Neurocan Is Upregulated in Injured Brain and in Cytokine-Treated Astrocytes

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The Journal of Neuroscience, April 1, 2000, 20(7):2427-2438

Neurocan Is Upregulated in Injured Brain and in Cytokine-Treated Astrocytes
Richard A. Asher¹, Daniel A. Morgenstern¹^,², Penny S. Fidler¹^,², Kathryn H. Adcock¹^,², Atsuhiko Oohira³, Janet E. Braistead⁶, Joel M. Levine⁴, Richard U. Margolis⁵, John H. Rogers¹, and James W. Fawcett¹^,²
¹ Physiological Laboratory, University of Cambridge, Cambridge CB2 3EG, United Kingdom, ² Centre for Brain Repair, University of Cambridge, Forvie Site, Cambridge CB2 2PY, United Kingdom, ³ Department of Perinatology, Institute for Developmental Research, Kasugai, Aichi 480-03, Japan, ⁴ Department of Neurobiology and Behavior, State University of New York, Stony Brook, New York 11794, ⁵ Department of Pharmacology, New York University Medical Center, New York, New York 10016, and ⁶ Molecular Neurobiology Laboratory, Salk Institute for Biological Studies, La Jolla, California 92138

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Injury to the CNS results in the formation of the glial scar, a primarily astrocytic structure that represents an obstacleto regrowing axons. Chondroitin sulfate proteoglycans (CSPG) aregreatly upregulated in the glial scar, and a large body of evidencesuggests that these molecules are inhibitory to axon regeneration.We show that the CSPG neurocan, which is expressed in the CNS,exerts a repulsive effect on growing cerebellar axons. Expressionof neurocan was examined in the normal and damaged CNS. Frozensections labeled with anti-neurocan monoclonal antibodies 7 dafter a unilateral knife lesion to the cerebral cortex revealedan upregulation of neurocan around the lesion. Western blot analysisof extracts prepared from injured and uninjured tissue also revealedsubstantially more neurocan in the injured CNS. Western blot analysisrevealed neurocan and the processed forms neurocan-C and neurocan-130to be present in the conditioned medium of highly purified ratastrocytes. The amount detected was increased by transforminggrowth factor $beta$ and to a greater extent by epidermal growth factorand was decreased by platelet-derived growth factor and, to alesser extent, by interferon $gamma$ . O-2A lineage cells were also capableof synthesizing and processing neurocan. Immunocytochemistry revealedneurocan to be deposited on the substrate around and under astrocytesbut not on the cells. Astrocytes therefore lack the means to retainneurocan at the cell surface. These findings raise the possibilitythat neurocan interferes with axonal regeneration after CNSinjury.

Key words: chondroitin sulfate; EGF; extracellular matrix; glial scar; proteoglycan; regeneration; TGF $beta$

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The inability of neurons to regenerate within the adult mammalian CNS is a result of the innately poor regenerative abilityof many CNS neurons and the inhibitory nature of the adult mammalianCNS. This inhibition is attributable to molecules associated withCNS myelin and those associated with the glial scar, a structurethat in its mature form contains mostly astrocytes and can constitutean impediment to regrowing axons (for review, see Fawcett andAsher, 1999).

Various in vitro experiments have shown that astrocytes can inhibit axon growth. Astrocytes cultured as a three-dimensionaltissue, astrocytes from injured adult rat optic nerve and injuredcerebral cortex, and astrocytes removed from the injured adultCNS attached to nitrocellulose filter material were all nonpermissivefor the growth of various axonal types (Smith et al., 1986; Fawcettet al., 1989, Bähr et al., 1995, Le Roux and Reh, 1996). Variouslines of evidence suggest that inhibition by astrocytes is attributableat least in part to chondroitin sulfate proteoglycans (CSPGs).Comparison between permissive and inhibitory astrocyte cell linesshowed that inhibitory cells produced inhibitory CSPGs, the activityof which could be reduced by chondroitinase, xylosides, and chlorate,all of which affect the glycosaminoglycan (GAG) component of proteoglycans.Three-dimensional astrocyte cultures were also rendered more permissiveby chlorate (Smith-Thomas et al., 1994, 1995), and axon growthon reactive astrocytes removed from the adult CNS on filter materialwas increased by treatment with chondroitinase (McKeon et al.,1991, 1995).

CSPGs are implicated in the inhibition of axon regeneration in the injured CNS in vivo. There is substantial upregulationof CSPG production in the glial scar after CNS injury, as revealedby antibodies that bind to the chondroitin sulfate GAG chains(McKeon et al., 1991; Laywell et al., 1992; Frisen et al., 1995;McKeon et al., 1995; Barker et al., 1996; Gates et al., 1996).Experiments in which sensory neurons were implanted into adultwhite matter tract showed substantial regeneration, but growthstopped at CSPG-rich sites of injury (Davies et al., 1997, 1999).Treatment of an axotomy injury with chondroitinase allowed regenerationof CNS axons (Moon et al., 1999). Axon growth on cryosectionsof normal and injured spinal cord was improved by pretreatmentof the sections with chondroitinase (Zuo et al., 1998). A proteoglycanpreparation from injured brain also had outgrowth-inhibitory effects,which were relieved with chondroitinase (Bovolenta et al., 1993).

One effect of the inhibitory CSPGs is interference with the neuronal growth-promoting effects of laminin (McKeon et al., 1991,1995). Pretreatment of explanted glial scar astrocytes with chondroitinaseled to an increase in neurite outgrowth, which was inhibited bylaminin function-blocking antibodies (McKeon et al., 1991, 1995).The increased growth on chondroitinase-treated cryosections describedabove was largely inhibited by laminin-blocking antibodies (Zuoet al., 1998), and inhibitory CSPGs produced by inhibitory astrocytecell lines and astrocytes were able to block the axon growth-promotingeffects of laminin (Smith-Thomas et al., 1994, 1995; Fidler etal., 1999).

In the present study we have examined the expression of neurocan, a CSPG with well documented axon growth-inhibitory propertiesin CNS injuries, in various glial cell types, and have determinedthe effects of injury-related cytokines on itsproduction.

Some of these data have been published previously in abstract form (Asher et al., 1998).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Surgical procedures
Adult female Sprague Dawley rats (Charles River, Margate, UK; approximate body weight, 200 gm) were anesthetized under halothane,and the head was held in a stereotaxic apparatus with the incisorbar 2.5 mm below the interaural line. A fine scalpel blade wasinserted stereotaxically and vertically into the brain, througha parasagittal dorsal craniotomy, to a depth of 3 mm below thedura and 2-3 mm lateral to the midline. The knife was then movedin the horizontal plane to produce a lesion 5-6 mm in length,midway between lambda and bregma. The operation was performedunilaterally (on the right-hand side) with the other hemisphereserving as a control. After 7-8 d, the animals were terminallyanesthetized with an intraperitoneal injection of sodium pentabarbitoneand decapitated. The brain was rapidly removed and immediatelyfrozen on dry ice and stored at $-$ 70°C or prepared for frozen sectioning.All procedures were conducted in compliance with the UK Animals(Scientific Procedures) Act1986.

