Regulation of AMPA Receptor GluR1 Subunit Surface Expression by a 4.1N-Linked Actin Cytoskeletal Association

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The Journal of Neuroscience, November 1, 2000, 20(21):7932-7940

Regulation of AMPA Receptor GluR1 Subunit Surface Expression by a 4.1N-Linked Actin Cytoskeletal Association
Lei Shen, Feng Liang, Loren D. Walensky, and Richard L. Huganir
Howard Hughes Medical Institute, Department of Neuroscience, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21205

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The synaptic localization, clustering, and immobilization of neurotransmitter receptors and ion channels play important rolesin synapse formation and synaptic transmission. Although severalproteins have been identified that interact with AMPA receptorsand that may regulate their synaptic targeting, little is knownabout the interaction of AMPA receptors with the cytoskeleton.In studies examining the interaction of the AMPA receptor GluR1subunit with neuronal proteins, we determined that GluR1 interactswith the 4.1G and 4.1N proteins, homologs of the erythrocyte membranecytoskeletal protein 4.1. Using the yeast two-hybrid system anda heterologous cell system, we demonstrated that both 4.1G and4.1N bind to a membrane proximal region of the GluR1 C terminus,and that a region within the C-terminal domain of 4.1G or 4.1Nis sufficient to mediate the interaction. We also found that 4.1Ncan associate with GluR1 in vivo and colocalizes with AMPA receptorsat excitatory synapses. Disruption of the interaction of GluR1with 4.1N or disruption of actin filaments decreased the surfaceexpression of GluR1 in heterologous cells. Moreover, disruptionof actin filaments in cultured cortical neurons dramatically reducedthe level of surface AMPA receptors. These results suggest thatprotein 4.1N may link AMPA receptors to the actincytoskeleton.

Key words: GluR1; protein 4.1; cytoskeleton; synaptic; AMPA receptor; yeast two-hybrid

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Glutamate is the major excitatory neurotransmitter in the CNS. Glutamate receptors consist of three subclasses, namely AMPA,kainate, and NMDA receptors, based on their physiological andpharmacological properties (Hollmann and Heinemann, 1994). Thesereceptors are heteromeric complexes of homologous subunits, whichcombine to form a variety of receptor subtypes. The synaptic targeting,clustering, and immobilization of glutamate receptors are crucialfor efficient excitatory synaptic transmission. Recent studieshave identified a variety of proteins that may play a role inthe aggregation and immobilization of neurotransmitter receptors(Sheng and Kim, 1996; Kim and Huganir, 1999). For example, thePSD95/DIg/Z0-1 (PDZ) domain containing-protein postsynaptic density95 (PSD-95)/synapse-associated protein 90 (SAP90) and its familymembers SAP102 and PSD-93/Chapsyn-110 have been shown to physicallyassociate with the C termini of the NMDA receptor subunits andmay be involved in the synaptic localization of NMDA receptors(Sheng and Kim, 1996; Kornau et al., 1997; O'Brien et al., 1998a).Genetic studies in Drosophila have revealed that the discs-large(DLG) protein, a PSD-95 related protein, is essential for thesynaptic clustering of Shaker-type K⁺ channels (Tejedor et al., 1997). The C termini of the AMPA receptorshave also been shown to interact with several PDZ domain-containingproteins such as glutamate receptor interacting protein (GRIP)/AMPAbinding protein (ABP) (Dong et al., 1997; Srivastava et al., 1998),protein interacting with C-kinase (PICK1) (Xia et al., 1999),and SAP97 (Leonard et al., 1998) via their C-terminal T/SXV motifs.These interactions are thought to be important for the sortingand synaptic expression of thesereceptors.

