A Developmental Change in NMDA Receptor-Associated Proteins at Hippocampal Synapses

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The Journal of Neuroscience, February 1, 2000, 20(3):1260-1271

A Developmental Change in NMDA Receptor-Associated Proteins at Hippocampal Synapses
Nathalie Sans¹, Ronald S. Petralia¹, Ya-Xian Wang¹, Jaroslav Blahos II¹, Johannes W. Hell², and Robert J. Wenthold¹
¹ Laboratory of Neurochemistry, National Institute on Deafness and Other Communication Disorders, National Institutes of Health, Bethesda, Maryland 20892, and ² Department of Pharmacology, University of Wisconsin, Madison, Wisconsin 53706-1532

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The membrane-associated guanylate kinases [Chapsyn-110/postsynaptic density-93 (PSD-93), synapse-associated protein-90 (SAP-90)/PSD-95,and SAP-102] are believed to cluster and anchor NMDA receptorsat the synapse and to play a role in signal transduction. We haveinvestigated the developmental changes in expression of theseproteins in rat hippocampus using biochemical analyses and quantitativeimmunogold electron microscopy. At postnatal day 2 (P2), SAP-102was highly expressed, whereas PSD-93 and PSD-95 were low. SAP-102expression increased during the first week, stayed stable throughP35, and showed a reduced expression at 6 months. From P2 through6 months, PSD-93 and PSD-95 increased. For PSD-95, the percentof labeled synapses increased almost threefold with age, whereasthe number of gold particles per labeled synapse did not changesignificantly, suggesting that the increase in PSD-95 is attributableprimarily to an increase in the number of synapses containingPSD-95. In contrast, for SAP-102, both percent labeled synapsesand the number of gold particles per labeled synapse decreasedduring this time. From Western blots of hippocampus and immunogoldanalysis of CA1 synapses, the high expression of NR2B at P2 coincideswith the high level of SAP-102 at synapses, whereas the laterexpression of NR2A coincides with that of PSD-93 and PSD-95. Todetermine whether the changes in PSD-93/95 and SAP-102 reflectpreferred associations with NR2A and NR2B, respectively, we measuredco-immunoprecipitation in the adult hippocampus. These studiessuggest that there is a preference for complexes of NR2A/PSD-93/95and NR2B/SAP-102. These results indicate that individual receptor-associatedproteins may have specific functions that are critical to synapsedevelopment.

Key words: MAGUKs; PSD-93; PSD-95; SAP-102; glutamate receptors; postsynaptic density; hippocampus

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The postsynaptic density (PSD), a highly organized cytoskeletal structure found adjacent to the postsynaptic membrane of excitatorysynapses, is believed to play a role in the organization of receptorsand related proteins involved in synaptic signaling. A numberof proteins enriched in the PSD have been characterized (for review,see Kennedy, 1993, 1997); one of these, synapse-associated protein-90(SAP-90)/postsynaptic density-95 (PSD-95), was initially identifiedbased on its abundance in the isolated PSD (Cho et al., 1992;Kistner et al., 1993). Later studies showed that PSD-95 interactswith the C terminus of NMDA receptor NR2 subunits, suggestingthat PSD-95 may play a role in the synaptic anchoring and organizationof NMDA receptors (Kornau et al., 1995; Niethammer et al., 1996).Three additional proteins, structurally related to PSD-95, havebeen identified: SAP-97/hdlg (Lue et al., 1994; Müller et al.,1995), Chapsyn-110/PSD-93 (Brenman et al., 1996b; Kim et al.,1996), and SAP-102 (Lau et al., 1996; Müller et al., 1996) (forreview, see Sheng, 1996; Sheng and Kim, 1996; Kornau et al., 1997).These proteins have three PDZ (for PSD-95, Dlg, ZO-1/Dlg-homologousregion) domains, one Src homology 3 domain, and one guanylatekinase-like domain and are generically referred to as membrane-associatedguanylate kinases (MAGUKs). In addition to interacting with NMDAreceptors, MAGUKs interact with a series of other proteins thathave structural, and perhaps signaling, functions at the synapse(for review, see Nagano et al., 1998; Kim and Huganir, 1999).

The patterns of expression of SAP-97, PSD-93, PSD-95, and SAP-102 are distinct but overlapping in brain. Although not rigorouslystudied, many neurons appear to express multiple MAGUKs, raisingquestions about their structural and functional relationships.In transfected cells, PSD-93 and PSD-95 induce the clusteringof NMDA receptors and can form heteromeric complexes (Kim et al.,1995, 1996), indicating that if multiple MAGUKs are present atthe same PSD, they may be structurally coupled. The possibilitythat individual MAGUKs can substitute for one another is suggestedby the results of a study showing that mice carrying a truncatedform of PSD-95 exhibited changes in NMDA receptor-related plasticityyet retained most aspects of normal NMDA receptor function (Migaudet al., 1998).

NMDA and AMPA receptors show distinct patterns of postnatal development at CA1 synapses in the hippocampus. NMDA receptorsare present at synapses in the postnatal day 2 (P2) animal, indicatingthat the NMDA receptor anchoring and organizational machineryis already mature at P2 (Petralia et al., 1999). However, studieson the gross developmental properties of MAGUKs show marked differencesamong the different members (Cho et al., 1992; Müller et al.,1996; Song et al., 1999; Wyszynski et al., 1999). This suggeststhat individual MAGUKs may have specific functions that are criticalfor synapsedevelopment.

In the present study, we investigated the expression of MAGUKs in the hippocampus of adult and developing rats. Our resultsshow a dramatic difference in the development of synaptic PSD-93and PSD-95 compared with that of SAP-102, indicating that a switchin the NMDA receptor anchors plays a major role in changes insynaptic plasticity in the developinganimal.

