Schwann Cell Type V Collagen Inhibits Axonal Outgrowth and Promotes Schwann Cell Migration via Distinct Adhesive Activities of the Collagen and Noncollagen Domains

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The Journal of Neuroscience, August 15, 2001, 21(16):6125-6135

Schwann Cell Type V Collagen Inhibits Axonal Outgrowth and Promotes Schwann Cell Migration via Distinct Adhesive Activities of the Collagen and Noncollagen Domains
Michael A. Chernousov, Richard C. Stahl, and David J. Carey
Sigfried and Janet Weis Center for Research, Geisinger Clinic, Danville, Pennsylvania 17822-2613

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previously, we reported the cloning of $alpha$ 4 type V collagen, a novel member of the collagen type V gene family that is expressedby Schwann cells in developing peripheral nerves (Chernousov etal., 2000). The present study was performed to investigate theeffects of this collagen on the adhesion and migration of premyelinatingSchwann cells and neurite outgrowth from embryonic dorsal rootganglion neurons. Purified $alpha$ 4(V)-containing collagen isolatedfrom Schwann cell conditioned medium (collagen type V_SC) promotedmigration of Schwann cells but inhibited outgrowth of axons fromrat embryo dorsal root ganglia. Collagen type V_SC blocked axonaloutgrowth in the presence of otherwise active substrates suchas collagen type IV, indicative of active inhibition. The noncollagenN-terminal domain of $alpha$ 4(V) promoted Schwann cell adhesion, spreading,and migration. These processes were inhibited by soluble heparinbut not by function-blocking antibodies against $alpha$ 1- and $alpha$ 2-integrins.The collagen domain of pepsin-digested collagen type V was poorlyadhesive for Schwann cells. The type V collagen domain but notthe $alpha$ 4(V) N-terminal domain blocked neurite outgrowth from dorsalroot ganglion neurons. In cocultures of dorsal root ganglion neuronsand Schwann cells, collagen type V_SC promoted axon fasciculationand association of axons with Schwann cells. These results suggestthat in embryonic peripheral nerves, collagen type V_SC plays adual role in regulating cell migration. This represents a heretoforeunrecognized function of peripheral nerve collagen fibrils inregulating patterns of peripheral nerve growth duringdevelopment.

Key words: Schwann cell; axonal outgrowth; extracellular matrix; cell migration; collagen; integrins; heparan sulfate

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

During development cellular interactions with the extracellular matrix (ECM) regulate many aspects of cell function, includingmigration, cytoskeletal organization, proliferation, and differentiation.Interactions of cells with ECM molecules are mediated by cellsurface receptors that display a range of binding specificities.The best-studied ECM receptors are the integrins (Hynes, 1992;Clark and Brugge, 1995). These transmembrane heterodimers bindECM proteins and cytoplasmic structural and signaling proteins,thereby providing a mechanism for regulating cell function viaECM contact. Other proteins have also been shown to function asECM receptors. The syndecan transmembrane proteoglycans, for example,bind ECM proteins via their attached heparan sulfate chains (Saundersand Bernfield, 1988; Elenius et al., 1990; Sanderson et al., 1992;Chernousov et al., 1996). Syndecans are also linked to cytosolicstructural proteins (Rapraeger et al., 1986; Carey et al., 1996)and signaling proteins (Oh et al., 1997; Granes et al., 1999),providing an additional pathway for transduction of ECM-dependentsignaling.

Our laboratory has been investigating the function of ECM proteins in the developing peripheral nervous system. We identifieda heparin-binding protein that is expressed by Schwann cells inembryonic and early postnatal nerves (Chernousov et al., 1996;Chernousov et al., 1999). Molecular cloning identified this proteinas a member of the type V collagen family, which we called $alpha$ 4(V)-collagen(Chernousov et al., 2000). $alpha$ 4(V)-collagen exhibits several unusualproperties that are likely to influence its biological function.This collagen chain binds the heparan sulfate proteoglycan syndecan3 with high affinity (K_d, ~0.2 nM) through an interaction withthe proteoglycan heparan sulfate chains (Chernousov et al., 1996).In contrast to other fibril-forming collagens, type V collagensoften retain their N-terminal noncollagenous domains (Linsenmayeret al., 1993; Moradi-Ameli et al., 1994). This occurs to a highdegree for $alpha$ 4(V)-collagen chains synthesized by Schwann cellsand in developing peripheral nerves in vivo (Chernousov et al.,2000).

During the period in which $alpha$ 4(V)-containing collagen molecules are expressed by Schwann cells, the nerves are in a dynamicstate of axonal growth and Schwann cell proliferation and migration(Webster et al., 1973). Many ECM proteins, including some collagens,promote the outgrowth of axons from cultured neurons (Hynes andLander, 1992), as well as migration of Schwann cells. Thus, ECMmolecules might function as contact-dependent guidance cues. Contact-dependentrepulsive signals also provide important cues that direct nervefiber growth (Tessier-Lavigne and Goodman, 1996). Such functionshave also been ascribed to some ECM proteins, notably tenascin(Gotz et al., 1996), particular laminin isoforms (Patton et al.,1997), and chondroitin sulfate proteoglycans (Dou and Levine,1995; Brittis et al., 1995; Zuo et al., 1998).

