Regulated Expression and Subcellular Localization of Syndecan Heparan Sulfate Proteoglycans and the Syndecan-Binding Protein CASK/LIN-2 during Rat Brain Development

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The Journal of Neuroscience, September 1, 1999, 19(17):7415-7425

Regulated Expression and Subcellular Localization of Syndecan Heparan Sulfate Proteoglycans and the Syndecan-Binding Protein CASK/LIN-2 during Rat Brain Development
Yi-Ping Hsueh and Morgan Sheng
Howard Hughes Medical Institute and Department of Neurobiology, Massachusetts General Hospital and Harvard Medical School, Boston, Massachusetts 02114

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The syndecan family of cell surface heparan sulfate proteoglycans interacts via their cytoplasmic C-terminal tail with thePDZ domain of CASK/LIN-2, a membrane-associated guanylate kinasehomolog. The syndecan-CASK interaction may be involved in intercellularsignaling and/or cell adhesion. Here we show that syndecan-1 tosyndecan-4 have distinctive mRNA distributions in adult rat brainby in situ hybridization, with syndecan-2 and -3 being the majorsyndecans expressed in neurons of the forebrain. At the proteinlevel, syndecan-2 and -3 are differentially localized within neurons;syndecan-3 is concentrated in axons, whereas syndecan-2 is localizedin synapses. The synaptic accumulation of syndecan-2 occurs latein synapse development. CASK is a cytoplasmic-binding partnerfor syndecans, and its subcellular distribution changes strikinglyduring development, shifting from a primarily axonal distributionin the first 2 postnatal weeks to a somatodendritic distributionin adult brain. This change in CASK distribution correlates temporallyand spatially with the expression patterns of syndecan-3 and -2,consistent with the association of both of these syndecans withCASK in vivo. In support of this, we were able to coimmunoprecipitatea complex of CASK and syndecan-3 from brain extracts. Our resultsindicate that specific syndecans are differentially expressedin various cell types of the brain and are targeted to distinctsubcellular compartments in neurons, where they may serve specializedfunctions. Moreover, CASK is appropriately expressed and localizedto interact with both syndecan-2 and -3 in different compartmentsof the neuron throughout postnataldevelopment.

Key words: syndecan; CASK/LIN-2; heparan sulfate proteoglycan; MAGUK; subcellular targeting; axon

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The syndecan family of transmembrane proteins comprises a major class of cell surface heparan sulfate proteoglycans (HSPGs).Currently, four members have been identified in mammals: syndecan-1,syndecan-2/fibroglycan, syndecan-3/N-syndecan, and syndecan-4/ryudecan(for review, see Bernfield et al., 1992; David, 1993; Carey, 1997).The extracellular functions of syndecans are primarily mediatedby their heparan sulfate (HS) glycosaminoglycan (GAG) side chains,which have affinity for a wide variety of secreted molecules andextracellular matrix (ECM) components. Recent interest in cellsurface HSPGs stems particularly from the discovery that theyare important for the binding and action of polypeptide growthfactors, as well as for cell-matrix and cell-cell interactions(for review, see Bernfield et al., 1992; David, 1993; Schlessingeret al., 1995; Couchman and Woods, 1996; Carey, 1997;). In thiscontext, cell surface HSPGs such as syndecans can be regardedas "coreceptors" that function to present or concentrate polypeptidefactors for their specific high-affinity receptor tyrosine kinases(for review, see Schlessinger et al., 1995; Carey, 1997).

In addition to binding to polypeptide signaling factors, HS also binds to ECM components including fibronectin, collagen,and laminin and to the cell surface protein neural CAM. Many studieshave implicated cell surface HSPGs in cell adhesion and tissuemorphogenesis (for review, see Bernfield et al., 1992; David,1993; Carey, 1997). On the basis of their ability to mediate dynamiccell-matrix interactions and to bind to diverse polypeptide signalingfactors, syndecan HSPGs could play a supporting role in many aspectsof neural development, including cell migration, neurite extension,and synapse assembly and plasticity. We have recently discoveredthat syndecan-2 is concentrated in synaptic junctions of adultrat brain (Hsueh et al., 1998). This has been confirmed by Ethelland Yamaguchi (1999) who additionally showed that overexpressionof syndecan-2 in neurons alters the morphological developmentof dendritic spines. However, not much is known about which othersyndecans are specifically expressed in neurons, how they aredistributed at the subcellular level, and how their expressionpatterns are regulated during development of the nervoussystem.

CASK, the mammalian homolog of Caenorhabditis elegans LIN-2, is a protein of the membrane-associated guanylate kinase homolog(MAGUK) superfamily. It contains a Ca²⁺/calmodulin-dependent kinase-like domain at its N terminal, inaddition to a PDZ domain, an SH3 domain, and a guanylate kinase-likedomain that characterizes all MAGUK proteins (Hata et al., 1996;Hoskins et al., 1996; Dimitratos et al., 1997). In C. elegans,LIN-2 together with LIN-7 and LIN-10 (two other PDZ proteins)forms a ternary protein complex that plays a critical role inbasolateral localization of LET-23, an epidermal growth factorreceptor homolog, in epithelial cells (Kaech et al., 1998). Ahomologous ternary protein complex has been demonstrated in mammalianbrain, although the functional significance of the mammalian LIN-2/LIN-7/LIN-10complex remains to be determined (Butz et al., 1998). In additionto binding to LIN-7 and LIN-10 homologs, CASK has been shown tointeract via its PDZ domain with the C terminals of neurexins(Hata et al., 1996) and syndecans (Cohen et al., 1998; Hsueh etal., 1998). Neurexins and syndecans are transmembrane proteinsthat share a similar cytoplasmic C-terminal sequence (-EYYV and-EFYA, respectively) and a common involvement in cell-cell orcell-ECM interactions (for review, see Missler et al., 1998).The intracellular interaction with CASK, or other PDZ proteinssuch as syntenin (Grootjans et al., 1997), may link neurexinsand syndecans to the cytoskeleton (Cohen et al., 1998) or to intracellularsignalingpathways.

