Deposition of the NG2 Proteoglycan at Nodes of Ranvier in the Peripheral Nervous System

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The Journal of Neuroscience, October 15, 2001, 21(20):8119-8128

Deposition of the NG2 Proteoglycan at Nodes of Ranvier in the Peripheral Nervous System
Sandra Martin, Angela K. Levine, Zhi Jiang Chen, Yvonne Ughrin, and Joel M. Levine
Department of Neurobiology and Behavior, State University of New York at Stony Brook, Stony Brook, New York 11794

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The node of Ranvier is a complex macromolecular assembly of ion channels and other proteins that is specialized for the rapidpropagation of the action potential. A full understanding of theprocesses responsible for the assembly and maintenance of thenode requires first the identification and characterization ofthe proteins found there. Here we show that NG2, a structurallyunique chondroitin sulfate proteoglycan, is a molecular componentof the node of Ranvier in the peripheral nervous system. In adultsciatic nerve, NG2 is (1) associated with thin, elongated fibroblast-likecells, (2) on some but not all basal laminae, and (3) at nodesof Ranvier. At the nodes, NG2 is restricted to the nodal gap andis absent from the paranodal or juxtaparanodal region. In dissociatedcell cultures of adult sciatic nerve, perineurial fibroblastsbut not Schwann cells express NG2 on their surfaces. Approximately45% of the total NG2 in peripheral nerves is in a soluble, ratherthan particulate, subcellular compartment. NG2 is also presentin membrane fractions that also contain high levels of voltage-dependentsodium channels, caspr, and neuron-glia related cell adhesionmolecule. These medium-density membranes likely correspond tothe nodal and paranodal region of the axon-Schwann cell unit.These results suggest a model in which perineurial fibroblastssecrete or shed NG2, which subsequently associates with nodesof Ranvier. The growth-inhibitory and anti-adhesive propertiesof NG2 may limit the lateral extension of myelinating Schwanncells as nodes mature. NG2 may also participate in the barrierfunctions of the perineurial linings of thenerve.

Key words: node of Ranvier; perineurium; nerve-blood barrier; chondroitin sulfate proteoglycan; NG2; extracellular matrix

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Many axons of the peripheral nervous system use a saltatory mode of action potential conduction in which current flow is restrictedto small gaps in the myelin sheath known as nodes of Ranvier.This adaptation allows for faster conduction of the action potentialwithout a corresponding increase in axon diameter. The node ofRanvier is a complex macromolecular assembly of the voltage-dependention channels necessary for the generation of the action potentialand of other proteins whose main functions appear to be organizingand maintaining the specialized and distinct membranous subdomainsof the nodal region (for review, see Vabnick and Shrager, 1998;Arroyo and Scherer, 2000; Peles and Salzer, 2000; Rasband andSchrager, 2000). For example, the type 6 isoform of the voltage-dependentsodium channels is found at extremely high density at nodes ofRanvier in the rat peripheral nervous system (Caldwell et al.,2000). Interactions between the cytoplasmic domain of sodium channelsubunits and ankyrin G may stabilize these high-density clustersin adult nerve (Kordeli et al., 1995; Malhotra et al., 2000).Similarly, voltage-dependent potassium channels of the Shakerfamily are excluded from the nodal gap but are present in thejuxtaparanodal region of the axon (Wang et al., 1993; Mi et al.,1995). The septate junctions between myelinating glial cells andthe axolemma may function to restrict the distribution of channels(Rosenbluth, 1976). The axonal proteins caspr and contactin arelikely components of these junctions, but their glial bindingpartners remain unknown (Einheber et al., 1997; Menegoz et al.,1997; Rios et al., 2000). Other proteins enriched at nodes ofRanvier include cell adhesion and extracellular matrix molecules(Rieger et al., 1986; Martini et al., 1990; Davis et al., 1996).Given the functional importance of the node of Ranvier and thedisastrous consequences of demyelinating diseases that disruptnodal structure, it is important to identify molecular componentsof the node and to understand their functionsthere.

Proteoglycans are major constituents of peripheral nerves and have been implicated in the regulation of axon growth and regeneration(Fitch and Silver, 1997). Because proteoglycans can interact withboth extracellular matrix molecules and cell surface molecules,the deposition of these multifunctional molecules at nodes mayhelp organize these complexstructures.

