Cupidin, an Isoform of Homer/Vesl, Interacts with the Actin Cytoskeleton and Activated Rho Family Small GTPases and Is Expressed in Developing Mouse Cerebellar Granule Cells

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The Journal of Neuroscience, October 1, 1999, 19(19):8389-8400

Cupidin, an Isoform of Homer/Vesl, Interacts with the Actin Cytoskeleton and Activated Rho Family Small GTPases and Is Expressed in Developing Mouse Cerebellar Granule Cells
Yoko Shiraishi¹^,²^,³, Akihiro Mizutani¹^,³, Haruhiko Bito⁴, Kazuko Fujisawa⁴, Shuh Narumiya⁴, Katsuhiko Mikoshiba¹^,³, and Teiichi Furuichi¹^,²
¹ Department of Molecular Neurobiology, Institute of Medical Science, The University of Tokyo, Minato-ku, Tokyo 108-8639 , Japan, ² Laboratory for Molecular Neurogenesis and ³ Developmental Neurobiology, Brain Science Institute, The Institute of Physical and Chemical Research (RIKEN), Wako, Saitama 351-0198, Japan, and ⁴ Department of Pharmacology, Kyoto University Faculty of Medicine, Sakyo-ku, Kyoto 606-8315, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A developmentally regulated Homer/Vesl isoform, Cupidin (Homer 2a/Vesl-2 $Delta$ 11), was isolated from postnatal mouse cerebellumusing a fluorescent differential display strategy. The strongestexpression of Cupidin was detected in the cerebellar granule cellsat approximately postnatal day 7. Cupidin was enriched in thepostsynaptic density fraction, and its immunoreactivity was concentratedat glomeruli of the inner granular layer when active synaptogenesisoccurred. Cupidin protein could be divided into two functionaldomains: the N-terminal portion, which was highly conserved amongHomer/Vesl family proteins, and the C-terminal portion, whichconsisted of a putative coiled-coil structure, including severalleucine zipper motifs. The N-terminal fragment of Cupidin, whichwas able to associate with metabotropic glutamate receptor 1 (mGluR1),also interacted with F-actin in vitro. In keeping with this, F-actinimmunocytochemically colocalized with Cupidin in cultured cerebellargranule cells, and a Cupidin-mGluR1-actin complex was immunoprecipitatedfrom crude cerebellar lysates using an anti-Cupidin antibody.On the other hand, the C-terminal portion of Cupidin bound toCdc42, a member of Rho family small GTPases, in a GTP-dependentmanner in vitro, and Cupidin functionally interacted with activated-Cdc42in a heterologous expression system. Together, our findings indicatethat Cupidin may serve as a postsynaptic scaffold protein thatlinks mGluR signaling with actin cytoskeleton and Rho family proteins,perhaps during the dynamic phase of morphological changes thatoccur during synapse formation in cerebellar granulecells.

Key words: Cupidin/Homer 2a/Vesl-2 $Delta$ 11; cerebellar development; granule cell; mGluR; actin cytoskeleton; Rho family small GTPases

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuronal migration, neurite extension, and synaptogenesis are three distinct steps that are essential for the maturation ofa neuron and the development of the nervous system. In rodentcerebellar granule cells, in particular, migration and synaptogenesisare sequentially initiated and accomplished within the first 3weeks after birth (Rakic, 1971; Hatten, 1997). During this period,postmitotic granule cells in the external germinal layer (EGL)start to migrate downward into the molecular layer (ML), crawlingalong processes of Bergmann glia, until they reach their finaldestination in the internal granular layer (IGL). In parallelwith these events, the granule cells also extend their T-shapedaxons called parallel fibers (PFs) in the ML. The PFs form synapseswith the growing dendrites of Purkinje neurons. In the IGL, theaxodendritic connections (glomeruli) are formed between the mossyfibers (MFs)-Golgi neurons and the dendrites of the granule cells(Altman and Bayer, 1996).

What are the critical cellular and molecular events in these developmental processes? One fundamental challenge lies in understandingthe mechanisms of dynamic changes performed by the neurons inresponse to extracellular cues available at cell-cell and cell-matrixcontacts and to various classes of diffusible factors and chemicalneurotransmitters. It is believed that extracellular cues directneuronal migration and specify synapse formation with the appropriatetargets during axonal and dendritic outgrowth. Very little, however,is known about the intracellular signaling machinery that regulatesthe motility and shape of cerebellar neurons during these activeneurogenetic stages. To elucidate the molecular basis of theseneuronal events, we have begun to identify genes specificallyexpressed at a distinct stage of the postnatal cerebellar developmentusing a fluorescence differential display (FDD) technique (Itoet al., 1994). We were especially interested in isolating geneswhose expression peaked at approximately postnatal day 7 (P7),because this period matches with the time window when most ofthe dynamic cellular changes described above occur (Altman andBayer, 1996).

Here, we report the isolation of a gene named Cupidin (CPD), which fulfills the criteria of developmentally regulated cerebellargene. Cupidin was named after the Roman god of love, Cupid, becauseCupidin mediated the association of several distinct classes ofmolecules thought to be remote: the actin-cytoskeleton, Rho familyproteins, and metabotropic glutamate receptor 1 $alpha$ (mGluR1 $alpha$ ). Whilethis work was in progress, two other groups independently reportedthe isolation of an isoform of Homer (Brakeman et al., 1997) orVesl (Kato et al., 1997) that was essentially identical to Cupidin,named Homer 2a (Xiao et al., 1998) or Vesl-2 $Delta$ 11 (Kato et al.,1998). Homer/Vesl was initially characterized as an immediateearly gene induced by synaptic-activity (Kato et al., 1997; Brakemanet al., 1997). Here, we show that Cupidin is developmentally regulatedand is enriched at synapses on cerebellar granule cell dendrites.Furthermore, a potential link between mGluR and synaptic actincytoskeleton via Cupidin issuggested.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fluorescence differential display. FDD was performed according to Ito et al. (1994). In brief, 2.5 µg of DNA-free total RNAs,prepared from cerebella of ICR mice (Nippon SLC, Shizuoka, Japan)at various developmental stages [embryonic day 18 (E18), P0, P3,P7, P12, P15, P21, and 8-week-old], were reverse-transcribed usinga Superscript II reverse transcriptase (Life Technologies, Rockville,MD) in the presence of 2.5 µM anchored oligo-dT primers 5'-GT₁₅A-3'.PCR was performed using an ExTaq polymerase kit (Takara Shuzo,Kyoto, Japan), the anchored primer, and arbitrary primers (10-mer),essentially as described by Ito et al. (1994). Clone 13-2 wasgenerated using 5'-GTTTTCGCAG-3' as an arbitrary primer. The PCRproducts were separated on a 6% polyacrylamide gel and analyzedby a computerized-fluorescent image analyzer FluorImager (AmershamPharmacia Biotech, Piscataway, NJ) after staining with the fluorescentdye SYBR Green I (Takara Shuzo). Bands of interest were excisedfrom FDD gels and were reamplified as described previously (Itoet al., 1994). Reamplified DNA fragments were cloned into thepT7Blue TA cloning vector (Novagen, Madison, WI) and were sequencedby the dideoxy chain terminationmethod.

