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Previous Article | Next Article
The Journal of Neuroscience, July 1, 2002, 22(13):5393-5402
Gephyrin Interacts with Dynein Light Chains 1 and 2, Components of Motor Protein Complexes
Jens C. Fuhrmann1, Stefan Kins1, Philippe Rostaing2, Oussama El Far1, Joachim Kirsch1, Morgan Sheng3, Antoine Triller2, Heinrich Betz1, and Matthias Kneussel1 1 Max-Planck-Institute for Brain Research, Department of Neurochemistry, D-60528 Frankfurt/Main, Germany, 2 Laboratoire de Biologie Cellulaire de la Synapse, Institut National de la Santé et de la Recherche Médicale U497, Ecole Normale Supérieure, 75005 Paris, France, and 3 Center for Learning and Memory, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The clustering of glycine receptors and major subtypes of GABAA receptors at inhibitory synapses is mediated by the tubulin-binding protein gephyrin. In an attempt to identify additional components of inhibitory postsynaptic specializations, we performed a yeast two-hybrid screen using gephyrin as bait. Multiple positive clones encoded either the dynein light chain-1 (Dlc-1), also known as dynein LC8 and protein inhibitor of neuronal nitric oxide synthase, or its homolog Dlc-2. Dlc-1 protein bound efficiently to gephyrin in in vitro binding assays and colocalized with gephyrin during coexpression in HEK293 cells. The binding site for Dlc was mapped to a fragment of 63 amino acids within the central linker domain of gephyrin. In hippocampal neurons, endogenous Dlc protein was enriched at synaptic sites identified by synaptophysin and gephyrin immunostaining. Immunoelectron microscopy in spinal cord sections revealed Dlc immunoreactivity at the edges of postsynaptic differentiations, in close contact with cytoskeletal structures and at the periphery of the Golgi apparatus. Because Dlc-1 and Dlc-2 have been described as stoichiometric components of cytoplasmic dynein and myosin-Va complexes, our results suggest that motor proteins are involved in the subcellular localization of gephyrin.
Key words: gephyrin; cytoplasmic dynein; myosin-Va; Dlc-1; PIN; LC8; Dlc-2; inhibitory synapse; motor protein
INTRODUCTION
Efficient neurotransmission at chemical synapses requires a high local concentration of synaptic proteins, such as components of the neurotransmitter release machinery and postsynaptic receptors. At the molecular level, this high extent of synaptic specialization is thought to result from both targeted delivery of individual constituents and selective stabilization of correctly formed structures (Craig and Banker, 1994
; Hirokawa et al., 1996
-subunit (Meyer et al., 1995
In contrast to the wealth of data on anchoring mechanisms, little is known about the postsynaptic targeting of neurotransmitter receptors or scaffolding proteins. A first connection between a motor protein and postsynaptic cargo molecules was identified in the case of the mLin2/mLin7/mLin10/NMDA receptor complex and the kinesin isoform KIF17 (Setou et al., 2000
MATERIALS AND METHODS
Unless stated otherwise, chemicals were of analytical grade and purchased from Sigma (Taufkirchen, Germany).