Immunolabeling of frozen sections
Frozen, coronal sections (10 µm) were cut from unfixed tissue 7 d after lesion. Labeling was performed without fixation. Nonspecificbinding was blocked with PBS containing 3% BSA and 20 mM L-lysine(PBS/BSA/Lys). The sections were incubated with the 1G2 anti-neurocanmonoclonal antibody (mAb) (supernatant diluted 1:2) (Oohira etal., 1994), the 1F6 anti-neurocan mAb [supernatant diluted 1:2;Developmental Studies Hybridoma Bank (DSHB), Iowa City, IA] (Meyer-Puttlitzet al., 1995), or mouse IgG₁ (10 µg/ml in PBS/BSA/Lys) for 1 hr.Bound antibodies were visualized with biotinylated anti-mouseimmunoglobulins (1:100; Amersham, Little Chalfont, Bucks, UK)and Cy3-streptavidin (1.0 µg/ml; Jackson, West Grove, PA) in themanner described previously (Asher et al., 1995).

Sample preparation for SDS-PAGE
Brain tissue. Dissection was performed as rapidly as possible while the brain was unfreezing. A piece of tissue ~2 × 4 × 6mm containing the lesion was excised. A similar-sized piece wasdissected from the same location on the contralateral cortex.The tissue was immediately placed in 1.0 ml ice-cold extractionbuffer (0.05 M Tris-HCl, 0.15 M NaCl, pH 7.0) containing proteaseinhibitor cocktail (25× in 0.1 M phosphate buffer, pH 7.0; Roche,Lewes, East Sussex, UK) and homogenized in a Teflon-glass Douncehomogenizer. The homogenate was centrifuged at 13,000 × g for10 min at 4°C. Two additional extracts were made from the resultantpellet in the same way. The pellet was then rehomogenized in extractionbuffer containing, additionally, 1% Triton X-100 (Fluka, Gillingham,Dorset, UK) and incubated in an end-over-end shaker at 4°C for1 hr. Another detergent extract was then made from the resultantpellet in the same manner. Thus, the tissue was extracted threetimes with saline and then twice with detergent. The protein contentwas determined according to the method of Bradford (1976) usingthe Coomassie Plus Protein Assay Reagent (Pierce, Chester, Cheshire,UK) and BSA to generate the standard curve. One-half of each samplewas treated with 0.02 U chondroitinase ABC (protease-free, Roche)for 3 hr at 37°C.
Cultured cells. Conditioned medium was removed from the cells (astrocytes, O-2A progenitor cells, macrophages, or meningealcells) and added to a tube containing protease inhibitor cocktail.The conditioned medium was then centrifuged at 1000 × g for 10min at 4°C and concentrated in a Centricon 100 (Millipore, Watford,Herts, UK) to one-tenth of its initial volume. The protein contentof the extracts was determined in the manner described above.Chondroitinase ABC digestion was performed for 3 hr at 37°C using0.01 U of enzyme per milliliter of unconcentrated conditionedmedium.

Electrophoresis and Western blotting
SDS-PAGE was performed in 4 or 5% polyacrylamide gels with a 3% stacking gel under nonreducing conditions. Proteins were transferredto nitrocellulose (Hybond-C pure, Amersham) at 4°C for 15-18 hr,at a constant current of 150mA.
All subsequent procedures were performed at room temperature. The blots were rinsed twice in Tris-buffered saline (TBS, 0.9%NaCl, 10 mM Tris-HCl, pH 7.5) containing 0.05% Tween 20 (TBS/Tween)and incubated for an additional 40 min in TBS/Tween. All washesand antibody incubations were performed in TBS/Tween. The blotswere then incubated with one of the following antibodies: the1G2 anti-neurocan mAb (supernatant diluted 1:20-1:40), the 1F6anti-neurocan mAb (supernatant diluted 1:20-1:40), the rabbitanti-neurocan-N-terminal fragment pAb 291 (1:1000) (Matsui etal., 1994), the anti-versican mAb 12C5 (supernatant diluted 1:20)(Asher et al., 1991), a mouse myeloma-derived IgG₁ (1.1 µg/ml;Sigma, Poole, Dorset, UK), or rabbit immunoglobulins (1.0 µg/ml;Dako, High Wycombe, Bucks, UK) for 2 hr. For labeling with rabbitantibodies, blocking and dilution of the primary antibody wasperformed in TBS/Tween containing 5% dried milk powder and 20mM L-lysine. Reactive species were visualized with either peroxidase-conjugatedanti-mouse or anti-rabbit IgG (Vector, Peterborough, Cambs, UK)and a chemiluminescent substrate (National Diagnostics, Hull,Humberside, UK). The amount of protein in a given band was estimatedby densitometry using a Quantimet 500instrument.

