Reg1ulatory Role and Molecular Interactions of a Cell-Surface Heparan Sulfate Proteoglycan (N-syndecan) in Hippocampal Long-Term Potentiation

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (55)

Citing Articles via Google Scholar

Google Scholar

Articles by Lauri, S. E.

Articles by Rauvala, H.

Search for Related Content

PubMed

PubMed Citation

Articles by Lauri, S. E.

Articles by Rauvala, H.

Previous Article  |  Next Article

The Journal of Neuroscience, February 15, 1999, 19(4):1226-1235

Reg1ulatory Role and Molecular Interactions of a Cell-Surface Heparan Sulfate Proteoglycan (N-syndecan) in Hippocampal Long-Term Potentiation
S. E. Lauri¹^,², S. Kaukinen², T. Kinnunen², A. Ylinen³, S. Imai², K. Kaila¹, T. Taira¹, and H. Rauvala²
¹ Department of Biosciences, Division of Animal Physiology, 00014 University of Helsinki, Helsinki, Finland, ² Laboratory of Molecular Neurobiology, Institute of Biotechnology and Department of Biosciences, 00014 University of Helsinki, Helsinki, Finland, and ³ A. I. Virtanen Institute and Department of Neuroscience and Neurology, University of Kuopio, 70211 Kuopio, Finland

  ABSTRACT

Top
Abstract
Introduction
References

The cellular mechanisms responsible for synaptic plasticity involve interactions between neurons and the extracellular matrix.Heparan sulfates (HSs) constitute a group of glycosaminoglycansthat accumulate in the $beta$ -amyloid deposits in Alzheimer's diseaseand influence the development of neuron-target contacts by interactingwith other cell surface and matrix molecules. However, the contributionof HSs to brain function is unknown. We found that HSs play acrucial role in long-term potentiation (LTP), a finding that isconsistent with the idea that converging molecular mechanismsare used in the development of neuron-target contacts and in activity-inducedsynaptic plasticity in adults. Enzymatic cleavage of HS by heparitinaseas well as addition of soluble heparin-type carbohydrates preventedexpression of LTP in response to 100 Hz/1 sec stimulation of Schaffercollaterals in rat hippocampal slices. A prominent carrier proteinfor the type of glycans implicated in LTP regulation in the adulthippocampus was identified as N-syndecan (syndecan-3), a transmembraneproteoglycan that was expressed at the processes of the CA1 pyramidalneurons in an activity-dependent manner. Addition of soluble N-syndecaninto the CA1 dendritic area prevented tetanus-induced LTP. A majorsubstrate of src-type kinases, cortactin (p80/85), and the tyrosinekinase fyn copurified with N-syndecan from hippocampus. Moreover,association of both cortactin and fyn to N-syndecan was rapidlyincreased after induction of LTP. N-syndecan may thus act as animportant regulator in the activity-dependent modulation of neuronalconnectivity by transmitting signals between extracellular heparin-bindingfactors and the fyn signalingpathway.

Key words: long-term potentiation; synaptic plasticity; extracellular matrix; heparan sulfate proteoglycans; hippocampus; src family tyrosine kinases; cortactin

  INTRODUCTION

Top
Abstract
Introduction
References

Long-term potentiation (LTP) is a long-lasting augmentation of synaptic strength that has been suggested as a cellular mechanismunderlying learning and memory (Bliss and Collingridge, 1993;Larkman and Jack, 1995; Nicoll and Malenka, 1995). Considerableevidence suggests that the maintenance of LTP involves structuralrearrangements within neuronal connections (Lee et al., 1980;Chang and Greenough, 1984; Edwards, 1995) (but see also Sorraand Harris, 1998), a process that is critically dependent on cell-matrixinteractions. Antibodies or peptides inhibiting cell adhesionmolecules disrupt expression of LTP already at the early stages(Lüthi et al., 1994; Bahr et al., 1997; Tang et al., 1998), whichare dependent on the activity of protein kinases and phosphatases.Changes in kinase activity can directly influence synaptic transmissionby phosphorylation of postsynaptic neurotransmitter receptorsor components of the presynaptic releasing machinery (Walaas andGreengard, 1991; Smart, 1997). In addition, protein kinases, inparticular the src family tyrosine kinases, associate to and controlthe organization of the cytoskeleton, and may thereby regulatecellular morphology and biological functions dependent on it (Thomaset al., 1995; Lowell and Soriano, 1996).

Heparan sulfates (HSs) are glycosaminoglycans that influence cell-environment interactions by binding to a heterogeneous groupof growth factors, matrix ligands, and cell surface molecules(Gallagher, 1989; Rapraeger, 1993; Lindahl et al., 1994). In thenervous system, proteoglycans and factors binding to them havean important role in axonal guidance and synaptogenesis duringprenatal and early postnatal periods (Lander, 1993; Margolis etal., 1996; Rauvala and Peng, 1997). The majority of cell surfaceheparan sulfate proteoglycans belong to the family of syndecans,whose expression in rat brain is developmentally regulated (Bernfieldet al., 1992; Nolo et al., 1995; Carey, 1997). In addition, HSsand heparin-binding factors have been found to accumulate in the $beta$ -amyloid deposits in Alzheimer's disease (Snow et al., 1988,1994; Wisniewski et al., 1996) and are proposed to be importantfor the promotion, deposition, and persistence of the senileplaques.

Molecules whose cellular effects on the development of neuronal connections are modulated by or dependent on HS include atleast the neural cell adhesion molecule (NCAM) (Cole et al., 1986),fibroblast growth factors (FGFs) (Lander, 1993; Nurcombe et al.,1993), and heparin-binding growth-associated molecule (HB-GAM;Rauvala and Peng, 1997). Interestingly, all these three moleculeshave been found to influence LTP (Ishiyama et al., 1991; Lüthiet al., 1994; Lauri et al., 1998). Binding of HSs to several moleculesimplicated in synaptic plasticity suggests that HSs might playa key role in the regulation of brain function. Nevertheless,the possible role of HSs in synaptic transmission has not beenpreviouslyexamined.

Here we show that hippocampal LTP is critically dependent on heparan sulfates, and identify N-syndecan as a major heparansulfate proteoglycan expressed in the pyramidal neurons of hippocampus.The expression of N-syndecan as well as its interaction with theintracellular, cytoskeleton-regulating molecules cortactin andfyn-kinase was increased after LTP induction. Thus, we suggestthat N-syndecan is one of the molecules that modulate cell-matrixinteractions associated with synapticplasticity.

  MATERIALS AND METHODS

In vitro electrophysiological recordings and protein injections. Transverse slices (300-400 µm) were cut by means of a vibratomefrom the hippocampi of Wistar rats (100-200 gm), which were decapitatedunder deep pentobarbital anesthesia (30-40 mg/kg, i.p.). The sliceswere allowed to recover at room temperature for at least 60 minbefore any experiments were started. All the recordings were madeat +32°C in an interface-type chamber, which was perfused witha solution containing (in mM) NaCl 124, KCl 3, CaCl₂ 2, NaHCO₃25, NaH₂PO₄ 1.1, MgSO₄ 2, and glucose 10, and gassed with 5% CO₂and 95% O₂. A constant perfusion at a rate of ~1 ml/min was applied,except for the experiments with desulfated glycans, which weredone in a static perfusion (chamber volume, 1ml).

Extracellular recordings from CA1 stratum radiatum were made by using glass capillary microelectrodes filled with 150 mM NaCl.Intracellular current-clamp recordings were made from CA1 pyramidalneurons by using an Axoclamp 2A amplifier (Axon Instruments, FosterCity, CA) in active bridge mode. The intracellular electrodeswere filled with electrolyte solution that contained 1 M K⁺ methyl sulfate, 0.5 M K⁺ acetate, and 10 mM KCl, and their resistance was 70-120 M $Omega$ . Abipolar electrode was used for Schaffer collateral stimulation(pulse length, 100 µsec), and the stimulus intensity was adjustedto give a half-maximal field EPSP (fEPSP) amplitude. After atleast 10 min of stable baseline recording (0.05 Hz), LTP was inducedby high-frequency stimuli (100 Hz/1 sec), during which the pulselength was doubled. In some of the experiments (protein injections),induction of LTP in the slice was controlled by recording simultaneouslyan independent pathway. Asystant software package (MacMillan)was used for all data acquisition and analysis. The slope of fEPSPwas used as an indicator of synaptic efficacy and was calculatedbetween 20 and 80% of the maximalamplitude.