Reverse transcription-PCR analysis.A series of first strand cDNAs were produced by reverse-transcription (RT) from 20 ng oftotal cerebellar RNAs at the various developmental stages describedabove, using an oligo-dT primer. PCR was performed using a primerset corresponding to the end sequences of clone 13-2 (5'-CAGGGATGTTTAGATCTTCC-3'and 5'-GTGGTTGACAATGTCATGTC-3'). Cycling conditions were as follows:94°C for 3 min, 25 cycles of 94°C (15 sec), 55°C (2 min), and72°C (1 min), and finally at 72°C for 5 min. The PCR productswere analyzed as described above. To analyze tissue distribution,total RNAs prepared from various tissues of P7 mice were usedfor RT-PCR. RT-PCR for glyceraldehyde-3-phosphate dehydrogenase(GAPDH) was performed with primers 5'-GCCATCAACGACCCCTTCATTGACCTC-3'and 5'-GCCATGTAGGCCATGAGGTCCACCAC-3' as an internalcontrol.

Northern blot hybridization analysis. A total of 10 µg of poly(A⁺) RNA for each sample was resolved by gel electrophoresis andtransferred to a nylon membrane (Biodyne A; Pall BioSupport, EastHill, NY). The blot was hybridized with a random-primed [ $alpha$ -³²P]dCTP-labeled full-length Cupidin cDNAprobe.

In situ hybridization. Digoxigenin-labeled antisense or sense riboprobes were prepared from the nucleotide positions 647-1220[amino acids (aa) 154-343 plus termination codon] of the CupidincDNA using a digoxigenin-dUTP labeling kit (Boehringer Mannheim,Indianapolis, IN). Cryosections of mouse brain (20-µm-thick) werefixed in 4% paraformaldehyde for 15 min, washed twice in PBS,and treated with freshly prepared 50 µg/ml proteinase K (LifeTechnologies) for 10 min at room temperature. After acetylation,sections were subjected to the digoxigenin-based hybridizationprocedures (Kondo et al., 1997). Briefly, sections were incubatedin hybridization buffer containing 0.2 µg/ml digoxigenin-labeledriboprobes at 60°C overnight in a humid chamber. Hybridized sectionswere washed by successively immersing in 1× SSC (150 mM NaCl and15 mM sodium citrate, pH 7.0) (60°C, 10 min, twice), 2× SSC (37°C,10 min), 2× SSC containing 20 µg/ml RNaseA (37°C, 30 min), 2×SSC (37°C, 10 min), and 0.2× SSC (60°C, 30 min, twice). Hybridizationsignals were detected with the digoxigenin detection kit (BoehringerMannheim).

Cloning of mouse Cupidin (Homer 2a/Vesl-2 $Delta$ 11), Homer 1c/Vesl-1L, Homer 2b/Vesl-2, and Homer 3 cDNA. Clone 13-2 obtained fromFDD was used as a probe to clone mouse Cupidin cDNA. Approximately1 × 10⁶ plaques of a cDNA library constructed from P6 cerebella of C57Bl/6Jmice (a kind gift from Dr. M. E. Hatten, Rockefeller University,New York, NY) were screened using a ³²P-labeled probe. Sequencing was performed in both directions bythe dideoxy chain termination method using [ $alpha$ -³²P] dCTP and the BcaBest dideoxy sequencing kit (Takara Shuzo).Homology search with the sequences in the GenBank database wasperformed using the BLAST and FASTA programs. Mouse Homer 1c/Vesl-1L,Homer 2b/Vesl-2, and Homer 3 cDNAs were cloned by PCR-based methodwith specific primer pairs corresponding to the reported cDNAsequences (Xiao et al., 1998). All cDNA sequences cloned wereverified bysequencing.

Expression of glutathione S-transferase fusion proteins in Escherichia coli. Glutathione S-transferase (GST) fusion constructswere made by subcloning various parts of Cupidin cDNA into theGST fusion vector pGEX-KG, and the following constructs were obtained:pGEX-CPD (the full length; aa 1-343), pGEX-CPD/N (the N-terminal111 aa; aa 1-111), and pGEX-CPD/C (the C-terminal 232 aa; aa 112-343).The full-length cDNA of other Homer isoforms were also subclonedinto pGEX-KG. GST fusion proteins were expressed in E. coli JM109and affinity-purified with glutathione Sepharose 4B (AmershamPharmacia Biotech). For cosedimentation assay with F-actin, GSTfusion proteins were further purified through a Mono Q anion exchangecolumn (Amersham Pharmacia Biotech). Concentrations of proteinswere determined using a protein assay kit (Bio-Rad, Hercules,CA) with bovine serum albumin (BSA) as astandard.

Coprecipitation of mGluR1 $alpha$ and GST-CPD/N. P7 mouse cerebra and cerebella were homogenized in an ice-chilled glass Teflon Potterhomogenizer containing 9 vol of homogenizing buffer (0.32 M sucrose,5 mM Tris-HCl, pH 7.5, 1 mM EDTA, 0.1 mM PMSF, 10 µM pepstatinA, and 10 µM leupeptin). The homogenates were centrifuged at 1,000× g for 15 min at 4°C to obtain nuclei-free S1 fractions. Afteradding Trition X-100 to give a final concentration of 0.1%, theS1 fractions were centrifuged at 100,000 × g for 4°C for 1 hr.A 2 ml sample of the lysates (1 mg/ml protein concentration) wasincubated with 50 µg of GST-CPD/N for 1 hr at 4°C. After adding50 µl of glutathione Sepharose beads (50% slurry) (Amersham PharmaciaBiotech), the mixtures were incubated for another 1 hr. The beadswere extensively washed with wash buffer (20 mM Tris-HCl, pH 8.0,0.1 M NaCl, 0.1% Triton X-100, and 1 mM 2-mercaptoethanol). Boundproteins were dissolved in SDS-PAGE sample buffer and were subjectedto Western blot analysis with an anti-mGluR1 $alpha$ antibody (Ryo etal., 1993).

Cosedimentation assay with F-actin. Actin was isolated from acetone powders prepared from chicken skeletal muscle, as describedby Pardee and Spudich (1982). To obtain F-actin, G-actin was allowedto polymerize for 30 min at room temperature by addition of MgCl₂and KCl to final concentrations of 2 and 10 mM, respectively.GST and GST fusion proteins, purified through Mono Q column chromatography,were precleared by centrifugation at 140,000 × g for 20 min atroom temperature before use. F-actin and GST fusion proteins weremixed at concentration of 500 and 280 µg/ml, respectively, ina polymerization buffer (10 mM Tris-HCl, pH 7.0, 50 mM KCl, 1mM MgCl₂, and 1 mM ATP). After incubation for 30 min at room temperature,the mixtures were applied to Ultra-Clear tubes (Beckman Instruments,Fullerton, CA) containing a 30% sucrose cushion in the polymerizationbuffer and were centrifuged at 140,000 × g for 20 min at roomtemperature. The resulting pellets were resuspended to the initialassay volume of the polymerization buffer. Equal amounts of boththe supernatant and the resuspended pellet were then analyzedby 10% SDS-PAGE.

Preparation of anti-Cupidin antibody and coimmunoprecipitation assay. A rabbit polyclonal antibody against Cupidin was raisedagainst a His-tagged CPD/C (aa 112-343) that was bacterially expressed.After preabsorption with GST-Homer 1c immobilized on Sepharose4B (Amersham Pharmacia Biotech), the residual antisera were affinity-purifiedagainst the GST-CPD/C covalently coupled to CNBr-activated Sepharose4B. P7 mouse cerebella (2 gm, wet weight) were homogenized in18 ml of 10 mM Tris-HCl, pH 7.5, 100 mM NaCl, 50 mM KCl, 1% NP-40,5 mM MgCl_2, 1 mM EGTA, 0.1 mM PMSF, 10 µM pepstatin A, and 10µM leupeptin. The homogenate was centrifuged at 16,000 × g for20 min at 4°C, and the supernatant were precleared with ProteinA/G resin (50% slurry) (Cytosignal Inc., Irvine, CA). Aliquotsof the supernatant (125 µl) were incubated with either the affinity-purifiedanti-Cupidin polyclonal antibody or the preimmune serum for 4hr at 4°C and then with an equal amount of Protein A/G resin (50%slurry) for 30 min at 4°C. After washing the resin with homogenizingbuffer five times, bound proteins were analyzed by Western blottingwith the anti-Cupidin, anti-actin (Sigma, St. Louis, MO), or anti-mGluR1 $alpha$ antibodies.

