Activation of Silent Synapses by Rapid Activity-Dependent Synaptic Recruitment of AMPA Receptors

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The Journal of Neuroscience, August 15, 2001, 21(16):6008-6017

Activation of Silent Synapses by Rapid Activity-Dependent Synaptic Recruitment of AMPA Receptors
Dezhi Liao, Robert H. Scannevin, and Richard Huganir
Department of Neuroscience, Howard Hughes Medical Institute, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Many recent studies have shown that excitatory synapses can contain NMDA receptor responses in the absence of functional AMPAreceptors and are therefore postsynaptically silent at restingmembrane potentials. The activation of silent synapses via therapid acquisition of AMPA receptor responses may be importantin synaptic plasticity and neuronal development. Our recent immunocytochemicalstudies that used cultured hippocampal neurons have provided evidencefor "morphological silent synapses" that physically contain NMDAreceptors but no AMPA receptors. Here we show that the activationof NMDA receptors by spontaneous synaptic activity results inthe rapid recruitment of AMPA receptors into these morphologicalsilent synapses within minutes. In parallel, we find a significantincrease in the frequency of AMPA receptor-mediated miniatureEPSCs (mEPSCs). NMDA receptor activation also results in a mobilizationof calcium/calmodulin (CaM) kinase II to synapses and an increasein the phosphorylation of surface AMPA receptors on the majorCaM kinase II phosphorylation site. These results demonstratethat AMPA receptors can be modified and recruited rapidly to silentsynapses via the activation of NMDA receptors by spontaneous synapticactivity.

Key words: long-term potentiation; long-term depression; synaptic plasticity; GluR1; calcium/calmodulin-dependent protein kinase II; mEPSC

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the CNS the majority of excitatory synaptic transmission occurs at glutamatergic synapses and is mediated via the AMPA-,NMDA-, and kainate-type glutamate receptors (Hollmann and Heinemann,1994). Models of synaptic plasticity, such as long-term potentiation(LTP) and long-term depression (LTD) of glutamatergic synapses,are believed to underlie the cellular basis of learning and memoryin the adult brain and the activity-dependent regulation of synapseformation in developing brain (Bliss and Collingridge, 1993; Malenka,1994; Katz and Shatz, 1996). The molecular mechanism of such synapticplasticity, however, is not known. Current evidence suggests thatactivity-dependent changes in synaptic strength, such as LTP andLTD, result at least in part from changes in AMPA receptor-mediatedresponses (Kauer et al., 1988; Muller et al., 1988; Davies etal., 1989; Liao et al., 1992). These changes may be attributableto altered levels of AMPA receptors in the postsynaptic membrane,altered receptor properties, or a combination of these twomechanisms.

It has been reported previously that AMPA receptors are phosphorylated and dephosphorylated during LTP and LTD, respectively,and that this may lead to changes in the ion channel conductanceor open channel probability of AMPA receptors during these processes(Barria et al., 1997a; Benke et al., 1998; Lee et al., 1998, 2000;Derkach et al., 1999; Banke et al., 2000). Numerous recent studiessuggest that the level of synaptic AMPA receptors also can bemodulated by activity-dependent mechanisms (Kim and Huganir, 1999;Turrigiano, 2000). Both electrophysiological and morphologicalstudies have indicated that a significant fraction of glutamatergicsynapses contains NMDA receptors without detectable AMPA receptors(Isaac et al., 1995; Liao et al., 1995, 1999; Durand et al., 1996;Nusser et al., 1998; Petralia et al., 1999). Such synapses wouldbe postsynaptically silent under normal resting potentials becauseof the voltage-dependent blockade of NMDA receptors by magnesium(Mayer et al., 1984; Nowak et al., 1984). Whole-cell recordingsin brain slices demonstrate that such silent synapses can be activatedvia the acquisition of AMPA receptor-mediated responses afteran LTP-inducing protocol that lasts only minutes (Isaac et al.,1995; Liao et al., 1995). The cellular mechanism underlying thisrapid acquisition of AMPA receptor responses in silent synapsesis notclear.

Several groups have reported that the chronic blockade of synaptic activity with CNQX or TTX for hours or days can cause aslow modulation in the amount of postsynaptic AMPA receptors inneuronal cultures (O'Brien et al., 1998; Turrigiano et al., 1998).It also has been reported that synaptic AMPA receptors in hippocampalcultures can be dispersed or internalized rapidly after a briefapplication of glutamate or an electrical LTD induction protocol(Lissin et al., 1998, 1999; Carroll et al., 1999). Moreover, ithas been reported recently that recombinant green fluorescentprotein-tagged (GFP-tagged) GluR1 subunits can be mobilized rapidlyto dendritic spines within minutes after a burst of high-frequencystimuli in cultured hippocampal slices (Shi et al., 1999; Hayashiet al., 2000). However, there is no direct morphological evidencethat activity can regulate rapidly the recruitment of native AMPAreceptors into silentsynapses.

In this paper we have analyzed the rapid NMDA receptor- and activity-dependent modulation of synaptic AMPA receptors in bothlow-density hippocampal cultures and high-density cortical cultures.These cultured neurons have a large number of morphological silentsynapses that contain clustered NMDA receptors but no detectableclustered AMPA receptors. Combining immunocytochemical and electrophysiologicaltechniques, we demonstrate that these silent synapses rapidlybecome responsive to synaptically released glutamate via the recruitmentof AMPA receptors after the activation of NMDAreceptors.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuronal cultures. Low-density hippocampal cultures from 18-d-old embryonic rats were prepared as reported previously (Bankerand Cowan, 1977). Neurons were plated onto 60 mm Petri dishes(Becton Dickinson, Bedford, MA) at a density of 120,000-200,000cells per dish. Some dishes contained five coverslips per dishat a density of 1 × 10⁶ cells per dish. In some cultures, D,L-aminophosphonovalerate(D,L-APV; 200 µM) was added to the culture medium to chronicallyblock NMDA receptors at 5 d afterplating.

