Differential Cellular and Subcellular Localization of AMPA Receptor-Binding Protein and Glutamate Receptor-Interacting Protein

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The Journal of Neuroscience, January 15, 2001, 21(2):495-503

Differential Cellular and Subcellular Localization of AMPA Receptor-Binding Protein and Glutamate Receptor-Interacting Protein
Alain Burette¹, Latika Khatri², Michael Wyszynski³, Morgan Sheng³, Edward B. Ziff², and Richard J. Weinberg¹
¹ Department of Cell Biology and Anatomy, University of North Carolina, Chapel Hill, North Carolina 27599, ² Howard Hughes Medical Institute and Department of Biochemistry, New York University Medical School, New York, New York 10016, and ³ Howard Hughes Medical Institute and Department of Neurobiology, Massachusetts General Hospital and Harvard Medical School, Boston, Massachusetts 02114

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Excitatory synaptic currents in the mammalian brain are typically mediated by the neurotransmitter glutamate, acting at AMPAreceptors. We used immunocytochemistry to investigate the distributionof AMPA receptor-binding protein (ABP) in the cerebral neocortex.ABP was most prominent in pyramidal neurons, although it was alsopresent (at lower levels) in interneurons. ABP and its putativebinding partners, the GluR2/3 subunits of the AMPA receptor, exhibitedprominent cellular colocalization. Under appropriate processingconditions, colocalization could also be documented in puncta,many of which could be recognized as dendritic spines. However,a sizable minority of GluR2/3-positive puncta were immunonegativefor ABP. Because glutamate receptor-interacting protein (GRIP)may also anchor GluR2, we studied the relative distribution ofABP and GRIP. There was extensive colocalization of these twoantigens at the cellular level, although GRIP, unlike ABP, wasstrongest in nonpyramidal neurons. Different parts of a singledendrite could stain selectively for ABP or GRIP. To further characterizethis heterogeneity, we investigated punctate staining of neuropilusing synaptophysin and the membrane tracer DiA to identify probablesynapses. Some puncta were comparably positive for both ABP andGRIP, but the majority were strongly positive for one antigenand only weakly positive or immunonegative for the other. Thisheterogeneity could be seen even within adjacent spines of a singledendrite. These data suggest that ABP may act as a scaffold forAMPA receptors either in concert with or independently fromGRIP.

Key words: cerebral cortex; pyramidal neurons; PDZ; scaffolding proteins; GluR2/3; AMPA receptors; ABP; GRIP

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ionotropic glutamate receptors concentrate at the plasma membrane overlying the excitatory postsynaptic density (PSD) (forreview, see Ottersen and Landsend, 1997; Conti and Weinberg, 1999;Nusser, 2000). Investigation of the molecular basis for this phenomenonled to the discovery that PSD-95, a novel protein concentratedat the PSD, binds to the NMDA receptor (for review, see Kennedy,1997; O'Brien et al., 1998). PSD-95 is one of a family of proteinsexpressing PDZ domains, modular sites for protein-protein interactionshared by PSD-95, the Discs-large protein in Drosophila, and ZO-1,a protein found at the epithelial zonula occludens (for review,see Ponting et al., 1997; Sheng and Wyszynski, 1997). The secondPDZ domain of PSD-95 binds to the C-terminal motif of the NR2subunit (Kornau et al., 1995; Niethammer et al., 1996). Besideshelping to anchor NMDA receptors, PSD-95 may regulate second-messengerpathways by bringing the receptor into proximity with downstreamsignaling molecules such as the scaffolding molecule InaD, thePDZ domains of which are crucial organizers of the Drosophilaphototransduction cascade (for review, see Ziff, 1997; Cravenand Bredt, 1998; Migaud et al., 1998; Scott and Zuker, 1998).

Synapses in cerebral cortex and hippocampus commonly coexpress NMDA and AMPA receptors (Bekkers and Stevens, 1989; Kharaziaet al., 1996; He et al., 1998; Takumi et al., 1999; Nusser, 2000).However, NMDA and AMPA receptors lie at different loci withinthe synaptic active zone (Kharazia and Weinberg, 1997; Somogyiet al., 1998). Yeast two-hybrid screens have identified glutamatereceptor-interacting protein (GRIP), a protein containing sevenPDZ domains that can bind to the AMPA subunit GluR2 in vitro (Donget al., 1999), and more recently, AMPA receptor-binding protein(ABP), and its splice variant, ABP-L, sometimes termed GRIP-2,a homologous protein coded on a different gene (Srivastava etal., 1998; Bruckner et al., 1999; Dong et al., 1999; Wyszynskiet al., 1999). Biochemical evidence indicates an association betweenseveral PDZ domains of ABP and the C termini of the GluR2/3 subunits(Dong et al., 1999; Wyszynski et al., 1999), but there is no structuralevidence that ABP is actually associated with synaptic glutamatereceptors in intact brain. Moreover, it remains unclear what thefunctional significance of two related AMPA-binding proteins maybe. Do they function in concert to help organize the AMPA receptorsignaling pathway, or do they act independently? If the two proteinsact cooperatively, both must be at the same synapse. However,GRIP in cerebral neocortex concentrates in specific classes ofinhibitory local circuit neurons, whereas the limited evidenceavailable suggests a more widespread distribution for ABP (Srivastavaet al., 1998; Burette et al., 1999; Dong et al., 1999).