The four mammalian syndecans (as well as Drosophila and C. elegans syndecans) share the same -EFYA C-terminal motif that mediatesbinding to the PDZ domain of CASK (Hsueh et al., 1998), suggestingthat CASK might associate with all syndecan members in vivo. Wehave recently provided immunohistochemical evidence of an interactionbetween CASK and syndecan-2 in synaptic junctions of adult brain(Hsueh et al., 1998). At the subcellular level, however, CASKis more widely distributed than the synaptically localized syndecan-2(Hsueh et al., 1998), raising the possibility that CASK associateswith other syndecans in nonsynaptic regions of the neuron. However,little is known about the expression patterns of the differentsyndecans in relation to CASK or how these relationships changeduring development of the ratbrain.

To characterize the extent of CASK-syndecan interactions in vivo, we investigated the expression patterns of CASK and of thedifferent syndecans in developing and mature rat brain. We focusedon syndecan-2 and -3 after determining that they were the majorneuronal syndecans of the forebrain. Syndecan-2 and -3 show contrastingexpression profiles during development and segregated distributionwithin neurons. Syndecan-3 is more highly expressed in developingbrain and concentrated in axons. Syndecan-2 is more strongly expressedin mature brain and localized in synapses. CASK protein levelsare high throughout development, but its distribution changesfrom an axonal pattern (where it colocalizes with syndecan-3)to a somatodendritic pattern (where it overlaps with syndecan-2).These findings are consistent with the binding of syndecan-2 and-3 to CASK at different times in development and in differentcompartments of the neuron. In support of this biochemical association,we report for the first time the coimmunoprecipitation of CASKand syndecan from brainextracts.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In situ hybridization. ³⁵S-labeled RNA probes were synthesized by in vitro transcription using T7 and SP6 RNA polymerase. Thetranscription templates were generated by PCR and correspondedto rat syndecan-1 [nucleotide (nt) +90 to +615], syndecan-2 (nt $-$ 22 to +454), syndecan-3 (nt +143 to +626), and syndecan-4 (nt+1 to +414). These templates represent the poorly conserved ectodomainsof each syndecan. T7 and SP6 promoters were included in antisenseand sense PCR primers,respectively.

Antibodies. Rabbit polyclonal syndecan-2 peptide antibodies (Syn-2C) and CASK peptide antibodies have been described (Hsuehet al., 1998). CASK murine monoclonal antibodies K56A/50.1, K56A/57.1,and K56A/95.1 were raised against a glutathione S-transferasefusion containing amino acids 317-415 of rat CASK (Cohen et al.,1998) in collaboration with Dr. James Trimmer (State Universityof New York, Stony Brook, NY). These three monoclonal antibodiesare specific for CASK and give identical results on immunoblottingand immunostaining (Y.-P. Hsueh, unpublished observations). Syndecan-3cytoplasmic domain antibodies (Syn-3C) were raised in rabbitsagainst the synthetic peptide SYTLEEPKQASVTYQK. Rabbit polyclonalantibodies against the ectodomain of syndecan-3 (Syn-3ecto) werea gift of Dr. David Carey (Geisinger Clinic, Danville, PA). Murinemonoclonals to MAP2, synaptophysin, and calbindin-D were purchasedfrom Sigma (St. Louis,MO).

DNA constructs. Rat syndecan-2 cDNA was generously provided by Dr. Graham Cowling (Manchester University, Manchester, UK)and subcloned into the KpnI and EcoRI sites of mammalian expressionvector GW1-CMV. Syndecan-3 cDNA was kindly provided by Dr. DavidCarey and subcloned into GW1-CMV. The coding sequences of syndecan-1and -4 were amplified from rat brain mRNA by reverse transcription-PCRand subcloned into the KpnI and EcoRI sites of GW1-CMV.

Transfection, immunocytochemistry, and immunohistochemistry. Transfection of COS-7 cells using lipofectamine and subsequentimmunocytochemistry were performed as described (Hsueh and Sheng,1999). For rat brain immunohistochemistry, floating sections atdifferent ages were prepared and processed as described (Hsuehet al., 1998) with slight modifications. After perfusion and fixation,postnatal day 21 (P21) rat brains were directly sliced with avibratome, whereas P3, P7, and P15 rat brains were embedded in2-3% agarose before slicing on the vibratome at 50 µm thickness.For immunostaining using Syn-3ecto antibodies, tyramide signalamplification (TSA direct kit; NEN Life Science Products, Boston,MA) was applied according to the manufacturer's directions toconserve antibody and enhance signal. The staining pattern usingthe TSA kit was identical to that using standard indirect immunofluorescencemethods. Fluorescence was viewed with a Zeiss Axioskop microscopeor a Bio-Rad (MRC-1000; Hercules, CA) confocal microscope. Imageswere prepared for publication with AdobePhotoShop.

Immunoprecipitation and immunoblotting for HSPG syndecans. For immunoprecipitation from rat brain extracts, 10 µg of affinity-purifiedSyn-3C antibodies was incubated with 60 µl of a 1:1 slurry ofprotein A Sepharose in 100 mM sodium borate buffer, pH 8.0, at4°C overnight. Free antibodies were removed by washing with sodiumborate buffer three times. These antibody-protein A Sepharosepellets were used for immunoprecipitation. One-week-old rat brainswere minced and homogenized with a Polytron in PBS. The extractwas cleared of nuclei, unbroken cells, etc., by centrifugationat 930 × g for 10 min at 4°C. The postnuclear supernatant wassolubilized with 1% Triton X-100 in PBS at 4°C for 1 hr and dialyzedagainst 0.1% Triton X-100 in PBS at 4°C overnight. Insoluble materialwas pelleted by centrifugation at 37,000 × g for 1 hr. Detergent-solubilizedextract (1 mg of protein) was incubated with antibody-proteinA Sepharose at 4°C for 3-4 hr. The precipitates were washed with0.1% Triton X-100 in PBS three times and with 10 mM Tris, pH 7.5,once. Bound proteins were eluted from beads in SDS sample bufferand immunoblotted as described (Kim et al., 1994). Briefly, proteinswere separated on a TBE/urea 3-15% polyacrylamide gradient gel(40 mM Tris, 60 mM boric acid, 0.8 mM EDTA, 1 mM sodium sulfate,and 2.7 M urea; 7.5% cross-linking) with TBE running buffer containing0.1% SDS and were transferred onto Immobilon-N (Millipore, Bedford,MA).