The restricted pattern of expression and unusual biochemical properties suggest that $alpha$ 4(V)-containing collagen molecules mightperform important functions in developing nerves. This paper presentsour findings on adhesion and migration-promoting activities ofSchwann cell type V collagen. The results demonstrate that Schwanncell type V collagen is multifunctional and displays domain-specificeffects on axonal outgrowth and Schwann celladhesion.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Purification of Schwann cell collagen type V. Collagen type V was isolated from cultures of neonatal rat Schwann cells asdescribed previously (Chernousov et al., 2000). Briefly, conditionedmedium of ascorbate-treated Schwann cells was collected and fractionatedby salt precipitation, anion exchange chromatography, and heparinaffinity chromatography. The elution of collagen type V was monitoredby immunoblot analysis using antibodies specific for the $alpha$ 4(V)-collagensubunit (previously called p200). The purity of the final preparationwas verified by SDS-PAGE and silver staining. Pepsinized bovineplacenta type V collagen was obtained from Chemicon (Temecula,CA).

Preparation of the recombinant $alpha$ 4(V) N-terminal domain. The noncollagenous N-terminal domain (NTD) of $alpha$ 4(V)-collagen was expressedas a His-tagged recombinant protein in bacterial cells. The cDNAcoding for this domain (corresponding to amino acids 30-369; Chernousovet al., 2000) was generated by PCR amplification using sequence-specificprimers and full-length $alpha$ 4(V) cDNA as the template. The cDNA productwas subcloned into plasmid pET30-a⁺ (Novagen, Madison, WI) for transformation and induction of expressionin Escherichia coli cells (strain BL21-pLysS). The recombinantprotein was purified from cell lysates by Ni²⁺ affinity chromatography. Purity of the final product was verifiedby SDS-PAGE.

Schwann cell migration assay. Multiwell plastic dishes (4-well, Nunc, Naperville, IL; or 12-well, Corning, Corning, NY) werecoated with purified ECM proteins (10 µg/ml in 50 mM Tris-HCl,pH 7.5, and 0.1 M NaCl) overnight at 37°C at a coating densityof 2 µg/cm². The protein solution was removed by aspiration, and the wellswere rinsed with water and air-dried.

Dorsal root ganglia were dissected from 18-d-gestation rat embryos. The capsules were removed, and the ganglia were placedonto the coated dishes and covered with ~50 µl of serum-free medium.The medium consisted of a 1:1 mixture of DMEM and Ham's F-12 mediumsupplemented with 100 µg/ml apotransferrin, 5 µg/ml insulin, 1.4mM L-glutamine, 200 nM progesterone, 100 µm of putrescine, 30nM selenium, and 250 ng/ml heregulin peptide (Rahmatullah et al.,1998). Heregulin was added to the medium to promote Schwann cellsurvival and differentiation (Grinspan et al., 1996; Syroid etal., 1996). Heregulins also have been shown to stimulate Schwanncell migration (Mahanthappa et al., 1996). The ganglia were incubatedat 37°C in a humidified tissue culture incubator in at atmosphereof 7% CO₂. On the following day, sufficient medium was added tocover the bottoms of the culture wells, and the incubation wascontinued. Schwann cells that migrated from the ganglia were visualizedby phase contrast microscopy and photographed. Migration was quantitatedby measuring the distance on photomicrographs from the edge ofa ganglion to the leading edge of migrating Schwann cells, i.e.,the cohort of cells that had migrated the greatest distance fromthe ganglion. Three measurements were made in different directionsof radial migration for each ganglion and averaged. Collagen typeI was obtained from Collaborative Biomedical Products. Collagentype IV was from Becton Dickinson (Mountain View, CA). Laminin(mouse EHS) was from Sigma (St. Louis, MO). Human plasma fibronectinwas purchased fromChemicon.

Neurite outgrowth assays. Neurite outgrowth assays were similar to the Schwann cell migration assays, except that the serum-freemedium contained nerve growth factor in place of heregulin peptide.In some experiments the ganglia were dissociated to single-cellsuspensions before plating onto ECM-coated dishes. Ganglia weredissociated by incubation for 30 min in 0.05% trypsin in calcium-and magnesium-free HBSS and trituration through a small-bore pipette.Trypsin activity was stopped by addition of soybean trypsin inhibitor(0.05%).

Assays to determine the effects of combinations of ECM proteins were performed as follows. Dishes were first coated with asingle purified ECM protein as described above. The followingday, ~50 µl of a second ECM protein (10 µg/ml) was applied asa single drop to the center of the dry well. The dishes were incubatedfor 2 hr at 37°C. The solution was removed, and the wells wererinsed with water and air dried. This procedure produces an areain which the dish is coated with an approximately equimolar ratioof the two ECM proteins. Dorsal root ganglia were placed on thesedishes and incubated for up to 4 d. Outgrowth of axons was visualizedand quantitated as describedabove.