Glial cell culture
All cell culture reagents were purchased from Life Technologies (Paisley, UK), unless stated otherwise. Glial cell cultureswere prepared from the brains of newborn rats <3 d old. The cerebralcortices of six to eight rats were freed of meninges and collectedin HBSS. The tissue was then transferred to DMEM (with 4.5 g/lD-glucose, Glutamax I, and sodium pyruvate) containing 10% fetalcalf serum (FCS), 100 U/ml penicillin, 100 µg/ml streptomycin,50 µg/ml gentamicin, and 2.5 µg/ml amphotericin B (Fungizone),and dissociated by passage through needles of decreasing size(19, 21, 23, and 25 ga). The suspension was filtered (withoutforce) through 70 µm nylon mesh (BioDesign, Carmel, NY) and dispensedinto four or five 75 cm² poly-D-lysine-coated tissue culture flasks. Ninety percent ofthe medium was replaced the next day with fresh medium lackingthe antibiotics and anti-mycotic, and the cells were subsequentlyfed every thirdday.
Between the 8th and 12th days, the cultures were shaken to remove the macrophages and progenitor cells that sit on top ofthe (astroglial) monolayer. The adherent cells were passaged (withthe use of 0.25% trypsin, 1 mM EDTA) into 25 cm² poly-D-lysine-coated flasks at a split ratio of 1:1 and maintainedin serum-containing medium. Two days after a confluent monolayerhad been reestablished, the serum-containing medium was replacedwith serum-free DMEM containing 6.25 µg/ml insulin, 6.25 µg/mltransferrin, 6.25 ng/ml selenious acid, 1.25 mg/ml bovine serumalbumin, 5.35 µg/ml linoleic acid (as ITS+; Collaborative BiomedicalProducts, Bedford, MA), 6.3 ng/ml progesterone (Sigma), 16 µg/mlputrescine (Sigma), 50 µg/ml L-ascorbic acid (Sigma), and 16 µMcytosine arabinoside (Ara-C, Fluka). The cells were maintainedfor two periods of 4 d in this medium, at the end of which theywere invariably free of any contaminating progenitor cells. Occasionally,microglial-like cells were visible, and these were eliminatedby treatment with 10 mM L-leucine methyl ester (Sigma) for 30min (Giulian and Baker, 1986). The cells were grown for an additional2-3 d in the same medium lacking Ara-C.
For the preparation of astrocyte-conditioned medium, each flask was washed once with DMEM, and 2.5 ml of serum-free DMEM containingthe cytokine or growth factor under investigation was added for2-8 d. Information pertaining to the source and concentrationof the cytokines and growth factors is presented in Table 1.To investigate neurocan processing, astrocytes were maintainedfor 4 d in serum-free DMEM containing one of the following proteaseinhibitors: anti-thrombin III (0.1 U/ml), aprotinin (1.0 µg/ml),tissue inhibitor of metalloproteinase-2 (TIMP-2, 0.2 µg/ml), leupeptin(1.0 µg/ml), E-64 (1.0 µg/ml; Calbiochem, Nottingham, Notts, UK),cathepsin B inhibitor II (1.0 µg/ml; Calbiochem), or $alpha$ ₂-macroglobulin(10 µg/ml). Unless stated otherwise, inhibitors were purchasedfrom Roche and added fresh eachday.
Cultures enriched for O-2A progenitor cells were derived from the cells dislodged during the shaking of the primary culture.The cell suspension was filtered through 35 and 15 µm nylon meshand then preplated on uncoated tissue culture plastic to depleteit of macrophages and astrocytes. The nonattached cells from one75 cm² flask were dispensed into one poly-D-lysine-coated 25 cm² flask in DMEM containing 10% FCS. The cells were allowed to adherefor 2-3 hr, and the medium was changed to serum-free DMEM containingITS+, 10 ng/ml fibroblast growth factor 2 (FGF2; Roche), and 10ng/ml platelet-derived growth factor (PDGF-AB; R & D, Abingdon,Oxon, UK). This was collected after 2 d and replaced with thesame medium, or with the same medium lacking the growthfactors.
Cultures of meningeal cells were established from the meninges of four to six newborn rat brains by enzymatic dissociationwith 0.2% collagenase and 0.1% trypsin. These cells were grownto confluence in DMEM/10% FCS. For the preparation of conditionedmedium, the cells were grown for 4 d in DMEM containing 1% FCSand ITS+.

Stripe assays
Neurocan, phosphacan, NG2, and L1 were purified as described previously (Rauch et al., 1991; Dou and Levine 1994). The stripeassay was carried out as described by Baier and Klostermann (1994),with minor modifications. Acid-washed glass coverslips were coatedwith poly-L-lysine (100 µg/ml in water) overnight, washed, andthen coated again with immunoaffinity-purified L1 (2 µg/ml, 2-3hr, 37°C). The coverslips were washed in PBS and air-dried, andnarrow stripes of the test proteins (10 µg/ml) were applied usinga silicon matrix. After 1 hr at 37°C, the coverslips were removedfrom the matrices, washed in complete medium (DMEM, 10% FCS),and stored in complete medium until ready foruse.
Explants of postnatal day (P) 4-5 rat cerebellum or P0 cortex were placed on top of the coverslips and grown for 48 hr incomplete medium. For the cerebellar explants, the medium was supplementedwith 20 mM KCl. Patterns of neurite outgrowth were visualizedwith either phase-contrast or fluorescence optics after stainingthe living cultures with carboxy-methyl fluorescein (MolecularProbes, Eugene, OR). In some cases, trace amounts of fluorescein-conjugateddextran (Molecular Probes) were added to the stripe-making solutionto aid in the visualization of thestripes.

Immunocytochemistry
Astrocytes and O-2A progenitor cells were grown on poly-D-lysine-coated glass coverslips. Neurocan labeling was performedat room temperature on living cells in Liebovitz's L-15 medium(Life Technologies) containing 2% FCS (L-15/FCS). The cells werewashed once in L-15/FCS and incubated with the 1G2 anti-neurocanmAb (supernatant diluted 1:2), the 1F6 anti-neurocan mAb (supernatantdiluted 1:2), the 1D1 anti-neurocan mAb (ascites diluted 1:100;DSHB), or the rabbit anti-neurocan-N-terminal fragment polyclonalantibody (pAb) 291 (1:1000) for 20 min. The cells were washedthree times with L-15/FCS and then incubated with biotinylatedanti-mouse immunoglobulins or biotinylated anti-rabbit immunoglobulins(1:100; Amersham) for 20 min. The cells were washed as beforeand incubated with Cy3-streptavidin (1 µg/ml) for 20 min. Finally,the cells were washed three times in L-15/FCS and once in PBSand fixed in cold ( $-$ 20°C) methanol for 2 min. Glial fibrillaryacidic protein (GFAP) labeling was performed on methanol-fixedcells with rabbit anti-GFAP (20 µg/ml, Dako) and FITC anti-rabbitIgG (7.5 µg/ml, Jackson). Labeling with the A2B5 (an O-2A cellmarker; American Type Culture Collection, Manassas, VA) and 5A5(anti-polysialylated N-CAM, DSHB) mAbs was also performed on livingcells, in the manner described above. Nuclei were labeled withHoechst No. 33342 (Sigma) for 30 min. Sterile testicular hyaluronidase(type IV, Sigma) was added directly to astrocytes growing on glasscoverslips in serum-free medium to a final concentration of 20or 100 µg/ml, and incubation continued for 3 hr at 37°C in a CO₂-containingatmosphere.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurocan inhibits neurite outgrowth

To determine whether neurocan is inhibitory to axon outgrowth, we used a stripe assay as described in Materials and Methods.In this assay, as axons grow out of small explants of developingneural tissue, they can choose to grow on different regions ofthe substrate. Molecules that are inhibitory or nonpermissivefor axonal extension are avoided in this assay (Baier and Klostermann,1994). As shown Figure 1, C and D, the axons that extend out ofeither cerebellar or cortical explants avoid the neurocan stripesand elongate preferentially on L1. Similar results were obtainedwhen the stripes were made with either phosphacan or NG2, twoother CSPGs that are inhibitory to neurite outgrowth (data notshown). The pattern of neurite outgrowth on surfaces coated withstripes of BSA on top of L1 was indistinguishable from that observedon coverslips coated uniformly with L1. Thus, when given a choice,growing axons avoid neurocan.