High-density cortical cultures from 17- or 18-d-old embryonic rats were prepared as reported previously (Ghosh and Greenberg,1995). Neurons were plated onto 60 mm Petri dishes (Becton Dickinson),with some dishes containing five coverslips per dish at a densityof 6 × 10⁶ cells per dish. Dishes that were used for biochemical experimentscontained no coverslip. D,L-APV (200 µM) was added into the culturemedium at 4 d after plating, and the same concentration of D,L-APVwas maintained until usage. Thereafter, the cortical neurons werefed twice per week with feeding medium that had been incubatedwith glial cellsovernight.

Induction protocol for synaptic targeting of AMPA receptors. High-density cortical neurons chronically treated with 200 µMD,L-APV were incubated in artificial CSF [aCSF; containing (inmM) 125 NaCl, 2.5 KCl, 26.2 NaHCO₃, 1 NaH₂PO₄, 11 glucose, 2.5CaCl₂, and 1.25 MgCl₂ at 37°C plus 5% CO₂] in a tissue culturechamber for ~15-20 min. Although sometimes an increase in thenumber of AMPA receptor clusters was observed after the withdrawalof D,L-APV for 5 min (data not shown), a more consistent changeoften was induced by a treatment for ~15 min. In control experiments,200 µM D,L-APV was added to aCSF to block the NMDAreceptors.

Withdrawal of D,L-APV alone in low-density hippocampal cultures was unable to induce a rapid mobilization of AMPA receptors.Most likely the low-density cultures lack the high levels of spontaneousactivity that are necessary to provide both sufficient postsynapticdepolarization and released glutamate for the activation of NMDAreceptors. In another protocol to induce synaptic targeting ofAMPA receptors, we added glycine to aCSF to enhance the NMDA receptorchannel opening and removed Mg²⁺ to allow for the activation of NMDA receptors at hyperpolarizingpotentials. Cultured neurons were incubated in aCSF containing2.5 mM Ca²⁺, 100 µM glycine, and no added Mg²⁺ in a tissue culture chamber for ~15-20 min. This protocol caninduce a rapid mobilization of AMPA receptors in low-density hippocampalcultures growing in culture medium either with or without D,L-APV.

Immunocytochemistry. As described previously (Liao et al., 1999), cultured neurons were fixed successively with 4% paraformaldehyde,4% sucrose in PBS (4°C, 20 min), and then with $-$ 20°C, 100% methanol(incubated at 4°C, ~10-15 min); next the neurons were permeabilizedwith 0.2% Triton X-100 (4°C, ~10-15 min). Coverslips with neuronswere blocked in 10% donkey serum in PBS for ~30-60 min and thenincubated with primary antibodies dissolved in 10% donkey serumin PBS. All primary rabbit polyclonal antibodies were affinity-purifiedand conjugated either to Cy3 (red; Amersham Pharmacia Biotech,Arlington Heights, IL) or to Fluorescein-Ex (green; MolecularProbes, Eugene, OR). Mouse monoclonal primary antibodies werevisualized with anti-mouse IgG antibodies linked to fluoresceinisothiocyanate (FITC; green), rhodamine (red), or AMCA (blue;Jackson ImmunoResearch Laboratories, West Grove,PA).

Two rabbit polyclonal antibodies against the C terminus of the GluR1 subunit and the GluR 2/3 subunit, respectively, wereused to detect AMPA receptor subunits. In most of the presenteddata the GluR1 and GluR2/3 antibodies were added together to detectAMPA receptors. A rabbit polyclonal antibody against the N terminusof the NMDA receptor 1 (NR1) subunit was used to detect this obligatorysubunit of functional NMDA receptors. A mouse monoclonal antibody(MAB3119, Chemicon, Temecula, CA) was used to detect the $alpha$ -isoformof calcium/calmodulin (CaM) kinase II (Erondu and Kennedy, 1985).

The visual field was moved blindly to a random site on a coverslip. In coverslips that were double-stained with antibodiesagainst NR1 and AMPA receptor subunits, we first found and focusedon a pyramidal neuron under the fluorescent channel that detectedthe NR1 staining. Thereafter, images of both NR1 subunits andAMPA receptor subunits were sampled by a digital camera (PrincetonInstruments, Trenton, NJ) and analyzed with the MetaMorph ImagingSystem (Universal Imaging, West Chester, PA). In coverslips thatwere double-stained with synaptophysin and another antibody, thestaining of synaptophysin was used for searching and focusing.Both NMDA and AMPA receptor clusters were significantly brighterthan their surrounding areas. Almost all of them were marked asregions of interest by the computer when we set a threshold offluorescent intensity that was slightly higher than the distantdendritic shafts but lower than cell body and proximal dendriticshafts. We included only those regions with an area >5 pixelsand <500 pixels. The upper threshold limit for this selectionwas used to exclude the cell body and proximal dendritic shafts,which have much larger area than spines. We used a 100× objectiveto acquire our images (1 µm = 15 pixels; 1 µm² = 225 pixels). Most of the clusters were <1 µm² because the peripheral area of the selected cluster was not included.All regions of interest marked by the computer were compared withclusters that had been identified visually by the experimenter.Poor images without sharp NMDA receptor clusters and AMPA receptorclusters were discarded. Synaptophysin and CaM kinase II clustersare not sharp enough to be counted with this method. In the high-densityneuronal cultures we were not able to trace dendrites and to normalizethe number of receptor clusters to dendritic length. However,we have found that the density of synapses is similar betweencoverslips in sister cultures and is distributed randomly on thecoverslip, allowing us to analyze the number of clusters per fieldand reliably compare the number of receptor clusters between culturedishes. In low-density hippocampal cultures the number of receptorclusters was normalized with the dendritic length after all ofthe dendritic branches in an image were traced and measuredmanually.