These considerations motivated us to ask whether ABP colocalizes with GluR2/3, and if so, whether ABP and GRIP colocalize.We provide direct evidence for synaptic colocalization of ABPwith GluR2/3 in the adult cerebral cortex and document an unexpectedlycomplex pattern of colocalization between ABP andGRIP.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antiserum. ABP antibody was generated by immunizing rabbits with a peptide corresponding to amino acids 759-774, lying withinits unique C-terminal L2 region. An extra C-terminal Cys was includedto permit glutaraldehyde conjugation to keyhole limpet hemocyanin(KLH) (Srivastava et al., 1998). This antibody recognizes bothABP and ABP-L/GRIP-2. Two anti-GRIP antibodies were used. Antibody1756/B.O. was raised in rabbits against a hexahistidine-taggedfusion protein incorporating GRIP amino acids 664-1112, includingPDZ6 and extending to the C terminus of the protein (for characterization,see Wyszynski et al., 1998, 1999). Because of concerns regardingpossible cross-reaction, we also used a second affinity-purifiedantibody that was generated by immunizing rabbits with a peptidecorresponding to GRIP amino acids 1084-1100 (SDWSEQNSAFFQQPSHG),conjugated to KLH through a cysteine added to the N terminus ofthe peptide (S. deSouza and E. Ziff, unpublished observations);this region of GRIP is not shared by ABP, making the possibilityof cross-reactionunlikely.

Tissue preparation. All procedures related to the care and treatment of animals were in accordance with institutional andNational Institutes of Health guidelines. Nine male Sprague Dawleyrats (200-350 gm) (Charles River Laboratories, Raleigh NC) wereused for this study. Animals were deeply anesthetized with sodiumpentobarbital (60 mg/kg, i.p.). After intracardiac injection ofheparin, six rats were perfused through the heart with saline,followed by freshly depolymerized 4% paraformaldehyde in phosphatebuffer (PB; 0.1 M, pH 7.4). Transverse sections 20-70 µm thickwere cut on a vibratome and collected in cold PB. To assess whetherlimited antibody access consequent to aldehyde cross-linking mayinfluence results, we perfused five animals with 0.5% paraformaldehyde,followed by a saline flush. In additional experiments, we performedpartial proteolysis on material fixed with 4% paraformaldehyde(Watanabe et al., 1998; Burette et al., 1999); before the immunohistochemicalincubations, sections were treated at 37°C for 10 min with pepsin(2 U/ml in acetic acid, 0.5 M) (Sigma, St. Louis,MO).

To assess antibody specificity, we performed experiments on transfected cells; C1-ABP (Wyszynski et al., 1999) (S. DeSouza,L. Khatri, and E. B. Biff, unpublished observations) or GRIP expressionplasmids were introduced into HeLa cells using Effectene lipofectionreagents (Qiagen, Valencia, CA). At 48 hr after transfection,cells were fixed for 10 min in 0.5% depolymerized paraformaldehydein PB or for 2 hr in 4% paraformaldehyde inPB.

ABP immunostaining. For immunoperoxidase, free-floating sections fixed with 4% paraformaldehyde were treated for 30 min with3% H₂O₂ in PBS, pH 7.4 (to quench endogenous peroxidase activity),and then preincubated in 10% normal donkey serum (to block secondaryantibody binding sites). Sections were incubated in primary antibodyto ABP (1:1000 dilution) overnight on a shaker at room temperature.Sections were then incubated for 3 hr in biotinylated anti-rabbitantibody (1:200) (Vector Laboratories, Burlingame, CA) and for1 hr in ExtrAvidin-peroxidase complex (1:5000) (Sigma); peroxidasewas histochemically visualized with diaminobenzidine. Processedsections were mounted on gelatin-coated slides and coverslippedwith DPX mountant (BDH Chemicals, Poole,UK).

For immunofluorescence, tyramide signal amplification (TSA) permitted the use of primary antibody at dilutions of 1:10,000-1:20,000(for tissue fixed with 4% paraformaldehyde), and 1:40,000-1:100,000(for tissue fixed with 0.5% paraformaldehyde). After overnightincubation in primary antibody and repeated washes in PBS containing0.1% Tween 20 (PBS-T), the sections were reacted for 2 hr at roomtemperature with biotinylated secondary antibody (1:200 in PBS)(Jackson ImmunoResearch, West Grove, PA). Biotin was localizedby TSA (Renaissance direct) (DuPont NEN, Wilmington, DE); tissuewas incubated in PBS containing 0.5% blocking reagent for 30 min,then incubated in streptavidin-HRP (diluted 1:100 in PBS) foran additional 30 min. Three washes with PBS-T were followed bya 5-7 min application of tyramide conjugated to FITC or Cy3, diluted1:50 in amplification diluent, and then washed with PBS-T.

To obtain a better appreciation of the relationship between cellular morphology and immunostaining, we used the membrane tracerDiA (Molecular Probes, Eugene, OR), which labels even the finestneuronal processes. DiA crystals were applied with a micropipettedirectly to some of the immunostained sections, which were thenstored at 4°C for 24-72 hr. Sections were mounted on gelatin-coatedslides and either air-dried and cleared with xylene before beingcoverslipped with Fluoromount (Gurr BDH, Toronto, Canada) or directlycoverslipped with Vectashield mounting medium (VectorLaboratories).

Multiple labeling. The first primary antibody was amplified with TSA, whereas the second and third primary antibodies wererevealed with conventional fluorescent staining (Hunyady et al.,1996; Shindler and Roth, 1996). Sections were immunoprocessedfor ABP as described above. After the application of the dye-conjugatedtyramide and preincubation in 1% BSA in PBS-T, the second primaryantibodies (either GRIP or GluR2/3 antibody, at dilutions of 1:1,000-1:2,000for material fixed with 4% paraformaldehyde and 1:5,000-1:10,000,for material fixed with 0.5% paraformaldehyde) were applied overnight.Immunoreactivity was visualized with donkey anti-rabbit conjugatedto rhodamine (Jackson ImmunoResearch). Sections labeled for ABPand GluR2/3 were then processed for synaptophysin (clone SVP-38,1:1,000) (Sigma) or DiA labeling. Sections labeled for ABP andGRIP were then processed for synaptophysin, GluR2/3 (goat antibodySc-7610) (Santa Cruz Biotechnology, Santa Cruz, CA), orDiA.