Primary cultures of rat cortical neurons. After trypsinization and mechanical dissociation, cortical neurons from embryonicday 16 (E16)-E17 rat embryos were resuspended in DMEM supplementedwith 10% FCS and 10% horse serum and plated on coverslips coatedwith poly-L-lysine (1 mg/ml) at densities of 2-4 × 10⁵ per 18 mm coverslip. Immunofluorescence staining was performedat 4-7 d in vitro.

Subcellular fractionation of rat brain extracts. Subcellular fractions of adult rat brain were prepared as described (Huttneret al., 1983). Briefly, rat brain Dounce homogenate was centrifugedat 1000 × g to remove nuclei and other large debris [first pellet(P1)]. The supernatant was centrifuged at 10,000 × g to obtaina crude synaptosomal fraction (P2), which was subsequently lysedwith hypotonic buffer and centrifuged at 25,000 × g to pelleta lysed synaptosomal membrane fraction (LP1). The supernatant(LS1) was then centrifuged at 165,000 × g to obtain a crude synapticvesicle fraction (LP2) and soluble fraction (LS2). The supernatantabove the P2 fraction (S2) was centrifuged at 165,000 × g to obtaina soluble fraction (S3) and a light membrane fraction (P3). Fordevelopmental studies, P2 fractions were collected from the ratsat the ages of E14, E18, P3, P7, P15, P22, andP42.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Differential expression of syndecan mRNAs in rat brain

To identify which syndecans might interact with CASK in neurons in vivo, we analyzed by in situ hybridization (ISH) the expressionpatterns of the four known syndecans. Each of the syndecans hasa different distribution in the adult rat brain (Fig. 1). Syndecan-1mRNA is expressed almost exclusively in the cerebellum (Fig. 1A);no signal was detected in the forebrain. Syndecan-2 is widelyexpressed, with high levels in the dentate gyrus of the hippocampalformation and in the granule cell layer of the cerebellum, moderatelevels in the striatum and cerebral cortex, and low levels inthe thalamus (Fig. 1C). Syndecan-3 is expressed strongly in granulecells and Purkinje cells of the cerebellum and moderately in thehippocampal formation, cerebral cortex, and thalamus (Fig. 1B;data not shown). Syndecan-4 mRNA is distributed in a diffuse cellularpattern throughout the rat brain, including white matter regions(Fig. 1D), suggesting that it is expressed specifically in glialcells. This is more obvious by emulsion autoradiography, whichshows a pattern of syndecan-4 expression typical of astrocytes(hippocampal region is shown in Fig. 1H). Syndecan-4 also exhibitsa glial pattern of ISH in other parts of the brain (data not shown).

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Figure 1. In situ hybridization analysis of syndecan mRNAs in adult rat brain. A-D, Syndecan-1 (A); syndecan-3 (B); syndecan-2 (C); syndecan-4 (D). E, F, Sense strand negative controls for syndecan-2 (E) and syndecan-4 (F). Syndecan-1 and -3 sense stand negative controls also gave no significant ISH signal (data not shown). G, H, Higher magnification (emulsion autoradiography) views of syndecan-2 (G) and syndecan-4 (H) distribution in the hippocampus, showing glial expression of syndecan-4. cc, Corpus callosum; Ch, choroid plexus; DG, dentate gyrus; GC, granule cell layer of the cerebellum; St, striatum; syn, syndecan; Th, thalamus. Scale bars, 400 µm.

In contrast to that for syndecan-4, the ISH signal for syndecan-2 and -3 in the hippocampus is concentrated over neuronalcell bodies of the dentate granule cell layer and the CA1/CA3pyramidal cell layers (Fig. 1G; data not shown). Thus both syndecan-2and -3 are expressed predominantly in neurons. In summary, theseISH studies reveal syndecan-2 and -3 to be the major neuronalsyndecans of the forebrain, whereas syndecan-4 is expressed specificallyin glial cells. Because of our particular interest in the functionsand interactions of syndecans in neurons of the forebrain, wefocus in this report on syndecan-2 and -3.

Specificity of syndecan-2 and -3 antibodies

To study syndecan-2 and -3 at the protein level, we raised rabbit polyclonal antibodies against specific peptide sequencesin the intracellular C-terminal tail of syndecan-2 and -3 (Fig.2A). By immunoblotting and by immunocytochemistry, Syn-2C antibodieswere able to recognize syndecan-2 expressed heterologously inCOS-7 cells (Fig. 2B,C). As is typical for HSPGs, heterologouslyexpressed syndecan-2 ran on immunoblots as a highly heterogeneoussmear of bands, ranging in apparent size from ~40 to ~200 kDaon TBE/urea gels (Fig. 2B). Syn-2C antibodies showed significantcross-reactivity with syndecan-4 but not syndecan-1 or -3 (Fig.2B,C). This is not surprising because the cytoplasmic tails ofsyndecan-2 and -4 are the most closely related within the syndecanfamily (see Fig. 2A).

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Figure 2. Characterization of Syn-2C and Syn-3C antibodies. A, Amino acid alignment of the cytoplasmic C-terminal tails of syndecan-1 to -4 is shown. Syn-2C and Syn-3C antibodies were raised against the underlined peptide sequences in the cytoplasmic domains of syndecan-2 and -3, respectively. Dashes represent gaps in the sequence introduced to maximize alignment of conserved sequences. B, Specificity of Syn-2C and Syn-3C antibodies was tested by immunoblotting using COS-7 cells transfected with syndecan-1, -2, -3, or -4 or vector alone, as indicated. Syn-2C recognizes heterologously expressed syndecan-2 and cross-reacts with syndecan-4. Syn-3C-1 specifically recognizes two protein bands (~83 kDa, arrow; ~130 kDa, arrowhead) in COS-7 cells transfected with syndecan-3 but not other syndecans. Similar results were obtained with Syn-3C-2 antibodies (data not shown). Syn-3ecto antibodies also recognize the ~83 kDa band, as well as a broad high-molecular weight smear that likely represents more fully modified, cleaved forms of syndecan-3. C, Specificity of Syn-2C and Syn-3C antibodies on immunofluorescence staining of COS cells transfected with syndecan-1, -2, -3, or -4, as indicated, is shown. D, Syn-3C antibodies immunoprecipitate syndecan-3 from rat brain extracts. Immunoprecipitation with affinity-purified Syn-3C antibodies (Syn-3C-1 and Syn-3C-2 are from different rabbits) was performed using P8 rat brain extracts. Immunoprecipitates were immunoblotted with Syn-3ecto or Syn-3C antibodies, as indicated. Control immunoprecipitations were performed with nonimmune purified rabbit IgGs (IgG). The ~150 kDa band is indicated by an arrow, and the 150-250 kDa smear is indicated by the bracket. An input lane contains 10% of the detergent extract used for immunoprecipitation (IP).