  MATERIALS AND METHODS

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INTRODUCTION
MATERIALS AND METHODS
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Antibody production and purification. Antibodies against MAGUKs used are listed in Table 1. To raise antibodies against SAP-90/PSD-95(JH62092), the peptide VERREWSRLKAKDWGSS corresponding to residues494-510 of SAP-90 (Kistner et al., 1993) was synthesized by thesolid-phase method, coupled to BSA using glutaraldehyde, and dialyzedagainst PBS, pH 7.4 (Hell et al., 1993). The T60 anti-PSD-95 rabbitpolyclonal antibody was generated against a 6xHis fusion proteincorresponding to residues 228-299 of the PSD-95 sequence (Choet al., 1992). cDNA fragments encoding the first 105 amino acidresidues of SAP-97 and the first 119 amino acid residues of SAP-102were amplified by PCR and subcloned in pGEX-2T (Pharmacia, Piscataway,NJ). The glutathione S-transferase (GST)-SAP-97 and GST-SAP-102fusion proteins were expressed in Escherichia coli (BL21; Novagen,Madison, WI) and purified following a protocol described in Leonardet al. (1998). For affinity purification, antisera against SAP-90/PSD-95(JH62092), SAP-97 (JH62426), or SAP-102 (JH62514) were incubatedfor 2-4 hr with the SAP-90-derived peptide coupled to cyanogenbromide-activated Sepharose (Amersham Pharmacia Biotech, Piscataway,NJ) (Hell et al., 1993) or GST-SAP-97(1-105) or GST-SAP-102(1-119)cross-linked with dimethyl pimelimidate to glutathione-Sepharose(Bar-Peled and Raikhel, 1996), respectively. Antibodies were elutedwith 5 ml of 3 M MgCl₂, and the eluate was diluted immediatelywith 10 ml of Tris-buffered saline (TBS) and concentrated usinga Centriprep 30 concentrator from Amicon (Beverly, MA) (Hell etal., 1993).


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Table 1. Summary of antibodies against MAGUKs used

Three anti-PSD-93 antibodies and the guinea pig anti-SAP-102 antibody were kindly provided by Dr. D. S. Bredt (Universityof California, San Francisco, CA) (Table 1).

The glutamate receptor antibodies were characterized previously. Rabbit polyclonal antibodies were anti-GluR1 and anti-GluR2/3(Wenthold et al., 1992), T46 anti-NR1 (Petralia et al., 1994a),T58 anti-NR2A and T51 anti-NR2B (Christie et al., 1999), T12 anti-NR2A/B(Petralia et al., 1994b). Mouse monoclonal antibodies were anti-NR1(clone 54.1; PharMingen, San Diego, CA), anti-NR2A (2F6.3D5; Hartveitet al., 1994; a gift from Dr. I. Bartke, Boehringer Mannheim,Mannheim, Germany), anti-NR2B (Transduction Laboratories, Lexington,KY). Affinity-purified horseradish peroxidase-conjugated donkeyanti-rabbit and sheep anti-mouse secondary antibodies were purchasedfrom Amersham Pharmacia Biotech. Affinity-purified horseradishperoxidase-conjugated swine anti-goat and rabbit anti-guinea pigantibodies were purchased from Boehringer Mannheim (Indianapolis,IN).

Transfection of HEK293 cells. cDNAs in eukaryotic expression vectors were kindly provided by the following: SAP-97 (Dr. MorganSheng), PSD-93 and PSD-95 (Dr. David S. Bredt), and SAP-102 (Dr.Richard L. Huganir). HEK293 cells were transfected using a standardcalcium phosphate precipitation method using the CalPhos MammalianTransfection Kit (Clontech, Palo Alto, CA). Transfected cellswere incubated for 36 hr, washed, and harvested in PBS containing0.5 mM EDTA. After centrifugation, cells were resuspended in 50mM Tris-HCl, pH 7.5, containing a mixture of protease inhibitors(1 mM EDTA, 1 mM AEBSF, 50 µg/ml leupeptin, 10 µg/ml pepstatin,and 10 µg/ml aprotinin) and sonicated. Cell membranes were solubilizedin SDS sample buffer and boiled for 10min.

Preparation of tissue extracts. Hippocampi were dissected from P2, P10, P35, and 6-month-old Sprague Dawley rats and placedin ice-cold PBS, pH 7.4. Frozen hippocampi were homogenized inPBS, and then an equal volume of 2× SDS sample buffer was added,and the samples were boiled. Protein concentrations were measuredusing a BCA kit (Pierce, Rockford, IL) or a protein assay kit(Bio-Rad, Hercules, CA). Twenty micrograms of proteins were loadedin each lane for a subsequent Western blotanalysis.

Immunoprecipitation. Immunoprecipitation experiments were performed as described previously (Blahos and Wenthold, 1996). Wholehippocampus or the CA1 region of P35 Sprague Dawley rats was homogenizedwith a Polytron in 50 mM Tris-HCl, pH 7.4, containing the proteaseinhibitor mixture described above. Membranes were sedimented bycentrifugation (100,000 × g, 30 min, 4°C) and solubilized in 1%deoxycholate (DOC), 50 mM Tris-HCl, and 1 mM EDTA, pH 9, for 45min at 37°C. Insoluble material was removed by centrifugation.Triton X-100 was added to a final concentration of 0.1%, and thesupernatant was dialyzed for 16 hr against 50 mM Tris, pH 7.5,containing 0.1% Triton X-100. Insoluble material was removed bycentrifugation, and the supernatant was stored at $-$ 80°C untilthe immunoprecipitation reactions were performed. For immunoprecipitation,10 µl of the appropriate antiserum was added to 50 µl (resuspendedresin) of protein A- or protein G-agarose beads (Pierce, Rockford,IL) in PBS containing 0.1% Triton X-100 for at least 2 hr at 4°C.Protein A or protein G beads were then pelleted, washed in PBSplus 0.1% Triton X-100, and incubated with 1 ml of the detergent-solubilizedfraction at 4°C with constant rotation. The beads were then washedwith 50 mM Tris-HCl, pH 7.5, containing 0.1% Triton X-100 and150 mM NaCl. After the last wash, the beads were resuspended in2× SDS sample buffer (100 µl) and boiled for 3 min. After thechemiluminescence detection, films were scanned using a MolecularDynamics (Sunnyvale, CA) densitometer to estimate the amount ofimmunoreactivity in the bound fractions compared with that inthe corresponding input fraction. Different amounts of the inputwere run and compared with the boundfraction.