Organotypic hippocampal cultures were prepared from 9- to 11-d-old rats by the method of Stoppini et al. (1991). After 10-12d in culture, the slices were incubated for 15 hr with heparitinase(heparinase III, Sigma, St. Louis, MO) (1 U/ml) or bovine serumalbumin (BSA) (0.01%), and transferred to the recording chamberfor the measurement ofLTP.

N-syndecan was purified from rat brain as described (Raulo et al., 1994), and dialyzed against PBS before use. The proteinwas pressure-injected (Perfusor 1-300; B. Braun Melsungen AG)with a micropipette into the dendritic area of CA1 between stimulationand recording electrodes within 0.3 mm distance from the recordingsite. The protein ( $approx$ 3 × 0.3 µl) was applied by three brief injectionswithin 5 min. According to previous data, pressure-injected proteinsof sizes of 150 kDa (IgG; total amount, 0.5 pmol) and 18 kDa (HB-GAM;total amount, 1 pmol) can be detected by immunostaining in a 400-µm-thickhippocampal slice in a round-shaped area of a diameter of ~200µm and 1 mm, respectively (Ronn et al., 1995; Lauri et al., 1998).Based on the data above and the Stokes-Einstein relation, injectedN-syndecan (210 kDa, 0.1 pmol) is expected to spread into an areawith a diameter of ~50 µm.

In vivo electrophysiology. Male Wistar rats (250-300 gm) were anesthetized with urethane (1.3 gm/kg) and placed in a stereotaxicapparatus. The scalp was removed, and a small (1.5 × 1.5 mm) bonewindow was drilled above the hippocampus (the anteromedial edgeat anteroposterior = 3.3 and lateral = 2.2 mm from bregma). Apair of stimulating electrodes (60 µm wire) was lowered simultaneouslywith the recording electrode. The positioning of the recordingelectrode to CA1 stratum radiatum was based on stereotaxic coordinates,evoked responses, and on CA1 pyramidal cell unit monitoring. Thepair of stimulating electrodes was positioned into the same layer0.5 mm laterally. The signals were amplified by a Brownlee Model440 instrumentation amplifier and stored on a hard disk for off-lineanalysis. After a stable baseline recording, LTP was induced withthe same stimulation patterns as in vitro (100 Hz/1 sec) usinga stimulation intensity that yields a half-maximal fEPSP amplitude.During the recordings, the electrical activity of the hippocampuswas followed through oscilloscope and an audiomonitor, and noepileptiform discharges were observed. If potentiation of thefEPSP slope was <30% 1 hr after the high-frequency stimulation(HFS), the experiment was rejected. Control rats received thesame number of pulses at 0.05 Hz. The rats were perfusion-fixedfor immunohistochemistry and in situ hybridization 3-4 hr afterthe stimulation, a time period known to result in changes in theexpression of activity-regulated genes (Armstrong and Montiminy,1993; Silva and Giese, 1994).

In situ hybridization and immunohistochemistry. Anesthetized Wistar rats were perfused transcardially with 0.9% saline followedby 0.5% glutaraldehyde and 4% paraformaldehyde in 0.1 M sodiumphosphate buffer (pH 7.4; 5 min). A part of brain containing thehippocampi was removed and post-fixed overnight with 4% paraformaldehyde.Alternatively, hippocampal slices (400 µm) were fixed after electrophysiologicalrecordings with 4% paraformaldehyde in 0.1 M sodium phosphatebuffer, pH 7.4, for at least 4 hr. Fixed tissue was cryoprotectedin PBS containing 15% sucrose for several days, and 40 µm cryosectionswere cut transversally and treated in a free-floating state throughthe in situ or immunolabelingprocedures.

Antibodies against heparan sulfate 10E4 epitope were from Seikagaku Corporation (Tokyo, Japan) and were used for immunohistochemistryat a concentration of 10 µg/ml. Affinity-purified antibodies againstan N-terminal peptide of N-syndecan (described in Nolo et al.,1995) were used for immunohistochemistry at a concentration of0.1 µg/ml. The immunostain was visualized with biotinylated secondaryantibodies and the Vector Laboratories (Burlingame, CA) immunoperoxidasereagents. For electron microscopy, the stained sections were post-fixedwith 1% osmium tetroxide (1 hr), dehydrated in ethanol series,and embedded in Epon. Ultrathin sections (60 nm) were cut, stainedwith uranyl acetate and lead citrate, and examined by a transmissionelectron microscope (Jeol 1200;Jeol).

Sense and antisense digoxigenin-labeled RNA probes were synthesized in the presence of digoxigenin-11-UTP (Boehringer Mannheim,Indianapolis, IN) with T7 and T3 RNA polymerases from a linearizedpBluescript vector containing the full-length N-syndecan sequence,and were used at the concentration of 20 ng/ml. The hybridizationwas performed as described (Lauri et al., 1996), and the hybridizationsignal was detected by alkaline phosphatase-conjugated anti-digoxigenin-Fabfragments. The stained sections were digitized with an OlympusAX70 Provis microscope and a Photometrics Sensys CCD camera. Image-ProPlus 3.0 software was used for quantification of the intensityof the in situ and immunostain from the digitized images of thesections.

HB-GAM affinity chromatography and immunoblotting. HB-GAM binding proteins were purified from crude extracts of adult rathippocampi by HB-GAM affinity chromatography as described (Rauloet al., 1994). Bound proteins were eluted with a linear NaCl gradient,and the fractions were analyzed on 3-12% gradient SDS-PAGE. Tovisualize both proteins and proteoglycans, the gels were stainedwith Alcian blue-silver nitrate (Møller et al., 1993). Aliquotsof the fractions were digested with nitrous acid or heparitinase(10 U/ml, 15 hr) to remove carbohydrate side chains or incubatedwith 50 µM herbimycin A (Calbiochem, La Jolla, CA). Kinase activitywas assayed as described (Kinnunen et al., 1998).

For analysis of N-syndecan-binding components after induction of LTP, the CA1 region of a hippocampal slice was rapidly dissectedand frozen in liquid nitrogen 10 or 20 min after high-frequencySchaffer collateral stimulation. CA1 regions from nontreated slicesof the same animals were prepared for controls. The tissue washomogenized in ice-cold PBS containing 1% Nonidet P-40, 2 µg/mlaprotinin, 1 mM Na₃VO_4, 1 mM NaF, 0.7 µg/ml leupeptin, 0.5 µg/mlpepstatin, and 1 mM phenylmethylsulfonylfluoride. Lysates from5-10 slices were combined, and samples of equal protein concentrationwere submitted to precipitation with HB-GAM-Sepharose (15 hr,+4°C). After washing with PBS containing 0.3 M NaCl, N-syndecanand associated components were eluted from the precipitates withheparin (10 µg/ml) in the presence of 0.3 M NaCl or with 0.6 MNaCl.