For syndecan-3, two rabbit antisera raised against the same peptide (termed Syn-3C-1 and Syn-3C-2) gave essentially identicalresults (Fig. 2; data not shown). Neither of these Syn-C antibodiesshowed reactivity against syndecan-1, -2, or -4, but they didspecifically recognize two bands on Western blots of syndecan-3-transfectedCOS-7 cells (a major band of ~83 kDa; a minor band of ~130 kDa;Fig. 2B). Syn-3C antibodies were also specific for syndecan-3by immunofluorescence staining (Fig. 2C).

Interestingly, the pattern of Western bands recognized by Syn-3C (directed against the cytoplasmic tail of syndecan-3) differedfrom that seen by Syn-3ecto antibodies [which are specific foran extracellular region of syndecan-3 (Carey et al., 1992)]. TheSyn-3ecto antibodies recognized the ~83 kDa band in common withSyn-3C antibodies but in addition revealed a strong smear of syndecan-3immunoreactivity that extended well beyond ~200 kDa (Fig. 2B,compare middle with right panels). The heterogeneity of bandsseen by the Syn-3ecto antibodies is typical of HSPGs on proteingels. The simplest explanation for the difference between theimmunoblotting patterns of Syn-3C and Syn-3ecto antibodies isthat the majority of the higher molecular weight species (thesmear) consists of syndecan-3 that has lost its short cytoplasmictail. Such an interpretation is consistent with the known extracellularcleavage of syndecan HSPGs, which occurs at a site close to themembrane in both cultured cells and in vivo (Carey et al., 1997;Subramanian et al., 1997). The ~83 kDa band presumably representsan "immature" form of syndecan-3 that has been partially modifiedbut not yet cleaved, thus maintaining the connection between cytoplasmicandectodomains.

To explore this issue further in vivo, we reasoned that unless all of syndecan-3 in the brain is cleaved at the juxtamembranesite, Syn-3C antibodies should immunoprecipitate a subset of endogenoussyndecan-3 that should also be recognized by Syn-3ecto antibodies.Indeed, Syn-3C immunoprecipitates from brain extracts at P8 containeda high-molecular weight smear that was reactive for Syn-3ectoantibodies (Fig. 2D, left). This result indicates that uncleaved("intact") syndecan-3 is present in these brain extracts; in addition,it provides further evidence of the correct specificity of bothsyndecan-3 antibodies. As expected, Syn-3C immunoprecipitatescontained a high-molecular weight smear that was recognized bySyn-3C antibodies (Fig. 2D, right). Significantly, however, theSyn-3C antibodies precipitated only ~5% of the Syn-3ecto immunoreactivityfrom the extract, whereas in the same reaction, ~30-50% of theSyn-3C immunoreactivity was precipitated (Fig. 2D, compare leftwith right panels). If syndecan-3 was completely intact, equalfractions of intracellular and extracellular domains should coprecipitate;our finding therefore implies that the Syn-3ecto epitope is associatedwith the Syn-3C epitope with a stoichiometry of much less thanone. The simplest explanation of these results is that a majorityof syndecan-3 in the brain is cleaved at the juxtamembrane site,thereby separating the ectodomain from the cytoplasmic domain.Note also that Syn-3C antibodies recognize a lower band of syndecan-3(~150 kDa) in the brain more prominently than do Syn-3ecto antibodies(Fig. 2D, arrow). This band likely represents an immature intactsyndecan-3, which constitutes a larger proportion of the Syn-3C-immunoreactivepool than of the Syn-3ecto-immunoreactive pool. With postnatalmaturation of the brain, this ~150 kDa band becomes increasinglyprominent relative to the higher molecular weight smear on Syn-3Cimmunoblots (data not shown; see Fig. 3), suggesting that thehigher molecular weight forms of syndecan-3 are more completelycleaved as brain development progresses. In summary, brain syndecan-3runs as a high-molecular weight smear, as expected for a HSPG;and the majority of high-molecular weight syndecan-3 lack thecytoplasmic domain, presumably because of juxtamembrane cleavageof theprotein.

Differential biochemical fractionation of cytoplasmic and extracellular epitopes of syndecan-3 in brain

We investigated the subcellular distribution of syndecan-3 protein by biochemical fractionation of brain homogenates. Interestingly,the fractionation profile of bands recognized by Syn-3C was verydifferent from that recognized by Syn-3ecto antibodies (Fig. 3).In adult brain, Syn-3C recognizes predominantly the ~150 kDa bandnoted previously, whereas Syn-3ecto labels predominantly a broadsmear of M_r ~150-250 kDa (Fig. 3A). The ~150 kDa band must thereforecontain the cytoplasmic domain of syndecan-3 and can be consideredan immature uncleaved form of syndecan-3. As befits an intacttransmembrane protein, this ~150 kDa Syn-3C-reactive band is foundonly in particulate or membrane fractions such as P1, P2, andLP1 and not in the soluble fraction S3. The bulk of this syndecan-3species [which we will term "syndecan-3(C150)" because it containsthe cytoplasmic tail and runs at ~150 kDa] is present in the P1fraction, which is enriched in cell soma, nuclei, and nuclei-associatedmembranes (Fig. 3). In contrast, the Syn-3ecto-reactive smearof ~150-250 kDa (which we will term "syndecan-3ecto") purifiespredominantly into the microsome-enriched fraction (P3) and thesoluble fraction (S3) of brain. (S2 also contains abundant syndecan-3ecto,but this is the parent fraction from which S3 and P3 are derived).The solubility of the ~150-250 kDa smear recognized by Syn-3ectobut not by Syn-3C antibodies is entirely consistent with thisset of polypeptides being extracellularly cleaved syndecan-3 thathas been "shed" from the membrane without its transmembrane andcytoplasmic domains. This shedding need not be from the cell surfacebut could also be occurring within the lumen of intracellularmembrane compartments. Such a possibility is consistent with theabundance of the Syn-3ecto-reactive smear in P3 (microsome-enrichedfraction) and in LP2 (a synaptic vesicle-enriched fraction thatis isolated after hypotonic lysis of the P2 synaptosomal fraction).The differential fractionation of Syn-3C- and Syn-3ecto-immunoreactivebands in the brain extends the COS cell results, strongly supportingthe idea that the majority of endogenous syndecan-3 is cleavedand shed from the membrane in vivo.

