Role of Actin in Anchoring Postsynaptic Receptors in Cultured Hippocampal Neurons: Differential Attachment of NMDA versus AMPA Receptors

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The Journal of Neuroscience, April 1, 1998, 18(7):2423-2436

Role of Actin in Anchoring Postsynaptic Receptors in Cultured Hippocampal Neurons: Differential Attachment of NMDA versus AMPA Receptors
Daniel W. Allison¹, Vladimir I. Gelfand¹, Ilan Spector², and Ann Marie Craig¹
¹ Department of Cell and Structural Biology, University of Illinois, Urbana, Illinois 61801, and ² Department of Physiology and Biophysics, State University of New York, Stony Brook, New York 11794

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We used actin-perturbing agents and detergent extraction of primary hippocampal cultures to test directly the role of theactin cytoskeleton in localizing GABA_A receptors, AMPA- and NMDA-typeglutamate receptors, and potential anchoring proteins at postsynapticsites. Excitatory postsynaptic sites on dendritic spines containeda high concentration of F-actin that was resistant to cytochalasinD but could be depolymerized using the novel compound latrunculinA. Depolymerization of F-actin led to a 40% decrease in both thenumber of synaptic NMDA receptor (NMDAR1) clusters and the numberof AMPA receptor (GluR1)-labeled spines. The nonsynaptic NMDAreceptors appeared to remain clustered and to coalesce in cellbodies. $alpha$ -Actinin-2, which binds both actin and NMDA receptors,dissociated from the receptor clusters, but PSD-95 remained associatedwith both the synaptic and nonsynaptic receptor clusters, consistentwith a proposed cross-linking function. AMPA receptors behaveddifferently; on GABAergic neurons, the clusters redistributedto nonsynaptic sites, whereas on pyramidal neurons, many of theclusters appeared to disperse. Furthermore, in control neurons,AMPA receptors were detergent extractable from pyramidal cellspines, whereas AMPA receptors on GABAergic neurons and NMDA receptorswere unextractable. GABA_A receptors were not dependent on F-actinfor the maintenance or synaptic localization of clusters. Theseresults indicate fundamental differences in the mechanisms ofreceptor anchoring at postsynaptic sites, both regarding the anchoringof a single receptor (the AMPA receptor) in pyramidal cells versusGABAergic interneurons and regarding the anchoring of differentreceptors (AMPA vs NMDA receptors) at a single class of postsynapticsites on pyramidal cell dendritic spines.

Key words: actin; postsynaptic density; AMPA receptor; NMDA receptor; GABA receptor; dendritic spine; PSD-95

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The mechanisms responsible for localizing neurotransmitter receptors to their sites of function at postsynaptic specializations,presumably via attachment to the cytoskeleton, are not well understoodfor the major synapse types in the mammalian brain. At the neuromuscularjunction, acetylcholine receptors are anchored to the actin cytoskeletonby association with rapsyn/43K and additional linker proteins(for review, see Carbonetto and Lindenbaum, 1995; Sanes, 1997).On spinal cord neurons, there is evidence that inhibitory glycinereceptors are anchored by attachment to gephyrin (Kirsch and Betz,1993), which binds tubulin and is highly dependent on microtubulesand partially dependent on actin microfilaments for its localization(Kirsch et al., 1991; Kirsch and Betz, 1995). The specific concentrationsof GABA_A receptors in inhibitory postsynaptic membranes (Somogyiet al., 1989; Craig et al., 1994) and of members of all glutamatereceptor classes (AMPA/kainate, NMDA, and metabotropic) in excitatorypostsynaptic membranes (Petralia and Wenthold, 1992; Baude etal., 1993; Craig et al., 1993; Aoki et al., 1994; Nomura et al.,1994; Petralia et al., 1994; Rao and Craig, 1997) indicate thatthese receptors must be anchored in some manner by cytoskeletalelements, although there is little direct evidence. The functionalstate of the NMDA subtype of glutamate receptor is also mechanosensitiveand regulated in a calcium-dependent manner by the actin cytoskeleton(Rosenmund and Westbrook, 1993; Paoletti and Ascher, 1994).

Many transmembrane proteins are anchored to actin via a direct linkage through bridging proteins, whereas other membrane proteinsare thought to be trapped loosely within membrane domains formedby spectrin-based corrals (for review, see Bennett and Gilligan,1993; Beck and Nelson, 1996). The scaffold for attachment of synapticreceptors likely resides in the postsynaptic density (PSD), anelectron-dense and detergent-resistant core region of the postsynapticspecialization just beneath the membrane (Peters et al., 1991;Kennedy, 1997). Excitatory (asymmetric) synapses contain pronouncedPSDs and most often occur on dendritic spines, structures thatlack neurofilaments and microtubules but are dominated by highconcentrations of actin filaments oriented longitudinally in theneck and forming a lattice in the head (Fifkova and Delay, 1982;Matus et al., 1982; Cohen et al., 1985; Harris and Kater, 1994).Thus it is very likely that actin filaments are intimately involvedin controlling spine shape and may mediate cytoskeletal attachmentof glutamate receptors and interacting postsynaptic proteins.

Recently several potential glutamate receptor anchoring proteins have been identified including $alpha$ -actinin-2, calmodulin, andPDZ domain proteins specific for NMDA receptors (PSD-95/SAP90,chapsyn/PSD-93, and SAP102), AMPA receptors (GRIP), and classI metabotropic receptors (Homer) (Kornau et al., 1995; Ehlerset al., 1996; Kim et al., 1996; Muller et al., 1996; Brakemanet al., 1997; Dong et al., 1997; Wyszynski et al., 1997). Of theseproteins found to interact with glutamate receptors, the onlyone known to interact with conventional cytoskeletal elementsis $alpha$ -actinin-2, an actin cross-linking protein. However, becausemost of these receptor-interacting proteins consist of numerousinteraction domains, they may form such a highly cross-linkednetwork that they do not require association with conventionalcytoskeletal elements for their localization or stabilizationof bound receptors.

Here we used actin-perturbing agents and detergent extraction of primary hippocampal cultures to test directly the roles ofactin filaments in localizing GABA_A receptors, AMPA- and NMDA-typeglutamate receptors, and the NMDA receptor-interacting proteinsPSD-95 and $alpha$ -actinin-2 at postsynaptic sites.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cell cultures. Rat hippocampal cultures were prepared using previously described methods (Banker and Cowan, 1977; Goslin andBanker, 1991). Briefly, hippocampi were dissected from 18 d ratembryos and dissociated using trypsin and trituration througha Pasteur pipette. The neurons were plated on coverslips coatedwith poly-L-lysine in minimal essential medium (MEM) with 10%horse serum at an approximate density of 2400 cells/cm². After the neurons had attached to the substrate, they were transferredto a dish containing a glial monolayer and maintained for up to3 weeks in serum-free MEM with N2 supplements. For studies ofthe NMDA receptor, the cultures were treated chronically from14-21 d in culture with 100 µM 2-amino-5-phosphonovalerate (APV)as described previously (Rao and Craig, 1997). Cytochalasin Dor latrunculin A were added directly to the culture medium fromconcentrated DMSO stocks. Reversal of the effects of latrunculinA was accomplished after a 24 hr treatment in latrunculin A bya 24 hr reversal in a fresh glial dish with conditioned MEM plusN2 supplements lacking latrunculin A. Cytochalasin D was obtainedfrom Sigma (St. Louis, MO). Latrunculin A was isolated from theRed Sea sponge Negombata (known previously as Latrunculia magnifica)as described previously (Groweiss et al., 1983). In brief, samplesof the sponge were lyophilized and extracted for 8 hr in hexane,followed by extraction in chloroform. The resulting liquid phasewas collected and chromatographed twice on Sephadex columns followedby a Silica H column to yield the pure compound. The structureof the pure compound was confirmed by nuclear magnetic resonancespectroscopy. Latrunculin A is now also available from MolecularProbes (Eugene, OR).