For optimal z-axis resolution, semithin plastic sections were prepared after immunofluorescence processing. Sections werethen dehydrated and flat-embedded in Lowicryl HM20 (Polysciences,Warrington, PA). After polymerization, 1 µm sections were cut,heat-mounted on slides, and coverslipped withFluoromount.

To control for possible cross-reaction between the first primary antibody and the second secondary antibody (both raised inrabbit), the tissue was processed as described above, except thatthe second primary antibody was omitted. These sections were uniformlynegative for the staining of the secondary antibodies. Moreover,we obtained consistent experimental results when the order ofthe first two primary antibodies wasreversed.

Microscopy and data analysis. Sections were examined with a Leitz DMR microscope under bright field, Nomarski, or epifluorescenceillumination. Fluorescent images were acquired with a cooled charge-coupleddevice camera (Princeton Instruments, Trenton, NJ) coupled toa Macintosh computer. IP Lab software (Scanalytics, Fairfax, VA)was used for image acquisition and initial processing. For optimalresolution of thick sections, images were acquired with a LeicaTCS confocal microscope. With optical sectioning, it was possiblewith this instrument to assess continuity of processes throughthe thickness of asection.

Quantification of puncta was performed on confocal images from randomly selected cortical fields. Images were acquired witha 100× oil objective with a pinhole diameter of 1.3 optical units(OUs) and 1× magnification. Quantification of immunopositive spinesidentified by DiA was performed on 25 µm confocal z-axis stacks,acquired with a 63× oil objective with a pinhole diameter of 1.3OU and 1×magnification.

We also used the confocal instrument as a photometer to assess immunofluorescence staining of cells quantitatively. Randomlyselected cortical fields were displayed at high magnificationon the Leica TCS host computer screen. Neurons well defined byeither ABP or GRIP immunocytochemistry were outlined, and meanpixel values of the outlined region were computed. Normalizedimmunofluorescence was computed as [(mean pixel value of cell) $-$ (mean pixel value of background)]/[(mean pixel value of brightestcell measured on section) $-$ (mean pixel value of background)],yielding a dimensionless photometric value between 0 (immunofluorescenceat background level) and 1 (the brightest cell measured). We usedCorel Draw v.9 (Corel, Ontario, Canada) to sharpen images, adjustbrightness and contrast level, and compose finalplates.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Distribution of ABP

Most neurons in cerebral cortex were immunopositive for ABP. Both weakly and strongly stained neurons were present in allcortical layers (Fig. 1A). Some of these could be identified aspyramidal neurons (Fig. 1B); others were nonpyramidal cells ofvarious shapes and sizes. The degree of staining varied accordingto cell type: pyramidal neurons were generally more intenselystained for ABP than were nonpyramidal neurons. A few nonpyramidalneurons (<1% of all labeled neurons) were particularly intenselyimmunopositive, with a characteristic pattern of staining mainlyrestricted to the edge of the cell, at or adjacent to the plasmamembrane (Fig. 1B, inset). Although scattered through the cortex,these neurons were most frequently encountered in layers I-III.Except for these "ABP-intense" neurons, staining was typicallypatchy within proximal dendrites and somatic cytoplasm, excludingthe nucleus. Immunopositive puncta were observed throughout theneuropil, particularly in layers I and II. We interpret thesepuncta as dendritic branches cut in cross-section, rather thanimmunoreactive synapses, because no clear association with thepresynaptic marker synaptophysin could be detected in double-labelingexperiments (data not shown).

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Figure 1. Immunostaining for ABP in cerebral cortex. A, Immunoperoxidase staining in 40-µm-thick tissue section, fixed with 4% paraformaldehyde. ABP immunoreactivity was found in neurons throughout all layers of cortex. B, Detail from layer V. Arrow points to a pyramidal neuron; staining is organized into patches in the soma and proximal part of the apical dendrite (arrowheads). Inset shows a nonpyramidal neuron with a characteristic ABP-intense pattern of staining concentrated at the edge of the cell. Scale bars: A, 100 µm; B, 20 µm; inset, 10 µm.

The apparent lack of synaptic staining was unexpected, considering published evidence from postembedding immunoelectron microscopy(Srivastava et al., 1998). We reasoned that if ABP acts to anchorGluR2, it may be complexed with other proteins within the postsynapticdensity, thus limiting antibody access. To explore whether theremay be an occult synaptic pool of ABP only poorly detected withstandard preembedding methods, we performed immunocytochemistryon sections pretreated with pepsin and on tissue only weakly fixedwith paraformaldehyde. With both techniques, staining of punctain the neuropil was considerably enhanced. Unfortunately, proteolytictreatment caused substantial damage to tissue sections and impairedcytoplasmic staining. The most satisfactory results were obtainedfrom sections weakly fixed by 0.5% paraformaldehyde (Fig. 2).This procedure markedly increased the detection of antigen whilesuppressing background and thus provided optimal visualizationof the cellular and subcellular distribution of ABP. In this material,intense patchy staining was observed in somata and proximal dendritesand in puncta throughout the neuropil (Fig. 2A,B). Double-labelingexperiments showed a close relationship between many of thesepuncta and synaptophysin (Fig. 2C), indicating that weak fixationby 0.5% paraformaldehyde allowed the detection of the synapticpool of ABP. Of 873 synaptophysin-positive puncta, 281 (32%) wereassociated with an ABP-positive punctum. Conversely, of 370 ABP-positivepuncta, 281 (76%) showed juxtaposition or partial overlap witha synaptophysin-positive punctum (Fig. 3A), suggesting that mostimmunocytochemically identified ABP puncta were synaptic. Thissynaptic localization was confirmed by double labeling with themembrane tracer DiA, which showed that many dendritic spines containABP (Fig. 2D,E).

