampal neurons(Fig. 4). We measured the levels of surface-expressed and totalimmunoreactivity for the GluR1-4 and NR1 antibodies using intactand Triton X-100 permeabilized, paraformaldehyde-fixed neurons.The paraformaldehyde fixation prevented the detachment of cellsfrom the cell culture plate throughout the experiment. The integrityof the plasma membrane in paraformaldehyde-fixed cells was confirmed,using an antibody specific to the intracellular C-terminal domainof GluR2/3 AMPA receptor subunits (Chemicon). This antibody wasunable to interact with the intracellular C-terminal domain ofGluR2/3 in paraformaldehyde-fixed neurons without Triton X-100permeabilization (data not shown). In each of the neuronal cultures,immunoreactivity was normalized to protein levels, as describedin Materials and Methods.

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Figure 4. Quantification of developmental changes in surface-expressed and total AMPA and NR1 immunoreactivity on cultured hippocampal neurons using cell ELISA. Immunoreactivity for the NR1 NMDA receptor subunit (A, B) and GluR1-4 AMPA receptor subunits (C, D) was compared in paraformaldehyde-fixed, nonpermeabilized (surface-expressed, B, D) and 1% Triton X-100 permeabilized (total, A, C) cells after 3, 10, or 17 d in vitro using an ELISA-based assay. The total immunoreactivity for NR1 and GluR1-4 subunits (A, C) was expressed as the percentage of the immunoreactivity obtained after 17 d in culture. The surface immunoreactivity for NR1 and GluR1-4 subunits (B, D) was expressed as the percentage of the total immunoreactivity after 3, 10, or 17 d in vitro. For each experiment, a minimum of three parallel samples was used. *p < 0.001 compared with samples in other age groups.

Total NR1 expression increased by ~15% between days 3 and 10 in culture, but then remained essentially unchanged. Betweendays 3 and 17 the surface expression of NR1 protein was relativelyconstant at ~70% (Fig. 4A,B).

In contrast, we observed an ~1.5 fold increase in the total AMPA receptor subunit protein expression between days 3 and 10in culture. This increase then stabilized between days 10 and17 in culture (Fig. 4C). The surface expression of AMPA receptorsubunit proteins increased approximately twofold between days3 and 10 in culture and then remained essentially the same (~63%)until day 17 (Fig. 4D).

Our cell ELISA data indicate that ~60% of AMPA receptors and ~70% of NMDA receptors are surface-expressed in hippocampal neuronsafter 10 d in culture. This is consistent with the results ofcell surface biotinylation, cross-linking, and proteolysis studiesin cultured hippocampal neurons (Hall and Soderling, 1997a,b)and in cerebellar granule cells (Huh and Wenthold, 1999).

There is a developmental shift of surface-expressed NMDA and AMPA receptors to synaptophysin-immunopositive sites

Antibodies that recognize extracellular epitopes were used to analyze the surface distribution of AMPA and NMDA receptorsin living hippocampal neurons. For the localization of synapses,immunostained cells were first fixed and permeabilized with methanol,followed by a second immunostaining with anti-synaptophysin antibody.Synaptophysin is a widely used marker protein of presynaptic specializations.Cultured neurons were used at 3 time points; 3-5, 7-10, or 14-20d inculture.

After 3-5 d in culture, the majority of GluR1-4-positive (~79%; Fig. 5A), NR1-positive (~85%; Fig. 6A), and GluR2-positive(~82%; Fig. 6C) clusters colocalized with synaptophysin immunoreactivity,suggesting that most, but not all, NMDA and AMPA clusters arelocated at synapses (Fig. 7A). A relatively small percentage ofthe total synaptophysin-immunoreactive puncta colocalized withGluR1-4 (~45%; Fig. 5A) or GluR2 (~27%; Fig. 6C), indicating thatthe majority of synapses do not contain AMPA receptors at 3-4d in culture (Fig. 7B).

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Figure 5. Colocalization of GluR1-4 and synaptophysin in hippocampal neurons in culture for 3 and 14 d. Colocalization (yellow) of GluR1-4 (red) and synaptophysin (Syn, green) on hippocampal neurons in culture for 3 (A) and 14 (B) d. The individual immunoreactivity for GluR1-4 and synaptophysin (Syn) in regions highlighted in the boxes are shown in the side panels. At 3-5 d in culture (A), 79 ± 5% of surface-expressed GluR1-4 puncta (4 fields, 950 puncta) contained synaptophysin-immunoreactive puncta. At 14-20 d in culture, 98 ± 1% of surface-expressed GluR1-4 puncta (4 fields, 375 puncta) contained synaptophysin-immunoreactive puncta. At 3-5 d in vitro 45 ± 5% of total synaptophysin puncta (4 fields, 950 puncta) contained GluR1-4 immunoreactivity, which increased to 67 ± 2% (4 fields, 375 puncta) at 14-20 d in vitro. Scale bars, 10 µm.