The actin cytoskeleton has also been found to be critical for the immobilization of these receptors (Allison et al., 1998;Kim and Lisman, 1999). Recent studies in hippocampal neurons inculture have shown that disruption of F-actin decreased the numberof clusters of NMDA and AMPA receptors on dendritic spines, suggestingthe immobilization of these receptors depends on the integrityof the F-actin network (Allison et al., 1998). This observationwas further supported by electrophysiological studies (Kim andLisman, 1999; Krucker et al., 2000), which indicated that dynamicactin filaments are important for basal synaptic transmissionas well as induction and maintenance of long-term potentiation.In addition, several cytoskeletal proteins have been shown toassociate with NMDA receptors. $alpha$ -Actinin-2, a member of the spectrin-dystrophinfamily of actin-binding proteins, binds to the C termini of boththe NR1 and NR2B subunits of the NMDA receptor (Wyszynski et al.,1997). The neurofilament light chain and Yotiao, a novel cytoskeletalprotein with a coiled-coil structure, have also been found tointeract with the C terminus of the NR1 subunit (Ehlers et al.,1998; Lin et al., 1998). However, the direct or indirect interactionof cytoskeletal proteins with AMPA receptors has not been reported.Here we used the yeast two-hybrid system to identify that proteins4.1G and 4.1N, homologs of the erythrocyte membrane cytoskeletalprotein 4.1, can interact with the GluR1 subunit of the AMPA receptor.Protein 4.1, originally identified in red blood cells and calledred blood cell protein 4.1 (4.1R), is critical for the organizationand maintenance of the spectrin-actin cytoskeleton and for theattachment of the cytoskeleton to the cell membrane through interactionwith integral membrane proteins such as glycophorin C and Band3 (Tyler et al., 1979; Anderson and Lovrien, 1984; Pasternacket al., 1985). The erythrocyte 4.1R has a 30 kDa N-terminal domainthat interacts with glycophorin C, calmodulin, and p55 (Tanakaet al., 1991; Hemming et al., 1994; Marfatia et al., 1994, 1995),a 16 kDa domain critical for membrane association, a 10 kDa domaincontaining the binding site for spectrin and actin complexes,and a 22-24 kDa C-terminal domain (CTD) whose function is forthe most part unknown. 4.1G is ubiquitously expressed in cells,whereas 4.1N is enriched in neurons (Walensky et al., 1999). Both4.1G and 4.1N share homology to 4.1R at the 10, 16, and 22-24kDa domains but are distinct at their N-terminal domains. Ourresults show that both 4.1G and 4.1N bind to a membrane proximalregion in the C terminus of GluR1, and a consensus region withinthe CTDs of 4.1G and 4.1N is sufficient to mediate the binding.Protein 4.1N also associates with GluR1 in vivo and colocalizeswith AMPA receptors in excitatory synapses. Moreover, we foundthat GluR1 truncation mutants lacking the membrane proximal regioncapable of 4.1 binding have decreased plasma membrane expression.Overexpression of the CTDs of 4.1 or disruption of the F-actionnetwork also resulted in reduced GluR1 surface expression. Thesedata suggest that protein 4.1G and 4.1N may serve to cross-linkAMPA receptors to the actin cytoskeleton at excitatorysynapses.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Yeast two-hybrid screening and interaction assay. The cDNA corresponding to the C-terminal tail (the last 82 amino acids,8.5 kDa) of rat GluR1 was amplified by PCR and subcloned in-frameinto the SalI-BglII site of the pPC97 yeast vector containingthe GAL4 DNA-binding domain (Chevray and Nathans, 1992). Thisbait plasmid was then transformed into yeast strain PJ69-4A (Jameset al., 1996). Yeast two-hybrid screening (Fields and Song, 1989)was performed using a random-primed cDNA library from rat hippocampus(Dong et al., 1997) subcloned into the SalI-NotI site of the pPC86vector containing the GAL4 activation domain (Chevray and Nathans,1992). Positive clones were selected on plates lacking leucine,tryptophan, and adenine and confirmed by growth on quadruple minusplates (Leu $-$ , Trp $-$ , Ade $-$ , and His $-$ ) with 2 mM 3-aminotriazoleand by liquid assay for $beta$ -galactosidase activity (Reynolds andLundblad, 1989).

The yeast two-hybrid system was also used to investigate the interaction between protein 4.1G and GluR1. The C-terminal domainof GluR1 with various truncations was subcloned into the pPC97vector, and the CTD of rat 4.1G (see Fig. 4B) was subcloned intothe pPC86 vector. Combinations of these constructs (one in pPC97and the other in pPC86) were co-transformed into PJ69-4A yeastcells and selected on Leu $-$ and Trp $-$ plates for double transformants,which were further plated on quadruple minus plates (Leu $-$ , Trp $-$ ,Ade $-$ , and His $-$ ) with 2 mM 3-aminotriazole to test for interaction.Any interaction detected was also confirmed by liquid assay for $beta$ -galactosidase activity. Vector pPC97 or pPC86 with no insertwas used in controlexperiments.

Cell cultures and transfection. HEK 293T cells and COS cells were maintained in minimal essential medium (MEM; Life Technologies,Gaithersburg, MD) with 10% fetal bovine serum (Life Technologies)and 0.5% L-glutamine. The cDNA of the full-length rat GluR1 orits various mutants or the full-length protein 4.1N was subclonedinto the mammalian expression vector pRK5. cDNAs were also subclonedinto the mammalian expression vector pRK5 bearing a myc or hemagglutinintag upstream of the cloning site where indicated. Five to 10 µgof each cDNA were used to transfect HEK 293T cells, and additionalpRK5 vector DNA was added when necessary to equalize the totalamount of DNA transfected. Transfection was done by calcium phosphatecoprecipitation, as described (Blackstone et al., 1992a). After36-48 hr, the cells were harvested and solubilized in immunoprecipitationbuffer (in mM: 5 EDTA, 5 EGTA, 1 Na₃VO₄, 10 Na pyrophosphate,and 50 NaF in PBS, pH 7.4) with 1% Triton X-100 at 4°C for 1 hr.Cell lysates were centrifuged at 100,000 × g for 10 min at 4°C,and the supernatant was either immediately used for immunoprecipitationor stored at $-$ 80°C.

Neuronal cultures. Low-density hippocampal neurons were cultured following the standard procedure described by Goslin andBanker (1991). Sprague Dawley rats of embryonic day 17 were usedto culture cortical neurons as described with minor modification(Ghosh and Greenberg, 1995). Cells were maintained in MEM supplementedwith 5% heat-inactivated horseserum.