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Figure 1. Neurocan is avoided by growing axons. A, A cerebellar explant growing on an L1-coated coverslip. Note the uniform halo of growing neurites. B, A cerebellar explant growing on an L1-coated coverslip with stripes of BSA (25 µg/ml). As in A, neurite outgrowth is uniform. C, A cerebellar explant growing on an L1-coated coverslip with stripes of neurocan (10 µg/ml). Axons extend in thin bundles with wider gaps between the bundles. As shown in E, the wide gaps contain the added molecules (in this case neurocan), and the narrow bands are the L1-coated substrate. D, A cortical explant growing on an L1-coated coverslip with neurocan (10 µg/ml) stripes. As in C, wide gaps separate narrow bands of outgrowth. E, Fluorescein-dextran-containing stripes (+) form wide gaps that alternate with narrow bands of uncoated substrate ( $-$ ). A, B, C, and E are epifluorescence illumination; D is phase-contrast optics.

Neurocan expression is upregulated in response to CNS injury

Neurocan expression was examined in frozen sections cut 7 d after a unilateral knife lesion to the cerebral cortex. This revealeda substantial increase in neurocan expression around the lesion,in comparison to the uninjured side (Fig. 2). The 1G2 (anti-neurocan-C)and 1F6 (anti-neurocan-N-terminal fragment) mAbs labeled in anidentical manner. Neurocan expression was increased for a distanceof ~100 µm from the wound edge in the cortical gray matter, butthe increased expression was spread over a greater distance inthe underlying white matter, extending for up to 0.5 mm on eitherside of the injury. In the surrounding normal brain, there wasgenerally much higher expression in white matter than in gray,a notable exception being the labeling of the gray matter adjacentto the midline and medial to the lesion known as the retrosplenialagranular cortex.

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Figure 2. Immunolocalization of neurocan in a CNS lesion. Coronal frozen sections were labeled with the anti-neurocan mAb 1G2 7 d after a knife lesion to the cerebral cortex. The images in a and b were taken with a 10× objective, and those in c and d were taken with a 20× objective. The dorsal surface of the brain is uppermost. Labeling is apparent around the lesion (b, d), which is clearly lacking on the uninjured side (a, c). Scale bar, 100 µm.

Western blot analysis of neurocan expression in the brain

Neurocan has been described in at least four forms: intact neurocan and three smaller forms resulting from proteolytic cleavageof the intact molecule. The C-terminal fraction of the moleculeis known as neurocan-C, whereas there are two species from theN-terminal end of 130 and 90 kDa. The 130 kDa fragment containsthe 1F6 antibody binding site and was therefore detected in ourexperiments, whereas the 90 kDa fragment does not (Meyer-Puttlitzet al., 1995). We refer to these N-terminal fragments as neurocan-130and neurocan-90. All of the species carry chondroitin sulfate.Neurocan-C and neurocan-130 are thought to arise as a result ofa single proteolytic cleavage between amino acids 638 and 639(Rauch et al., 1992; Matsui et al., 1994). This event is referredto as processing, and the smaller neurocan fragments are referredto as the processed forms. The domain structure of neurocan isshown in Figure 3. On Western blots with the antibodies used inour experiments, neurocan is seen as broad indistinct smears,which on chondroitinase treatment resolve into bands of 270 kDa(intact neurocan), 150-163 kDa (neurocan-C), and 122-130 kDa (neurocan-130).To detect these bands we have used three antibodies. Monoclonalantibody 1G2 recognizes intact neurocan and neurocan-C, and mAb1F6 and pAb 291 recognize intact neurocan and neurocan-130.

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Figure 3. Domain structure of neurocan. The two processed fragments detected in the present experiments, neurocan-130 and neurocan-C, are thought to arise as a result of a single proteolytic cleavage on the C-terminal side of met⁶³⁸. Both fragments carry chondroitin sulfate. The 1G2 and 1D1 mAbs recognize epitopes in the C-terminal half of neurocan and react with neurocan-C. The 1F6 mAb and pAb291 recognize structures in the N-terminal half of neurocan and react with neurocan-130. Ig, Immunoglobulin; PTR, proteoglycan tandem repeat; CS, chondroitin sulfate; EGF, epidermal growth factor; CRP, complement regulatory protein.

Neurocan expression in the injured CNS was examined by Western blotting using extracts made from tissue dissected from aroundthe lesion and from control unlesioned cortex. Three serial Tris-bufferedsaline extracts and two Triton X-100 extracts were prepared frominjured brain and its uninjured equivalent in the manner describedin Materials and Methods. In extracts from normal and damagedCNS, the vast majority of all three forms of neurocan was presentin the first saline extract, although it was also detectable inthe two subsequent saline extracts (results not shown). Very littleneurocan was found in the detergentextracts.

Comparison of the first saline extract from injured brain with that from uninjured brain revealed a clear increase in intactneurocan expression in response to the lesion (Fig. 4). The twoextracts were equalized for total protein. In the absence of areducing agent (Fig. 4a), detection of the two smaller processedforms was hampered by nonspecific binding; this problem was greatlyalleviated by the use of a reducing agent. In blots made underreducing conditions, it was possible to see that intact neurocanwas greatly upregulated in the injured CNS, with a slight increasein neurocan-C (Fig. 4b). Under reducing conditions, CNS-derivedintact neurocan migrated at ~275 kDa, neurocan-C at 163 kDa, andneurocan-130 at 122 kDa.

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Figure 4. Western blot analysis of neurocan expression in injured brain. Tris-buffered saline extracts were prepared from injured and uninjured cerebral cortex, and either left untreated ( $-$ ) or treated with (+) chondroitinase ABC (chABC). The extracts were equalized for protein (15 µg in a; 8 µg in b, c), run in a 5% gel either with (b, c) or without (a) a reducing agent (0.2 M DTT), and transferred to nitrocellulose. The blots were labeled for neurocan with either the 1G2 or 1F6 mAb. Both mAbs react with intact (275 kDa) neurocan. The 1G2 mAb recognizes an epitope in the C-terminal half of neurocan and so reacts with neurocan-C, whereas 1F6 recognizes an epitope in the N-terminal half of neurocan and so reacts with neurocan-130. An upregulation of intact neurocan was clearly evident in the injured brain extracts. This difference was apparent whether or not the chondroitin sulfate was removed with chondroitinase ABC (a). The level of neurocan-C was also slightly increased (b). The band just below the 170 kDa marker (arrowhead) is nonspecific. Size determinations were made in a 5% gel by comparison of their relative mobilities with those of laminin (400 kDa), nonreduced $alpha$ ₂-macroglobulin (340 kDa), myosin (204 kDa), $alpha$ ₂-macroglobulin (170 kDa), and $beta$ -galactosidase (116 kDa).

Densitometric analysis of the intact neurocan core protein revealed a ~4.8-fold increase in response to the injury (from Fig.4a, without a reducing agent). On shorter exposures, the chondroitinase-treatedintact neurocan band was seen to consist of three discrete bands.These are likely to result from differences in glycosylation.Neurocan is produced by various cell types (see below), and theseare likely to attach different types and/or amounts ofcarbohydrate.