SDS-PAGE and immunoblot analysis. Proteins were separated with SDS-PAGE (4-20% gradient gels) and transferred to an Immobilon-Pmembrane (Millipore, Bedford, MA). Membranes were incubated with5% (w/v) skim milk in TBS containing 0.05% Tween 20 overnightat 4°C. Membranes were washed and incubated with primary antibodyat concentrations noted in Table 1 or using the following concentrations:GluR1, 0.5 µg/ml; GluR2/3, 0.15 µg/ml; T46 NR1, 0.5 µg/ml; clone54.1 NR1, 1:5000; T58 NR2A, 1:2000; NR2A (2F6.3D5), 1:5000; T51NR2B, 1:4000; NR2B monoclonal, 2.0 µg/ml; and T12 NR2A/B, 0.5µg/ml. Immunoreactive bands were visualized with chemiluminescence(Pierce). To reprobe, blots were stripped by shaking in 2% (w/v)SDS, 62.5 mM Tris-HCl, pH 6.8, and 100 mM $beta$ -mercaptoethanol for30 min at 60°C. Each experiment was repeated several times, andrepresentative blots are shown. For quantification, films werescanned, and densitometry was done using a Molecular Dynamicsdensitometer.

Postembedding immunogold immunocytochemistry. The postembedding method has been described (Petralia et al., 1997, 1998, 1999;Rubio and Wenthold, 1997; Wang et al., 1998; Zhao et al., 1998)and is modified from a previous study (Matsubara et al., 1996).Sprague Dawley rats were anesthetized and perfused with 4% paraformaldehydeplus 0.5% glutaraldehyde in 0.1 M phosphate buffer. Two animalswere used for P2, P10, and P35 and one animal for 6 months forthe main studies of PSD-95 (TL) and SAP-102 (JH62514). One animalper age (P2, P10, and P35) was used for additional antibodies[PSD-95 (JH62092), SAP-102 (GP-DB), PSD-93 (GP-DB), and PSD-93(AL)]. Parasagittal sections of the hippocampus were cryoprotectedin 30% glycerol and frozen in liquid propane in a Leica (Vienna,Austria) EM CPC (Universal Cryoworkstation). Frozen sections wereimmersed in 1.5% uranyl acetate in methanol at $-$ 90°C in a LeicaAFS freeze-substitution instrument, infiltrated with LowicrylHM-20 resin at $-$ 45°C, and polymerized with ultraviolet light.Thin sections of the hippocampus were incubated in 0.1% sodiumborohydride plus 50 mM glycine in TBS and 0.1% Triton X-100 (TBST),followed by 10% normal goat serum (NGS) in TBST, primary antibodyin 1% NGS in TBST, and immunogold (10 nm; Amersham Pharmacia Biotech)in 1% NGS in TBST plus 0.5% polyethylene glycol, and the sectionswere stained finally in uranyl acetate and lead citrate. For doublelabeling using antibodies made in different species, sectionswere incubated with two primary antibodies [PSD-95 (TL) monoclonalplus either SAP-102 (JH62514) or GluR2/3 polyclonal (2 µg/ml)]and later incubated with two immunogolds (15 nm goat anti-mouseand 5 nm goat anti-rabbit). Other combinations included PSD-95(TL) plus NR2A/B (T12; 4 µg/ml) or PSD-93 (AL), using 5 nm goatanti-mouse plus 10 nm goat anti-rabbit or 10 nm goat anti-mouseplus 5 nm goat anti-rabbit, respectively. For double labelingusing antibodies made in the same species, the first primary antibodyand the corresponding immunogold-conjugated antibody (5 nm gold)were applied, sections were exposed to paraformaldehyde vaporat 80°C for 1 hr, and the second primary antibody and its corresponding10 nm gold antibody were applied the following day (Wang and Larsson,1985; Matsubara et al., 1996; Zhao et al., 1998). Primary antibodycombinations using this method included SAP-102 (JH62514) followedby NR2A/B or PSD-93 (AL) followed by SAP-102 (JH62514). Controlsincluded the absence of the primary antibodies and incubationin 10 nm goat anti-rabbit or 10 nm goat anti-mouse or 5 nm goatanti-rabbit plus 15 nm goat anti-mouse immunogold, each for P2,P10, and P35. Gold labeling was very rare in controlsections.

Immunogold particles were counted in the postsynaptic density and cleft, as in previous studies (Wang et al., 1998; Zhao etal., 1998; Petralia et al., 1998, 1999). All synapses were countedin a selected portion of the CA1 stratum radiatum of the hippocampus,as in a previous study (Petralia et al., 1999). Synapses wereevaluated for the number of gold particles per synapse (both labeledand unlabeled) or number of gold particles per labeled synapse;labeled synapses had one or more gold particles. The number ofgold particles per unit length of the synapse was not calculatedbecause the results of such measurements done in conjunction withthe previous study were generally similar to the number of goldparticles per synapse (R. S. Petralia, J. A. Esteban Y.-X. Wang,J. G. Partridge, H.-M. Zhao, R. J. Wenthold, and R. Malinow, unpublisheddata). A lack of significant developmental change in synapse lengthseems to be typical of synapses of the CNS (Vaughn, 1989; Zhaoet al., 1998). All micrographs used in the figures were processedwith Adobe (Mountain View, CA) Photoshop 4.0 to optimize brightnessandcontrast.