Preparation of P2 fraction from brain tissue. Brain tissue from male Sprague Dawley rats, 4-6 weeks old, was homogenized in10 volumes of buffered sucrose (0.32 M sucrose in 4 mM HEPES,pH 7.4, with protease inhibitors antipain, chymotrypsin, leupeptin,and Trasylol, and 0.1 mM PMSF) in a glass-Teflon homogenizer.The homogenate was centrifuged at 800 × g for 10 min, the supernatantwas then subjected to another centrifugation at 9000 × g for 15min. The supernatant from the second centrifugation, the crudesynaptosomal fraction (P2), was either immediately used for immunoprecipitationor stored at $-$ 80°C. For immunoprecipitation, the P2 fraction wasfirst solubilized in 1% sodium deoxycholate at 36°C for 30 min,followed by adding 0.1 volume of 1% Triton X-100 in 50 mM Tris-Cl,pH 9.0, and the preparation was centrifuged for 10 min at 100,000× g (Luo et al., 1997). The supernatant was then used forimmunoprecipitation.

Deletion mutagenesis of GluR1. Deletion mutants of GluR1 were generated by PCR-based site-directed mutagenesis (Quick Change;Stratagene, La Jolla, CA) according to the instructions of themanufacturer. Throughout this paper, unless otherwise specified,R1*875, R1*823, R1*812, and R1*807 were C-terminal deletions fromamino acids 875, 823, 812, and 807, respectively as numbered byHollmann et al. (1989), in which the first amino acid starts afterthe signal peptide sequence. Deletion constructs were confirmedby sequencing, and the expression of the mutants was verifiedby Westernblot.

Coimmunoprecipitation and immunoblotting. Immunoprecipitation was performed as previously described (Lau et al., 1996; Luoet al., 1997) with modifications. For each reaction, ~250 µg ofsolubilized HEK 293T cell lysate or solubilized rat brain P2 preparationwas first incubated with 25 µl of 1:1 slurry of protein A/SepharoseCL-4B (Amersham Pharmacia Biotech, Arlington Heights, IL; preparedin PBS, pH 7.4) at 4°C for 1 hr to clarify any nonspecific bindingto protein A from the lysate. At the same time, 5-10 µg of affinity-purifiedpolyclonal antibodies, 1 µl of unpurified rabbit serum containingspecific polyclonal antibodies, or 1 µl of mouse ascites containingspecific monoclonal antibodies was preincubated with 25 µl of1:1 slurry of protein A/Sepharose for 1 hr, and the protein A-antibodycomplex was spun down at 3000 rpm for 2 min. The clarified supernatantsof the lysates were then added to the antibody-bound protein Abeads, and the mixture was incubated for 2 hr at 4°C. After immunoprecipitation,the complex was spun down and washed once with 1% Triton X-100in immunoprecipitation buffer (IPB), once with 1% Triton X-100in IPB containing additional 0.5 M NaCl, and finally once withIPB. The proteins were eluted by Laemmli sample buffer (Laemmli,1970) and were separated by SDS-PAGE. The gels were transferredto a polyvinylidene difluoride (PVDF) membrane (Millipore, Bedford,MA), and the membranes were immunoblotted as described previously(Lau et al., 1996). Control coimmunoprecipitation reactions wereperformed by using preimmune serum or by preabsorption of theantibodies with their immunogenic peptide at a concentration of50 µg/ml. The antibodies used in the experiments have been previouslydescribed: anti-GluR1 C-terminal antibody (Blackstone et al.,1992b), anti-GluR1 N-terminal antibody (Mammen et al., 1997a),and anti-4.1N antibody (Walensky et al., 1999). All coimmunoprecipitationswere performed at least three times with similarresults.

Cell surface biotinylation. COS cells were used in cell surface biotinylation analyses. Twenty-four hours after transfection,cells were biotinylated with 1 mg/ml sulfo-NHS-S-S-biotin (Pierce,Rockford, IL) for 20 min at 4°C, using previously described methodswith minor modifications (Mammen et al., 1997b). To precipitatebiotinylated proteins, supernatants of cell lysate were mixedwith UltraLink immobilized neutravidin beads (Pierce) and rotatedfor 2 hr at 4°C. The beads were washed five times with IPB andthen eluted with SDS-PAGE sample buffer supplemented with 50 mMDTT for 1 hr at 37°C. Protein biotinylation was efficiently reversedby DTT in this procedure. Both total and biotinylated proteinswere resolved by SDS-PAGE, transferred to PVDF membranes, andprobed with an anti-GluR1 N-terminal antibody. Alkaline phosphatase-conjugatedanti-rabbit IgG (Pierce) was used as secondary antibody to visualizethe specific signals by chemifluorescence (ECF) substrate (AmershamPharmacia Biotech). The membranes were dried between filter papersand scanned in Storm 860 (Molecular Dynamics, Sunnyvale, CA) at700-900 V. The scanned digital images were quantitated using ImageQuantsoftware (Molecular Dynamics). The amount of GluR1 surface expressionwas analyzed by determining the relative ratio of biotinylatedGluR1 to total GluR1. By checking the ratio of the control samplesloaded at different concentrations, we found that the ECF methodgave a better linear signal than conventional chemiluminescence(ECL)detection.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of interaction between GluR1 and protein 4.1G using the yeast two-hybrid system

To identify proteins interacting with the cytosolic tail of GluR1, the last 82 amino acids of GluR1 were used as bait in ayeast two-hybrid screen against a randomly primed rat brain hippocampalcDNA library. Among 100 million independent colonies screened,only 9 positive clones were isolated, which were all homologousto the erythrocyte cytoskeletal protein 4.1R. The amino acid sequenceof four of the clones were identical to the CTD of protein 4.1G,a novel homolog of erythrocyte protein 4.1 (Walensky et al., 1998).The other five positive clones were also homologous to the CTDof protein 4.1, but no identical match with any cloned memberof the protein 4.1 family of proteins was found. On the basisof sequence homology, these positives could be splice variantsor homologs of protein 4.1G.