To further our understanding of the functions of proteoglycans in the peripheral nervous system, we have examined the distributionof the NG2 chondroitin sulfate proteoglycan (CSPG) in adult ratsciatic nerve. NG2 is a well characterized integral membrane proteoglycanfound principally on the surfaces of oligodendrocyte precursorcells (OPCs) in the CNS (Levine and Nishiyama, 1996). OPCs sendprocesses to nodes of Ranvier in the CNS (Butt et al., 1999),although the significance of these cellular processes is not known.Here we show that NG2 is present in adult rat sciatic nerve. Immunofluorescence,cell culture experiments, and biochemical analysis suggest a modelin which NG2 is synthesized and secreted by perineurial fibroblastsand subsequently associates with nodes of Ranvier and severalbasal laminae. By virtue of its anti-adhesive and growth-inhibitingproperties (Dou and Levine, 1994; Fidler et al., 1999), NG2 atnodes of Ranvier may function to limit the lateral extension ofthe Schwann cell during the late stages of myelination and ofnodematuration.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Immunofluorescence. Adult rats were anesthetized with ketamine-xylazine and decapitated, and the sciatic nerve was rapidlyremoved. After a brief rinse in ice-cold PBS, whole nerves werefixed in freshly prepared 4% paraformaldehyde in 0.1 M phosphatebuffer, pH 7.4, at 4°C for not more than 1 hr and then cryoprotectedby immersion in 30% sucrose and 0.1 M phosphate buffer. Ten micrometersections were cut at a longitudinal or frontal plane using acryostat.

For the detection of specific antigens, the following antibodies were used: NG2, rabbit anti-NG2 and mouse monoclonal antibodyD31.10 (Levine and Card, 1987); myelin basic protein, monoclonalantibody 382 (Chemicon, Temecula, CA); p75 low-affinity neurotrophinreceptor, antibody 1554 (Chemicon); thy1.1 antigen, monoclonalantibody 1406 (Chemicon); ankyrin G, monoclonal antibody 4G3F8(Zymed, San Francisco, CA); S100 $beta$ protein, monoclonal antibodySH-B1 (Sigma, St. Louis, MO); neuron-glia related cell adhesionmolecule (NrCaM), rabbit antisera 837 (M. Grumet, Rutgers StateUniversity of New Jersey, Piscataway, NJ); all known mammaliansodium channel isoforms, monoclonal antibody K58/35.1 (Rasbandet al., 1999; a gift from J. Trimmer, State University of NewYork, Stony Brook, NY); and caspr, rabbit anti-caspr (J. Trimmer).Antibodies against laminin B2 chain (monoclonal antibody D18)and s-laminin (antibody C4) were obtained from the DevelopmentalStudies Hybridoma Bank (Iowa City, IA). Immunofluorescence stainingmethods were similar to those described previously (Levine andCard, 1987; Levine et al., 1993). Nuclei were visualized afterincubating the sections in Hoechst 33258 (0.5 µg/ml; Sigma). Insingle- and double-labeled fluorescence studies, Cy3-conjugatedgoat anti-mouse (Jackson ImmunoResearch, West Grove, PA) and FITC-conjugatedgoat anti-rabbit (SBTA; Fisher Scientific, Pittsburgh, PA) antibodieswere used. In the absence of the primary antibodies, no stainingwas observed with these fluorochrome-conjugated reagents. Sectionsand cultures were examined either with a Zeiss (Thornwood, NY)Axiovert microscope equipped with phase contrast and fluorescenceoptics or with a Zeiss Axioplan microscope equipped with fluorescenceand Nomarski optics. Images were taken using either film or adigital camera. In some of the figures, the images were pseudocoloredand digitally merged using Metamorph image-processing software(Universal Imaging Corp., West Chester, PA). Figure plates wereprepared using Adobe Photoshop (Abode Systems, Inc., MountainView,CA).

Teased sciatic nerve fibers were prepared as described previously (Rasband et al., 1998) and immunofluorescently stained asdescribedabove.