Immunoblotting and biotinylation of surface proteins. Cortical neurons were grown as described in the presence of D,L-APVfor 3-4 weeks and were subjected to the described induction protocol.After induction all of the dishes were cooled on ice and washedtwo times with ice-cold aCSF. Cultures then were incubated withaCSF containing 1 mg/ml sulfo-NHS-LC-biotin (Pierce Chemical,Rockford, IL) for 20 min on ice. Unreacted biotinylation reagentwas quenched by three successive 5 min washes in ice-cold TBS(50 mM Tris pH 7.5, 150 mM NaCl). Cultures were lysed in modifiedRIPA buffer [1% Triton X-100, 0.1% SDS, 0.5% deoxycholic acidand (in mM) 10 NaPO₄, 150 NaCl, 2 EDTA, 50 NaF, 10 sodium pyrophosphate,10 iodoacetamide, 1 sodium orthovanadate, and 1 phenylmethylsulfonylfluoride plus (in µg/ml) 2 aprotinin, 1 leupeptin, 2 antipain,and 10 benzamide] on ice and then harvested with a cell scraper.Crude lysates were cleared by centrifugation at 14,000 × g for15 min at 4°C. A portion of the supernatant was added to SDS samplebuffer for use as the total input for each sample. The remainingsupernatant was diluted to a final volume of 1 ml in RIPA buffer.Then 100 µl of 50% NeutrAvidin agarose (Pierce Chemical) was added,and the samples were rotated for 3 hr at 4°C. Next the NeutrAvidinagarose was washed five times with RIPA buffer, and the boundproteins were eluted into SDS sample buffer by boiling for 15min. Total protein and isolated biotinylated proteins were fractionatedby SDS-PAGE and electroblotted onto Immobilon-P membrane (Millipore,Bedford, MA). Membranes were immunoblotted with affinity-purifiedantibodies against either GluR1 AMPA receptor subunits or thephosphorylation site-specific antibody against phosphorylatedS831 of the GluR1 subunit (Roche et al., 1996; Mammen et al.,1997). All immunoblots were visualized by ECL development (AmershamPharmacia Biotech) and quantified on a Storm Imaging System (MolecularDynamics, Sunnyvale, CA). Surface expression was determined bycalculating the ratio of the cell surface signal (signal fromNeutrAvidin pull-down lane/percentage of total pull-down loadedon gel) and dividing this by the total input (signal in totalinput lane/percentage of total input loaded on gel) for each sample.For all experiments the input and pull-down samples were loadedon the same gels to minimize variability in different immunoblots.Loading controls were performed in all experiments to verify thelinearity of quantified signals. Reported data represent the mean± SE for the given number of dishes each for control and experimentalgroups harvested from four different dates of culturepreparation.

Detection of phosphorylation of AMPA receptors. A phosphorylation site-specific antibody raised against a synthetic phosphopeptide(phosphorylated on serine 831) corresponding to the C terminusof GluR1 (GluR1-S831-P) has been well characterized previously(Roche et al., 1996; Mammen et al., 1997). This antibody was usedfor quantitative immunoblot analysis of total extract and cellsurface proteins. Then the levels of GluR1-S831-P were comparedwith the respective levels of total GluR1 to determine the relativeamount of the subunit population that wasphosphorylated.

Electrophysiology. Whole-cell voltage-clamp recordings were established in high-density cortical neurons with a holding potentialat $-$ 55 to $-$ 60 mV in aCSF (at 32°C, 95% O₂/5% CO₂) with 200 µMD,L-APV, 1 µM TTX, and 100 µM picrotoxin (a GABA_A blocker). Theinternal solution in the patch electrode contained (in mM) 100cesium gluconate, 40 HEPES, 2 Na-ATP, 0.3 GTP, 5 MgCl₂, 5 glutathione,and 0.2 EGTA, pH-adjusted to 7.2 with CsOH. All recordings werefiltered at 2 kHz. Series and input resistance was checked every5 sec. Experiments with a series resistance >20 M $Omega$ or with a changeof series or input resistance >15% were discarded. There was nosignificant difference in the series resistances recorded at neuronswith or without the withdrawal of D,L-APV (5.9 ± 0.8 vs 5.8 ±0.6 M $Omega$ ; p > 0.05) and also no difference in input resistance (220.5± 75 vs 248.3 ± 25 M $Omega$ ; p > 0.05). The resting potential was slightlymore negative than the holding potential ( $-$ 55 to $-$ 60 mV) becausethe holding current was 0 to +20 pA at the moment when the plasmamembrane was broken through. One recording sweep lasting 200 msecwas sampled for every 1 sec. Detection criteria for miniatureEPSCs (mEPSCs) included peak amplitudes >3 pA and a fast risetime and a slow decay time. A typical recording lasted ~20-30min. The starting point, the peak, and the ending point of a mEPSCwere identified visually. The rise time was measured as the distancebetween the starting point and the peak. The decay time was measuredas the distance between the ending point and the peak. To minimizevariability in the density and maturation of recorded corticalneurons, we performed equal numbers of testing and control experimentsin neurons from the same batch of cultures eachday.

