Dystroglycan Is Selectively Associated with Inhibitory GABAergic Synapses But Is Dispensable for Their Differentiation

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The Journal of Neuroscience, June 1, 2002, 22(11):4274-4285

Dystroglycan Is Selectively Associated with Inhibitory GABAergic Synapses But Is Dispensable for Their Differentiation
Sabine Lévi¹, R. Mark Grady¹, Michael D. Henry², Kevin P. Campbell², Joshua R. Sanes¹, and Ann Marie Craig¹
¹ Washington University, Department of Anatomy and Neurobiology, St. Louis, Missouri 63110, and ² Howard Hughes Medical Institute, Departments of Physiology and Biophysics and of Neurology, University of Iowa College of Medicine, Iowa City, Iowa 52242

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The dystrophin glycoprotein complex (DGC) is a multimolecular complex that links the extracellular matrix to the cytoskeleton.The DGC is present at the skeletal neuromuscular junction andrequired for its maturation and maintenance. Members of the DGCare also expressed in brain. We used cultured hippocampal neuronsto analyze the distribution, regulation, and role in synaptogenesisof the major transmembrane component of the DGC, dystroglycan;one of its extracellular ligands, agrin; and one of its cytoskeletalbinding partners, dystrophin. $alpha$ -Dystroglycan, $beta$ -dystroglycan,and dystrophin clustered at a subset of inhibitory synapses containingGABA_AR subunits $alpha$ 1, $alpha$ 2, and $gamma$ 2, and the inhibitory receptor anchoringprotein gephyrin. DGC components were not detected at excitatoryglutamatergic synapses. Dystroglycan is the first identified adhesivemacromolecule at mature GABA synapses. Developmentally, dystroglycanclustered at synaptic loci after synaptic vesicles, GABA_AR, andgephyrin, the latter being closely associated with GABA_AR at allstages of synaptogenesis analyzed. Analysis of gephyrin $-$ / $-$ , agrin $-$ / $-$ , and mdx mouse hippocampal neurons in culture indicated thatsynaptic clustering of dystroglycan occurs independently of gephyrin,agrin, and dystrophin. In dystroglycan-deficient neurons, culturedfrom a conditional mutant strain, GABAergic synapses differentiatedwith clusters of gephyrin and GABA_AR apposed to synaptic terminals,but these synapses did not contain detectable dystrophin. Thusthe DGC is not essential for GABAergic synaptogenesis but is likelyto function in modulating inhibitory synapses or conferring specializedproperties on a subset ofthem.

Key words: synaptogenesis; GABA receptor; gephyrin; dystrophin; agrin; mdx

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The development of central inhibitory GABAergic synapses involves the formation of high-density clusters of GABA_A receptors(GABA_ARs) opposite GABAergic terminals. The mechanisms of inhibitorysynaptic differentiation are not well understood, especially incomparison with molecular events at the mammalian skeletal neuromuscularjunction (NMJ) (for review, see Sanes and Lichtman, 1999) andat central excitatory glutamatergic synapses (for review, seeSheng and Pak, 1999; Garner et al., 2000). At the NMJ, nerve-derivedagrin signaling through MuSK is necessary for the formation ofacetylcholine receptor (AChR) clusters opposite nerve terminals.The dystrophin-associated glycoprotein complex (DGC) is necessaryfor stabilization of AChR clusters and morphological maturationof the postsynaptic apparatus (Deconinck et al., 1997; Grady etal., 1997, 2000; Adams et al., 2000; Jacobson et al., 2001). Atglutamatergic synapses, a number of scaffolding proteins includingPSD-95, GKAP, Shank, GRIP, and PICK1 function in receptor localizationwithin the postsynaptic cell. The trans-synaptic signaling moleculesare not yet well defined but may include neuroligins, cadherins,ephrins and Eph receptors, and Narp (Craig and Lichtman, 2001;Klein, 2001). At GABAergic synapses, gephyrin is concentratedwithin the postsynaptic domain and is reported to be essentialfor synaptic clustering of GABA_AR $alpha$ 2 and $gamma$ 2 subunits in hippocampalneurons (Kneussel et al., 1999). However, gephyrin is only partiallyrequired for synaptic clustering of GABA_AR $alpha$ 2 and $gamma$ 2 subunitsin retina and spinal cord and is not required for synaptic clusteringof other $alpha$ subunits (Fischer et al., 2000; Kneussel et al., 2001).The trans-synaptic signaling molecules are not yet defined forGABAergicsynapses.

A role for dystrophin in GABAergic synaptogenesis was recently suggested by Kneussel et al. (1999). Dystrophin is a largecytoskeletal protein of the $alpha$ $-$ actinin/ $beta$ $-$ spectrin family. Mutationsin dystrophin result in Duchenne and Becker muscular dystrophies(Hoffman and Kunkel, 1989). The DGC provides a transmembrane linkagebetween the extracellular matrix and the cytoskeleton of musclefibers (for review, see Henry and Campbell, 1999; Blake and Kroger,2000). A core component of the DGC is dystroglycan, which is composedof an extracellular $alpha$ subunit and a transmembrane $beta$ subunit, derivedby proteolytic cleavage and glycosylation of a single precursor(Ibraghimov-Beskrovnaya et al., 1992). Dystroglycan binds dystrophinand utrophin intracellularly and binds several matrix moleculesincluding agrin, laminin, and perlecan extracellularly. Targeteddeletion of dystroglycan in mice leads to a deficiency in formationof basement membranes and early embryonic lethality (Williamsonet al., 1997), showing that the DGC has widespreadfunctions.