Ligand overlay assay with Rho small GTPases. Bacterially expressed GST-Rho family protein fusions (GST-RhoA, GST-RhoA^A37, GST-Rac1, and GST-Cdc42) and GST-Citron were purified throughglutathione Sepharose column chromatography according to the proceduredescribed previously (Fujisawa et al., 1998). A 1 µg sample ofGST-CPD, GST-CPD/C, and GST-Citron and 3 µg of GST and GST-CPD/Nwere separated by 10% SDS-PAGE and blotted onto nitrocellulosemembrane (Hybond-ECL; Amersham Pharmacia Biotech). Ligand overlayassay was performed as described previously (Matsui et al., 1996).Briefly, after the GST-fusion proteins on the blots were renatured,the protein blots were probed by incubating with each GST-Rhofamily fusion protein loaded with either [³⁵S]GTP $gamma$ S or [³⁵S]GDP $beta$ S at an equal specific activity. After washing three times,the ligand-bound blots were air-dried, and the radioactivitieswere analyzed with a Bioimaging analyzer BAS2000 (Fujix, Tokyo,Japan).

Coimmunoprecipitation of Cupidin and GST-Rho family proteins. Cerebella (0.5 gm, wet weight) from P7 mice were homogenizedin 5 ml of a buffer (10 mM HEPES-KOH, pH 7.4, 100 mM NaCl, 50mM KCl, 5 mM MgCl_2, 1 mM EGTA, 1% NP-40, 0.1 mM PMSF, 10 µM pepstatinA, and 10 µM leupeptin) and then centrifuged at 16,000 × g for20 min at 4°C, and the supernatant was precleared with ProteinG Sepharose beads (Amersham Pharmacia Biotech) for 1 hr at 4°C.Five micrograms of GST, GST-RhoA, GST-Rac1, or GST-Cdc42 expressedin E. coli were incubated with a nucleotide-loading buffer (25mM Tris-HCl, pH 8.0, 2 mM EDTA, 100 mM NaCl, 1 mM MgCl_2, 0.05%Tween 20, 5 mM DTT, and 100 µM GDP or GTP $gamma$ S) for 20 min at 30°C,and the reaction was stopped by adding a quarter volume of stopsolution (25 mM Tris-HCl, pH 8.0, 20 mM MgCl₂, and 100 µM GDPor GTP $gamma$ S). The nucleotide-loaded GST proteins were sequentiallyincubated with the cerebellar supernatants for 1 hr at 4°C witheither the affinity-purified anti-Cupidin polyclonal antibodyor the preimmune serum for 1 hr at 4°C and then with Protein GSepharose beads (50% slurry) for 30 min at 4°C. After washingthe beads with homogenizing buffer five times, proteins boundto the beads were analyzed by Western blotting using an anti-GSTantibody (Amersham PharmaciaBiotech).

Cross-linking assay of Cupidin with Rho family proteins. GST or GST-Rho family proteins expressed in E. coli were loaded witheither GTP $gamma$ S or GDP as described above. GST-CPD proteins weredigested with thrombin, and then GST-free CPD proteins were purifiedthrough Mono Q column. Each protein sample was finally dialyzedagainst a cross-linking buffer (10 mM HEPES-NaOH, pH 7.5, 2 mMEDTA, 1 mM MgCl_2, 0.05% Tween 20, 5 mM DTT, and 1 mM GDP). CPDprotein (25 µg/ml) and each GST-Rho family protein (25 µg/ml)were mixed and incubated for 1 hr at room temperature. Dimethylpimalidate (DMP) (Pierce, Rockford, IL) was added to give a finalconcentration of 10 mM and incubated for another 1 hr at roomtemperature. Equal amount of the DMP-treated protein mixtureswas analyzed by Western blotting using the anti-GSTantibody.

Transient expression of Cupidin in mammalian cells. Cupidin cDNA was subcloned into the pEF-BOS plasmid (Mizushima and Nagata,1990). Green fluorescent protein (GFP)-fused Cupidin (GFP-CPD),GFP-CPD/N, and GFP-CPD/C expression plasmids were constructedby subcloning the corresponding parts of Cupidin cDNA into thepEGFP-C3 (Clontech, Palo Alto, CA). Madin-Darby canine kidney(MDCK) cells were transiently transfected with GFP-CPD expressionplasmids by lipofection using Lipofectamine Plus (Life Technologies).HeLa cells were transiently transfected with pEF-BOS-CPD, pEF-BOS-myc-taggedCdc42^V12, or both. After 30 hr incubation, the cells were fixed in 4%paraformaldehyde, and GFP-fluorescence was observed. For visualizationof intracellular F-actin organization, the cells were probed withTexas Red-conjugated phalloidin. For detection of nontagged CPD,the samples were incubated with the anti-CPD antibody, followedby an FITC-conjugated secondary antibody. Fluorescent images werevisualized using a confocal microscope (MRC1024; Bio-Rad). Imageswere acquired digitally or on films, and pseudocoloring was performedusing Photoshop 3.5 (Adobe, San Jose,CA).

Subcellular fractionation. Subcellular fractionation of P7 mouse cerebella was performed exactly as described previously (Huttneret al., 1983; Carlin et al., 1980).

Immunohistochemistry. Cerebellar granule cells were prepared from P2 ICR mouse cerebella as described previously (Yuzaki andMikoshiba, 1992). The culture was highly enriched in granule cells,and after 14 d in vitro (DIV), only a few calbindin-positive Purkinjecells (2-5 Purkinje cells per 10⁵ plating cells) were detected. In brief, the cerebella from P2mice were treated with 0.1% trypsin (Sigma) and 0.05% DNase I(Boehringer Mannheim) in Ca²⁺-Mg²⁺-free HBSS (Sigma) for 13 min at 37°C. The cells were washed withCa²⁺-Mg²⁺-free HBSS, dissociated by repeated passage through a micropipettetip (200 µl size) in Ca²⁺-Mg²⁺-free HBSS containing 0.05% DNase I and 12 mM MgSO_4, and thenrinsed with the culture medium. Dispersed cells were plated ata density of 2 × 10⁵ cells onto poly-L-lysine (Sigma)-coated glass coverslips (12mm diameter; Matsunami, Tokyo, Japan) in serum-free defined medium:Eagle's medium supplemented with 1 mg/ml BSA, 10 µg/ml insulin,0.1 nM L-thyroxine, 0.1 mg/ml transferrin, 1 µg/ml aprotinin (allfrom Sigma), 30 nM selenium (Merck, Darmstadt, Germany), 0.25%(w/v) glucose, 2 mM glutamin, 2 mg/ml sodium bicarbonate, 0.1mg/ml streptomycin (Meiji, Tokyo, Japan), and 100 U/ml penicillin(Banyu Pharmaceutical Co., Tokyo, Japan). The cultures were maintainedin a humidified atmosphere of 5% CO₂ in air at 37°C. After 7,14, and 21 DIV, respectively, the cells were fixed with 4% paraformaldehydeand treated as described below. For native tissues, ICR mice (P4,P7, P21, and adult) were transcardially perfused with 4% paraformaldehydein PBS( $-$ ), and excised brains were immersed for 2 hr in the samefixative and cryosectioned (8-µm-thick). For immunoreaction, fixedcultured cells or brain sections were preincubated with 2% normalgoat serum and 2% normal horse serum in PBS( $-$ ) for 1 hr and thenincubated with the affinity-purified anti-Cupidin (1.3 µg/ml)and mouse anti-synaptophysin (Sigma) antibodies for 1 hr at roomtemperature. After washing with PBS( $-$ ), the samples were incubatedwith the FITC-conjugated goat anti-rabbit IgG antibody (VectorLaboratories, Burlingame, CA) for Cupidin staining and with TexasRed-conjugated horse anti-mouse IgG antibody (Vector Laboratories)for synaptophysin staining. To visualize F-actin, samples wereincubated with Texas Red-conjugated phalloidin. Immunofluorescencewas observed using a Zeiss (Oberkochen, Germany) Axiophot epifluorescencemicroscope. Conventional immunodetection was also performed byusing diaminobenzidine (DAB) and horse radish peroxidase-conjugatedsecondary antibody. Immunospecificity to Cupidin was confirmedby parallel experiments using the preimmune serum or anti-Cupidinantibody preincubated with excess amounts of the antigenicpolypeptide.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of clone 13-2, a transcript transiently induced during the development of cerebellar cortex