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Figure 3. Subcellular fractionation and biochemical association of syndecan-3 and CASK in rat brain. A, Immunoblotting of subcellular fractions of rat brain with Syn-3C, Syn-3ecto, and CASK antibodies. B, Coimmunoprecipitation of CASK and syndecan-3 from P7 rat brain extracts by affinity-purified Syn-3C-1 antibodies. Negative control precipitations were performed with purified nonimmune rabbit IgG (lane 2) or after preincubation of Syn-3C-1 antibody with antigenic peptide (pep) (lane 4). Input lanes contain 10% (for Syn-3C immunoblot) or 5% (for CASK and PSD-95 immunoblots) of the detergent extract used for immunoprecipitation. Immunoprecipitates were probed for syndecan-3, CASK, and PSD-95. The arrow and bracket are described in Figure 2D. H, Total homogenate; other fractions are described in Materials and Methods.

Perhaps because of the low sensitivity of these antibodies and/or the low expression levels of endogenous syndecan-2, ourSyn-2C antibodies were unable to detect signals by Western blottingof rat brain, despite being able to recognize syndecan-2 overexpressedin COS cells. Another possibility is that the Syn-2C antibodiesrecognize a folded conformation of syndecan-2 that is destroyedby SDS-PAGE. Thus we were unable to investigate fractionationbehavior and shedding of syndecan-2 in vivo. CASK, a cytoplasmicprotein, is widely distributed among membrane and soluble fractionsin rat brain (Fig. 3A).

In a previous study we were unable to show coimmunoprecipitation of CASK and syndecan-2 from brain extracts (Hsueh et al.,1998), probably because our Syn-2C antibodies were inadequate.With the better antibodies against syndecan-3, however, we wereable to coimmunoprecipitate CASK with syndecan-3 antibodies (Fig.3B). This coimmunoprecipitation was eliminated by preincubatingthe Syn3-C antibodies with the immunogen peptide and is not seenwith nonspecific IgGs, testifying to its specificity. Moreover,PSD-95 was not coprecipitated with syndecan-3 and CASK (Fig. 3B).These results confirm that CASK is associated with syndecan-3in a protein complex in vivo.

Regional distribution of syndecan-3 in rat brain

We next used immunohistochemistry to examine the distribution of syndecan-3 in rat brain. Throughout postnatal developmentand in all regions of the brain, white matter tracts and axonpathways were the predominant structures stained by both Syn-3Cand Syn-3ecto antibodies (Fig. 4; data not shown). A quantitativedifference only was noticed in that syndecan-3 immunostainingis stronger at P3, P7, and P15 than in the adult, consistent witha higher level of syndecan-3 expression at early postnatal stages(Carey et al., 1997). In P7 rat brain, both Syn-3ecto and Syn-3Cshowed very similar fiber-like staining in axon tracts and inwhite matter, e.g., the corpus callosum (Fig. 4D,E), fimbria,and alveus of the hippocampus (Fig. 4B,C). These data suggestthat syndecan-3 protein is concentrated in axons. However, significantdifferences were noted between the staining pattern of Syn-3Cversus Syn-3ecto antibodies. In addition to the strong axonaland white matter staining, Syn-3C antibodies gave weaker signalsthat were not detected by Syn-3ecto antibodies: for instance,in the pyramidal neurons of the cerebral cortex (compare Fig.4D vs E) and in the dentate gyrus and region CA3 of the hippocampus(Fig. 4B vs C). Overall, the Syn-3C immunohistochemistry patternis consistent with the ISH results. Syn-3C labeling was virtuallyabolished by preincubation of the antibodies with the antigenicpeptide (Fig. 4F), indicating the specificity of the Syn-3C immunostaining.The differences that exist between the Syn-3C- and Syn-3ecto-stainingpatterns may be accounted for by the shedding of the ectodomainof syndecan-3 after extensive cleavage of that occurs in the brain(see above). The cleaved syndecan-3 ectodomain may be relativelydispersed in the tissue or lost during the permeabilization andwashing steps of the immunostaining procedure, hence giving riseto the reduced staining with Syn-3ecto antibodies. Nevertheless,staining with both Syn-3C and Syn-3ecto antibodies indicates thatsyndecan-3 is concentrated in axon tracts of the brain, in agreementwith previous reports (Nolo et al., 1995; Carey et al., 1997).

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Figure 4. Localization of syndecan-3 in P7 rat brain by DAB immunohistochemistry. A, Syn-3C immunoreactivity is highly concentrated in axonal pathways [e.g., the fimbria (fi) and alveus (alv) of the hippocampal formation], the cc, and axon tracts running through the thalamus (arrowheads). B-E, Staining patterns of antibodies Syn-3C (B, D) and Syn-3ecto (C, E) are compared in the hippocampal formation (B, C) and cerebral cortex (D, E). F, Preincubation with Syn-3C antigenic peptide blocks the Syn-3C immunostaining of the corpus callosum and alveus; weak background staining of cell bodies of CA1 remains. G, Syn-3C antibodies strongly label the white matter (w) of the cerebellum. dg, Dentate gyrus; P, Purkinje cell layer. Scale bar: A, 400 µm; B--E, G, 350 µm; F, 150 µm.

Confocal immunofluorescence microscopy confirmed the association of syndecan-3 with axons (Fig. 5). Bright syndecan-3 stainingwas seen on axons of the mossy fiber tract (Fig. 5A), axons ofthe corpus callosum, stria terminalis, and cerebellar white matter(Fig. 5B-D), and axons of cerebellar basket cells (Fig. 5E1).

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Figure 5. Axonal localization of Syn-3C immunoreactivity in adult rat brain, revealed by immunofluorescence microscopy. Localization of syndecan-3 in axons is shown in the dentate gyrus of the hippocampus (A), the corpus callosum (B), the stria terminalis (C), the white matter of the cerebellum (an axon bundle is cut in cross section) (D), and basket cells of the cerebellum (E). In E1 and E2, the same field is double labeled by Syn-3C (E1) and synaptophysin (E2) antibodies. M, Molecular layer of the cerebellum; mf, mossy fiber tract; p, Purkinje cell bodies. Scale bar, 40 µm.