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Figure 2. ABP immunofluorescent staining after fixation with 0.5% paraformaldehyde. A, B, Intense patchy staining was observed in somata (arrows) and dendrites. C, Numerous immunoreactive puncta were also present in the neuropil. These puncta often showed juxtaposition or partial overlap with synaptophysin (Syn.)-positive terminals (arrowheads on insets corresponding to the 3 boxes in main panel) and were thus likely to correspond to synapses. D, E, To elucidate the relationship of these puncta to cell processes, we performed double labeling with the membrane tracer DiA (in z-axis stack, as illustrated by representative optical sections). Dense cellular staining of a small pyramidal neuron (D, E, arrows) contrasts with weaker ABP immunostaining in a nonpyramidal neuron (asterisk). DiA staining reveals that ABP concentrates at spines; most of these are likely to be on dendritic branches originating from pyramidal neurons (D, arrowheads; E, insets, arrowheads), but a few are on sparsely spiny dendrites of nonpyramidal neurons (E, curved arrows). Scale bars: A, B, 10 µm; C, 20 µm; insets, 5 µm; D, E, 25 µm.

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Figure 3. Chart summarizing the quantitative data on synaptic localization of ABP and its colocalization with GluR2/3 and GRIP. A, A close relationship between ABP puncta and synaptophysin was observed in the neuropil; 76% of ABP puncta showed juxtaposition or partial overlap with a synaptophysin-positive punctum. B, Seventy-one percent of GluR2/3-positive puncta were likely to be synaptic (as defined by synaptophysin), and 65% of GluR2/3-positive spines (identified by DiA) were immunopositive for ABP. C, Of puncta likely to represent synapses (as defined by synaptophysin) that were immunopositive for either ABP or GRIP, 40% colocalized ABP and GRIP, 31% were selectively positive for ABP, and 28% were selectively positive for GRIP. Results were similar for dendritic spines; of the spines immunopositive for either ABP or GRIP, 42% were stained for both ABP and GRIP, 32% for ABP alone, and 26% for GRIP alone.

Colocalization of ABP with AMPA receptor subunits

Previous studies have shown that ABP interacts with both GluR2 and GluR3 in vitro. If it also binds these subunits in vivo,one would expect ABP immunostaining in neurons immunopositivefor GluR2/3. We therefore performed double labeling for ABP andAMPA receptors using antibodies that recognized both GluR2 andGluR3 subunits. Patterns of immunostaining for GluR2/3 were similarto previous reports (Petralia and Wenthold, 1992). In the cerebralcortex, GluR2/3 antibodies stained somata and dendrites of a largepopulation of pyramidal cells and also stained a substantial numberof nonpyramidal cells. Double labeling showed that many GluR2/3-immunopositiveneurons also expressed high levels of ABP, but a substantial fractionexpressed ABP at low or undetectable levels. In contrast, thevast majority of ABP-positive cells also stained for GluR2/3,with the exception of the scattered ABP-intense neurons, whichgenerally lacked GluR2/3 (Fig. 4A,B).

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Figure 4. Colocalization of ABP with GluR2/3. A, B, Double labeling for ABP and GluR2/3 in layers I-II (A) and III (B), after fixation with 4% paraformaldehyde. Most GluR2/3-positive cells contained ABP immunoreactivity (A, arrows), with the exception of scattered ABP-intense neurons (arrowheads). In the neuropil, GluR2/3 puncta were seldom associated with ABP puncta after strong fixation. C, Double labeling for ABP and GluR2/3 in a large pyramidal neuron of layer V, after fixation with 0.5% paraformaldehyde. In somata and proximal dendrites, ABP patches were sometimes associated with GluR2/3 patches, but many GluR2/3 patches were distinct from ABP patches. In contrast with the labeling after fixation with 4% paraformaldehyde, ABP-immunopositive puncta in the neuropil usually also stained for GluR2/3 (arrows), although some GluR2/3-positive puncta did not stain for ABP (arrowheads). Micrographs are from a 30 µm frozen section (A), a 1-µm-thick plastic section (B), and a 50 µm frozen section (C). Scale bars: A, 50 µm; B, C, 20 µm.

In somata, patches of ABP immunoreactivity occasionally colocalized with GluR2/3 patches, but more typically, these patchesseemed independently organized (Fig. 4C). Considering the denselabeling for both antigens, the overall impression was of a lackof association. In contrast, punctate colocalization of ABP andGluR2/3 was often observed in the neuropil (Fig. 4B,C), althoughsome GluR2/3 puncta were immunonegative for ABP. By combiningimmunolabeling with DiA, we could demonstrate that although manydendritic spines were immunopositive for both markers, many otherswere positive for GluR2/3 but not ABP (Fig. 5).

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Figure 5. Partial colocalization of ABP with GluR2/3 in spines. DiA staining (A3) reveals spiny dendrites (boxed regions are shown at higher magnification in B, C). Many of the spines are immunopositive for both ABP and GluR2/3 (arrowheads), whereas others are positive for only GluR2/3 (arrows). Scale bars: A, 10 µm; B, C, 2 µm.

