Regulation of GluR1 by the A-Kinase Anchoring Protein 79 (AKAP79) Signaling Complex Shares Properties with Long-Term Depression

doi:20026277

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (75)

Citing Articles via Google Scholar

Google Scholar

Articles by Tavalin, S. J.

Articles by Scott, J. D.

Search for Related Content

PubMed

PubMed Citation

Articles by Tavalin, S. J.

Articles by Scott, J. D.

Previous Article  |  Next Article

The Journal of Neuroscience, April 15, 2002, 22(8):3044-3051

Regulation of GluR1 by the A-Kinase Anchoring Protein 79 (AKAP79) Signaling Complex Shares Properties with Long-Term Depression
Steven J. Tavalin¹, Marcie Colledge¹, Johannes W. Hell², Lorene K. Langeberg¹, Richard L. Huganir³, and John D. Scott¹
¹ Howard Hughes Medical Institute, Vollum Institute, Oregon Health Sciences University, Portland, Oregon 97201, ² Department of Pharmacology, University of Iowa, Iowa City, Iowa 52242, and ³ Howard Hughes Medical Institute, Department of Neuroscience, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21205

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Second messengers regulate synaptic plasticity by influencing the balance between kinase and phosphatase activity. One targetof this balance is the phosphorylation state of the AMPA receptorglutamate receptor 1 (GluR1) subunit. Hippocampal long-term depression(LTD) is a calcium-dependent downregulation of synaptic AMPA receptorcurrents associated with dephosphorylation of Ser845, a cAMP-dependentprotein kinase (PKA) site on GluR1. Recruitment of kinases andphosphatases to the AMPA receptor might enable modulation of AMPAreceptor function. The neuronal A-kinase anchoring protein AKAP79/150interacts with PKA and the calcium-dependent protein phosphatasePP2B and is linked to the AMPA receptor GluR1 subunit by synapse-associatedprotein 97 (SAP97), a membrane-associated guanylate kinase familyprotein. Here we demonstrate that AKAP79 not only promotes basalphosphorylation of Ser845 but also confers a calcium- and PP2B-mediateddownregulation to GluR1 receptor currents. This AKAP79-dependentdownregulation is contingent on the local presence of PKA, Ser845of GluR1, and a PDZ (postsynaptic density 95/Discs large/zonaoccludens 1)-domain interaction between GluR1 and SAP97, all ofwhich support basal phosphorylation of the receptor. These findingssuggest that the AKAP79 signaling complex is sufficient to coupleintracellular calcium levels to the PKA phosphorylation stateof GluR1. Thus, the integration of intracellular signals relevantfor LTD may be transduced to GluR1 by the AKAP79 signalingcomplex.

Key words: AKAP79; kinase; phosphatase; cAMP; calcium; AMPA receptor; synaptic plasticity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activity-dependent alterations in AMPA receptor-mediated synaptic transmission such as long-term potentiation (LTP) and long-termdepression (LTD) are thought to provide a cellular basis for informationstorage (Malenka and Nicoll, 1999). As reviewed recently (Winderand Sweatt, 2001), calcium entry through NMDA-type glutamate receptorstriggers both forms of synaptic plasticity. High levels of intracellularcalcium achieved during LTP upregulate synaptic strength by preferentiallyactivating the calcium/calmodulin-dependent protein kinase II(CaMKII). In contrast, the lower calcium concentrations that occurduring LTD may downregulate synaptic strength by favoring a phosphatasecascade involving PP2B and protein phosphatase 1 (PP1). Thus,the balance between kinase and phosphatase activity has been proposedto be a critical determinant for controlling the degree of synapticefficacy by regulating the phosphorylation state of synaptic substrates.Recent evidence suggests that LTP and LTD are reflected in thephosphorylation state of the AMPA receptor glutamate receptor1 (GluR1) subunit (Barria et al., 1997; Kameyama et al., 1998;Lee et al., 1998, 2000). However, the mechanisms by which GluR1phosphorylation and dephosphorylation are orchestrated remainunclear.

A-kinase anchoring proteins (AKAPs) bind to the regulatory subunits of protein kinase A (PKA) and target PKA to various subcellularcompartments, providing a mechanism to efficiently regulate thephosphorylation state of relevant substrates (Colledge and Scott,1999). The multivalent anchoring protein AKAP79 (AKAP150 in rodents)associates with PP2B and PKC, in addition to PKA, and is enrichedat postsynaptic sites of hippocampal neurons (Carr et al., 1992b;Coghlan et al., 1995; Klauck et al., 1996; Colledge et al., 2000;Sik et al., 2000). Recently, we demonstrated that AKAP79/150 andGluR1 are linked together by synapse-associated protein 97 (SAP97),facilitating basal phosphorylation of Ser845 on GluR1 (Colledgeet al., 2000). Phosphorylation of Ser845 enhances native and recombinantAMPA receptor currents (Roche et al., 1996; Banke et al., 2000).Ser845 is basally phosphorylated (Mammen et al., 1997) and isselectively dephosphorylated during LTD (Kameyama et al., 1998;Lee et al., 1998, 2000). Although the AKAP79/150 signaling complexmay facilitate Ser845 phosphorylation, a corresponding mechanismfor the dephosphorylation of this site remains to beidentified.

Disruption of PKA function should favor phosphatase activity reducing AMPA receptor currents. Indeed, previous studies indicatethat PKA inhibition produces synaptic depression that occludessubsequent LTD (Kameyama et al., 1998). Similarly, peptide-mediateddisruption of AKAP-PKA interactions attenuates AMPA receptor currentsand synaptic events (Rosenmund et al., 1994). Therefore, we soughtto identify whether a phosphatase contributes to AMPA receptordownregulation when PKA anchoring is disrupted and whether theAKAP79/150 can account for this modulation. Here, we report thatPP2B regulates hippocampal AMPA receptor currents in oppositionto anchored PKA. Furthermore, we demonstrate that this dual PKA-and PP2B-dependent regulation of AMPA receptor currents can bereconstituted by coexpression of AKAP79 with GluR1. AKAP79-dependentregulation of GluR1 occurs at Ser845 and depends on protein-proteininteractions that promote basal phosphorylation at this site.Our data suggest that the AKAP79/150 signaling complex is sufficientto support modulation of the phosphorylation state of GluR1 ina manner analogous toLTD.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell cultures. Glass coverslips (22 × 22 mm) were coated overnight with 100 µg/ml poly-D-lysine and 10 µg/ml laminin. Neuronalcells were plated on a bed of glial cells. Hippocampi were removedfrom neonatal Sprague Dawley rats (1- to 3-d-old). Tissue wasdissociated by papain treatment and trituration through Pasteurpipettes and suspended in media consisting of MEM, 10% FBS, andpenicillin-streptomycin (P/S), and plated at a density of 250,000cells/ml for glial cells. Glutamate at 100 µM was added for 15min to kill off neuronal cells and washed with media. Glial cultureswere allowed to grow for 1 week until they reached confluence.Neurons were prepared in the same manner, except that glutamatewas omitted and cells were plated at 150,000 cells/ml. After 6hr cells, were washed with Neurobasal media with B27 supplement,0.5 mM L-glutamine, and P/Sadded.