N-syndecan was immunoblotted using affinity-purified polyclonal antibodies against the N-terminal or C-terminal peptide ofN-syndecan as described (Raulo et al., 1994). The C-terminal andN-terminal antibodies detected N-syndecan in a similar mannerin hippocampal fractions. The C-terminal antibody was producedin rabbits using a synthetic peptide corresponding to the full-lengthcytoplasmic moiety of rat N-syndecan as an immunogen. Productionof immunosera and affinity purification of the antibodies on peptide-Sepharosecolumn as well as immunoblotting of tyrosine kinases, HS, andcortactin were performed as described (Rauvala, 1989). Polyclonalanti-src (SRC-2), anti-pp60^c-src, anti-yes, and anti-fyn antibodies were from Santa Cruz Biotechnology(Santa Cruz, CA). Monoclonal anti-cortactin (p80/85) antibodywas from Upstate Biotechnology (Lake Placid, NY). Heparan sulfate-containingproteins were immunoblotted with antibodies against heparan sulfate10E4 epitope (Seikagaku Corporation) from hippocampal slices dissolvedin SDS-PAGE buffer (40 µl/slice). All Western blots were developedusing enhanced chemiluminescence (ECL; Amersham, Buckinghamshire,England), and quantified according to the optical density of theproteinbands.

  RESULTS

Heparitinase treatment prevents LTP in area CA1 of acute and cultured hippocampal slices

To investigate the role of HS-type carbohydrates in synaptic transmission and plasticity, hippocampal slices (300 µm) wereincubated for 3 hr with heparitinase (heparinase 3) or in similarconditions without the enzyme (control slices). This treatmentreduced the HS content of the slices ~50% (total area of histologicallydetected HS immunoreactivity was 54 ± 6% of control, and the opticaldensity of anti-HS-reactive bands in Western blots was 56 ± 8%of control). After heparitinase treatment, no LTP was observedafter a 100 Hz/1 sec HFS, whereas in control slices a long-lastingsynaptic potentiation was induced (Fig. 1A). Removal of HS didnot affect single stimulus-evoked (0.05 Hz) synaptic responsesat the Schaffer collateral-CA1 synapses (Fig. 1B). Also, the initialpost-tetanic potentiation 1-2 min after the HFS was not affectedby heparitinase (heparitinase 217 ± 20%, control 205 ± 18%), indicatingthat intact HS was needed for expression of early LTP, but notfor baseline synaptic transmission or induction of short-termpotentiation in the time scale <5 min.

View larger version (21K):
[in this window]
[in a new window]
Figure 1. Enzymatic cleavage of heparan sulfate prevents LTP but has no effect on single pulse-evoked synaptic responses in the area CA1 of hippocampal slices. A, Effect of HFS on the fEPSP slope in rat hippocampal slices (300 µm) preincubated with heparitinase-0.2% BSA (20 U/ml; volume, 500 µl; 3 hr; +24°C) ( $bullet$ ) or 0.2% BSA only ( $open circle$ ) (average ± SEM; n = 7 on both groups; p < 0.01; Student's t test). fEPSP traces before and 30 min after the HFS are shown superimposed on the right. B, Slopes of fEPSPs plotted as a function of presynaptic fiber volley (psfv) amplitude show the lack of effect of heparitinase on baseline synaptic responses. Data were obtained from five heparitinase-treated ( $bullet$ ) and five control ( $open circle$ ) slices (average ± SEM shown).

In acute slices, a rather high heparitinase concentration (20 U/ml) was needed for removal of HS and inhibition of LTP. Therefore,the experiment was repeated in hippocampal slice cultures (Stoppiniet al., 1991), which allowed a prolonged exposure (15 hr) to theenzyme. A similar inhibition of HFS-induced synaptic potentiationwas seen in slice cultures treated with a low concentration (1U/ml) of heparitinase (potentiation of the fEPSP slope 15 minafter the HFS 178 ± 16% in controls and 95 ± 15% in heparitinase-treatedcultures; n =4).

Sulfation pattern of heparin-type glycans has a critical effect on their capability to influence LTP

As an alternative approach to study the effect of HS on synaptic plasticity, soluble heparin-type glycans were added to theperfusion solution of hippocampal slices while recording synapticresponses in the area CA1. Purification of HS as well as the selectivedesulfation of the glycans was done as described previously (Maccaranaet al., 1993). Synaptic potentiation induced by HFS was markedlyinhibited in the presence of heparin at a low concentration (100ng/ml), but not by another polyanionic glycosaminoglycan, chondroitinsulfate (Fig. 2A). Heparin did not influence post-tetanic potentiationor baseline synaptic responses evoked by low-frequency stimulation(0.05 Hz) at the concentration used. Interestingly, selectively2-O- or 6-O-desulfated heparin did not influence LTP (Fig. 2B),indicating that the 2-O-sulfated iduronic acid units as well asglucosamine 6-O sulfate groups of heparin are essential for theinhibition of LTP.

View larger version (28K):
[in this window]
[in a new window]
Figure 2. Heparin prevents LTP in a manner dependent on the sulfation pattern of the glycan, but has no effect on pharmacologically isolated NMDA receptor-mediated responses. A, Effect of heparin (n = 8) and chondroitin sulfate (CS) (n = 7) on LTP. Both glycans were bath-applied at the concentration of 100 ng/ml as shown by the bar. Top traces show sample fEPSPs before (a) and after (b) application of the glycan, and 60 min after HFS (c). B, Pooled data showing the effect of selectively 2-O-desulfated (2-O-ds) and 6-O-desulfated (6-O-ds) heparins on LTP. Because the desulfated glycans were available in low amounts, these experiments were performed in static perfusion (volume, 1 ml). The values represent fEPSP slope (% from control ± SEM; n = 4) 30 min after the HFS (*p < 0.01; one-way ANOVA with Tukey post hoc comparison). C, Averaged amplitude of NMDA receptor-mediated responses recorded under current clamp from CA1 pyramidal neurones in the presence of 10 µM NBQX and 100 µM PiTX. Application of heparin (0.5 µg/ml) (shown by the bar) did not affect the amplitude of these responses (n = 3) at the resting membrane potential. The lack of effect of heparin on the voltage dependence of NMDA responses is shown in D.

Because induction of LTP in area CA1 is dependent on the activation of the NMDA receptors (Collingridge et al., 1983), wetested the possibility that heparin might have a direct influenceon the NMDA receptor activation. NMDA receptor-mediated responseswere recorded from CA1 pyramidal neurons with intracellular microelectrodesunder current clamp in the presence of 10 µM 6-nitro-7-sulfamoylbenzoquinoxaline(NBQX; Tocris Cookson) and 100 µM picrotoxin (Sigma). Heparinhad no apparent effect on pharmacologically isolated, NMDA receptor-mediatedresponses in terms of their voltage dependence or the responseamplitude at the resting membrane potential (Fig. 2C,D).

N-syndecan is isolated from hippocampus as a plasticity-associated heparan sulfate proteoglycan

Because the above data pointed to an important role of heparin-type glycans in LTP, we next pursued to identify the HS carrierproteins involved. We chose to use HB-GAM affinity chromatographyto purify plasticity-associated heparan sulfate proteoglycans(HSPGs) from crude extracts of adult rat hippocampi, because (1)a similar sulfation pattern of heparin is needed for both itsbinding to HB-GAM (Kinnunen et al., 1996) and for inhibition ofLTP, and (2) application of HB-GAM inhibits LTP in the area CA1(Lauri et al., 1998). In a salt gradient elution, two components(400 and 200 kDa) with a broad electrophoretic mobility were elutedfrom the HB-GAM affinity columns at a reasonably high (0.4-0.6M) NaCl concentration. After nitrous acid cleavage of the glycanside chains, the 200 kDa component was reduced to a 120 kDa bandand was identified by Western blotting as the core protein ofN-syndecan (syndecan-3) (Fig. 3A), a transmembrane HSPG enrichedin neuronal cells (Carey et al., 1992). Significantly, the carbohydratesof hippocampal N-syndecan were quantitatively cleaved by the sameenzyme (heparitinase) that was used to inhibit LTP (Fig. 3B).In contrast, the 400 kDa component did not contain HS but wasdigested by chondroitinase (data not shown).