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Figure 6. Colocalization of NR1 and GluR2 with synaptophysin in hippocampal neurons in culture for 4 and 14 d. Colocalization (yellow) of NR1 (green; A, B) or GluR2 (green; C, D) and synaptophysin (Syn, red) on hippocampal neurons in culture for 4 (A, C) and 14 (B, D) d. The individual immunoreactivity for NR1, GluR2, and synaptophysin (Syn) in regions highlighted in the boxes are shown in the bottom panels. At 3-5 d in culture (A), 85 ± 3% of surface-expressed NR1 puncta (6 fields, 748 puncta) contained synaptophysin-immunoreactive puncta. At this age 61 ± 7% of the total synaptophysin puncta (6 fields, 748 puncta) contained NR1. At 14-20 d in culture (B), 96 ± 2% of surface-expressed NR1 puncta (4 fields, 413 puncta) contained synaptophysin-immunoreactive puncta, whereas 63 ± 4% of total synaptophysin puncta (4 fields, 413 puncta) colocalized with NR1. At 3-5 d in culture (C), 82 ± 6% of surface-expressed GluR2 puncta (3 fields, 381 puncta) contained synaptophysin-immunoreactive puncta, whereas 27 ± 10% of the total synaptophysin (3 fields, 418 puncta) contained GluR2. At 14-20 d in culture (D) 89 ± 4% of surface-expressed GluR2 (4 fields, 366 puncta) contained synaptophysin-immunoreactive puncta, and 62 ± 3% of the total synaptophysin (4 fields, 366 puncta) contained GluR2. Scale bars, 5 µm.

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Figure 7. Quantification of developmental changes in the colocalization of AMPA and NMDA receptor subunit proteins and synaptophysin. A, The majority of surface NR1 (), GluR1-4 ( $black-square$ ), and GluR2 () clusters colocalized with the presynaptic marker protein synaptophysin. B, The percentage of the total synaptophysin-immunoreactive puncta containing NR1 () remained the same, whereas GluR1-4 ( $black-square$ ) and GluR2 () increased during development. Mean and SE was calculated based on at least three independent determinations; *p < 0.001 compared with samples in the 14- to 20-d-old groups.

After 14-20 d in culture almost all the surface GluR1-4 (~98%; Fig. 5B), NR1 receptors (~96%; Fig. 6B), and a majority ofthe surface GluR2-containing clusters (~89%; Fig. 6D) were colocalizedwith synaptophysin. At this age there was also an increase inthe percentage of the total synaptophysin-immunoreactive punctacontaining GluR1-4 (~67%; Fig. 5B) or GluR2 (~62%; see Fig. 6D).The percentage of the total synaptophysin-positive puncta containingNR1 (~60%) remained essentially the same during development (Fig.7B).

The developmental increase in the percentage of synaptophysin-positive puncta expressing AMPA receptors could be attributableto the appearance of AMPA receptors at synapses that (1) previouslyonly expressed NMDA receptors or (2) did not express either classof iGluR. To distinguish between these possibilities we have performedcolocalization studies of AMPA and NMDAreceptors.

During development, NMDA receptors are expressed at the synapse before AMPA receptors

After 3-5 d in culture, numerous NR1 clusters were detected on the surface of pyramidal-shaped neurons (Fig. 8A). At thisage, only ~41 and ~29% of the NR1 clusters colocalized with GluR1-4or GluR2, respectively (Figs. 8A, 9A).

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Figure 8. Surface distribution of GluR1-4 and NR1 immunoreactivity during development of living hippocampal neurons in culture. Surface distribution of GluR1-4 (red) and NR1 (green) immunoreactivity on living hippocampal neurons in culture for 5 (A), 10 (B), and 14 (C) d. Areas of colocalization are shown in yellow on the left panels. The individual immunoreactivities for GluR1-4 and NR1 in region highlighted in the box are shown in the right panels. In 3- to 5-d-old living neurons (A) 41 ± 6% of surface-expressed NR1 puncta (5 fields, 610 puncta) contained GluR1-4 puncta. This increased to 59 ± 7% (8 field, 1255 puncta) and 59 ± 5% (6 field, 875 puncta) after 7-10 (B) and 14-20 d (C) in culture, respectively. Scale bars, 10 µm.