Immunocytochemistry. For immunocytochemistry not involving NMDA receptors, neurons were fixed at 20-23 d in culture in warm4% paraformaldehyde and 4% sucrose in PBS for 15 min and werepermeabilized with 0.25% Triton X-100 for 5 min. The cultureswere incubated with 10% bovine serum albumin (BSA) for 30 minat 37°C to block nonspecific staining and were incubated withthe primary antibodies in 3% BSA. For stainings involving theNMDAR1 antibody, the 3-week neurons were simultaneously fixedand permeabilized in methanol for 15 min at $-$ 20°C, followed bythe 10% BSA block and primary antibody staining. Primary antibodiesused included guinea pig anti-GluR1 antiserum (gift of R. L. Huganir,Johns Hopkins University; 1:1600), rabbit anti-GluR1 affinity-purifiedantibody (Upstate Biotechnology, Lake Placid, NY; 1:1000), andmonoclonal antibody 54.1 to NMDAR1 (PharMingen, San Diego, CA;1:100-1:5000 depending on the lot) for the glutamate receptors.Presynaptic sites were labeled with either a rabbit antiserumG95 against synaptophysin (gift of P. DeCamilli, Yale University;1:8000) or a monoclonal antibody against the synaptic vesicleprotein SV2 (gift of K. M. Buckley, Harvard University; 1:50).Microtubule-associated proteins were stained with a rabbit antiserumagainst MAP2 (#266; gift of S. Halpain, Scripps Institute; 1:20,000)and a monoclonal antibody against dephospho-tau-1 (BoehringerMannheim, Indianapolis, IN; 1:400). F-actin was labeled with rhodaminephalloidin (Molecular Probes; 1:10,000). $alpha$ -Actinin was stainedwith monoclonal antibody EA-53 (Sigma; 1:20,000), and PSD-95 wasstained with a guinea pig antiserum (gift of M. Sheng, HarvardUniversity; 1:300). Neurons were incubated in primary antibodiesfor 2 hr at 37°C and in appropriate secondary antibodies for 45min at 37°C. Secondary antibodies were conjugated to fluorescein,Texas Red, or 7-amino-4-methylcoumarin-3-acetic acid (Vector Laboratories,Burlingame, CA; 1:200-1:600). The coverslips were mounted in elvanolwith 2% 1,4-diazabicyclo[2,2,2]octane. Fluorescent images of theneurons were obtained using a Zeiss Axioskop microscope with a63×, 1.4 numerical aperture lens and a Photometrics series 250cooled CCD camera. Images were prepared for presentation usingOncorImage and Adobe Photoshop software.

Quantitation. To quantitate the data from the immunocytochemistry, neurons were chosen randomly for image acquisition (forGluR1/synaptophysin/phalloidin, 20 cells each from five separateexperiments for paired control and latrunculin A treatments; forNR1/synaptophysin, 10 cells each from five separate experimentsfor paired control and latrunculin A treatments). All image analysiswas performed such that the experimenter was blind to the treatmentgroup. For each neuron, two dendrites were chosen for analysisfrom the phase contrast image, and their length was measured.To count GluR1 or NR1 clusters per dendrite length, we processedthe digital images using Oncor imaging software. Before we measuredfluorescence intensities, images were background subtracted bya dark field image and divided by the image of a uniform fluorescencefield to normalize for potential nonuniformity in illumination.Images were subjected to a user-defined intensity threshold toselect spines or clusters (with intensity approximately twofoldor greater above the parent dendrite), a selection for the regionof interest, and a count of the number of clusters or spines alongeach chosen dendrite. For NR1, all clusters on spines and shaftswere counted (see Fig. 8), whereas for GluR1, the diffuse labelingof dendritic shafts was high, and we could only reliably observeGluR1 clusters on spines (see Fig. 5). Hence we report "GluR1-labeledspines" that are equivalent to spiny GluR1 clusters. The datawere compiled in Microsoft Excel, analyzed in Statview, and plottedusing CricketGraph.

Western blot analysis. Hippocampal cultures were grown at a density of 14,300 cells/cm² and used at 18-19 d in culture for Western blot analysis. Forextraction, the neurons were treated with 1% Triton X-100 and4% polyethylene glycol (PEG; molecular weight, 40,000) in BRB80buffer (80 mM PIPES, 1 mM MgCl₂, and 1 mM EGTA) for 5 min, rinsedin BRB80, and scraped into sample buffer for Western blots; afew coverslips were also fixed for staining. Nonextracted cultureswere scraped into warm PBS, collected by centrifugation, and resuspendedin Laemmli buffer. The samples were analyzed by SDS-PAGE and blottedonto nitrocellulose. Blots were probed with antibodies againstGluR1 (Upstate Biotechnology; 1:5000) and NMDAR1 (PharMingen;1:1000). HRP-conjugated secondary antibodies (Jackson ImmunoResearch,West Grove, PA; 1:10,000) were used in combination with chemiluminescentSuper-Signal HRP substrate (Pierce, Rockford, IL) to produce thesignals on x-ray film before digital scanning. Blots were thenstripped with SDS and $beta$ -mercaptoethanol, reprobed with monoclonalantibody C4 against actin (Boehringer Mannheim; 1:1000) and apolyclonal antibody against $alpha$ -actinin-2 (4B2; gift of M. Shengand A. H. Beggs, Harvard University; 1:2000), and visualized asdescribed above.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Actin filaments and AMPA receptors are concentrated in dendritic spines

Primary cultures from embryonic rat hippocampus develop excitatory synapses on dendritic spines with morphologies similarto those seen in vivo, although sometimes with a less pronouncedPSD (Bartlett and Banker, 1984; Papa et al., 1995). Postsynapticclusters of both AMPA- and NMDA-type glutamate receptors developon the neurons and are generally numerous by 3 weeks in appropriatecultures (Craig et al., 1993; Rao and Craig, 1997). The pyramidalneurons form both spiny and shaft glutamatergic postsynaptic sites,whereas the GABAergic neurons, which comprise ~7% of the culturedneurons, develop primarily shaft synapses (Craig et al., 1993;Benson et al., 1994).

We show here that excitatory synapses on dendritic spines in culture exhibit high concentrations of F-actin (Fig. 1C), asdo dendritic spines in vivo (Matus et al., 1982). Embryonic rathippocampal neurons in low density culture were triple-labeledwith rhodamine phalloidin for F-actin and with antibodies forthe AMPA-type glutamate receptor subunit GluR1 and for synaptophysinas a marker for presynaptic terminals (Fletcher et al., 1991).In mature neurons ( $>=$ 3 weeks in culture), these three proteinsappeared concentrated together at synaptic sites on dendriticspines (Fig. 1). F-actin was also present in a filamentous patternthroughout the rest of the neuron, but the highest concentrationswere observed at dendritic spines. Essentially all dendritic spinesthat stained positive for GluR1 were enriched for F-actin. F-actinwas detectable at low levels but not concentrated at dendriteshaft synapses, including shaft synapses containing clusters ofeither GluR1 or GABA receptors (data not shown).