In the course of a systematic FDD study of genes expressed in the developing mouse cerebellum, we identified a PCR productof 323 base pairs, named clone 13-2, with a characteristic expressionpattern: the 13-2 transcript was detected from as early as E18up to P21, with a peak at P7 (Fig. 1A, arrowhead). This time profilecoincided with important events in the development of cerebellarcortex, such as migration of granule cells, dendrogenesis of Purkinjecells, and formation of synapses. RT-PCR analysis using a primerset corresponding to both ends of clone 13-2 confirmed this characteristicdevelopmental expression pattern (Fig. 1B), which was furthersupported by a Northern analysis with a full-length cDNA probe(Fig. 1C, arrowhead). RT-PCR using RNAs prepared from P7 miceshowed that the expression of clone 13-2 was widespread and foundin various tissues at different levels (Fig. 1D).

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Figure 1. Isolation, detection, and expression pattern of clone 13-2/Cupidin during cerebellar development and in various tissues. A, FDD analysis. Cupidin was first detected as a developmentally induced band named clone 13-2, indicated by an arrowhead. B, RT-PCR analysis in the developing cerebellum. RT-PCR for Cupidin was performed using an inner primer set corresponding to the internal sequences of the cloned FDD band. GAPDH was used as an RT-PCR control. C, Poly(A)⁺ RNA (10 µg) was transferred onto a nylon membrane. ³²P-labeled full-length Cupidin cDNA was used as a probe. As a control, a ³²P-labeled GAPDH cDNA was used. D, RT-PCR analysis in various tissues of P7 mice. E, In situ localization of clone 13-2/Cupidin mRNA in the mouse cerebellum. Parasagittal sections of cerebella at P7 and adult stage were probed with the digoxigenin-labeled antisense cRNA probe prepared using a fragment (647-1220 nt) of Cupidin cDNA as a template. The antisense probe recognized two splicing variant forms of Cupidin. Specificity of labeling signals was confirmed using the sense probe (data not shown). PL, Purkinje cell layer. Magnification, 400×. Scale bar, 100 µm.

Cellular localization of clone 13-2 was examined in the developing mouse cerebellum by in situ hybridization analysis (Fig.1E). The cRNA probe used was able to recognize two transcriptsof 1.8 and 6 kb in size, presumably produced by alternative splicing,both of which were predominantly expressed at P7, whereas thesignal of 6 kb transcript was slightly detected at adult (datanot shown). At P7, a strong signal was observed in the majorityof differentiating granule cells in the IGL in addition to migratinggranule cells within the ML. In adult, the signals in the IGLwere greatly reduced, and a very faint signal, probably causedby the 6 kb transcript, was observed in the Purkinje cells (Fig.1E). Together, these results indicated that the expression ofclone 13-2 in the granule cells was induced at either the migratingstage in the ML or the differentiating stage in the IGL, suggestingthat its expression was spatiotemporally regulated during thedevelopment of the cerebellarcortex.

Clone 13-2 is derived from a transcript encoding a multimodular protein, Cupidin

The cDNA sequence of clone 13-2 obtained from FDD showed no homology with any DNA sequence available on the GenBank database.Because clone 13-2 was likely to represent a 3'-noncoding sequenceadjacent to the poly(A⁺) tail, we isolated a full-length cDNA from a P6 mouse cerebellarcDNA library. The entire sequence of the isolated cDNA consistedof 1761 nucleotides, and a putative open reading frame of 343aa (calculated molecular mass of 39,461 Da) was found upstreamof the nucleotide sequence for clone 13-2. From the hydropathyand secondary structure prediction, it was suggested that thisprotein was likely to be a soluble protein with a long $alpha$ -helicalstretch spanning from Ser-90 to near the C-terminal end. Thisprotein contained Arg-81 and 87-GlyLeuGlyPhe-90 sequence, reminiscentof a minimal PDZ [postsynaptic density (PSD)/Discs large/zonaoccludens-1] domain consensus sequence (Fig. 2A). The putativeC-terminal $alpha$ -helical region included several leucine zipper motifsand was predicted to form a coiled-coil structure. Homology searchrevealed that this protein was a close relative of Homer (Brakemanet al., 1997; Kato et al., 1997) and was subsequently found tobe identical to Homer 2a/Vesl-2 $Delta$ 11 (Kato et al., 1998; Xiao etal., 1998). All members of the Homer family share a highly conservedN-terminal 120 aa region homologous to the EVH1 domain [Enabled(Ena)/vasodilator-stimulated phosphoprotein (VASP) homology] (31%aa identity). Interestingly, we found that the C-terminal regionof this protein from Ser-90 to the C terminus revealed a weakidentity (22%) with a portion of Citron, which includes the Rho/Racbinding region and a part of the leucine zipper motif (Madauleet al., 1995) (Fig. 2B).

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Figure 2. Schematic structure of Cupidin and the specificity of anti-Cupidin antibody. A, Schematic representation of the structure of Cupidin and its truncation mutants. CPD is characterized by two major regions: an EVH1-like region, including a single PDZ consensus motif, and a Citron-like coiled-coil region, including leucine zippers. CPD/N (aa 1-111) and CPD/C (aa 112-343) were constructed by deleting the C-terminal portion and the N-terminal portion, respectively. B, Sequence alignment of Cupidin with Citron, a putative target protein for Rho GTPase. Identical amino acids are shaded. The Rho-binding region of Citron is underlined. The C-terminal region of Cupidin (Leu-112 to Leu-336) exhibited a weak identity (22%) with a portion of Citron, including its Rho-binding region. C, Affinity-purified anti-Cupidin antibody specifically recognized a doublet band (44 and 46 kDa) in lysates of P7 mouse cerebellum (20 µg). The bottom 44 kDa band comigrated with Cupidin (CPD- $alpha$ ) expressed in HeLa cells. The top 46 kDa band comigrated with a splice variant of Cupidin (CPD- $beta$ ) expressed in HeLa cells. The antibody did not recognized other Homer family members, Homer 1c and Homer 3.

This identified protein thus contained multiple putative protein-protein interaction motifs and appeared to be a good candidateas an adapter molecule that mediates the association and bindingof distinct classes of proteins. We hereafter refer to this proteinas Cupidin (Homer 2a/Vesl-2 $Delta$ 11).