Synapses used in this study showed characteristic features of asymmetric synapses: postsynaptic density, cleft, and presynapticvesicles. As noted by Petralia et al. (1999), synapses increasein number with age. Also, immature-looking synapses are more commonat early ages. Fiala et al. (1998), using serial sections andthree-dimensional analysis, suggest that there are four stagesin the development of postsynaptic structures of most excitatoryspine synapses in the CA1 region: filopodia, dendrite shaft synapse,stubby protrusion, and mature spine. In our study, we dividedpostsynaptic structures into three groups: dendrite shafts, protuberances,and spines. Protuberances are wider than long and may includeboth the stubby protrusions and the enlarged bases of filopodiadescribed by Fiala et al. (1998). Our "spine" category may includesome examples of enlarged apices of filopodia (especially at theearly postnatal ages), which would not be identifiable in ourmaterial without serial reconstruction. Consistent with Fialaet al. (1998), synapses at P2 were mostly on dendrite shafts.In contrast, in adults, most synapses were on spines, and dendriteshaft synapses wererare.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antibody characterization

Several commercially available and donated antibodies were tested by immunoblotting of transfected cell membranes and hippocampushomogenates to determine specificity (Fig. 1). Some of the antibodiesrecognized more than one member of the MAGUK family of proteinsreflecting the sequence similarities among these proteins. Althoughsuch antibodies may be appropriate for Western blotting becauseof the different molecular weights of the proteins, they are notacceptable for immunocytochemistry to identify a single protein.Furthermore, some antibodies could not be used because they failedto interact with their antigens after processing for postembeddingstaining. For immunogold immunocytochemistry, based on specificityand reactivity, the following were used: both antibodies to SAP-102,PSD-95 (TL and JH62092), and PSD-93 (AL). In Western blots ofhippocampus, these antibodies detected a single band that co-migratedwith the appropriate protein in the transfected cell samples.To allow direct comparisons, the same antibodies were used forWestern blotting. For immunoprecipitation, SAP-97 (JH62426), PSD-93(AL), either the PSD-95 (T60) or the PSD-95 (clone 7E3-1B8), andSAP-102 (JH62514) were effective. The PSD-95 (T60) has a slightcross-reaction with SAP-97, but the low expression of SAP-97 inthe hippocampus allows us to use this antibody as one specificfor PSD-95. The PSD-95 (clone 7E3-1B8) antibody has a slight cross-reactionwith PSD-93 but does not cross-react with SAP-102. The PSD-95antibody from TL is less effective for immunoprecipitation.

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Figure 1. Specificity of antisera to MAGUKs. Western blot analysis reveals that the SAP-97 antiserum does not cross-react with the other PDZ proteins and gives a band corresponding to ~120 kDa in HEK293 transfected cells. As shown previously (Müller et al., 1995), SAP-97 is not heavily expressed in hippocampus. The anti-rabbit PSD-93 polyclonal antibodies (AL and R-DB) show the same specificity for PSD-93 in transfected cells and in adult hippocampus. In rat hippocampus, at least two bands at ~103-110 kDa can be detected. By similar analysis, the SAP-102 (JH62514 or GP-DB) antibodies recognize their antigens but show no cross-reactivity with the other members of the MAGUK family. PSD-95 (TL and JH62092) antibodies are the most specific antibodies against PSD-95 available. T60 anti-PSD-95 is a polyclonal antibody that reacts with PSD-95 as strong as with SAP-97 in transfected cells. In hippocampus, in addition to the 95 kDa specific band, we find two additional lighter bands at ~170 and 85 kDa. The arrows indicate a nonspecific band which appears only in transfected cells. AL, Alomone Laboratories; GP, guinea pig; Gt, goat; R, rabbit; TL, Transduction Laboratories.

Western blot analysis of rat hippocampus shows different patterns for PSD-93/PSD-95 versus SAP-102 during development

As an initial step, we determined the patterns of expression of AMPA and NMDA receptor subunits and MAGUKs during postnataldevelopment in the hippocampus (Figs. 2, 3). AMPA receptor subunitsand the NR1 subunit showed similar patterns of development witha general increase with time after birth. Individually, NR2A andNR2B showed opposite patterns: NR2A immunoreactivity was undetectableat P2 and began to be elevated from P10 to 6 months, whereas NR2Bwas strongly expressed at P2 and showed a substantial decreaseby 6 months. However, the combination of NR2A and NR2B, determinedwith an antibody that recognized both subunits, showed a patternsimilar to that of NR1 and the AMPA receptor subunits. Analysisof the MAGUKs showed that SAP-102 was already highly expressedat P2. The SAP-102 expression increased during the first weekand remained similar through P35 with a reduction in expressionat 6 months. The temporal patterns of expression of both PSD-93and PSD-95 are similar. PSD-93 and PSD-95 were expressed at lowlevels with detection beginning at P10 and increasing throughoutdevelopment. SAP-97 expression in the hippocampus was detectedbut at a level lower than that seen in other brain areas suchas cortex and cerebellum (data not shown). Western blots labeledfor PSD-93 and SAP-102 showed several bands, probably reflectingthe presence of splice variants, which have been reported forboth proteins (Brenman et al., 1996a,b; Müller et al., 1996).Other antibodies to the same proteins showed comparable patternsof expression during development (data not shown).

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Figure 2. Patterns of developmental expression of the glutamate receptor subunits GluR1, GluR2/3, NR1, NR2A/B, NR2A, and NR2B. P2, P10, P35, and 6 month (6M) rat hippocampus homogenates (20 µg of protein/lane) were analyzed by SDS-PAGE and immunoblotting with affinity-purified antibodies: GluR1 (9T), GluR2/3 (25-8), NR1 (clone 54.1), NR2A/B (T12), NR2A (T58), and NR2B (T51). At all ages, samples analyzed with the different antibodies were obtained from the same preparation of hippocampus. Histograms show the relative amount of protein (in percent P35). Levels were measured by densitometric scanning of Western blots.

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Figure 3. Patterns of developmental expression of MAGUKs. P2, P10, P35, and 6 month (6M) rat hippocampus homogenates (20 µg of protein/lane) were analyzed by SDS-PAGE and immunoblotting with antibodies against PSD-93 (AL), SAP-102 (JH62514), and PSD-95 (TL). At all ages, samples analyzed with the different antibodies were obtained from the same preparation of hippocampus. Histograms show the relative amount of protein (in percent P35). Levels were measured by densitometric scanning of Western blots.

