Repellent Guidance of Regenerating Optic Axons by Chondroitin Sulfate Glycosaminoglycans in Zebrafish

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The Journal of Neuroscience, February 1, 2002, 22(3):842-853

Repellent Guidance of Regenerating Optic Axons by Chondroitin Sulfate Glycosaminoglycans in Zebrafish
Catherina G. Becker and Thomas Becker
Zentrum für Molekulare Neurobiologie Hamburg, Universität Hamburg, D-20246 Hamburg, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We analyzed the role of chondroitin sulfate (CS) glycosaminoglycans, putative inhibitors of axonal regeneration in mammals,in the regenerating visual pathway of adult zebrafish. In theadult, CS immunoreactivity was not detectable before or afteran optic nerve crush in the optic nerve and tract but was constitutivelypresent in developing and adult nonretinorecipient pretectal brainnuclei, where CSs may form a boundary preventing regeneratingoptic fibers from growing into these inappropriate locations.Enzymatic removal of CSs by chondroitinase ABC after optic nervecrush significantly increased the number of animals showing erroneousgrowth of optic axons into the nonretinorecipient magnocellularsuperficial/posterior pretectal nucleus (83% vs 42% in controls).In vitro, a substrate border of CSs, but not heparan sulfates,strongly repelled regenerating retinal axons from adult zebrafish.We conclude that CSs contribute to repellent axon guidance duringregeneration of the optic projection inzebrafish.

Key words: CNS regeneration; extracellular matrix; chondroitin sulfate proteoglycans; heparan sulfate; chondroitinase ABC; tenascin-R; retinal ganglion cell axons; neurite outgrowth

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fish and amphibians, in contrast to mammals, are capable of regenerating lesioned axon tracts in the adult CNS (for review,see Martin et al., 1994; Bernhardt, 1999). Regenerative failureof mammalian CNS axons is, at least in part, attributed to inhibitorymolecules that are expressed by glial cells (for review, see Fawcettand Geller, 1998; Qiu et al., 2000). Expression of chondroitinsulfate (CS)-carrying proteoglycans (CSPGs) is increased in aCNS lesion site, where these molecules may form a barrier to regrowingaxons (for review, see Fawcett and Asher, 1999; Bovolenta andFernaud-Espinosa, 2000). CSs contribute to this inhibition, becausetreatment of lesion sites with chondroitinase renders these moresupportive to axon growth in vitro (McKeon et al., 1995; Zuo etal., 1998) and in vivo (Yick et al., 2000; Moon et al., 2001).

During development, CSs (and also their core proteins; Dou and Levine, 1994; Garwood et al., 1999) play a complex role inaxon guidance (for review see Silver, 1994). Application of chondroitinaseor purified CSs alters the route of optic axons (Brittis et al.,1992; Chung et al., 2000) and other axons (Anderson et al., 1998;Bernhardt and Schachner, 2000). Although in some systems, CSsappear to exclude axons, suggesting a repelling function for axons(Snow et al., 1990; Oakley and Tosney, 1991; for review, see Faissnerand Steindler, 1995), in others, axons appear to prefer CS substrates(Bicknese et al., 1994; Faissner et al., 1994). In yet others,there is a complex distribution of CSs in the pathway of growingaxons (Fernaud-Espinosa et al., 1996; Wilson and Snow, 2000),which led to the suggestion that CSs may anchor other moleculesthat guide axons in the extracellular matrix (Emerling and Lander,1996). Finally, in vitro experiments indicate that reactions ofdeveloping axons to CSs depend on the mode by which the glycansare presented (soluble, homogeneous, or as a step gradient; Snowand Letourneau, 1992; Challacombe and Elam, 1997; Hynds and Snow,1999), on the composition of CS side chains (Faissner et al.,1994; Braunewell et al., 1995; Clement et al., 1998; Nadanakaet al., 1998), and on the neuronal cell type analyzed (Snow andLetourneau, 1992; Fernaud-Espinosa et al., 1994; Dou and Levine,1995).

The optic projection of adult zebrafish regenerates spontaneously after a lesion and precisely reinnervates its former targetsin the brain (C. G. Becker et al., 2000). The optic projectionof teleost fish, including zebrafish (Marcus et al., 1999), iscontinuously growing, such that positive (adhesive and attractive)and negative (repellent and inhibitory) guidance molecules thatare developmentally downregulated in mammals are still presentin the adult fish brain (C. G. Becker et al., 2000; Petrauschet al., 2000). These molecules supposedly guide newly growingand regenerating optic axons to their correcttargets.

We show here that digestion of constitutively present CSs in nonretinorecipient pretectal nuclei increases invasion of thesenuclei by regenerating optic axons in adult zebrafish. A boundaryof CSs in vitro repels retinal axons. This indicates a repellentguidance function of CSs for opticaxons.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals
Adult (body length >2 cm, age >4 months) and developing (age 5 d to 4 weeks) zebrafish, Danio rerio, were taken from our breedingcolony or bought at a local pet shop. Before surgery, adult fishwere maintained in groups of 10 animals at a 14/10 hr light/darkcycle and a temperature of 27°C. After surgery, individual fishwere kept in 2 l tanks. Fish were fed dried fish food and livebrine shrimp. All animal experiments were approved by the Universityand State of Hamburg animal care committees and conformed to NationalInstitutes of Healthguidelines.

Reagents
To detect CSs, we used the CS-56 antibody (Sigma, Deisenhofen, Germany), which recognizes chondroitin-4 sulfate and chondroitin-6sulfate (Avnur and Geiger, 1984). The antigen of the CS-56 antibodyis liable to digestion with purified protease-free chondroitinsulfate ABClyase (chondroitinase, EC 4.2.2.4; Saikagaku, Tokyo,Japan), which was used in this study for in vivo and in vitroexperiments. As an additional enzyme for in vivo experiments,we used heparinase III (heparinase, EC 4.2.2.8; Sigma). Antibody2B6 (Saikagaku) was used to detect "sugar stub" neoepitopes createdby chondroitinase treatment in immunohistochemistry (Moon et al.,2001). Tenascin-R was detected with the mouse monoclonal antibody597 (Pesheva et al., 1989).