Evidence is also accumulating for a function of the DGC at central neuronal synapses. Dystrophin and dystroglycan are concentratedin photoreceptor terminals, and DMD patients and mdx3cv mice withreduced expression of dystrophin isoforms show an altered electroretinogramindicating impaired synaptic transmission under conditions ofdark adaptation (Blake and Kroger, 2000). DGC components dystroglycan,dystrophin, the short dystrophin isoforms Dp140 and Dp71, dystrobrevins,and syntrophins are abundant in brain, and some are concentratedin postsynaptic density fractions (Kim et al., 1992; Blake etal., 1999; Moukhles and Carbonetto, 2001). Dystroglycan bindstwo cell surface proteins thought to be involved in synaptogenesis:agrin and neurexin (Bowe et al., 1994; Campanelli et al., 1994;Gee et al., 1994; Sugiyama et al., 1994; Sugita et al., 2001).Previous immunolocalization studies suggested a concentrationof dystrophin at a subset of postsynaptic sites (Lidov et al.,1990) and dystroglycan at excitatory spine synapses (Tian et al.,1997; Zaccaria et al., 2001). A recent study found a selectiveassociation of dystrophin with GABAergic synapses (Knuesel etal., 1999). Kneussel et al. (1999) further reported a 38% reductionin immunofluorescent clusters of GABA_AR $alpha$ 2 subunit in hippocampaltissue of mdx mice, which lack the long form of dystrophin. Thesedata all suggest that the DGC may function as a trans-synapticsignal for some aspect of central neuron synapticdifferentiation.

We explore here the role of the DGC complex in synaptic differentiation by analysis of wild-type and mutant hippocampal neuronsin culture. We found that the DGC is selectively associated witha subset of inhibitory GABAergic synapses but is not detectableat excitatory glutamatergic synapses. Dystroglycan clustered atsynaptic loci after synaptic vesicles, GAD, GABA_AR, and gephyrin.Gephyrin, agrin, and dystrophin were not required for synapticclustering of dystroglycan. Despite the potential of dystroglycanas a synaptogenic cell adhesion protein, we show using mutantmouse cultures that dystroglycan is not required for synapticclustering of GAD, gephyrin, or major GABA_AR subtypes. Thus theDGC is a gephyrin-independent complex associated with the maturationof a subset of inhibitorysynapses.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Genotyping. The agrin-null mice were generated by a ~9 kb DNA deletion in the agrin gene corresponding to most of the agrincoding region (from the BamHI site in exon 6 downstream of exon33), which was replaced by the neomycin resistance gene (Lin etal., 2001). In the gephyrin $-$ / $-$ mice, the sequences responsiblefor initiating transcription and translation and exon 1 of thegephyrin gene were deleted and replaced with the neomycin resistancegene (Feng et al., 1998). Animals were maintained as heterozygoteson a C57/129 hybrid background. Embryos were genotyped by PCRamplification as described previously (Feng et al., 1998; Linet al., 2001). Mdx mice (C57BL/10ScSn) were purchased from JacksonLaboratories (Bar Harbor, ME). Conditional mutant DG lox/lox micewere generated by introduction of a loxP-neo cassette in the firstintron and a loxP site in the second intron of the mouse DG gene(Saito et al., 2001; Moore et al., 2002). The DG lox/lox miceare viable and fertile and exhibited no phenotypicabnormalities.

Cell culture. Primary cultures were prepared from embryonic hippocampi using previously described methods (Goslin et al.,1998). Rat hippocampi were dissected at embryonic day (E) 18,mouse hippocampal cultures were prepared from individual embryosat E17. Tissues were dissociated by trypsinization and triturationand plated at 4000 cells per square centimeter onto poly-L-lysine-coatedglass coverslips. After cells were allowed to attach in minimalessential medium (MEM) with 10% horse serum, they were transferredand maintained up to 5 weeks by growing them over rat glial feedersin serum-free MEM with N2 supplements. Cytosine arabinoside wasadded after 2 d to inhibit glial proliferation. The neurons wereused at 7-35 d after plating for immunocytochemicalstaining.

Neuron infection with adenovirus-Cre. The defective adenovirus vector expressing Cre was obtained from F. L. Graham (McMasterUniversity, Hamilton, Canada) (Anton and Graham, 1995). The viruswas propagated and amplified in 293 cells, a permissive humancell line that supplies the E1 function in trans, and purifiedby CsCl gradient centrifugation (Graham and Prevec, 1995). Thetiter (2 × 10¹⁰ pfu/ml) was determined by plaque assay. At 7 d in culture, wild-typeand DG lox/lox neurons on coverslips were transferred from theirhome dishes into a sterile incubation chamber. Adenovirus-Crewas diluted in warm conditioned culture medium, and neurons wereinfected with a multiplicity of infection (MOI) 10 for 1 hr at37°C. Most of the virus-containing medium was then removed, andcoverslips were transferred back to their home dishes over glialfeeders and maintained for another 12 d beforeimmunostaining.

Antibodies. The following mouse monoclonal antibodies were used: GAD6 against glutamic acid decarboxylase (1:2; DevelopmentalStudies Hybridoma Bank, University of Iowa, Iowa City, IA), mAb7aagainst gephyrin (5 µg/ml; Cedarlane, Hornby, Canada), VIA4.1against $alpha$ $-$ dystroglycan (20 µg/ml, IgG1; Upstate Biotechnology,Lake Placid, NY), 43DAG1/8D5 against $beta$ $-$ dystroglycan (1:25, IgG2a;Novocastra Laboratories, Newcastle, UK), Dys-2, which recognizesthe last 17 C-terminal amino acids common to all the forms ofdystrophin (Dy8/6C5, 1:20, IgG1; Novocastra Laboratories), andmicrotubule-associated protein 2 (MAP2; Chemicon International,Temecula, CA). Rabbit antibodies were used against synapsin I(0.4 µg/ml; Chemicon), SynGAP (1:1000; Affinity Bioreagents),and glutamic acid decarboxylase 65 and 67 kDa (GAD, 1:200; Chemicon).A human antibody against gephyrin was used (CSF861, 1:100; giftfrom P. de Camilli, Yale University) (Butler et al., 2000) thatgave an identical pattern of immunoreactivity as mAb7a. Antibodiesraised in the guinea pig against the GABA_AR $gamma$ 2 subunit (1:2000), $alpha$ 2 subunit (1:3000), and $alpha$ 1 subunit (1:2000) were gifts from J.-M.Fritschy (University of Zurich, Switzerland) (Fritschy and Mohler,1995). A rat antibody against NCAM was also used (H28, 1:200)(Gennarini et al., 1984). Primary antibodies were visualized withfluorochrome-conjugated secondary antibodies (2.5 µg/ml; VectorLaboratories, Burlingame, CA) or with biotin-conjugated secondaryantibody (2.5 µg/ml) followed by fluorochrome-conjugated streptavidin(500 ng/ml). The fluorochromes used were fluorescein, Texas Red,and 7-amino-4-methylcoumarin-3-acetic acid. For simultaneous detectionof monoclonal primary antibodies, Alexa Fluor 488 goat anti-mouseIgG1 (1:1000; Molecular Probes, Eugene, OR) and Alexa Fluor 594goat anti-mouse IgG2a (1:200; Molecular Probes) subtype-specificsecondary antibodies wereused.