Schwann cell adhesion assays. Twenty-four-well plates were coated with ECM proteins (20 µg/ml in 20 mM Tris-HCl, pH 7.6, and0.1 M NaCl) at a coating density of 2 µg/cm² overnight at 37°C. After removing the protein solution and washingwith Tris buffer, the dishes were blocked with 1% BSA in Trisbuffer for 1 hr at 37°C. Schwann cells were isolated from newbornrat sciatic nerves and cultured in DMEM, 10% fetal bovine serum,and 2 µM forskolin as described previously (Carey and Stahl, 1990).For adhesion assays, Schwann cells were released by trypsinizationand resuspended in serum-free medium with heregulin. The cellswere added to the ECM-coated wells and incubated for 3 hr at 37°C.In some experiments, inhibitors of cell adhesion were used. Function-blockinghamster monoclonal anti-integrin $alpha$ 1 (clone Ha31/8) and anti-integrin $alpha$ 2 (clone Ha1/29) antibodies were obtained from Dr. Victor Koteliansky(Biogen, Cambridge, MA). Function-blocking hamster monoclonalanti- $beta$ 1-integrin antibody (clone Ha2/5) was purchased from PharMingen(San Diego, CA). These antibodies or a control hamster monoclonalantibody was added to the attachment medium at a concentrationof 10 µg/ml. Heparin (10 µg/ml) was also used as a competitiveinhibitor of heparan sulfate-dependent binding interactions. Atthe end of the incubation period, the medium was aspirated, andthe wells were washed with DMEM to remove nonadherent cells. Attachedcells were fixed with 3% paraformaldehyde in PBS and stained with0.5% crystal violet in 10% ethanol for 20 min. After extensivewashing with water, bound dye was solubilized with 1% SDS, andthe absorbance was read at a wavelength of 595 nm. All adhesionexperiments were done in duplicate and repeated at least twotimes.

Experiments to investigate Schwann cell spreading were performed in the same way, except that the cells were incubated for24 hr. Cell spreading was visualized by phase contrastmicroscopy.

Immunofluorescence microscopy. Immunofluorescent staining of cultured Schwann cells and neurons was performed as describedpreviously (Carey and Stahl, 1990). Mouse monoclonal anti-neurofilamentantibody and goat anti-mouse IgG coupled to fluorescein isothiocyanatewas obtained from Sigma. Rabbit anti-S100 antibodies were fromDako (Glostrup, Denmark). Goat anti-rabbit IgG conjugated withTexas Red-X was obtained from Molecular Probes (Eugene,OR).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Type V collagen synthesized by Schwann cells promotes Schwann cell migration

Type V collagen was purified from conditioned medium of ascorbate-treated Schwann cells. As described previously, type V collagensynthesized by Schwann cells (collagen type V_SC) is a heterotrimerthat contains $alpha$ 4(V) and $alpha$ 1(V) collagen chains (Chernousov et al.,2000). The ability of collagen type V_SC to promote Schwann cellmigration was investigated and compared with the activities ofother ECM proteins that are also present in the peripheral nerveECM. For these experiments, rat embryo dorsal root ganglia wereplaced on ECM-coated plastic dishes and cultured in serum-freemedium that lacked neurotrophic agents but contained heregulin,a growth factor that promotes Schwann cell survival and differentiation(Grinspan et al., 1996; Syroid et al., 1996). Under these conditions,outgrowth of axons from the ganglia was not observed on any substrate.Schwann cells migrated from ganglia cultured on collagen typeI, collagen type IV, collagen type V_SC (Fig. 1A), and laminin(data not shown). Identification of the migrating cells as Schwanncells was confirmed by staining with the cell-specific markerS100 (data not shown). Quantitation of Schwann cell migrationrevealed that the collagens and laminin were significantly betterat stimulating migration than control substrata (Fig. 1B).

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Figure 1. Schwann cell migration and axonal outgrowth on ECM-coated surfaces. A, Rat embryo dorsal root ganglia were cultured in serum-free medium with heregulin on dishes coated with the indicated ECM proteins. The ganglia were incubated for 4 d and examined by phase contrast microscopy. B, Schwann cell migration was quantitated as described in Materials and Methods, and the results are displayed graphically. The values shown are the mean ± SD for measurements made on four separate cultures. C, Rat embryo dorsal root ganglia were cultured on dishes coated with the indicated ECM proteins in serum free medium with nerve growth factor. The micrographs show outgrowth from individual ganglia after 4 d in culture. D, Axonal outgrowth was quantitated after 4 d in culture, and the results are shown graphically. The values shown are the mean ± SD for measurements made on four separate cultures. IV, Collagen type IV; Ln, laminin; I, collagen type I; V_SC, collagen type V_SC; con, control (uncoated plastic).

Collagen type V_SC inhibits axonal outgrowth

The ability of collagen type V_SC to promote outgrowth of axons from rat embryo sensory neurons was also examined and comparedwith outgrowth-promoting activities of other ECM proteins. Forthese experiments, rat embryo dorsal root ganglia were placedon plastic dishes coated with matrix proteins and cultured inserum-free medium that contained nerve growth factor. On dishescoated with laminin, collagen type I, or collagen type IV, theganglia produced dense radial outgrowths of axons (Fig. 1C). Theaxonal nature of these processes was confirmed by staining withanti-neurofilament antibodies (data not shown). In contrast, gangliaplated on dishes coated with collagen type V_SC failed to producesignificant outgrowth of axons (Fig. 1C). Quantitation of axonaloutgrowth is shown in Figure 1D. Dishes coated with laminin, collagentype I, or collagen type IV produced outgrowths that were significantlylonger than control dishes. In contrast, axonal outgrowth on collagentype V_SC-coated dishes was indistinguishable from that ofcontrols.