Immunohistochemistry combined with tracing of optic axons
Fluorescence immunolabeling of a 14-µm-thick cryosection of fresh-frozen adult and larval tissues was performed as describedpreviously (Becker et al., 1995). Binding of primary antibodieswas detected with the appropriate Cy3-labeled secondary antibodies(Dianova, Hamburg, Germany). The specificity of CS labeling wastested by removing the antigen before staining with chondroitinase(Becker et al., 1995). This treatment completely abolished labelingof CS-56 in the nonretinorecipient pretectal brain nuclei (seeResults). Fluorescence intensity was measured using Universityof Texas Health Science Center (San Antonio, TX) Image Tools forWindows.
For simultaneous visualization of the optic projection and CS distribution, optic nerves were labeled with biocytin (see below).Animals were perfused with 4% paraformaldehyde, and their brainswere embedded in 4% agar and sectioned at 40 µm with a vibratome(Leica, Hamburg, Germany). Biocytin was detected with Cy2-coupledstreptavidin (Dianova); CSs were detected using the CS-56 antibodyand a Cy3-coupled secondary antibody (Dianova). The sections weremounted in Moviol (Merck, Darmstadt, Germany) and viewed undera laser scanning microscope (Zeiss, Oberkochen, Germany) usingargon and krypton lasers, with appropriate emission and detectionwavelengths.

Organotypic retinal cell culture
Preparation of in vitro substrates. Substrates were prepared similarly to a previously published protocol (Becker et al.,1999). All solutions were prepared in PBS; all incubations wereperformed at room temperature; and all washes were done threetimes in PBS, unless indicated differently. Tissue culture wells(35 mm) with a glass bottom (MatTek, Ashland, MA) were coatedwith poly-D-lysine (0.05% in 0.5 M borate buffer) for 2 hr, washed,and air-dried. Wells were then incubated with nitrocellulose dissolvedin methanol according to the method of Lagenaur and Lemmon (1987).Wells were again coated with poly-D-lysine for 2 hr, washed, andair-dried. A mixture of CSs A, B, and C (100 µg/ml; Sigma) orheparan sulfates (HSs, 100 µg/ml; Sigma) were mixed with rhodamine-dextran(1 mg/ml; Molecular Probes, Eugene, OR) and spotted as 8 µl dropletsat 4°C overnight. After washing, laminin (Sigma) was coated onthe surface of the entire well at a concentration of 1.7 µg/mlat 4°C overnight. Wells were washed and immediately used for explantculture. Test substrates were never allowed to dry out throughoutthe coatingprocedure.
Efficient coating of CSs, HSs, and laminin was demonstrated by immunolabeling of substrate spots on cell culture surfacesat the end of cell culture experiments. CS immunoreactivity wasliable to chondroitinase digestion. Immunolabeling for lamininshowed homogeneous coating on the test substrate spot and nextto it (data notshown).
Retinal explant culture. Animals received a bilateral conditioning optic nerve crush 7 d before retinal explant preparation,as published previously for serum-free amphibian retinal explantculture (Becker et al., 1999). Animals were deeply anesthetizedand decapitated, and the eyes were collected in HBSS. Eyes werequickly rinsed in 70% ethanol, and the retinas were dissectedand chopped into 400 × 400 µm squares on a tissue chopper (McIlwain,Gomshall, UK). Squares were washed in HBSS and L-15 tissue culturemedium (Invitrogen, Karlsruhe, Germany) containing N2 supplements(Sigma) and transferred to a medium-filled tissue culture well.Explants were oriented with fine forceps to attach them to theculture substratum with the vitreous side down next to the substrateborder. Culture wells were placed in a humidified chamber, andneurites were allowed to grow out at 26°C for 3-4d.
Quantification of border interactions. The effect of substrate borders on axon outgrowth from retinal explants was quantifiedas described previously (Becker et al., 1999, T. Becker et al.,2000). Because fascicles accumulated at the border at the endof the incubation period (3-4 d; see Fig. 4A), interactions ofindividual fascicles with the substrate border could not be counted.Therefore, border interactions were scored for whole explants.Explants for which virtually all axon fascicles were preventedfrom crossing the substrate border at the end of the incubationperiod were counted and expressed as a percentage of all explantsextending axon fascicles that contacted the substrateborder.

Optic nerve crush and in vivo injections of chondroitinase
For optic nerve lesions of adult zebrafish, individuals were anesthetized by immersion in 0.033% aminobenzoic acid ethylmethylester(MS222; Sigma) for 5 min. One eye was gently lifted from its socket,and the exposed optic nerve was crushed behind the eyeball undervisual control using watchmaker's forceps as described previously(C. G. Becker et al., 2000). At 6 and 13 d after the lesion, animalswere reanesthetized; a small part of the skull overlying the tectumwas removed; and ~0.3 µl of chondroitinase (2 U/ml in 50 mM Tris-HCl,60 mM Na-acetate, and 0.1% bovine serum albumin, pH 7.86) wasinjected into the third ventricle using a glass needle attachedto a micromanipulator. Control animals received either only anoptic nerve crush or injections of either vehicle or 2 U/ml heparinaseIII at 6 and 13 d after optic nerve crush. As a rule, animalswere processed for tracing of regenerated optic fibers at 24 dafter the lesion if not indicatedotherwise.

Tracing
Tracing of optic axons with biocytin was done as described previously (C. G. Becker et al., 2000). Briefly, small pieces ofgelatin foam (Gelfoam; Upjohn, Kalamazoo, MI) soaked with biocytin(Sigma) were prepared. Fish were anesthetized, and the nerve wasexposed as described for the crush. To apply the Gelfoam pledget,the nerve was cut, and the pledget was immediately positionedat the stump of the optic nerve attached to the brain. The tracerwas allowed to be transported for 2.5 hr, and fish were killedby an overdose of aminobenzoic acid ethylmethylester (0.1% for5 min) and perfused with 2% paraformaldehyde and 2% glutaraldehydein PBS, pH 7.3. Perfused brains were sectioned at 50 µm on a vibratome,and the signal was developed using the Vectastain ABC kit (VectorLaboratories, Burlingame, CA) with diaminobenzidine assubstrate.