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Figure 1. Coclustering of GluR1 and F-actin at synapses on dendritic spines of cultured rat hippocampal neurons. A, Phase contrast imageof a typical pyramidal neuron at 3 weeks in culture (boxed areashows region enlarged in B-D). B-D, Staining with an antibodyagainst the synaptic vesicle protein SV2 to label presynapticterminals (B), with rhodamine phalloidin to label F-actin (C),and with an antibody against the GluR1 subunit of the AMPA-typeglutamate receptor (D). GluR1 and F-actin were present at highconcentrations at some spiny synapses (arrowheads). In contrast,synapses on dendrite shafts of pyramidal neurons did not exhibithigh concentrations of F-actin or of GluR1 (arrow); these maycorrespond to glutamatergic synapses lacking concentration ofthe AMPA receptor or to GABAergic synapses. Scale bars, 10 µm.

Actin filaments within spines are particularly stable but can be disrupted with latrunculin A

We set out to disrupt actin filaments at postsynaptic sites to determine the effects on clustering and/or synaptic localizationof neurotransmitter receptors and of potential anchoring proteins.Disruption of F-actin is typically achieved in most cell typesusing cytochalasin D or related compounds. Cytochalasin D hasmany effects on actin; one activity is to cap the fast-growingplus end of the actin filament, preventing further polymerization.Because of other processes that sever actin filaments, this generallyleads to a loss of filaments of normal length and an abundanceof very short actin filaments (Cooper, 1987). To test its effectivenesson hippocampal cultures, we incubated neurons after 3 weeks inculture in several concentrations of cytochalasin D ranging upto 10 µg/ml. After up to 24 hr of treatment, the cultures werefixed and stained with rhodamine phalloidin (Fig. 2E,G). The F-actinwithin the somata and neurite shafts was effectively reduced bycytochalasin D, but F-actin was still concentrated within thespines, similar to the control neurons. This result indicatesthat the filamentous actin within dendritic spines is selectivelyresistant to destruction by cytochalasin D.

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Figure 2. Disruption of neuronal F-actin and its effect on GluR1-labeled spines. Neurons were stained at 3 weeks in culture with rhodaminephalloidin to label F-actin (A, C, E, G, I, K, M, O) and withan antibody against GluR1 (B, D, F, H, J, L, N, P). The smallerboxes (C, D, G, H, K, L, O, P) show enlarged regions from theneurons above (arrowheads represent spines). There were many spineswith concentrations of both F-actin and GluR1 in control neurons(A-D) and after treatment with 10 µg/ml cytochalasin D for 24hr (E-H). Although much of the cortical actin was disrupted bycytochalasin D, the spines were still positive for both F-actin(E, G) and GluR1 (F, H). In contrast, after a 24 hr treatmentwith 5 µM latrunculin A, most of the F-actin was depolymerized(I, K) with a corresponding loss of GluR1-labeled spines (J, L).Some neurons exhibited apparently "deflated" spines after latrunculinA treatment, protrusions close to the shafts lacking F-actin (M,O) but still containing concentrations of GluR1 (N, P). Scalebars, 10 µm.

Because we were unable to depolymerize F-actin in spines using cytochalasin D, we tried another actin-specific drug with adifferent mechanism of action. Latrunculin A, a compound isolatedfrom the Red Sea sponge Negombata, binds to monomeric actin witha 1:1 stoichiometry, thus sequestering G-actin and resulting innet actin filament depolymerization. This compound has provento be effective on many cell types including mouse neuroblastomaN1E-115 cells (Spector et al., 1989). Treatment of hippocampalcultures with 1.3-5 µM latrunculin A for up to 48 hr gave verydifferent results from the cytochalasin D treatment. Treatmentwith 5 µM latrunculin A for 24 hr (Fig. 2I,K,M,O) resulted ina loss of F-actin from both the shafts of the neurites and thedendritic spines. In most cases, the F-actin staining was completelyundetectable in the neurons; occasionally, a few small patchesremained in the shafts of the neurites but not in the spines.

After 2 hr of latrunculin A treatment, the neurons resembled the 24 hr cytochalasin D treatment; F-actin was somewhat reducedin these neurons but still fairly abundant, particularly in dendriticspines (Fig. 3B). By 9 hr, some neurons exhibited no F-actin staining,whereas other neurons still exhibited considerable F-actin inshafts and in spines (Fig. 3C). By 24 hr of latrunculin A treatment,there was no detectable rhodamine phalloidin staining in mostneurons (Fig. 3D), except for the occasional staining of someshort, extremely stable filaments within cell bodies or dendriteshafts. Treatment with latrunculin A for 48 hr was toxic; 24 hrwas therefore chosen for the following studies.

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Figure 3. Time course of the effects of latrunculin A in disrupting actin polymers. Hippocampal neurons were treated at 3 weeks in culturewith 5 µM latrunculin A, fixed at time 0 (A) or after 2 hr (B),9 hr (C), or 24 hr (D) of treatment, and stained for F-actin withrhodamine phalloidin. After 2 hr of latrunculin A treatment, corticalF-actin was reduced but still detectable and in particular wasconcentrated in dendritic spines. After 9 hr of latrunculin Atreatment, most of the F-actin was depolymerized, although therewere still some dendrite shaft regions (C) and a few spines containingF-actin (data not shown). After latrunculin A treatment for 24hr, the neurons were almost devoid of F-actin staining, and F-actin-labeledspines were not observed. The images in A-D were taken at thesame exposure and scaled equally to preserve the differences inF-actin staining. Scale bar, 10 µm.

The effects of a 24 hr latrunculin A treatment were reversible and thus did not cause any irreparable damage to the cell.Figure 4A-D shows neurons treated for 24 hr with latrunculin Aand then allowed to recover for another 24 hr in latrunculin A-freemedia. This was sufficient time for the F-actin to repolymerizewithin these cells, as seen with rhodamine phalloidin, and sufficienttime for many of the spines to reform. This observation may indicateeither that latrunculin A simply removes actin from the spines,deflating them, or possibly that the mechanism for forming newspines can occur within the 24 hr time period. Latrunculin A treatmenthad no effect on neuronal polarity or on the distribution of presynapticterminals. The microtubule-associated proteins MAP2 (a dendriticmarker; Caceres et al., 1984) and tau (an axonal marker; Mandelland Banker, 1996) exhibited their normal polarized distributionsafter 24 hr of latrunculin A treatment (Fig. 4E,F). The synapticvesicle protein synaptophysin also exhibited its usual punctatestaining pattern indicating clustering in presynaptic terminals(see Fig. 7). Given evidence that F-actin may be important inorganizing synaptic vesicles within terminals (Hirokawa et al.,1989), there may be ultrastructural differences within the terminals,but we observed no effects on synaptophysin or SV2 localizationat the light microscopic level.

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Figure 4. Reversal of latrunculin A effects and maintenance of neuronal polarity. Hippocampal neurons were treated for 24 hr with latrunculinA (E, F) and in some cases were allowed to recover for an additional24 hr in latrunculin A-free media (A-D; C and D show enlargedregions of A and B). A 24 hr reversal lead to a complete recoveryof the normal F-actin staining pattern and GluR1 clustering ondendritic spines (F-actin, A, C; GluR1, B, D). As a control forthe specificity of latrunculin A, the distributions of the microtubule-associatedproteins MAP2 (a dendritic marker, E) and tau (an axonal marker,F) were shown to be unaffected by the 24 hr latrunculin A treatment.There was no difference in the staining patterns between latrunculinA-treated (E, F) and paired control (data not shown) neurons.Arrowheads indicate axons that are tau-positive and MAP2-negative.Scale bars, 10 µm.