To map the interaction site on GluR1, we used the yeast two-hybrid interaction assay and serial deletions of GluR1 C terminus.As shown in Figure 1, deleting the PDZ domain ligand containedin the last 10 amino acids of GluR1 did not abolish its interactionwith protein 4.1G. Deletion constructs of GluR1 up to amino acid823 of GluR1 still interacted with protein 4.1G, whereas deletionafter amino acid 812 abolished the interaction (Fig. 1). Controlexperiments using a vector that only expresses the GAL4 DNA bindingdomain did not interact (Fig. 1). These results suggest that themembrane proximal region between amino acids 812 and 823 in theC terminus of GluR1 is important for the interaction with protein4.1G.

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Figure 1. Yeast two-hybrid analysis of GluR1 and protein 4.1G interaction. The cytosolic tail of GluR1 and its various deletions were subcloned into yeast vector pPC97 containing the GAL4 DNA binding domain. The CTD of protein 4.1G was subcloned into pPC86 containing the GAL4 activation domain and co-transformed with GluR1 constructs into yeast. Double transformants were selected and scored for growth on plates lacking leucine, tryptophan, adenine, and histidine and for lacZ activity. Those that tested positive for interaction are designated +; those that tested negative are designated $-$ .

Association of GluR1 with protein 4.1N and 4.1G in transfected HEK 293T cells

To confirm that GluR1 interacts with 4.1G, we examined whether they formed a complex in transfected HEK 293T cells. HEK 293Tcells were transiently transfected with a construct encoding thefull-length GluR1 with and without a construct encoding the CTDof protein 4.1G (4.1GCTD). After 2 d the cells were harvestedand solubilized with 1% Triton X-100, and the cell lysates weresubjected to immunoprecipitation using an anti-GluR1 antibody.As shown in Figure 2A, immunoprecipitation of protein 4.1GCTDfrom co-transfected 293T cell lysates resulted in the specificco-immunoprecipitation of GluR1 (lane 3). The recent isolationof protein 4.1N (Walensky et al., 1999), a novel neuronal homologof protein 4.1 highly related to 4.1G, and identification of itsassociation with the postsynaptic density and localization atdendritic spines (Walensky et al., 1999) raise the possibilitythat GluR1 may also interact with 4.1N. Co-immunoprecipitationexperiments from HEK293 cells transfected with GluR1 and 4.1Nshowed that, similar to 4.1G, 4.1N associates with GluR1 in thissystem (Fig. 2B).

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Figure 2. Association of GluR1 with 4.1G and 4.1N in HEK 293T cells. A. Coimmunoprecipitation of 4.1GCTD with GluR1 from 293T cells. Full-length GluR1 and myc-tagged 4.1GCTD were transfected into 293T cells either individually (lanes 1, 2) or together (lane 3). The transfected cells were solubilized with 1% Triton X-100, and the solubilized cell lysates were immunoprecipitated with anti-myc antibody. The immunoprecipitates were resolved on SDS-PAGE followed by immunoblotting with anti-GluR1 C-terminal antibody (top panel). The presence of myc-tagged 4.1GCTD (middle panel) and GluR1 (bottom panel) in the input for immunoprecipitation was confirmed by immunoblotting with anti-myc and anti-GluR1 C-terminal antibodies, respectively. IP, Immunoprecipitation; IB, immunoblot; same for other legends. B, Coimmunoprecipitation of 4.1N with GluR1 from 293T cells. Full-length GluR1 and full-length 4.1N were transfected into 293T cells either individually (lanes 1, 2) or combined (lanes 3, 4). The immunoprecipitation from cell lysates is the same as in A, except here the anti-GluR1 C-terminal antibody is used. The immunoprecipitates were resolved on SDS-PAGE and probed with anti-4.1N antibody (top panel). As a control experiment in lane 4, the anti-GluR1 C-terminal antibody was preincubated with its specific antigen before immunoprecipitation (see Materials and Methods). The presence of 4.1N (middle panel) and GluR1 (bottom panel) in the input for immunoprecipitation was confirmed by Western blot using anti-4.1N and anti-GluR1 antibodies, respectively.

To confirm the yeast two-hybrid data that indicated that the membrane proximal region between amino acids 812 and 823 in theGluR1 C terminus is important for interaction, we generated C-terminaldeletion mutants of GluR1 and tested their ability to associatewith protein 4.1G/4.1N in transfected HEK 293T cells. Deletionof the C terminus of GluR1 after amino acid 823 (R1*823) did notdisrupt its coimmunoprecipitation with 4.1G (Fig. 3B) or 4.1N(data not shown), whereas deletion of GluR1 at amino acid 812(R1*812) or 807 (R1*807) eliminated the co-immunoprecipitationwith both 4.1G (Fig. 3B) and 4.1N (data not shown). These resultsagree with the yeast two-hybrid analysis and provide additionalevidence that the membrane proximal region from amino acid 812to 823 is important for the binding of GluR1 to 4.1G and N.