Production of purified glial cultures

The glial scar that develops after CNS injury contains astrocytes, oligodendrocyte precursors, microglia, and meningeal cells.To ascertain which of these cell types is responsible for theincreased amounts of neurocan, we examined its expression in culturesof purified glial cell types. Astrocyte cultures had to be aspure as possible and free of O-2A progenitor cells, which arealso capable of secreting neurocan (see below). Although shakingthe culture was found to be an effective means of removing O-2Acells and macrophages, some small, round, phase-bright cells remainedattached to the monolayer. These cells were identified as pre-O-2Acells (Ben-Hur et al., 1998), rather than O-2A cells, on the basisof their reactivity with the 5A5 mAb against polysialylated N-CAM(Dodd et al., 1988). The use of an anti-mitotic was found to bea highly effective means of ridding a (confluent) astrocyte monolayerof these highly proliferative cells. The combination of shakingand treatment with leucine methyl ester removed all of the visible,top-dwelling macrophages. More than 95% of the monolayer cellswere astrocytes, insofar as they were GFAP positive. Culturesof O-2A lineage cells were generated by shaking the top-dwellingcells from mixed glial cell cultures, removing microglia and astrocytesby preplating on plastic, and then driving O-2A cell divisionwith FGF2 and PDGF. These cultures contained small numbers ofastrocytes, generally <5%. Meningeal cell cultures were producedby dissociation of meninges stripped from the P0 rat brain. Microglialcultures were made from cells dislodged from mixed glial culturesby light shaking and purified by selecting cells that adheredto plastic that was not tissue culture-treated.

Neurocan is present in astrocyte-conditioned medium

Western blot analysis of astrocyte-conditioned medium with the anti-neurocan mAb 1G2 revealed two broad regions of reactivity,one migrating between ~290 and 425 kDa and the other between 170and 220 kDa. After treatment with chondroitinase ABC, these smearswere resolved into two discrete bands of ~270 and 150 kDa (Fig.5). The 270 kDa band represents the intact neurocan core protein.The 150 kDa species corresponds to the C-terminal half of neurocan(Rauch et al., 1992; Matsui et al., 1994) and is therefore referredto as neurocan-C. A rabbit antiserum raised against a 16 aminoacid peptide (amino acids 483-498) contained within the N-terminalhalf of rat neurocan (Matsui et al., 1994) was also reactive withthe 270 kDa species and with an additional species of (approximately)130 kDa (Fig. 5). The 1F6 mAb, which recognizes an epitope inthe N-terminal half of neurocan (Meyer-Puttlitz et al., 1995),behaved in a similar manner, i.e., it was reactive with the 270and 130 kDa species (Fig. 5). This 130 kDa fragment correspondsto a fragment from the N-terminal half of neurocan and is referredto as neurocan-130. Astrocyte-conditioned medium therefore containsthree species that react with neurocan antibodies: intact neurocan(270 kDa) and two fragments generated by proteolytic cleavage(processing) of the intact molecule, neurocan C (150 kDa) andneurocan-130 (130 kDa).

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Figure 5. Three distinct neurocan species are present in astrocyte-conditioned medium. Western blot analysis of astrocyte (astro) and O-2A lineage cells (O-2A) conditioned medium with anti-neurocan-C (1G2), anti-neurocan-130 (1F6), and anti-versican (12C5) mAbs, and a rabbit antiserum raised against neurocan-130 (pAb291). In chondroitinase-treated (+) conditioned medium, the 1G2 and 1F6 mAbs and pAb291 all recognized the same 270 kDa species (neurocan core protein). The 1G2 mAb was also reactive with a 150 kDa species (neurocan-C), whereas the 1F6 mAb and pAb291 were also reactive with a 130 kDa species (neurocan-130). Without previous chondroitinase treatment, neurocan migrated as a high M_r, polydisperse species (neurocan + GAG). Neurocan core protein and neurocan-C were also detected in O-2A cell-conditioned medium. To demonstrate the specificity of these antibodies, the same samples were probed with an anti-versican mAb. No versican reactivity was detected in astrocyte-conditioned medium. A single, high M_r species was seen in chondroitinase-treated O-2A cell-conditioned medium. This does not correspond to any of those recognized by the neurocan antibodies. No reactivity was seen when a mouse monoclonal IgG₁ was used as the primary antibody (data not shown). Size determinations were made in a 4% gel by comparison of relative mobilities with those of the following proteins: laminin (400 kDa), nonreduced $alpha$ ₂-macroglobulin (340 kDa), myosin (212 kDa), $alpha$ ₂-macroglobulin (170 kDa), and $beta$ -galactosidase (116 kDa).

An antibody (12C5) against the closely-related CSPG versican and a myeloma-derived IgG₁ (MOPC₂₁) were used as negative controls.No 12C5-reactive species were detected in astrocyte-conditionedmedium, although a single, high M_r species was seen in O-2A-conditionedmedium (Fig. 5 and see below). No reactivity whatsoever was seenwhen the MOPC₂₁ IgG₁ was used as the primaryantibody.

Astrocytes process neurocan

To be certain that the 130 and 150 kDa species arose during the culture period and were not an artifact of the storage, concentration,and/or chondroitinase treatment, astrocyte-conditioned mediumwas added, immediately after collection, to a tube containingprotease inhibitor cocktail and centrifuged to remove any detachedcells and debris. Half of the conditioned medium was then addedto hot, two times sample buffer, and boiled immediately for 5min. The other half was treated with protease-free chondroitinaseABC for 3 hr at 37°C. Both samples were then subjected to Westernblot analysis without being concentrated or frozen (Fig. 6a).

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Figure 6. a, The presence of the three forms of neurocan is not an artifact of storage, concentration, or chondroitinase treatment. The same three bands are seen whether conditioned medium is analyzed before or after storing, concentrating, or chondroitinase treatment. b, Protease inhibitors do not affect neurocan processing. Astrocytes were grown in the presence of aprotinin (1.0 µg/ml), anti-thrombin III (0.1 inhibitor U/ml), or TIMP-2 (0.2 µg/ml) for 4 d. Each inhibitor was added fresh each day. Conditioned medium was concentrated and treated with chondroitinase ABC, and an equal amount of total protein (150 µg) was applied to each lane. The blot was labeled with the 1G2 mAb (left) and then relabeled with the 1F6 mAb (right). Neither serine protease (aprotinin and anti-thrombin III) nor metalloproteinase (TIMP-2) inhibitors prevented the processing of neurocan.