Depolymerization of F-actin reduces the number of GluR1-labeled spines in pyramidal neurons

AMPA receptors on pyramidal neurons seemed to depend on F-actin both for synaptic localization and for the maintenance ofclusters (Figs. 2, 5). These observations are based on qualitativeand quantitative immunofluorescence analyses of control versuslatrunculin A-treated 3-week cultured neurons stained with antibodiesagainst GluR1 and synaptophysin along with rhodamine phalloidinfor F-actin visualization. Randomly selected, multiply innervatedcells were analyzed to determine the number of GluR1-labeled spinesper dendrite length (Fig. 5A,B). Control neurons averaged fromfive separate cultures had 21.7 ± 0.8 (mean ± SEM) GluR1-labeledspines per 100 µm of dendrite length, consistent with previousresults showing that GluR1 labels only a subpopulation of spines(Rao and Craig, 1997). This value decreased significantly to 13.6± 0.6 (mean ± SEM) GluR1-labeled spines per 100 µm of dendritelength after latrunculin A treatment of the neurons (t test, p< 0.0001; see Fig. 5 for complete set of data). No single latrunculinA-treated neuron exhibited what would be classified as typicalspines. Many latrunculin A-treated cells exhibited no GluR1-labeledspines (Fig. 2I-L). However, other neurons still exhibited whatwe have termed deflated spines after latrunculin A treatment (Fig.2M-P). All of the spines, including these deflated spines, remainedopposed to presynaptic terminals. Thus the lack of a normal spinestructure did not necessarily cause the entire synapse to breakdown; ~40% of the synapses lost AMPA receptor clusters, but therest retained AMPA receptor clusters on these deflated spines.

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Figure 5. GluR1-labeled spines decrease in number after latrunculin A treatment. The number of GluR1-labeled dendritic spines per 100µm of dendrite length was counted for 200 control and 200 latrunculinA-treated dendrites. A, B, Typical counts for regions of controland latrunculin A-treated dendrites, respectively. Arrowheadsrepresent clusters of GluR1 on dendritic spines. Many of the spinesremaining after latrunculin A treatment resemble the smaller deflatedspines that are typical of this treatment. C, These data werethen compiled into a graph in histogram form, with the black barsrepresenting control neurons and the gray bars the latrunculinA-treated neurons. Control neurons exhibited 21.68 ± 0.81 (mean± SEM) spines per 100 µm, whereas latrunculin A-treated neuronshad only 13.57 ± 0.64 (mean ± SEM) spines per 100 µm. This representsa significant decrease in spine number (t test, p < 0.0001). Scalebars, 10 µm.

We did not observe any nonsynaptic clusters of GluR1 resulting from latrunculin A treatment of pyramidal neurons. Althoughthere is significant staining for GluR1 along dendrite shaftsand so shaft clusters may have been more difficult to observe,the data are most consistent with the idea that the AMPA receptorsdispersed from many of the spiny clusters after actin depolymerization.After removal of latrunculin A, apparently normal GluR1-labeledspines recovered within 24 hr (Fig. 4B,D). This recovery may involvereclustering of existing receptors or insertion of new receptorsbut was fairly rapid compared with the protracted time courseof initial development of these GluR1-labeled spines (Craig etal., 1993).

Depolymerization of F-actin perturbs the synaptic localization of GluR1 clusters on GABAergic neurons

In contrast to the results on pyramidal neurons, AMPA receptors on GABA cells seemed to depend on F-actin for synaptic localizationbut not for the maintenance of clusters (Fig. 6). Figure 6A-Ddemonstrates the staining for GluR1 on a typical GABAergic cell(Craig et al., 1993), with intensely labeled receptor clustersat synapses on the dendrite shafts and low levels of nonsynapticreceptor. To determine whether these shaft GluR1 clusters weredispersed by actin disruption, we randomly selected GABAergicneurons by phase contrast in latrunculin A-treated and matchedcontrol cultures and classified them for the presence or absenceof GluR1 clusters. Actin depolymerization did not disperse GluR1from clusters on GABA cells. In the control neurons, 57.2% (n= 145) of the GABAergic cells had easily identifiable GluR1 clusters;with latrunculin A treatment, 61.5% (n = 143) of the GABAergiccells had GluR1 clusters. However, although GluR1 clusters stillremained after actin depolymerization, these clusters were usuallyno longer synaptic (Fig. 6E-H). Thus unlike the results on pyramidalneurons, although F-actin is not necessary for the maintenanceof an AMPA receptor cluster on the GABA cells, it is necessaryfor proper synaptic localization.

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Figure 6. GABAergic neurons exhibit nonsynaptic GluR1 clusters after actin depolymerization. A-D, A typical GABAergic neuron immunostainedfor GluR1 (A, enlarged region in C) and the synaptic vesicle proteinSV2 (B, enlarged region in D) is shown. GluR1 formed clusterson the dendrite shafts opposite SV2-labeled terminals in controlneurons (arrowheads in C, D). E-H, After latrunculin A treatmentto depolymerize F-actin, GluR1 still formed clusters on GABAergicneurons (E, G). However, the GluR1 clusters were no longer localizedto synaptic sites defined by SV2-labeled terminals (F, H) butappeared to be randomly distributed in dendrites at nonsynapticsites (arrowheads in G, H). Scale bars, 10 µm.

Loss of F-actin affects the synaptic distribution of the NMDA receptor

NMDA receptor clusters were partially dependent on F-actin for synaptic localization but not for cluster maintenance (Figs.7, 8). In cultured hippocampal neurons under conditions of spontaneousactivity, the NMDA receptor is partially nonsynaptic; to inducea more spiny synaptic localization, we used chronic treatmentwith NMDA receptor antagonists (Rao and Craig, 1997). The patternof localization of the essential NR1 subunit compared with synaptophysinreveals mainly synaptic shaft and spiny NR1 clusters (Fig. 7A,B).Neurons were treated, as before, with 5 µM latrunculin A for 24hr to test the effect of actin depolymerization on NMDA receptordistribution (Fig. 7C,D). The total number of NR1 clusters per100 µm of dendrite length decreased from 73.8 ± 2.7 for the controlneurons to 44.6 ± 1.8 (mean ± SEM) for the latrunculin A-treatedneurons (t test, p < 0.0001; see Fig. 8 for complete set of data).This decrease in cluster number involved a selective decreasein the number of synaptic NR1 clusters from 68 to 39 clustersper 100 µm of dendrite length, with no change in the number ofnonsynaptic NR1 clusters. In addition, in the latrunculin A-treatedcells, numerous very large nonsynaptic clusters were present incell bodies and sometimes proximal dendrites (Fig. 7C,D) so that,overall, it appeared that the raw number of receptors changedvery little (this apparent increase in nonsynaptic receptor isnot represented in the numbers above, because it occurred mainlyin cell bodies, and only dendritic clusters were counted). Theseresults suggest that latrunculin A treatment induces a partialrelease of NMDA receptor clusters from the cytoskeleton at thesynapse, dissociating the NMDA receptor cluster from its localizationwithin the spines and resulting in movement of the clusters awayfrom synapses. Unlike AMPA receptors, the NMDA receptors did notdisperse but remained clustered or reformed clusters at the nonsynapticsites.

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Figure 7. NR1 clusters depend partially on F-actin for their synaptic localization. Control neurons (A, B) or latrunculin A-treatedneurons (C, D) were immunolabeled for the essential NMDA receptorsubunit NR1 (A, C) and for the synaptic marker synaptophysin (B,D). In control neurons, NR1 formed primarily synaptic clusters(94% synaptic) on both dendrite shafts and on spines (arrowheads).After treatment with latrunculin A, synaptic NR1 clusters werestill present but reduced in number. There was also an apparentincrease in the number of large nonsynaptic clusters located indendrite shafts and cell bodies (arrows). All of these neuronswere pretreated with APV from 14-21 d in culture to induce thesynaptic NR1 pattern (see Rao and Craig, 1997). Scale bar, 10µm.