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Figure 3. Requirement of a membrane proximal region for association of GluR1 with proteins 4.1G and 4.1N. A, Schematic diagram of GluR1 deletion constructs used in B. B, The membrane proximal region in the GluR1 C terminus is required for binding to protein 4.1G. Full-length and C-terminal deletions of GluR1 were transfected with 4.1GCTD, and then solubilized cell lysates were immunoprecipitated with anti-myc antibody. The immunoprecipitates were subjected to SDS-PAGE and Western blot with anti-GluR1 N-terminal antibody (top panel). The presence of myc-tagged 4.1GCTD (middle panel) and GluR1 and its deletions (bottom panel) in the input for immunoprecipitation was confirmed by Western blot using anti-myc and anti-GluR1 N-terminal antibodies, respectively.

The CTDs of protein 4.1G and 4.1N contain a highly conserved C-terminal region and a variable N-terminal region (Fig. 4B).To test whether this conserved region is responsible for the interactionwith GluR1, we generated constructs containing the variable andconserved regions of 4.1NCTD (Fig. 4B, 4.1NCTDv, 4.1NCTDc) andtested their interaction with GluR1 in 293T cells. As shown inFigure 4C, the conserved but not the variable region of 4.1NCTDinteracted with GluR1 (lanes 4, 2, respectively). Similar resultswere obtained for 4.1GCTD (data not shown).

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Figure 4. A consensus region within 4.1N is sufficient for interaction with GluR1. A, Schematic diagram of domain structures of 4.1N and 4.1G. The two proteins have significant homology at the membrane association domain, spectrin-actin binding domain, and CTD but have little homology at the N-terminal domain. B, Sequence alignment of CTDs of 4.1N and 4.1G. Identical amino acid residues are boxed and darkly shaded; conserved residues are boxed and lightly shaded. The alignment shows that CTDs of the two proteins contain a variable N-terminal region (4.1NCTDv) and a highly conserved C-terminal region (4.1NCTDc). C, Association of the consensus region of 4.1NCTD with GluR1. A myc-tagged variable region (myc-4.1NCTDv; lanes 1, 2) or consensus region (myc-4.1NCTDc; lanes 3, 4) of 4.1NCTD or the entire 4.1NCTD (myc-4.1NCTD; lanes 5, 6) was co-transfected with vector (lanes 1, 3, 5) or with GluR1 (lanes 2, 4, 6) into 293T cells. Immunoprecipitations were performed on solubilized cell lysates using anti-myc antibody followed by SDS-PAGE and immunoblotting with anti-GluR1 antibody (top panel). The presence of GluR1 (middle panel) and myc-tagged proteins (bottom panel) in the input for immunoprecipitation was confirmed by Western blot using anti-GluR1 C-terminal and anti-myc antibodies, respectively.

Protein 4.1N associates with AMPA receptors in vivo and colocalizes with AMPA receptors in excitatory synapses

To see whether AMPA receptors can associate with 4.1N in vivo, we performed coimmunoprecipitation experiments from brain lysates.Briefly, rat brain membrane preparations were solubilized with1% deoxycholate, and then the AMPA receptors were immunoprecipitatedwith an antibody against the N terminus of the GluR2 subunit.GluR1 antibodies were not used in this experiment, because theanti-N-terminal GluR2 antibody gives more efficient immunoprecipitationof AMPA receptors in these extracts. As shown in Figure 5A, protein4.1N specifically co-immunoprecipitated with the AMPA receptorcomplex. Preabsorption of the antibody with antigen before theimmunoprecipitation abolished the coimmunoprecipitation (Fig.5A, lane 3), and PSD-95, a protein known to associate with NMDAreceptors, did not coimmunoprecipitate. We were unable to performcoimmunoprecipitation experiments to examine for the associationof 4.1G and GluR1 from brain membrane preparations, because wedo not have a specific anti-4.1G antibody.

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Figure 5. Protein 4.1N interacts with GluR1 in vivo and colocalizes with AMPA receptor complex in excitatory synapses. A, Rat brain membrane preparation (P2) was solubilized with 1% deoxycholate and immunoprecipitated with either anti-GluR2 N-terminal antibody (lane 2) or the same antibody with antigen preabsorption (lane 3). The immunoprecipitated complex and the input (lane 1) were resolved by SDS-PAGE and probed with anti-4.1N (top panel), anti-GluR1 C-terminal (upper middle panel), anti-GluR2 C-terminal (lower middle panel), and PSD-95 (bottom panel) antibodies. B, Primary hippocampal neurons were double-stained with monoclonal anti-GluR2 antibody (Chemicon, Temecula, CA) and polyclonal anti-4.1N antibody as primary antibodies, followed by rhodamine-conjugated anti-mouse IgG and FITC-conjugated anti-rabbit IgG as secondary antibodies. The staining was visualized and digitized using a fluorescent microscope (Zeiss, Thornwood, NY) with a digital camera controlled by the Metamorph program (Universal Imaging, West Chester, PA). Arrows and arrowheads indicate the area of colocalization.

Previous studies have shown that 4.1N can be detected in PSD fractions and is localized at excitatory synapses (Walensky etal., 1999). We therefore investigated whether 4.1N colocalizedwith AMPA receptors in neurons. Figure 5B shows the staining ofprimary hippocampal neuronal cultures using an anti-GluR2 antibodyto label AMPA receptors and an anti-4.1N antibody. The dendriticstaining pattern of 4.1N is reminiscent of cytoskeleton structureand is enriched in a number of dendritic spines that colocalizewith GluR2 (arrows).