To determine whether collagen type V_SC actively inhibited axonal outgrowth, the effects of combinations of collagen type V_SCand an active substratum were examined. Composite substrata wereprepared in which different regions of the same culture dish werecoated with an outgrowth-promoting protein (e.g., collagen typeIV) or with the outgrowth-promoting protein and collagen typeV_SC. As shown in Figure 2A, ganglia placed on regions coated withcollagen type IV produced robust axonal outgrowth. Within thesame culture dish, ganglia placed on regions that also containedcollagen type V_SC failed to produce axonal outgrowth (Fig. 2B).In contrast to the effect on axonal outgrowth, migration of non-neuronalcells from the ganglia was observed on the composite substrata.Similar results were obtained when laminin was used in place ofcollagen type IV (data not shown). When collagen type V_SC wasreplaced in this assay by the active substrate collagen type I,similar levels of axonal outgrowth were observed in the singlyor doubly coated areas of the dishes (Fig. 2C,D), demonstratingthat the coating method did not inhibit axonal outgrowth. Whenganglia were placed on a collagen type IV substratum adjacentto an area that also contained collagen type V_SC, axonal outgrowthwas observed into the area lacking the latter collagen. In contrast,axons failed to extend into the region that contained collagentype V_SC, despite the presence of the outgrowth-promoting ECMprotein (Fig. 2E). Together, these results demonstrate that collagentype V_SC inhibits axonal outgrowth.

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Figure 2. Inhibition of axonal outgrowth by collagen type V_SC. Dishes were coated with collagen type IV, and then a part of each dish was also coated with collagen type V_SC (B, E) or collagen type I (D). Rat embryo dorsal root ganglia were cultured on these dishes for 4 d in serum-free medium with nerve growth factor. A, Outgrowth from a ganglion (G) placed on a region that contained only collagen type IV. Only a portion of the radial outgrowth is shown. B, Lack of outgrowth from a ganglion placed on a region that contained both collagen type IV and collagen type V_SC. C, D, Outgrowth from ganglia placed on regions containing only collagen type IV (C) or both collagen type IV and collagen type I (D). E, Ganglia placed near the border generated axonal outgrowth into areas that contained only collagen type IV (left of dashed line) but not into areas that contained both collagen type IV and collagen type V_SC (right). This image was enhanced to better display the axonal outgrowth. Scale bar, 500 µm.

Domain-specific adhesive functions of collagen type V

Collagen type V_SC contains a large collagen triple-helical domain and an N-terminal noncollagenous domain (Chernousov et al.,2000) (Fig. 3A). A series of experiments were performed to determinewhich of these domains mediated the effects of collagen type V_SCon Schwann cell migration and axonal outgrowth. The NTD of collagen $alpha$ 4(V) was expressed as a recombinant His-tagged protein. Effortsto express the collagen domain in the native triple-helical conformationwere unsuccessful. Because of the low yield of purified collagentype V from Schwann cells, the collagen domain of pepsin-digestedbovine type V collagen was used for these experiments.

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Figure 3. Effects of the $alpha$ 4(V) NTD and collagen domain of type V collagen on Schwann cell migration. A, Diagram illustrating the proposed domain structure of collagen type V_SC. B, Rat embryo dorsal root ganglia were plated on dishes coated with the indicated proteins and cultured for 4 d in serum-free medium with heregulin. Schwann cell (SC) migration was quantitated as described in Materials and Methods. Data shown are mean ± SD of measurements made on four ganglia. *Values that are significantly different from control values. C, Schwann cell migration from dorsal root ganglion explants was visualized by phase contrast microscopy. Fn, Fibronectin; IV, collagen type IV; pep V, pepsinized collagen type V; con, control dishes (uncoated plastic).

Schwann cell migration
The ability of the $alpha$ 4(V) NTD and type V collagen domain to induce Schwann cell migration was examined. Schwann cells migratedfrom dorsal root ganglion explants on dishes coated with the NTD,fibronectin, or collagen type IV (Fig. 3B,C). Migration of Schwanncells on dishes coated with pepsin-digested type V collagen wasonly slightly better than migration on control dishes. The cellsmigrating on the NTD were well spread, similar to what was observedon fibronectin or collagen type IV. In contrast, Schwann cellsmigrating on pepsin-digested collagen type V or control disheswere not well spread (Fig. 3C). These results demonstrate thatthe NTD but not the collagen domain promotes Schwann cellmigration.

Schwann cell adhesion and spreading
To investigate the Schwann cell-collagen type V interaction further, Schwann cell adhesion to ECM-coated dishes was measuredusing a dye-based assay. As shown in Figure 4A, in this short-termassay (3 hr), Schwann cells adhered to the ECM proteins collagentype IV and laminin and to the $alpha$ 4(V) NTD but failed to adhereto pepsinized type V collagen.