Yeast two-hybrid screening. A cDNA fragment encompassing the open reading frame of the gephyrin splice variant p1 (Prior et al., 1992
Coimmunoprecipitation. A cDNA fragment encompassing the open reading frame of Dlc-1 was amplified by PCR and subcloned into a pcDNA3 vector (Invitrogen, Karlsruhe, Germany) that contained sequence encoding the myc epitope tag at the 5' end of the polylinker (kind gift from E. E. Evers, Max-Planck-Institute for Brain Research, Frankfurt, Germany) to allow expression as an N-terminally myc-tagged protein. A previously described pcDNA3-gephyrin construct was used to express untagged gephyrin protein (Grosskreutz et al., 2001
GST pulldown assays. The cDNA sequence of Dlc-1 (including 84 bp of 5'-UTR) was recovered from pJG4-5 by restriction digest with EcoRI/XhoI and subcloned into pGEX5X-1 (Amersham Biosciences). To generate a control construct, the same 5'-UTR fragment and sequence encoding amino acids 1-15 of Dlc-1 followed by a stop codon were amplified by PCR and cloned into the EcoRI/XhoI sites of pGEX5X-1. pGEX5X-1-gephyrin was obtained by subcloning an EcoRI/XhoI fragment from the gephyrin cDNA p1 (Prior et al., 1992
Heterologous expression in HEK293 cells. pEGFP-N3-gephyrin encodes a gephyrin-enhanced green fluorescent protein (EGFP) fusion protein and was generated by replacing the stop codon in the gephyrin cDNA p1 (Prior et al., 1992
Primary cultures of rat hippocampal neurons. Hippocampi were dissected from embryonic day 18 (E18) rat embryos (Wistar) and incubated with 0.5 mg/ml papain and 10 µg/ml DNase I in PBS containing 10 mM glucose for 15 min at 37°C. After washing once in DMEM supplemented with 10% (v/v) fetal calf serum (Invitrogen), 25 µg/ml pyruvate, and 2 mM glutamine, cells were dissociated by trituration and seeded in DMEM containing supplements at a density of 30,000-60,000 cells per well onto 14 mm glass coverslips coated with poly-L-ornithine (1.5 µg/ml). After 3 hr, the medium was replaced with Neurobasal medium containing 2 mM glutamine, 25 µg/ml pyruvate, and 2% (v/v) B27 supplement (Invitrogen). All media contained 50 IU/ml penicillin and 50 µg/ml streptomycin (Invitrogen). At 3 d in vitro (DIV), 3 µM 1-
/
Transfection of hippocampal neurons. Neurons cultured at a density of 60,000 cells/14 mm coverslip were transfected at day 12 or 13 in vitro by a calcium phosphate precipitation protocol. Per well, 2 µg of DNA in 12.5 µl of 250 mM CaCl2, mixed with the same amount of 2× N,N-bis-(2-hydroxyethyl)-2-aminoethane sulfonic acid-buffered saline, pH 6.95, were added to the culture medium. For each transfection, 0.5 µg of gephyrin expression vector and 1.5 µg of pcDNA3 vector (Invitrogen) were used. The precipitate was carefully removed after 1 hr and replaced by 350 µl of conditioned medium and 150 µl of fresh Neurobasal medium.
Immunofluorescence staining. Cells were fixed with 4% (w/v) paraformaldehyde (PFA)-PBS for 12 min, permeabilized with 0.2% (v/v) Triton X-100 for 4 min, and then blocked with 1% (w/v) bovine serum albumin (Applichem, Darmstadt, Germany) in PBS for 30 min. Antibody staining was performed by incubation for 2 hr with primary antibodies and 45 min for secondary antibodies in blocking buffer. GFP was visualized by autofluorescence. The following antibodies were used: monoclonal antibody mAb7 against gephyrin (Pfeiffer et al., 1984
Immunoelectron microscopy. Adult Sprague Dawley rats were anesthetized with pentobarbital (60 mg/kg body weight) and intracardially perfused with 4% (w/v) PFA and 0.1% (w/v) glutaraldehyde in PBS. After dissection, the cervical spinal cord was kept overnight in 4% PFA at 4°C. Vibratome sections (100 µm) were cryoprotected [3 hr in 20% (v/v) glycerol and 20% (w/v) saccharose in PBS], permeabilized by freeze thawing, extensively rinsed in PBS, and immersed for 20 min in 50 mM ammonium chloride and for 30 min in PBS containing 0.1% (w/v) gelatin (PBSg). For the detection of Dlc, vibratome sections were incubated for 12 hr at 4°C in PBSg with rabbit anti-Dlc antibody (1:10), and antibody binding sites were detected using a goat biotinylated (1:100 in PBSg; Vector Laboratories, Burlingame, CA) or nanogold-coupled anti-rabbit antibody (1:100 in PBSg; Nanoprobe, Stony Brook, NY). For detection of gephyrin, a monoclonal antibody was used (1:100; Alexis, San Diego, CA). The biotinylated antibodies were revealed using an ABC immunoperoxidase method (Elite Vectastain; Vector Laboratories) (for details, see Colin et al., 1998
RESULTS
Identification of Dlc-1 and Dlc-2 as interaction partners of gephyrin