View larger version (30K):
[in this window]
[in a new window]
Figure 3. N-syndecan is isolated as the major HB-GAM-binding HSPG from adult hippocampus. A, Adult rat hippocampi (10 gm wet tissue) were solubilized in octyl glucoside and fractionated by salt gradient elution on HB-GAM-Sepharose. Alcian blue-silver staining was used to detect both proteins and proteoglycans, and it revealed a proteoglycan-type smear in fractions eluting at 0.4-0.6 M NaCl (fractions 9-13). The figure shows a Western blot of fractions deglycosylated by nitrous acid. The immunoblot was stained with affinity-purified antibodies against N-syndecan. B, Western blot of the hippocampal fractions with anti-N-syndecan antibodies showing that heparitinase digestion reduces the 200 kDa proteoglycan (lane 1) to a 120 kDa core protein (lane 2).

To test directly whether N-syndecan actually influences synaptic plasticity, its effect on LTP was examined in a set of experimentsin which N-syndecan was applied into the hippocampal slice. N-syndecanwas purified from postnatal rat brain (Raulo et al., 1994) andpressure-injected into the CA1 dendritic area close to the recordingsite. An independent, noninjected pathway was recorded in thesame slice to control induction of LTP. Injection of N-syndecanblocked HFS-induced LTP without affecting post-tetanic potentiationor baseline synaptic responses (Fig. 4). A number of control injectionswith physiological saline did not influence LTP (Fig. 4). Giventhat soluble N-syndecan inhibits ligand binding to the endogenoustransmembrane proteoglycan at the concentration used (20 µg/ml)(Kinnunen et al., 1996), the above results suggest that N-syndecanis an essential part of the machinery supporting activity-evokedneuronal plasticity in the area CA1 of adult hippocampus.

View larger version (23K):
[in this window]
[in a new window]
Figure 4. Effect of soluble N-syndecan on LTP. After a stable baseline recording, N-syndecan (20 µg/ml) ( $bullet$ ) was pressure-injected into the CA1 dendritic area close to the recording site (arrow). Control injections were performed with saline ( $open circle$ ). LTP was induced by HFS 10 min after the injection. The data represents the average ± SEM of six experiments (p < 0.05; Student's t test). Sample responses before (a) and after (b) injection, and 30 min after high-frequency stimulation (c) are shown.

N-syndecan is expressed in the processes of CA1 pyramidal neurons in an activity-dependent manner

In situ hybridization with antisense-N-syndecan RNA probes in hippocampal cryosections showed that N-syndecan mRNA is expressedin all the pyramidal neurons of the hippocampus proper as wellas in the granule cells of the dentate gyrus (Fig. 5A). The senseprobe used as a control showed no reactivity (Fig. 5B). Immunostainingagainst N-syndecan showed that expression of the protein productwas strongest in the alveus, in the hilar region of the dentategyrus, and in the CA3 stratum radiatum. N-syndecan immunoreactivitywas localized to fiber-like structures (Fig. 5C), which were identifiedas nonmyelinated neuronal processes by immunoelectron microscopy(Fig. 5D).

View larger version (140K):
[in this window]
[in a new window]
Figure 5. Expression of N-syndecan in adult rat hippocampus. In situ hybridization with antisense (A) and sense (B) N-syndecan RNA probes in hippocampal sections. Light microscopic (C) and electron microscopic (D) visualization of N-syndecan immunoreactivity in CA3 stratum radiatum. In (D), the arrows point to anti-N-syndecan immunoperoxidase labeling at the surface of neuronal processes (7500× magnification). Parallel control stainings with nonimmune rabbit IgG showed no reactivity (data not shown).

Several molecules that are involved in activity-induced plasticity show changes in the level or pattern of expression as aconsequence of an LTP-inducing high-frequency stimulation (Armstrongand Montiminy, 1993; Silva and Giese, 1994; Ghosh and Greenberg,1995). Therefore, we tested the effect of LTP induction on expressionof N-syndecan in hippocampus. High-frequency stimulation (100Hz/1 sec) of Schaffer collaterals resulted in a long-lasting potentiationof the fEPSP slope in urethane-anesthetized rats (173 ± 7%; n= 3; Fig. 6A). Control rats received the same amount of stimuluspulses at low frequency (0.05 Hz). In situ hybridization as wellas the immunostain against N-syndecan was quantified from areasCA1, CA3, and dentate gyrus of 10 sections from control and 20sections from high-frequency-stimulated hippocampi. The quantifiedsections were from the same batch of color development reactions,thus comparable with each other. Sample sections of these stainingsare shown on Figure 6. Expression of N-syndecan mRNA was clearlyincreased in the stimulated area CA1 4 hr after induction of LTP(stain intensity 261 ± 19% from control; p < 0.01, Student's ttest) (Fig. 6B,C). N-syndecan mRNA expression was also slightlyincreased in the area CA3 and in the granule cells of dentategyrus (154 ± 19% and 159 ± 8%, respectively), suggesting thatneuronal activity in response to electrical stimulation is ratherwidely distributed in an intact hippocampus. At the protein level,immunoreactivity against N-syndecan was most clearly increasedin the CA1 stratum radiatum, where neuronal processes were stainedwith N-syndecan antibodies in stimulated animals, but hardly atall in nonstimulated animals (area of N-syndecan immunoreactivity220 ± 15% from control in area CA1, p < 0.01; 146 ± 16% in areaCA3, and 156 ± 22% in the hilus of dentate gyrus) (Fig. 6D,E).In addition to the immunostaining of neuronal fibers, N-syndecanimmunoreactivity was often found at the periphery of synapticterminals after induction of LTP (Fig. 6F). This might reflecta change in the localization of N-syndecan after an HFS. Alternatively,low levels of N-syndecan expressed in the synaptic structuresof control animals might not be detected by the antibodies. Asimilar induction of N-syndecan expression was also observed invitro in the area CA1 of hippocampal slices 2-4 hr after an LTP-inducingHFS (data not shown).

View larger version (114K):
[in this window]
[in a new window]
Figure 6. Changes in the expression of N-syndecan after LTP induction. In vivo recording showing the effect of 100 Hz/sec Schaffer collateral stimulation on the fEPSP slope. Sample fEPSPs before and 1 hr after the HFS are shown on the right (A). In situ hybridization with antisense N-syndecan probes in hippocampus of a control animal (B) and after induction of LTP (C). Note that these sections are not comparable to Figure 5 because of different duration of color development. Light microscopic pictures from the area CA1 showing a low level of N-syndecan immunoreactivity in control animals (D) and the enhanced staining of neuronal fibers after HFS (E). Electron microscopic micrograph showing N-syndecan immunostaining at the periphery of presynaptic and postsynaptic structures (arrows) in the CA1 dendritic area of a stimulated hippocampus (F) (15,000× magnification).

Hippocampal N-syndecan copurifies with fyn-kinase/cortactin in a manner that is increased by an LTP-inducing high-frequency stimulation

Recent biochemical and cell biological studies have shown that the cytosolic tail of N-syndecan binds to a tyrosine kinase-activeprotein complex containing pp60-src, fyn, and the F-actin-bindingsrc substrate cortactin (p80/85) (Kinnunen et al., 1998). Becausetyrosine kinase activity is required for synaptic plasticity (O'Dellet al., 1991; Abe and Saito, 1993; Boxall et al., 1996), the presenceof src family kinases and their substrates in the affinity-purifiedhippocampal fractions containing N-syndecan was investigated.A strong, herbimycin-sensitive kinase activity copurified withN-syndecan from hippocampus (data not shown). Immunoblotting ofthe N-syndecan-containing fractions from two different isolationsindicated the presence of an src family tyrosine kinase and cortactin(Fig. 7A). Unlike in the developing brain (c.f. Kinnunen et al.,1998), only fyn of the src-type kinases copurified with N-syndecanfrom adult hippocampus (Fig. 7B).

View larger version (18K):
[in this window]
[in a new window]
Figure 7. Hippocampal N-syndecan copurifies with cortactin and the tyrosine kinase fyn. A, Western blot of the HB-GAM affinity-purified hippocampal extracts showing copurification of N-syndecan, cortactin, and an src family kinase to fractions 9-13. The polyclonal antibody against src family (SRC-2) recognizes fyn, c-src, and yes-kinases. B, Immunoblotting of the fractions with monoclonal antibodies detects fyn but no other src family kinases in the N-syndecan containing hippocampal fractions.