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Figure 8. NR1 clusters decrease in number after latrunculin A treatment. The number of NR1 clusters per 100 µm of dendrite length wasobtained by quantifying data from 100 control and 100 latrunculinA-treated dendrites. A, B, Regions of a control dendrite stainedfor NR1 and synaptophysin, respectively. C, D, Regions of a latrunculinA-treated dendrite stained for NR1 and synaptophysin, respectively.Arrowheads represent clusters of receptor on both spines and theshaft of the dendrites that colocalize with synaptophysin andare therefore synaptic. Arrows show NR1 clusters that do not exhibitsynaptophysin staining and are thus classified as nonsynaptic.E, The data were then compiled into a graph in histogram form,with the black bars representing control neurons and the graybars the latrunculin A-treated neurons. Control neurons exhibited73.82 ± 2.72 (mean ± SEM) spines per 100 µm, whereas latrunculinA-treated neurons had only 44.60 ± 1.78 (mean ± SEM) spines per100 µm. This represents a significant decrease in total clusternumber (t test, p < 0.0001). The number of nonsynaptic clusterson the dendrites did not change after latrunculin A treatment(5.86 ± 0.38 to 5.96 ± 0.45), and so the total change representsa selective decrease in synaptic NR1 clusters. The number of nonsynapticclusters also appeared to increase in the cell bodies, which werenot included in the quantitation. Scale bars, 10 µm.

Actin depolymerization differentially affects the NMDA receptor interacting proteins $alpha$ -actinin-2 and PSD-95

We next examined the distributions of two of the NMDA receptor binding proteins, $alpha$ -actinin-2 and PSD-95, that may form a linkbetween the receptor and the cytoskeleton. In hippocampal cultures, $alpha$ -actinin-2 and PSD-95 are both concentrated with NMDA receptorsat many excitatory postsynaptic sites (Fig. 9) (Wyszynski et al.,1997). After treatment with latrunculin A, $alpha$ -actinin-2 was completelydispersed from its typical localization at spiny synapses (Fig.9E,G). The complete dispersal of $alpha$ -actinin-2 paralleled the nearcomplete loss of actin filaments, despite the continued presenceof some synaptic NMDA receptor clusters with latrunculin A treatment.In contrast, PSD-95 was less drastically affected by actin depolymerization.PSD-95 still clustered and colocalized with NMDA receptor clusters(Fig. 9M,O), but as was seen for NR1, the PSD-95 clusters appearedto be reduced in number and shifted toward a more nonsynapticdistribution.

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Figure 9. Differential effect of actin depolymerization on the NMDA receptor-interacting proteins $alpha$ -actinin-2 and PSD-95. Control (A-D)or latrunculin A-treated (E-H) neurons were immunolabeled forboth $alpha$ -actinin-2 (A, C, E, G) and GluR1 (B, D, F, H). $alpha$ -Actinin-2was often concentrated in dendritic spines of control neurons,partially colocalizing with GluR1 (arrowheads in A-D) (Rao etal., 1998). After latrunculin A treatment, $alpha$ -actinin-2 immunoreactivitywas no longer clustered or associated with any remaining GluR1clusters (arrowheads in E-H). In contrast, PSD-95 (I, K, M, O)colocalized closely with NR1 (J, L, N, P) in both control (I-L)and latrunculin A-treated (M-P) neurons (arrowheads). Scale bars,10 µm.

The localization of the inhibitory GABA_A receptor is not dependent on F-actin

GABA_A receptors, visualized with an antibody against the $beta$ 2/3 subunits, cluster on dendrite shafts specifically opposite GABAergicterminals in hippocampal cultures (Craig et al., 1994). GABAergicsynapses lack immunoreactivity for PSD-95 and $alpha$ -actinin-2 butinstead contain concentrations of gephyrin, the putative glycinereceptor-anchoring protein (Craig et al., 1996; Rao et al., 1998).Here we tested the dependence of synaptic GABA_A receptor clusterson F-actin by comparing the distribution of the receptor in controlversus latrunculin A-treated hippocampal cultures (Fig. 10). Incontrol neurons, the GABA_A receptor was present in a typical patternof thin elongated clusters that colocalize with synaptophysin.Qualitatively there were no apparent differences between controland latrunculin A-treated neurons for GABA_A receptor staining(compare Fig. 10A-D with E-H). Most neurons had prominent synapticclusters of the GABA_A receptor with the typical elongated morphology,regardless of the degree of actin polymerization.

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Figure 10. GABA_A receptors do not depend on F-actin for clustering or synaptic localization. Control neurons (A-D) or latrunculin A-treatedneurons (E-H) were immunolabeled for the GABA_A receptor $beta$ 2/3 subunits(A, C, E, G) and the synaptic marker SV2 (B, D, F, H). The GABA_Areceptor distribution appeared to be unaffected by actin depolymerization.Typical elongated GABA_A receptor clusters were present on shaftsof both control and latrunculin A-treated neurons, and these wereopposite synaptic terminals (arrows). Scale bars, 10 µm.

NMDA receptors are detergent insoluble whereas AMPA receptors are readily extractable from pyramidal neurons

As reported above, F-actin depolymerization affects both AMPA and NMDA receptors in different ways and depending on the celltype. To assess the cytoskeletal attachment of receptors, we treatedliving neurons with the nonionic detergent Triton X-100 to extractthe plasma membrane and freely floating receptors, leaving cytoskeletal-boundreceptors and the PSD associated with the detergent-insolublefraction (Cotman et al., 1974; Cohen et al., 1977; Kennedy, 1997).Similar studies have been done to demonstrate cytoskeletal attachmentof acetylcholine receptors at spontaneous clusters in culturedmuscle cells by resistance to Triton X-100 extraction (Priveset al., 1982).

We used Western blot analysis to determine the relative amounts of nonextractable actin and receptors from control versuslatrunculin A-treated hippocampal cultures (Fig. 11). As expectedwithout extraction, the level of actin remained relatively constantin the control and latrunculin A-treated groups (Fig. 11E). Incontrol cultures, ~50% of the actin was detergent extractable,consistent with reports that the monomeric actin pool makes up~50% of the total actin in most cells (Bray and Thomas, 1976).After actin depolymerization with latrunculin A, almost all ofthe actin became extractable with Triton X-100 (Fig. 11E, lane4). This result confirms the action of latrunculin A in shiftingthe pool of filamentous, nonextractable actin to the pool of monomeric,detergent-extractable actin in the neurons. The levels of theactin binding protein $alpha$ -actinin-2 varied in parallel with thatof actin (Fig. 11F), supporting the conclusion from the immunofluorescencestaining that the cytoskeletal association of $alpha$ -actinin-2 is completelydependent on F-actin.