To identify novel gephyrin-binding proteins, we performed a yeast two-hybrid screen using the full-length gephyrin clone p1 as bait. From ~2.3 × 106 clones of an adult rat brain library, 150 LEU2- and lacZ-positive clones were isolated. Among these, 32 independent clones coded for rat Dlc-1/PIN [for protein inhibitor of neuronal nitric oxide synthase (nNOS)] (Jaffrey and Snyder, 1996
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Figure 1. Interaction between gephyrin and Dlc-1/2 in the yeast two-hybrid system. A, Amino acid sequence of rat Dlc-1 and Dlc-2. Identity is indicated by a vertical bar. B, Schematic diagram showing the results from yeast two-hybrid analysis of the interaction between gephyrin and Dlc-1/Dlc-2. Interaction was assayed by lacZ/LEU2 reporter gene induction on agar plates and scored as + (blue color visible after 24 hr; this is comparable with gephyrin interacting with the cytoplasmic loop of the GlyR
To identify the exact region of gephyrin that interacts with Dlc-1/2, we generated deletion constructs and tested their binding to Dlc-1/2 in the yeast two-hybrid system. A fragment encompassing amino acids 153-348 of gephyrin, which link the N- and C-terminal domains bearing homology to enzymes involved in molybdenum cofactor biosynthesis (Prior et al., 1992
Gephyrin binds to Dlc-1/2 in vitro
Coimmunoprecipitation and GST pulldown assays were used to substantiate the interaction of gephyrin and Dlc-1/2 biochemically. Myc-tagged Dlc-1 and gephyrin were expressed in HEK293 cells and immunoprecipitated using antibodies specific for the myc epitope or gephyrin. Both recombinant proteins were expressed efficiently, in addition, lower amounts of endogenous gephyrin and Dlc-1/2 could be detected (Fig. 2A). Both endogenous and recombinant gephyrin were specifically coprecipitated by anti-myc antibodies, because no enrichment was observed when myc-Dlc-1 was omitted from the transfection. When anti-gephyrin antibodies were used for precipitation, myc-Dlc-1 was similarly enriched in the immunoprecipitate (Fig. 2A). This interaction was specific because only low amounts (data not shown) of myc-Dlc-1 could be precipitated when gephyrin was not overexpressed.
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Figure 2. Binding between gephyrin and Dlc-1/2 in vitro. A, Dlc-1 tagged with a myc epitope coimmunoprecipitates with gephyrin from transfected HEK293 cells. Myc-Dlc-1 and gephyrin were expressed alone or in combination, and the presence of the recombinant proteins, as well as lower amounts of endogenous proteins, were confirmed in the input lanes. Complexes between myc-Dlc-1 and gephyrin were precipitated by either myc- or gephyrin-specific antibodies immobilized on protein G-Sepharose. Both endogenous and recombinant gephyrin were specifically coimmunoprecipitated with myc-Dlc-1, and antibodies against gephyrin precipitated myc-Dlc-1 when gephyrin was overexpressed. IP, Immunoprecipitate; G, gephyrin; HC, antibody heavy chains; LC, antibody light chains; Dlc, Dlc-1/2. B, GST-Dlc-1 pulls down gephyrin from rat brain. Glutathione Sepharose beads were loaded with either GST-Dlc-1 or a truncated control protein. Beads containing GST-Dlc-1, but not the control protein, retained gephyrin from the brain lysate, as demonstrated by immunoblotting with a gephyrin-specific antibody. C, GST-gephyrin specifically enriches Dlc-1/2 from rat brain. The experiment was performed as in B using GST-gephyrin and GST as the negative control. Detection with an antibody recognizing Dlc-1 and Dlc-2 revealed specific binding to GST-gephyrin. D, Amino acids 181-243 of gephyrin are required for interaction with Dlc-1. Wild-type and mutant gephyrin-GFP were expressed in HEK293 cells and tested for binding to GST-Dlc-1. Gephyrin-GFP (top band) and endogenous gephyrin (bottom band) were specifically retained by GST-Dlc-1, whereas gephyrin( 181-243)-GFP (middle band) did not bind. No significant binding was detected when a truncated control protein was used instead of GST-Dlc-1 (data not shown).
In additional experiments, GST pulldown assays were performed with both GST-Dlc-1 and GST-gephyrin to isolate interacting proteins from a rat brain lysate. A fusion protein of GST and Dlc-1 (GST-Dlc-1) and a control protein encoding a truncated GST-Dlc-1 protein (amino acids 1-15 of Dlc-1 only) or GST-gephyrin and GST, respectively, were expressed in Escherichia coli. Glutathione-Sepharose beads loaded with these GST fusion proteins were incubated with rat brain lysate. Gephyrin was specifically retained on beads charged with GST-Dlc-1 but did not bind to beads containing the truncated control protein (Fig. 2B). In complementary assays, Dlc-1/2 was specifically enriched upon binding to GST-gephyrin, whereas no interaction with GST alone was observed (Fig. 2C). Thus, the interaction of gephyrin with Dlc-1/2 could be verified by two independent biochemical assays.