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Figure 9. Surface distribution of GluR2 and NR1 immunoreactivity during development of living hippocampal neurons in culture. Surface distribution of GluR2 and NR1 immunoreactivity on living hippocampal neurons in culture for 3 (A), 8 (B), and 14 (C) d. Colocalization (yellow) of GluR2 (red) and NR1 (green) immunoreactivity on living hippocampal neurons. The individual immunoreactivities for GluR2 and NR1 in region highlighted in the box are shown in the side panels. In 3- to 5-d-old neurons (A) 29 ± 5% of surface-expressed NR1 puncta (3 fields, 240 puncta) contained GluR2 puncta. This increased to 57 ± 11% (3 fields, 124 puncta) and 67 ± 2% (3 fields, 173 puncta) after 7-10 (B) and 14-20 d (C) in culture, respectively. Scale bars, 5 µm.

After 7-10 d in culture, the percentage of NR1 clusters that colocalized with GluR1-4 and GluR2 increased by ~1.5- and 2-fold,respectively, to ~60% (Figs. 8B, 9B), decreasing the number ofNR1 only synapses to ~40%.

After 14-20 d in culture, the percentage of NR1 clusters colocalized with GluR1-4 remained the same (~60%), whereas colocalizationwith GluR2 moderately increased (Figs. 8C, 9C).

These results suggest a developmental rearrangement in the distribution of AMPA receptors within neurons, such that thereis an increase in the targeting of AMPA receptors to NMDA receptorcontaining synapses between days 3 and 20 in culture (Fig. 10A-D).

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Figure 10. Quantification of developmental changes in the colocalization of AMPA and NMDA receptor subunit proteins. The percentage of GluR1-4 (A) and GluR2 (B) clusters that contain NR1 on the surface of living hippocampal neurons at different time points. The number of NR1 clusters containing GluR1-4 (C) or GluR2 (D) increased on the surface of living hippocampal neurons during development. E, The number of GluR2-containing GluR1-4 clusters increased between day 3 and 20 in culture. F, Schematic diagram of two potential molecular mechanisms by which the relative increase in synaptic GluR2 can decrease Ca²⁺ influx at synapses by forming Ca²⁺-impermeable AMPA receptors. Mean and SE was calculated based on at least three independent determinations; *p < 0.001 compared with samples in the 14- to 20-d-old groups.

These experiments also revealed an unexpected difference between the colocalization of NR1/GluR1-4 versus NR1/GluR2 at 3-5d in culture and raised the possibility of developmental changesin surface expressed AMPA receptor subunit composition. We thereforecompared the distribution of GluR1-4 and GluR2 subunitsdirectly.

The number of AMPA receptor clusters containing GluR2 subunits increased during development

At 3-5 d in culture ~67% of GluR1-4-positive puncta contained GluR2 immunoreactivity. This ratio increased to ~78% at 7-10d in vitro. After 14 d, colocalization was almost complete (~96%;Fig. 10E). These data are consistent with the increase in GluR2/NR1(Fig. 10D) and GluR2/synaptophysin (Fig. 7B) colocalization duringdevelopment, when compared to changes in GluR1-4/NR1 (Fig. 10C)and GluR1-4/synaptophysin (Fig. 7B) colocalization ratios. Theseresults indicate an increase in GluR2 subunit-containing AMPAreceptors during development (Fig. 10E).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antibodies that recognize all subunit combinations of surface expressed AMPA and NMDA receptors

To allow us to perform studies on live, developing neurons we used site-directed antibodies against extracellular epitopesthat should recognize all NMDA and AMPA receptors. AMPA receptorswere identified with antibodies raised against fusion proteinsderived from the TM3-TM4 linker region of the GluR1_flop subunit.The use of these GluR1-4-specific antibodies eliminated the possibilitythat the observed changes are attributable to changes in subunitcomposition of AMPA receptors during development or differentialtargeting of individual subunits in neurons. NMDA receptors wereidentified by antibodies against N-terminal residues 436-450 ofthe NR1 subunit. NR1 is part of every NMDA receptor expressedat the cell surface, and the selected sequence is identical inall splice variants of this protein, but different in other iGluRsubunits.