Interaction with the Rho family small GTPase proteins through the C-terminal region

To examine the relevance of the several putative protein-protein interaction domains, we constructed two deletion mutantsof Cupidin, CPD/N and CPD/C, comprising the N-terminal first 111aa and the C-terminal 232 aa (residues 112-343), respectively(Fig. 2A).

We investigated a possible interaction of Cupidin with Rho family GTPases, because the C-terminal region of Cupidin showedsome homology to the Rho binding site of Citron (Madaule et al.,1995) (Fig. 2B). Using a filter-overlay assay, filters, blottedwith GST-CPD, GST-CPD/N, GST-CPD/C, GST-Citron (GST fused to CitronRho-binding region), and GST were probed with GST-RhoA, GST-RhoA^A37 (GST fused to an effector-binding incompetent mutant of RhoA)(Matsui et al., 1996), GST-Rac1 (GST fused to Rac1), and GST-Cdc42(GST fused to Cdc42), in the presence of either [³⁵S]GTP $gamma$ S or [³⁵S]GDP $beta$ S. As shown in Figure 3A, GST-CPD (lane 1) and GST-CPD/C(lane 3) were intensely labeled with the [³⁵S]GTP $gamma$ S-bound form of GST-RhoA, GST-Rac1, and GST-Cdc42, but onlyweakly with that of GST-RhoA^A37. In contrast, the labeling intensity of GST-Citron (lane 4) wasmuch stronger with [³⁵S]GTP $gamma$ S-bound GST-RhoA compared with the other [³⁵S]GTP $gamma$ S-bound probes, which appears to be consistent with theprevious report (Madaule et al., 1995). For GST-CPD, GST-CPD/C,and GST-Citron, labeling intensities detected with [³⁵S]GDP $beta$ S-bound probes were inferior to those with all [³⁵S]GTP $gamma$ S-bound forms. Neither GST-CPD/N (lane 2) nor GST alone(lane 5) showed any significant labeling with any probes used.These results indicated that the C-terminal region of Cupidin,which shares a weak homology to the Rho/Rac-binding domain ofCitron, was able to interact with Rac1 and Cdc42, as well as RhoA,in a GTP-dependent manner in vitro. A similar result was obtainedwith the other isoforms of CPD (Homer 1c, Homer 2b, and Homer3) (data not shown).

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Figure 3. Cupidin interacts with Rho family small GTPases. A, Direct binding of RhoA, Rac1, and Cdc42 to GST-fused Cupidin in a ligand overlay assay. GST-CPD (lane 1), GST-CPD/N (lane 2), GST-CPD/C (lane 3), GST-Citron (lane 4), and GST (lane 5) were separated by SDS-PAGE, blotted onto nitrocellulose membranes, and probed with [³⁵S]GTP $gamma$ S-bound (top) or [³⁵S]GDP $beta$ S-bound (bottom) forms of each GST-fused Rho family GTPases (RhoA, RhoA^A37, Rac1, Cdc42), as indicated at the top. B, In vitro binding of Cupidin to Cdc42 in a coimmunoprecipitation assay. GST, GST-RhoA, GST-Rac1, and GST-Cdc42, loaded with either GTP $gamma$ S or GDP, were mixed with P7 mouse cerebellar lysates. Each aliquot was immunoprecipitated with either the anti CPD antibody (CPD Ab) or preimmune serum (pre) and was analyzed by Western blot using the anti-GST antibody. Loaded nucleotides and composition of the analyzed mixtures are indicated at the top of each lane. Input, The equivalent mixture without being subjected to immunoprecipitation. C, A cross-link assay of Cupidin. GST, GST-RhoA, GST-Rac1, and GST-Cdc42, loaded with either GTP $gamma$ S or GDP, were mixed with GST-free Cupidin protein. Each aliquot was treated with the cross-linker DMP and analyzed by Western blotting using the anti-GST antibody. Loaded nucleotides and the compo-sition of the analyzed mixture are indicated at the top of each lane. Note that, by cross-linking in the presence of CPD, a part of Cdc42 loaded with GTP $gamma$ S (GTP $gamma$ S-Cdc42) enters a higher molecular weight complex, indicated by arrows.

To confirm the interaction between Cupidin and Rho family small GTPases, we performed two other sets of in vitro binding experiments.First, we tested whether exogenously added GDP- or GTP- loadedRho family proteins were able to be coprecipitated with endogenousCPD proteins from P7 mouse crude cerebellar lysates. We raiseda rabbit polyclonal anti-CPD antibody using a recombinantly expressedC-terminal portion of Cupidin as an antigen. The C terminus showeda very limited homology among Homer/Vesl-family proteins. Theaffinity purified anti-CPD antibody recognized two splice variantsof Cupidin (CPD- $alpha$ , Homer 2a/Vesl-2 $Delta$ 11; CPD- $beta$ , Homer 2b/Vesl-2)(Fig. 2C, top) but did not significantly cross-react with eitherrecombinant Homer 1c or Homer 3 bacterially expressed (Fig. 2C,bottom). The anti-CPD antibody immunoprecipitated both CPD- $alpha$ andCPD- $beta$ from P7 cerebellar lysates. Addition of GDP- or GTP $gamma$ S-loadedRho family proteins did not change the efficiency of immunoprecipitationof cerebellar Cupidin protein with the antibody. Under this condition,the anti-CPD antibody could coprecipitate GST-Cdc42 in the presenceof GTP $gamma$ S but not of GDP (Fig. 3B). Furthermore, we studied thedirect interaction between Cupidin and Rho family proteins usingDMP, a protein cross-linker with a 9.2 Å spacer arm. After cross-linkingwithout Cupidin, GST-Rho family proteins remained monomeric, irrespectiveof whether GDP or GTP $gamma$ S was loaded, as judged by their respectivemobility on SDS-PAGE (Fig. 3C, left). When Cupidin was coincubatedin these cross-linking reaction mixture, only GTP $gamma$ S-loaded Cdc42could form a complex with Cupidin, which represented the mobilityshift to a higher molecular weight band calculated as ~100 and~150 kDa (Fig. 3C, right). These results suggested that Cdc42could directly interact with Cupidin in a GTP-dependent manner.Although the detection is limited under experiment shown above,an interaction between Cupidin and RhoA or Rac1 cannot be excludedand remains to bestudied.

It is known that the activation of Cdc42 contributes the formation of filopodial protrusions at the cell periphery (Kozmaet al., 1995). To determine whether Cupidin could interact withCdc42 in vivo, we examined the functional effect of overexpressingCupidin on Cdc42 phenotype of HeLa cells expressing Cdc42^V12, a constitutively active mutant of Cdc42 (Takaishi et al., 1997).Under our experimental conditions, 58% of HeLa cells expressingCdc42^V12 indeed formed filopodia-like microspike structures (Fig. 4, n= 300). Eighteen percent of the remaining cells showed atypicalaggregation of F-actin in the cytoplasm, whereas 24% displayedother phenotypes, such as thickening of cortical actin filamentsand blebbings at the cell surface (data not shown). The latterpresumably represented the agonal state of the cells because ofthe prolonged expression of Cdc42^V12. In contrast, the cells overexpressing Cupidin alone showed noobvious change in cell shape (Fig. 4). By coexpressing both Cupidinand Cdc42^V12, however, cells with the proportion showing the typical microspikesdrastically decreased (Fig. 4); only 2% of the cells (n = 300)showed microspike formation, 33% was in agonal state, and 65%was as the control with no obvious peripheral change. These resultsindicated that Cupidin somehow interfered Cdc42-induced microspikeformation.