Human embryonic kidney 293 (HEK293) cells were obtained from American Type Culture Collection (Manassas, VA) at passage 31and were used at passages 33-40. HEK293 cell cultures were maintainedin DMEM with 10% FBS (HyClone, Logan, UT) and P/S. For electrophysiology,HEK293 cells were plated at low density (~50,000 cells) on 35mm culture dishes (Falcon, Franklin Lakes, NJ). For biochemistry,HEK293 cells were plated at ~50% confluence on 10 cmdishes.

Expression constructs. GluR1_flip was in the pRK5 vector, and AKAP18-green fluorescent protein (GFP) and AKAP79-GFP were inpcDNA3, as described previously (Colledge et al., 2000). Dr. TomSoderling (Vollum Institute, Portland, OR) provided GluR1_flipS831Aand GluR1_flipS845A in the pRK5 vector. AKAP79(1-360)-GFP in pcDNA3was provided by Dr. Mark Dell'Acqua (University of Colorado HealthSciences Center, Denver, CO). Dr. Craig Garner (University ofAlabama at Birmingham, Birmingham, AL) provided the SAP97 construct.Dr. John Adelman (Vollum Institute, Portland, OR) provided theCD4 cell surface marker in a JPA vector. GluR1_flipT887A was constructedby site-directed mutagenesis and inserted into pcDNA3.1 usingthe TOPO TA cloning kit (Invitrogen, San Diego,CA).

Electrophysiology. Pyramidal-shaped neurons from cultures at 5-12 d in vitro were selected for recordings. HEK293 cells weretransfected by the calcium phosphate method. One microgram ofeach construct was used per dish for electrophysiological experiments.For these experiments, the CD4 cell surface marker was also includedas a transfection marker. Twenty-four hours after transfection,cells were visually selected for recording by adherence of CD4antibody-coated beads. GFP epifluorescence confirmed the expressionof the correspondingAKAP.

Whole-cell recordings were made with an Axopatch 200B amplifier (Axon Instruments, Foster City, CA). Patch pipettes (2-4 M $Omega$ )contained (in mM): 140 Cs methanesulfonate, 10 HEPES, 5 adenosinetriphosphate (Na salt), 5 MgCl2, 0.2 CaCl2, and 1 or 10 of eitherBAPTA or EGTA, pH 7.4. Peptides were added to the pipette solutionfrom frozen concentrated stocks. Extracellular solution contained(in mM): 150 NaCl, 5 KCl, 1.8 or 0 CaCl2, 10 HEPES, and 10 glucose,pH 7.4. TTX (1 µM) and (+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d]cyclohepten-5,10-imine maleate (MK-801) (1 µM) were included forneuronal recordings. Glutamate, cyclothiazide, domoate, SYM-2206,8-bromo-cAMP, cyclosporin A, and okadaic acid were added fromfrozen stocks. Solution exchanges were accomplished through aseries of flow pipes. Flow pipes were controlled by solenoid valvesand moved into position by a piezoelectric bimorph. HEK293 cellswere lifted off the bottom of the dish to speed the solution exchangetime. Neuronal AMPA receptor currents were evoked by 1 sec applicationsof domoate at 30 sec intervals. The AMPA receptor-selective antagonistSYM-2206 (100 µM) inhibited current responses by 94.7 ± 1.6% (n= 3; data not shown), indicating that domoate-activated currentswere predominantly mediated by AMPA receptors. GluR1 receptorcurrents were evoked by 500 msec application of glutamate in thepresence of cyclothiazide at 30 sec intervals. Currents were digitizedat 5 kHz and filtered at 1 kHz with a Digidata 1200B board andClampex 7 software (Axon Instruments). Series resistance (85-95%)and whole-cell capacitance compensation were used and routinelymonitored throughout the experiments. Only neurons with seriesresistance <12 M $Omega$ and HEK293 with series resistance <6 M $Omega$ wereincluded for analysis. All experiments were initiated within 1min of establishing the whole-cell configuration and were performedat a holding potential of $-$ 60 mV at 20°C.

For experiments in which phosphatase inhibitors were used, cells were pretreated with the inhibitors, and recordings wereperformed in the continued presence of the inhibitor. Pretreatmentperiods were 5 min for cyclosporin A (1 µM) and 15 min for okadaicacid (1 µM). In approximately one-half (three of seven for controland five of 10 for AKAP79) of the okadaic acid experiments inHEK293 cells, okadaic acid (1 µM) was also included in the pipettesolution. Because identical results were obtained under theseconditions, the data werepooled.

Current amplitudes of recombinant GluR1 receptors varied considerably for all conditions tested (range of 150-10,000 pA),likely because of differences in transfection efficiency. We observedno significant difference in current amplitudes between conditions.No correlation between the results obtained and current densitywere observed. For each experiment, currents were normalized tothe amplitude of current from the initial agonist application.All data are expressed as means ± SEM. Statistical significancewas determined by ANOVA, followed by Student's ttest.

Immunoprecipitations and immunoblotting from transfected HEK293 cells. For immunoprecipitation from heterologous cells, HEK293cells were transfected at 50-70% confluence in 10 cm plates bythe calcium phosphate method, using 4 µg of each cDNA constructper plate. Twenty-four to 48 hr after transfection, cells wererinsed in PBS and lysed in 400 µl of IP buffer (10 mM phosphate,150 mM NaCl, 5 mM EDTA, 5 mM EGTA, and 1% Triton X-100) containingprotease inhibitors. For GluR1 phosphorylation experiments, phosphataseinhibitors were also included (10 mM sodium pyrophosphate, 50mM sodium fluoride, 1 mM sodium orthovanadate, 1 µM okadaic acid,1 µM microcystin, and 1 µM cyclosporin). Cells were incubatedon ice for 30 min and then centrifuged at 40,000 × g for 30 min.Supernatants were incubated with 3 µg of antibody or control nonimmuneIgG and 30 µl of prewashed protein A agarose beads. An anti-GluR1C-terminal antibody was used to immunoprecipitate GluR1. For immunoprecipitationof endogenous SAP97 from HEK293 cells, a rabbit polyclonal antibodythat specifically recognizes SAP97 but not other membrane-associatedguanylate kinase (MAGUK) family member proteins was used (Valtschanoffet al., 2000). AKAP18-GFP was immunoprecipitated with affinity-purifiedrabbit polyclonal antibody [V064 (Fraser et al., 1998)]. AKAP79-GFPand AKAP79(1-360)-GFP were immunoprecipitated with 918I (ICOS,Bothell, WA). After overnight incubation at 4°C, the immunoprecipitateswere washed three times with IP buffer. Bound proteins were elutedwith SDS sample buffer and analyzed byimmunoblotting.