Because of the rapid inhibition of LTP by soluble N-syndecan and heparin-type glycans, we presumed that fast alterations inthe interaction of N-syndecan with the intracellular componentsmight take place. To test this premise, N-syndecan and the componentsbinding to it were isolated from the area CA1 of hippocampal slices10 or 20 min after induction of LTP by HB-GAM-Sepharose precipitation(Fig. 8, legend). Interestingly, we found that association ofcortactin to N-syndecan was repeatedly increased within 10 min,and even more within 20 min after an LTP-inducing HFS in the areaCA1 (Fig. 8A,B). An increase was seen also in the associationbetween fyn and N-syndecan, however, this was significant only20 min after LTP induction (Fig. 8). The observed changes in theassociation of N-syndecan to cortactin/fyn are in agreement withthe hypothesis that endogenous N-syndecan is involved in the molecularmechanisms of LTP stabilization.

View larger version (16K):
[in this window]
[in a new window]
Figure 8. Association between N-syndecan and cortactin/fyn is increased by an LTP-inducing HFS. A, Western blot from HB-GAM-Sepharose-precipitated extracts from the area CA1 of hippocampal slices, which have been maintained under control conditions or in which LTP has been induced by HFS. N-syndecan and components associated to it were displaced from HB-GAM-Sepharose by heparin (10 µg/ml). The amount of cortactin was markedly increased after 20 min but already increased 10 min after HFS. An increase in the amount of N-syndecan-associated fyn was also detected. B, Quantification of N-syndecan, cortactin, and fyn from immunoblots of four independent experiments. N-syndecan was detected similarly in the samples from control and stimulated slices (*p < 0.05; Student's t test).

  DISCUSSION

Recent imaging studies have shown an amazingly high mobility of dendritic spines in neuronal cell culture (Fischer et al.,1998), suggesting that morphological rearrangements occurringat a temporal scale of a few minutes could contribute to the mechanismsunderlying the expression of LTP. Consistently, manipulation ofcell-matrix contacts, which can have a profound influence on cellularmorphology, affects already the early steps of LTP. The most rapideffect is caused by antibodies against adhesion molecules of theIg superfamily (NCAM and L1), which reduce already the post-tetanicpotentiation caused by the LTP-inducing high-frequency stimulation(Lüthi et al., 1994). Inhibition of cadherin family-mediatedcell adhesion considerably reduces LTP within 10 min, but doesnot affect the size of post-tetanic potentiation (Tang et al.,1998). Integrin-mediated processes seem to be involved in thelater steps of LTP stabilization, because, in contrast to NCAMand cadherins, block of integrin-mediated adhesion reduces LTPalso when applied after the LTP-inducing stimulus (Bahr et al.,1997; Stäubli et al., 1998).

The data presented here indicate that heparin-type glycans, a group of molecules involved in the modulation of cell-matrixassociation, have a critical role in activity-dependent synapticplasticity. Modulating interactions of endogenous components withheparan sulfates by enzymatic removal of HS or by addition ofsoluble heparin-type glycans inhibited LTP. These manipulationshad no effect on the baseline synaptic responses or on the immediatepost-tetanic potentiation after HFS, indicating that heparin-dependentinteractions are specifically needed for the stabilization oflong-termpotentiation.

HSs are thought to act by regulating the assembly of active signaling complexes at the cell surface by interacting with severalmolecules (e.g., NCAM, FGFs, and HB-GAM) (Fig. 9). In cell culture,soluble heparin inhibits the biological activity of HB-GAM (alreadyat a concentration of 0.1 µg/ml) (Kinnunen et al., 1996) as wellas adhesion mediated by NCAM (100 µg/ml) (Cole et al., 1986),while it enhances activation of FGF receptors in a manner thatis concentration-dependent (Rapraeger, 1993; Lindahl et al., 1994).The cellular effects of soluble heparin are profoundly affectedby its sulfation pattern (Maccarana et al., 1993; Kinnunen etal., 1996). In the present experiments, the requirements in thesulfation of heparin for inhibition of LTP were similar to thosereported previously for its binding to HB-GAM (Kinnunen et al.,1996). Although the structural requirements in heparin are somewhatdifferent for its binding to HB-GAM and basic fibroblast growthfactor (bFGF), these proteins can act as competitive ligands forHS (shown for N-syndecan, see Raulo et al., 1994). In hippocampus,application of HB-GAM and antibodies against NCAM inhibit LTP(Lüthi et al., 1994; Lauri et al., 1998), and FGF enhances LTP(Seifert et al., 1990; Ishiyama et al., 1991). Interestingly,NCAM antibodies affect post-tetanic potentiation, but FGF, HB-GAM,heparin, and N-syndecan do not. It appears that HSs can regulateLTP through multiple ligand interactions and that the cellularconsequences of an HFS might be critically dependent on the balancebetween different heparin-binding molecules available.

View larger version (30K):
[in this window]
[in a new window]
Figure 9. A schematic picture depicting interactions of N-syndecan with intracellular and extracellular molecules in the regulation of neuronal plasticity.

Heparan sulfate-containing extracellular proteins reported to be expressed in hippocampus include at least agrin (O'Connoret al., 1995) and syndecan-2 (Hsueh et al., 1998). Agrin is akey element inducing postsynaptic as well as presynaptic differentiationin the developing neuromuscular junction (Gautam et al., 1996;Kleiman and Reichardt, 1996). In the CNS, agrin expression isdevelopmentally regulated and enhanced by neuronal activity (O'Connoret al., 1995; Cohen et al., 1997), suggesting a role for agrinin the differentiation of central synapses. In a recent publicationby Hsueh et al. (1998), syndecan 2 was reported to be expressedin adult hippocampal neurons and to localize to synaptic structures.In the present study, however, N-syndecan (syndecan-3) was identifiedas a prominent heparan sulfate proteoglycan in hippocampus. Onanti-heparan sulfate immunoblots, a smear-like band comigratingwith N-syndecan was the major HS-containing component in adulthippocampal tissue (data not shown). Other bands of the sizesof ~400 and 80 kDa were also recognized, these might representagrin-type proteins and syndecan-2. Additional HS-containing proteinsmight be expressed in amounts too low to be detected by this method.Nevertheless, N-syndecan seems to represent the most prominentcell-surface HS carrier protein in adulthippocampus.

N-syndecan is a transmembrane HSPG, which binds bFGF (Chernousov and Carey, 1993) and has been proposed to regulate neuritegrowth and axonal guidance in the developing nervous system byacting as a receptor or co-receptor for HB-GAM (Raulo et al.,1994; Nolo et al., 1995; Kinnunen et al., 1996). In addition,N-syndecan can rapidly mediate localization of mRNA to cell processesin response to extracellular matrix contact in a manner that isdependent on tyrosine kinase activity (Fages et al., 1998). Althoughthe total amount of N-syndecan in adult brain is low (Carey etal., 1992; Nolo et al., 1995), we found that a high regional expressionof both N-syndecan mRNA and its protein product is maintainedin the adult hippocampus, and this expression is enhanced by anLTP inducing HFS. Furthermore, rat brain N-syndecan inhibitedLTP when applied in a soluble form to the CA1 dendritic area,consistently with the idea that N-syndecan is part of the machinerysupporting synaptic plasticity inhippocampus.