Deletion of 4.1 binding region attenuates GluR1 plasma membrane expression in heterologous cells

It has been well documented that the protein 4.1 family of proteins functions in membrane protein-cytoskeletal interactions(Bennett and Gilligan, 1993). Postsynaptic spines are enrichedwith F-actin, which directly contacts the PSD (Harris and Kater,1994). Maintenance of synaptic transmembrane proteins often requirestheir cytoskeleton attachment. We therefore explored whether disruptionof the interaction of GluR1 with the endogenous 4.1G in heterologouscells would affect the membrane trafficking of GluR1. GluR1 mutantswith (R1*823) or without (R1*812) the membrane proximal regionrequired for 4.1G/4.1N association were expressed in heterologouscells, and the plasma membrane expression of GluR1 was analyzedusing cell surface biotinylation and quantitative immunoblottingtechniques (Fig. 6). GluR1-transfected cells were treated witha water-soluble, membrane-impermeable derivative of biotin tolabel proteins on the cell surface. Biotinylated molecules werethen isolated by neutravidin beads, and a comparison of the steady-statelevels of surface wild-type (WT) and mutant GluR1 subunits wasanalyzed by SDS-PAGE and quantitative ECF immunoblot analyses.The overall expression of the two mutant GluR1 subunits was similar,and both proteins were associated with intracellular and plasmamembrane fractions, similar to WT GluR1 (data not shown). In contrast,the levels of surface expression of the two mutant receptors detectedusing biotinylation techniques were significantly different (Fig.6). The GluR1 subunit capable of binding 4.1N and 4.1G (R1*823)was efficiently expressed on the surface, in sharp contrast tothe GluR1 mutant (R1*812), which does not interact with 4.1. Deletionof the whole C-terminal domain (R1*807) rendered a similar resultto R1*812 (data not shown). These results suggest that the interactionof GluR1 with endogenous 4.1G in COS cells may regulate the plasmamembrane expression of GluR1.

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Figure 6. Deletion of the GluR1 4.1 binding region reduces surface expression of GluR1. The membrane proximal region in the GluR1 C terminus is important for receptor surface expression. COS cells were transfected with pRK5 (Mock), GluR1*812 (R1*812), or GluR1*823 (R1*823). Surface expression of GluR1 was determined by biotinylation, as described in Materials and Methods. Samples from total cell lysates (Total) and biotinylated samples (PM) were analyzed for GluR1. For quantitation, the signals from biotinylated samples were divided by the total GluR1 signals to obtain the ratio of surface expression for GluR1*823 (R1*823) and GluR1*812 (R1*812). The ratio of surface expression of GluR1*812 was normalized to that of GluR1*823 to obtain the relative value of surface expression. n = 3. The error bar indicates SEM.

Actin filaments are required for maintenance of surface GluR1 in heterologous cells

Previous studies have suggested that the cortical cytoskeleton is involved in synaptic targeting of AMPA receptors (Allisonet al., 1998; Kim and Lisman, 1999). To determine whether theactin cytoskeleton, possibly through a 4.1 association, regulatedthe surface expression of GluR1, we analyzed the effect of cytoskeletaldisrupting agent latrunculin A (an actin polymerization inhibitor)on the plasma membrane distribution of wild-type and mutant GluR1subunits (Fig. 7). COS cells transfected with wild-type GluR1or the two GluR1 mutants with and without the 4.1 binding region(R1*823 and R1*812) were treated with latrunculin A for 2 hr.Interestingly, latrunculin A drastically reduced surface expressionof WT GluR1 (Fig. 7A) and the GluR1 mutant (R1*823) that is capableof 4.1 binding (Fig. 7B) but had no effect on the GluR1 mutant(R1*812) that is unable to bind 4.1 (Fig. 7B). The total amountof GluR1 was not affected by latrunculin A treatment. These resultsindicate that the 4.1 binding region is important for the latrunculininhibition of GluR1 surface expression and suggest that 4.1 isimportant for the attachment of GluR1 with the actin cytoskeleton.

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Figure 7. F-actin regulates GluR1 surface expression in COS cells. A, Disruption of F-actin inhibits surface expression of GluR1 in COS cells. COS cells were transiently transected with WT GluR1. Twenty-four hours after the transfection, either DMSO or a concentrated DMSO stock of latrunculin A (Lat.A) was added to the culture medium. Final concentration of latrunculin A is 5 µM. Cells were further incubated at 37°C for 2 hr before cell surface biotinylation. Samples from cell lysates (Total) and biotinylated samples (PM) were analyzed for GluR1 using an anti-GluR1 N-terminal antibody. For quantitation, the biotinylated samples were normalized to total GluR1 signals to obtain the ratio of surface expression for the control and latrunculin-treated cells. The ratio of surface expression of the latrunculin-treated cells was normalized to that of control cells to express the relative surface expression. n = 3. The error bar indicates SEM. B. The C-terminal membrane proximal region of GluR1 is important for latrunculin inhibition of surface expression. COS cells transfected with pRK5 (Mock), R1*812, or R1*823 were treated with either DMSO (Lat.A $-$ ) or latrunculin A (Lat.A +), as described in Materials and Methods. For quantitation, the signals from biotinylated samples were normalized to the total GluR1 signal to obtain the ratio of surface expression. The ratio of the surface expression was then normalized to that of R1*823 without latrunculin. R1*823, R1*823+Lat.A, R1*823 without or with latrunculin A, respectively; R1*812, R1*812+Lat.A, R1*812 without or with latrunculin A, respectively. n = 3. Error bars indicate SEM.