Data analysis. All data are reported as mean ± SE. Sample size n refers to the number of images processed in immunocytochemistry,the number of neurons in whole-cell recordings, and the numberof dishes analyzed in biotinylation experiments. Group t testwas used to test the difference between the control and testinggroups, and ANOVA was used to compare differences among severalgroups; *p < 0.05, **p < 0.01, and ***p < 0.001.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have shown previously that low-density hippocampal cultures contain many "morphological silent synapses," synapses thatcontain NMDA receptors but no AMPA receptors, and that the proportionof these silent synapses can be increased by chronic treatmentwith the NMDA receptor antagonist D,L-APV (Liao et al., 1999).In these previous studies, however, we were unable to obtain rapidactivity-dependent changes in AMPA receptor distribution, possiblybecause of a low level of spontaneous activity in these cultures.To circumvent this problem, we examined AMPA receptor targetingby using high-density cortical neuronal cultures that have muchhigher levels of spontaneous activity (Murphy et al., 1992). Tomaximize the number of silent synapses in the cortical cultures,we maintained them in NMDA receptor antagonists (Liao et al.,1999). Then the distribution of glutamate receptors in the culturedcortical neurons (23-26 DIV) was analyzed with the use of AMPAand NMDA receptor antibodies. The neurons were fixed, permeabilized,and double-labeled with a NMDA receptor NR1 subunit antibody directlycoupled to FITC (green) and with GluR1 and GluR2/3 AMPA receptorsubunit antibodies directly coupled to Cy3 (red). The corticalneurons contained a dense network of neurites with a high densityof NMDA receptor clusters (Fig. 1A,B). In contrast, the neuronshad a diffuse distribution of AMPA receptors in the dendritesand contained few clusters of AMPA receptors (Fig. 1A,B). Therelatively few AMPA receptor clusters colocalized (>95%) withthe NMDA receptor clusters (Fig. 1A,B); however, most of the NMDAreceptor clusters (55.7% ± 3%; n = 20) did not contain colocalizedAMPA receptor clusters. The immunocytochemical labeling of boththe diffuse and clustered receptors was blocked specifically bypreincubation of the antibodies with the appropriate antigen (datanot shown). To examine whether these receptor clusters were synaptic,we double-labeled the neurons with antibodies against NMDA orAMPA receptors and an antibody to the synaptic marker synaptophysin(Fig. 1C-F). Similar to low-density hippocampal cultures (Liaoet al., 1999), >90% of the receptor clusters colocalized with,or juxtaposed to, synaptophysin immunostaining, indicating thatthey are synaptic. These results demonstrate that, as with thelow-density hippocampal cultures, many excitatory synapses inthese high-density cortical cultures are "morphologically silent"and contain clustered NMDA receptors but no colocalized clusteredAMPA receptors.

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Figure 1. Many morphological silent synapses exist in high-density cultured cortical neurons chronically treated with D,L-APV. A, Double staining of high-density cultured cortical neurons by antibodies against AMPA receptor subunits (GluR1/2/3, left) and an NMDA receptor subunit (NR1, right). B, Enlarged images (2×) from A [left, GluR1/2/3; middle, NR1; right, overlay of GluR1+GluR2 (red) and NR1 (green)]. Scale bar: B, D, F, 10 µm. C, Double staining of AMPA receptor subunits (GluR1/2/3, left) and synaptophysin (right). D, Enlarged images (2×) from C [left, GluR1+GluR2; middle, synaptophysin; right, overlay of GluR1+GluR2 (red) and synaptophysin (green)]. E, Double staining of NMDA receptor subunit (NR1, left) and synaptophysin (right). F, Enlarged images (2×) from E [left, NR1; middle, synaptophysin; right, overlay of NR1 (red) and synaptophysin (green)].

Despite the large number of "silent synapses" in these cultures, whole-cell recordings of the cortical neurons showed a robustnetwork activity (data not shown) with bursts of high-frequencyspontaneous synaptic activity (with frequency >100 Hz; duration~5-10 sec). We hypothesized that this activity might be able totrigger rapid NMDA receptor-dependent recruitment of functionalAMPA receptors into silent synapses. To test this idea, we removedthe D,L-APV from the chronically treated cortical neurons andthen fixed the neurons 15-20 min later. Control neurons were maintainedin D,L-APV. The neurons were fixed, permeabilized, and labeledwith both GluR1 and GluR2/3 antibodies to analyze the AMPA receptordistribution. As discussed above, the cultures maintained in thepresence of D,L-APV contained a large number of dendrites thathad a diffuse distribution of AMPA receptors and contained fewsynaptic clusters of AMPA receptors (Fig. 2A, top panels). Thiswas in stark contrast to cultures that had the D,L-APV removed,in which the AMPA receptors had been redistributed rapidly withinthe dendrites, forming clusters (Fig. 2A, bottom panels). In aquantitative analysis we found that the withdrawal of D,L-APVsignificantly increased the number of AMPA receptor clusters by49% (from 622 ± 36 to 926 ± 26 per field; p < 0.001; n1 = 20,n2 = 20; Fig. 2D). No significant change was observed in the numberof NR1 receptor clusters (from 1340 ± 50 to 1261 ± 38 per field;p > 0.05; n1 = 20, n2 = 20; Fig. 2E). Similar to the control,we found that >95% of AMPA receptor clusters were colocalizedwith NR1 clusters after D,L-APV removal (Fig. 2A, bottom panels).We estimated the proportion of silent synapses by analyzing thepercentage of NR1 clusters that were not colocalized with AMPAreceptors. After the withdrawal of D,L-AP the proportion of silentsynapses significantly decreased from 54.1 to 26.2% (p < 0.001;Fig. 2G). Withdrawal of D,L-APV had no significant effect on thefluorescent intensity of either NMDA clusters or AMPA receptorclusters; however, we noticed a significant decrease in the apparentsize of NR1 clusters after the withdrawal of D,L-APV (from 68.9to 57.5 pixels; p < 0.001; 1 µm = 15 pixels, 1 µm² = 225 pixels; Fig. 2G) and a small increase in the apparent sizeof AMPA receptor clusters (from 71 to 75 pixels; p = 0.049; Fig.2F).