Immunocytochemistry. Coverslips used for $beta$ $-$ dystroglycan immunostaining were fixed with methanol for 10 min at $-$ 20°C. For otherantigens, neurons were fixed with warmed 4% paraformaldehyde/4%sucrose in PBS for 15 min at room temperature and permeabilizedfor 5 min with 0.25% Triton X-100 in PBS. For surface GABA_AR detection,living neurons were incubated with antibodies against GABA_AR $gamma$ 2or GABA_AR $alpha$ 2 extracellular epitopes (1:1000) for 1 hr at 37°C inconditioned culture medium, washed, and fixed. Nonspecific stainingwas blocked for 30 min in 10% BSA at 37°C, and neurons were incubatedin 3% BSA overnight at room temperature for primary antibodiesand for 45 min at 37°C for secondary antibodies. For multiple-labelingexperiments, antibodies were incubated simultaneously. Coverslipswere mounted in Tris-HCl, glycerol, polyvinyl alcohol with 2%1.4-diazobicyclo[2.2.2] octane. Fluorescence and phase-contrastimages were captured with a Photometrics series 250 cooled CCDcamera mounted on a Zeiss Axioscope microscope with a 63× 1.4numerical aperture lens using Metamorph imaging software. Imageswere prepared for printing using Adobe Photoshop 5software.

Quantitative analysis. The number of synaptic gephyrin, GABA_AR $gamma$ 2, and $beta$ $-$ dystroglycan puncta per 100 µm dendrite length andthe proportion of clusters that were synaptic were determinedon neurons immunolabeled for synapsin, GABA_AR $gamma$ 2, and either gephyrinor $beta$ $-$ dystroglycan after 1, 2, 3, and 5 weeks in culture usingMetamorph imaging software (Rao et al., 2000). One dendrite perneuron was chosen, and images were subjected to a user-definedintensity threshold to select clusters. GABA_AR $gamma$ 2, gephyrin, or $beta$ $-$ dystroglycan clusters were classified as synaptic if they wereapposed to synapsin-immunoreactive puncta. Apposition was determinedby first generating a binary mask from the thresholded synapsinimage and widening the regions representing the presynaptic punctaby one pixel all around. Any cluster in the thresholded GABA_AR $gamma$ 2,gephyrin, or $beta$ $-$ dystroglycan images that had any pixel overlapwith the binarized dilated synapsin mask was considered synaptic.A second mask containing the synaptic GABA_AR $gamma$ 2 clusters was thencompared with the thresholded gephyrin or $beta$ $-$ dystroglycan imagesto determine the percentage of synaptic GABA_AR $gamma$ 2 clusters exhibitingpixel overlap (colocalization) with either gephyrin or $beta$ $-$ dystroglycan.Similarly, a mask containing the synaptic gephyrin or $beta$ $-$ dystroglycanclusters was compared with the thresholded GABA_AR $gamma$ 2 image to determinepercentage of clusters colocalized. The percentage of $beta$ $-$ dystroglycanclusters colocalized with gephyrin, $alpha$ $-$ dystroglycan, dystrophin,or SynGap was measured from double-labeling experiments at 3 weeks.Clusters were defined by visually thresholding all images. Thethresholded $beta$ $-$ dystroglycan image was then used to generate a binarymask, and all clusters that exhibited any pixels above thresholdin the paired images were counted as colocalized. Surface areasof clusters and of the entire dendrite regions were also recorded.All measures were obtained from 20 neurons, 10 each from two independentcultures. Mean values ± SEM were calculated using StatView F.4.11software (Abacus Concepts, Inc.).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

$beta$ $-$ Dystroglycan is concentrated at a subset of inhibitory GABAergic synapses in cultured hippocampal neurons

To test for association between the DGC and synapses, the distribution of the essential DGC component $beta$ -dystroglycan was determinedin relation to several synaptic antigens by double- and triple-labelimmunofluorescence in cultured hippocampal neurons (Fig. 1). Thesecultures develop functional inhibitory and excitatory synapseswith molecularly specialized clusters of GABA_AR opposite GABAergicterminals and AMPA and NMDA receptor opposite glutamatergic terminals(Craig et al., 1994; Rao et al., 1998). $beta$ -Dystroglycan formedclusters along the soma and dendrites of many but not all of theneurons. The pattern of $beta$ $-$ dystroglycan clusters was reminiscentof the pattern of GABAergic synapses, including a selective associationwith proximal versus distal dendrites (Benson and Cohen, 1996).Indeed, most $beta$ $-$ dystroglycan clusters colocalized with synapsin(Fig. 1A). By quantitative measures, which may yield a low estimatebecause some clusters may have fallen below threshold, a similarpercentage (65 ± 5%) of $beta$ $-$ dystroglycan clusters exhibited overlapwith synapsin puncta as did clusters of GABA_AR $gamma$ 2 (72 ± 4%) orgephyrin (63 ± 3%). Furthermore, synaptic $beta$ $-$ dystroglycan clustersalso colocalized with GABA_AR $gamma$ 2 (70 ± 7% colocalization) (Fig.1A), indicating a specific concentration at GABAergic synapses.A concentration of $beta$ $-$ dystroglycan at GABAergic synapses was alsovisually apparent in neurons double-labeled for $beta$ $-$ dystroglycanand GAD or gephyrin (Fig. 1B,C).