Quantification of fibers invading the magnocellular superficial/posterior pretectal nucleus
Invading fibers in the magnocellular superficial/posterior pretectal nucleus had circuitous trajectories and could not becounted individually. We determined the area taken by these fibersin cross sections of the magnocellular superficial and the posteriorpretectal nuclei using the Neurolucida image analysis setup andsoftware (MicroBrightField Europe, Magdeburg, Germany). Becausewe could not detect a clear anatomical border between the magnocellularsuperficial and the posterior pretectal nuclei, they were treatedas one continuous area. All slides were coded so that the experimenterwas blind to the treatment of the individual fish analyzed. Thepretectal complex of brain nuclei that are immunopositive forCSs extends over 100-150 µm (i.e., two to three sections). Theoutlines of the parvocellular superficial, accessory, and magnocellularsuperficial/posterior pretectal nuclei (identified by the conspicuouscells at the borders of these nuclei) and the terminal fieldsin the dorsal accessory optic nucleus and in the central pretectalnucleus were marked under the microscope at a magnification of400×. The area covered by fibers invading the magnocellular superficial/posteriorpretectal nucleus was also outlined. The magnocellular superficial/posteriorpretectal nucleus was scored as being invaded by retinal ganglioncell axons when labeled axons were present in at least two consecutivesections. This is because fibers of the passing optic tract oftenobscured the magnocellular superficial/posterior pretectal nucleusin the most rostral section in which this nucleus was contained.Because the intensity of the label in the optic projection varied,only fish were analyzed in which the terminal fields in the dorsalaccessory optic nucleus and the central pretectal nucleus, whichborder the magnocellular superficial/posterior pretectal nucleus,were labeled. Brain nuclei were identified according to the methodof Wullimann et al. (1996).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

New fibers are continuously added to the optic projection in adult zebrafish because of sustained growth of the retina. Thesefibers terminate in the likewise growing optic tectum (the largestterminal field of optic axons) in a retinotopic manner. In thepretectum, the parvocellular superficial pretectal nucleus receivesretinotopic innervation. Other terminal fields in the pretectalarea are present in the central pretectal nucleus and in the dorsalaccessory optic nucleus. Directly adjacent to these nuclei, thereis a complex of pretectal nuclei embedded in the optic projectionthat does not receive retinal fibers and is intensely CS-immunopositive(Fig. 1). These nuclei are the magnocellular superficial pretectalnucleus, the posterior pretectal nucleus, and the accessory pretectalnucleus. The magnocellular superficial pretectal nucleus, whichis situated medially to the caudal end of the parvocellular superficialpretectal nucleus, continues caudally into the posterior pretectalnucleus. (Because we were unable to find a clear anatomical separationfor these two nuclei, they will be referred to as the magnocellularsuperficial/posterior pretectal nucleus in the analysis of invadingfibers.) The accessory pretectal nucleus is situated directlylateral to the posterior pretectal nucleus (Wullimann et al.,1996).

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Figure 1. Semischematic representation of the distribution of optic fibers (A, B) and CS (C, D) in the pretectum of adult zebrafish. The same two consecutive transverse sections are shown in A and B and C and D; dorsal is at the top; lateral is left. A and C are 60 µm rostral to B and D. The presence of optic fibers in A and B and CS immunoreactivity in C and D is indicated by black filling of brain structures. Optic fibers are present in the parvocellular superficial pretectal nucleus (PSp), the central pretectal nucleus (CPN), the dorsal accessory optic nucleus (DAO); the optic tectum (TO; innervation not indicated), and the ventral optic tract (VOT) and dorsal optic tract (DOT). The magnocellular superficial pretectal nucleus (PSm), the accessory pretectal nucleus (APN), and the posterior pretectal nucleus (PO) are free of optic fibers but are strongly CS-immunopositive. Outlines of brain nuclei are taken from Wullimann et al. (1996). Scale bar, 100 µm.

After an optic nerve crush, the entire optic projection is restored. Fibers start to regrow by 1 week after the lesion, arefrequently found on the tectum by 2 weeks after the lesion and,avoiding nonretinorecipient pretectal nuclei, have reinnervatedall former targets by 4 weeks after the lesion (C. G. Becker etal., 2000).

Selective presence of CSs in nonretinorecipient pretectal brain nuclei

To analyze a possible role of CSs for normally growing optic fibers, regenerating optic fibers, or both, the distributionof CS immunoreactivity was analyzed in the optic pathway of unlesionedadult control animals and in animals that had received an opticnerve crush 7-21 d before analysis. In mice and salamanders, alesion-induced increase of CS immunoreactivity in the optic nervehas been reported (Becker et al., 1995; Selles-Navarro et al.,2001). However, in lesioned optic nerves of zebrafish, CS immunoreactivitywas not increased at the crush site or caudal to it (Fig. 2A-C).In the retina (data not shown), optic nerve (Fig. 2A-C), chiasm(data not shown), optic tract (Fig. 2D,F), tectum (Fig. 2D), andother targets of optic axons, such as the parvocellular superficialpretectal nucleus (Fig. 2E,F) and the dorsal accessory optic nucleus(Fig. 2H), CS immunoreactivity was very low in unlesioned andlesioned animals. In contrast, nonretinorecipient pretectal nuclei,the accessory pretectal nucleus, the magnocellular superficialpretectal nucleus, and the posterior pretectal nucleus, were intenselylabeled by CS antibodies in lesioned and unlesioned animals withoutdetectable differences in fluorescence intensity between the lesionedand unlesioned situation (Fig. 2D-H). Large cells at the bordersof these nuclei, which are probably neurons, appeared most stronglyimmunopositive (Fig. 2E,H). A lack of labeling after digestionof tissue sections with chondroitinase showed that the signalof antibody CS-56 was specific (data not shown).