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Figure 2. Mobilization of AMPA receptors into silent synapses via the activation of NMDA receptors by spontaneous synaptic activity. A, Double staining of high-density cultured cortical neurons by antibodies against AMPA receptor subunits (left, GluR1/2/3) and an NMDA receptor subunit (middle, NR1) after the neurons were incubated in aCSF in the presence (top panels) and absence (bottom panels) of D,L-APV. Right panels are overlays of the left and middle panels (GluR1/2/3, red; NR1, green). B, Double staining of high-density cultured cortical neurons by antibodies against AMPA receptor subunits (GluR1/2/3, red) and synaptophysin (green) after the withdrawal of D,L-APV. C, Double staining of NR1 (red) and synaptophysin (green) after the withdrawal of D,L-APV. Scale bar: A-C, 10 µm. D, The number of AMPA receptor clusters (GluR1 and GluR2/3) is increased significantly after the withdrawal of D,L-APV (filled bars) compared with control (open bars; neurons incubated in aCSF with D,L-APV). TTX and 0 mM Ca²⁺ blocked this increase. E, Withdrawal of D,L-APV had a negligible effect on the number of NR1 clusters. F, The effect of withdrawal of D,L-APV on the apparent size of AMPA receptor clusters and NR1 clusters. G, The proportion of silent synapses was decreased significantly after the withdrawal of D,L-APV (filled bars) compared with control (open bars). Silent synapses refer to synapses that contain only clustered NR1 receptors but no clustered AMPA receptors (GluR1 and GluR2/3). *p < 0.05; ***p < 0.001.

To test whether these new AMPA receptor clusters were truly synaptic, we double-labeled ~26- to 30-d-old high-density corticalneurons with antibodies against synaptophysin and AMPA receptorsubunits (GluR1 plus GluR2/3) after incubation with or withoutD,L-APV for ~15-20 min. As shown in Figure 2B, almost all of theAMPA receptor clusters were colocalized or adjacent to a synaptophysincluster after the withdrawal of D,L-APV. In another set of experimentsthe cultures were double-stained with an anti-synaptophysin andan anti-NR1 antibody after incubation with or without D,L-APV.Similar to AMPA receptors, >95% of the NR1 clusters were colocalizedor juxtaposed to synaptophysin staining after the withdrawal ofD,L-APV (Fig. 2C). To examine whether the synaptic recruitmentof AMPA receptors is attributable to the activation of NMDA receptorsby the observed high-frequency spontaneous synaptic responses,we used TTX to block sodium channel-mediated action potentials.In the presence of TTX the withdrawal of D,L-APV had no significanteffect on the number of AMPA receptor clusters (from 607 ± 29to 591 ± 32 per field; p > 0.05; n1 = 20, n2 = 20; Fig. 2D) orNMDA receptor clusters (from 1310 ± 45 to 1340 ± 48 per field;p > 0.05; n1 = 20, n2 = 20; Fig. 2E) and the proportion of silentsynapses (from 53.6 to 55.8%; p > 0.05; Fig. 2G). To test furtherwhether the mobilization of AMPA receptors was dependent on synapticactivity, we removed Ca²⁺ from the aCSF bath solution to block the release of presynapticvesicles. In aCSF with 0 mM Ca²⁺ the withdrawal of D,L-APV did not affect the number of AMPA receptorclusters significantly (from 611 ± 31 to 565 ± 25 per field; p> 0.05; n1 = 20, n2 = 20; Fig. 2D) or NMDA receptor clusters (from1402 ± 44 to 1361 ± 36 per field; p > 0.05; n1 = 20, n2 = 20;Fig. 2E) or the number of silent synapses (from 56.6 to 58.4%;p > 0.05; Fig. 2G). These results indicate that activation ofNMDA receptors can induce a rapid mobilization of AMPA receptorsinto morphological silent synapses that previously contained onlyNMDA receptors but no AMPAreceptors.

We next wanted to determine whether the new synaptic AMPA receptor clusters were present on the cell surface. Using the sameinduction protocol, we labeled the surface GluR1 receptors onlive neurons with an antibody against the N terminus of GluR1.Withdrawal of D,L-APV significantly increased the number of surfaceGluR1 clusters (from 672 ± 45 to 976 ± 37 per field; p < 0.001;n1 = 20, n2 = 20; Fig. 3A,B) but had no significant effect onthe number of NR1 clusters (from 1330 ± 43 to 1328 ± 38 per field;p > 0.05; n1 = 20, n2 = 20; Fig. 3A,B). The proportion of morphologicalsilent synapses significantly decreased from 50.2 to 26% (p <0.001; Fig. 3B).

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Figure 3. GluR1 AMPA receptor subunits were mobilized to the synaptic surface after the withdrawal of D,L-APV. A, Double staining of high-density cultured cortical neurons by antibodies against the N terminus of surface GluR1 subunits (left) and the C terminus of NR1 subunits (right) after these neurons were incubated in aCSF in the presence (top) and absence (bottom) of D,L-APV. B, The number of surface GluR1 clusters was increased (left) and the proportion of silent synapses was decreased (right) after the withdrawal of D,L-APV (filled bars) compared with control (open bars). ***p < 0.001.

LTP induction results in the long-lasting increases in AMPA receptor responses. To examine whether the synaptic recruitmentof AMPA receptors in our system is a long-term effect, we removedD,L-APV from the neurons for 15 min and then placed them backinto culture medium containing D,L-APV for 2 hr. Under these conditionswe observed a persistent increase in the number of AMPA receptorclusters (from 434 ± 18 to 685 ± 19 per field; p < 0.001; n1 =20, n2 = 20; Fig. 4A,B) and a persistent decrease in the amountof silent synapses (from 65 to 46%; p < 0.001; Fig. 4A,B).

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Figure 4. Changes in synaptic AMPA receptors induced by the withdrawal of D,L-APV can persist for at least 2 hr. A, Double staining of high-density cultured cortical neurons by antibodies against NR1 subunits and GluR1 subunits after these neurons were incubated in aCSF in the presence (top) and absence (bottom) of D,L-APV for ~15-20 min and then returned to culture medium with D,L-APV for 2 hr. B, An increase in the number of AMPA clusters (left) and a decrease in the proportion of silent synapses (right) can persist for 2 hr after the withdrawal of D,L-APV. ***p < 0.001.