The following primary antibodies were used for immunoblotting: rabbit polyclonal to AKAP79 (5.6 µg/ml, 1:2500; 918I; ICOS),mouse monoclonal to PKA type II regulatory subunits $alpha$ and $beta$ (1:500dilution; Transduction Laboratories, Lexington, KY), mouse monoclonalagainst PP2B (1:300 dilution; Transduction Laboratories), rabbitpolyclonal antibody against SAP97 (Valtschanoff et al., 2000),rabbit polyclonal to C-terminal region of GluR1 (1:1000 dilution;Upstate Biotechnology, Lake Placid, NY), and rabbit polyclonalphospho-specific antibody against ser845 of GluR1 (Mammen et al.,1997) (1:250dilution).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

PP2B underlies rundown of hippocampal AMPA receptor current

We recorded whole-cell AMPA receptor currents from cultured hippocampal neurons in response to the nondesensitizing agonistdomoate (10 µM). Under control conditions, the amplitude of AMPAreceptor currents was relatively stable during the recording period(Fig. 1A, open squares) (control, 89.6 ± 4.6% of initial currentremaining, n = 5). Ht31, a 24 amino acid peptide correspondingto the type II regulatory subunit (RII)-binding domain of a humanthyroid AKAP, was used as a competitive antagonist of PKA anchoring(Carr et al., 1992a). As shown previously (Rosenmund et al., 1994),disrupting PKA anchoring by inclusion of Ht31 (1 µM) within thewhole-cell pipette solution caused a significant time-dependentreduction of AMPA receptor currents (Fig. 1A, filled triangles)(Ht31, 61.5 ± 3.8%, n = 7; p < 0.01). This Ht31-induced rundownis calcium dependent because it was prevented when experimentswere performed in the absence of extracellular calcium (Fig. 1B,open squares, filled triangles) (control, 91.7 ± 3.9%, n = 6;Ht31, 84.5 ± 3.1%, n = 6). When calcium influx through voltage-gatedcalcium channels was blocked by cadmium (200 µM), Ht31-inducedrundown still occurred, although there was a selective attenuationof the late phase of the rundown (Fig. 1C, open squares, filledtriangles) (control, 89.4 ± 2.2%, n = 5; Ht31, 73.3 ± 1.7%, n= 6). Given that NMDA receptors were blocked by the combined presenceof magnesium and MK-801, these data suggest that calcium entrythrough calcium-permeable AMPA receptors may promote the initialphase of the rundown. Collectively, these data indicate that calciumis required for the phenomenon and that multiple sources of calciuminflux contribute to the Ht31-induced rundown.

View larger version (32K):
[in this window]
[in a new window]
Figure 1. Disruption of PKA anchoring promotes a PP2B-mediated rundown of hippocampal AMPA receptor currents. Whole-cell recordings were performed from cultured hippocampal neurons. Summary of time course of AMPA receptor currents is presented. Responses were normalized to the peak amplitude from the initial current evoked in response to domoate (10 µM). A, Displacement of PKA by whole-cell dialysis of Ht31 (1 µM) leads to rundown of AMPA receptor currents. Insets show representative first and last responses from a control cell and one in which Ht31 was included in the pipette. The number of observations for each condition is indicated. B, The Ht31-induced rundown is prevented when experiments were performed in the absence of extracellular recording solution. C, Experiments performed in the presence of 200 µM cadmium indicate that voltage-gated calcium channels contribute to a late phase of the rundown. Dotted line depicts Ht31 data from A for comparison. D, Bar graph summarizing the effect of phosphatase inhibitors on the rundown. Cyclosporin A (CsA; 1 µM) treatment prevents Ht31-induced rundown of AMPA receptor currents. *p < 0.01 compared with cyclosporin A alone. Inhibition of PP1/PP2A by okadaic acid (OA; 1 µM) partially reduced the Ht31 mediated rundown. **p < 0.01 compared with okadaic acid alone.

Exogenous application of the calcium- and calmodulin-dependent protein phosphatase PP2B decreases the open probability ofAMPA receptors, a property regulated by the PKA phosphorylationsite on GluR1 (Banke et al., 2000). Therefore, we tested whetherPP2B might be an effector, downstream of calcium, for the Ht31-inducedrundown. In the presence of the PP2B-selective antagonist cyclosporinA (1 µM), Ht31 no longer produced rundown (control, 89.7 ± 3.8%,n = 5; Ht31, 83.7 ± 2.9%, n = 7; p > 0.2) (Fig. 1D). In contrast,the PP1/PP2A-selective antagonist okadaic acid (1 µM) only partiallyreduced the rundown (control; 88.4 ± 3.1%, n = 6; Ht31, 71.8 ±1.8%, n = 7; p < 0.01) (Fig. 1D). Given that the rundown is observedonly during disruption of PKA anchoring, these data suggest thatPP2B is the predominant phosphatase counteracting the action ofanchored PKA. The dual regulation of hippocampal AMPA receptorsby anchored PKA and PP2B is consistent with the AKAP79/150-directedlocation of PKA and PP2B at postsynaptic sites (Coghlan et al.,1995; Colledge et al., 2000).

Coordinate regulation of GluR1 phosphorylation by the AKAP79 signaling complex

To test directly whether an AKAP79/150 complex regulates AMPA receptor currents, we attempted to reconstitute "rundown" inHEK293 cells. Homomeric GluR1 receptors were expressed alone (control)or together with one of two plasma membrane-targeted neuronalanchoring proteins: AKAP79 or AKAP18 (also referred to as AKAP15)(Dell'Acqua et al., 1998; Fraser et al., 1998; Gray et al., 1998).As shown in Figure 2, both anchoring proteins associate with endogenousPKA in HEK293 cells. The RII subunit of PKA was coimmunoprecipitatedwith either AKAP79 or AKAP18 (Fig. 2A, top panel). In contrast,endogenous PP2B copurified with AKAP79 but not with AKAP18 (Fig.2A, bottom panel). We then tested whether these AKAPs could enhancephosphorylation of Ser845, a known PKA site in the cytoplasmictail of GluR1. Basal phosphorylation of Ser845 of GluR1 was enhancedby coexpression of AKAP18 (241 ± 47% over control, n = 4; p <0.01) (Fig. 2B) and AKAP79 (183 ± 32% over control, n = 7; p <0.01) (Fig. 2B). These findings suggest that AKAP-mediated recruitmentof PKA to the plasma membrane facilitates phosphorylation of Ser845.

View larger version (43K):
[in this window]
[in a new window]
Figure 2. Selective PP2B-mediated downregulation of GluR1 receptor currents by coexpression of AKAP79. A, Selective association of AKAP79 with endogenous PP2B. Extracts from HEK293 cells transfected with either AKAP18-GFP or AKAP79-GFP were immunoprecipitated with their respective antibodies or control IgG antibodies. Immunoprecipitates were blotted with anti-RII antibodies (top) or anti-PP2B antibodies (bottom). Although both AKAP18 and AKAP79 coimmunoprecipitated RII as expected, only AKAP79 coimmunoprecipitated PP2B. B, Basal phosphorylation of the PKA site, Ser845, of GluR1 is enhanced by coexpression of membrane-targeted AKAPs. GluR1 was expressed alone (control) or with either AKAP18 or AKAP79 in HEK293 cells. Extracts from HEK293 cells were immunoprecipitated with antibodies against the C-terminal tail of GluR1. Phosphorylation of Ser845 was determined by blotting with phospho-specific antibodies to Ser845 (top). Total amount of GluR1 was determined by blotting with the C-terminal GluR1 antibody (middle). Results from experiments are summarized (bottom). The relative amount of GluR1 phosphorylation was quantified by determining the ratio of signals from the phospho-Ser845 antibody to that from the C-terminal antibody. For each experiment, data were normalized to the GluR1 alone (group control). The number of experiments is indicated in parentheses. C, Whole-cell recordings were performed from transfected HEK293 cells. Summary of time course of recombinant GluR1 receptor currents. Responses were normalized to the peak amplitude from the initial current evoked in response to glutamate (1 mM) in the presence of cyclothiazide (100 µM). HEK293 cells were transfected with GluR1 alone (control) or with either AKAP18 or AKAP79. GluR1 currents selectively rundown when cotransfected with AKAP79. The pipette solution contained 1 mM BAPTA. The number of observations for each condition is indicated. Unless otherwise indicated, all subsequent figures are presented in the same manner. Insets show representative first and last responses from control, AKAP18, and AKAP79 cells. D, Blocking rises in intracellular calcium by elevating the concentration of BAPTA in the pipette solution to 10 mM prevents the AKAP79-dependent rundown of GluR1 receptor currents. E, Experiments performed in the absence of extracellular calcium indicate that the AKAP-dependent rundown is calcium dependent and suggest that calcium entry is required for the rundown. F, Bar graph summarizing effects of phosphatase inhibitors on the Ht31-induced rundown. Inhibition of PP2B activity by cyclosporin A (1 µM) but not PP1/PP2A by okadaic acid (1 µM) prevents the AKAP79-dependent rundown. *p < 0.05 compared with control. **p < 0.05 compared with okadaic acid alone.