To assess the relative frequencies of synapses of these two types, we performed triple immunolabeling for GluR2/3, ABP, andsynaptophysin (data not shown). Of 522 GluR2/3-positive punctalikely to be synaptic (as defined by synaptophysin), 373 (71%)were also immunopositive for ABP (Fig. 3B). Using a second approachto identify putative synaptic labeling, we found that of 54 GluR2/3-positivespines (identified by DiA), 35 (65%) were also immunopositivefor ABP (Fig. 3B). That a negative spine could be adjacent toan immunopositive spine (Fig. 5B) documents a high level of chemicalheterogeneity, even within a single dendritictwig.

Colocalization of ABP and GRIP

That ABP and GluR2/3 exhibit only partial colocalization suggests that a sizable fraction of GluR2/3-positive synapses maylack ABP. This led us to explore the relationship between ABPand GRIP, another putative GluR2/3 scaffold. Because ABP (outsideits L2 region) is homologous to GRIP, there is the theoreticalpossibility of cross-reaction between GRIP antisera and ABP. Toassess this possibility, we performed immunofluorescence on transfectedcells. ABP immunoreactivity was detected in ABP-transfected cells,but not in GRIP-transfected cells (Fig. 6A). Likewise, immunoreactivityfor GRIP (antibody 1756/B.O.) was detected in GRIP-transfectedcells, but not in ABP-transfected cells (Fig. 6B). These datasuggest that there was no significant cross-reaction between ABPand GRIP antibodies, at least at the concentration used in thiswork. To verify the reliability of our results, the observationsreported below were qualitatively confirmed using a second GRIPantibody, prepared against a peptide sequence not shared by ABP(deSouza and Ziff, unpublished observations).

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Figure 6. Specificity of the ABP and GRIP antibodies used in the present study. A, Immunofluorescence for ABP. B, Immunofluorescence for GRIP (1756/B. O.). ABP was detected in HeLa cells transfected with ABP (A, arrows), but not in GRIP-transfected cells. Likewise, GRIP was detected in GRIP-transfected cells (B, arrowheads), but not in ABP-transfected cells. Scale bars, 50 µm.

Cellular staining for GRIP was consistent with previous reports (Wyszynski et al., 1998; Burette et al., 1999; Dong et al.,1999): GRIP stained dendrites and somata of nonpyramidal neuronsscattered throughout cortex, and pyramidal cells were only weaklyimmunopositive. Most GRIP-positive cells also contained ABP, andvice versa (Fig. 7A). Cells strongly immunopositive for ABP (mainlypyramidal neurons) were weakly stained for GRIP, whereas cellsstrongly immunopositive for GRIP (a subset of nonpyramidal neurons)were weakly stained for ABP; in contrast, the scattered ABP-intenseneurons were usually strongly positive for both proteins (Fig.7A). Photometry of cells from random high-power fields (see Materialsand Methods) confirmed this impression (Fig. 8): immunofluorescencefor ABP was significantly (p < 0.001; two-sided t test) strongerfor pyramidal cells (mean normalized brightness, 0.640 ± 0.040;n = 23) than for nonpyramidal neurons (0.286 ± 0.033; n = 32),whereas immunofluorescence for GRIP was significantly (p < .001)weaker for pyramidal cells (0.360 ± 0.039) than for other neurons(0.629 ± 0.033).

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Figure 7. Partial immunocolocalization of ABP with GRIP. A, Double labeling for ABP and GRIP in the cerebral cortex; tissue fixed with 4% paraformaldehyde. Most ABP-positive cells contained GRIP immunoreactivity, and vice versa. However, cells strongly immunopositive for ABP (small arrows) were weakly stained for GRIP, whereas cells strongly immunopositive for GRIP (arrowheads) were weakly stained for ABP. Scattered ABP-intense neurons were strongly positive for both proteins (curved arrows). B, C, Double labeling for ABP and GRIP after fixation with 0.5% paraformaldehyde. Intrasomatic patches of ABP immunoreactivity were generally distinct from patches of GRIP. A differential distribution of ABP and GRIP was often observed within the dendritic arborization. B, A proximal dendrite and one of its branches (arrows) were stained for both proteins, but the other branch was stained for GRIP alone (arrowheads). C, The proximal apical dendrite was stained for both proteins (arrows), but more distal regions were stained for ABP alone (arrowheads); likewise, the proximal basal dendrite was stained for both proteins (arrows), but distal branches were stained for GRIP alone (arrowheads). Insets show that many puncta in the neuropil colocalized both ABP and GRIP (arrowheads), but a number of puncta were selectively positive for either GRIP or ABP. Scale bars: A, 50 µm; B, C, 10 µm; inset, 5 µm.

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Figure 8. Relative intensities of ABP and GRIP immunofluorescence in cerebral cortex. Intensity of somatic labeling was measured in 103 neurons spanning all cortical layers from a representative double-stained section. Confocal images were captured, and mean photometric intensities of red and green channels were computed for each that was well defined in either channel; data were normalized from 0 (tissue background) to 1 (brightest cell measured) for each channel. Open triangles represent morphologically identified pyramidal cells, filled circles represent nonpyramidal neurons, and dots represent neurons that could not be clearly identified. The two types of neurons form distinct clusters; pyramidal neurons generally stained strongly for ABP and not for GRIP, whereas nonpyramidal neurons stained strongly for GRIP and not for ABP. Outlying cells, top right, were exceptionally large. A cluster of cells near the origin was stained too weakly to permit clear identification.

Subcellular colocalization was not the rule within the cell body; intrasomatic patches of ABP immunoreactivity were generallydistinct from patches stained for GRIP (Fig. 7B,C). In some cases,ABP and GRIP were differentially distributed within a single dendriticarborization: the proximal dendrite was stained for both proteins,but secondary dendrites were stained for either ABP or GRIP alone(Fig. 7B,C). Beyond suggesting differential transport and/or targetingof the two proteins, these data provide further evidence thatthe two antibodies recognized differentantigens.