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Figure 2. CS immunoreactivity is not increased after optic nerve crush but is constitutively present in specific pretectal brain nuclei. A-C, Longitudinal sections through the optic nerve are shown; the retina is at the top. CS immunoreactivity is low in the unlesioned optic nerve (A) and is not altered 7 d after an optic nerve crush (B). The crush site is indicated by an arrow in the phase-contrast image in C, corresponding to B. D, Cross section through a brain. Dorsal is at the top; lateral is left. CS immunoreactivity in an unlesioned animal is very low in the optic tract (OT) and the tectum (TO) but intense in the magnocellular superficial/posterior pretectal nucleus (PSm/PO) and the accessory pretectal nucleus (APN). The arrow points to CS-immunopositive meninges. E-H, Visualization of biocytin-labeled optic fibers (green) and CS immunoreactivity (red) using confocal laser scanning microscopy. Orientations are the same as in D. E, The rostral magnocellular superficial pretectal nucleus (red) is contiguous with the parvocellular superficial pretectal nucleus (PSp), which receives dense retinal fibers in an unlesioned animal. CS immunoreactivity is more intense at the border of the magnocellular superficial pretectal nucleus (arrowheads) than in its center. F, Three weeks after a lesion, CS immunoreactivity in the rostral (Figure legend continued.) magnocellular superficial pretectal nucleus is comparable with that in unlesioned controls, and optic fibers have grown back through the optic tract (OT) and reinnervate the parvocellular superficial pretectal nucleus (PSp). G, In a more caudal cross section through the diencephalon, the accessory pretectal nucleus (APN) and the magnocellular superficial/posterior pretectal nucleus (PSm/PO) are strongly labeled by CS antibodies 3 weeks after the lesion. Regenerating fibers grow around these nuclei. H, At a higher magnification, intensely CS-immunopositive cells (arrows) are detectable at the medial border of the magnocellular superficial/posterior pretectal nucleus in an animal 3 weeks after an optic nerve crush. Fibers with small protrusions, which are probably terminals in the dorsal accessory optic nucleus (DAO) and smooth fibers, which are probably fibers of passage, grow along this boundary. Scale bar, 100 µm (for A-C), 200 µm (for D), 75 µm (for E-G), 25 µm (for H).

The CS-expressing brain nuclei are embedded in the optic tract with terminal fields of optic fibers in the parvocellular superficialpretectal nucleus, in the central pretectal nucleus, and in thedorsal accessory optic nucleus surrounding them (Fig. 1). To furthercorrelate the presence of CSs with the absence of optic fibersin nonretinorecipient nuclei, tracing of optic axons was combinedwith CS immunohistochemistry in unlesioned animals and those thathad received an optic nerve crush 3 weeks before analysis. Therewas virtually no overlap between axon labeling and CS immunoreactivityat the border of the nonretinorecipient brain nuclei. In fact,nonlesioned and regenerating optic fibers grew in close associationwith the borders of these nuclei, but only very few of the axonscrossed these borders (Fig. 2E-H).

Thus, a crush lesion of the optic nerve does not produce a possible CS barrier to axonal regeneration at the lesion site orin the optic pathway. The distribution of CS immunoreactivityand axons at the border of the nonretinorecipient pretectal nuclei,however, is consistent with the possibility that CSs provide anegative guidance signal for regenerating optic axons. This signalmay also be read by growing axons of newly generated adult retinalganglion cells in unlesionedanimals.

CS immunoreactivity in the developing diencephalon

To analyze whether CSs in nonretinorecipient pretectal nuclei could also have a guidance function for the developing opticprojection, we studied the developmental expression of CSs inthe diencephalon. By 3 d of development, the first axons retinotopicallyinnervate the tectum (Stuermer, 1988) and have established 10distinct extratectal terminal fields, corresponding to those ofthe adult optic projection (Burrill and Easter, 1994). However,at 5 d of development, we failed to label CSs in the diencephalon(data not shown). Diffuse CS immunoreactivity was observed inthe diencephalon by 8 d of development (Fig. 3A,C). By 4 weeksof development, when the brain is still rapidly growing, CS immunoreactivitywas found in the developing pretectum, concentrated at the borderof an ovoid nucleus (Fig. 3B,D). This pattern is similar in theadult. CS immunoreactivity was low in all other parts of the developingoptic pathway. Thus, early optic axons (<8 d of development) maynot be guided by CSs in the diencephalon, but at later stagesof development, CSs could contribute to guidance of optic axons.

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Figure 3. CS immunoreactivity is present in the pretectum during development. Cross sections through whole larvae are shown; dorsal is at the top; arrowheads in A and B indicate the brain midline; in C and D, lateral is left. A, C, At 8 d of development, weak CS immunoreactivity is present in the pretectum (arrows). At higher magnification (C), the characteristic small punctate appearance of CS labeling is visible (C, arrow). Large spots of immunoreactivity (C, arrowheads) are an artifact from material that separated from the intensely immunopositive cartilage (A, asterisks). Meninges are also CS-immunopositive (C, asterisks). B, D, By 28 d of development, immunoreactivity is distributed in a ring-like pattern in the lateral diencephalon (arrows), resembling the adult configuration. D is a higher magnification of B. Cartilage (D, asterisk) is intensely labeled. Scale bars: A, B, 100 µm; C, D, 50 µm.

Inhibition of regenerating adult retinal axons at a CS border in vitro

To analyze whether regenerating adult optic axons of zebrafish are sensitive to a CS border and whether CSs are sufficientto repel these axons, they were confronted with a CS border inorganotypic retinal culture (Fig. 4). For maximal axon outgrowth,adult fish received a conditioning bilateral optic nerve crush1 week before explantation of retinal tissue. This treatment elicitsoutgrowth of retinal ganglion cell axons of mice (T. Becker etal., 2000), salamanders (Becker et al., 1999), and goldfish (Bastmeyeret al., 1991). Retinal explants were placed next to the borderof a substrate spot of CSs. Laminin was present in these cultureswithin and around the spot area at a concentration that is sufficientto promote outgrowth of retinal axons. Neurites grew out of theexplants by 24 hr. Judged by the rapid and polarized outgrowthof long fibers, similar to that of retinal ganglion cell axonsof the closely related goldfish under the same culture conditions,it was concluded that these axons were most likely retinal ganglioncell axons of zebrafish. Interactions with the substrate borderwere analyzed by 3-4 d in vitro. For 77.8 ± 9.25% (SEM) of theretinal explants (n = 42 explants), virtually all axonal fasciclesshowed a turning response at a substrate border of CSs and didnot penetrate the substrate spot, despite the fact that lamininwas present within the CS substrate spot (Fig. 4A,E). In contrast,spots of HSs, which are also highly charged sulfated glycosaminoglycans,were readily invaded by axonal fascicles. Only 7.7 ± 7.70% ofthe explants (n = 14 explants) were unable to grow axons ontoan HS substrate spot (Fig. 4B,E). As an additional control, CSspots were digested with chondroitinase. This treatment abolishedthe border for axons of all explants analyzed (n = 16 explants;Fig. 4C-E). Inhibition of axon growth at the CS border was statisticallyhighly significant compared with HS border experiments (Fisher'sexact test, p = 0.0003) and chondroitinase-digested CS substratespots (Fisher's exact test, p < 0.0001). Thus, CSs are sufficientto turn adult retinal axons of zebrafish away from a substrateborder in vitro.