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Figure 4. Schwann cell adhesion and spreading on ECM proteins. A, Schwann cells were plated on dishes coated with the indicated ECM proteins and incubated in serum-free medium with heregulin. Schwann cell adhesion was measured after 3 hr using the crystal violet assay. Values shown are mean ± SD for three separate measurements. B, Schwann cells or fetal rat fibroblasts were plated on dishes coated with the indicated ECM proteins and incubated in serum-free medium with heregulin. Schwann cell spreading was monitored by phase contrast microscopy. Ln, Laminin; Fn, fibronectin; IV, collagen type IV; pep V, pepsinized collagen type V; pep V-Fb, rat embryo fibroblasts plated on pepsinized type V collagen.

Schwann cell spreading was examined after overnight incubation on ECM-coated dishes. Schwann cells spread extensively on theECM proteins laminin, fibronectin, and collagen type IV as wellas on the $alpha$ 4(V) NTD (Fig. 4B). On these adhesive substrata, Schwanncells extended thin processes that terminated in flattened lamellopodia.Although some adhesion to the collagen domain of pepsinized typeV collagen was evident in this assay, Schwann cells failed tospread or to extend processes. In contrast, fetal rat fibroblastsadhered to and spread normally on pepsinized type V collagen (Fig.4B). Together, these results support the conclusion that the primaryadhesive interaction between Schwann cells and collagen type Vis through the noncollagenous N-terminaldomain.
To explore the mechanism of Schwann cell adhesion to the NTD, receptor-specific inhibitors were used. For comparison, theeffects of these inhibitors on adhesion to collagen type IV werealso determined. The best-characterized cellular receptors forcollagen molecules are $alpha$ 1 $beta$ 1- and $alpha$ 2 $beta$ 1-integrins (Dickeson et al.,1999; Knight et al., 2000; Nykvist et al., 2000), which are expressedby Schwann cells (Hsiao et al., 1991; Milner et al., 1997). Thefunction-blocking monoclonal anti- $alpha$ 1-integrin antibody inhibitedSchwann cell adhesion to collagen type IV by ~50% (Fig. 5A). Theanti- $alpha$ 2-integrin antibody alone produced only a small inhibition,but the anti- $alpha$ 1 and anti- $alpha$ 2 antibodies together inhibited adhesionto collagen IV by ~80%. The anti- $beta$ 1-integrin antibody inhibitedSchwann cell adhesion to collagen type IV by 72%. The glycosaminoglycanheparin produced only a modest inhibition of Schwann cell adhesionto collagen IV. In contrast to these results, Schwann cell adhesionto the NTD was not significantly inhibited by the anti- $alpha$ 1- or- $alpha$ 2-integrin antibodies (Fig. 5A) and was only modestly inhibitedby the anti- $beta$ 1-integrin antibody (Fig. 5B). Schwann cell adhesionto the NTD was inhibited almost completely, however, by heparin(Fig. 5A,B). These results suggest that Schwann cells adhere tocollagen type IV primarily by an $alpha$ 1 $beta$ 1-integrin-dependent mechanismand to the NTD by a different mechanism.

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Figure 5. Inhibition of Schwann cell adhesion and spreading on collagen type IV and $alpha$ 4(V) NTD. A, B, Schwann cells were plated on dishes coated with collagen type IV or $alpha$ 4(V) NTD and incubated for 3 hr in serum-free medium with heregulin alone or in medium with the anti- $alpha$ 1-integrin antibody ( $alpha$ 1), the anti- $alpha$ 2-integrin antibody ( $alpha$ 2), both antibodies ( $alpha$ 1+2), the anti- $beta$ 1-integrin antibody ( $beta$ 1), a control hamster monoclonal antibody (con Ab), or 10 µg/ml heparin (hep). Adhesion was measured by the crystal violet assay. Values that were significantly different from controls are indicated (*p < 0.05; **p < 0.01). C, Schwann cells were plated on dishes coated with collagen type IV (col IV) or the $alpha$ 4(V) NTD and incubated for 24 hr in serum-free medium with heregulin alone or in medium with the anti- $alpha$ 1-integrin antibody ( $alpha$ 1), the anti- $alpha$ 2 integrin antibody ( $alpha$ 2), a control hamster monoclonal antibody (con Ab), or 10 µg/ml heparin (hep). Schwann cell spreading was monitored by phase contrast microscopy. The micrographs from the left and right sets of panels were from different experiments.

This conclusion was further supported by experiments that examined the effects of the inhibitors on Schwann cell spreading.As shown in Figure 5C, Schwann cell spreading on collagen typeIV was blocked by the anti- $alpha$ 1-integrin antibody, whereas the anti- $alpha$ 2integrin antibody and heparin had little effect. In contrast,Schwann cell spreading on the NTD was blocked completely by heparinbut was not affected by the anti-integrin antibodies (Fig. 5C).
In light of the inhibitory effect of collagen type V_SC on neurite outgrowth described above, an experiment was performed todetermine whether either the NTD or the collagen domain of collagentype V inhibited Schwann cell adhesion. Schwann cell adhesionto collagen type IV or laminin was measured in the absence orpresence of pepsinized collagen V or the NTD. As shown in Figure6, pepsinized type V collagen partially inhibited adhesion tocollagen type IV (35% inhibition) or laminin (36% inhibition).The presence of the NTD produced a slight increase in adhesionto dishes coated with collagen type IV or laminin. The collagendomain failed to significantly inhibit adhesion of Schwann cellsto the NTD (Fig. 6).