The GST pulldown assay was also used to confirm the relevance of the Dlc-binding motif characterized in the yeast two-hybrid system. The cDNA sequence corresponding to amino acids 181-243 of gephyrin, which were sufficient for Dlc binding in the yeast-two hybrid system (Fig. 1B), was deleted, yielding gephyrin(
Colocalization of gephyrin and Dlc-1/2 in HEK293 cells
To investigate whether gephyrin and Dlc-1/2 interact in mammalian cells, we expressed both proteins in HEK293 cells and examined their subcellular localization. Under these conditions, gephyrin spontaneously forms cytoplasmic aggregates (Meyer et al., 1995
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Figure 3. Recombinant and endogenous Dlc-1/2 colocalize with gephyrin in transfected HEK293 cells. A, Gephyrin-GFP overexpression leads to the formation of characteristic aggregates in HEK293 cells (arrow), whereas myc-Dlc-1 transfected alone displays a diffuse cytoplasmic distribution (B). Endogenous Dlc protein is localized in the cytoplasm with no obvious compartmentalization (C). Both endogenous and recombinant Dlc proteins also show nuclear localization to a variable degree. D, Double transfection of gephyrin-GFP (green) and myc-Dlc-1 (red) leads to recruitment of Dlc-1 to gephyrin aggregates (arrows), indicating an interaction between both proteins. Overlap of both signals is indicated yellow in the merged picture. E, In cells transfected with cDNA for gephyrin-GFP alone, endogenous Dlc protein (red) colocalizes with aggregates of gephyrin (green, arrows). Merge is shown in yellow. Note the homogenous distribution of Dlc in the untransfected cell to the left. F, Gephyrin-GFP(
Human Dlc-1 and, to a lesser extent, Dlc-2 are expressed in a variety of tissues, including kidney (Naisbitt et al., 2000
We also expressed gephyrin(
Dlc-1/2 show both cytoplasmic and synaptic localization in cultured neurons
To examine whether Dlc-1/2 colocalize with gephyrin at inhibitory synapses, we stained primary hippocampal neurons differentiated for 20 d in vitro with antibodies against Dlc. In addition to a granular cytoplasmic distribution, similar to that observed in HEK293 cells, punctate Dlc immunoreactivity was found along the plasma membrane of dendrites and cell bodies (Fig. 4A,B). By double labeling, this pattern was compared with the localization of gephyrin and a general presynaptic marker protein, synaptophysin. The Dlc-immunoreactive punctae colocalized well with the synaptophysin signal, indicating synaptic localization (Fig. 4A). A major fraction, but not all, of the Dlc-positive sites also stained positive for gephyrin (Fig. 4B, arrow indicates lack of colocalization). A similar result was obtained in spinal cord neurons cultured for 16 d in vitro (data not shown). The incomplete colocalization of Dlc-immunoreactive punctae with gephyrin, but good correlation with synaptophysin-positive terminals, indicates that Dlc is enriched at inhibitory and excitatory synapses.
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Figure 4. Gephyrin and Dlc colocalize at inhibitory synapses in cultured hippocampal neurons. Hippocampal neurons were cultured for 20 DIV and stained for the indicated proteins. A, Colocalization of Dlc and synaptophysin at synaptic sites. The merged image shows synaptophysin immunoreactivity in red and Dlc staining in green; overlapping signals are yellow. Dlc is not exclusively synaptic but displays prominent cytosolic staining in addition. Insets, 2× magnification. B, Colocalization of Dlc and gephyrin at inhibitory synapses. Many, but not all, Dlc-positive punctae stain positive for gephyrin. Display as in A. C-E, Dependence of the degree of membrane-associated Dlc immunoreactivity on culture density. Hippocampal neurons were plated at densities of 30,000 (C), 40,000 (D), or 60,000 (E) per 14 mm coverslip and allowed to differentiate for 20 DIV. Dlc staining reveals variable ratios of cytosolic and submembranous Dlc signal intensity. Note the high number of fine neurites, likely to represent both axons and dendrites, in the high-density culture. Scale bars, 10 µm.