Development of PSD-95/SAP-102 proteins at the synapse

Immunogold labeling for PSD-95 (TL) and for SAP-102 (JH62514) in the CA1 region of the hippocampus was concentrated alongthe postsynaptic membrane and in the postsynaptic density (Fig.4). For PSD-95, labeling in synapses increased approximately threefoldfrom P2 to adult (P35) but showed little or no increase from P35to 6 months (Table 2, Fig. 4C). The percent labeled synapsesdoubled from P2 to adult, whereas there was only a small increasein the number of gold particles in a labeled synapse during thistime; the latter increase was not significant for any age. Thisindicates that the increase in PSD-95 during development is attributableprimarily to an increase in the number of synapses containingPSD-95.

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Figure 4. A, Immunogold labeling of PSD-95 in the CA1 stratum radiatum of the hippocampus. Postembedding immunogold labeling (10 nm) was performed using either of two PSD-95 antibodies (b-e, g, h, M, TL; a, f, R, JH), at P2 (a, b), P10 (c, d), P35 (e, f), and 6 months (g, h). p, Presynaptic terminal. Postsynaptic structures include dendrite shafts (b, synapse in a, top right) and spines (c-h); the synapse in the bottom left of a is at the enlarged base of a filopodium extending to the left (data not shown). Scale bar, 0.3 µm. Representative micrographs were chosen to illustrate the increase in PSD-95 labeling in synapses with age. B, Immunogold labeling of SAP-102 in the CA1 stratum radiatum of the hippocampus. Postembedding immunogold labeling (10 nm) was done using either of two SAP-102 antibodies (a, b, d-f, h, i, R, JH; c, g, GP-DB) at P2 (a-c), P10 (d, e), P35 (f, g), and 6 months (h, i). p, Presynaptic terminal. Postsynaptic structures include dendrite shafts (b), protuberances (a, c), and spines (d-i). Scale bar, 0.3 µm. Representative micrographs were chosen to illustrate the decrease in SAP-102 labeling in synapses with age. C, Summary of developmental changes in the number of gold particles per synapse and the number of gold particles per labeled synapse (see Table 2) at P2, P10, P35, and 6 months (6M). Error bars indicate SE.


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Table 2. Summary of immunogold labeling for PSD-95 and SAP-102

In contrast to PSD-95, labeling for SAP-102 in synapses decreased by approximately half from P2 to adult and decreased furtherby 6 months (Table 2, Fig. 4C). Both the percent labeled synapsesand the number of gold particles in a labeled synapse decreasedduring development, unlike the pattern seen for PSD-95. This indicatesthat the decrease in SAP-102 during development depends on a decreasein the number of synapses containing SAP-102 and on the densityof SAP-102 labeling in asynapse.

To determine whether PSD-95 and SAP-102 are present in the same synapse, double labeling was done. Percent double labelingfor SAP-102 and PSD-95 was highest at P35 (31%), when both thedensity at synapses and percent labeled synapses have similarvalues for the two proteins (Fig. 5). Lower levels of double labelingwere found at P2 (13%), P10 (16%), and 6 months (17%), all timeswhen the number of gold particles per synapse is very differentbetween the two proteins. Overall, the developmental changes inpercent double-labeling appear to reflect only a random distribution;we find no evidence for synapse populations that contain onlySAP-102 or only PSD-95.

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Figure 5. Double labeling for SAP-102 (R, JH; 5 nm gold) and PSD-95 (M, TL; 15 nm gold) in the CA1 stratum radiatum of the hippocampus, at P2 (a, b), P10 (c, d), and P35 (e-j). Five nanometer gold in a, c, e, and g is indicated by arrowheads and shown at a higher magnification in b, d, f, and h, respectively. p, Presynaptic terminal. Postsynaptic structures include dendrite shafts (a, b), protuberances (c, d), and spines (e-j). Scale bar: a, c, 0.3 µm; e, g, i, j, 0.2 µm; b, d, f, h, 0.1 µm. Representative micrographs were chosen to illustrate the decrease in SAP-102 and the increase in PSD-95 in synapses with age, and to show examples of single- and double-labeled synapses in adults.

A number of other antibodies were used to confirm the above findings. Other antibodies to PSD-95 (JH62092; Fig. 4A) and SAP-102(GP-DB; Fig. 4B) showed similar patterns of increasing and decreasinglabeling, respectively, during development. Thus for PSD-95 (JH62092),percent labeled synapses increased with age: P2, 16%; P10, 29%;P35, 42%; for SAP-102 (GP-DB), percent labeled synapses decreasedwith age: P2, 76%; P10, 61%; P35, 33%. An antibody to PSD-93 (AL)showed a pattern of increasing labeling of synapses from P2 toadult that was very similar to the pattern obtained with the twoPSD-95 antibodies (Fig. 6). In contrast, another PSD-93 antibody(GP-DB), which recognizes PSD-93, as well as PSD-95, SAP-97, andSAP-102, showed an increase in labeling from P2 to P10 but littlechange from P10 to adult, probably reflecting simultaneous changesin several proteins (data not shown).

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Figure 6. Immunogold labeling of PSD-93 (R, AL) in the CA1 stratum radiatum of the hippocampus. Postembedding immunogold labeling (10 nm) was performed at P2 (a), P10 (b), and P35 (c). p, Presynaptic terminal. Postsynaptic structures include dendrite shafts (a, b) and spines (c). Scale bar, 0.3 µm. Representative micrographs were chosen to illustrate the increase in PSD-93 labeling in synapses with age, similar to that seen for PSD-95.

Finally, to determine whether PSD-93 is present in the same synapses as PSD-95 or SAP-102, double-labeling was done in adults.Sixteen percent of synapses (n = 116) were double-labeled forPSD-93 (AL) and SAP-102 (JH62514), whereas 33% (n = 106) weredouble-labeled for PSD-93 (AL) and PSD-95 (TL). Thus, PSD-93 co-localizeswith both SAP-102 and PSD-95 in these synapses and may co-localizemore commonly with PSD-95.

Comparison of labeling for PSD-95 and SAP-102 in different postsynaptic structures (shaft, protuberance, or spine) duringdevelopment did not reveal any consistent pattern (data not shown).However, there was an indication that, at least for SAP-102 atP2, SAP-102 is lower (gold/synapse) in dendrite shaft synapsesthan in spine synapses. This would be consistent with a modelin which most dendrite shaft synapses at P2 develop into spinesynapses (Fiala et al., 1998), and SAP-102 levels increase inthe initial stages of synapsedevelopment.