To rule out that the mobilization of AMPA receptors was induced directly by action potentials via NMDA receptor-independentpathways, we added TTX to the aCSF bath solution to block actionpotentials and then removed D,L-APV and Mg²⁺ in the presence of exogenous glycine to allow for the activationof NMDA receptors by the spontaneous release of glutamate. Althoughnot as dramatic, under this condition the withdrawal of D,L-APValso significantly increased the number of AMPA receptor clusters(from 468 ± 26 to 592 ± 15 per field; p < 0.001; n1 = 20, n2 =20; Fig. 5A,B), had no effect on the number of NR1 clusters (from1167 ± 36 to 1116 ± 29 per field; p > 0.05; n1 = 20, n2 = 20;Fig. 5A,B), and decreased the number of silent synapses significantlyfrom 59.8 to 46.7% (p < 0.001; Fig. 5B).

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Figure 5. Mobilization of AMPA receptors can be induced in the presence of TTX in D,L-APV-treated high-density cortical neurons. A, Double staining of NMDA receptor subunits (NR1) and AMPA receptor subunits (GluR1/2/3) in neurons that had been incubated in aCSF (with 1 µM TTX, 100 µM glycine, and no added Mg²⁺) in the presence (top) and absence (bottom) of D,L-APV. B, The addition of glycine and the withdrawal of Mg²⁺ significantly increased the number of AMPA receptor clusters (left) and decreased the proportion of silent synapses even in the presence of TTX (right). ***p < 0.001.

Interestingly, a similar protocol also could be used to recruit rapidly the AMPA receptors in low-density hippocampal culturesdespite the low intrinsic activity in these cultures. As withthe TTX-treated cortical cultures, the activation of NMDA receptorsin the low-density hippocampal cultures by D,L-APV and Mg²⁺ removal in the presence of exogenous glycine increased the numberof AMPA receptor clusters (from 29.7 ± 3.3 to 88.8 ± 8.0/100 µmof dendrite; p < 0.001; n1 = 20, n2 = 20; Fig. 6A,B) and reducedthat number of silent synapses at hippocampal neurons from 73.8to 23% (Fig. 6C). After this paradigm the silent synapses almostdisappeared in one-half of the analyzed neurons, in which almostall of the AMPA clusters were colocalized with NR1 clusters (>90%;Fig. 6A, bottom two panels). The recruitment of AMPA receptorto synapses also could be observed in the absence of chronic treatmentof the neurons with D,L-APV. Although the initial proportion ofsilent synapses in cultures grown in normal medium was lower thanthe D,L-APV-treated cultures, the removal of Mg²⁺ in the presence of exogenous glycine increased the number ofAMPA receptor clusters from 55.4 ± 4.8 to 98.6 ± 7.3/100 µm ofdendrite (p < 0.001; n1 = 20, n2 = 20; Fig. 6E) and decreasedthe proportion of silent synapses (from 53.4 to 18.2%; Fig. 6F).

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Figure 6. Rapid mobilization of AMPA receptors into silent synapses via the activation of NMDA receptors in low-density hippocampal cultures. A, Double staining of low-density hippocampal neurons that had been treated chronically with D,L-APV by antibodies against an NMDA receptor subunit (NR1) and AMPA receptor subunits (GluR1/2/3). Top two panels, A neuron that had been incubated in aCSF with 100 µM glycine, 200 µM D,L-APV, and no added Mg²⁺ for 15 min. Bottom two panels, A neuron that had been incubated in similar aCSF without D,L-APV. B, The number of AMPA clusters was increased significantly via the activation of NMDA receptors by glycine and 0 Mg²⁺. C, The proportion of silent synapses was decreased significantly via the activation of NMDA receptors. D-F are similar to A-C, with the use of neurons that had been grown in culture medium in the absence of D,L-APV. Open bars, Neurons that had been incubated in aCSF containing glycine, D,L-APV, and no added Mg²⁺; filled bars, neurons that had been incubated in aCSF containing glycine, no D,L-APV, and no added Mg²⁺. ***p < 0.001.

If the AMPA receptors delivered into silent synapses were functional, we would expect to see a parallel increase in mEPSCresponses after the withdrawal of D,L-APV. We induced synaptictargeting of AMPA receptors by incubating cortical neurons withaCSF in the absence of D,L-APV for 15-20 min. Thereafter, mEPSCresponses mediated via AMPA receptors were recorded in aCSF [2.5mM Ca²⁺and (in µM) 200 D,L-APV, 1 TTX, 100 picrotoxin at 32°C] with whole-cellvoltage clamp. Withdrawal of D,L-APV significantly increased thefrequency of mEPSCs (from 0.87 ± 0.15 to 2.1 ± 0.28 responses/200msec; p < 0.01; n1 = 12, n2 = 12; Fig. 7A,B), although it hada negligible effect on the mean peak amplitude (from 12.3 ± 0.6to 12.1 ± 0.7 pA; p > 0.05; Fig. 7C), rise time (from 2.4 ± 0.1to 2.5 ± 0.1 msec; p > 0.05), and decay time (from 8.9 ± 0.5 to8.9 ± 0.4 msec; p > 0.05; Fig. 7C). In the presence of TTX thewithdrawal of D,L-APV no longer had any obvious effect on thefrequency of mEPSCs (from 1.1 ± 0.25 to 0.93 ± 0.11 responses/200msec; p > 0.05; n1 = 6, n2 = 6; Fig. 7B). In aCSF with 0 mM Ca²⁺ the withdrawal of D,L-APV also had no significant effect on thefrequency of mEPSCs (from 0.87 ± 0.14 to 0.84 ± 0.12 responses/200msec; p > 0.05; n1 = 9, n2 = 9; Fig. 7B). These results suggestthat silent synapses can acquire AMPA receptor-mediated responsesafter the activation of NMDA receptors by the spontaneous synapticactivity. Although we did not detect a significant change in themean amplitude of mEPSCs after D,L-APV removal, the distributionof the mEPSC amplitudes shifted and contained higher percentagesof large (>30 pA) and small (<10 pA) mEPSC responses (Fig. 7D).