Of puncta immunopositive for either ABP or GRIP, we identified 683 that were likely to represent synapses because they eitheroverlapped or were adjacent to synaptophysin-positive puncta.Of these, 274 (40%) colocalized ABP and GRIP, 216 (31%) were selectivelypositive for ABP, and 193 (28%) were selectively positive forGRIP (Fig. 3C). Consistent with this finding, of 53 spines immunopositivefor either ABP or GRIP (as revealed by DiA staining), 22 (42%)were stained for both ABP and GRIP, 17 (32%) for ABP alone, and14 (26%) for GRIP alone (Figs. 3C, 8A,B). The three types of immunostaining(i.e., ABP only, GRIP only, and colocalization of both) couldbe observed on adjacent spines of the same dendrite (Fig. 9A,B).These results, together with the quantitative data on ABP stainingof GluR2/3-positive synapses described above, are consistent withthe possibility that all GluR2/3-positive synapses contain eitherABP or GRIP or both. We then examined spines triple-labeled withGluR2/3, ABP, and GRIP. This combination of labeling requiredhistochemical procedures that yielded suboptimal staining, butwe were able to confirm colocalization of GluR2/3-positive spineswith both of these scaffolding proteins in different combinations(Fig. 9C,D).

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Figure 9. Partial colocalization of ABP with GRIP in GluR2/3-immunoreactive spines. A, B, DiA staining reveals a pyramidal neuron stained for both ABP and GRIP. B, Higher-magnification view of spiny dendrites shown in A. Some spines are immunopositive for both ABP and GRIP (curved arrows), whereas others are immunopositive for ABP alone (straight arrows) or GRIP alone (arrowheads). Note that spines with two different chemical profiles originate from the same dendrite. C, D, Triple immunostaining for ABP, GRIP, and GluR2/3. C, Two vertically directed dendrites are visible on the right. One is immunopositive for GRIP and GluR2/3 (arrowheads) but shows virtually no staining for ABP. The other (boxed areas) is immunostained for all three antigens. D, Enlargement of boxed areas shows GluR2/3-positive spines immunopositive for both ABP and GRIP (curved arrows), for ABP only (straight arrows), and GRIP only (arrowheads), all associated with the same dendrite. Scale bars: A, 10 µm; B, 50 µm; C, 20 µm; D, 3 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Using multiple-label immunocytochemistry, we have characterized the cellular and subcellular expression of ABP and its relationshipswith GluR2/3 and GRIP. Immunostaining for ABP in the cerebralcortex was strong in pyramidal neurons and weaker in nonpyramidalneurons. All three antigens were also found at synapses, but onlyafter proteolytic pretreatment or in weakly fixed tissue, suggestingthat ABP/GRIP may be so tightly complexed with AMPA receptorsand other proteins at the synapse that antibody access is severelyrestricted (Ye et al., 2000).

ABP associates with GluR2/3 in vivo

In vitro evidence suggests a role for ABP in anchoring AMPA receptors. Yeast two-hybrid assays show that ABP can bind viaits PDZ domains 3, 5, and 6 to the C termini of GluR2 and GluR3;furthermore, ABP copurifies with GluR2 in the PSD fraction ofbrain homogenate (Srivastava et al., 1998). The multiple labelingexperiments reported here are consistent with the idea that ABPand GluR2/3 interact in vivo. Although ABP is expressed almostexclusively in GluR2/3-containing neurons, high-resolution imagesshow little subcellular colocalization of the two antigens insomata and proximal dendrites. In contrast, colocalization inthe neuropil is prominent, and a large fraction of this colocalizationis likely to be synaptic, as shown by its association with dendriticspines and with synaptophysin. Together, these observations suggestthat ABP is not involved in cytoplasmic receptor trafficking,but may play an important role at or near the synapse. The roleof ABP in the small group of ABP-intense, GluR2/3-negative cellsremains unclear. For their morphology, location, and intense stainingfor GRIP, we suspect that these are likely to represent a specializedpopulation of GluR1-rich GABAergic interneurons (Burette et al.,1999), suggesting that ABP and GRIP play some scaffolding roleunrelated to GluR2/3 in theseneurons.

ABP and GRIP are differentially expressed

Notwithstanding extensive cellular colocalization of GRIP and ABP, the relative intensity of labeling for the two antigensvaried: cells strongly immunopositive for ABP (mainly pyramidalneurons) were typically weakly stained for GRIP, whereas cellsstrongly immunopositive for GRIP (mainly nonpyramidal neurons)were weakly stained for ABP. Sparsely spiny or aspiny dendriteslikely to originate from nonpyramidal neurons (and previouslyshown to express GRIP at high levels) (Burette et al., 1999) typicallycontained markedly less ABP than did spinydendrites.

We used both dendritic spines and synaptophysin as light microscopic proxies to investigate patterns of synaptic colocalization.Both proxies are dominated by pyramidal neurons: spines originateoverwhelmingly from pyramidal neurons, but even a random sampleof asymmetric synapses (as revealed by synaptophysin) will bedominated by axospinous synapses, considering the relative infrequencyof excitatory synapses on dendritic shafts in neocortex (Feldman,1984). Keeping this caveat in mind, our data suggest that althoughmany of these synapses contained both GRIP and ABP, the majoritywere positive for only one of the proteins. Thus, ABP and GRIPmust be independently regulated; that the three types of immunostaining(ABP only, GRIP only, and colocalization) could be observed onadjacent spines of the same dendrite shows that this regulationis very tight indeed. Notwithstanding the differential distributionof the two antigens, we conclude from the present results thatmost, or perhaps all, GluR2/3-containing synapses in cerebralcortex include either ABP orGRIP.