GluR1 surface expression is attenuated by overexpression of the CTDs of 4.1

The CTDs of proteins 4.1N and 4.1G were used to further explore the specific effect of 4.1 homologs on F-actin-dependent surfaceanchoring of GluR1. Because the CTDs are sufficient for associationwith GluR1 but do not contain the domain for spectrin and actinbinding (Fig. 4A), we postulated that they could serve as "dominantnegative" constructs to examine the role of 4.1 in GluR1 surfaceexpression. CTDs or the vector were cotransfected with differentGluR1 constructs in COS cells, and the steady-state levels ofsurface GluR1 were analyzed by biotinylation techniques. Overexpressionof either 4.1N or 4.1G CTD specifically attenuated the surfaceexpression of the R1*823 mutant containing the C-terminal 4.1binding region but not the R1*812 mutant lacking this region (Fig.8). These results indicate that the CTDs may disrupt the interactionof GluR1 with endogenous 4.1 and support the idea that F-actinand 4.1N association affects GluR1 surface expression. Combinedwith previous actin disruption studies, our data suggest that4.1N and 4.1G serve as a link between GluR1 and cortical cytoskeletonthat is required for GluR1 plasma membrane stability.

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Figure 8. Overexpression of CTDs of 4.1 attenuated GluR1 surface expression. COS cells were cotransfected using R1*812 or R1*823, together with pRK5 (vector), 4.1GCTD (myc-4.1GCTD), or 4.1NCTD (myc-4.1NCTD). Both CTDs were myc-tagged. Transfected cells were incubated at 37°C for 24 hr, followed by cell surface biotinylation, as described in Materials and Methods. A, Immunoblots. Top panel, Total cell lysates blotted with anti-myc antibody; middle panel, total cell lysates blotted with anti-GluR1 N-terminal antibody; bottom panel, biotinylated samples blotted with anti-GluR1 N-terminal antibody. B, Quantitation of surface expression. The signals from biotinylated samples were normalized to the total GluR1 signal to obtain the ratio of surface expression and then normalized to the surface expression of GluR1*823 to obtain the relative value of surface expression. n = 3. Error bars indicate SEM.

Actin filaments are required for maintenance of surface GluR1 in cortical neurons

Latrunculin A was also used to investigate the importance of the actin cytoskeleton in the surface expression of AMPA receptorsin neurons (Fig. 9A). Rat cortical neurons were cultured in vitrofor 3 weeks and treated with 5 µM latrunculin A for 2 hr (Allisonet al., 1998). The biotinylation assay was then used to quantifysurface expression of GluR1. As seen in the COS cells, latrunculinA inhibited the surface expression of GluR1 in neurons. Theseresults suggest that surface expression of GluR1 in neurons mayalso be regulated by a 4.1-mediated interaction with the actincytoskeleton.

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Figure 9. Actin cytoskeleton is required for synaptic maintenance of AMPA receptors. A, Actin polymerization is required for synaptic maintenance of AMPA receptors. Cultured rat hippocampal neurons were treated with either DMSO (Lat.A $-$ ) or latrunculin A (Lat.A +) followed by cell surface biotinylation (Biotin +, $-$ ) as described in Materials and Methods. Samples from cell lysates (Total) and biotinylated samples (PM) were analyzed for GluR1 via anti-GluR1 antibody. Samples of immunoblots (top panel) and a summary of quantitation (bottom panel) are presented. For quantitation, the signals from biotinylated samples were normalized to total GluR1 signals to obtain the ratio of surface expression [PM/Total (%)]. DMSO, Lat.A, GluR1 without or with latrunculin A, respectively. n = 4. Error bars indicate SEM. B, Schematic model of AMPA receptor-actin cytoskeleton cross-linking by 4.1N. The interaction of the GluR1 subunit with protein 4.1N and SAP97 may link surface AMPA receptors to the cortical actin cytoskeleton network underneath the synaptic plasma membrane and PSD.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Excitatory synapses on dendritic spines are enriched in actin filaments, which are oriented longitudinally in the neck andform a lattice in the spine head (Fifkova and Delay, 1982; Matuset al., 1982; Cohen et al., 1985; Harris and Kater, 1994). Previousstudies have shown that the actin network is important for thesynaptic localization and immobilization of glutamate receptors(Allison et al., 1998). In this study we have shown that the AMPAreceptor subunit GluR1 interacts with the actin-associated proteins4.1N and 4.1G. Proteins 4.1N and 4.1G bind to GluR1 in vitro,using both the yeast two-hybrid system and a mammalian heterologousexpression system. In addition, we show that 4.1N colocalizeswith AMPA receptors in excitatory synapses in hippocampal neuronsin culture and is associated with GluR1 in vivo in rat brain.Deletion analysis demonstrated that a stretch of 11 amino acidsin the membrane proximal region in the GluR1 C terminus is requiredfor 4.1N binding, whereas a consensus region within the CTDs of4.1G and 4.1N is sufficient to mediate the interaction. In exploringthe functional significance of this interaction, we found thatGluR1 truncation mutants that lack the 4.1 binding region havereduced surface expression in heterologous cells. Moreover, overexpressionof the CTDs of 4.1N and 4.1G, which should disrupt the interactionof GluR1 with endogenous 4.1G, attenuated GluR1 surface expression.Disruption of the F-actin network with latrunculin A also resultedin decreased plasma membrane GluR1 both in heterologous cellsand in cultured neurons. These results suggest that protein 4.1Nmay play a functional role in the anchoring of AMPA receptorsto the actin cytoskeleton and stabilizing the surface expressionof the receptors. Recent studies have shown that the membraneproximal 39 amino acids of the GluR1 C terminus appear to be importantfor its sorting to dendrites (Ruberti and Dotti, 2000), suggestingthat binding of protein 4.1 may be involved in this sortingprocess.