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Figure 4. A substrate border of CSs but not HSs repels regenerating optic axons in vitro. A-D, Substrate borders of CSs (A), HSs (B), and CSs after chondroitinase treatment (C) are indicated by small arrows. The position of the substrate border was visualized under fluorescence optics as shown in D, which is taken from the same area depicted in C. Fibers grow from retinal explants that are located in the top left corner. Although fibers are deflected at a CS border (A), they readily invade a substrate spot of HSs (B). The repellent activity of a CS border is abolished after treatment of the substrate with chondroitinase (C). Arrowheads in B and C indicate fibers that crossed the substrate border. E, Quantification of the percentage of explants showing deflection of axons at a substrate border. Inhibition of axon growth at a CS border was statistically highly significant compared with HS borders or chondroitinase (CSase)-digested CS substrate spots (Fisher's exact test, p $<=$ 0.0003; n = number of explants observed). Scale bar, 100 µm (for A-D).

Increased invasion of the magnocellular superficial/posterior pretectal nucleus by regenerating optic fibers after chondroitinase injections in vivo

To determine whether endogenous CSs contribute to negative guidance of regenerating optic axons in vivo, CSs were removedfrom the diencephalon during regeneration using chondroitinase.First, an effective protocol to remove CSs was developed, andthen invasion of optic fibers into nonretinorecipient pretectalnuclei during regeneration was compared between chondroitinase-injectedand heparinase-injected, vehicle-injected, and uninjected controlanimals.

Chondroitinase was injected into the third ventricle of unlesioned animals, and the presence of CSs was analyzed 1 and 7 dafter the injection. Although the enzyme was not targeted to thepretectum by this way of application, no general effects in thebrain were expected, because CSs were highly localized to thepretectum. At 1 d after the injection CS, immunoreactivity wascompletely abolished in the diencephalon (three animals; Fig.5A-C). At 7 d after the injection, CS immunoreactivity was presentin the nonretinorecipient pretectal nuclei (three animals; Fig.5D), albeit at a significantly lower labeling intensity than inuninjected brains (Fig. 5A), which were processed in parallel.Reappearing CS immunoreactivity was strongest around the somataof large neurons at the border of these pretectal nuclei (Fig.5D). Successful removal of CSs from the brain was additionallycontrolled for by detecting neoepitopes (sugar stubs) createdby chondroitinase injection in vivo with antibody 2B6. The antibodydid not show appreciable labeling in uninjected animals (Fig.5E). At 1 d after chondroitinase injection, pretectal nuclei werelabeled in a pattern highly similar to that labeled by the CSantibody CS-56 in uninjected animals (Fig. 5F). Radial glial cellsin the brainstem that are immunopositive for CSs in uninjectedanimals were also labeled in chondroitinase-injected animals byantibody 2B6, indicating widespread diffusion of the enzyme. Thus,CSs were efficiently removed by chondroitinase, and injectionshad to be repeated every 7 d to remove newly expressed CSs.

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Figure 5. CS immunoreactivity but not tenascin-R immunoreactivity is removed from the magnocellular superficial pretectal nucleus of adult zebrafish in vivo by different enzymes. Cross sections are shown; dorsal is at the top; lateral is left. A-D, At 1 d after chondroitinase injection (B), no CS immunoreactivity is detectable with antibody CS-56 in the magnocellular superficial pretectal nucleus compared with uninjected controls (A). C, Phase-contrast image corresponding to B. D, At 7 d after injection, weak CS immunoreactivity is detectable with antibody CS-56 around large neurons in the magnocellular superficial pretectal nucleus (arrows). However, immunoreactivity is generally considerably lower than in uninjected controls (A). E, F, At 1 d after chondroitinase injection (F), chondroitin sulfate stub immunoreactivity, indicating successful removal of CSs, is increased in the magnocellular pretectal nucleus compared with uninjected controls (E). G, H, Chondroitinase injection does not alter tenascin-R immunoreactivity 1 d after injection (H) compared with uninjected controls (G). I, J, CS immunoreactivity is reduced but still detectable in the magnocellular superficial pretectal nucleus 1 d after heparinase injection (J) compared with uninjected controls that were processed on the same slide (I). Scale bar, 100 µm.

To control whether another component of the extracellular matrix was also compromised by the enzyme treatment, immunohistochemistryfor tenascin-R was performed in chondro-itinase-injected animals.Tenascin-R is an inhibitory extracellular matrix protein thatbinds CSPGs (Xiao et al., 1997). The molecule is expressed innonretinorecipient brain nuclei by probably the same large cellsthat are CS-immunopositive at the border of these nuclei, as shownby immunohistochemistry (Fig. 5G) and in situ hybridization (C.G. Becker, J. Schweitzer, T. Becker, and M. Schachner, unpublishedobservations). The distribution of tenascin-R immunoreactivitywas not altered 1 d after chondroitinase treatment (Fig. 5H).CSs had been efficiently removed in these animals, as shown bythe absence of CS labeling on alternating sections. This indicatesthat the enzyme treatment did not alter the distribution of anotherextracellular matrix molecule in nonretinorecipient pretectalbrainnuclei.

Axons start to regrow by ~1-2 weeks after optic nerve crush, and retinotopic reinnervation of the tectum appeared completeby 4 weeks after the lesion (C. G. Becker et al., 2000). To minimizethe number of repeated injections but still having a large numberof regenerating axons at the level of the pretectum, optic nerveswere crushed, and chondroitinase was injected 6 and 13 d afterthe lesion. Trajectories of regenerated axons were analyzed 24d after the lesion if not indicatedotherwise.

Because it is known that a number of axons commit errors in pathway selection (e.g., with respect to laterality at the chiasmand selection of optic nerve brachia during normal regeneration)(C. G. Becker et al., 2000), invasion of nonretinorecipient pretectalnuclei was analyzed in uninjected unlesioned (normal) animalsand in uninjected animals that had received an optic nerve crush.In normal animals, the magnocellular superficial, accessory, andposterior pretectal nuclei were essentially free of optic fiberslabeled by biocytin application to the optic nerve in all animalsanalyzed (zero of six animals had fibers in nonretinorecipientpretectal brain nuclei). In animals that had received an opticnerve crush without concomitant enzyme treatment, fibers grewabnormally into the magnocellular superficial/posterior pretectalnuclei in 47% of the animals analyzed (7 of 15 animals; see Fig.7C). Thus, there is a proportion of animals showing erroneousgrowth of optic axons into the magnocellular superficial/posteriorpretectal nucleus during normal regeneration, confirming previousfindings in goldfish (Springer, 1981).