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Figure 1. $beta$ $-$ Dystroglycan is concentrated at a subset of inhibitory GABAergic synapses. Rat hippocampal neurons were fixed at 3 weeks in culture and immunostained for combinations of $beta$ -dystroglycan ( $beta$ $-$ DG, all panels, green) and either GABA_AR $gamma$ 2 (A, red) and synapsin (A4, blue) or the synthetic enzyme for GABA, GAD, a marker of GABAergic terminals (B, red), or the inhibitory postsynaptic scaffolding protein gephyrin (C, red), or the excitatory postsynaptic marker SynGAP (D, red). $beta$ $-$ Dystroglycan formed clusters colocalized with GABA_AR $gamma$ 2, GAD, and gephyrin. Almost all $beta$ $-$ dystroglycan clusters localized to inhibitory synapses (arrowheads, yellow puncta in A3, B2, C2; white puncta in A4), but not all inhibitory synapses contained concentrations of $beta$ $-$ dystroglycan (arrows, red puncta in A3, B2, C2; pink puncta in A4). $beta$ $-$ dystroglycan (D, arrowheads) was not detected at excitatory glutamatergic synapses labeled with SynGAP (D, arrows; note the absence of yellow puncta in D3). Scale bar, 10 µm.

The close association between $beta$ $-$ dystroglycan and GABA_AR, gephyrin, and GAD strongly suggests a selective accumulation of $beta$ $-$ dystroglycanat inhibitory synapses and not excitatory synapses. This ideawas confirmed by comparing the distribution of $beta$ $-$ dystroglycanwith that of SynGAP or GKAP, PSD-95-binding proteins that areselectively localized to excitatory glutamatergic synapses (Naisbittet al., 1997; Chen et al., 1998; Kim et al., 1998). We observedSynGAP or GKAP clusters and $beta$ $-$ dystroglycan clusters in distinctnonoverlapping distributions along dendrites (Fig. 1D) (and datanot shown). Only 13 ± 4% of $beta$ $-$ dystroglycan clusters colocalizedwith SynGAP. In contrast, 78 ± 3% of $beta$ $-$ dystroglycan clusters colocalizedwith gephyrin. In these same dendrites, $beta$ $-$ dystroglycan occupiedonly 0.9 ± 0.1% of the total surface area, SynGAP occupied 4.4± 3.3%, and gephyrin occupied 2.8 ± 0.2%. The apparent colocalizationbetween $beta$ $-$ dystroglycan and SynGAP could represent random overlapor a low level of true colocalization, as reported previouslyfor PSD-95 with GAD (9.6% colocalization) in these cultures (Raoet al., 2000). However, the colocalization of $beta$ $-$ dystroglycan withgephyrin is clearly nonrandom and is similar to that found previouslyfor GABA_AR with GAD (68% colocalization) (Rao et al., 2000). Thus $beta$ $-$ dystroglycan is preferentially associated with inhibitory synapsesin hippocampal neurons. Dystroglycan is the first identified adhesivemacromolecule at mature GABAergicsynapses.

Many clusters of GAD, gephyrin, and GABA_AR $gamma$ 2 were not colocalized with detectable $beta$ $-$ dystroglycan (Fig. 1A-C, arrows) (forquantification, see Table 1), indicating that high concentrationsof $beta$ $-$ dystroglycan were present only at a subset of inhibitorysynapses. $beta$ $-$ Dystroglycan was found at GABAergic synapses on bothpyramidal neurons and interneurons. Because GABA_A receptors arepentameric heteroligomers derived from combinations of at least17 different subunits (Hevers and Luddens, 1998), we tested whether $beta$ $-$ dystroglycan might associate with a particular receptor composition.We found $beta$ $-$ dystroglycan clusters colocalized with a subset ofclusters of GABA_AR subunits $alpha$ 1, $alpha$ 2, $gamma$ 2, and $beta$ 2/3 (Figs. 1, 3,4) (and data not shown), indicating no particular associationwith any of these subunits.


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Table 1. Quantification of the developmental synaptic accumulation of GABA_AR $gamma$ 2, gephyrin, and $beta$ -dystroglycan

$alpha$ $-$ Dystroglycan, $beta$ $-$ dystroglycan, and dystrophin colocalize at GABAergic synapses

We tested for the presence of other components of the DGC in the hippocampal neurons and detected $alpha$ $-$ dystroglycan and dystrophin(Fig. 2) but not utrophin (data not shown). $alpha$ $-$ Dystroglycan anddystrophin appeared to colocalize with $beta$ $-$ dystroglycan (Fig. 2A,B).Quantitation yielded colocalization values of 66 ± 3 and 63 ±4% for $beta$ $-$ dystroglycan with $alpha$ $-$ dystroglycan and dystrophin, respectively.The concentration of $alpha$ $-$ dystroglycan at GABAergic synapses wasconfirmed visually by colocalization with GABA_AR $alpha$ 1 and synapsin(Fig. 2C). These results suggest that $alpha$ $-$ dystroglycan, $beta$ $-$ dystroglycan,and dystrophin form a complex at GABAergic synaptic sites.

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Figure 2. $alpha$ -Dystroglycan and dystrophin form part of the DGC at GABAergic synases. Hippocampal neurons were fixed at 3-5 weeks in culture and immunostained for combinations of $beta$ -dystroglycan (A, red) and $alpha$ -dystroglycan (A, green), $beta$ -dystroglycan (B, red), and dystrophin (B, green), or $alpha$ -dystroglycan (C, green), GABA_AR $alpha$ 1 (C, red), and synapsin (C, blue). $alpha$ -Dystroglycan and dystrophin completely colocalized with $beta$ -dystroglycan (arrowheads, yellow puncta in A3, B3). $alpha$ -Dystroglycan also colocalized with GABA_AR $alpha$ 1 (arrowheads, yellow puncta in C3) at synapses (white puncta in C4) on the interneuron shown in C. Note the absence of $alpha$ -dystroglycan at some synaptic GABA_AR $alpha$ 1 (arrows, pink puncta in C4). Scale bar, 10 µm.