To test the effect of AKAP coexpression on GluR1 function, we recorded nondesensitizing whole-cell GluR1 receptor currentsevoked by application of glutamate (1 mM) in the presence of cyclothiazide(100 µM). Cells expressing GluR1 alone (Fig. 2C, open squares)(control, 83.8 ± 5.1%, n = 7) and those cells coexpressing AKAP18(Fig. 2C, filled circles) (AKAP18, 85.2 ± 4.8%, n = 8) exhibitedrelatively stable currents over the 15 min recording period. Incontrast, coexpression of AKAP79 resulted in a spontaneous time-dependentreduction in GluR1 receptor currents (Fig. 2C, filled triangles)(AKAP79, 60.0 ± 5.3%, n = 9; p < 0.01). The magnitude and timecourse of this effect was similar to the rundown observed whenHt31 was applied to hippocampal neurons (Fig. 1A).

Because AKAP79 also binds to PP2B, we hypothesized that the AKAP79-dependent rundown might be attributable to dephosphorylationof GluR1 by anchored PP2B. Inclusion of 10 mM BAPTA in the whole-cellpipette prevented the AKAP79-dependent rundown (Fig. 2D, opensquares, filled circles, filled triangles) (control, 83.4 ± 4.9%,n = 6; AKAP18, 83.8 ± 5.6%, n = 7; AKAP79, 80.6 ± 2.7%, n = 7).Similar concentration-dependent effects were obtained when EGTAwas used to buffer intracellular calcium (AKAP79 plus 1 mM EGTA,66.6 ± 5.7%, n = 7; AKAP79 plus 10 mM EGTA, 85.9 ± 2.4%, n = 6;p < 0.05; data not shown). These data are consistent with calcium-dependentPP2B activity. In addition, the AKAP79-dependent rundown was preventedwhen currents were recorded in the absence of extracellular calcium(Fig. 2E, open squares, filled triangles) (control, 96.4 ± 6.7%,n = 5; AKAP79, 91.7 ± 3.2%, n = 5). This suggests that calciumentry, presumably through homomeric GluR1 receptors, triggersthe AKAP79-dependent rundown. Most importantly, the AKAP79-dependentrundown was blocked by the PP2B inhibitor cyclosporin A (Fig.2F) (control, 88.8 ± 6.4%, n = 6; Ht31, 92.9 ± 2.8%, n = 7). Incontrast, the PP1/PP2A inhibitor okadaic acid did not block theAKAP79-dependent rundown (Fig. 2F) (control, 83.6 ± 2.4%, n =7; Ht31, 65.1 ± 5.5%, n = 10; p < 0.05), although a reductionin the rate of rundown was observed (data not shown). These datasuggest that a pool of PP2B associated with AKAP79 is requiredforrundown.

Regulation of GluR1 receptor currents by AKAP79-anchored PKA

We reasoned that if phosphorylated Ser845 on the AMPA receptor is the substrate for AKAP79-anchored PP2B, then expressionof AKAP79 forms unable to anchor the kinase should blunt the basalphosphorylation of the channel and the concomitant rundown ofGluR1 receptor currents. To test this hypothesis, we used a truncatedanchoring protein, AKAP79(1-360), that lacks the PKA anchoringsite. Coprecipitation experiments confirmed that the RII subunitof PKA was not present in AKAP79(1-360) immunocomplexes, whereasRII was enriched in wild-type AKAP79 immunocomplexes (Fig. 3A).As anticipated, the AKAP79-dependent rundown was absent when AKAP79(1-360)was coexpressed with GluR1 (Fig. 3A) (AKAP79, 60.0 ± 5.3%, n =9; AKAP79(1-360), 87.2 ± 4.6%, n = 5; p < 0.01). Ongoing studiesindicate that the determinants for PP2B and SAP97 binding to AKAP79are contained within the AKAP(1-360) construct (K. L. Dodge, M.Colledge, and J. D. Scott, unpublished observations). Therefore,the absence of rundown observed with AKAP79(1-360) is unlikelyto be attributable to the lack of PP2B or its ability to forma complex with GluR1 but rather attributable to its inabilityto facilitate basal phosphorylation of GluR1. In addition, a moreconservative disruption in the AKAP79-PKA interaction site bysingle proline mutation, which prevents cAMP-dependent phosphorylationof Ser845 (Colledge et al., 2000), also reduces the rundown (datanot shown). Collectively, these data suggest that the presenceof PKA in the complex is a prerequisite for the phenomenon.

View larger version (46K):
[in this window]
[in a new window]
Figure 3. GluR1 is regulated by AKAP79-anchored PKA. A, Top, Extracts from HEK293 cells transfected with AKAP79 and AKAP79(1-360) were immunoprecipitated with antibodies to AKAP79 and blotted with antibodies against the RII subunit. AKAP79(1-360) does not coimmunoprecipitate RII and thus is unlikely to bind PKA inside cells. Bottom, Parallel electrophysiology experiments demonstrate that PKA anchoring is required for the AKAP79-dependent rundown. Ex, Extract; IP, immunoprecipitate; wt, wild type. B, HEK293 cells were transfected with GluR1 alone or with either AKAP18 or AKAP79. Acute application of 8-bromo-cAMP, a cell-permeant cAMP analog, prevents the AKAP79-dependent rundown but does not affect the time course of current responses from control or AKAP18 cells (compare with Fig. 2C). C, The effect of cAMP on GluR1 receptor currents, from cells cotransfected with AKAP79, was blocked by inclusion of the PKA-anchoring inhibitory peptide Ht31 (1 µM) or the specific PKA inhibitory peptide PKI (1 µM) in the whole-cell recording pipette solution. These results indicate that prevention of AKAP79-dependent rundown by 8-bromo-cAMP was attributable to activation of a pool of anchored PKA. AKAP79 plus cAMP data from Figure 3B are shown for comparison.