After injections of the BSA-containing vehicle solution during regeneration, 38% of the animals exhibited fibers in the magnocellularsuperficial/posterior pretectal nucleus (6 of 16 animals; Figs.6A,B, 7B). This indicates that the injection of a protein solutionduring optic fiber regeneration did not increase the proportionof animals showing erroneous growth of optic axons into the magnocellularsuperficial/posterior pretectal nucleus.

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Figure 6. Retinal ganglion cell axons invade the magnocellular superficial/posterior pretectal nucleus after chondroitinase treatment. Vibratome cross sections (50 µm in thickness) through the brain are shown. Optic fibers are labeled with biocytin in brown. Cell somata are counterstained with neutral red; dorsal is at the top; lateral is left. No fibers are detectable in the magnocellular superficial/posterior pretectal nucleus (PSm/PO) 3 weeks after a lesion of the contralateral optic nerve in a vehicle injected animal at low (A) and high magnification (B). In a chondroitinase-treated animal, fibers are present in the magnocellular superficial/posterior pretectal nucleus 3 weeks after a lesion of the contralateral optic nerve, depicted at low (C) and high magnification (D) of the same section. In the vehicle- and chondroitinase-injected cases, fibers are present in the central pretectal nucleus (A, C, CPN) and the dorsal accessory optic nucleus (B, D, DAO), which served as an internal control for efficient labeling of the optic projection. Note that the section in C includes a part of the parvocellular superficial pretectal nucleus (PSp), which is reinnervated by optic fibers, whereas the section depicted in A is slightly more caudal and contains the accessory pretectal nucleus (APN) next to the magnocellular superficial/posterior pretectal nucleus (PSm/PO). Scale bars: C, 100 µm (for A, C); D, 40 µm (for B, D).

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Figure 7. Outlines of the areas invaded by regenerating optic fibers in sections of the magnocellular superficial/posterior pretectal nucleus after different treatments. Chartings of all cases that received chondroitinase (A), vehicle (B), no injection (C), or heparinase injection (D) after contralateral optic nerve crush are shown; dorsal is at the top; lateral is left. The magnocellular superficial/posterior pretectal nucleus stretches over two to three cross sections. These are depicted in columns for the individual cases. All chartings are organized as in the first case in B, with the most rostral section on the bottom and the most caudal section on the top (R $right-arrow$ C). The parvocellular superficial (PSp), magnocellular superficial (PSm), accessory (APN), central (CPN), and posterior (PO) pretectal nuclei, as well as the dorsal accessory optic nucleus (DAO), are outlined as indicated for the first case in B. The area taken by fibers invading the magnocellular superficial/posterior pretectal nucleus in cross sections is black. Fibers reinnervating their regular terminal fields in the dorsal accessory optic nucleus and the central pretectal nucleus are gray. Fibers reinnervating the parvocellular superficial pretectal nucleus after a lesion have been omitted for clarity. Animals were scored as having fibers invading the magnocellular superficial/posterior pretectal nucleus when fibers were present in these nuclei in at least two consecutive sections (see Materials and Methods). Cases are sorted accordingly (+, invasion of fibers; $-$ , no invasion of fibers), and the percentages of cases with fibers in the magnocellular superficial/posterior pretectal nucleus are given. The proportion of cases with fibers in the magnocellular superficial/posterior pretectal nucleus after chondroitinase treatment is highly significantly increased (p = 0.003) compared with vehicle-injected and uninjected controls. *Note that the heparinase preparation contained chondroitinase activity (see Results). Scale bar, 200 µm.

In contrast, chondroitinase injections resulted in fiber invasion of the magnocellular superficial/posterior pretectal nucleusin 83% of the experimental animals (10 of 12 animals; Figs. 6C,D,7A), which was significantly more (Fisher's exact test, p = 0.01)than in the combined controls (uninjected and vehicle-injected).To obtain an indication of whether the invasion of the magnocellularsuperficial/posterior pretectal nucleus was transient in chondroitinase-injectedanimals, six animals received chondroitinase injections on days6 and 13 after the lesion and were allowed to survive for 90 dafter the optic nerve crush. Invasion of the magnocellular superficial/posteriorpretectal nucleus was found in 83% of these fish (five of sixanimals), the same percentage as for animals analyzed 24 d afterthe crush (10 of 12). Hence, the erroneous invasion of the magnocellularsuperficial/posterior pretectal nucleus appears to persist forat least 3 months after a lesion of the optic nerve. Because CSsreappear 7 d after the last chondroitinase injection, which wason day 13 after the lesion, this finding suggests that reappearingCSs do not influence the fibers already present in the magnocellularsuperficial/posterior pretectal nucleus. Testing all chondroitinase-injectedanimals (short- and long-term survivors) against uninjected andvehicle-injected animals showed statistically highly significantdifferences in growth of fibers into the magnocellular superficial/posteriorpretectal nucleus (Fisher's exact test, p = 0.003).

As an additional control, animals were injected with another glycosaminoglycan-degrading enzyme, heparinase III, which releasesHSs from the extracellular matrix. However, immunohistochemistryafter heparinase injection revealed a diminished labeling intensityfor CSs that was intermediate between that in uninjected controlsand in chondroitinase injected animals at 1 (four animals) and7 (two animals) d after the injection in all animals analyzed.Although CS immunoreactivity was completely abolished 1 d afterchondroitinase injection, it was reduced to ~60-80% of uninjectedcontrols after heparinase injection (compare Fig. 5A,B,I,J). Thedegree of reduction of CSs was estimated by measuring the relativefluorescence intensity in confocal sections of the pretectum (seeMaterials and Methods). This indicates that this heparinase preparationalso contained a modest chondroitinase activity. After heparinaseinjections, 64% (7 of 11; Fig. 7D) of the animals had fibers inthe magnocellular superficial/posterior pretectal nucleus. Thisvalue was intermediate between those for chondroitinase-injectedand control animals, correlated with the intermediate chondroitinaseactivity in this preparation. Thus, the small increase in theproportion of animals with fibers in the magnocellular superficial/posteriorpretectal nucleus after heparinase III treatment (~22% comparedwith vehicle-injected and uninjected controls) probably reflectsa specific dose effect of chondroitinase in the enzyme preparation.However, we cannot exclude that the effect could be attributableto digestion of HSs, because these may have functions similarto CSs (Garcia-Abreu et al., 2000). Heparinase treatment of sectionsfrom glial scar tissue has been found to augment axon growth onthese sections in vitro but to a lesser extent than chondroitinasetreatment (McKeon et al., 1995).