Axonal distribution of CASK in developing rat brain

Because CASK is complexed with syndecan-3, at least in part (Fig. 3B), we examined whether CASK might also be localized inaxons. In adult rat brain, CASK is distributed predominantly ina somatodendritic pattern, with enrichment at synaptic sites (Hsuehet al., 1998). However, in contrast to PSD-95, CASK is expressedthroughout brain development, with protein levels at embryonicstages (E14 and E18) as high, if not higher, as in adult brain(Fig. 6A). Immunohistochemistry was performed to determine CASKlocalization from P3 to P42. At P3, CASK immunoreactivity is indeedprominently found in axon tracts and white matter, such as thecorpus callosum, mossy fiber tract, alveus, and fimbria of thehippocampus and the internal capsule and white matter of the cerebellum(Fig. 6B,C). In this respect, the distribution of CASK is remarkablysimilar to that of syndecan-3 in the first week or so after birth[compare Figs. 4A with 6B (P7)]; thus CASK is appropriately locatedto be interacting with syndecan-3 in axons of developing brain.In addition to the axonal staining, however, CASK immunoreactivityis also present in a somatodendritic pattern, even in early postnatalbrain. With increasing age, CASK staining in the forebrain andcerebellum shifts progressively from a predominantly axonal patternto a predominantly somatodendritic pattern (Fig. 6B,C) (Hsuehet al., 1998). By the end of the third week, CASK is barely detectablein white matter but found mostly in a somatodendritic distribution,e.g., in Purkinje cells of the cerebellum (Fig. 6C) and in pyramidalcells of the forebrain (Hsueh et al., 1998) (data not shown).As noted above, the levels of syndecan-3 in axons also fall afterthe first 2 weeks of postnatal development.

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Figure 6. Expression and subcellular distribution of CASK during rat brain development. A, Developmental expression of CASK in rat brain. Ten micrograms of brain membrane fractions from rats at the indicated ages were immunoblotted with CASK and PSD-95 antibodies. B, C, Immunohistochemistry for CASK in forebrain (B) and cerebellum (C) at the indicated postnatal ages. Scale bars: A, 1 mm; B, 0.5 mm.

Axonal distribution of syndecan-3 and CASK in cultured cortical neurons

To confirm further the axonal distribution of syndecan-3 and CASK in neurons, we performed immunofluorescence staining inprimary cortical cultures. In double-labeling experiments, Syn-3Cantibodies stained long, fine processes that were positive forTau but negative for MAP2, indicating the specific localizationof syndecan-3 in axons (Fig. 7Aa,Ab). Similar results were obtainedfor cultured hippocampal neurons (data not shown). Preincubationwith the immunogen peptide for Syn-3C blocked Syn-3C stainingof axons (Fig. 7Ac), indicating the specificity of the signal.CASK antibodies also stained axons intensely, and by double labeling,CASK could be shown to colocalize with syndecan-3 in the sameaxons (Fig. 7Ad). In addition, CASK was also present in dendriticprocesses that were negative for syndecan-3 (Fig. 7Ad). Thus,the immunocytochemistry of cultured neurons is consistent withfindings in the brain; syndecan-3 is concentrated in axons, whereasCASK is both dendritic and axonal. The overlapping distributionof CASK and syndecan-3 in axons and their coimmunoprecipitationfrom brain extracts are consistent with the direct associationof CASK and syndecan-3 in the axonal compartment.

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Figure 7. Syndecan-3 is localized in axons but excluded from synapses. A, Axonal localization of syndecan-3 in cultured cortical neurons. Double immunofluorescence labeling of cultured cortical neurons with Syn-3C and MAP2 (a), Syn-3C and Tau (b, c), and Syn-3C and CASK monoclonal K56A/50 (d) is shown. In c, Syn-3C antibodies were preincubated with syndecan-3 antigenic peptide. Each set of images (a1-a3, b1-b3, etc.) represents the same field visualized for syndecan-3 (Cy3, red; left) or for MAP2, Tau, or CASK (FITC, green; middle). The right image is an overlay of the first two (showing colocalization in yellow). B, Subcellular segregation of syndecan-2 and -3 in adult rat brain, revealed by double immunostaining with synaptophysin. Sections were double labeled with Syn-2C and synaptophysin antibodies (synap.) (a, c) or Syn-3C and synaptophysin antibodies (b, d). Confocal images were collected from the granule cell layer (GCL) of the cerebellum (a, b) and region CA4 of the hippocampus (c, d). Syndecan-2 and -3 were visualized by Cy3 (red), and synaptophysin was visualized by FITC (green) secondary antibodies. Scale bars, 20 µm.

Differential subcellular localization of syndecan-2 and -3

Syndecan-2 is localized in central neuronal synapses (Hsueh et al., 1998), where it is highly colocalized with synaptophysin(Fig. 7B). By contrast, the pattern of labeling of syndecan-3shows no overlap with synaptophysin staining, even in neuropilregions of the brain (Fig. 7B). Thus syndecan-2 (in synapses)and syndecan-3 (in axons) are segregated in complementary compartments;syndecan-3 seems to be mainly axonal in distribution, with littleencroachment into axonterminals.

The Syn-2C antibodies cross-react with syndecan-4, which is expressed in glial cells in vivo (see Figs. 1, 2). The synapticSyn-2C immunoreactivity is unlikely to arise from glial cells,however, because our previous immunogold EM studies have shownthe Syn-2C labeling to be specifically associated with the postsynapticdensity and the presynaptic terminal at brain synapses (Hsuehet al., 1998). Moreover, we have not observed glial staining inthe brain with our Syn-2C antibodies, suggesting that their cross-reactivityin vivo is notsignificant.

Developmental pattern of syndecan-2 expression

HSPGs bind to extracellular matrix proteins and signaling factors; thus changes in HSPG expression and distribution couldplay a role in neuronal migration, neurite extension, and synapseformation during development of the nervous system. We found noobvious change in the axonal distribution of syndecan-3 duringpostnatal brain development, except for a sharp reduction in stainingintensity after the first 2 weeks. Because syndecan-2 is enrichedat synaptic junctions and may play a role in synaptogenesis, wewere particularly interested in the developmental regulation ofsyndecan-2 distribution. We examined in detail the pattern ofSyn-2C staining during the development of the cerebellum, whichprogresses through a well-characterized postnatal maturation inthe rat. Syn-2C labeling during cerebellar synaptogenesis wascompared with the distribution of synaptophysin (Fig. 8A). Inaddition, we used anti-calbindin-D antibody (which strongly labelsPurkinje cells and their dendrites) to delineate Purkinje cellsand the molecular layer of the developing cerebellar cortex (Fig.8B).