Possible functional implications

Synaptic AMPA receptors appear to be more firmly anchored at GABAergic (nonpyramidal) cells than at pyramidal neurons (Allisonet al., 1998). In the light of the present evidence, this suggeststhat AMPA receptors are less mobile at GRIP-enriched synapsesthan at ABP-enriched synapses. This raises the possibility thatGRIP might bind GluR2/3 more firmly than does ABP; it would beinteresting to test this hypothesis directly. Heterologous expressionexperiments suggest that ABP and GRIP may copolymerize to formlarge scaffolds within the PSD (Srivastava et al., 1998; Donget al., 1999), leading to the more general hypothesis that theratio of ABP/GRIP may control the mobility of GluR2/3 within thesynapse. Because addition of new AMPA receptors to the synapsemay underlie some forms of long-term potentiation (LTP) (for review,see Malinow, 1998; Malenka and Nicoll, 1999; Turrigiano, 2000),the limited available evidence suggesting more robust LTP in pyramidalthan in nonpyramidal neurons (McMahon and Kauer, 1997; Laezzaet al., 1999; McBain et al., 1999) is consistent with thishypothesis.

In addition to their role as receptor anchors, both GRIP and ABP are likely to act as a molecular scaffold, organizing intracellularsecond-messenger cascades. Notwithstanding their close homology(64-93% in their six PDZ domains), it seems likely that the twoproteins have different binding affinities for intracellular kinasesand phosphatases that may be important in synaptic plasticity(Torres et al., 1998; Bhalla and Iyengar, 1999; Bruckner et al.,1999; Bloomfield and Ziff, 2000; Soderling and Derkach, 2000)(M. Wyszynski and M. Sheng, unpublished observations). Interestingly,the novel RasGEF GRASP-1 binds to the seventh PDZ domain of GRIPand its ABP homolog, ABP-L, but not to ABP (which lacks the seventhPDZ domain) (Ye et al., 2000), suggesting functional consequencesof ABP splice variant regulation. The present research pointsto the need for further study of potential intracellular bindingpartners for these scaffoldingmolecules.

  FOOTNOTES

Received July 31, 2000; revised Oct. 25, 2000; accepted Oct. 30, 2000.