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Figure 4. Cupidin overexpression affects Cdc42^V12 phenotype in HeLa cells. Overexpression of CPD alone (left panels), myc tagged-Cdc42^V12 alone (middle panels), or both (right panels) in HeLa cells. Transfected cells were stained using the anti CPD antibody (FITC), anti-myc antibody (Cy5), and Texas Red-phalloidin. Top panels are superimposed composite images using three pseudocolors (green for CPD, red for phalloidin, and blue for myc tagged-Cdc42^V12). Note that filopodia-like microspike structures were visible in Cdc42^V12-overexpressed cells, as indicated by arrows. However, few such structures were induced in cells overexpressing either CPD alone or CPD and Cdc42^V12. Scale bar, 60 µm.

Cupidin interacts with F-actin and mGluR1 $alpha$ through its N-terminal region

Next, we asked whether the EVH1-like domain present in Cupidin could interact in some way with F-actin, because the VASP/Enafamily proteins containing the EVH1 domain are known to be associatedwith actin filaments, either directly or indirectly (Gertler etal., 1996). As shown in Figure 5A, GST-CPD/N and GST-CPD/C weresubjected to an in vitro cosedimentation assay with F-actin. Inthe presence of F-actin, a substantial fraction of GST-CPD/N (43%)was recovered into the pellet fraction after high-speed centrifugation.However, neither GST-CPD/C nor GST alone was coprecipitated withF-actin. The full-length Cupidin fused to GST was also coprecipitatedwith F-actin (data not shown). These results indicated that F-actincould interact with Cupidin through the N-terminal first 111 aa.

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Figure 5. Cupidin interacts with F-actin and mGluR1 $alpha$ . A, F-actin binding to Cupidin in a cosedimentation assay. GST, GST-CPD/N, and GST-CPD/C were incubated with (+) or without ( $-$ ) F-actin prepared from chicken skeletal muscles and then centrifuged. Equivalent protein amounts of the supernatant (S) and pellet (P) fractions were separated by SDS-PAGE and stained with Coomassie Brilliant Blue (CBB). A representative result of five independent experiments is shown here. The arrows indicate the position of actin, and the arrowheads represent each GST-fusion protein. B, Binding of Cupidin to mGluR1 $alpha$ in a pull down assay. The S1 fraction prepared from P7 mouse cerebellum or cerebrum was incubated with GST-CPD/N protein and then immobilized onto glutathione-Sepharose beads. After extensive washing, GST-CPD/N-bound proteins were extracted with SDS-PAGE sample buffer and were analyzed by Western blotting using an anti-mGluR1 $alpha$ polyclonal antibody. Lane 1, Input (the same amounts of lysates used for the assay were loaded); lane 2, eluate from a GST-bound column; lane 3, eluate from a GST-CPD/N bound column. C, Coimmunoprecipitation of both mGluR1 and actin from P7 mouse cerebellar lysates using the anti-CPD antibody. The immunoprecipitates obtained with either the preimmune serum (lane 2) or the affinity-purified anti-CPD polyclonal antibody were examined by Western blotting with the indicated antibodies (anti-CPD, anti-actin, and anti-mGluR1 $alpha$ ). Lane 1 is the detergent extract of P7 mouse cerebellum. The arrow indicates Cupidin signal, and the asterisk indicates the heavy chain of IgG. D, Primary-cultured mouse cerebellar granule neurons at 7 DIV were triple-stained with an anti-CPD polyclonal antibody (FITC; a), Texas Red-phalloidin (b), and an anti-synaptophysin monoclonal antibody (Cy5; c) and observed by confocal microscopy. d is a superimposed composite images of a-c using three pseudocolors (green for CPD, red for phalloidin, and blue for synaptophysin). Arrows indicate representative positions at which the three pseudocolors overlapped. Scale bar, 10 µm.

All members of the Homer/Vesl family have been shown to interact with the group I mGluRs through the N-terminal region: theN-terminal 131 aa of Homer 1/Vesl-1 and the N-terminal 2-141 aaof Homer 2/Vesl-2 (Kato et al., 1998). We showed that GST-CPD/Ncould pull down mGluR1 $alpha$ from lysates of both cerebellum and cerebrumof P7 mice (Fig. 5B, lane 3), indicating that the N-terminal 111aa are sufficient not only for F-actin interaction but also formGluR1 $alpha$ binding.

We further examined whether Cupidin was indeed able to form a protein complex with F-actin and mGluR1 $alpha$ in the developing cerebellum.Anti-Cupidin antibody, recognizing both splicing forms of Cupidin(Fig. 2C), could coimmunoprecipitate both actin and mGluR1 $alpha$ fromthe detergent extracts of P7 mouse cerebellar lysates (Fig. 5C),thus supporting the possibility as to formation of a Cupidin-mGluR-actincomplex, to some part of which CPD- $beta$ may alsocontribute.

Subcellular localization of Cupidin

To address the relevance of Cupidin-actin interaction, we examined the subcellular localization of Cupidin in primary-culturedcerebellar granule cells. Cupidin immunoreactivity was observedin a patchy and punctate pattern along the dendrite of granulecells (Fig. 5D, a). Texas Red-conjugated phalloidin labeled theF-actin in the neurites in a punctate manner (Fig. 5D, b). Interestingly,many F-actin-positive puncta appeared to overlap with Cupidin-positiveones. The immunoreactivity for synaptophysin, a presynaptic markerprotein, was simultaneously visualized to clarify synaptic sites(Fig. 5D, c). The merged image of the triple staining revealedthat a large number of the Cupidin-positive and F-actin-positivepuncta were in close proximity to the synaptophysin-positive synapticstructures (Fig. 5D, d), suggesting that Cupidin may colocalizewith F-actin at granule cellsynapses.

We next examined the subcellular localization of overexpressed GFP-CPD in MDCK cells, a canine epithelial cell line. The GFPfluorescence for Cupidin was diffusely localized throughout thecytoplasm and was occasionally seen in a punctate pattern thathad the appearance of a stack in Golgi-like structures. Notably,the strong intensity of GFP fluorescence was remarkable at regionsof cell-cell contacts at which Texas-Red fluorescence for F-actinwas also the highest (Fig. 6, left panels). A similar prominenceof GFP fluorescence at cell-cell contact sites was observed inHeLa cells overexpressing GFP-CPD (data not shown). Interestingly,GFP fusions with either truncated form of Cupidin, GFP-CPD/N orGFP-CPD/C, overexpressed in MDCK cells were no longer localizedat the cell-cell contact sites, suggesting that both the N-terminaland the C-terminal domains of CPD are required for this localization.Together with the in vitro binding to F-actin (Fig. 5A,C), bothtypes of subcellular localizations in cerebellar granule cellsand in MDCK cells are consistent with the idea that Cupidin mayaccumulate at structures in which the actin cytoskeleton concentrates.

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Figure 6. Localization of Cupidin overexpressed in MDCK cells at sites of cell-cell contact. MDCK cells overexpressing GFP-CPD (left panels), GFP-CPD/C (middle panels), and GFP-CPD/N (right panels) were stained with Texas Red-phalloidin. Middle panels show GFP images, bottom panels show F-actin images overlapping cell-cell contact sites, and top panels show the merged images. Note that overexpressed GFP-CPD specifically concentrated at cell-cell contact sites, as indicated by arrows, whereas both overexpressed GFP-CPD/N and GFP-CPD/C widely localized throughout the cytoplasm. Scale bars, 10 µm.