We further reasoned that if PP2B activity causes channel rundown, then enhanced PKA activation might counteract the phosphataseeffect. Accordingly, application of 8-bromo-cAMP (100 µM), a cell-permeablecAMP analog, prevented the AKAP79-dependent rundown, althoughit had little effect in control or AKAP18-expressing cells (Fig.3B). Furthermore, the AKAP79-dependent rundown was restored inthe presence of 8-bromo-cAMP when Ht31 (1 µM) or PKI (1 µM), aPKA-specific inhibitor, were included within the whole-cell pipettesolution (Fig. 3C) (control, 92.4 ± 5.2, n = 7; Ht31, 65.2 ± 6.2%,n = 5; p < 0.05; PKI, 44.3 ± 5.5%, n = 5; p < 0.01). Under theseconditions, rundown attributable to inhibition of PKA by PKI occurredwith a faster time course and to a greater extent than rundownbecause of displacement of PKA by the Ht31 peptide, as might havebeen anticipated from previous studies (Rosenmund et al., 1994).Collectively, these data indicate that 8-bromo-cAMP preventedthe AKAP79-dependent rundown by activation of a pool of anchoredPKA. Thus, activation of the pool of PKA associated with AKAP79can overcome the action of the targeted pool of PP2B. Importantly,in the presence 8-bromo-cAMP, coexpression of AKAP79 and GluR1is sufficient to produce an Ht31-induced rundown matching thetime course and extent of that observed in neurons. This reconstitutionof neuronal AMPA receptor behavior further suggests that the AKAP79/150signaling complex likely is the endogenous mediator for regulationof hippocampal AMPA receptor currents by PKA andPP2B.

Modulation of GluR1 by AKAP79 occurs at Ser845

Although PP2B inhibition or PKA activation can prevent the AKAP79-dependent rundown, it is not clear whether both enzymesact on the same site. Therefore, phosphorylation site mutantsof GluR1 were used to determine the locus of regulation. Mutationof Ser831 to alanine (S831A) did not affect AKAP79-dependent rundown(Fig. 4A, open squares, filled triangles) (control, 85.0 ± 4.1%,n = 6; AKAP79, 60.7 ± 8.7%, n = 6; p < 0.05), indicating thatthis CaMKII/PKC site is not involved. In contrast, mutation ofSer845 to alanine (S845A) abolished AKAP79-dependent rundown (Fig.4B, open squares, filled triangles) (control, 88.6 ± 2.3%, n =7; AKAP79, 95.6 ± 7.7%, n = 8). Thus, AKAP79-mediated modulationof recombinant GluR1 receptor currents occurs selectively at Ser845,a known PKA site, consistent with the notion that basal phosphorylationof this site is a prerequisite for the rundown.

View larger version (21K):
[in this window]
[in a new window]
Figure 4. AKAP79-dependent regulation of GluR1 receptor currents occurs selectively at Ser845. HEK293 cells were transfected with GluR1 phosphorylation site mutants either alone (control) or with AKAP79. GluR1 receptor currents were evoked as in Figure 2C. A, AKAP79-dependent rundown still occurs when Ser831 is mutated to alanine (S831A), indicating that Ser831 is not involved in the rundown. B, Ser845 is the site of regulation for the AKAP79-dependent rundown because GluR1 receptor currents from an alanine mutant of Ser845 (S845A) do not rundown when cotransfected with AKAP79.

A PDZ interaction at the C terminus of GluR1 is required for regulation by AKAP79

The cytoplasmic tail of GluR1 interacts with a PDZ (postsynaptic density 95/Discs large/zona occludens 1) domain on the MAGUKprotein SAP97 (Leonard et al., 1998). Recently, we demonstratedthat SAP97 also associates with AKAP79, facilitating basal phosphorylationof Ser845 on GluR1 by targeting PKA to GluR1 (Colledge et al.,2000). Thus, we were interested in whether SAP97 might alter theAKAP79-selective rundown. In fact, immunoblot analysis demonstratedthat SAP97 is endogenously expressed in these cells (Fig. 5A).Importantly, both GluR1 and AKAP79 were coimmunoprecipitated withendogenous SAP97 (Fig. 5A), suggesting that a GluR1/SAP97/AKAP79complex is formed in HEK293 cells. To test whether endogenousSAP97 contributes to AKAP79-dependent GluR1 regulation, we useda GluR1-Thr887 to alanine mutant (T887A) that does not interactwith SAP97 (Colledge et al., 2000). Coexpression of AKAP79 didnot cause rundown of these mutant GluR1 receptor currents (Fig.5B, filled squares, filled triangles) (T887A, 86.2 ± 4.5%, n =5; T887A plus AKAP79, 82.7 ± 5.6, n = 5). Thus, a PDZ-domain-mediatedinteraction at the C-terminal tail of GluR1 appears to be requiredfor the AKAP79-dependent modulation of recombinant AMPA receptors.SAP97 is, at present, the only such protein that can interactwith both the C-terminal tail of GluR1 and AKAP79 and is endogenouslyexpressed in HEK293 cells. Therefore, our results are consistentwith the hypothesis that formation of a GluR1/SAP97/AKAP79 complexfacilitates basal phosphorylation of Ser845 and thereby providesa target for the AKAP79-anchored PP2B.

View larger version (25K):
[in this window]
[in a new window]
Figure 5. AKAP79-dependent rundown requires a PDZ-domain interaction at the C terminal of GluR1. A, HEK293 cells were transfected with GluR1 and AKAP79. Extracts were immunoprecipitated with antibodies to SAP97 and blotted for SAP97, AKAP79, and GluR1. Endogenous SAP97 is present in HEK293 cells (top). Transfected GluR1 and AKAP79 are coimmunoprecipitated with the endogenous SAP97, suggesting that a GluR1/SAP97/AKAP79 complex forms during cotransfection of GluR1 and AKAP79. IP, Immunoprecipitating antibody. B, HEK293 cells were transfected with an alanine mutant of Thr887 of GluR1 (T887A) in the presence or absence of AKAP79. Time course of GluR1 receptor currents indicate that a PDZ-domain interaction between GluR1 and endogenous SAP97 is likely required for the AKAP79-dependent rundown because it did not occur with the T887A mutant.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recent advances suggest that multiple cellular processes contribute to long-term modifications of synaptic strength, suchas LTP and LTD. However, the molecular mechanisms responsiblefor their orchestration remain unclear (Malenka and Nicoll, 1999;Sanes and Lichtman, 1999; Luscher et al., 2000). It is well establishedthat kinases and phosphatases are critical in the induction andexpression of synaptic plasticity (Winder and Sweatt, 2001). Indeed,regulation of the phosphorylation state of the AMPA receptor islikely to be one of the earliest events associated with LTP andLTD expression (Malenka and Nicoll, 1999; Luscher et al., 2000;Soderling and Derkach, 2000). Although considerable effort hasfocused on defining the kinases that mediate AMPA receptor phosphorylation,less is known about the phosphatases that catalyze the reversereaction.