The results of this experiment were identical to those described above. Importantly, in the absence of chondroitinase treatment,the 1G2 mAb was reactive with two polydisperse species, the smallerof which (170-220 kDa) corresponds to neurocan-C with attachedGAG (Fig. 6a). As before, treatment with chondroitinase ABC resolvedthese polydisperse species into two discrete bands of ~270 and150 kDa. These findings indicate that (GAG-bearing) neurocan-Cexists in astrocyte-conditioned medium before chondroitinase ABCdigestion and that astrocytes are therefore capable of generatingthe smaller neurocanspecies.

The processing of neurocan is thought to involve a single proteolytic cleavage between amino acids 638 and 639. To find outwhether inhibition of extracellular proteases might reduce orprevent neurocan processing by astrocytes, we investigated theeffects of adding serine protease inhibitors (aprotinin and anti-thrombinIII) and a metalloproteinase inhibitor (TIMP-2) to astrocyte cultures.None of these inhibitors had any effect on neurocan processing,in that the levels of both processed fragments appeared unchanged(Fig. 6b). We also investigated the effects of cysteine proteaseinhibitors (leupeptin, E-64, and cathepsin B inhibitor II) and $alpha$ ₂-macroglobulin, an endoproteinase inhibitor. None of these inhibitorsprevented neurocan processing, in that levels of neurocan-C appearedunaltered (data notshown).

Neurocan is found on the substrate around astrocytes but not on the cell surface

To obtain further evidence for the astrocytic origin of neurocan, astrocyte cultures were double-labeled for neurocan andGFAP. Labeling of living cells revealed deposits of substrate-boundneurocan in the immediate vicinity of most GFAP-positive cells(Fig. 7). The cells themselves were not labeled. The applicationof the same procedure to methanol-fixed cells, which gives theantibody access to the inside of the cell and its ventral (lower)surface, revealed that neurocan was located under and/or insideastrocytes. With time, neurocan came to cover the entire substrate,although it remained visibly concentrated around astrocytes. The1G2, 1F6, and 1D1 mAbs and the polyclonal anti-neurocan-N-terminalfragment labeled in an identical manner. Treatment with transforminggrowth factor (TGF) $beta$ , epidermal growth factor (EGF), or interferon $gamma$ (IFN- $gamma$ ) had no effect on this staining pattern. Neurocan labelingwith either the 1G2 or 1F6 mAb was not affected by pretreatmentof the cells with testicular hyaluronidase, indicating that theattachment of neurocan to the substrate is not dependent on hyaluronate.

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Figure 7. Astrocytes incorporate neurocan into a pericellular, substrate-bound ECM in vitro. Living astrocytes were labeled with the anti-neurocan mAb 1G2 (b), fixed in methanol, and labeled with rabbit antibodies against GFAP (a). Labeling for neurocan was seen on the substrate around GFAP-positive cells. Scale bar, 25 µm.

Neurocan is present in the conditioned medium of O-2A cells

We examined conditioned medium from O-2A cell cultures with the 1G2 antibody. Intact neurocan and neurocan-C were detectablein the conditioned medium of O-2A lineage cells (Fig. 5). Theamount of neurocan in O-2A-conditioned medium was comparable orgreater than that found in astrocyte-conditioned medium, so thefew contaminating astrocytes could not have been responsible formore than a fraction of the neurocan present in O-2A-conditionedmedium. Versican was also detected in the conditioned medium ofO-2A lineage cells. The anti-versican mAb 12C5 recognized a singlespecies of high M_r that required chondroitinase ABC treatmentto enter the gel (Fig. 5).

As with astrocytes, O-2A lineage cells did not label for neurocan. Unlike astrocytes, however, neurocan was not seen on thesubstrate around these cells; neither was it seen under the cellsin permeabilized cultures. This implies that O-2A lineage cellsproduce and process neurocan but do not produce the other extracellularmatrix component that mediates the attachment of neurocan to thesubstrate.

Other cell types

Neurocan was not detectable in the conditioned medium of macrophages or meningeal cells derived from newborn rat brain (datanotshown).

Cytokines influence neurocan expression in astrocytes

Cytokines and growth factors implicated in CNS injury and astrogliosis were screened for their effect on neurocan expressionin astrocytes. The amount of neurocan in astrocyte-conditionedmedium was assessed by immunoblotting with the 1G2 mAb. Screeningexperiments indicated that TGF $beta$ and EGF led to an increase inthe amount of neurocan present in astrocyte-conditioned mediumand that IFN- $gamma$ , interleukin-1 $beta$ (IL-1 $beta$ ), and PDGF-AB led to adecrease (Fig. 8). Tumor necrosis factor $alpha$ , ciliary neurotrophicfactor, leukemia inhibitory factor, interleukin-6, and FGF2 werewithout obvious effect. Astrocytes were exposed to cytokines foreither 4 or 6 d at the concentrations given in Table 1.

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Figure 8. Cytokines influence neurocan expression in cultured astrocytes. The cells were grown for 6 d in the presence of 10 ng/ml of the cytokine, and the conditioned medium was concentrated and digested with chondroitinase ABC and an equal volume (65 µl) was applied to each lane. The blot was labeled with the anti-neurocan mAb 1G2. An increase in the amount of neurocan was seen in response to TGF $beta$ and to a greater extent with EGF. PDGF, IFN- $gamma$ , and IL-1 $beta$ brought about a decline in the amount of neurocan that was detected.


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Table 1. Sources and concentrations of cytokines and growth factors

The effect of TGF $beta$ was most apparent after 2 and 4 d but rather less so after 6 and 8 d (Fig. 9). The more robust responseto EGF was evident at all time points, however. Dose-responseexperiments indicated that 1.0 ng/ml TGF $beta$ was optimal, insofaras 0.1 ng/ml had no discernible effect, and 10 ng/ml did not havea significantly greater effect than 1.0 ng/ml (Fig. 10). EGF wasineffective at 0.1 and 1.0 ng/ml and only brought about an increasein neurocan expression at 10 ng/ml (Fig. 10). When EGF and TGF $beta$ were used in combination, the effect was no greater than thatseen with EGF alone. IFN- $gamma$ and IL-1 $beta$ , and to a lesser extent PDGF,partially negated the effects of EGF (Fig. 10).

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Figure 9. Time course of effects of TGF $beta$ and EGF on neurocan expression in astrocytes. Cultured astrocytes were treated with TGF $beta$ (10 ng/ml) or EGF (10 ng/ml) for 2, 4, 6, or 8 d. The conditioned medium was concentrated and treated with chondroitinase ABC, and an equal amount of protein (200 µg) was applied to each lane. The blot was labeled with the anti-neurocan mAb 1F6. TGF $beta$ and EGF led to an increase in the amount of neurocan detected at all time points. The EGF-induced increase was at all time points greater than that of TGF $beta$ .