The regional distribution of the GluR1-4 and NR1 receptor subunit immunoreactivity was analyzed in the adult rat brain usinga histoblot procedure (Tönnes et al., 1999). The direct transferof native proteins from unfixed frozen tissue sections to an immobilizingmatrix offers improved accessibility of the transferred proteinsfor immunochemical analysis. The histoblot patterns obtained agreewell with previous autoradiographic studies using AMPA and NMDAreceptor-selective radioligands (Monaghan et al., 1984; Boweryet al., 1988; Insel et al., 1990) and are consistent with thecellular distribution of different AMPA and NMDA receptor subunitmRNAs (Pellegrini-Giampietro et al., 1991; Monyer et al., 1994;Standley et al., 1995). However, some of the previously publishedimmunocytochemical studies performed on fixed tissue reportedmore uniform distribution of labeling for AMPA receptor subunitsin different layers of the cerebral cortex (Petralia and Wenthold,1992). This difference could be attributable to the fact thatsynaptic receptors may be relatively inaccessible in the fixedtissue, or there are regional differences in mechanical properties,tissue permeability, or myelin content. The expression of bothGluR1-4 and NR1 proteins is strongest in the hippocampus, thereforecultured hippocampal neurons provide a good model system to studythe targeting of native AMPA and NMDAreceptors.

Both AMPA and NMDA receptors concentrate at synaptic sites on the cell surface during development

In our study, most NMDA receptor clusters colocalized with the presynaptic marker synaptophysin. However, despite its extensiveuse as a synaptic marker, we cannot formally exclude the possibilitythat synaptophysin might sometimes occur at nonsynaptic loci orthat some synapses might lack synaptophysin. Our results are consistentwith electrophysiological data showing that the distribution ofthe presynaptic and postsynaptic terminals are rapidly synchronized,and most synapses have NMDA receptors throughout development (Tovarand Westbrook, 1999). As neurons develop, synapses acquire AMPAreceptors. The ~1.5 fold increase in the relative number of GluR1-4-positivesynaptic puncta correlates only partially with the results ofthe cell-ELISA experiments, which indicate an approximately twofoldincrease in total surface expression of GluR1-4 subunits overa similar period of time. This suggests an increase in both thenumber of AMPA receptor-containing synapses and the density ofAMPA receptors at synapses. This result agrees well with electrophysiologicaldata showing that the developmental increase in AMPA receptorEPSCs is attributable to both an increase in synapse number andan increase in quantal size (Gomperts et al., 2000).

In the present study we have detected a small but significant proportion of extrasynaptic clusters of both AMPA and NMDA receptors.This observation is consistent with previous studies on AMPA (Richmondet al., 1996; Nusser et al., 1998) and NMDA receptors (Aoki etal., 1994; Liao et al., 1999) using cultured neurons and immunocytochemicalmethods. Here we have found a developmental decrease in the proportionof extrasynaptic clusters of both NMDA and AMPA receptors. Thismay be induced by the activity of newly formed synapses (Rao andCraig, 1997).

NMDA receptor containing synapses progressively acquire AMPA receptors in developing hippocampal neurons

Recent studies have indicated that AMPA and NMDA receptor accumulation at excitatory synapses is independently regulated (Gompertset al., 1998; Archibald et al., 1999; Liao et al., 1999; Lissinet al., 1999; Lüscher et al., 1999; Noel et al., 1999; Petraliaet al., 1999; Shi et al., 1999; Takumi et al., 1999; Gompertset al., 2000). Early in postnatal development most excitatoryhippocampal synapses contain functional NMDA receptors withoutdetectable AMPA receptor responses (Isaac et al., 1995; Liao etal., 1995; Durand et al., 1996). During the first two postnatalweeks, synapses acquire functional AMPA receptors (Durand et al.,1996). Our results are consistent with the evidence that expressionand synaptic delivery of AMPA and NMDA receptor subunits are differentand that these processes are developmentally regulated in hippocampalneurons. The molecular mechanisms regulating this differentialtargeting remain largely unknown, but proteins that interact directlywith AMPA and NMDA receptor subunits are likely to play centralroles in this process (Dong et al., 1997; Kornau et al., 1997;Nishimune et al., 1998; O'Brien et al., 1998a; Osten et al., 1998;Song et al., 1998; Dev et al., 1999; Lüscher et al., 1999; Lüthiet al., 1999; Noel et al., 1999; Wyszynski et al., 1999; Xia etal., 1999; Man et al., 2000).