While investigating the subcellular localization of Dlc proteins in cultured hippocampal neurons, we noticed a variability between individual cells in the extent of synaptic Dlc immunoreactivity that seemed to depend on the density of neighboring cells and neurites. Therefore, we plated hippocampal cultures at different densities and performed immunostaining for Dlc after 20 d in vitro. In high-density cultures (60,000 cells per coverslip) (Fig. 4E), Dlc immunoreactivity was intensely cytoplasmic, with almost no detectable enrichment at synaptic sites. At lower cell densities (30,000 and 40,000 cells per coverslip) (Fig. 4C,D), the synaptic localization of Dlc became apparent and cytosolic staining decreased to low levels (Fig. 4C). The same observation was made in cultures maintained for 11 DIV (data not shown), excluding effects on cell survival. The presence of Dlc immunoreactivity at inhibitory postsynaptic sites provides evidence for a physiological relevance of the interaction between Dlc-1/2 and gephyrin in neurons. Our findings also suggest that this interaction is subject to a regulatory process that might be linked to the extent of cell interactions.
Postsynaptic localization of Dlc demonstrated by immunoelectron microscopy
The enrichment of Dlc at synaptic sites was examined at the EM level in the ventral spinal cord in which neuronal activity is controlled by glycine- and GABA-mediated inhibition (Todd et al., 1996
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Figure 5. Ultrastructural localization of Dlc immunoreactivity in neurons. A1-A2, Detection of Dlc immunoperoxidase associated electron-dense deposits (arrows) at postsynaptic differentiations adjacent to synaptic boutons containing pleiomorphic populations of synaptic vesicles. Note that not all postsynaptic differentiations associated with a synaptic bouton contain Dlc-associated immunoreactivity (asterisk in A2). B, Detection of Dlc-associated electron-dense deposits (arrow) in front of a synaptic bouton containing spherical synaptic vesicles. C, Detection of Dlc-IR at the membrane of the Golgi apparatus (Go) with gold-toned silver-intensified nanogold particles (arrows). D, Two examples of simultaneous detection of gephyrin-associated electron-dense immunoperoxidase deposits and Dlc-associated gold-toned silver-intensified nanogold particles (arrows). Note that the Dlc immunoreactivity predominates at the periphery of the postsynaptic differentiations. Scale bar: A1, 0.50 µm; A2, 0.85 µm; B, 0.30 µm; C, 0.44 µm; D1, 0.40 µm; D2, 0.60 µm.
Dlc binding is not essential for the synaptic localization of gephyrin in neurons
Dlc-1 has been proposed to serve as an adaptor between the cytoplasmic dynein motor complex and cargo molecules (King, 2000
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Figure 6. Gephyrin targeting to inhibitory synapses in transfected hippocampal neurons does not require the Dlc-binding domain. A, GFP-gephyrin accumulates at inhibitory synapses. Hippocampal neurons cultured for 12 DIV were transfected with pEGFP-C2-gephyrin. After 20 hr, cells were fixed and stained for VIAAT (red) to indicate inhibitory terminals. GFP autofluorescence is shown in green, and merge between red and green channels is shown in yellow. GFP-gephyrin forms numerous hotspots near the plasma membrane of cell body and dendrites, the large majority of which colocalize with VIAAT immunoreactivity. B, GFP-gephyrin(
Quantification of the colocalization between GFP-gephyrin clusters and VIAAT immunoreactivity by automated image analysis yielded values of 62.8 and 72.4%, respectively, for the cells shown in Figure 6, A and B. We applied this analysis to the complete data sets of two independent experiments, regardless of GFP-gephyrin expression levels. The actual numbers thus are not absolute but can be used for comparison of the two GFP-gephyrin constructs. For GFP-gephyrin, we obtained colocalization values of 46.1 ± 4.2% (mean ± SEM; n = 21 cells) and 38.6 ± 3.5% (n = 30), and clusters of GFP-gephyrin(
Gephyrin is able to oligomerize into higher-order structures (Kirsch et al., 1995
DISCUSSION
Gephyrin binds to dynein light chains 1 and 2
Here, we used yeast two-hybrid screening to identify Dlc-1/2 as novel binding partners of the postsynaptic scaffolding protein gephyrin. Deletion analysis showed that this interaction was mediated by amino acids 181-243 of gephyrin. Gephyrin bound to GST-Dlc-1 in a pulldown assay, whereas a gephyrin mutant lacking amino acids 181-243 displayed no binding. Also, gephyrin and Dlc proteins were found to interact in transfected HEK293 cells, as evident from coimmunoprecipitation and the recruitment of both recombinant and endogenous Dlc-1/2 to cytoplasmic gephyrin aggregates. In conclusion, we showed by four independent approaches that gephyrin binds to Dlc proteins and that amino acids 181-243 of gephyrin are both necessary and sufficient to mediate this interaction.