This work was supported by National Institutes of Health Grants NS35527 (R.J.W.), AG13620 (E.B.Z.), and NS35050 (M.S.). E.B.Z.is an investigator and M.S. is an assistant investigator of theHoward Hughes Medical Institute. We thank R. J. Wenthold for antibodiesagainst GluR2/3.
Correspondence should be addressed to Richard Weinberg, Department of Cell Biology and Anatomy, CB 7090, University of NorthCarolina, Chapel Hill, NC 27599. E-mail: rjw{at}med.unc.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Allison DW, Gelfand VI, Spector I, Craig AM (1998) Role of actin in anchoring postsynaptic receptors in cultured hippocampal neurons: differential attachment of NMDA versus AMPA receptors. J Neurosci 18:2423-2436[Abstract/Free Full Text].
Bekkers JM, Stevens CF (1989) NMDA and non-NMDA receptors are colocalized at individual excitatory synapses in cultured rat hippocampus. Nature 341:230-233[Medline].
Bhalla US, Iyengar R (1999) Emergent properties of networks of biological signaling pathways. Science 283:381-387[Abstract/Free Full Text].
Bloomfield S, Ziff EB (2000) Novel interactions with AMPA receptor binding protein. Soc Neurosci Abstr 26:527.
Bruckner K, Pablo Labrador J, Scheiffele P, Herb A, Seeburg PH, Klein R (1999) EphrinB ligands recruit GRIP family PDZ adaptor proteins into raft membrane microdomains. Neuron 22:511-524[ISI][Medline].
Burette A, Wyszynski M, Valtschanoff JG, Sheng M, Weinberg RJ (1999) Characterization of glutamate receptor interacting protein-immunopositive neurons in cerebellum and cerebral cortex of the albino rat. J Comp Neurol 411:601-612[ISI][Medline].
Conti F, Weinberg RJ (1999) Shaping excitation at glutamatergic synapses. Trends Neurosci 22:451-458[ISI][Medline].
Craven SE, Bredt DS (1998) PDZ proteins organize synaptic signaling pathways. Cell 93:495-498[ISI][Medline].
Dong H, Zhang P, Song I, Petralia RS, Liao D, Huganir RL (1999) Characterization of the glutamate receptor-interacting proteins GRIP1 and GRIP2. J Neurosci 19:6930-6941[Abstract/Free Full Text].
Feldman LF (1984) Morphology of the neocortical pyramidal neuron. In: Cerebral cortex (Peters A, Jones EG, eds), pp 123-189. New York: Plenum.
He Y, Janssen WG, Morrison JH (1998) Synaptic coexistence of AMPA and NMDA receptors in the rat hippocampus: a postembedding immunogold study. J Neurosci Res 54:444-449[ISI][Medline].
Hunyady B, Krempels K, Harta G, Mezey E (1996) Immunohistochemical signal amplification by catalyzed reporter deposition and its application in double immunostaining. J Histochem Cytochem 44:1353-1362[Abstract].
Kennedy MB (1997) The postsynaptic density at glutamatergic synapses. Trends Neurosci 20:264-268[ISI][Medline].
Kharazia VN, Weinberg RJ (1997) Tangential synaptic distribution of NMDA and AMPA receptors in rat neocortex. Neurosci Lett 238:41-44[ISI][Medline].
Kharazia VN, Phend KD, Rustioni A, Weinberg RJ (1996) EM colocalization of AMPA and NMDA receptor subunits at synapses in rat cerebral cortex. Neurosci Lett 210:37-40[ISI][Medline].
Kornau HC, Schenker LT, Kennedy MB, Seeburg PH (1995) Domain interaction between NMDA receptor subunits and the postsynaptic density protein PSD-95. Science 269:1737-1740[Abstract/Free Full Text].
Laezza F, Doherty JJ, Dingledine R (1999) Long-term depression in hippocampal interneurons: joint requirement for pre- and postsynaptic events. Science 285:1411-1414[Abstract/Free Full Text].
Malenka RC, Nicoll RA (1999) Long-term potentiation: a decade of progress? Science 285:1870-1874[Abstract/Free Full Text].
Malinow R (1998) Silencing the controversy in LTP? Neuron 21:1226-1227[Medline].
McBain CJ, Freund TF, Mody I (1999) Glutamatergic synapses onto hippocampal interneurons: precision timing without lasting plasticity. Trends Neurosci 22:228-235[ISI][Medline].
McMahon LL, Kauer JA (1997) Hippocampal interneurons express a novel form of synaptic plasticity. Neuron 18:295-305[ISI][Medline].
Migaud M, Charlesworth P, Dempster M, Webster LC, Watabe AM, Makhinson M, He Y, Ramsay MF, Morris RG, Morrison JH, O'Dell TJ, Grant SG (1998) Enhanced long-term potentiation and impaired learning in mice with mutant postsynaptic density-95 protein. Nature 396:433-439[Medline].
Niethammer M, Kim E, Sheng M (1996) Interaction between the C terminus of NMDA receptor subunits and multiple members of the PSD-95 family of membrane-associated guanylate kinases. J Neurosci 16:2157-2163[Abstract/Free Full Text].
Nusser Z (2000) AMPA and NMDA receptors: similarities and differences in their synaptic distribution. Curr Opin Neurobiol 10:337-341[ISI][Medline].
O'Brien RJ, Lau LF, Huganir RL (1998) Molecular mechanisms of glutamate receptor clustering at excitatory synapses. Curr Opin Neurobiol 8:364-369[ISI][Medline].
Ottersen OP, Landsend AS (1997) Organization of glutamate receptors at the synapse. Eur J Neurosci 9:2219-2224[ISI][Medline].
Petralia RS, Wenthold RJ (1992) Light and electron immunocytochemical localization of AMPA-selective glutamate receptors in the rat brain. J Comp Neurol 318:329-354[ISI][Medline].
Ponting CP, Phillips C, Davies KE, Blake DJ (1997) PDZ domains: targeting signalling molecules to sub-membranous sites. BioEssays 19:469-479[ISI][Medline].
Scott K, Zuker CS (1998) Assembly of the Drosophila phototransduction cascade into a signalling complex shapes elementary responses. Nature 395:805-808[Medline].
Sheng M, Wyszynski M (1997) Ion channel targeting in neurons. BioEssays 19:847-853[ISI][Medline].
Shindler KS, Roth KA (1996) Double immunofluorescent staining using two unconjugated primary antisera raised in the same species. J Histochem Cytochem 44:1331-1335[Abstract].
Soderling TR, Derkach VA (2000) Postsynaptic protein phosphorylation and LTP. Trends Neurosci 23:75-80[ISI][Medline].
Somogyi P, Tamas G, Lujan R, Buhl EH (1998) Salient features of synaptic organisation in the cerebral cortex. Brain Res Brain Res Rev 26:113-135[Medline].
Srivastava S, Osten P, Vilim FS, Khatri L, Inman G, States B, Daly C, DeSouza S, Abagyan R, Valtschanoff JG, Weinberg RJ, Ziff EB (1998) Novel anchorage of GluR2/3 to the postsynaptic density by the AMPA receptor-binding protein ABP. Neuron 21:581-591[ISI][Medline].
Takumi Y, Ramirez-Leon V, Laake P, Rinvik E, Ottersen OP (1999) Different modes of expression of AMPA and NMDA receptors in hippocampal synapses. Nat Neurosci 2:618-624[ISI][Medline].
Torres R, Firestein BL, Dong H, Staudinger J, Olson EN, Huganir RL, Bredt DS, Gale NW, Yancopoulos GD (1998) PDZ proteins bind, cluster, and synaptically colocalize with Eph receptors and their ephrin ligands. Neuron 21:1453-1463[ISI][Medline].
Turrigiano GG (2000) AMPA receptors unbound: membrane cycling and synaptic plasticity. Neuron 26:5-8[ISI][Medline].
Watanabe M, Fukaya M, Sakimura K, Manabe T, Mishina M, Inoue Y (1998) Selective scarcity of NMDA receptor channel subunits in the stratum lucidum (mossy fibre-recipient layer) of the mouse hippocampal CA3 subfield. Eur J Neurosci 10:478-487[ISI][Medline].
Wyszynski M, Kim E, Yang FC, Sheng M (1998) Biochemical and immunocytochemical characterization of GRIP, a putative AMPA receptor anchoring protein, in rat brain. Neuropharmacology 37:1335-1344[ISI][Medline].
Wyszynski M, Valtschanoff JG, Naisbitt S, Dunah AW, Kim E, Standaert DG, Weinberg R, Sheng M (1999) Association of AMPA receptors with a subset of glutamate receptor-interacting protein in vivo. J Neurosci 19:6528-6537[Abstract/Free Full Text].
Ye B, Liao D, Zhang X, Zhang P, Dong H, Huganir RL (2000) GRASP-1: a neuronal RasGEF associated with the AMPA receptor/GRIP complex. Neuron 26:603-617[ISI][Medline].
Ziff EB (1997) Enlightening the postsynaptic density. Neuron 19:1163-1174[ISI][Medline].

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