Relationship between NMDA receptor subunits and PSD-95 and SAP-102

The developmental patterns of PSD-95 and SAP-102, both from Western blots of hippocampus and immunogold analysis of CA1 synapses,suggest a possible relationship between these proteins and theNR2 subunits NR2A and NR2B. In particular, the high expressionof NR2B at young ages coincides with the earlier expression ofSAP-102, whereas the later expression of NR2A coincides with thatof PSD-93 and PSD-95. This raises the possibility that SAP-102is primarily associated with NR2B and that PSD-93 and PSD-95 areprimarily associated with NR2A. To test this hypothesis, we didco-immunoprecipitation analyses on NR2A, NR2B, SAP-97, PSD-93,PSD-95, and SAP-102. DOC-solubilized membranes from whole hippocampusor from the CA1-CA2 region of P2 and P35 rats were immunoprecipitatedwith anti-NR2A, anti-NR2B, anti-PSD-97, anti-PSD-93, anti-PSD-95,and anti-SAP-102 antibodies and analyzed by Western blotting usingantibodies to NMDA receptor subunits (NR1, NR2A, and NR2B), PSD-97,PSD-93, PSD-95, and SAP-102 and AMPA receptor subunits (as controls).Co-immunoprecipitation of NR2A and NR2B occurred to some extentin both whole hippocampus (Fig. 7A) and CA1-CA2 (Fig. 7B), consistentwith several reports showing that NMDA receptor complexes thatcontain NR2A, NR2B, and NR2A/NR2B co-exist in individual neurons(Blahos and Wenthold, 1996; Kew et al., 1998). Antibodies to NR2Aor NR2B co-immunoprecipitated both PSD-95 and SAP-102 with anapparent preference for NR2A/PSD-95 and NR2B/SAP-102 (Fig. 7).Moreover, PSD-93, PSD-95, and SAP-102 co-immunoprecipitated bothNR2A and NR2B with a preference for NR2A/PSD-93/95 and NR2B/SAP-102(Fig. 8). The interaction cannot be quantified directly, becausedifferent antibodies, which are likely to have different affinities,were used. However, an indication of the interactions can be obtainedby comparing the relative amounts of co-immunoprecipitating protein.Using this approach, we find that 3.8 ± 0.3% of PSD-95 and 3.7± 0.5% of SAP-102 co-immunoprecipitated with NR2A, whereas 2.3± 0.4% of PSD-95 and 6.2 ± 0.5% of SAP-102 co-immunoprecipitatedwith NR2B (for PSD-95, n = 7; for SAP-102, n = 7). Immunoprecipitationwith antibodies to PSD-95 and SAP-102 showed similar results:2.9 ± 0.3% of NR2A and 1.9 ± 0.4% of NR2B co-immunoprecipitatedwith PSD-95, whereas 1.6 ± 0.3% of NR2A and 3.3 ± 0.5% of NR2Bco-immunoprecipitated with SAP-102 (for NR2A, n = 9; for NR2B,n = 6). Thus, these analyses support a slight but not completepreference for NR2A/PSD-95 and NR2B/SAP-102 association. PSD-93tends to behave as PSD-95 and interacts mostly with NR2A. At P2,when few NR2A complexes were found and PSD-93 or PSD-95 was poorlyexpressed, only NR2B co-immunoprecipitated with SAP-102 and viceversa (Fig. 9). SAP-97 was not abundant in the hippocampus, butsome GluR2/3/SAP-97 complexes were found (Fig. 8). Moreover, SAP-97did not seem to associate with NMDA receptors in the hippocampus,although an interaction between SAP-97 and NR2A has been shownin yeast experiments (Bassand et al., 1999).

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Figure 7. Co-immunoprecipitation of PSD-95 and SAP-102 with NR2 subunits. Whole hippocampus (A) or the CA1-CA2 region of the hippocampus (B) was solubilized in 1% DOC, and GluR2/3, NR2A, or NR2B were immunoprecipitated using 25-8 (GluR2/3) antibody, T58 NR2A serum, or T51 NR2B serum. Ten microliters of the total soluble protein (S) and 10 µl of the bound immunoprecipitate fractions were resolved by SDS-PAGE and probed with GluR2/3 (25-8), NR1 (clone 54.1), NR2A (2F6.3D5), NR2B (TL), PSD-95 (TL), and SAP-102 (JH62514). Because the immunoprecipitates were resuspended in 0.1 volume of the original soluble fraction, the bound sample is 10 times more concentrated than the total soluble fraction.

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Figure 8. Co-immunoprecipitation of NR subunits with PSD-93, PSD-95, or SAP-102 in whole hippocampus. Hippocampi were solubilized in 1% DOC, and SAP-97, PSD-93, PSD-95, and SAP-102 were immunoprecipitated using JH62426, PSD-93 AL, T60, or JH62514 sera, respectively. Ten microliters of the total soluble protein input (S) and 10 µl of the bound immunoprecipitate fractions were separated by SDS-PAGE, immunoblotted, and incubated with antibodies against GluR2/3 (25-8), NR1 (clone 54.1), NR2A (2F6.3D5), NR2B (TL), SAP-97 (JH62426), PSD-93 (R-DB), PSD-95 (TL), or SAP-102 (JH62514). Because the immunoprecipitates were resuspended in 0.1 volume of the original soluble fraction, the bound sample is 10 times more concentrated than the total soluble fraction.

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Figure 9. Comparison of co-immunoprecipitation of PSD-95 and SAP-102 with NR2 subunits at P2 and P35. P2 and P35 hippocampi were solubilized in 1% DOC, and the same amount of protein was used for immunoprecipitation of NR2A and NR2B using T58 NR2A or T51 NR2B sera, respectively. Total soluble protein (S) and the bound immunoprecipitate fractions were resolved by SDS-PAGE and probed with NR2A (2F6.3D5), NR2B (TL), PSD-95 (TL), and SAP-102 (JH62514).