Approximately half of the apparent molecular mass of N-syndecan is comprised of heparan sulfates, which are exceptionallyheparin-like in their structure, especially because of their veryhigh proportion of both 2-0- and 6-0-sulfated monosaccharide residues(Kinnunen et al., 1996). The heparin-type glycan structure ofN-syndecan appears biologically important because both selective2-0-desulfation and 6-0-desulfation destroyed the ability of glycansto inhibit LTP. Brain N-syndecan is more heterogeneous in itscarbohydrate structure than heparin, for which reason a higherconcentration of soluble N-syndecan than heparin is required forspecific inhibition of HS-dependent cellular processes. Interestingly,the concentrations of N-syndecan and heparin that were found toinhibit LTP are quite similar to those inhibiting HB-GAM-inducedneurite outgrowth in forebrain neurons (Kinnunen et al., 1996).Furthermore, both the HB-GAM-induced neurite outgrowth (Rauvalaet al., 1994) and LTP are inhibited by the heparinase that hydrolyzesbrain N-syndecan. These findings are compatible with the viewthat N-syndecan interacts with HB-GAM/FGF-type ligands to regulateLTP.

In cultured brain neurons, N-syndecan-mediated neurite extension is dependent on the interaction of the cytosolic tail ofN-syndecan with src kinase/cortactin (Kinnunen et al., 1998).In adult hippocampus, N-syndecan was associated to cortactin andthe tyrosine kinase fyn. In addition, an ~100 kDa protein, detectedin Western blotting by a monoclonal antibody against the PDZ domain,coprecipitated with N-syndecan as well as cortactin from hippocampalextracts (S. Lauri, T. Kinnunen, and H. Rauvala, unpublished results).The molecular size of this protein matches that of a recentlyidentified syndecan-binding protein CASK/LIN-2 (Hsueh et al.,1998) that belongs to the PDZ domain-containing family of guanylatekinases that are thought to act as a scaffold at the membraneand coordinate localization of multiple proteins in the synapticstructures (Sheng, 1996; Craven and Bredt, 1998). The associationof cortactin/fyn to N-syndecan increased already 10 min afteran LTP-inducing stimulation, and, because shorter time periodswere not screened, it is possible that the association was enhancedeven faster. Determination of the causal relation between expressionof LTP and the post-tetanic increase in the size of the intracellularcomplex associating to N-syndecan warrants further studies. However,the change in the association as such suggests that N-syndecanmediates transmembrane signals between extracellular heparin-bindingmolecules and src-type kinases after induction of LTP. The involvementof src family kinases in synaptic plasticity is supported by therecent findings showing that src activity is increased by HFS,and activation of endogenous src causes synaptic potentiation(Lu et al., 1998). Furthermore, Grant et al. (1992) have reportedthat fyn $-$ / $-$ , but not c-src-deficient mice have a specific defectin hippocampal structure and loss ofLTP.

Tyrosine phosphorylation by src family kinases can directly influence the function of NMDA- and AMPA-type glutamate receptors(Yu et al., 1997; Lu et al., 1998). In addition, src-type kinasesare proposed to regulate cellular morphology by phosphorylatingcytoskeleton-associated components (Thomas et al., 1995; Lowelland Soriano, 1996). One of these src substrates is cortactin,which modulates cross-linking of filamentous actin in cell processesin a manner that is dependent on phosphorylation state of cortactin(Huang et al., 1997). Cortactin is also known to accumulate atdeveloping neuromuscular synapses (Peng et al., 1997). The activity-dependentcoupling between N-syndecan and cortactin suggests that N-syndecanparticipates in the mechanisms of cytoskeletal reorganizationon induction of LTP and provides evidence for a novel mechanismconnecting neuronal activity to the modulation of neuronal connectivity(Fig. 9).

A pathological overexpression of HSs has been observed in the brains of Alzheimer's patients. Biochemical studies have shownthat HS protects A $beta$ peptide from degradation by proteases (Gupta-Bansalet al., 1995). On the other hand, A $beta$ (1-40) inhibits the functionof heparanases (Bame et al., 1997), providing an explanation forthe accumulation of both HS and amyloid in the nervous systemof the Alzheimer's patients. Taken together, the present findingssuggest important implications for HSs in the neuronal dysfunctionobserved in Alzheimer'sdisease.

  FOOTNOTES

Received April 27, 1998; revised Sept. 21, 1998; accepted Dec. 1, 1998.

This work was supported by the Academy of Finland and the Sigrid Jusélius foundation. We thank Prof. Ulf Lindahl for theheparin-type glycans, and Seija Lehto and Kirsi Kenkkilä forexcellent technicalassistance.
Correspondence should be addressed to Heikki Rauvala, Laboratory of Molecular Neurobiology, P.O. Box 56 (Viikinkaari 5), FIN-00014University of Helsinki,Finland.