Dystroglycan accumulates at GABAergic synapses late in development, after accumulation of synaptic vesicles, gephyrin, and GABA_ARs

We next determined the developmental time course of association of $beta$ $-$ dystroglycan with GABAergic synapses and compared thiswith the time course of synaptic accumulation of gephyrin. Weused triple-label immunocytochemistry with antibodies to synapsin,GABA_AR $gamma$ 2, and either gephyrin or $beta$ $-$ dystroglycan and analyzed thedistribution patterns both qualitatively (Fig. 3) and quantitatively(Table 1).

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Figure 3. Gephyrin coclusters with GABA_AR at synaptic sites very early during synaptogenesis, whereas $beta$ $-$ dystroglycan accumulates at a subset of synaptic GABA_AR clusters only late in development. Cultures were fixed at 1 (A, D), 2 (B, E), and 3 weeks (C, F) and triple-stained for synapsin (A1-F1), GABA_AR $gamma$ 2 (A2-F2), and gephyrin (A3- C3) or $beta$ $-$ dystroglycan (D3-F3). The number of gephyrin and GABA_AR $gamma$ 2 clusters increased in parallel during in vitro development. At all stages in culture, GABA_AR $gamma$ 2 clusters apposed to presynaptic sites were colocalized with gephyrin (arrowheads). At 1 week in culture, almost all postsynaptic GABA_AR $gamma$ 2 clusters were devoid of detectable $beta$ $-$ dystroglycan. At 2 weeks, $beta$ $-$ dystroglycan was clustered at a few synaptic sites. The number of synaptic $beta$ $-$ dystroglycan clusters increased between 2 and 3 weeks in culture. The proportion of GABA_AR $gamma$ 2 coclustered with $beta$ $-$ dystroglycan increased in parallel. Arrowheads indicate GABA_AR $gamma$ 2 colocalized with gephyrin or $beta$ $-$ dystroglycan; arrows show GABA_AR $gamma$ 2 clustering independently of $beta$ $-$ dystroglycan. Scale bar, 10 µm.

At 1 week in culture, a few neurons displayed GABA_AR $gamma$ 2 and gephyrin clusters apposed to presynaptic terminals around somataand dendrites (Fig. 3A). The density of postsynaptic gephyrinand GABA_AR $gamma$ 2 clusters increased in parallel, rapidly during thesecond week and more slowly during the third week in culture (Fig.3B,C). Most synaptic gephyrin and GABA_AR $gamma$ 2 clusters colocalizedat all stages analyzed; the colocalization values in Table 1represent an underestimate because some clusters for each antigenfell below the threshold for quantitation. The early associationof gephyrin with developing synaptic GABA_AR is consistent witha function of gephyrin in synapse assembly and initial GABA_ARclustering.

The developmental localization profile was very different for $beta$ $-$ dystroglycan. At 1 week in culture, very little $beta$ $-$ dystroglycanimmunoreactivity was detected, and synaptic GABA_AR $gamma$ 2 clusterswere rarely colocalized with $beta$ $-$ dystroglycan (Fig. 3D). Over thenext 2 weeks, progressively more $beta$ $-$ dystroglycan clusters weredetected, and more GABA_AR $gamma$ 2 clusters were colocalized with $beta$ $-$ dystroglycan(Fig. 3E,F). Quantitative analysis indicated a steady continuousdevelopmental increase in synaptic $beta$ $-$ dystroglycan for at least2 additional weeks (to 5 weeks in vitro; data not shown), in contrastto the earlier rapid increase and later plateau levels of synapticgephyrin. However, even at this late stage of development manysynaptic GABA_AR $gamma$ 2 clusters were devoid of detectable $beta$ $-$ dystroglycan.Thus dystroglycan appeared to be associated with only a subsetof mature GABAergic synapses. It is not clear whether $beta$ $-$ dystroglycanwould eventually associate at high level with all mature GABAergicsynapses or whether it associates with a distinct subpopulation.It is also possible that dystroglycan concentrates at all GABAergicsynapses, but the levels at some synapses may fall below the detectionthreshold.

Genetic analysis of the requirements for synaptic clustering of the dystrophin glycoprotein complex

We tested major dystroglycan binding partners and components of GABAergic synapses for their role in synaptic localizationof dystroglycan. We first analyzed hippocampal cultures from mdxmice, which lack the full-length form of dystrophin, a major intracellularbinding partner for dystroglycan. Visually, mdx neurons exhibitednormal accumulations of $beta$ -dystroglycan at GAD-labeled synapses(Fig. 4B) compared with wild type (Fig. 4A). Immunofluorescencewith a monoclonal antibody that recognizes both full-length andshort forms of dystrophin was greatly reduced, although some immunoreactivitywas colocalized with $beta$ $-$ dystroglycan (Fig. 4F). Thus some shortforms of dystrophin as well as full-length dystrophin are complexedwith dystroglycan at GABAergic synapses. Furthermore, full-lengthdystrophin is not essential for assembly of the DGC at GABAergicsynapses.

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Figure 4. Agrin, dystrophin, and gephyrin are not required for localization of dystroglycan to GABA synapses. Individual cultures were grown from hippocampi of wild-type (A, E, G), mdx (B, F), agrin $-$ / $-$ (C), and gephyrin $-$ / $-$ (D, H) mice and analyzed after 17-19 d. Neurons were immunolabeled for combinations of GAD (red, A-D) and $beta$ $-$ dystroglycan (green, A-D); $beta$ $-$ dystroglycan (red, E, F) and dystrophin (green, E, F); or GABA_AR $alpha$ 2 (red, G, H) and $beta$ $-$ dystroglycan (green, G, H). In mdx, agrin $-$ / $-$ , and gephyrin $-$ / $-$ neurons, clusters of $beta$ $-$ dystroglycan apposed to GAD were observed as in wild-type neurons (yellow puncta in A3, B3, C3, D3). Even in mdx neurons, clusters of some dystrophin isoforms were still observed with the dys2 antibody (F2), and these colocalized with $beta$ $-$ dystroglycan (yellow puncta in F3). In wild-type neurons, $beta$ $-$ dystroglycan always colocalized with GABA_AR $gamma$ 2 (yellow puncta in G3), but in the absence of gephyrin, $beta$ $-$ dystroglycan clusters were often found without punctate GABA_AR $gamma$ 2 immunoreactivity (red puncta in H3). In all images, arrowheads indicate colocalization; arrows in H show $beta$ $-$ dystroglycan clustering independently of GABA_AR $gamma$ 2. Scale bar, 10 µm.