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Figure 6. Effect of the $alpha$ 4(V) NTD and pepsinized collagen type V on Schwann cell adhesion. Schwann cells were plated on dishes coated with the indicated ECM proteins and incubated for 3 hr in serum-free medium with heregulin. Schwann cell adhesion was measured by the crystal violet assay. IV, Collagen type IV; pep. V, pepsinized collagen type V; Ln, laminin. Values that are significantly different from collagen type IV or laminin alone are indicated (*p < 0.05; **p < 0.01). Note that the value for pepsinized collagen type V plus the NTD is not significantly different from that of the NTD alone.

Neurite outgrowth
To identify the domain of collagen type V_SC responsible for inhibition of neurite outgrowth, rat embryo dorsal root gangliawere plated on dishes coated with combinations of collagen typeIV and the NTD or pepsin-digested type V collagen. As shown inFigure 7A, in serum-free medium with nerve growth factor, theneurons produced a dense radial outgrowth on collagen type IV.Addition of the NTD to collagen type IV-coated dishes produceda moderate but statistically significant increase in axonal outgrowth.In contrast, addition of either collagen type V_SC or pepsin-digestedcollagen type V to collagen type IV-coated dishes caused essentiallycomplete inhibition of neurite outgrowth. These results demonstratethat the collagen domain is responsible for the collagen typeV_SC-dependent inhibition of neurite outgrowth. On dishes coatedwith the NTD alone, extensive neurite outgrowth was observed (Fig.7B). The NTD did not reverse the inhibitory effect of the pepsin-digestedcollagen domain on neurite outgrowth.

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Figure 7. Effects of the $alpha$ 4(V) NTD and collagen domain of type V collagen on neurite outgrowth by dorsal root ganglion neurons. A, Dorsal root ganglia were placed on dishes coated with collagen type IV and either no additional proteins (none), the NTD, collagen type V_SC (+ SC col V), or pepsinized type V collagen (+ pep col V). The ganglia were incubated in serum-free medium with nerve growth factor for 4 d. The micrographs show neurite outgrowth, as visualized by phase contrast microscopy, for representative ganglia. Neurite outgrowth was quantitated as described in Materials and Methods, and the results are displayed graphically. Values shown are mean ± SD for measurements made on four ganglia for each condition. B, Dorsal root ganglia were placed on dishes coated with pepsinized collagen type V (pep col V), the NTD, or an equimolar ratio of pepsinized collagen type V and NTD. The ganglia were incubated, and neurite outgrowth was measured as for A. SC V, Collagen type V_SC; pep-V, pepsinized collagen type V. Values that differ significantly from controls are indicated (*p < 0.05; **p < 0.005).

Collagen type V_SC promotes fasciculation of DRG axons

The results presented above demonstrate distinct adhesive activities of the noncollagenous NTD and collagen domains of collagentype V_SC. The net effect of these activities on the organizationof developing axons and Schwann cells was examined by platingdissociated rat embryo dorsal root ganglion cells, consistingof neurons and Schwann cells, on dishes coated with various substrata.As shown in Figure 8, when the cells were plated on dishes coatedwith collagen type IV (Fig. 8A,E) or collagen type I (Fig. 8B),the axons produced an apparently random pattern of outgrowth.Some of the axons were associated with Schwann cells, but manywere bereft of Schwann cell contact. Essentially identical resultswere obtained when the dissociated cells were plated on laminin(data not shown). In contrast to these results, when the cellswere plated on dishes coated with collagen type V_SC (Fig. 8C,F)the axon-Schwann cell units were organized into discrete bundles,and all the axons were closely associated with Schwann cells.This pattern of growth more closely replicated the organizationdisplayed by embryonic Schwann cells and axons in vivo.

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Figure 8. Organization of Schwann cell-axon units on ECM-coated surfaces. A-F, Dissociated rat embryo dorsal root ganglion neurons and Schwann cells were plated on dishes coated with collagen type IV (A, E), collagen type I (B), collagen type V_SC (C, F), or uncoated plastic (D). The cells were cultured in serum-free medium with nerve growth factor for 4 d. A-D, Low-power phase contrast images. E, F, Higher-power views of cultures stained with anti-neurofilament antibodies (green, stains axons), anti-S100 antibodies (red, stains Schwann cells), and 4',6-diamidino-2-phenylindole (blue, stains Schwann cell nuclei). (Note that superimposition of blue and red produce magenta.) Scale bars, 100 µm. G, H, Dorsal root ganglion explants were placed on dishes coated with laminin (G) or laminin plus collagen type V_SC (H) and cultured in serum-free medium with nerve growth factor for 4 d. Axons were photographed using phase contrast optics near the site where they emerged from the ganglia.

A similar effect was also observed with dorsal root ganglion explant cultures. Neurites produced by ganglia plated on lamininformed a dense carpet of thin processes (Fig. 8G) that includedboth naked axons as well as Schwann cell-associated axons. Onlaminin-coated dishes, collagen type V_SC produced a dose-dependentinhibition of neurite outgrowth (data not shown). When gangliawere plated on dishes coated with a laminin/collagen type V_SCratio that permitted some axons to emerge, these axons formedlarger, discrete bundles that also contained Schwann cells (Fig.8H).