A qualitative examination of double labeling for SAP-102 and NR2A/B or PSD-95 and NR2A/B at P2, P10, and P35 showed some doublelabeling at all ages, although no particular pattern was evident(data not shown). This is not surprising because the NR2A/B antibodyrecognizes both subunits and cannot distinguish between individualpatterns of NR2A or NR2B. Specific antibodies for NR2A and NR2Bwere not used for immunocytochemistry, because they recognizeadditional proteins. In addition to distinctive synaptic associations,single-label studies with antibodies to PSD-95, SAP-102, and NMDAreceptors and double labeling for SAP-102 and NR2A/B showed thatall of these proteins are present in nonsynaptic surface specializations(Fiala et al., 1998). These structures resemble postsynaptic densities;they are adjacent to various nonsynaptic structures or to an emptyfluid-filled space (a common feature in the neuropil at earlypostnatal ages). Nonsynaptic surface specializations were mostcommon at P2, when they labeled commonly with antibodies to NR1,NR2A/B, and SAP-102 and less commonly with antibody to PSD-95(Fig. 10).

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Figure 10. Immunogold labeling (10 nm gold) of NR1 (a, b), NR2A/B (c-e), PSD-95 (f, g; M, TL), and SAP-102 (h-j; R, JH) in nonsynaptic surface specializations (arrowheads) in the CA1 stratum radiatum of the hippocampus at P2. Scale bar, 0.2 µm.

SAP-102, PSD-95, and AMPA receptors

We have previously demonstrated that the synaptic expression of AMPA receptors in hippocampal synapses occurs later in developmentthan does that of NMDA receptors (Petralia et al., 1999), raisingthe possibility that PSD-95 synaptic expression is related tothe acquisition of AMPA receptors at these synapses. To test this,double-labeling analysis was done with antibodies to the AMPAreceptor subunits GluR2/3 and PSD-95. Analysis was done at P10when expression of both proteins is relatively low in synapses(29% of synapses were labeled for PSD-95, and 38% were labeledfor GluR2/3; Petralia et al., 1999). However, only 10% of thesynapses were double-labeled (data not shown), suggesting thatthere is no apparent relationship between the expression of GluR2/3and PSD-95 in synapses duringdevelopment.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the present study, we investigated the synaptic association of SAP-97, PSD-93, SAP-102, and PSD-95 during postnatal developmentin the rat hippocampus. Our major findings show that (1) SAP-102is present at high levels at most synapses at P2 and decreasesthrough 6 months of age, whereas PSD-95 and PSD-93 are low atP2 and increase through 6 months; (2) Increases in synaptic PSD-95are attributable primarily to an increase in the number of synapsescontaining PSD-95, whereas decreases in SAP-102 result from adecrease in both the number of synapses containing SAP-102 andthe density of SAP-102 labeling in the synapse; (3) immunogoldco-localization shows that multiple MAGUKs are expressed at thesame synapse, indicating that PSD-93 and PSD-95 may be added tosynapses that already contain SAP-102; (4) the developmental increasein synaptic PSD-93/95 correlates with increases in NR2A; immunoprecipitationdoes not show a strict relationship between NR2A and PSD-93/95or NR2B and SAP-102 but indicates a preference for this patternof interaction; and (5) the developmental increase in PSD-95 alsocorrelates with the increase in synaptic AMPA receptors, but co-localizationanalysis does not show a relationship between PSD-95 and AMPAreceptors at individualsynapses.

Our results show that SAP-102 is highly expressed at CA1-CA2 synapses in young rats and tends to decline with development.In contrast, PSD-93 and PSD-95 appear to be expressed later, whenAMPA receptors are common at these synapses. These patterns fitthose previously reported for whole brain, as determined withWestern blotting or in situ hybridization (Cho et al., 1992; Mülleret al., 1996; Song et al., 1999; Wyszynski et al., 1999), suggestingthat the developmental pattern we find at hippocampal synapsesmay be common to all CNS synapses. The dramatic enrichment ofSAP-102 at young synapses, when other members of the MAGUK familyare faintly expressed, may indicate an important role for SAP-102in synaptogenesis. On the other hand, the expression of PSD-93and PSD-95 later in development shows that these two proteinsare not required for the early expression of NMDA receptors atsynapses and suggests a role for these proteins in the matureand less plastic synapse. The number of synapses that are immunolabeledwith PSD-95 antibodies increases sharply during development, butthe number of gold particles per labeled synapse, reflecting thenumber of PSD-95 molecules present at the synapse, does not significantlychange from P2 through 6 months of age. Such a pattern of expressionsuggests that the acquisition of PSD-95 may be regulated at thelevel of the individual synapse, rather than reflecting the totalcellular expression levels as indicated by Western blots. Thedecrease in synaptic SAP-102 with age is gradual, suggesting thatthe synaptic expression may be related to the general cellularlevels of SAP-102, like that seen on Western blots. These differentpatterns of acquisition and loss also suggest that the switchfrom SAP-102 to PSD-95 is not a simple replacement of NMDA receptoranchors.

Our results highlight several differences between expression determined by Western blotting and expression determined by immunocytochemistryof the synapse. For example, the Western blot analysis shows asignificant increase in SAP-102 protein during the first weekafter birth and a decrease between P35 and 6 months. However,the percent of synapses labeled and the particles per labeledsynapse decrease gradually with age, with P2 showing the highestlabeling. These discrepancies could arise in two ways. First,our Western blots are of the entire hippocampus, whereas our immunocytochemistryis restricted to synapses on CA1-CA2 pyramidal cell dendrites.Expression patterns may vary in different areas and cell typesof the hippocampus. Second, total cellular expression and synapticexpression may not match. We tend to favor this explanation, becauseSAP-102 is abundant in cytoplasm (Müller et al., 1996; our unpublisheddata). Furthermore, the AMPA receptor subunit GluR1 can show developmentalchanges in intracellular levels that do not match changes in synapticlevels (Shi et al., 1999).