Agrin is a major dystroglycan-binding protein expressed by central neurons as well as at the NMJ. We showed previously thatagrin isoforms containing the z splice insert, which are requiredfor neuromuscular synaptogenesis, are not required for synapticaccumulation of GABA_AR $beta$ 2/3 opposite GAD-positive terminals (Serpinskayaet al., 1999). However, some z-minus agrin was expressed by thehypomorphic mutants used in our previous study, and it is knownthat z-minus agrin binds more strongly to dystroglycan than doesz-plus agrin (Sugiyama et al., 1994). We therefore analyzed hippocampalneurons from a newly generated agrin mutant that is a completenull for all forms of agrin (Lin et al., 2001). As reported previously,synapse formation proceeded on schedule in agrin $-$ / $-$ mutants.Specifically, agrin $-$ / $-$ neurons showed normal accumulations of $beta$ $-$ dystroglycan at GAD-labeled synapses (Fig. 4C). Thus, althoughagrin binds dystroglycan, it is not required for accumulationof the DGC at GABAergicsynapses.

The postsynaptic anchoring protein gephyrin appears at synapses earlier than dystroglycan and is reportedly essential forsynaptic accumulation of GABA_AR $alpha$ 2 and $gamma$ 2 subunits in hippocampalculture (Kneussel et al., 1999). We cultured embryonic hippocampalneurons from gephyrin $-$ / $-$ mice for 17-19 d and then assayed fordystroglycan and dystrophin localization to GABA synapses (Fig.4D,H) (and data not shown). Accumulation of GAD-positive GABAergicpresynaptic specializations, at sites distinct from excitatorypostsynaptic specializations, occurred normally in the gephyrin $-$ / $-$ neurons. We found that gephyrin was not required for accumulationof dystroglycan or dystrophin at GABAergic synapses (Fig. 4D)(and data not shown). $beta$ $-$ Dystroglycan immunoreactivity in the gephyrin $-$ / $-$ neurons was indistinguishable from wild type (Fig. 4A,D).In the absence of gephyrin, many $beta$ $-$ dystroglycan clusters werefound lacking detectable immunoreactivity for GABA_AR $gamma$ 2, a findingnot common in wild-type neurons (Fig. 4G,H). In addition, lowlevels of GABA_AR $gamma$ 2 clustering persist, opposing some GAD-positiveterminals in the absence of gephyrin (data not shown), and inthese cases $beta$ $-$ dystroglycan colocalized with some GABA_AR $gamma$ 2 clusters.Thus the DGC appears to be completely independent of gephyrin:it neither requires gephyrin for accumulation at GABA synapsesnor compensates for the loss of gephyrin, at least not by anychange in association of dystrolgycan with GABA_ARclusters.

Dystroglycan is required for association of dystrophin but not for differentiation of GABAergic synapses

Although a DGC containing short dystrophin isoforms and/or utrophin can form in the absence of full-length dystrophin (Blakeand Kroger, 2000), it is thought that no DGC can form in the absenceof dystroglycan. Thus to test more directly the potential functionof the DGC in GABAergic synaptogenesis, we analyzed dystroglycan $-$ / $-$ neurons in culture (Figs. 5, 6). Because dystroglycan $-$ / $-$ mice die early in embryogenesis before development of the brain(Williamson et al., 1997), we used a conditional dystroglycanmutant (Saito et al., 2001; Moore et al., 2002). In these mice,lox sites have been inserted into introns that flank the firstcoding exon of the dystroglycan gene. These insertions have nodetectable effect on dystroglycan expression but act as recognitionsites for Cre recombinase. Introduction of this recombinase leadsto excision of the first exon, generating a protein-null mutantallele. We therefore prepared cultures from hippocampi of conditionalmutant heterozygotes and then treated the cultures with adenovirus-Creto inactivate dystroglycan. For the experiments described here,we wanted to assess roles of dystroglycan in synaptogenesis perse, separate from possible roles in earlier steps, such as differentiationor process outgrowth. We therefore introduced the adenovirus-Creat 7 d in culture, subsequent to attachment of neurons to thesubstrate and initial outgrowth of axons and dendrites but beforethe time at which dystroglycan is detected at GABA synapses incontrol neurons. As controls, we used neurons that bore the conditionalallele but were not treated with adenovirus and virus-treatedneurons from wild-type mice.

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Figure 5. Dystroglycan is not required for the differentiation of neuronal dendritic and axonal compartments and synaptic terminals. Hippocampal neurons were cultured from wild-type (A) or DG lox/lox (B-E) mice, incubated at 7 d in culture with adenovirus-Cre (A, C-E) or not (B), and analyzed at 17-19 d. Neurons were immunolabeled for combinations of $beta$ $-$ dystroglycan (A1, B1, C1) and synapsin (A2, B2, C2), GAD (D), MAP2 (E1), and NCAM (E2). Synaptic $beta$ $-$ dystroglycan clusters (arrowheads) were detected in wild-type neurons treated with adenovirus-Cre (A) and in DG lox/lox neurons not treated with virus (B), but not in most DG lox/lox neurons treated with adenovirus-Cre (C, arrows; representative of 94% of the neurons). Presynaptic terminals (C, arrows) including GABA synapses (D, arrowheads) formed normally in the absence of dystroglycan. Dystroglycan was also not required to elaborate dendrites (arrowheads) and axons (E, arrows). Scale bar, 10 µm.