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Figure 11. Detergent extraction to assess cytoskeletal anchoring of glutamate receptors. A, B, GluR1 staining of pyramidal neurons fromthe same culture taken at the same exposure either unextracted(A) or after extraction with Triton X-100 (B) is shown. Detergentextraction induced an obvious decrease in the amount of GluR1immunoreactivity and a change in the distribution pattern includinga complete loss of GluR1 immunoreactivity from dendritic spines.C, In contrast, detergent-extracted GABAergic neurons retainedGluR1 clusters with a typical distribution pattern; these clusterswere presumably at synaptic sites, although we were unable toconfirm this directly because the synaptic markers SV2 and synaptophysinwere extracted by Triton X-100 (data not shown). D, After TritonX-100 extraction, NR1 immunoreactivity on pyramidal neurons wasalso indistinguishable from that of unextracted neurons. Scalebar: A-D, 10 µm. E-H, Western blot analyses of unextracted controlneurons (lane 1), control neurons extracted with 1% Triton X-100(lane 2), latrunculin A-treated unextracted neurons (lane 3),and latrunculin A-treated, Triton X-100-extracted neurons (lane4) are shown. Protein loading was normalized to cell number suchthat lanes 2 and 4 contain protein derived from twice as manyneurons as lanes 1 and 3. These blots were probed with antibodiesagainst actin (E), $alpha$ -actinin-2 (F), GluR1 (G), and NR1 (H). Verylittle actin remained in the latrunculin A-treated, extractedneurons (E, lane 4), indicating that most of the F-actin was depolymerizedby latrunculin A and therefore extractable. $alpha$ -Actinin-2 was alsonearly completely extractable after latrunculin A treatment (F);although it can also bind NMDA receptors, it apparently is highlydependent on F-actin for cytoskeletal attachment. Surprisingly,GluR1 was partially (~75%) extractable with or without F-actinpresent (evident by the decreased signal in lanes 2 and 4 of Grelative to lanes 1 and 3, despite the twofold greater loadingof lanes 2 and 4). This result is consistent with the loss ofGluR1 immunoreactivity from pyramidal neurons after extraction(B). NR1 (H), on the other hand, did not seem to be detergentextractable even with latrunculin A treatment (because the relativesignal intensities correspond to the loading differences).

We next examined the effects of Triton X-100 extraction on the receptors GluR1 and NR1. Approximately 75% of the GluR1 wasdetergent extractable in the control cells; this proportion wasnot affected by the disruption of F-actin (Fig. 11G). Stainingof these extracted neurons indicated that GluR1 immunoreactivitywas greatly reduced on the pyramidal neurons (Fig. 11B). Althoughthere was still some faint staining in the cell body, the typicalsynaptic clusters on spines were extracted. However, the stainingfor the GluR1 receptor on the GABAergic neurons appeared unchangedafter Triton X-100 extraction (Fig. 11C). This implies that thereis more than one mechanism responsible for the localization ofAMPA receptors, one resistant to Triton X-100 on GABA cells andanother mechanism disrupted by Triton X-100 on pyramidal neurons.

In contrast to GluR1, NR1 was virtually unextractable, even with the disruption of F-actin (Fig. 11H). An extracted neuronstained for NR1 is shown in Figure 11D, with its typical synapticclusters still present. The large spherical nonsynaptic NR1 clustersalso appeared resistant to Triton X-100 extraction. The postsynapticdensity is a highly insoluble structure, and these results indicatethat the integrity of at least some components of this structureis not dependent on F-actin. The NR1 binding protein $alpha$ -actinin-2was extracted after latrunculin treatment, whereas PSD-95, likeNR1, was primarily not extractable in the presence or absenceof F-actin (data not shown).

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

From this study, several conclusions can be drawn about the relationship between postsynaptic proteins and their link to theneuronal cytoskeleton. (1) F-actin within dendritic spines isless dynamic than is the rest of the cellular actin. (2) AMPAreceptors are readily detergent extractable from spines. Afteractin depolymerization, GluR1-labeled spines are reduced in number,and the remaining GluR1 clusters appear on collapsed spine-likestructures lacking F-actin but still localizing to synaptic sites.(3) Synaptic AMPA receptors are anchored differently on GABA celldendrite shafts, being resistant to detergent extraction and dependenton F-actin for their synaptic localization but not for the existenceof clusters. (4) NMDA receptor clusters are also resistant todetergent extraction and partially depend on F-actin for theirsynaptic localization but not for the maintenance of clusters.(5) The NMDA receptor-interacting proteins PSD-95 and $alpha$ -actinin-2behave differently after actin depolymerization. PSD-95 redistributeswith the NMDA receptor, whereas $alpha$ -actinin-2 completely dispersesdespite the continued presence of some synaptic NMDA receptorclusters. (6) The localization of inhibitory GABA_A receptors appearsunchanged by actin depolymerization. These findings are summarizedin Figure 12A.

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Figure 12. Diagrammatic summary of results (A) and model (B). A, In control neurons, GluR1 exhibits a cell type-specific synaptic distribution,spiny on pyramidal neurons and clustering on the shafts of GABAergicneurons. NMDAR1 shows both spiny and shaft clusters on the pyramidalneurons; in this case, some of the shaft clusters are nonsynaptic(represented by the lack of a presynaptic terminal). The spinyNR1 clusters are immunopositive for both PSD-95 and $alpha$ -actinin-2,but the shaft NR1 clusters contain only PSD-95. GABA_A receptorsare found as synaptic shaft clusters on pyramidal neurons. Afterlatrunculin A treatment to depolymerize actin, GluR1-labeled spinesare decreased in number with the remaining spines being much smallerand devoid of F-actin. GluR1 shaft clusters on GABAergic neuronsare no longer synaptic. Synaptic NR1 clusters are also decreasedin number after actin depolymerization, and there appear to bemore and/or larger nonsynaptic NR1 clusters. $alpha$ -Actinin-2 becomescompletely diffuse with the loss of F-actin, but PSD-95 remainscoclustered with both synaptic and nonsynaptic NMDA receptors.The inhibitory GABA_A receptor (GABA_AR) is apparently unaffectedby latrunculin A treatment. Detergent extraction leads to a completeloss of GluR1 on the spines of pyramidal neurons but has no affecton GluR1 clusters on the shafts of GABAergic neurons. Both NR1(and its interacting proteins $alpha$ -actinin-2 and PSD-95) and GABA_Areceptors are not readily detergent extractable but remain tightlyanchored at presumptive synaptic sites (synaptophysin is readilyextractable, but the receptor staining patterns remain unchanged).B, The above data lead to a model for distinct mechanisms foranchoring of neurotransmitter receptors to the cytoskeleton, notonly between different receptor types at a single site but alsofor the same receptor within different cell types. Particularlyfor GluR1 clusters on spines, the mechanism is not well understood.Many possibilities exist: a weak, detergent-extractable interaction,a spectrin-based corral, preferential membrane addition, or someother mechanism. The same receptor is anchored in a differentmanner in GABAergic neurons, possibly by the PDZ protein GRIP.The NMDA receptor forms clusters on spines and dendritic shaftsin the presence of PSD-95 whether $alpha$ -actinin-2 is present or not,suggesting a more central role for PSD-95 in anchoring NMDA receptorsand a possible modulatory role for $alpha$ -actinin-2. The GABA_AR, whichcolocalizes with gephyrin, may be anchored to the microtubulecytoskeleton through gephyrin.

Stability of F-actin within dendritic spines

F-actin within the dendritic spines exhibited a markedly increased stability compared with the rest of the neuronal cellularactin network, as revealed by treatment with either cytochalasinD (24 hr) or latrunculin A (2-9 hr). There are several actin bindingproteins present within dendritic spines, including $alpha$ -actinin-2,fodrin, and MAP2 (all of which can cross-link actin filaments)and also $alpha$ -adducin, drebrin, and myosin (Caceres et al., 1983;Carlin et al., 1983; Morales and Fifkova, 1989; Seidel et al.,1995; Hayashi et al., 1996; Wyszynski et al., 1997). All of theseproteins and probably more may be involved in the maintenanceof the actin cytoskeleton within the dendritic spine. The effectof actin depolymerization on spine structure, shown here by theapparent loss of both GluR1- and NR1-labeled spines (Figs. 2,5, 7, 8) and the presence of GluR1-labeled protrusions that appearto be collapsed spine-like structures, supports a central rolefor F-actin in maintaining spine shape. The selective stabilityof F-actin in spines also suggests that the regulation of spineshape is functionally important to the neuron and that this regulationis accomplished independently of the regulation of F-actin inthe bulk of the neuron. Given the specificity and reversibilityof its effects (Fig. 4), latrunculin A may prove to be a usefuland powerful tool in further studying dendritic spine function.