Here, we identify PP2B as the predominant phosphatase-opposing modulation of hippocampal AMPA receptors by anchored PKA. Furthermore,we show that expression of the neuronal anchoring protein AKAP79/150,which associates with PKA, PP2B, and SAP97, is sufficient to appropriatelymodulate recombinant GluR1 receptor currents. Our data suggestthat the balance between kinase and phosphatase activity is animportant determinant in the regulation of both native and recombinantAMPA receptor currents. In both systems, PP2B acts in oppositionto anchored PKA. One difference between the two systems is howreadily AMPA receptor downregulation occurs. In hippocampal neurons,which endogenously express AKAP150, AMPA receptors currents arerelatively stable. In contrast, a spontaneous rundown of GluR1receptor currents is observed in HEK293 cells coexpressing AKAP79.This difference can be explained if the native system possessesenhanced PKA activity and/or reduced calcium entry in responseto AMPA receptor activation compared with the HEK293 cell system.Indeed, manipulation of a single variable, the extent of PKA activityby application of 8-bromo-cAMP, is sufficient to adjust the balancebetween kinase and phosphatase activities so that recombinantAMPA receptor currents behave exactly like their native counterparts(compare Figs. 1A, 3C). Because AKAP79/150 is the major AKAP ofthe postsynaptic density (Carr et al., 1992b), our reconstitutionof the protein-protein interactions that are present in neurons,as well as neuronal AMPA receptor behavior, strongly suggeststhat the endogenous AKAP79/150 signaling complex likely servesas the mediator for regulation of hippocampal AMPA receptor currentsby PKA andPP2B.

Our data suggest that AKAP79/150-associated PP2B plays an important role in the regulation of GluR1 currents. However, themechanism by which the phosphatase is activated when bound toAKAP79 has not been fully characterized. In vitro, PP2B activityis reduced to ~25% when bound to the anchoring protein (Coghlanet al., 1995). This low level of AKAP79-associated phosphataseactivity may be sufficient to dephosphorylate Ser845 given thatthe enzyme is precisely targeted to its substrate. Alternatively,the anchoring protein may serve a protective role. By limitingPP2B activity, AKAP79/150 may preclude inappropriate dephosphorylationand downregulation of synaptic AMPA receptors at resting calciumlevels. This latter hypothesis is an attractive mechanism becauseprevious studies have shown that PP2B has an extremely high affinityfor calcium (Klee et al., 1998) and might otherwise be activatedduring basal synaptic transmission. More recently, we showed thatPP2B may be excluded from the complex when AKAP79 is bound bypostsynaptic density-95 (Colledge et al., 2000). Preliminary datasuggests that PP2B may likewise be excluded from the complex whenAKAP79 is bound by SAP97 (S. J. Tavalin, M. Colledge, and J. D.Scott, unpublished observations). However, our functional dataindicate that endogenous PP2B and SAP97 are important for AKAP79-dependentregulation of GluR1. Indeed, both endogenous PP2B and SAP97 arefound to associate with overexpressed AKAP79 in HEK293 cells.Thus, dynamic alterations in the composition of the signalingcomplex may give rise to functionally distinct pools of AKAP79,which contribute to GluR1 regulation. Thus, a variety of controlmechanisms may ensure that only neuronal activity of the appropriateduration, intensity, and/or frequency would activate PP2B sufficientlyto overcome basal PKA activity, resulting in dephosphorylationof Ser845 of the GluR1subunit.

PP2B-mediated regulation of the AMPA receptor may be specific to the hippocampus, because recent studies suggest that PP1is the predominant phosphatase regulating striatal AMPA receptorcurrents (Yan et al., 1999; Feng et al., 2000). These neuronsdisplay a spontaneous rundown of AMPA receptor currents that isprevented by PP1 inhibition, disruption of PP1 targeting, andstimulation of dopamine receptors that are coupled to cAMP production(Yan et al., 1999). Interestingly, the scaffolding protein spinophilinhas been proposed to contribute to PP1-mediated regulation ofstriatal AMPA receptors (Yan et al., 1999; Feng et al., 2000).Thus, different brain regions may use distinct molecular scaffoldsof kinases and phosphatases to regulate AMPAreceptors.

Regulation of native and recombinant AMPA receptor currents by the AKAP79/150 signaling shares several properties with LTD,including calcium dependence, modulation by PP2B and PKA, andregulation of the phosphorylation state of Ser845 (Mulkey andMalenka, 1992; Mulkey et al., 1994; Kameyama et al., 1998; Leeet al., 1998, 2000). In addition, the compartmentalized natureof AKAP79-dependent GluR1 regulation is consistent with a postsynapticand spatially restricted mechanism for LTD generation, a propertythat likely contributes to the input specificity of homosynapticLTD (Kandler et al., 1998; Dodt et al., 1999). Together, our datasuggest that the AKAP79/150 signaling complex may provide a mechanismto enable the calcium-dependent downregulation of these receptorsduringLTD.

Recent evidence suggests that GluR1 interacts with SAP97 predominantly in the biosynthetic and secretory pathway and that,after a limited time after targeting to the plasma membrane, theydissociate from one another (Sans et al., 2001). Because AKAP79/150targets independently to the plasma membrane (Dell'Acqua et al.,1998), we propose that AKAP79-dependent regulation of GluR1 isinitiated by the recruitment of GluR1 by SAP97 to AKAP79/150,resulting in formation of the previously described GluR1/SAP97/AKAP79complex, which favors basal phosphorylation of Ser845 (Colledgeet al., 2000). Once Ser845 is phosphorylated by AKAP79-anchoredPKA, activity-induced elevations in intracellular calcium resultingin activation of AKAP79-anchored PP2B lead to GluR1 downregulation.Although this system may be well poised to respond to local elevationsof calcium, more generalized elevations of intracellular calciumfrom a variety of sources of appropriate magnitude would alsobe expected to activate AKAP79-anchored PP2B. This would satisfythe rather loose calcium signaling requirements for LTD (Cummingset al., 1996) and contribute to the diversity of stimulation protocolsthat can result in AMPA receptor downregulation. Although ourdata suggest that putative calcium-permeable AMPA receptors mayactivate AKAP79/150-anchored PP2B in hippocampal neurons, it mustbe emphasized that this source of calcium is revealed only duringdisruption of PKA anchoring. In contrast, NMDA receptors and voltage-gatedcalcium channels are likely to represent the major physiologicalsources of calcium for AMPA receptor downregulation via AKAP79/150-anchoredPP2B.

A prevailing view suggests that a phosphatase cascade leading to activation of PP1 underlies hippocampal LTD (Mulkey et al.,1993, 1994; Bear and Malenka, 1994; Malenka and Nicoll, 1999).In this model, the role for PP2B is to dephosphorylate the heat-stablephosphatase inhibitor protein inhibitor-1, thereby relieving inhibitionof the PP1 catalytic subunit. PP1 is proposed to be the terminalphosphatase catalyzing reactions leading to LTD. In fact, we didobserve noticeable alterations of the Ht31-induced rundown inneurons after inhibition of PP1/PP2A by okadaic acid. Given thatthe domoate-evoked currents we monitored consisted of both synapticand extrasynaptic AMPA receptors, it is possible that this okadaicacid-sensitive component of rundown represents AKAP79-anchoredPP2B regulation of the synaptic population of AMPA receptors viathe phosphatase cascade model. In contrast, our data does implicatePP2B as directly controlling a substantial fraction of hippocampalAMPA receptor currents independent of PP1 activity. These dataare supported by our experiments in HEK293 cells, which indicatethat AKAP79-anchored PP2B directly regulates Ser845 of GluR1.Thus, our data provide an alternate signaling pathway by whichPP2B may regulate the phosphorylation state of a substrate implicatedin synapticplasticity.