Cupidin is localized at sites undergoing active synaptogenesis in the developing mouse cerebellum

To gain further insight into the possible role of Cupidin in the developing cerebellum, we next attempted to characterizethe distribution of Cupidin in mouse cerebellum using both immunohistochemicaland biochemicalapproaches.

An immunohistochemical study with the anti-Cupidin antibody showed that the immunoreactive signals were predominantly localizedin the ML and the IGL of P7 mouse cerebellum (Fig. 7A). Most ofthe immunoreactivity in the IGL was observed as puncta with strongsignal intensity in small clear spaces surrounded by granule cellsoma. The localization of presynaptic synaptophysin immunoreactivityseemed to substantially overlap with that of the Cupidin-positivepunctate structures. This result raised the possibility that theCupidin signals in the IGL might correspond to glomeruli formedat the synaptic junctions between the MF-Golgi neuron terminalsand the granule cell dendrites (Fig. 7, insets A', B'). Subcellularfractionation of P7 cerebellar extracts (Fig. 7C) demonstratedthat Cupidin, together with its alternative splicing variant CPD- $beta$ ,was abundant in the crude synaptosomal fraction (P2'). Furthersubfractionation revealed that Cupidin, along with PSD-95, wasenriched in the synaptic heavy membrane (LP1) and in the PSD fractions.These data indicated that, at P7, Cupidin exists in the postsynapses,most likely in the PSD area.

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Figure 7. The cellular and subcellular distribution of Cupidin. (A, A', B, B') A sagittal cerebellar section of P7 mouse was immunostained with an anti-Cupidin antibody (A, A') and an anti-synaptophysin antibody (B, B'). Magnification: A, B, 400×; A', B', 1000× of IGL region. Examples that Cupidin signals could be overlapped with synaptophysin signals are indicated by arrows. PL, Purkinje cell layer. C, Crude synaptosomes from P7 mouse cerebellum were prepared by differential centrifugation (P2'), lysed hypotonically, and fractionated into heavy membranes (LP1), synaptic vesicles (LP2), and cytosol (LS2). PSD fractions were prepared from LP1 fractions. Proteins (25 µg) from each fraction were subjected to Western blot using the antibodies against the indicated proteins. An arrow indicates the signal of Cupidin.

The developmental profile of synaptic expression of Cupidin was further examined. In line with our data obtained from theFDD, RT-PCR, and Northern analysis, the expression of 44 kDa Cupidin(CPD- $alpha$ ) was most prominent at approximately P7 in the developingmouse cerebellum (Fig. 8A). On the other hand, a 46 kDa long splicingisoform (probably CPD- $beta$ ) was upregulated until P7, and its expressionlevel stayed relatively constant from then onward (Fig. 8A). Theimmunohistochemical study using cerebellar sections at variousstages (Fig. 8B) and the immunocytochemical analysis using culturedcerebellar granule neurons (Fig. 8C) confirmed a sharp declinein the Cupidin immunoreactivity of granule cells after P7 and7 DIV, respectively. The Cupidin-immunoreactive signals in theIGL of P7 cerebellum seemed to be concentrated in glomeruli inwhich active synaptogenesis was undergoing. In adult, most immunoreactivitywas weakly detected in the Purkinje cell dendrites and soma. Consideringthe developmental expression profile seen in Figure 8A, the signalsseen in the adult cerebellum were probably attributable to theexpression of the 46 kDa CPD- $beta$ . The striking temporal profile,along with a transient concentration at the cerebellar granulecell synapses, indicates that Cupidin gene expression may be tightlycoupled with the formation of new synapses in the cerebellar cortex.

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Figure 8. Synaptic expression of Cupidin in granule cells during the development of the cerebellar cortex. A, Western blot analysis for developmental expression of Cupidin in the cerebellum. Whole lysates of mouse cerebellum at various stages were examined by Western blotting using the anti-CPD antibody. The expression of the top 46 kDa signal persisted even after P7, whereas the expression of the bottom 44 kDa Cupidin was peaked at approximately P7 and then was hardly detectable in adult lysates. B, Sagittal sections of P7, P14, and adult mouse cerebella were immunostained with the anti-CPD antibody ( $alpha$ -CPD Ab.; top panels) and anti-synaptophysin antibody ( $alpha$ -Syn. Ab.; bottom panels), followed by HRP-based DAB-H₂O₂ reaction. Apparently, a high intensity of CPD signals in the IGL was prominent at P7 and then diminished onwards. In contrast, synaptophysin signals in IGL were increased both in size and intensity, indicating the maturation of glomeruli. PL, Purkinje cell layer. Magnification, 400×. Scale bar, 40 µm. C, Primary cultured mouse cerebellar granule neurons at 7, 14, and 21 DIV were costained with the anti-CPD antibody ( $alpha$ -CPD Ab.; left panels) and the anti-synaptophysin antibody ( $alpha$ -Syn. Ab.; right panels) and observed using confocal microscopy. Note that a large number of punctate CPD-signals again peaked at 7 DIV, in contrast to the lasting increase in synaptophysin-signals until 21 DIV. Scale bar, 50 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Isolation of Cupidin, a Homer/Vesl isoform, as a developmentally regulated gene in cerebellar cortex

In the course of a systematic study of genes that are developmentally regulated in the mouse cerebellum, we have identifieda clone encoding a multimodular protein, Cupidin. Cupidin wassubsequently found to be identical to Homer 2a/Vesl-2 $Delta$ 11 (Katoet al., 1998; Xiao et al., 1998). Our study indicates that Cupidingene expression is highly regulated in the postnatal developingcerebellar granule cells. Although there was no isoform-specificprobes that could distinguish Cupidin (CPD- $alpha$ ) from splicing isoformCPD- $beta$ (Homer 2b/Vesl-2), our data clearly demonstrates that bothCupidin mRNA and protein expressions are strongest at P7 in cerebellargranule cells while these neurons were undergoing active synaptogenesis.The Cupidin immunoreactivity decreased from the IGL afterwards,and CPD- $beta$ might also show the same expression profile in granulecells. However, CPD- $beta$ expression in whole cerebellum drasticallyincreased at approximately P7 and continued to adult stage. Inadult cerebellum, CPD- $beta$ appeared to localize in Purkinje celldendrites and soma. These data suggest that the alternative splicingof Cupidin and CPD- $beta$ is highly development-specific and that Cupidinand CPD- $beta$ may be involved in a cell type-specificregulation.

Cupidin as a scaffold protein linking mGluR with actin cytoskeleton

Cupidin was structurally marked by two regions: the N-terminal region (the N terminus to residue 111) and the C-terminal region(residue 112 to the C terminus). We showed that the N-terminalregion could bind both mGluR1 $alpha$ and F-actin, although we couldnot rule out the possibility that the latter interaction may involveother intermediate molecules. Although the N-terminal region ofCupidin contains a single Gly-Leu-Gly-Phe sequence preceded withArg (residues 81-90), just as seen in several typical PDZ domainssome of which are known to associate with various kinds of plasmamembrane proteins (Doyle et al., 1996; Sheng, 1996), the flankingsequence, especially the sequence after the Gly-Leu-Gly-Phe, hasno aa homology with any other PDZ domainproteins.

Although mGluR1 $alpha$ is predominantly expressed in Purkinje cells of adult cerebellum, it was reported that both mGluR1 $alpha$ mRNA(Shigemoto et al., 1992; Bessho et al., 1993) and protein (Baudeet al., 1993; Ryo et al., 1993) were detected in the granule cellsat a low level. It was also reported that mGluR1 $alpha$ immunoreactivitywas localized in the glomerulus (Baude et al., 1993), a structurein which synapses are formed between the granule cells and MFs-Golgineurons. In the present study, we have shown that Cupidin probablyforms a complex with mGluR1 $alpha$ in the P7 mouse cerebellum. Thus,in the developing granule cells, Cupidin may play a role in mGluR1 $alpha$ signaling.