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Figure 8. Coordinate layer-specific expression of syndecan-2 and synaptophysin in developing rat cerebellum. Double-label immunofluorescence of the cerebellum at P3, P7, P15, and P22 with Syn-2C and synaptophysin antibodies (A) or with Syn-2C and calbindin antibodies (B). Synaptophysin and calbindin were used as markers for synapses and Purkinje cells, respectively. Each pair of images represents confocal images of the same field visualized for one or the other antibody, as indicated. Scale bars, 100 µm.

From as early as P3 through adulthood, the layer-specific pattern of Syn-2C staining matches that of synaptophysin (Fig. 8A).At P3, coexpression of syndecan-2 and synaptophysin occurs inthe developing Purkinje cell layer (P) and in the internal granularlayer (IGL). In contrast, both syndecan-2 and synaptophysin areabsent from the external granular layer (EGL), where the granulecells are immature. Expression of syndecan-2 and synaptophysinincreases in parallel, such that at P7 and P15, there is veryintense labeling in the developing molecular layer (ML), withnotable sparing of Purkinje cell bodies. During these first 2weeks, syndecan-2 and synaptophysin also become increasingly expressedin the IGL, where the distributions of both proteins graduallycondense into glomerular structures by P22 (Fig. 8A). The correlateddistribution and intensity of Syn-2C and synaptophysin stainingsuggest that syndecan-2 is being selectively expressed in thoseareas of the developing cerebellum that are undergoing activesynaptogenesis, namely, in the molecular layer, where granulecell parallel fiber axons are synapsing with Purkinje cell dendrites,and in the IGL, where granule cell dendrites form glomerular synapseswith ascending mossy fibers. In the mature cerebellum (P22), theintensity of Syn-2C staining falls, particularly in the deeperhalf of the molecular layer. At this stage, the glomeruli of thegranule cell layer are the most prominent sites of Syn-2C as wellas synaptophysin staining. In summary, the temporal and spatialpattern of syndecan-2 distribution in the developing cerebellumbroadly matches that of the synaptic marker synaptophysin, indicatingthat expression of syndecan-2 occurs in step withsynaptogenesis.

Interestingly, high-resolution confocal imaging reveals that syndecan-2 does not colocalize with synaptophysin at early developmentaltime points. Syn-2C immunoreactivity is highly punctate in natureas early as P3 in the cerebellum, as is synaptophysin (Fig. 9,left). However, at P3, the syndecan-2 puncta were less abundantthan synaptophysin hot spots and showed little overlap with them.During the next 2 weeks of postnatal development, however, thedegree of colocalization of syndecan-2 and synaptophysin increased.By P22, the distribution of syndecan-2 almost exactly matchedthe distribution of synaptophysin-positive synapses (Fig. 9, left).Similar results were obtained in region CA3 of the hippocampus.At P3 and P7, Syn-2C immunoreactivity is present in cell bodiesof the pyramidal cell layer and in a punctate pattern in the stratumlucidum; these puncta colocalized poorly with synaptophysin (Fig.9, right). With maturation, the level of syndecan-2 staining inpyramidal cell bodies decreased, whereas punctate syndecan-2 colocalizationwith synaptophysin increased in the stratum lucidum. Collectively,these data indicate that the accumulation of syndecan-2 in synapsesis a relatively late event in synapse assembly, occurring afterclustering of synaptophysin.

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Figure 9. Synaptic localization of syndecan-2 occurs late in synapse development. Relationship of Syn-2C and synaptophysin staining in the IGL of the cerebellum and in the CA3 region of the hippocampus during postnatal development examined by double-label immunofluorescence confocal microscopy at P3, P7, P15, and P22. Syn-2C is visualized by Cy3 (red), and synaptophysin is visualized by FITC (green). The composite images show colocalization in yellow. P, Pyramidal cell layer; sl, stratum lucidum. Scale bars: IGL, 10 µm; CA3, 20 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Differential subcellular distribution of syndecan-2 and -3 in neurons

In this study we have shown that each member of the syndecan family of cell surface HSPGs exhibits a distinctive cell type-specificexpression pattern in rat brain. Syndecan-1 is primarily restrictedto cerebellar granule cells, whereas syndecan-4 is specificallyexpressed in glial cells. Recently, Ethell and Yamaguchi (1999)have found by immunostaining that syndecan-4 is specifically expressedby astrocytes in hippocampal culture, in agreement with our ISHfindings in vivo. In forebrain neurons, syndecan-2 and -3 (thelatter known previously as neuronal- or N-syndecan) are predominant.The functional significance of these cell type-specific expressionpatterns isunknown.

Even though their mRNAs are expressed within overlapping populations of neurons, syndecan-2 and -3 are segregated at the proteinlevel within neurons. Syndecan-2 is specifically localized tosynapses (see also Hsueh et al., 1998), whereas syndecan-3 isconcentrated in axons. What might be the mechanism underlyingthe differential subcellular distribution of these two neuronalsyndecans? Targeting determinants for syndecan-2 and -3 may existin the extracellular or intracellular domains of these transmembraneproteins. The extracellular regions of all syndecans show limitedsequence similarity except at sites of GAG chain addition. Thisweak conservation of primary structure has con-ventionally beeninterpreted as reflecting the fact that it is the HS side chainsrather than the core protein that mediate the important extracellularinteractions of syndecans. However, it remains possible that targetingsignals are contained in the divergent extracellular regions.By contrast, there is high sequence conservation in the shortcytoplasmic C-terminal tails of syndecans (see Fig. 2A) (for review,see Bernfield et al., 1992; David, 1993; Carey, 1997; Rapraegerand Ott, 1998). The C-terminal sequence -EFYA has been shown tobind to the PDZ domains of syntenin (Grootjans et al., 1997) andCASK (Cohen et al., 1998; Hsueh et al., 1998). Because all syndecansshare an identical -EFYA C-terminal sequence, it seems unlikelythat their subcellular segregation can be primarily dictated bydifferential interactions with CASK, syntenin, or other PDZ domainproteins. Indeed, the -EFYA C-terminal motif is not required forthe localization of syndecan-2 in dendritic spines (Ethell andYamaguchi, 1999). Outside of the C terminal and the juxtamembraneregion, however, significant sequence differences between syndecansoccur in the middle of the cytoplasmic tail. This region of syndecan-4is reported to bind specifically to protein kinase C (Oh et al.,1997). It is possible that the "middle" cytoplasmic domain ofsyndecans can associate with different intracellular proteinsinvolved in targeting and/or signaling. Domain swap experimentsbetween syndecan-2 and -3 would be a reasonable approach to sortout the mechanisms for the differential targeting of these proteins.More challenging will be figuring out why different syndecansshould be specifically sorted to distinct regions of theneuron.