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Figure 7. Withdrawal of D,L-APV significantly increased the frequency of mEPSC responses. A, Left, Ten representative consecutive traces recorded from a neuron after 15 min of incubation in aCSF in the presence of D,L-APV. A, Right, Ten similar traces after incubation in aCSF in the absence of D,L-APV. B, Withdrawal of D,L-APV significantly increased the frequency of mEPSC responses (filled bars) compared with control (open bars). TTX and 0 mM Ca²⁺ blocked this increase. C, Withdrawal of D,L-APV had a negligible effect on the peak amplitude (left) and the rise time and decay time (right) of EPSC responses. D, The probability of mEPSC responses over a wide range of peak amplitudes. In all, 50 consecutive sweeps were selected from each recorded neuron and pooled to calculate the probability for mEPSC responses occurring at each 1 pA interval of peak amplitude. **p < 0.01.

Many previous reports have indicated that CaM-dependent kinase II plays a critical role in the induction of LTP (Silva etal., 1992; Giese et al., 1998; Soderling and Derkach, 2000). Recentstudies also have shown that CaM kinase II is recruited rapidlyto synapses after LTP induction in hippocampal slices (Ouyanget al., 1997, 1999; Shen and Meyer, 1999), where it phosphorylatesthe AMPA receptor GluR1 subunit of the AMPA receptor (Barria etal., 1997b; Lee et al., 2000). To examine whether similar processesoccurred in the high-density cortical cultures, we analyzed thedistribution of CaM kinase II and the phosphorylation of GluR1before and after D,L-APV removal. Using immunocytochemical techniqueswith CaM kinase II antibodies, we found that, similar to LTP inhippocampal slices, the activation of NMDA receptors in corticalcultures induced a rapid mobilization of CaM kinase II to synapses(Fig. 8A,B). In contrast, no corresponding increase was observedin the control cultures maintained in D,L-APV (Fig. 8A,B). Moreover,using Western blot techniques with a phosphorylation site-specificantibody against the major CaM kinase II site on GluR1 (serine831), we found that phosphorylation of serine 831 was significantlyincreased in total cell extracts (0.227 ± 0.010 to 0.418 ± 0.034;p < 0.005; n1 = 6, n2 = 6; Fig. 8C,D). Interestingly, this increasedphosphorylation occurred preferentially on surface receptors isolatedwith the use of surface biotinylation techniques (from 0.132 ±0.008 to 0.317 ± 0.028; p < 0.001; n1 = 6, n2 = 6; Fig. 8E,F).Subtraction of the GluR1-S831-phospho surface signal from theGluR1 total reveals that, although phosphorylated at a basal level,there is only a small, but nonsignificant, increase in GluR1-S831phosphorylation of intracellular AMPA receptors (from 0.336 ±0.137 to 0.421 ± 0.174; p > 0.05; n1 = 6, n2 = 6). Phosphorylationof GluR1 serine 845 was not detectable in these experiments (datanot shown). These results demonstrate that the activation of NMDAreceptors by spontaneous activity in cultured cortical neuronscan induce coincident and rapid translocation of AMPA receptorsand CaM kinase II to synapses and increased CaM kinase II phosphorylationof the GluR1 AMPA receptor subunit.