Ionotropic glutamate receptors (iGluRs) bind to PDZ domain-based adapter proteins such as glutamate receptor-interacting protein(GRIP) (for certain AMPA receptor subunits) and PSD-95 (for severalNMDA receptor subunits), and it is known that PSD-95 can anchoriGluRs to dendritic F-actin via actin-binding protein actinin(Allison et al., 1998). The present study suggests that Cupidinmay provide a physical link between mGluRs and the synaptic actincytoskeleton. The N-terminal region of Cupidin has a weak overallhomology to the EVH1 domain of the VASP/Ena family, which includesVASP (Reinhard et al., 1992), Drosophila Enabled/mouse Ena homolog(Mena) (Gertler et al., 1996), and Wiscott-Aldrich syndrome protein(WASP) (Symons et al., 1996). One of the common features of thisprotein family is thought to be the regulation of actin cytoskeleton,perhaps through the shared EVH1 domain present in the N-terminalregion. We have found that Cupidin appears to have the abilityto form a stable complex with F-actin via its N-terminal regioncontaining the EVH1-like domain. The immunocytochemical studiesand coimmunoprecipitation experiments also clearly indicated thatCupidin is likely to interact with the actin cytoskeleton in developinggranule cells. In a quantitative point of view, only a limitedfraction of Cupidin could bind to F-actin by our in vitro F-actinbinding experiments. This low efficiency in the in vitro Cupidin-F-actininteraction suggests that other accessory or intermediate protein(s)may be involved in the interaction between Cupidin and actinfilaments.

The C-terminal two-thirds of Cupidin has been predicted to be an $alpha$ -helical, coiled-coil structure containing several leucinezipper motifs (Fig. 2A). Isoforms of Homer/Vesl have been proposedto multimerize through their C-terminal ends (Kato et al., 1998;Xiao et al., 1998). In the present study, we have further identifiedthe C-terminal region as the possible interaction domain withRho family small GTPase proteins, a well-established class ofcytoskeletal regulators. Together with the synaptic localization,Cupidin may act as a scaffold protein that links multiple signalingmolecules, including G-protein-coupled cell surface receptor suchas mGluR1, the actin cytoskeleton, and Rho-family proteins, especiallyat sites making synaptic contacts in the developing granulecells.

A possible interaction between Cupidin protein complex and Rho family small GTPases

Members of the Rho small GTPase family play important roles in regulation of the actin cytoskeleton in a wide variety of organisms,ranging from yeast to mammals (for review, see Narumiya et al.,1997) and have been implicated in neuronal migration, dendriteoutgrowth, and axon guidance (Luo et al., 1996; Threadgill etal., 1997). Recently, the molecular interaction between a Rho-targetprotein, Citron, and PSD-95 has been demonstrated (Furuyashikiet al., 1999).We here have found that, in ligand overlay assay,Cupidin could potentially interact with RhoA, Rac1, and Cdc42in a GTP-dependent manner through the C-terminal two-thirds homologousto the Rho binding site of Citron. It should be noted that thethree different in vitro studies we performed to assess thesepossible interactions always revealed that Cupidin interactedwith Cdc42. The heterologous expression studies revealed thatCupidin overexpression inhibited the active Cdc42 induced microspikeformation in HeLa cells. Although the most likely explanationfor this inhibition may be the displacement of Cdc42 by overexpressedCupidin, it remains possible that Cupidin may function as a regulatorof Cdc42. Whether Cupidin may be involved in the regulation ofcell shape during synaptogenesis, possibly via Rho family GTPases,will be the subject of furtherstudies.

The heterologous expression experiments in MDCK cells showed that Cupidin appeared to be colocalized with certain actin-associatedstructures at the cell-cell junctions. Indeed, it was reportedthat Rho family proteins may play a regulatory role in cell-celladhesion in MDCK cells (Takaishi et al., 1997) and that GTPase-activatingprotein-containg Ile-Gln motifs, a target for Cdc42 and Rac1,is localized at cell-cell contact regions (Kuroda et al., 1996).Thus, the binding of Rho family members may be important in regulatingthe cellular localization of Cupidin or its association with othertargetproteins.

A Cupidin-linked signaling complex in the developing cerebellum

The present study suggests that Cupidin interacts with several signaling molecules, including mGluR1 $alpha$ , F-actin, and perhapsRho family small GTPases. We have also shown that Cupidin proteinis predominantly expressed in punctate structures in the IGL andthe ML of P7 mouse cerebellum. Furthermore, Cupidin-positive structuresseems to correspond to the MF-granule cell synapses, glomeruli,and the PF-Purkinje cell dendrite synapses during the period whenactive synaptogenesis is occurring. In the primary-cultured granulecell neurites, Cupidin protein substantially colocalizes withF-actin in close vicinity to the synaptophysin-positive punctatestructures.

A recent study noted that Homer protein appeared to bind the inositol 1,4,5-trisphosphate receptor (IP₃R) (Tu et al., 1998),an IP₃-gated Ca²⁺ release channel downstream of the mGluR1 signaling cascade (Furuichiand Mikoshiba, 1995). Because Cupidin is identical to the Homer2a isoform and its expression is tightly regulated in the developingcerebellar cortex, Cupidin may be a physical link between mGluR1and IP₃R. Whether Cupidin is implicated in a mGluR1-regulatedCa²⁺ signaling events during cerebellar development remains to beestablished.

In migrating granule cells, actin filament was observed in a subcortical rim of soma and in lamellipodial and filopodial extensionsof the leading process, whereas in the granule cell-extendingneurites, it was distributed in the periphery of the growth conebut was not enriched in the leading processes (Rivas and Hatten,1995). Because Cupidin binds F-actin and is expressed in migratingand neurite-extending granule cells, one might speculate a possiblerole for Cupidin in the cytoskeletal regulation required for cellmotility and/or dynamic changes in cell shape during the developmentof granulecells.

In conclusion, we have uncovered the intriguing molecular and developmental properties of a Homer/Vesl isoform, Cupidin. Cupidinappears to act as a scaffold protein linking multiple signalingmolecules, including mGluR1, F-actin, and perhaps Rho family smallGTPases. Because Cupidin expression is prominent in the earlydifferentiating granule cells and enriched at the synapses, aspecific involvement of Cupidin in regulating granule cell synaptogenesisissuggested.

  FOOTNOTES

Received May 27, 1999; accepted July 16, 1999.

This research was supported by grants from the Ministry of Education, Science, Sports, and Culture of Japan, the Ministryof Health and Welfare of Japan, the Asahi Glass Foundation, andthe Institute of Physical and Chemical Research (RIKEN). We thankDr. M. E. Hatten (Rockefeller University) for a cerebellar cDNAlibrary, Dr. K. Kaibuchi (Nara Institute of Science and Technology)for the plasmid construct of RhoA^A37 and for sharing the GST-Rho overlay assay protocol, Drs. K. Inokuchi(Mitsubishi Chemicals Institute of Life Science) and A. Kato (KyushuUniversity) for communicating unpublished results, Dr. T. Furuyashiki(Kyoto University) for sharing the GST-Rho pull-down assay protocol,and Dr. N. Watanabe (Kyoto University) fordiscussions.
Correspondence should be addressed to Dr. Teiichi Furuichi, Laboratory for Molecular Neurogenesis, Brain Science Institute,RIKEN, 2-1 Hirosawa, Wako, Saitama 351-0198,Japan.

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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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