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Figure 10. Effects of the concentration of TGF $beta$ and EGF on neurocan expression in astrocytes. Cultured astrocytes were treated with TGF $beta$ or EGF alone (0.1, 1.0, or 10 ng/ml), or with EGF (10 ng/ml) and IFN- $gamma$ (10 ng/ml), IL-1 $beta$ (10 ng/ml), or PDGF (10 ng/ml) for 4 d. The conditioned medium was concentrated and treated with chondroitinase ABC, and an equal volume (30 µl) was applied to each lane. The blot was labeled first with the anti-neurocan-C mAb 1G2 (above) and then with the anti-neurocan-130 mAb 1F6 (below). TGF $beta$ was effective at 1.0 and 10 ng/ml but not 0.1 ng/ml, whereas EGF was only effective in bringing about an increase in neurocan expression at 10 ng/ml. IFN- $gamma$ and IL-1 $beta$ appeared to override the effects of EGF. The EGF/IL-1 $beta$ combination led to an increase in the amounts of neurocan-C and neurocan-130, relative to that of unprocessed neurocan.

The effects of TGF $beta$ , EGF, IFN- $gamma$ , and PDGF were investigated in more detail (Fig. 11). Three separate astrocyte cultures (in25 cm² flasks) were treated with each cytokine (10 ng/ml) for 3 d. Theeffects seen previously were clearly reproduced. Each sample wasequalized for total protein, and the results are therefore indicativeof either an increase in neurocan synthesis or a decrease in itsdegradation or both. The scale of these effects was quantifiedby densitometry. TGF $beta$ brought about a ninefold increase and EGFa 23-fold increase in the amount of neurocan detected. PDGF reducedneurocan levels to ~20% of control, and IFN- $gamma$ brought about a50% reduction. TGF $alpha$ appeared as effective as EGF in stimulatingneurocan synthesis (data not shown). None of the treatments consistentlyaltered the ratios of intact to processed neurocan. To determinewhether these effects were caused simply by an effect on astrocyteproliferation, nuclei were counted in one of the cultures thatwere used for the neurocan analysis. TGF $beta$ , EGF, IFN- $gamma$ , and PDGFhad no effect on cell number, in comparison with untreated astrocytes,under these conditions. These experiments were conducted on wellestablished, confluent monolayers of astrocytes. These cells proliferaterapidly to form a monolayer, but cease to do so once it has beenestablished (i.e., they exhibit contact inhibition). None of thefactors tested had any effect on cell number, presumably becausethey were unable to overcome the effects of contact inhibition.

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Figure 11. Quantification of the effects of TGF $beta$ , EGF, IFN $gamma$ , and PDGF on neurocan expression in astrocytes. Three flasks of astrocytes were grown in the presence of each cytokine (10 ng/ml) for 3 d. The conditioned medium was treated with chondroitinase ABC, and an equal amount of protein (50 µg in a; 200 µg in b) was applied to each lane. The blot was labeled with the anti-neurocan mAb 1G2. The amount of neurocan core protein in each lane was quantified by densitometry. TGF $beta$ brought about a ninefold increase in the amount of neurocan detected, and EGF caused a 23-fold increase (c). PDGF reduced neurocan levels to ~20% of control, and IFN $gamma$ brought about a 50% reduction (d). The error bars represent SEM. By Student's t test, the effects of TGF $beta$ , EGF, and PDGF were significant with p < 0.01. The effects of IFN $gamma$ were less significant (p < 0.05).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurocan is an inhibitory CSPG

We demonstrate in this paper that neurocan arranged as stripes on an L1 substrate repels axons, causing them to be guidedalong the neurocan-free stripes. Previous in vitro experimentshave also shown that neurocan has inhibitory properties (Margolisand Margolis, 1997). Neurocan inhibits outgrowth from embryonicchick CNS neurons and from PC12D cells, probably through directneuronal effects (Freidlander et al., 1994; Katoh-Semba et al.,1998). Neurocan binds with high affinity to the cell adhesionmolecules N-CAM, L1/Ng-CAM, and TAG-1/axonin-1 (Friedlander etal., 1994; Milev et al., 1996), inhibits the homophilic bindingof N-CAM and L1/Ng-CAM (Grumet et al., 1993), inhibits neuronalattachment to N-CAM and L1/Ng-CAM (Friedlander et al., 1994),and inhibits L1/Ng-CAM-dependent neurite outgrowth from embryonicchick neurons (Friedlander et al., 1994). Neurocan also bindswith high affinity to tenascin (Grumet et al., 1994; Aspberg etal., 1997; Rauch et al., 1997; Milev et al., 1998a). In many cases,the inhibitory properties of CSPGs have been attributed to thechondroitin sulfate (Fichard et al., 1991; Brittis et al., 1992;Brittis and Silver, 1994; Smith-Thomas et al., 1994, 1995; Emerlingand Lander, 1996). The binding of neurocan to L1/Ng-CAM was largelydependent on chondroitin sulfate (Friedlander et al., 1994), implyingthat the ability of neurocan to interfere with neurite outgrowthon L1/Ng-CAM may also depend on chondroitin sulfate. The combinationof adhesion molecule and matrix binding may create large complexeswith widespread effects on cell surface and matrix interactionsand therefore multiple effects on axongrowth.

In vivo neurocan is present in many of the structures that guide axons by repulsion during development. It has been suggestedthat the presence of neurocan in the roof plate prevents the incomingdorsal root ganglion axons from crossing the midline (Katoh-Sembaet al., 1998), that neurocan repels retinal axons from the hypothalamusand epithalamus (Tuttle et al., 1998), and that neurocan is involvedin the formation of the barrel fields in the somatosensory cortex(Watanabe et al., 1995). The presence of neurocan in glial barriersin the developing nervous system and its inhibitory effects invitro make it entirely plausible that it would exert similar effectson regenerating axons in the glialscar.

Neurocan is upregulated in the injured CNS

Many previous studies have shown an upregulation of CSPG in CNS injuries. We have demonstrated that one of these CSPGs isneurocan. Immunolabeling showed that neurocan expression was greatlyincreased in vivo around a knife lesion to the cerebral cortex,and Western blot analysis of neurocan in saline extracts preparedfrom injured and noninjured tissue revealed considerably moreneurocan in the injured brain. It has been reported that neurocanis upregulated in response to spinal cord injury and entorhinalcortex lesions (Plant et al., 1998; Haas et al., 1999).

Source of neurocan

At various times the glial scar contains microglia, oligodendrocyte precursors, meningeal cells, astrocytes, and other celltypes. Of these, we show that astrocytes and oligodendrocyte precursorsare able to produceneurocan.