Relationship between F-actin and AMPA glutamate receptors

The Triton X-100 extraction of AMPA receptors from pyramidal cell spines reported here indicates that AMPA receptors are notcore components of the PSD but are less tightly linked to cytoskeletalstructures at postsynaptic sites. The PSD consists of synaptosomalcomponents that are insoluble in Triton X-100, with a core thatis also insoluble in sarcosinate (Cotman et al., 1974; Cohen etal., 1977; Kennedy, 1997). Biochemical preparations indicate thatthe PSD is enriched in actin, fodrin, dystrophin, $alpha$ -actinin-2,PSD-95/SAP90, GKAP/SAPAP, densin 180, CaM kinase II, NMDA receptors,and GABA_A receptors (for review, see Kennedy, 1997; also Matuset al., 1981; Kim et al., 1992, 1997; Takeuchi et al., 1997; Wyszynskiet al., 1997). Mirroring our results found in culture, whereasNMDA receptors and PSD-95 family members are not extracted byTriton from rat brain synaptosomes (Muller et al., 1996), AMPAreceptors are efficiently (75-85%) extracted by Triton from adultrat hippocampal tissue homogenates (Wenthold et al., 1996).

If GluR1 is not tightly anchored to the cytoskeleton at spines, then how can it become clustered there, which it apparentlydoes both in vivo and in cultured neurons (Petralia and Wenthold,1992; Craig et al., 1993)? The results with latrunculin A indicatethat both the existence of GluR1 clusters and their synaptic localizationare partially dependent on F-actin. One possibility is that thereis a direct protein-mediated link between AMPA receptors and theactin cytoskeleton but that the interactions are disrupted byTriton X-100. Alternatively, AMPA receptors may not be anchoredper se but rather localized by selective membrane addition and/ormembrane corrals. The cytoskeletal structure of PSDs at spinesconsists of a lattice of 3-5 nm filaments that could provide sucha fence or corral (Blomberg et al., 1977; Matus and Taff-Jones,1978; Landis et al., 1987), similar to the proposed spectrin-basedcorrals of erythrocytes (Bennett and Gilligan, 1993). In supportof these ideas, GluR1 clusters on spines are not as "tightly clustered,"i.e., the clusters never appear as brightly labeled above thediffuse labeling on the dendrite shafts as do NR1 clusters onspines or GluR1 clusters on the shafts of the GABA cells, at leastin primary cultured neurons. If this model is correct, one ofthe functions of spines may be to sequester AMPA receptors. Futuretests of this model, such as direct measurements of the mobilityof receptors within the membrane (e.g., Sheetz et al., 1980),will be required.

In contrast to AMPA receptors on pyramidal cells, AMPA receptors on GABAergic neurons behaved more as expected for proteinsanchored to the subsynaptic cytoskeleton. GluR1 on GABAergic neuronswas not extractable by Triton X-100 and was not dependent on F-actinfor the maintenance of clusters but was dependent on F-actin forthe synaptic localization of those clusters. These results areconsistent with a model whereby AMPA receptors bind to an interactingprotein such as GRIP (Dong et al., 1997) that clusters and attachesthem, directly or indirectly, to F-actin.

Relationship between F-actin and NMDA receptors

NMDA receptors on pyramidal neurons behaved as expected for proteins anchored to the subsynaptic cytoskeleton by a linkerprotein or series of linker proteins. NMDA receptors remainedclustered after actin depolymerization, implying the presenceof a cross-linking protein. However, in the absence of F-actin,many of the NR1 clusters appeared to be released from postsynapticsites and coalesced into large nonsynaptic cell body clusters,similar to those seen during early development of these cultures(Rao et al., 1998). Latrunculin A induced a 40% loss of synapticNMDA receptor clusters, the same percentage loss found for GluR1-labeledspines [ although there are differences in the numbers of NMDAvs AMPA receptor clusters in these cultures (Figs. 5 vs 8; discussedby Rao and Craig, 1997)]. The nonsynaptic clusters as well asthe synaptic NR1 clusters were resistant to Triton X-100 extraction,indicating some form of anchoring to the cytoskeleton.

Both synaptic and nonsynaptic NMDA receptor clusters, in the presence or absence of F-actin, were associated with PSD-95.PSD-95 by virtue of its multiple PDZ domains and ability to multimerizeby N-terminal disulfide linkages (Hsueh et al., 1997) may thusbe a core scaffolding molecule for the attachment of NMDA receptorsat both synaptic and nonsynaptic sites. The redistribution ofNR1 and PSD-95 with latrunculin A treatment observed here suggeststhat PSD-95 and associated NMDA receptors are linked, directlyor indirectly, to the actin-based cytoskeleton. However, somesynaptic PSD-95 and NMDA receptor clusters did remain in the absenceof detectable F-actin. It may be that a highly cross-linked aggregatecontaining NMDA receptors, PSD-95 family members, associated proteinssuch as GKAP/SAPAP, nNOS, and neuroligin (Brenman et al., 1996;Irie et al., 1997; Kim et al., 1997; Takeuchi et al., 1997), andpossibly other PSD proteins is sufficient to maintain a partialcomplement of postsynaptic components in the absence of F-actin.Using latrunculin A, we have been able to dissociate $alpha$ -actinin-2from NMDA receptor clusters, indicating that $alpha$ -actinin-2 is notnecessary for clustering or for synaptic localization of NMDAreceptors in pyramidal neurons. It seems likely that $alpha$ -actinin-2,competitively with calmodulin (Ehlers et al., 1996; Wyszynskiet al., 1997), plays more of a modulatory role in regulating NMDAreceptor function and perhaps localization in spines.

General mechanisms for anchoring postsynaptic receptors

A parallel can be drawn between this study and earlier studies of postsynaptic structure at the vertebrate neuromuscular junction.In this system, the acetylcholine receptor is anchored in thepostsynaptic muscle membrane by attachment to the actin-basedcytoskeleton. Extraction with Triton X-100 leaves spontaneousacetylcholine receptor clusters bound to the cytoskeleton (Priveset al., 1982), and treatment with cytochalasin D causes the receptorto disperse in small microclusters throughout the membrane (Connolly,1984). The molecules linking the receptor to F-actin are thoughtto include 43K/rapsyn with possibly some contribution from utrophin,dystrophin, and/or dystrobrevin (Carbonetto and Lindenbaum, 1995;Sanes, 1997).

The main conclusion of this study is that a single model cannot account for the diversity of results regarding receptor anchoringat postsynaptic sites on neurons (Fig. 12). For example, our resultsindicate different mechanisms underlying the localization of asingle receptor (the AMPA receptor) in pyramidal cells versusGABAergic interneurons and different mechanisms underlying thelocalization of different receptors (AMPA- vs NMDA-type glutamatereceptors) at a single class of postsynaptic sites on pyramidalcell dendritic spines. These differences in mechanisms may reflectdifferent sets of anchoring proteins linking the different receptortypes to the cytoskeleton, consistent with the proposed rolesfor gephyrin (for GABA_A receptors), the PSD-95 family (for NMDAreceptors), and GRIP (for some AMPA receptors). Many of the glutamatereceptors may bind more than one protein for anchoring to differentcomponents of the cytoskeleton and/or may use more than one modeof localization. AMPA receptor clusters on GABA cell dendriteshafts depended on F-actin for their synaptic anchoring but notfor the presence of clusters, implying the existence of a linkerprotein such as GRIP (Dong et al., 1997). Surprisingly, AMPA receptorclusters on dendritic spines were not tightly anchored and thusmay not require such a linker protein but may be localized byother mechanisms such as selective membrane insertion and/or membranecorrals. Future studies of the dynamics of AMPA and NMDA receptormembrane insertion and mobility will be required to test theseproposed mechanisms.