This effect of collagen type V_SC was not attributable simply to a lack of strong adhesion. Dissociated dorsal root ganglioncells plated on uncoated plastic dishes (Fig. 8D) produced a patternof growth that was similar to what was seen on collagen type Ior collagen type IV but with fewer totalcells.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The peripheral nervous system contains a biochemically complex ECM. Contact with the ECM regulates many aspects of nerve development,including axonal migration, and Schwann cell proliferation anddifferentiation (Chernousov and Carey, 2000). Previously, we reportedthe purification, characterization, and cloning of a novel collagentype V chain, $alpha$ 4(V), which is secreted by Schwann cells and bindswith high affinity to heparin-like glycosaminoglycans (Chernousovet al., 2000). This polypeptide, which we called p200, was identifiedinitially on the basis of its binding to the heparan sulfate proteoglycansyndecan 3 (Chernousov et al., 1996). The restricted expressionof $alpha$ 4(V) by Schwann cells during the late embryonic and earlypostnatal periods (Chernousov et al., 1999) suggested that Schwanncell type V collagen played a role in nervedevelopment.

Collagen type V_SC appears to have a dual function with respect to Schwann cell and axonal adhesion and migration. This collagenpromotes the migration of premyelinating Schwann cells in culturebut actively inhibits outgrowth of axons from rat embryo sensoryneurons. Collagen type V_SC blocks the neurite outgrowth-promotingactivities of other ECM proteins and prevents the growth of axonsinto areas where the collagen is present. These activities aremediated by different structural domains of the collagen. Thenoncollagen NTD promotes Schwann cell adhesion and migration,whereas the triple-helical domain inhibits neurite outgrowth.The latter domain was also poorly adhesive for Schwanncells.

The use of pepsinized placental type V collagen in these experiments was dictated by our inability to obtain sufficient quantitiesof either pepsinized collagen type V_SC from Schwann cells or recombinantcollagen domain trimers. Based on biochemical and expression data(Chernousov et al., 1999, 2000), the difference between placentaltype V collagen and Schwann cell type V collagen is the presenceof the $alpha$ 3 subunit in placental collagen and the $alpha$ 4 subunit inSchwann cell collagen. Pepsin digestion of these collagens removesthe noncollagenous N- and C-terminal domains, leaving the protease-resistanttriple-helical domain. The regions of greatest sequence divergencebetween the $alpha$ 3 and $alpha$ 4 chains are the noncollagenous domains, especiallythe N-terminal domains (Chernousov et al., 2000). The triple-helicaldomains are highly homologous, with 88% amino acid identity. Thisstructural similarity is supported by our finding that pepsinizedplacental type V collagen inhibits neurite outgrowth from dorsalroot ganglion neurons in a manner that is indistinguishable fromcollagen type V_SC. This result strongly suggests that inhibitionof neurite outgrowth is caused by the triple-helical collagendomain.

Our results suggest that collagen type V_SC is a member of the class of inhibitory axonal guidance cues that also includesthe netrin and ephrin families of proteins (Tessier-Lavigne andGoodman, 1996). This is in contrast to the activities of manyECM proteins, including most collagens, which promote outgrowthof axons from cultured neurons (McGarvey et al., 1984; Hynes andLander, 1992; Anton et al., 1994; Milner et al., 1997). Collagentype V_SC is not the only ECM protein with such inhibitory activity.Chondroitin sulfate proteoglycans isolated from the nervous system(Brittis et al., 1995), tenascin (Gotz et al., 1996), laminin11 (Patton et al., 1997), and agrin (Campagna et al., 1995) alsoinhibit axonal outgrowth from different types of neurons. Thisis the first report of such an activity by a fibril-forming collagenmolecule.

The mechanism by which collagen type V_SC inhibits neurite outgrowth is not known. The fact that inhibition of neurite outgrowthis observed in the presence of an outgrowth-promoting proteinsuggests that this is an active process. The outgrowth-inhibitingactivity resides in the triple-helical collagen domain. The triple-helicaldomains of type V collagens are similar in structure to thoseof other fibril-forming collagens, such as collagen type I (Prockopand Kivirikko, 1995). The best-characterized collagen receptorsare $alpha$ 1 $beta$ 1- and $alpha$ 2 $beta$ 1-integrins (Dickeson et al., 1999; Knight etal., 2000). Growth of axons from sympathetic neurons on collagentype IV has been shown to require $alpha$ 1 $beta$ 1-integrin (Lein et al.,1991). Rat embryo dorsal root ganglion neurons express these integrins.Function-blocking anti- $alpha$ 1- and $alpha$ 2-integrin antibodies inhibitneurite outgrowth by these neurons on collagen type IV (R. C.Stahl, M. A. Chernousov, and D. J. Carey, unpublished observations). $alpha$ 1 $beta$ 1- and $alpha$ 2 $beta$ 1-integrins also bind collagen type V (Nykvist etal., 2000). The different consequences of interaction with collagentype IV and collagen type V are difficult to reconcile with theseobservations.