Recent findings support a role for PP1 and PP2B in the activity-dependent endocytosis of AMPA receptors, a process that isalso thought to contribute to LTD (Beattie et al., 2000; Ehlers,2000; Lin et al., 2000; Luscher et al., 2000; Malinow et al.,2000). Interestingly, dephosphorylation of Ser845 appears to precedeAMPA receptors endocytosis in cultured neurons (Ehlers, 2000).As we demonstrated, AKAP79-dependent phosphorylation of Ser845is controlled, in part, by a PDZ-domain interaction between theC-terminal tail of GluR1 and SAP97 (Colledge et al., 2000). Accordingly,disruption of this interaction may lead to net internalizationof GluR1. Consistent with this, a recent study reported that aPDZ-domain interaction with the C-terminal of GluR1 is requiredfor CaMKII-dependent synaptic insertion of recombinant GluR1 receptorsduring LTP (Hayashi et al., 2000). Importantly, the T887A mutantof GluR1 resulted in a net decrease in the AMPA receptor-mediatedEPSC (Hayashi et al., 2000). Thus, it is tempting to speculatethat PKA-dependent phosphorylation of Ser845 via the AKAP79/150signaling complex may be a prerequisite for the postsynaptic insertionof GluR1 during LTP or may be required for retention of newlyincorporated AMPAreceptors.

  FOOTNOTES

Received Dec. 12, 2001; revised Dec. 12, 2001; accepted Jan. 14, 2002.

This work was supported by grants from the Medical Research Council of Canada (M.C.) and National Institutes of Health GrantsNS10202 (S.J.T.), NS35563 (J.W.H), and GM48321 (J.D.S.). We thankAnn Westphal and Jackie Soderling for preparation of the hippocampalcultures and Robert Mouton for preparation of HEK293 cells forbiochemical experiments. We thank Gary Westbrook for criticalreview of this manuscript and Craig Jahr and members of the Scottlaboratory for many criticaldiscussions.

Correspondence should be addressed to John D. Scott, Howard Hughes Medical Institute, Vollum Institute, Oregon Health SciencesUniversity, 3181 S.W. Sam Jackson Park Road, Portland, Oregon97201. E-mail: scott{at}ohsu.edu.

S. J. Tavalin's present address: Department of Pharmacology, University of Tennessee, Health Science Center, Memphis, TN38163.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Banke TG, Bowie D, Lee H, Huganir RL, Schousboe A, Traynelis SF (2000) Control of GluR1 AMPA receptor function by cAMP-dependent protein kinase. J Neurosci 20:89-102[Abstract/Free Full Text].
Barria A, Muller D, Derkach V, Griffith LC, Soderling TR (1997) Regulatory phosphorylation of AMPA-type glutamate receptors by CaM-KII during long-term potentiation. Science 276:2042-2045[Abstract/Free Full Text].
Bear MF, Malenka RC (1994) Synaptic plasticity: LTP and LTD. Curr Opin Neurobiol 4:389-399[Medline].
Beattie EC, Carroll RC, Yu X, Morishita W, Yasuda H, von Zastrow M, Malenka RC (2000) Regulation of AMPA receptor endocytosis by a signaling mechanism shared with LTD. Nat Neurosci 3:1291-1300[ISI][Medline].
Carr DW, Hausken ZE, Fraser ID, Stofko-Hahn RE, Scott JD (1992a) Association of the type II cAMP-dependent protein kinase with a human thyroid RII-anchoring protein. Cloning and characterization of the RII-binding domain. J Biol Chem 267:13376-13382[Abstract/Free Full Text].
Carr DW, Stofko-Hahn RE, Fraser ID, Cone RD, Scott JD (1992b) Localization of the cAMP-dependent protein kinase to the postsynaptic densities by A-kinase anchoring proteins. Characterization of AKAP 79. J Biol Chem 267:16816-16823[Abstract/Free Full Text].
Coghlan VM, Perrino BA, Howard M, Langeberg LK, Hicks JB, Gallatin WM, Scott JD (1995) Association of protein kinase A and protein phosphatase 2B with a common anchoring protein. Science 267:108-111[Abstract/Free Full Text].
Colledge M, Scott JD (1999) AKAPs: from structure to function. Trends Cell Biol 9:216-221[ISI][Medline].
Colledge M, Dean RA, Scott GK, Langeberg LK, Huganir RL, Scott JD (2000) Targeting of PKA to glutamate receptors through a MAGUK-AKAP complex. Neuron 27:107-119[ISI][Medline].
Cummings JA, Mulkey RM, Nicoll RA, Malenka RC (1996) Ca²⁺ signaling requirements for long-term depression in the hippocampus. Neuron 16:825-833[ISI][Medline].
Dell'Acqua ML, Faux MC, Thorburn J, Thorburn A, Scott JD (1998) Membrane-targeting sequences on AKAP79 bind phosphatidylinositol-4, 5-bisphosphate. EMBO J 17:2246-2260[ISI][Medline].
Dodt H, Eder M, Frick A, Zieglgansberger W (1999) Precisely localized LTD in the neocortex revealed by infrared-guided laser stimulation. Science 286:110-113[Abstract/Free Full Text].
Ehlers MD (2000) Reinsertion or degradation of AMPA receptors determined by activity-dependent endocytic sorting. Neuron 28:511-525[ISI][Medline].
Feng J, Yan Z, Ferreira A, Tomizawa K, Liauw JA, Zhuo M, Allen PB, Ouimet CC, Greengard P (2000) Spinophilin regulates the formation and function of dendritic spines. Proc Natl Acad Sci USA 97:9287-9292[Abstract/Free Full Text].
Fraser ID, Tavalin SJ, Lester LB, Langeberg LK, Westphal AM, Dean RA, Marrion NV, Scott JD (1998) A novel lipid-anchored A-kinase anchoring protein facilitates cAMP-responsive membrane events. EMBO J 17:2261-2272[ISI][Medline].
Gray PC, Johnson BD, Westenbroek RE, Hays LG, Yates JR, Scheuer 3rd T, Catterall WA, Murphy BJ (1998) Primary structure and function of an A kinase anchoring protein associated with calcium channels. Neuron 20:1017-1026[ISI][Medline].
Hayashi Y, Shi SH, Esteban JA, Piccini A, Poncer JC, Malinow R (2000) Driving AMPA receptors into synapses by LTP and CaMKII: requirement for GluR1 and PDZ domain interaction. Science 287:2262-2267[Abstract/Free Full Text].
Kameyama K, Lee HK, Bear MF, Huganir RL (1998) Involvement of a postsynaptic protein kinase A substrate in the expression of homosynaptic long-term depression. Neuron 21:1163-1175[ISI][Medline].
Kandler K, Katz LC, Kauer JA (1998) Focal photolysis of caged glutamate produces long-term depression of hippocampal glutamate receptors. Nat Neurosci 1:119-123[ISI][Medline].
Klauck TM, Faux MC, Labudda K, Langeberg LK, Jaken S, Scott JD (1996) Coordination of three signaling enzymes by AKAP79, a mammalian scaffold protein. Science 271:1589-1592[Abstract].
Klee CB, Ren H, Wang X (1998) Regulation of the calmodulin-stimulated protein phosphatase, calcineurin. J Biol Chem 273:13367-13370[Free Full Text].
Lee HK, Kameyama K, Huganir RL, Bear MF (1998) NMDA induces long-term synaptic depression and dephosphorylation of the GluR1 subunit of AMPA receptors in hippocampus. Neuron 21:1151-1162[ISI][Medline].
Lee HK, Barbarosie M, Kameyama K, Bear MF, Huganir RL (2000) Regulation of distinct AMPA receptor phosphorylation sites during bidirectional synaptic plasticity. Nature 405:955-959[Medline].
Leonard AS, Davare MA, Horne MC, Garner CC, Hell JW (1998) SAP97 is associated with the alpha-amino-3-hydroxy-5-methylisoxazole-4-propionic acid receptor GluR1 subunit. J Biol Chem 273:19518-19524[Abstract/Free Full Text].
Lin JW, Ju W, Foster K, Lee SH, Ahmadian G, Wyszynski M, Wang YT, Sheng M (2000) Distinct molecular mechanisms and divergent endocytotic pathways of AMPA receptor internalization. Nat Neurosci 3:1282-1290[ISI][Medline].
Luscher C, Nicoll RA, Malenka RC, Muller D (2000) Synaptic plasticity and dynamic modulation of the postsynaptic membrane. Nat Neurosci 3:545-550[ISI][Medline].
Malenka RC, Nicoll RA (1999) Long-term potentiation $---$ a decade of progress? Science 285:1870-1874[Abstract/Free Full Text].
Malinow R, Mainen ZF, Hayashi Y (2000) LTP mechanisms: from silence to four-lane traffic. Curr Opin Neurobiol 10:352-357[ISI][Medline].
Mammen AL, Kameyama K, Roche KW, Huganir RL (1997) Phosphorylation of the alpha-amino-3-hydroxy-5-methylisoxazole4-propionic acid receptor GluR1 subunit by calcium/calmodulin-dependent kinase II. J Biol Chem 272:32528-32533[Abstract/Free Full Text].
Mulkey RM, Malenka RC (1992) Mechanisms underlying induction of homosynaptic long-term depression in area CA1 of the hippocampus. Neuron 9:967-975[ISI][Medline].
Mulkey RM, Herron CE, Malenka RC (1993) An essential role for protein phosphatases in hippocampal long-term depression. Science 261:1051-1055[Abstract/Free Full Text].
Mulkey RM, Endo S, Shenolikar S, Malenka RC (1994) Involvement of a calcineurin/inhibitor-1 phosphatase cascade in hippocampal long-term depression. Nature 369:486-488[Medline].
Roche KW, O'Brien RJ, Mammen AL, Bernhardt J, Huganir RL (1996) Characterization of multiple phosphorylation sites on the AMPA receptor GluR1 subunit. Neuron 16:1179-1188[ISI][Medline].
Rosenmund C, Carr DW, Bergeson SE, Nilaver G, Scott JD, Westbrook GL (1994) Anchoring of protein kinase A is required for modulation of AMPA/kainate receptors on hippocampal neurons. Nature 368:853-856[Medline].
Sanes JR, Lichtman JW (1999) Can molecules explain long-term potentiation? Nat Neurosci 2:597-604[ISI][Medline].
Sans N, Racca C, Petralia RS, Wang YX, McCallum J, Wenthold RJ (2001) Synapse-associated protein 97 selectively associates with a subset of AMPA receptors early in their biosynthetic pathway. J Neurosci 21:7506-7516[Abstract/Free Full Text].
Sik A, Gulacsi A, Lai Y, Doyle WK, Pacia S, Mody I, Freund TF (2000) Localization of the A kinase anchoring protein AKAP79 in the human hippocampus. Eur J Neurosci 12:1155-1164[Medline].
Soderling TR, Derkach VA (2000) Postsynaptic protein phosphorylation and LTP. Trends Neurosci 23:75-80[ISI][Medline].
Valtschanoff JG, Burette A, Davare MA, Leonard AS, Hell JW, Weinberg RJ (2000) SAP97 concentrates at the postsynaptic density in cerebral cortex. Eur J Neurosci 12:3605-3614[ISI][Medline].
Winder DG, Sweatt JD (2001) Roles of serine/threonine phosphatases in hippocampal synaptic plasticity. Nat Rev Neurosci 2:461-474[ISI][Medline].
Yan Z, Hsieh-Wilson L, Feng J, Tomizawa K, Allen PB, Fienberg AA, Nairn AC, Greengard P (1999) Protein phosphatase 1 modulation of neostriatal AMPA channels: regulation by DARPP-32 and spinophilin. Nat Neurosci 2:13-17[ISI][Medline].