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Figure 8. CaM kinase II is mobilized rapidly into synapses, and phosphorylation of GluR1-S831 is upregulated in response to the synaptic targeting of AMPA receptors. A, B, Double staining of high-density cultured cortical neurons by antibodies against AMPA receptor subunits (GluR1/2/3) and an antibody against CaM kinase II (CaMK II) after the neurons were incubated in aCSF in the presence (A) and absence (B) of D,L-APV. Bottom panels in A and B show enlarged images (2×) of GluR1/2/3 (left), CaMK II (middle), and overlay of GluR1/2/3 (red) and CaMK II (green). C, Representative immunoblots of total proteins (in duplicate) immunoblotted with either anti-GluR1-C or anti-GluR-S831-P from control (D,L-APV to D,L-APV) and experimental (D,L-APV to aCSF) conditions. D, Quantitative analysis of immunoblots comparing the relative ratio of anti-GluR-S831-P immunostaining with anti-GluR1-C (y-axis) from control and experimental conditions. E, Similar blots as in C, but depicting two representative examples from isolated surface proteins. Arrowhead indicates the GluR1-S831-P band. F, Quantitative analysis of surface proteins comparing anti-GluR-S831-P with anti-GluR1-C (y-axis). **p < 0.01; ***p < 0.001.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Changes in AMPA receptor-mediated responses have been proposed to be important to various forms of synaptic plasticity, includingLTP and LTD (Raymond et al., 1993; Kim and Huganir, 1999; Turrigiano,2000). Electrophysiological studies have reported that a significantproportion of synapses in the CNS contains NMDA receptor responses,but no AMPA receptor responses (Isaac et al., 1995; Liao et al.,1995; Durand et al., 1996). Such synapses would be functionallysilent at normal resting membrane potentials because of the voltage-dependentblockade of NMDA receptors by Mg²⁺ (Mayer et al., 1984; Nowak et al., 1984). These silent synapsesprogressively become active via the acquisition of AMPA receptor-mediatedresponses during neuronal development and can be activated rapidlyduring LTP (Isaac et al., 1995; Liao et al., 1995; Durand et al.,1996; Wu et al., 1996). Recent evidence has suggested that theactivation of AMPA receptor responses is attributable to rapidchanges in the level of synaptic AMPA receptors (Shi et al., 1999;Hayashi et al., 2000). In these previous studies it was shownthat recombinant GFP-tagged GluR1 subunits expressed in organotypichippocampal slices can be recruited to synapses by LTP-inducingstimuli (Shi et al., 1999; Hayashi et al., 2000). In this currentstudy we combined immunocytochemical, biochemical, and electrophysiologicaltechniques to study the NMDA receptor-dependent synaptic deliveryof native AMPA receptor subunits in both high-density corticaland low-density hippocampal neuronal cultures. We predicted thathigh levels of spontaneous synaptic activity in cortical neuronalcultures might be able to activate NMDA receptors in a way similarto tetanus stimulation, a method often used to induce LTP. Toincrease the number of silent synapses in our cultures, we chronicallytreated the cultures with D,L-APV, starting at a very early stageof in vitro development. Similar to our previous studies in low-densityhippocampal cultures, D,L-APV treatment produced a large proportionof silent synapses in these high-density cortical cultures (Raoand Craig, 1997; Liao et al., 1999). After the withdrawal of D,L-APVthe vast majority of dendrites that previously contained diffuselydistributed AMPA receptors rapidly acquired clustered AMPA receptors.Withdrawal of D,L-APV also induced a parallel increase in thefrequency of mEPSC responses. A blockade of spontaneous activityby TTX or 0 mM Ca²⁺ prevented this synaptic delivery of AMPA receptors. These resultsindicate that the high levels of spontaneous synaptic activityin high-density cortical cultures can induce a rapid NMDA receptor-dependentmobilization of AMPA receptors into silent synapses. In addition,we found that we could circumvent the low level of spontaneousactivity in low-density hippocampal cultures and rapidly recruitAMPA receptors to synapses by activating NMDA receptors via theremoval of D,L-APV and Mg²⁺ in the presence of glycine. Our results are similar to a recentstudy published after the completion of this work, showing NMDAreceptor-dependent synaptic insertion of AMPA receptors in cultureddissociated hippocampal neurons (Lu et al., 2001).

Interestingly, the redistribution of AMPA receptors in these cultures is remarkably similar to the recently reported changeof GFP-tagged GluR1 subunits induced by a tetanus stimulationin organotypic hippocampal slices (Shi et al., 1999). This similaritysuggests that the redistribution of AMPA receptors in these twosystems may be induced by similar cellular processes. In thisstudy we further demonstrated that these newly acquired AMPA receptorclusters were located in synapses that were labeled by antibodiesagainst NMDA receptor NR1 subunits and synaptophysin. This indicatesthat the previously silent synapses in these cultures were activatedby the recruitment of native AMPA receptors. These data provideadditional direct evidence that the activation of silent synapsesmay mediate, in part, the long-term potential of synaptictransmission.

Previous studies have demonstrated that the GluR1 subunit is a substrate for CaM kinase II, PKC, and PKA (Roche et al., 1996;Barria et al., 1997b; Mammen et al., 1997) and that phosphorylationof the GluR1 subunit can increase AMPA receptor ion channel function(McGlade-McCulloh et al., 1993; Roche et al., 1996; Barria etal., 1997a,b; Benke et al., 1998; Derkach et al., 1999). Recentstudies in hippocampal slices have suggested that the modulationof AMPA receptor ion channel properties by protein phosphorylationmay be important in LTP and LTD (Soderling and Derkach, 2000).It has been reported that LTP induction in slice preparationsor glutamate treatment of neuronal cultures induces the rapidrecruitment of CaM kinase II to excitatory synapses (Ouyang etal., 1997, 1999). Moreover, LTP induction increases CaM kinaseII phosphorylation of serine 831 on the GluR1 subunit (Barriaet al., 1997a; Banke et al., 2000; Lee et al., 2000). As seenin these LTP studies in hippocampal slices, we also observed arapid synaptic targeting of CaM kinase II and an increase in GluR1-S831phosphorylation. This phosphorylation and its effect on channelkinetics may account in part for the observed changes in the distributionof mEPSC amplitudes, but it is not clear whether the synapticdelivery of AMPA receptors and the changes in mEPSC frequencyrequire the phosphorylation of serine 831. It is certainly possiblethat phosphorylation of this site regulates synaptic traffickingof the AMPA receptor in addition to regulating channel function.However, the regulation of synaptic recruitment of AMPA receptorsmay be via a distinct mechanism, which occurs in concert withand complements the modification of channel properties. The molecularand cellular mechanisms that regulate the mobilization of AMPAreceptors into postsynaptic silent synapses are still not clear.Studies in several laboratories have suggested that proteins thatinteract with AMPA receptor subunits, such as the PDZ-containingproteins GRIP1/2/ABP, PICK1, and SAP97 as well as membrane fusionfactor NSF, may regulate the function of AMPA receptors (Donget al., 1997, 1999; Nishimune et al., 1998; Osten et al., 1998;Song et al., 1998; Li et al., 1999; Noel et al., 1999; Hayashiet al., 2000). Future studies will be needed to elucidate therole of these proteins in LTP and the mechanism for the couplingof CaM kinase II activation to the regulation of AMPA receptordistribution.

  FOOTNOTES

Received March 28, 2001; revised May 14, 2001; accepted May 23, 2001.

This work was supported by the Howard Hughes Medical Institute and the National Institutes of Health. We thank Doreen Buryfor assistance in preparing thismanuscript.
Correspondence should be addressed to Dr. Richard L. Huganir, Department of Neuroscience, Howard Hughes Medical Institute,Johns Hopkins University School of Medicine, 725 North Wolfe Street,Baltimore, MD 21205. E-mail: rhuganir{at}jhmi.edu.

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