Recent studies have provided evidence that a network of PDZ domain-containing proteins may also play an important role inthe cellular targeting of glutamate receptors in the CNS (Shengand Kim, 1996; O'Brien et al., 1998a; Kim and Huganir, 1999).The PDZ domain-containing proteins PSD-95, SAP102, and SAP93 directlyinteract with NMDA receptor subunits, whereas the PDZ domain-containingproteins GRIP/ABP, PICK1, and SAP97 directly bind to AMPA receptorsubunits. PDZ domain-containing proteins in non-neuronal cellshave also been shown to be important as organizers of the corticalcytoskeletal network (Fanning and Anderson, 1996). For example,erythrocyte protein 4.1 interacts with the membrane protein p55,a palmitoylated erythrocyte membrane protein with a single PDZdomain and glycophorin C, and these interactions may serve tocouple glycophorin C to the actin cytoskeleton (Marfatia et al.,1994; Marfatia et al., 1995). In addition, human CASK, a homologof the Caenorhabditis elegans PDZ-containing protein LIN-2, hasbeen shown to bind protein 4.1 (Cohen et al., 1998). Moreover,recently it has been reported that the PDZ domain-containing proteinSAP97/hDlg, a member of the PSD-95 family, binds to 4.1 in epithelialcells (Lue et al., 1994). Interestingly, SAP97 is also localizedto excitatory synapses and has recently been shown to specificallybind to the C-terminal PDZ ligand of GluR1. These results suggestthat SAP97 and 4.1 may form a trimeric complex with GluR1 andcooperate in the regulation of the synaptic localization and immobilizationof AMPA receptors (Fig. 9B).

Various recent studies have indicated that the level of functional surface synaptic AMPA receptors can be modulated by activity-dependentmechanisms (Isaac et al., 1995; Liao et al., 1995, 1999; Rao andCraig, 1997; Lissin et al., 1998, 1999; O'Brien et al., 1998b;Turrigiano et al., 1998; Carroll et al., 1999; Shi et al., 1999).Both electrophysiological and morphological studies have indicatedthat chronic and rapid changes in synaptic activity can regulatereceptor surface expression providing homeostatic and acute mechanismsfor controlling synaptic efficiency. Chronic increases or decreasesin synaptic activity decrease or increase, respectively, the levelsof AMPA receptor surface expression (Rao and Craig, 1997; O'Brienet al., 1998b; Turrigiano et al., 1998). Moreover, patterns ofsynaptic firing that can result in rapid changes in synaptic transmission,such as those that induce long-term potentiation and long-termdepression, can result in rapid changes in the distribution ofAMPA receptors (Isaac et al., 1995; Liao et al., 1995, 1999; Raoand Craig, 1997; Lissin et al., 1998, 1999; O'Brien et al., 1998b;Turrigiano et al., 1998; Carroll et al., 1999; Shi et al., 1999).It is possible that the association of GluR1 with the membranecytoskeleton via 4.1N may be regulated and play a role in theseprocesses. The C-terminal domain of GluR1 contains the major sitesfor AMPA receptor phosphorylation (Roche et al., 1996; Mammenet al., 1997b, 1999), and phosphorylation of this region may regulate4.1 binding. Moreover, several studies in erythrocytes have shownthat phosphorylation of protein 4.1 regulates its interactionwith the actin cytoskeleton and membrane proteins (Pinder et al.,1995). Future investigation of the dynamic regulation of AMPAreceptor targeting will facilitate our understanding of the potentialrole of protein 4.1 in synapticplasticity.

  FOOTNOTES

Received May 30, 2000; revised Aug. 1, 2000; accepted Aug. 4, 2000.

This work was supported by the Howard Hughes Medical Institute and National Institutes of Health. We thank Jeff Bernhardtfor the making of GluR1 mutants, Xiaoqun Zhang for providing ratprimary hippocampal cultures, and Carol Doherty for making andpurifying anti-GluR1antibodies.
L.S. and F.L. contributed equally to thiswork.

Correspondence should be addressed to Dr. Richard L. Huganir, Howard Hughes Medical Institute, Department of Neuroscience,The Johns Hopkins University School of Medicine, 725 North WolfeStreet, PCTB 904, Baltimore, MD 21205. E-mail: rhuganir{at}jhmi.edu.

Dr. Walensky's present address: Department of Neurology, Children's Hospital, 300 Longwood Street, Boston, MA02115.

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