Interestingly, although the accessory pretectal nucleus was also efficiently freed of CS immunoreactivity by chondroitinasetreatment, erroneous growth of fibers into this nucleus was rarelyobserved and was not different between enzyme-injected fish andcontrols. This suggests the presence of additional repellent moleculesin this nucleus (seeDiscussion).

Although the proportion of animals exhibiting growth of fibers into the magnocellular superficial/posterior pretectal nucleuswas significantly increased by chondroitinase injections, thedensity of fibers and the average cross-sectional area taken byinvading fibers was not increased when control animals with fibersin the magnocellular superficial/posterior pretectal nucleus werecompared with chondroitinase-injected cases (Fig. 7). This suggeststhat chondroitinase treatment increases the probability of axonscrossing the intensely CS-positive border of the magnocellularsuperficial/posterior pretectal nucleus but does not influencegrowth of fibers once they have taken residence in thenucleus.

Erroneously growing fibers in the magnocellular superficial/posterior pretectal nucleus appear to enter this nucleus fromits ventrolateral margin, because they were present in this areain all animals in which the posterior pretectal nucleus was invaded(controls and chondroitinase-injected; Fig. 7). The reason whyfibers are prevented from invading the dorsal part of the magnocellularsuperficial/posterior pretectal nucleus or from overshooting theirgrowth into the diencephalon remains unclear. Possible terminalarborization in the ventral part of the magnocellular superficial/posteriorpretectal nucleus may be one reason why axons did not grow moredeeply into thenucleus.

Alterations of trajectories of optic fibers attributable to chondroitinase treatment were expected only in the pretectum,because CSs were not present at conspicuous levels in other partsof the optic pathway. To exclude any nonspecific alterations ofoptic fibers, the optic pathway outside the pretectum was alsoexamined in all experimental groups. In enzyme-injected and controlanimals with regenerating optic fibers, an increase in the numberof ipsilateral fibers was noted, which is in agreement with previousobservations (C. G. Becker et al., 2000). The shapes and sizesof terminal fields in thalamic targets of optic fibers and inthe tectum were comparable with those in unlesioned animals inall experimentalgroups.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study we show that in the injured optic pathway of adult zebrafish, CS immunoreactivity is not increased to detectablelevels by a lesion of the optic nerve. However, we provide invivo and in vitro evidence that constitutively present CSs atthe border of nonretinorecipient brain nuclei form a barrier foroptic axons during regeneration and thus provide negative guidanceinformation during target selection of theseaxons.

We observed increased growth of fibers into the magnocellular superficial/posterior pretectal nucleus after chondroitinasetreatment in vivo, which was probably a specific consequence ofthe removal of CSs rather than of a general destabilization ofthe extracellular matrix. Immunoreactivity for another componentof the extracellular matrix, tenascin-R (Pesheva et al., 1989),was unchanged in the nonretinorecipient pretectal brain nuclei,although tenascin-R binds at least one CSPG, namely phosphacan(Xiao et al., 1997), and may by itself carry CS side chains (Probstmeieret al., 2000a,b). Moreover, the percentage of animals with fibersin the magnocellular superficial/posterior pretectal nucleus aftertreatment with a heparinase (64%) preparation that contained alow chondroitinase activity (see Results) was intermediate betweenthose of control (41%) and chondroitinase-treated (83%) animals,suggesting a dose-dependent effect of CSs on optic axons at theborder of the magnocellular superficial/posterior pretectalnucleus.

Although chondroitinase treatment significantly increased the number of animals with fibers invading the magnocellular superficial/posteriorpretectal nucleus, a substantial proportion of uninjected andvehicle-injected animals (41%), in which the distribution of CSwas uncompromised, also showed growth of optic fibers into thisnucleus. One possible explanation for this is that, unlike newlygenerated axons in unlesioned animals, regenerating axons growas a front, i.e., a large number of growth cones encounter nonretinorecipientpretectal nuclei simultaneously in the absence of preexistingfibers, which could be a substrate for axonal fasciculation alongthe correct pathway. Thus, with a disturbed balance between attractiveand repellent cues, a fraction of the axons may commit navigationalerrors in a stochastic manner. Pathway errors may be amplifiedby fasciculation of axons along erroneous pathways. Pathway errorscommitted by regenerating optic axons in fish are well known phenomena(Springer, 1981; C. G. Becker et al., 2000).

Regenerating optic axons of zebrafish are probably repelled by CSs directly, as suggested by the fact that a CS substratespot in vitro induces neurites (which most likely are regeneratingretinal ganglion cell axons) from adult retinal explants to growaround its border. This finding is in agreement with data showingthat developing optic axons (Snow et al., 1991; Brittis et al.,1992; Snow and Letourneau, 1992) as well as other developing axons(Dou and Levine, 1995) of mammals are repelled by a border ofCSs in vitro. In contrast, specific CS epitopes promote neuriteoutgrowth (Faissner et al., 1994; Clement et al., 1998). SolubleCSs promote the growth of optic axons of goldfish (Challacombeand Elam, 1997). This underscores that the axonal reaction toCSs (Snow and Letourneau, 1992; Snow et al., 1996; Hynds and Snow,1999) and also to other matrix molecules, such as tenascins (Lochteret al., 1991, 1994; Lochter and Schachner, 1993; Pesheva et al.,1993; Taylor et al., 1993), depends on the way the molecules arepresented to the axons (as a homogeneous or step gradient substrateor soluble in the culture medium). The complex reactions of developingoptic axons in slice cultures of the optic chiasm of mice (Chunget al., 2000) to the removal of CSs may be related to the potentialrole of the spatial configuration in which the molecules are encounteredin a specific CNS structure. There is also evidence to suggestthat CSs are anchor points for guidance molecules (Emerling andLander, 1994, 1996).