Oohira et al. (1994) showed that astrocyte-conditioned medium contains neurocan, and we have confirmed this. We made strenuousefforts to ensure that these cultures were devoid of pre-O-2Aand O-2A progenitor cells and macrophages, and the few remainingcontaminating cells are likely to be meningeal cells, which wehave shown do not produce neurocan. In low-density astrocyte cultures,the only neurocan detectable by immunocytochemistry was foundon the substrate around (and under) GFAP-positive cells. Sucha distribution makes it highly likely that astrocytes are thesource of this neurocan. The pericellular, substrate-bound distributionof neurocan in cultured astrocytes is somewhat reminiscent ofthat of hyaluronic acid (Asher and Bignami, 1991), and given theability of neurocan to bind hyaluronic acid (Rauch et al., 1991),one might have expected that the attachment of neurocan to thesubstrate is mediated by hyaluronic acid. This is evidently notthe case, however, because hyaluronidase had no effect on theneurocan labeling around astrocytes. Neurocan was also detectedin the conditioned medium of O-2A lineage cells, and they toodid not label for neurocan. Neither did we observe labeling ofthe substrate around these cells. The binding of neurocan to thesubstrate must therefore be mediated by something that astrocytes,but not O-2A cells,produce.

Although neurocan is produced by astrocytes, it is not retained on the astrocyte cell surface. This may explain why conventionalastroglial monolayers support robust neurite outgrowth (Nobleet al., 1984), whereas three-dimensional cultures do not (Fawcettet al., 1989). We have shown previously that proteoglycans impedethe growth of axons in three-dimensional cultures, because sodiumchlorate, which prevents GAG sulfation, renders them more permissive(Smith-Thomas et al., 1995). In conventional monolayer cultures,neurocan is not retained at the cell surface and will be greatlydiluted by the medium, whereas in three-dimensional cultures itis trapped between the cells, where it would be in a positionto interfere with access to neurite outgrowth-promoting moleculesonastrocytes.

In situ hybridization has shown that neurocan mRNA is present in neurons in the postnatal cerebellum (Engel et al., 1996).Neurocan mRNA is also widely expressed in the late fetal forebrain,especially in the major neuronal cell layers (Engel et al., 1996).Curiously, neurocan immunoreactivity is much less widespread thanthe mRNA in late fetal forebrain, possibly because of translationalblock (Meyer-Puttlitz et al., 1996). Immediately after birth,neurocan immunoreactivity spreads throughout the cerebral cortex,and the cellular origin(s) of this neurocan has not been identified(Oohira et al., 1994; Tuttle et al., 1995). The ability of newbornrat brain astrocytes to produce neurocan in vitro suggests thatsome of this neurocan may be produced by astrocytes (Milev etal., 1998b). In addition, oligodendrocyte precursors appear inlarge numbers in the CNS at this time and may be another source,because these cells also produce neurocan in vitro. The strongneurocan immunoreactivity that we have seen in white matter tractsargues in favor of a glialorigin.

In the injured CNS, the appearance of the neurocan labeling is consistent with a glial origin and could be from astrocytesor from oligodendrocyte precursor cells, which are recruited toCNS injuries in large numbers (Levine, 1994). A recent study hasdemonstrated that in the injured CNS astrocytes can produce neurocan(Haas et al., 1999).

Neurocan processing

Neurocan exists as the full-length, intact form and as two smaller chondroitin sulfate-bearing species (Fig. 3). The two smallerspecies are thought to arise as a result of a single proteolyticcleavage between amino acids 638 and 639 (Rauch et al., 1992;Matsui et al., 1994). Northern blot analysis has shown a single(7.5 kb) neurocan transcript in P4 and adult rat brain (Rauchet al., 1992). This and the structure of the neurocan gene (Rauchet al., 1995) argue against the generation of the three formsof neurocan by alternative splicing. The most likely scenariois that the two smaller forms arise as a result of a single proteolyticcleavage. In vitro, astrocytes (and oligodendrocyte precursors)were themselves capable of processing neurocan. The generationof the smaller fragments was not affected, however, by the additionof (non-membrane permeant) serine or cysteine protease or metalloproteinaseinhibitors to the culture medium. These findings suggest thatprocessing occurs intracellularly. In the normal adult CNS theprocessed forms of the molecule predominate, but after injuryit was primarily the intact form of neurocan that wasupregulated.

Control of neurocan expression

What might cause the upregulation of neurocan in CNS lesions? TGF $beta$ has been implicated in the increased deposition of ECMin the glial scar. TGF $beta$ -neutralizing antibodies reduced the depositionof laminin, fibronectin (Logan and Berry, 1993; Lagord et al.,1999), and CSPG (Griffith and McKeon, 1999) in the glial scar.TGF $beta$ also increased the expression of tenascin (Smith and Hale,1997), laminin, and fibronectin (Baghdassarian et al., 1993) incultured astrocytes. We therefore investigated the control ofneurocan expression in astrocytes by cytokines known to be releasedin response to CNS injury. EGF/TGF $alpha$ and TGF $beta$ brought about anincrease in the amount of neurocan relative to the total proteincontent in the conditioned medium of these cells, whereas PDGFand IFN- $gamma$ brought about adecrease.

EGF has been shown to increase TGF $beta$ expression in astrocytes (Lindholm et al., 1992), and it is therefore possible that theeffects of EGF on astrocytes are mediated by TGF $beta$ . Alternatively,it is conceivable that EGF mimics the effects of TGF $alpha$ on astrocytes,the overexpression of which is sufficient to induce astrogliosisin vivo (Rabchevsky et al., 1998).

Inhibition in the glial scar

Neurocan is not the only CSPG that is upregulated in response to CNS injury. Other studies have shown increased expressionof NG2 (Levine, 1994; Grill et al., 1998), versican (Asher etal., 1999), decorin (Stichel et al., 1995), biglycan (Stichelet al., 1995), and phosphacan (McKeon et al., 1995; Barker etal., 1996). We hypothesize that TGF $beta$ or TGF $alpha$ /EGF or both inducean increase in the expression of neurocan in (reactive) astrocytesand that this and recruitment of neurocan-producing oligodendrocyteprecursors lead to the accumulation of this inhibitory CSPG atthe site of injury. The many complex effects of neurocan and otherCSPGs then impede axonalregeneration.

  FOOTNOTES

Received Dec. 27, 1999; accepted Jan. 5, 2000.

This work was supported by the Wellcome Trust, the International Spinal Research Trust, the Medical Research Council, andAction Research. We thank Dr. S. Jenner (Department of Physiology,Cambridge) for help with densitometry and Dr. R. W. Farndale (Departmentof Biochemistry, Cambridge) for use of the densitometer. The 5A5monoclonal antibody was obtained from the Developmental StudiesHybridoma Bank, which was developed under the auspices of theNational Institute of Child Health and Human Development and ismaintained by the Department of Biological Sciences at the Universityof Iowa, Iowa City,IA.
Correspondence should be addressed to James Fawcett, Physiological Laboratory, University of Cambridge, Downing Street, CambridgeCB2 3EG, UK. E-mail: jwf108{at}cam.ac.uk.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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