Other studies have also recently addressed developmental differences in the colocalization of AMPA and NMDA receptors. Inan immunogold-labeling study, the amount of immunolabeling persynapse was initially high and remained constant for NMDA receptors.In contrast, gold labeling was initially low and increased duringdevelopment for AMPA receptors (Petralia et al., 1999). In themost comparable study, the distribution of AMPA and NMDA receptorswas analyzed in fixed hippocampal neurons during development inculture (Liao et al., 1999). Our results are in general agreementwith the view that NMDA receptor only synapses are replaced byNMDA and AMPA receptor synapses during development, but thereare significant quantitative differences between the two studies.For example, at 1 week in vitro >90% of synapses are silent inthe study of Liao et al. (1999), whereas we find <50% silent synapsesat this time. There are several possible explanations for thisdifference: for example, (1) our experiments were performed onpostnatal cultures compared with embryonic cultures. (2) We labeledAMPA receptors with an antibody that recognizes all GluR1-4 subunits,whereas Liao et al. (1999) used GluR1 and GluR2/3 subunit-specificantibodies. (3) We labeled AMPA and NMDA receptors on the surfaceof neurons while they were still alive, whereas Liao et al. (1999)identified the total NMDA and AMPA receptor population after fixationandpermeabilization.

The use of living neurons offers distinct advantages over fixed or fixed and permeabilized cells, e.g., fixation can hinderaccess to epitopes by covalent cross-linking, and permeabilizationprovides access to intracellular pools of receptors that cloudsthe interpretation of the synaptic distribution of receptors.Finally, antibodies that label living neurons can be used to studyAMPA and NMDA receptor dynamics in physiologicalexperiments.

A pertinent issue, in immunocytochemical experiments on both living and fixed cells, is the possibility that low levels ofAMPA receptor protein could be misclassified as no AMPA receptorexpression because of a lack of sensitivity. This is analogousto the misclassification of failures in electrophysiological experiments.However, we do not consider this to be a major source of errorin our study because the mean intensity of the puncta were ~10-foldgreater than thebackground.

The subunit composition of surface-expressed AMPA receptors changes during development

The GluR2 subunit in the edited form is responsible for the calcium impermeability of AMPA receptors. Our data indicate thatearly in development a high proportion of AMPA receptors are presentat synapses that do not possess GluR2 immunoreactivity. However,after 2 weeks in culture the GluR2 immunoreactivity was presentin nearly every AMPA receptor-positive synapse. The relative increasein synaptic GluR2 can reduce Ca²⁺ influx by forming Ca²⁺-impermeable AMPA receptors on their own or in combination withother subunits (Fig. 10F). It is more likely that in hippocampalneurons GluR2 forms heteromeric AMPA receptor complexes with GluR1or GluR3 subunits (Wenthold et al., 1996). It is interesting tonote that the relative increase in synaptic GluR2 continues duringthe second week, when there are only moderate changes in the surfaceexpression and total amount of AMPA receptors, suggesting thatthis process is independently regulated. These results demonstratethat not only the expression and synaptic targeting of AMPA receptorsis regulated, but that the subunit composition is also under developmentalcontrol.

Since the submission of our manuscript, electrophysiological studies have provided additional support for our results. A rapidand long-lasting change in the subunit composition and Ca²⁺ permeability of AMPA receptors has been identified at cerebellarstellate cell synapses after synaptic activity (Liu and Cull-Candy,2000). Additionally, a new AMPA receptor-trafficking model forsynaptic plasticity has been proposed, which is based on the differentialtargeting of GluR2 subunit-containing AMPA receptors (Malinowet al., 2000).

  FOOTNOTES

Received May 17, 2000; revised July 25, 2000; accepted July 31, 2000.

We are grateful to the Medical Research Council, the Royal Society, and the Wellcome Trust for financial support. The mammalianexpression vector containing the genes coding for various ionotropicglutamate receptor subunits was the generous gift of Dr. H. Monyer(University of Heidelberg, Heidelberg,Germany).
L.P. and J.N. contributed equally to thiswork.

Correspondence should be addressed to Dr. Elek Molnar, Medical Research Council Centre for Synaptic Plasticity, Departmentof Anatomy, University of Bristol, School of Medical Sciences,University Walk, Bristol BS8 1TD, UK. E-mail: Elek.Molnar{at}bristol.ac.uk.

Dr. Noël's present address: Universite de Nice-Sophia Antipolis, Biologie cellulaire des compartiments calciques, Groupede neurobiologie fondamentale et clinique, EA 2674 Parc ValroseFaculte des sciences, 06108 Nice Cedex 2,France.

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ABSTRACT
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MATERIALS AND METHODS
RESULTS
DISCUSSION
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