  REFERENCES

Top
Abstract
Introduction
References

Abe K, Saito H (1993) Tyrosine kinase inhibitors, herbimycin A and lavendustin A, block formation of long-term potentiation in the dentate gyrus in vivo. Brain Res 621:167-170[Web of Science][Medline].
Armstrong R, Montiminy M (1993) Transsynaptic control of gene expression. Annu Rev Neurosci 16:17-29[Web of Science][Medline].
Bahr BA, Staubli U, Xiao P, Chun D, Ji Z-X, Esteban ET, Lynch G (1997) Arg-Gly-Asp-Ser-selective adhesion and the stabilization of long-term potentiation. J Neurosci 17:1320-1329[Abstract/Free Full Text].
Bame KJ, Danda J, Hassall A, Tumova S (1997) A $beta$ (1-40) prevents heparanase-catalyzed degradation of heparan sulfate glycosaminoglycans and proteoglycans in vitro. J Biol Chem 272:17005-17011[Abstract/Free Full Text].
Bernfield M, Kokenyesi R, Kato M, Hinkes MT, Spring J, Gallo RL, Lose EJ (1992) Biology of the syndecans: a family of transmembrane heparan sulfate proteoglycans. Annu Rev Cell Biol 8:365-393[Web of Science].
Bliss TVP, Collingridge GL (1993) A synaptic model of memory: long-term potentiation in the hippocampus. Nature 361:31-39[Medline].
Boxall AR, Lancaster B, Garthwaite J (1996) Tyrosine kinase is required for long-term depression in the cerebellum. Neuron 16:805-813[Web of Science][Medline].
Carey DJ (1997) Syndecans: multifunctional cell-surface co-receptors. Biochem J 327:1-16.
Carey DJ, Evans D, Stahl R, Asundi V, Conner K, Garbes P, Cizmeci-Smith G (1992) Molecular cloning and characterization of N-syndecan, a novel transmembrane heparan sulfate proteoglycan. J Cell Biol 117:191-201[Abstract/Free Full Text].
Chang FL, Greenough WT (1984) Transient and enduring morphological correlates of synaptic activity and efficacy change in the rat hippocampal slice. Brain Res 309:35-46[Web of Science][Medline].
Chernousov MA, Carey DJ (1993) N-syndecan (syndecan 3) from neonatal rat brain binds basic fibroblast growth factor. J Biol Chem 268:16810-16814[Abstract/Free Full Text].
Cohen NA, Kaufmann WE, Worley PF, Rupp F (1997) Expression of agrin in the developing and adult rat brain. Neuroscience 76:581-596[Web of Science][Medline].
Cole GJ, Loewy A, Glaser L (1986) Neuronal cell-cell adhesion depends on interactions of NCAM with heparin-like molecules. Nature 320:445-447[Medline].
Collingridge GL, Kehl SJ, McLennan H (1983) Excitatory amino acids in synaptic transmission in the Schaffer collateral-commisural pathway of the rat hippocampus. J Physiol (Lond) 334:34-46.
Craven SE, Bredt DS (1998) PDZ Proteins organize synaptic signalling pathways. Cell 93:495-498[Web of Science][Medline].
Edwards FA (1995) LTP: a structural model to explain the inconsistencies. Trends Neurosci 18:250-255[Web of Science][Medline].
Fages C, Kaksonen M, Kinnunen T, Punnonen E-L, Rauvala H (1998) Regulation of mRNA localization by transmembrane signalling: local interaction of HB-GAM with the cell surface localizes $beta$ -actin mRNA. J Cell Sci 111:3073-3080[Abstract].
Fischer M, Kaech S, Knutti D, Matus A (1998) Rapid actin-based plasticity in dendritic spines. Neuron 20:847-854[Web of Science][Medline].
Gallagher JT (1989) The extended family of proteoglycans: social residents of the pericellular zone. Curr Opin Cell Biol 1:1201-1218[Medline].
Gautam M, Noakes PG, Moscoso L, Rupp F, Scheller RH, Merlie JP, Sanes JR (1996) Defective neuromuscular synaptogenesis in agrin-defective mutant mice. Cell 85:525-535[Web of Science][Medline].
Ghosh A, Greenberg ME (1995) Calcium signalling in neurons: molecular mechanisms and cellular consequences. Science 268:239-247[Abstract/Free Full Text].
Grant SGN, O'Dell TJ, Karl KA, Stein PL, Soriano P, Kandel E (1992) Impaired long-term potentiation, spatial learning and hippocampal development in fyn mutant mice. Science 258:1903-1910[Abstract/Free Full Text].
Gupta-Bansal R, Frederickson RCA, Brunden KR (1995) Proteoglycan mediated inhibition of A beta proteolysis. A potential cause of senile plaque accumulation. J Biol Chem 2709:18666-18671.
Huang C, Ni Y, Wang T, Gao Y, Haudenschild CC, Zhan X (1997) Down-regulation of filamentous actin cross-linking activity of cortactin by src-mediated tyrosine phosphorylation. J Biol Chem 272:13911-13915[Abstract/Free Full Text].
Hsueh Y-P, Yang F-U, Kharazia V, Naisbitt S, Cohen AR, Weinberg RJ, Sheng M (1998) Direct interaction of CASK/LIN-2 and Syndecan heparan sulfate proteoglycan and their overlapping distribution in neuronal synapses. J Cell Biol 142:139-151[Abstract/Free Full Text].
Ishiyama J, Saito H, Abe K (1991) Epidermal growth factor and basic fibroblast growth factor promote the generation of long-term potentiation in the dentate gyrus of anaesthetized rats. J Neurosci Res 12:403-411.
Kinnunen T, Kaksonen M, Saarinen J, Kalkkinen N, Peng HB, Rauvala H (1998) Cortactin/Src-kinase signalling pathway is involved in N-syndecan-dependent neurite outgrowth. J Biol Chem 273:10702-10709[Abstract/Free Full Text].
Kinnunen T, Raulo E, Nolo R, Maccarana M, Lindahl U, Rauvala H (1996) Neurite outgrowth in brain neurons induced by heparin-binding growth-associated molecule (HB-GAM) depends on the specific interaction of HB-GAM with heparan sulfate at the cell surface. J Biol Chem 271:2243-2248[Abstract/Free Full Text].
Kleiman RJ, Reichardt LF (1996) Testing the agrin hypothesis. Cell 85:461-464[Web of Science][Medline].
Lander AD (1993) Proteoglycans in the nervous system. Curr Opin Neurobiol 3:716-723[Medline].
Larkman AU, Jack J (1995) Synaptic plasticity: hippocampal LTP. Curr Opin Neurobiol 5:324-334[Web of Science][Medline].
Lauri SE, Taira T, Kaila K, Rauvala H (1996) Activity-induced enhancement of HB-GAM expression in rat hippocampal slices. NeuroReport 7:1670-1674[Web of Science][Medline].
Lauri SE, Rauvala H, Kaila K, Taira T (1998) Effect of heparin-binding growth-associated molecule (HB-GAM) on synaptic transmission and early LTP in rat hippocampal slices. Eur J Neurosci 10:188-194[Web of Science][Medline].
Lee K, Schotler F, Oliver M, Lynch G (1980) Brief bursts of high-frequency stimulation produce two types of structural change in rat hippocampus. J Neurophysiol 44:247-258[Free Full Text].
Lindahl U, Lindholt K, Spillmann D, Kjellén L (1994) More to heparin than anticoagulation. Thrombosis Res 75:1-32[Web of Science][Medline].
Lowell CA, Soriano P (1996) Knockouts of Src-family kinases: stiff bones, wimpy T cells and bad memories. Genes Dev 10:1845-1857[Free Full Text].
Lu YM, Roder JC, Davidow J, Salter MW (1998) Src activation in the induction of long-term potentiation in CA1 hippocampal neurons. Science 279:1363-1367[Abstract/Free Full Text].
Lüthi A, Laurent J-P, Figurov A, Müller D, Schachner M (1994) Hippocampal long-term potentiation and neural cell adhesion molecules L1 and NCAM. Nature 372:777-779[Medline].
Maccarana M, Casu B, Lindahl U (1993) Minimal sequence in heparin/heparan sulfate required for binding of basic fibroblast growth factor. J Biol Chem 268:23898-23905[Abstract/Free Full Text].
Margolis RK, Rauch U, Maurel P, Margolis RU (1996) Neurocan and phosphacan: two major nervous tissue-specific chondroitin-sulfate proteoglycans. Perspect Dev Neurobiol 3:273-290[Web of Science][Medline].
Möller HJ, Heinegård D, Poulsen JH (1993) Combined Alcian blue and silver staining of subnanogram quantities of proteoglycans and glycosaminoglycans in sodium dodecyl sulfate -polyacrylamide gels. Anal Biochem 209:169-175[Web of Science][Medline].
Nicoll RA, Malenka RC (1995) Contrasting properties of two forms of long-term potentiation in the hippocampus. Nature 377:115-118[Medline].
Nolo R, Kaksonen M, Raulo E, Rauvala H (1995) Co-expression of heparin-binding growth-associated molecule (HB-GAM) and N-syndecan (Syndecan-3) in developing rat brain Neurosci Lett 191:39-42.
Nurcombe V, Ford MD, Wildschut JA, Bartlett PF (1993) Developmental regulation of neural response to FGF-1 and FGF-2 by heparan sulfate proteoglycan. Science 260:103-106[Abstract/Free Full Text].
O'Connor LT, Lauterborn JC, Smith MA, Gall CM (1995) Expression of agrin is altered following seizures in adult rat brain. Mol Brain Res 33:277-287[Medline].
O'Dell TJ, Kandel ER, Grant SGN (1991) Long-term potentiation in the hippocampus is blocked by tyrosine kinase inhibitors. Nature 353:558-560[Medline].
Peng HB, Xie H, Dai Z (1997) Association of cortactin with developing neuromuscular specializations. J Neurocytol 26:637-650[Web of Science][Medline].
Rapraeger AC (1993) The coordinated regulation of heparan sulfate, syndecans and cell behavior. Curr Opin Cell Biol 5:844-853[Medline].
Raulo E, Chernousov MA, Carey DJ, Nolo R, Rauvala H (1994) Isolation of a neuronal cell surface receptor of heparin binding growth-associated molecule (HB-GAM): identification as N-syndecan (syndecan-3). J Biol Chem 269:12999-13004[Abstract/Free Full Text].
Rauvala H (1989) An 18-kd heparin-binding protein of developing brain that is distinct from fibroblast growth factors. EMBO J 8:2933-2941[Web of Science][Medline].
Rauvala H, Peng HB (1997) HB-GAM and heparin-type glycans in the development and plasticity of neuron-target contacts. Prog Neurobiol 52:127-144[Web of Science][Medline].
Rauvala H, Vanhala A, Castren E, Nolo R, Raulo E, Merenmies J, Panula P (1994) Expression of HB-GAM (heparin-binding growth-associated molecule) in the pathways of developing axonal processes in vivo and neurite outgrowth in vitro induced by HB-GAM. Dev Brain Res 79:157-176[Medline].
Ronn LC, Bock E, Linnemann D, Jahnsen H (1995) NCAM-antibodies modulate induction of long-term potentiation in rat hippocampal CA1. Brain Res 677:145-151[Web of Science][Medline].
Seifert W, Föster F, Flott B, Terlau H (1990) Effects of a neurotrophic factor (FGF) on development, regeneration and synaptic plasticity of central neurons. Adv Exp Med Biol 268:395-399[Medline].
Sheng M (1996) PDZs and receptor channel clustering: rounding up the latest suspects. Neuron 17:575-578[Web of Science][Medline].
Silva A, Giese K (1994) Plastic genes are in! Curr Opin Neurobiol 4:413-420[Medline].
Smart TG (1997) Regulation of excitatory and inhibitory neurotransmitter-gated ion channels by protein phosphorylation. Curr Opin Neurobiol 7:358-367[Web of Science][Medline].
Snow AD, Mar H, Nochlin D, Kimata K, Kato M, Suzuki S, Hassell J, Wright TN (1988) The presence of heparan sulfate proteoglycans in the neuritic plaques and congophilic angiopathy in Alzheimer's disease. Am J Pathol 133:456-463[Abstract].
Snow AD, Sekiguchi R, Nochlin D, Fraser P, Kimata K, Mizutani A, Arai M, Schreier WA, Morgan DG (1994) An important role of heparan sulfate proteoglycan (perlecan) in a model system for the deposition and persistence of fibrillar A $beta$ -amyloid in rat brain. Neuron 12:219-234[Web of Science][Medline].
Sorra KE, Harris KM (1998) Stability in synapse number and size at 2 hr after long-term potentiation in hippocampal area CA1. J Neurosci 18:658-671[Abstract/Free Full Text].
Stäubli U, Chun D, Lynch G (1998) Time-dependent reversal of long-term potentiation by an integrin antagonist. J Neurosci 18:3460-3469[Abstract/Free Full Text].
Stoppini L, Buchs P-A, Muller D (1991) A simple method for organotypic cultures of nervous tissue. J Neurosci Methods 37:173-182[Web of Science][Medline].
Tang L, Hung CP, Schumann EM (1998) A role for the cadherin family of cell adhesion molecules in hippocampal long-term potentiation. Neuron 20:1165-1175[Web of Science][Medline].
Thomas SM, Soriano P, Imamoto A (1995) Specific and redundant roles of Src and Fyn in organizing the cytoskeleton. Nature 376:267-271[Medline].
Walaas ST, Greengard P (1991) Protein phosphorylation and neuronal function. Pharmacol Rev 43:299-349[Abstract].
Wisniewski T, Lalowski M, Baumann M, Rauvala H, Raulo E, Nolo R, Frangione B (1996) HB-GAM is a cytokine present in Alzheimer's and Down's syndrome lesions. NeuroReport 7:667-671[Web of Science][Medline].
Yu X-M, Askalan R, Keil GJ, Salter MW (1997) NMDA channel regulation by channel associated protein tyrosine kinase src. Science 275:674-678[Abstract/Free Full Text].