We investigated several mechanisms that may be involved in the regulation of the acquisition of PSD-93 and PSD-95. One explanationfor our results is that PSD-95 and SAP-102 are present at differentpopulations of synapses, and that the population containing PSD-95develops later than the one containing SAP-102. This seems unlikely,because at P2 most synapses (71%) contain SAP-102. Double-labelimmunogold analyses show that, at all ages, some synapses expressboth PSD-95 and SAP-102, as well as PSD-93 and PSD-95, indicatingthat there is a mixture of MAGUKs at any one synapse. Therefore,these data suggest that the addition of PSD-95 occurs predominantlyat synapses that already contain SAP-102. An alternative explanationis that early SAP102-containing synapses are lost, and new synapses,containing both SAP-102 and PSD-95, are formed. Our finding thatPSD-93, PSD-95, and SAP-102 can be co-localized at the same synapseis consistent with studies demonstrating interactions betweenindividual MAGUKs and indicates that these interactions occurat synapses and are likely to be functionally significant. PSD-95forms homomultimers via its N-terminal domain (Hsueh et al., 1997)and heteromultimers with PSD-93 (Kim et al., 1996). Also, it wasrecently demonstrated that SAP-102 and PSD-95 can interact witheach other in the presence of Ca²⁺ and calmodulin (Masuko et al., 1999).

Our data show a close correspondence between the developmental patterns of NR2B and postsynaptic SAP-102 and between the developmentalpatterns of NR2A and postsynaptic PSD-93/95. Such a pattern isexpected if NR2B is associated with SAP-102 and NR2A is associatedwith PSD-93/95, as has been proposed in the retina (Koulen etal., 1998a,b). To address this possibility, we studied the co-immunoprecipitationproperties of these proteins in the young and the adult hippocampus.In the P2 hippocampus, we find that NMDA complexes contain mainlyNR2B associated with SAP-102. In adult hippocampus, we find thatNMDA receptor complexes containing either NR2B alone or NR2A aloneare predominant, although some complexes are found containingboth NR2 subunits. These results are consistent with reports showingthat single neurons can contain three types of NMDA receptors,those with only NR2A, only NR2B, and both NR2A and NR2B (Kew etal., 1998). In these immunoprecipitation studies, we did not seean absolute bias for an association of NR2A and PSD-93/95 or NR2Band SAP-102, although quantitation showed relatively more PSD-95immunoprecipitating with NR2A and more SAP-102 immunoprecipitatingwithNR2B.

Our results indicate that in hippocampus, SAP-102 is the earlier developmental anchor that may be involved in organizing NMDAreceptors at synapses. These results differ from those reportedfor cultured hippocampal neurons by Rao et al. (1998), in whichit was found that PSD-93, PSD-95, and guanylate kinase-associatedprotein were often present at synapse-like structures before NMDAreceptors appeared. Thus, based on those results, it was suggestedthat PSD-93, PSD-95, and GKAP play a key role in synapse formation.More recently, Masuko et al. (1999) showed that SAP-102 and NR2Bco-localize at synaptic sites in cultured rat hippocampal neurons.Although SAP-102 and PSD-95 were not simultaneously studied incultures, the results of the culture studies (Rao et al., 1998)are inconsistent with ours, because we see NMDA receptors at synapsesbefore PSD-95. A likely explanation is that formation of synapsesin culture and in vivo are different, and that the mechanismscontrolling critical events, such as the association of a receptorwith a synaptic anchor, are not the same in culture as in vivo.Our results, however, would support the idea that SAP-102 is precedingthe appearance of NMDA receptors at the synapse or at least thatSAP-102 and NMDA receptors appear simultaneously at the synapticsites. In searching for structures that may represent the earlystages of a developing synapse, we have found nonsynaptic immunolabelingnear the plasma membrane for NR1, NR2A/B, SAP-102, PSD-95, anddouble-labeled SAP-102 and NR2A/B, most commonly at P2. SynapticRas-GTPase-activity protein, which interacts with SAP-102 andPSD-95 (Kim et al., 1998), also was common in these structures(N. Sans, R. S. Petralia, Y.-X Wang, and R. J. Wenthold, unpublisheddata). Many of these have a dense appearance (Fiala et al., 1998),like a postsynaptic density, and it is not possible to determinewhether they are new formations or remnants of formersynapses.

Because PDZ domains 1 and 2 of SAP-102 and PSD-95 (and PSD-93) are similar, the functional consequences of changing theseanchors may not be directly related to their association withNMDA receptors. Rather, it may reflect associations the anchorshave with other molecules (for review, see Nagano et al., 1998;Kim and Huganir, 1999). For the most part, these interactionshave not been demonstrated for all MAGUKs, but rather, it hasbeen assumed that similar interactions occur based on their sequencesimilarities. From our results, it is important to know whetherthe same proteins interact with PSD-95 and SAP-102. PSD-95-mutantmice show a normal pattern of NMDA receptor expression (Migaudet al., 1998). Because our results show that synapses expressboth SAP-102 and PSD-95 (as well as PSD-93), receptors that arenormally associated with PSD-95 would probably be linked withthe remaining two anchors. The plasticity differences in the PSD-95-mutantmice, enhanced long-term potentiation and an absence of long-termdepression, could arise from these abnormal associations. It willbe interesting to determine whether the changes in synaptic expressionof SAP-102 and PSD-95 during development are related to the physiologicalchanges that occur during the critical period of development inthe hippocampus and otherstructures.

  FOOTNOTES

Received Aug. 3, 1999; revised Nov. 15, 1999; accepted Nov. 15, 1999.

This work was supported by the National Institute on Deafness and Other Communication Disorders intramural program (R.J.W.)and by National Institutes of Health Grant NS 35563 (J.W.H.).We thank Dr. J. Fex and members of the laboratory of R.J.W. forcritical reading of thismanuscript.
N.S. and R.S.P. contributed equally to thispaper.

Correspondence should be addressed to Dr. Nathalie Sans, National Institute on Deafness and Other Communication Disorders,National Institutes of Health, Building 36, Room 5D08, Bethesda,MD, 20892. E-mail: sansn{at}nidcd.nih.gov.

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