A possible mechanism to explain these findings is that the collagen domain binds other nonintegrin receptors that generateoutgrowth-inhibitory signals. The nature of such receptors isunknown, but several candidates can be considered. Most collagens,including type V collagens, bind heparin-like glycosaminoglycans(San Antonio et al., 1994). A heparan sulfate binding site hasbeen localized to the triple-helical domain of collagen type V(Delacoux et al., 1998). Syndecan transmembrane proteoglycans,which can bind the triple-helical domains of heparin-binding collagens(Sanderson et al., 1994), are present in the growth cones of atleast some migrating axons (Raulo et al., 1994; Kinnunen et al.,1996). Syndecans have been shown to modulate kinase activity (Ohet al., 1997; Horowitz and Simons, 1998) and cytoskeletal organization(Carey et al., 1994; Granes et al., 1999) in a variety of cells.Evidence against a role for heparan sulfate proteoglycans comesfrom the fact that removal of the noncollagen NTD, which containsthe high-affinity heparin binding site of the $alpha$ 4(V) chain, hasno apparent effect on neurite outgrowth inhibition. The collagendomain does influence syndecan-3 binding by $alpha$ 4(V), however, becauseits removal by collagenase treatment lowers the apparent bindingaffinity for the proteoglycan (Chernousov et al., 1996). Othercollagen-binding receptors, such as the discoidin domain receptors,could also be involved in transducing the outgrowth inhibitorysignal. These transmembrane receptors contain cytoplasmic tyrosinekinase domains that are activated by collagen binding (Vogel etal., 1997). Discoidin domain receptor 1 has been shown to be involvedin modulating axon extension by cerebellar granule neurons (Bhattet al., 2000). These mechanisms are not mutually exclusive. Inhibitionof outgrowth could result from the combinatorial activation ofintegrin- and non-integrin-dependent receptor systems. Such acooperative mechanism has been demonstrated in the regulationof focal adhesion assembly by fibroblasts (Saoncella et al., 1999;Couchman and Woods, 2000).

Collagen type V_SC promotes migration of Schwann cells from dorsal root ganglion explants. Paradoxically, the type V collagendomain provides a poor substratum for Schwann cell adhesion. Thisfinding is also somewhat surprising, given the expression of functionalcollagen-binding integrins by Schwann cells. The $alpha$ 4(V) NTD, incontrast, avidly promotes Schwann cell adhesion and migration.Schwann cell adhesion to $alpha$ 4(V) does not require assembly intocollagen trimers (Chernousov et al., 1996), consistent with theimportance of the NTD in this process. The occurrence of a poorlyadhesive protein that promotes cell migration has been describedpreviously. For example, laminin and merosin are antiadhesivefor embryonic olfactory epithelial neurons but stimulate theirmigration in cell culture (Calof and Lander, 1991).

Schwann cell adhesion and spreading on the NTD appear to be mediated by a heparan sulfate-dependent mechanism, suggestingthat membrane heparan sulfate proteoglycans are the cellular receptorsthat bind this domain. The role of heparin-like glycosaminoglycansis consistent with the biochemical properties of collagen typeV_SC. The binding affinity of $alpha$ 4(V) for heparin-like glycosaminoglycansis significantly higher than the affinity of the closely related $alpha$ 1(V) chain (Chernousov et al., 2000). The high-affinity heparansulfate binding site is located in the NTD. $alpha$ 4(V)-Collagen bindswith high affinity to the transmembrane heparan sulfate proteoglycansyndecan-3 (Chernousov et al., 1996). $alpha$ 4(V) and syndecan-3 aresynthesized by Schwann cells during the same developmental periods.Both proteins are highly expressed in peripheral nerves relativeto levels in surrounding tissue (Carey et al., 1992, 1997; Chernousovet al., 1999). These findings suggest that syndecan-3 might bethe Schwann cell $alpha$ 4(V)receptor.

These findings suggest a novel function for collagen type V during development. Early in nerve development, peripheral axonsare organized into bundles that are bounded by Schwann cells andtheir processes (Webster et al., 1973). Later-developing axonsuse these bundles as tracks to direct their migration. Fasciculationof axons is produced by a combination of positive adhesive interactionsamong axons and repulsive signals that "hem in" the axons (Tessier-Lavigneand Goodman, 1996). As development proceeds, the axon bundlesbecome progressively subdivided by Schwann cell processes. Electronmicroscopic analysis of embryonic nerves has shown that collagenfibrils are distributed around the periphery of the axon-Schwanncell bundles (Webster et al., 1973). The presence of collagenmolecules that inhibit axonal migration would restrict the movementof axons away from the nerve bundles and promote fasciculation.At the same time, the NTD of collagen type V_SC would promote Schwanncell spreading and migration, facilitating Schwann cell ensheathmentof axons and the movement of Schwann cells along the growing nervefiber bundles. This model is supported by the effects of collagentype V_SC on the organization of sensory axons and Schwann cellsinculture.

  FOOTNOTES

Received Feb. 9, 2001; revised May 7, 2001; accepted May 24, 2001.

This work was supported by National Institutes of Health Grant NS21925. We thank Katrina Rothblum for help with expressionof the recombinant $alpha$ 4(V) N-terminal domain and Dr. Victor Kotelianskyfor the generous gift of function blocking anti-integrinantibodies.
Correspondence should be addressed to Dr. David J. Carey, Sigfried and Janet Weis Center for Research, 100 North Academy Avenue,Danville, PA 17822-2613. E-mail: djcarey{at}geisinger.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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