Multiple interaction partners of gephyrin are known (Kneussel and Betz, 2000
Subcellular localization of Dlc proteins in neurons
Immunostaining of cultured hippocampal neurons and immunoelectron microscopy of rat spinal cord sections revealed an enrichment of Dlc-1/2 at inhibitory synapses positive for gephyrin. Thus, an interaction between both proteins is likely to occur in neurons, in which gephyrin serves as a structural protein essential for the clustering of neurotransmitter receptors at inhibitory synapses. Dlc immunoreactivity was not enriched at all inhibitory synapses, however. In primary hippocampal neurons cultured at high density, Dlc immunoreactivity was distributed rather uniformly in the cytosol, and immunoelectron microscopy consistently identified a fraction of gephyrin-positive synapses negative for Dlc. This variability and the preferential localization of Dlc proteins at the edges of postsynaptic specializations suggest that Dlc-1/2 are unlikely to be structural components of inhibitory synapses.
Dlc-1/2 are also enriched in dendritic spines of hippocampal neurons, in which they colocalize with GKAP and PSD-95 (Naisbitt et al., 2000
Dlc-1/2 are subunits of cytoplasmic dynein and myosin-Va
Mammalian Dlc proteins were first described as light chains of cytoplasmic dynein (King et al., 1996
Dlc proteins form dimers in which both monomers can bind to ligands (Tochio et al., 1998
Evidence for an involvement of Dlc in dynein-mediated transport comes from Drosophila, in which Dlc-1 binds to swallow, a protein implicated in the microtubule-dependent asymmetric localization of bicoid mRNA in midoogenesis (Schnorrer et al., 2000
A possible role for motor proteins in gephyrin trafficking
The interaction of gephyrin with Dlc-1/2 suggests that the subcellular localization of gephyrin may depend on motor proteins. Active transport is known mainly for vesicular cargo, and an association with endomembranes has been demonstrated for other synaptic proteins that bind to motor proteins, e.g., the mLin-10/mLin-7/mLin-2 complex or PSD-95 (El-Husseini et al., 2000
Motor protein-mediated transport is a transient process that is likely to affect only a minor fraction of cargo proteins at a given time. Thus, the moderate enrichment of Dlc immunoreactivity at synaptic sites is compatible with the interpretation that Dlc proteins link gephyrin to an active transport process. In this context, complexes of gephyrin and Dlc-1/2 could represent either active motor units or cargo protein preselected for transport. We attempted to examine whether Dlc-1/2 and associated motor proteins might be required for the subcellular trafficking of gephyrin. However, our transfection experiments using mutant GFP-gephyrin(
The interaction of gephyrin with Dlc-1/2, i.e., subunits of cytoplasmic dynein and myosin-Va, supports the idea that gephyrin deposition at and/or removal from synapses may be regulated in a highly dynamic manner. A precise control of the number of gephyrin molecules is important for synaptic efficacy, because the size and density of the gephyrin scaffold will directly influence the number of postsynaptic receptors and thus the size of the synaptic response (Lim et al., 1999
FOOTNOTES Received Nov. 13, 2001; revised March 25, 2002; accepted April 10, 2002.
This work was funded by the Deutsche Forschungsgemeinschaft and Fonds der Chemischen Industrie. Jens Fuhrmann was supported by a predoctoral fellowship from the Boehringer Ingelheim Fonds. We thank Bruno Gasnier (Paris, France) for the gift of anti-VIAAT antibody and Ina Bartnik and Dagmar Magalei for expert technical assistance.
Correspondence should be addressed to Heinrich Betz, Max-Planck-Institute for Brain Research, Department of Neurochemistry, Deutschordenstrasse 46, D-60528 Frankfurt/Main, Germany. E-mail: neurochemie{at}mpih-frankfurt.mpg.de.
S. Kins's present address: Center for Molecular Biology, University of Heidelberg, Im Neuenheimer Feld 282, D-69120 Heidelberg, Germany.
J. Kirsch's present address: Department of Anatomy and Cellular Neurobiology, University of Ulm, Albert-Einstein-Allee 11, D-89069 Ulm, Germany.
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