  FOOTNOTES

Received Sept. 25, 1997; revised Jan. 16, 1998; accepted Jan. 21, 1998.

This work was supported by the Markey Charitable Trust, by National Institutes of Health Grants NS33184 to A.M.C. and GM52111-01to V.I.G., and by National Science Foundation Grant MCB 95-31231to V.I.G. We thank Anna S. Serpinskaya for excellent technicalassistance and J. Campanelli, A. Rao, and S. Rogers for commentson this manuscript.
Correspondence should be addressed to Dr. Ann Marie Craig, Department of Cell and Structural Biology, University of Illinois,B107 CLSL, 601 South Goodwin Avenue, Urbana, IL 61801.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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M. J. Hasbani, M. L. Schlief, D. A. Fisher, and M. P. Goldberg
Dendritic Spines Lost during Glutamate Receptor Activation Reemerge at Original Sites of Synaptic Contact
J. Neurosci., April 1, 2001; 21(7): 2393 - 2403.
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Q. Zhou, M.-Y. Xiao, and R. A. Nicoll
Contribution of cytoskeleton to the internalization of AMPA receptors
PNAS, January 23, 2001; (2001) 31573798.
[Abstract] [Full Text]

A. Burette, L. Khatri, M. Wyszynski, M. Sheng, E. B. Ziff, and R. J. Weinberg
Differential Cellular and Subcellular Localization of AMPA Receptor-Binding Protein and Glutamate Receptor-Interacting Protein
J. Neurosci., January 15, 2001; 21(2): 495 - 503.
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J. L. Bruses, N. Chauvet, and U. Rutishauser
Membrane Lipid Rafts Are Necessary for the Maintenance of the {alpha}7 Nicotinic Acetylcholine Receptor in Somatic Spines of Ciliary Neurons
J. Neurosci., January 15, 2001; 21(2): 504 - 512.
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L. Shen, F. Liang, L. D. Walensky, and R. L. Huganir
Regulation of AMPA Receptor GluR1 Subunit Surface Expression by a 4.1N-Linked Actin Cytoskeletal Association
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A. Matus
Actin-Based Plasticity in Dendritic Spines
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[Abstract] [Full Text]

Z. Dai, X. Luo, H. Xie, and H. B. Peng
The Actin-Driven Movement and Formation of Acetylcholine Receptor Clusters
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D. K. Meyer, C. Olenik, F. Hofmann, H. Barth, J. Leemhuis, I. Brunig, K. Aktories, and W. Norenberg
Regulation of Somatodendritic GABAA Receptor Channels in Rat Hippocampal Neurons: Evidence for a Role of the Small GTPase Rac1
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M. A. Torres and W. J. Nelson
Colocalization and Redistribution of Dishevelled and Actin during Wnt-induced Mesenchymal Morphogenesis
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D. W. Allison, A. S. Chervin, V. I. Gelfand, and A. M. Craig
Postsynaptic Scaffolds of Excitatory and Inhibitory Synapses in Hippocampal Neurons: Maintenance of Core Components Independent of Actin Filaments and Microtubules
J. Neurosci., June 15, 2000; 20(12): 4545 - 4554.
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R. D. Shoop, N. Yamada, and D. K. Berg
Cytoskeletal Links of Neuronal Acetylcholine Receptors Containing alpha 7 Subunits
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C. Racca, F. A. Stephenson, P. Streit, J. D. B. Roberts, and P. Somogyi
NMDA Receptor Content of Synapses in Stratum Radiatum of the Hippocampal CA1 Area
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S. N. Gomperts, R. Carroll, R. C. Malenka, and R. A. Nicoll
Distinct Roles for Ionotropic and Metabotropic Glutamate Receptors in the Maturation of Excitatory Synapses
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P. Penzes, R. C. Johnson, M. R. Alam, V. Kambampati, R. E. Mains, and B. A. Eipper
An Isoform of Kalirin, a Brain-specific GDP/GTP Exchange Factor, Is Enriched in the Postsynaptic Density Fraction
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A. F. Ernst, G. Gallo, P. C. Letourneau, and S. C. McLoon
Stabilization of Growing Retinal Axons by the Combined Signaling of Nitric Oxide and Brain-Derived Neurotrophic Factor
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R. Sattler, Z. Xiong, W.-Y. Lu, J. F. MacDonald, and M. Tymianski
Distinct Roles of Synaptic and Extrasynaptic NMDA Receptors in Excitotoxicity
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Q.-s. Liu and D. K. Berg
Actin Filaments and the Opposing Actions of CaM Kinase II and Calcineurin in Regulating alpha 7-Containing Nicotinic Receptors on Chick Ciliary Ganglion Neurons
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A. Dunaevsky, A. Tashiro, A. Majewska, C. Mason, and R. Yuste
Developmental regulation of spine motility in the mammalian central nervous system
PNAS, November 9, 1999; 96(23): 13438 - 13443.
[Abstract] [Full Text] [PDF]

R. Gerlai, N. Shinsky, A. Shih, P. Williams, J. Winer, M. Armanini, B. Cairns, J. Winslow, W.-Q. Gao, and H. S. Phillips
Regulation of Learning by EphA Receptors: a Protein Targeting Study
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Y. Shiraishi, A. Mizutani, H. Bito, K. Fujisawa, S. Narumiya, K. Mikoshiba, and T. Furuichi
Cupidin, an Isoform of Homer/Vesl, Interacts with the Actin Cytoskeleton and Activated Rho Family Small GTPases and Is Expressed in Developing Mouse Cerebellar Granule Cells
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L. D. Walensky, S. Blackshaw, D. Liao, C. C. Watkins, H.-U. G. Weier, M. Parra, R. L. Huganir, J. G. Conboy, N. Mohandas, and S. H. Snyder
A Novel Neuron-Enriched Homolog of the Erythrocyte Membrane Cytoskeletal Protein 4.1
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M. Wyszynski, J. G. Valtschanoff, S. Naisbitt, A. W. Dunah, E. Kim, D. G. Standaert, R. Weinberg, and M. Sheng
Association of AMPA Receptors with a Subset of Glutamate Receptor-Interacting Protein In Vivo
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C.-H. Kim and J. E. Lisman
A Role of Actin Filament in Synaptic Transmission and Long-Term Potentiation
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K. Hayashi and T. Shirao
Change in the Shape of Dendritic Spines Caused by Overexpression of Drebrin in Cultured Cortical Neurons
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R. Dingledine, K. Borges, D. Bowie, and S. F. Traynelis
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[Abstract] [Full Text] [PDF]

D. V. Lissin, R. C. Carroll, R. A. Nicoll, R. C. Malenka, and M. v. Zastrow
Rapid, Activation-Induced Redistribution of Ionotropic Glutamate Receptors in Cultured Hippocampal Neurons
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T. Furuyashiki, K. Fujisawa, A. Fujita, P. Madaule, S. Uchino, M. Mishina, H. Bito, and S. Narumiya
Citron, a Rho-Target, Interacts with PSD-95/SAP-90 at Glutamatergic Synapses in the Thalamus
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[Abstract] [Full Text] [PDF]

S. Halpain, A. Hipolito, and L. Saffer
Regulation of F-Actin Stability in Dendritic Spines by Glutamate Receptors and Calcineurin
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C. M. Hurt, F. Y. Feng, and B. Kobilka
Cell-type Specific Targeting of the alpha 2c-Adrenoceptor. EVIDENCE FOR THE ORGANIZATION OF RECEPTOR MICRODOMAINS DURING NEURONAL DIFFERENTIATION OF PC12 CELLS
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