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Figure 6. Dystroglycan is essential for association of dystrophin but not for differentiation of GABA synapses. Hippocampal neurons were cultured from DG lox/lox mice, incubated at 7 d in culture with adenovirus-Cre, and analyzed at 17-19 d. Neurons were immunolabeled for combinations of $beta$ $-$ dystroglycan (A1), dystrophin (A2), and synapsin (A3); $beta$ $-$ dystroglycan (B1), GABA_AR $alpha$ 2 (B2), and synapsin (B3); $beta$ $-$ dystroglycan (red, C1) and gephyrin (green, C2) overlaid on a phase-contrast image; gephyrin (red, D) and GABA_AR $gamma$ 2 (green, D); or GABA_AR $alpha$ 2 (red, E) and GAD (green, E). In the absence of dystroglycan, dystrophin did not form synaptic clusters (A), but GABA_AR subunits, gephyrin, GAD, and synapsin formed colocalized clusters (B-E) around somata and dendrites (C) indicating GABAergic synaptic differentiation. Arrows show absence of $beta$ -dystroglycan (A-C) and dystrophin (A) at synapses and GABA_AR (B) and gephyrin (C) clustering in the absence of $beta$ -dystroglycan; arrowheads indicate GABA_AR colocalized with gephyrin (D) and GAD (E). Scale bar, 10 µm.

Adenovirus-Cre treatment (at MOI 10) of wild-type neurons did not affect dystroglycan expression (Fig. 5A), whereas the sametreatment effectively excised dystroglycan from the vast majorityof cells in culture [6% of cells exhibited dystroglycan clustersafter adenovirus-Cre treatment vs 84% in sister cultures withoutvirus-mediated excision (Fig. 5, C vs B)]. The absence of dystroglycanfrom neurons after excision at 1 week in culture is consistentwith the result (Fig. 3) that these neurons have accumulated littleif any dystroglycan at earlier times. The dystroglycan $-$ / $-$ neuronscontinued to elaborate axons and dendrites for an additional 10-12d (analysis at 17-19 d in vitro) (Fig. 5E). Moreover, the neuronsformed numerous synapsin-rich presynaptic nerve terminals, includingsome that were GABAergic (GAD-positive) (Fig. 5C,D). Thus, althoughwe cannot rule out the possibility that low levels of dystroglycanare essential for initiation of neuronal differentiation, formationof elaborate processes and differentiation of nerve terminalscan occur in itsabsence.

In view of these results, we were able to use the Cre-expressing DG lox/lox cultures to ask whether dystroglycan was necessaryfor formation or maintenance of the postsynaptic membrane at GABAergicsynapses. We observed no dystrophin clusters in Cre-treated neurons(Fig. 6A) except for very few colocalized with the remaining dystroglycan.This defect was more striking than that documented above for mdxmice, indicating that dystroglycan is necessary for concentrationof both full-length and short forms of dystrophin at GABAergicsynapses. However, no other differences in GABAergic synapticdifferentiation were observed. Cre-excised DG lox/lox culturesformed colocalized accumulations of synaptic vesicles, GAD, gephyrin,and GABA_AR $alpha$ 1, $alpha$ 2 and $gamma$ 2 (Fig. 6B-E) ( $alpha$ 1 data not shown). Thepercentage of DG lox/lox neurons that exhibited synaptic clustersof GABA_AR $alpha$ 2 was 94% without adenovirus treatment and 89% afteradenovirus-Cre excision (data from the same neurons describedabove that showed the 78% loss of dystroglycan immunoreactivity).The amount of adenovirus required to effectively excise dystroglycanresulted in some degree of toxicity for wild-type neurons as wellas DG lox/lox. Thus rigorous quantitative analyses were precluded,and we cannot rule out the possibility of a small reduction inthe density of synaptic GABA_AR clusters attributable to loss ofdystroglycan. Nonetheless, these results indicate that dystroglycanis not a required signaling component for the fundamental aspectsof GABAergic synaptogenesis, formation of GABA_AR clusters oppositeGABAergicterminals.

  DISCUSSION

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ABSTRACT
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We report here four major results concerning the regulation and function of the DGC in central neurons. First, $alpha$ -dystroglycan, $beta$ -dystroglycan, and dystrophin are concentrated at a subset ofcentral neuron inhibitory GABAergic synapses. Dystroglycan isthe first adhesive macromolecule identified at mature GABA synapses.Second, dystroglycan accumulates at GABAergic synapses late indevelopment, after clustering of synaptic vesicles, GAD, gephyrin,and GABA_AR. Third, gephyrin, agrin, and full-length dystrophinare all dispensable for localization of dystroglycan to GABA synapses.Fourth, dystroglycan $-$ / $-$ neurons develop GABAergic synapses containingclusters of GABA_AR and gephyrin opposite GAD-labeled terminals.The only detectable defect in the absence of dystroglycan wasthe absence of dystrophin clusters at GABA synapses. Thus theDGC is not essential for assembly of GABAergic synapses but islikely to function in synapticmodulation.

Molecular assembly of GABAergic synapses

Our data indicate the following sequence of GABAergic synaptic assembly: presynaptic vesicle clusters, then gephyrin and GABA_AR,and then the DGC. In cultured spinal neurons, clustering of theGABA_AR opposite inhibitory terminals was observed before the accumulationof gephyrin (Dumoulin et al., 2000). We have also observed somesynaptic GABA_AR clusters in gephyrin $-$ / $-$ hippocampal neurons (ourunpublished data). Thus, in contrast to the early report of Kneusselet al. (1999) of a complete absence of GABA_AR clusters in gephyrin $-$ / $-$ hippocampal neurons, our data agree with the recent analysesof retinal cultures and spinal cord (Fischer et al., 2000; Kneusselet al., 2001) indicating the presence of some albeit reduced GABA_ARclusters in gephyrin $-$ / $-$ neurons. Interestingly, analysis of corticalcultures from GABA_AR $gamma$ 2 $-$ / $-$ mice revealed a large reduction insynaptic clustering of gephyrin as well as GABA_AR $alpha$ 1 and $alpha$ 2 (Essrichet al., 1998). However, direct binding between gephyrin and GABA_ARhas not been observed (Meyer et al., 1995), and the presence ofgephyrin at a synapse is not sufficient to induce accumulationof GABA_AR (Levi et al., 1999). One attractive idea was that gephyrinorganized the GABAergic postsynaptic membrane via interactionwith the DGC, but our results have excluded this possibility.Thus the precise role of gephyrin in GABAergic synaptogenesisremains to be defined, particularly how gephyrin functions toinduce or maintain the normal synaptic density of some GABA_ARsubunits and how this contributes to synapticfunction.