Proteolytic cleavage of syndecan

We obtained direct evidence of extracellular cleavage of syndecan-3 in vivo by the loss of linkage between the extracellularSyn-3ecto epitope and the cytoplasmic Syn-3C epitope. The greatmajority of syndecan-3 appears to lack the cytoplasmic tail, onthe basis of semiquantitative immunoprecipitation results (Fig.2D). Consistent with this idea is that syndecan-3 purified frombrain fails to react with an antibody directed against the cytoplasmicdomain (Bernfield et al., 1993).

The cleavage and shedding of the majority of syndecan ectodomains in vivo change the functional implications of syndecan action.Syndecans are generally considered cell surface HSPGs involvedin cell-matrix adhesion or low-affinity coreceptors for heparin-bindinggrowth and/or differentiation factors. After cleavage, however,syndecan ectodomains can be shed from the plasma membrane andassociate with the extracellular matrix rather than the cell surface.In this way, syndecan ectodomains may provide HSPGs to the ECM,perhaps contributing to an extracellular HSPG reservoir for retentionand storage of heparin-binding factors (Loeb and Fischbach, 1995;Loeb et al., 1999). It is also plausible that syndecan ectodomainsare coreleased with secreted molecules that bind to heparan sulfate,thereby acting as "chaperones" conveying heparin-binding factorsinto the extracellular space. We note, for instance, that syndecan-2is present in presynaptic terminals as well as at postsynapticsites (Hsueh et al., 1998) and that it may be part of an exocytosiscomplex via its interaction with CASK (Butz et al., 1998). Itwill be interesting therefore to determine whether the degreeof "shedding" is similar for all the syndecan family members andhow this process is regulated during development or in responseto neuralactivity.

Changing distribution of CASK during brain development and its axonal colocalization with syndecan-3

We showed previously that CASK is distributed in a somatodendritic pattern in adult brain and that it is coenriched with syndecan-2at synaptic junctions (Hsueh et al., 1998). Here we report thatthe subcellular distribution of CASK is prominently axonal inearly postnatal brain. In its developmental shift from an axonalto a synaptic distribution, CASK resembles several other proteinssuch as Fasciclin II (Zito et al., 1997); Discs large (Lahey etal., 1994), and Eph receptor tyrosine kinases (Torres et al.,1998). The functional significance of syndecan-3-CASK interactionsin developing axons remains to be determined. On the basis ofthe binding properties of cell surface HSPGs, we speculate thatthe syndecan-3-CASK complex may be involved in adhesive or signalingfunctions during axon growth, migration, and/or fasciculation.In this context, it is noteworthy that syndecan-3 has been isolatedas a receptor or coreceptor for the heparin-binding growth-associatedmolecule, a molecule that promotes neurite outgrowth (Raulo etal., 1994). Syndecan-3 has also been reported to copurify withcortactin and Fyn tyrosine kinase and to show increased expressionin response to synaptic activity (Lauri et al., 1999).

Neurexins, a highly heterogeneous family of neuronal cell surface proteins, are also binding partners for the PDZ domainsof CASK (Hata et al., 1996; Missler et al., 1998). Like that ofthe syndecans, neurexin immunoreactivity has been localized atsynapses (Ushkaryov et al., 1992) and on axons (Russell and Carlson,1997). It will be interesting to determine how the expressionlevel and subcellular distribution of neurexins are regulatedduringdevelopment.

Role of syndecan-2 in synapses

Although syndecan-2 is specifically localized in synapses in adult brain, our data suggest that its concentration in synapses(as defined by synaptophysin clusters) occurs relatively latein synapse development. Thus synaptic contacts form initiallyin the absence of detectable syndecan-2. Our results in vivo areconsistent with the findings of Ethell and Yamaguchi (1999) invitro. These investigators found that syndecan-2 was localizedspecifically in dendritic spines of cultured hippocampal neuronsbut that expression of syndecan-2 was detectable only after 2weeks in vitro and increased in the following weeks. This timecourse lags behind that of synapse formation in hippocampal culture(Rao et al., 1998). Moreover, forced expression of syndecan-2in neurons at an early stage in culture (when endogenous syndecan-2is not normally expressed) accelerated the development of dendriticspine morphology but did not affect the number of spines or synapses(Ethell and Yamaguchi, 1999). Taken together with the late accumulationof syndecan-2 in synapses, these findings imply that syndecan-2is involved in a late stage of synaptic development, such as themorphological maturation of dendritic spines, rather than in specifyingthe formation ofsynapses.

  FOOTNOTES

Received April 28, 1999; revised June 7, 1999; accepted June 10, 1999.

M.S. is Assistant Investigator of the Howard Hughes Medical Institute. This work was supported by National Institutes of HealthGrant NS35050 (M.S.). We thank James Trimmer and Lynn Buchwalderfor preparing the CASK monoclonal antibodies; David Carey forsyndecan-3 cDNA and syndecan-3ecto antibody; Graham Cowling forsyndecan-2 cDNA; Fu-Chia Yang, Jai-Up Kim, Sheila Rudolph, JerryLin, and Carlo Sala for experimental help and advice; DmitriyLeyfer and Merton Bernfield for advice on HSPG immunoblotting;and Elaine Aidonidis for help with thismanuscript.
Correspondence should be addressed to Dr. Morgan Sheng, Howard Hughes Medical Institute, Massachusetts General Hospital (Wellman423), 50 Blossom Street, Boston, MA02114.

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