Copyright © 1999 Society for Neuroscience 0270-6474/99/1941226-10$05.00/0

This article has been cited by other articles:

A. L. Lucido, F. Suarez Sanchez, P. Thostrup, A. V. Kwiatkowski, S. Leal-Ortiz, G. Gopalakrishnan, D. Liazoghli, W. Belkaid, R. B. Lennox, P. Grutter, et al.
Rapid Assembly of Functional Presynaptic Boutons Triggered by Adhesive Contacts
J. Neurosci., October 7, 2009; 29(40): 12449 - 12466.
[Abstract] [Full Text] [PDF]

A. Hienola, S. Tumova, E. Kulesskiy, and H. Rauvala
N-syndecan deficiency impairs neural migration in brain
J. Cell Biol., August 14, 2006; 174(4): 569 - 580.
[Abstract] [Full Text] [PDF]

E. Raulo, S. Tumova, I. Pavlov, M. Pekkanen, A. Hienola, E. Klankki, N. Kalkkinen, T. Taira, I. Kilpelainen, and H. Rauvala
The Two Thrombospondin Type I Repeat Domains of the Heparin-binding Growth-associated Molecule Bind to Heparin/Heparan Sulfate and Regulate Neurite Extension and Plasticity in Hippocampal Neurons
J. Biol. Chem., December 16, 2005; 280(50): 41576 - 41583.
[Abstract] [Full Text] [PDF]

A. Dityatev, G. Dityateva, V. Sytnyk, M. Delling, N. Toni, I. Nikonenko, D. Muller, and M. Schachner
Polysialylated Neural Cell Adhesion Molecule Promotes Remodeling and Formation of Hippocampal Synapses
J. Neurosci., October 20, 2004; 24(42): 9372 - 9382.
[Abstract] [Full Text] [PDF]

J. Chin, J. J. Palop, G.-Q. Yu, N. Kojima, E. Masliah, and L. Mucke
Fyn Kinase Modulates Synaptotoxicity, But Not Aberrant Sprouting, in Human Amyloid Precursor Protein Transgenic Mice
J. Neurosci., May 12, 2004; 24(19): 4692 - 4697.
[Abstract] [Full Text] [PDF]

T. M. Reeves, M. L. Prins, J. Zhu, J. T. Povlishock, and L. L. Phillips
Matrix Metalloproteinase Inhibition Alters Functional and Structural Correlates of Deafferentation-Induced Sprouting in the Dentate Gyrus
J. Neurosci., November 12, 2003; 23(32): 10182 - 10189.
[Abstract] [Full Text] [PDF]

M. GOTTE
Syndecans in inflammation
FASEB J, April 1, 2003; 17(6): 575 - 591.
[Abstract] [Full Text] [PDF]

M. Inatani, M. Honjo, A. Oohira, N. Kido, Y. Otori, Y. Tano, Y. Honda, and H. Tanihara
Spatiotemporal Expression Patterns of N-Syndecan, a Transmembrane Heparan Sulfate Proteoglycan, in Developing Retina
Invest. Ophthalmol. Vis. Sci., May 1, 2002; 43(5): 1616 - 1621.
[Abstract] [Full Text] [PDF]

C. E. Bandtlow and D. R. Zimmermann
Proteoglycans in the Developing Brain: New Conceptual Insights for Old Proteins
Physiol Rev, October 1, 2000; 80(4): 1267 - 1290.
[Abstract] [Full Text] [PDF]

N. Rouach, J. Glowinski, and C. Giaume
Activity-Dependent Neuronal Control of Gap-Junctional Communication in Astrocytes
J. Cell Biol., June 26, 2000; 149(7): 1513 - 1526.
[Abstract] [Full Text] [PDF]

I. Kilpelainen, M. Kaksonen, T. Kinnunen, H. Avikainen, M. Fath, R. J. Linhardt, E. Raulo, and H. Rauvala
Heparin-binding Growth-associated Molecule Contains Two Heparin-binding beta -Sheet Domains That Are Homologous to the Thrombospondin Type I Repeat
J. Biol. Chem., May 5, 2000; 275(18): 13564 - 13570.
[Abstract] [Full Text] [PDF]

Y. Nakagami, K. Abe, N. Nishiyama, and N. Matsuki
Laminin Degradation by Plasmin Regulates Long-Term Potentiation
J. Neurosci., March 1, 2000; 20(5): 2003 - 2010.
[Abstract] [Full Text] [PDF]

Y.-P. Hsueh and M. Sheng
Regulated Expression and Subcellular Localization of Syndecan Heparan Sulfate Proteoglycans and the Syndecan-Binding Protein CASK/LIN-2 during Rat Brain Development
J. Neurosci., September 1, 1999; 19(17): 7415 - 7425.
[Abstract] [Full Text] [PDF]

K. Kato, T. Kishi, T. Kamachi, M. Akisada, T. Oka, R. Midorikawa, K. Takio, N. Dohmae, P. I. Bird, J. Sun, et al.
Serine Proteinase Inhibitor 3 and Murinoglobulin I Are Potent Inhibitors of Neuropsin in Adult Mouse Brain
J. Biol. Chem., April 27, 2001; 276(18): 14562 - 14571.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (55)

Citing Articles via Google Scholar

Google Scholar

Articles by Lauri, S. E.

Articles by Rauvala, H.

Search for Related Content

PubMed

PubMed Citation

Articles by Lauri, S. E.

Articles by Rauvala, H.