The DGC detectably associated with only a subset of GABAergic synapses and only late in development. The DGC complex at GABAsynapses includes $alpha$ -dystroglycan, $beta$ -dystroglycan, full-lengthdystrophin, and dystrophin short forms (Figs. 2, 4). Full-lengthdystrophin has also been found at GABAergic synapses in hippocampaltissue (Knuesel et al., 1999). In mdx neurons lacking full-lengthdystrophin, dystroglycan and some dystrophin short forms stilllocalized to GABAergic synapses (Fig. 4). In contrast, in neuronslacking dystroglycan, dystrophin isoforms were not detected atGABA synapses (Fig. 6). Thus dystroglycan is an essential componentfor formation of the DGC complex at GABA synapses, but dystrophinis not. Furthermore, neither agrin nor gephyrin was required forassembly of the DGC at GABA synapses (Fig. 4). We could find noevidence of a genetic interaction between gephyrin and dystroglycanin the sense that either assembled at GABA synapses in the absenceof the other, and neither could compensate for loss of the other.Dystroglycan did not rescue GABA_AR clustering in the absence ofgephyrin, and gephyrin did not rescue dystrophin clustering inthe absence ofdystroglycan.

Function of the dystrophin-associated glycoprotein complex at GABAergic synapses

The presence of the adhesive macromolecule dystroglycan at GABA synapses raised the intriguing possibility that it might functionas a key trans-neuronal signal for synaptogenesis. Although wecould detect dystroglycan accumulated at only a subset of maturesynapses, it might be present at lower levels at developing GABAergicsynapses. The findings that $alpha$ -dystroglycan binds agrin and $alpha$ -and $beta$ -neurexins via their extracellular domains (Bowe et al.,1994; Campanelli et al., 1994; Gee et al., 1994; Sugiyama et al.,1994; Sugita et al., 2001) further supported this possibility.Agrin is essential for synaptogenesis at the NMJ (Sanes and Lichtman,1999; Lin et al., 2001), and acute inhibition of agrin expressionalters the morphological development of hippocampal neurons inculture (Bose et al., 2000). The apparent absence of phenotypein hippocampal cultures from agrin mutant mice (Fig. 4) (Serpinskayaet al., 1999) could result from compensatory mechanisms. Neurexinsare a large family of alternatively spliced neuron-specific surfaceproteins implicated in synaptic specificity (Missler et al., 1998).However, we find here that dystroglycan is not essential for GABAergicsynaptogenesis; GABA_AR clustered opposite GABA terminals in theabsence of dystroglycan (Fig. 6). These results do not rule outroles for agrin or neurexin, both of which have alternative receptors.For example, $beta$ -neurexins also bind neuroligin, an excitatory postsynapticprotein that can induce presynaptic specializations in contactingaxons (Song et al., 1999; Scheiffele et al., 2000). Moreover,it is still possible that dystroglycan is required for genesisof a small subset of GABA synapses; better methods for excisingdystroglycan without long-term side effects will be required totest this possibility. Compensatory mechanisms that may mask afunction for dystroglycan seem unlikely, because dystroglycanwas excised after 1 week in culture rather than from the onsetof development. Functional redundancy may occur for other componentsof the DGC, but this also seems unlikely for dystroglycan, asdemonstrated with respect to its roles in non-neuronal cells (Williamsonet al., 1997).

The other possibility, which we favor, is that dystroglycan plays a modulatory rather than an organizing function at manyGABAergic synapses. The cytoplasmic C terminus of $beta$ -dystroglycaninteracts with the Src homology 3 domains of Grb2, an adaptorprotein involved in signal transduction and cytoskeletal reorganization(Yang et al., 1995). Evidence from brain synaptosomes indicatesa Grb2-mediated interaction between $beta$ -dystroglycan and focal adhesionkinase, a tyrosine kinase involved in intracellular transductionpathways (Cavaldesi et al., 1999). Furthermore, Grb2 and dystrophincompete for binding to $beta$ -dystroglycan (Russo et al., 2000). Theseinteractions suggest that dystroglycan may be part of a dynamicallyregulated signal transductionpathway.

Taken together, our data suggest that the DGC forms a transmembrane linkage containing dystrophin, dystrophin short forms, $beta$ -dystroglycan, and $alpha$ -dystroglycan, which binds agrin and $alpha$ - and $beta$ -neurexins. The simplest model is that neurexins and agrin areon the presynaptic side, and dystroglycan and dystrophin are postsynapticat GABA synapses. However, there is little direct evidence (Lidovet al., 1990) to support this model, and the possibility thatthe DGC may be presynaptic needs to be tested by ultrastructurallocalization. Similar to its function at the NMJ (Adams et al.,2000; Grady et al., 2000; Jacobson et al., 2001), the DGC maybe involved in regulating GABA_AR stability or other aspects ofpostsynaptic response. Alternatively, similar to its functionin photoreceptors (Blake and Kroger, 2000), the DGC may be involvedin regulating GABA release. Finally, given the transmembrane natureof the complex, the DGC may be involved in regulating coordinatedaspects of presynaptic and postsynaptic plasticity at GABAsynapses.

  FOOTNOTES

Received Nov. 21, 2001; revised Feb. 26, 2002; accepted March 1, 2002.

This work was supported by National Institutes of Health Grants NS34448 and NS33184. M.D.H. was supported by a National ResearchService Award grant, and K.P.C is an investigator of the HowardHughes Medical Institute. We thank Dr. Jean-Marc Fritschy forgifts of antibodies and Huaiyang Wu for excellent technicalassistance.

Correspondence should be addressed to Dr. Ann Marie Craig, Department of Anatomy and Neurobiology, Washington University Schoolof Medicine, 660 South Euclid, Campus Box 8108, St. Louis, MO63110. E-mail: acraig{at}pcg.wustl.edu.

M. D. Henry's present address: Millenium Pharmaceuticals Inc., Cambridge, MA02139.

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