CSs are not the only axon-repellent molecules in the pretectum. The accessory pretectal nucleus, which is normally also stronglyCS-immunoreactive, did not show appreciable invasion of fibersafter removal of CSs. Moreover, erroneously growing fibers inthe magnocellular superficial/posterior pretectal nucleus afterCS removal were not as dense as in adjacent "appropriate" terminalfields of retinorecipient nuclei. Reappearing CSs may preventlate-coming axons from invading nonretinorecipient pretectal nuclei.However, there are additional molecules that could contributeto the inhibition of axon growth through the border of nonretinorecipientpretectal nuclei and could in part substitute for the functionof CSs after chondroitinase treatment. One of these moleculesmay be tenascin-R, because it also repels optic axons of chicks(Taylor et al., 1993), salamanders (Becker et al., 1999), andmice (T. Becker et al., 2000). In fact, tenascin-R immunoreactivityis stronger in the accessory pretectal nucleus than in the magnocellularsuperficial/posterior pretectal nucleus, which correlates withthe absence of invading fibers in the accessory pretectal nucleusafter chondroitinase treatment (data not shown). In addition,two axon-repellent semaphorins, sema Z1a (Shoji et al., 1998)and sema Z1b (Roos et al., 1999), are strongly expressed in thelarge neurons at the medial border of the magnocellular superficial/posteriorpretectal nucleus (D. Gimnopoulos, T. Becker, C. G. Becker, andM. Schachner, unpublishedobservations).

Repellent or inhibitory guidance by CSs may be important for regenerating as well as developing axons. In teleosts, the magnocellularsuperficial pretectal nucleus receives secondary visual inputfrom the tectum (Yoshimoto and Ito, 1993), and the separationof primary and secondary visual information is conceivably offunctional significance for the visual system. We could not detectCSs in the optic pathway at 5 d of development, when the initialprojections of optic fibers to extratectal targets (Burrill andEaster, 1994) and the tectum (Stuermer, 1988) are already in place.Shortly after that (8 d of development), however, diffuse CS immunoreactivitywas detectable in the pretectum. By 4 weeks of development, whenthe brain is still growing rapidly, CS immunoreactivity resemblesthe adult pattern. This suggests that pioneering fibers of theoptic projection may not be guided by CSs, but that with increasingcomplexity of the differentiating brain, this cue becomes importantfor the developing optic projection. The optic projection of fishgrows throughout life (Meyer, 1978; Marcus et al., 1999), correlatedwith the constitutive expression of positive (netrin-1; Petrauschet al., 2000) and negative (ephrin-A2 and -A5; C. G. Becker etal., 2000) guidance cues in the adult that are developmentallydownregulated in mammals (Wizenmann et al., 1993).

In zebrafish spontaneous axonal regeneration beyond a CNS lesion site may in part be attributable to the absence of CSs, whichin mammals are increased in expression at the lesion site. Wedid not find a lesion-induced increase in CS immunoreactivityin the optic nerve of zebrafish, whereas in the optic nerve (Selles-Navarroet al., 2001) and spinal cord of mammals (Davies et al., 1997,1999; Pasterkamp et al., 2001), detectability of CSs and theircore proteins (Levine, 1994; McKeon et al., 1999) is stronglyincreased after a lesion. However, increased expression of CSsin the injured optic nerve of the goldfish, which is closely relatedto zebrafish, has been described previously (Battisti et al.,1992). In the investigation on goldfish, other antibodies to CSshave been used than in our present analysis, and it is possiblethat the epitope recognized by the CS-56 antibody (Avnur and Geiger,1984; Sorrell et al., 1993) is not present in all CS-expressingstructures. Nevertheless, it has been shown that the CS epitopestructure recognized by CS-56 closely correlates with inhibitionof axon growth on glial cells in vitro (Fidler et al., 1999; Niederöstet al., 1999) and in glial scars in vivo (Davies et al., 1997,1999; Moon et al., 2001; Plant et al., 2001). Microtransplantedneurons that grow in the spinal white matter of rats stop growingwhen they encounter a CS-immunopositive lesion site (Davies etal., 1999). Recently, it has been shown that the removal of CSsat the lesion site in vivo induces regrowth of injured nigrostriatalfibers in rats (Moon et al., 2001).

Similar to CSs, some other inhibitory molecules thought to be responsible for the lack of axonal regeneration in adult mammalsmay be absent or removed from the spontaneously regenerating CNSof anamniotes. In vitro evidence suggests that the myelin inhibitorNogo-1 (Chen et al., 2000) is absent (Lang et al., 1995; Wanneret al., 1995) or expressed at lower levels (Sivron et al., 1994)in the regenerating CNS of fish and amphibians. Tenascin-R, anotheroligodendrocyte-derived inhibitor of axon growth (Pesheva et al.,1989), persists after optic nerve crush in mice (T. Becker etal., 2000) but disappears from the injured nerve of salamandersconcomitantly with regeneration of optic fibers (Becker et al.,1999).

In conclusion, the absence of growth-inhibitory molecules from lesioned pathways may contribute to spontaneous axonal regenerationafter injury in the CNS of anamniotes. In the present study, thiscorrelation is exemplified by the absence of CSs from a crushsite of the optic nerve of zebrafish. However, inhibitory or repellentmolecules may be very important for correct guidance, as shownby the repellent environment encountered by optic axons at theborder of CS-expressing nonretinorecipient pretectal brain nuclei.Extrapolated to the situation in mammals, our results suggestthat neutralization of inhibitory molecules along axonal pathwaysis one way to facilitate axon regrowth. However, inhibitory signalsmay be necessary at sites of pathway choices and in target areasof regenerating axons to accomplish correctguidance.

  FOOTNOTES

Received Aug. 20, 2001; revised Nov. 2, 2001; accepted Nov. 6, 2001.

This work was supported by Deutsche Forschungsgemeinschaft Grants Be1654/3 and Be1650/3-1. We thank Dr. Melitta Schachnerfor support, Drs. Melitta Schachner, Mario F. Wullimann, and UdoBartsch for helpful suggestions and critically reading this manuscript,Dr. Alexander Dityatev for help with statistical analyses, andVladimir Sytnyk for introduction to the confocalmicroscope.
Correspondence should be addressed to Dr. Catherina G. Becker, Zentrum für Molekulare Neurobiologie Hamburg, UniversitätHamburg, Martinistrasse 52, D-20246 Hamburg, Germany. E-mail:tcbecker{at}zmnh.uni-hamburg.de.

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