Copyright © 2002 Society for Neuroscience 0270-6474/02/2283044-08$05.00/0

This article has been cited by other articles:

Y. Lu, M. Zhang, I. A. Lim, D. D. Hall, M. Allen, Y. Medvedeva, G. S. McKnight, Y. M. Usachev, and J. W. Hell
AKAP150-anchored PKA activity is important for LTD during its induction phase
J. Physiol., September 1, 2008; 586(17): 4155 - 4164.
[Abstract] [Full Text] [PDF]

B. J. Tunquist, N. Hoshi, E. S. Guire, F. Zhang, K. Mullendorff, L. K. Langeberg, J. Raber, and J. D. Scott
Loss of AKAP150 perturbs distinct neuronal processes in mice
PNAS, August 26, 2008; 105(34): 12557 - 12562.
[Abstract] [Full Text] [PDF]

K. Schnizler, L. P. Shutov, M. J. Van Kanegan, M. A. Merrill, B. Nichols, G. S. McKnight, S. Strack, J. W. Hell, and Y. M. Usachev
Protein Kinase A Anchoring via AKAP150 Is Essential for TRPV1 Modulation by Forskolin and Prostaglandin E2 in Mouse Sensory Neurons
J. Neurosci., May 7, 2008; 28(19): 4904 - 4917.
[Abstract] [Full Text] [PDF]

M. Haines, L. M. Mao, L. Yang, A. Arora, E. E. Fibuch, and J. Q. Wang
Modulation of AMPA receptor GluR1 subunit phosphorylation in neurons by the intravenous anaesthetic propofol
Br. J. Anaesth., May 1, 2008; 100(5): 676 - 682.
[Abstract] [Full Text] [PDF]

S. J. Tavalin
AKAP79 Selectively Enhances Protein Kinase C Regulation of GluR1 at a Ca2+-Calmodulin-dependent Protein Kinase II/Protein Kinase C Site
J. Biol. Chem., April 25, 2008; 283(17): 11445 - 11452.
[Abstract] [Full Text] [PDF]

T. Nie, C. B. McDonough, T. Huang, P. V. Nguyen, and T. Abel
Genetic Disruption of Protein Kinase A Anchoring Reveals a Role for Compartmentalized Kinase Signaling in Theta-Burst Long-Term Potentiation and Spatial Memory
J. Neurosci., September 19, 2007; 27(38): 10278 - 10288.
[Abstract] [Full Text] [PDF]

E. A. Horne and M. L. Dell'Acqua
Phospholipase C Is Required for Changes in Postsynaptic Structure and Function Associated with NMDA Receptor-Dependent Long-Term Depression
J. Neurosci., March 28, 2007; 27(13): 3523 - 3534.
[Abstract] [Full Text] [PDF]

L. A. Gardner, S. J. Tavalin, A. S. Goehring, J. D. Scott, and S. W. Bahouth
AKAP79-mediated Targeting of the Cyclic AMP