Cell culture. Continuous cultures of highly purified Schwann cells were established according to the method of Brockes etal. (1979) and maintained in DMEM (Fisher Scientific) containing10% fetal calf serum, 2.5 µM forskolin (Sigma), and 20 ng/ml recombinanthuman heregulin- $beta$ 1 (amino acids 176-246; R & D Systems, Minneapolis,MN). To prepare dissociated cultures of adult rat sciatic nerve,animals were killed with CO₂, and the sciatic nerves removed,cleaned of fat and connective tissue, minced, and then incubatedfor 45 min at 37°C in solutions containing 0.25% trypsin (WorthingtonBiochemicals, Freehold, NJ) and 0.2% collagenase (Sigma). Thetissue was washed in serum-containing media and triturated bypassage through a series of flame-narrowed Pasteur pipettes. Thecells were plated onto poly-L-lysine-coated coverslips in DMEMcontaining 10% fetal calf serum. Cultures of newborn rat dorsalroot ganglia were established as described previously (Dou andLevine, 1994) except that the medium did not contain nerve growthfactor. Immunofluorescence staining of living cells was performedas described previously (Levine et al., 1993). All proceduresusing animals were approved by the university Institutional AnimalCare and UseCommittee.

Biochemical methods. SDS-gel electrophoresis and Western blotting were performed as described previously (Levine et al., 1998)using ECL reagents from Amersham Pharmacia Biotech (ArlingtonHeights, IL). For densitometric measurements, the x-ray filmswere scanned using a flat-bed scanner (Microtek, Torrance, CA)and quantitated using Metamorph software (Universal Imaging Corp.).To prepare total soluble and particulate fractions of adult sciaticnerve, frozen nerves (Pel-Freeze Biologicals, Rogers, AR) werehomogenized in 0.01 M Tris, pH 8.0, 1 mM EDTA, 2 mM PMSF, 0.1mM 1,10-phenanthroline, and 1 µg/ml leupeptin using a Polytron(Brinkmann Instruments, Westbury, NY) and centrifuged at 120,000× g at 4°C in an Optima TLX ultracentrifuge (Beckman Instruments,Palo Alto, CA). The pellet was rehomogenized in 1% SDS, 10 mMTris, pH 8.0, and 1 mM EDTA and boiled for 3-5 min. Any remaininginsoluble material was removed by centrifugation. Soluble andparticulate extracts of adult rat brainstem white matter wereprepared in an identical manner. In additional experiments, sciaticnerve and brainstem white matter was homogenized in solutionsof 1% NP-40, 0.15 M NaCl, 10 mM Tris, pH 8.0, and protease inhibitors.After 15 min on ice, the homogenate was centrifuged at 14,000× g for 10 min, and the supernatant was removed and kept. Extractswere digested with protease-free chondroitinase ABC (SeikagakuAmerica Inc.) as described previously (Dou and Levine, 1994).Protein was determined using a dye-binding assay (Bio-Rad, Hercules,CA). All biochemical reagents were from Sigma unless notedotherwise.

Subcellular fractionation. One hundred frozen rat sciatic nerves were used per fractionation. The nerves were homogenizedin 40 ml of 12% sucrose in 10 mM phosphate, pH 7.35, containing1 mM EDTA, 2 mM PMSF, 0.1 mM 1,10-phenanthroline, and 1 µg/mlleupeptin using a Polytron. Homogenization was complete when noconnective tissue was visible. The homogenate was layered overa discontinuous gradient of 20 and 45% sucrose and centrifugedfor 16 hr at 4°C and at 26,000 rpm using a Beckman SW27 rotor.The 20/45% sucrose interface was collected, diluted in 10 mM phosphatebuffer, and centrifuged again at 35,000 rpm (100,000 × g) for40 min using a Beckman 42 rotor. The 12/20% interface was alsocollected and concentrated as described above. We refer to thismaterial herein as PNS myelin (see Fig. 7). The resulting pelletwas resuspended in 12% buffered sucrose and homogenized usinga hand-held Dounce homogenizer, eight passes each of A and B pestles.The homogenate was layered over a second discontinuous gradientof 22, 27, and 35% sucrose. After overnight centrifugation at26,000 rpm in a Beckman SW27 rotor, all fractions including thepellet were retained. All fractions were concentrated by centrifugationat 100,000 × g and resuspended in 1% SDS, 10 mM Tris, pH 8.0,and 1 mM EDTA. One-fourth of the SDS extracts was denatured at37°C, whereas the remainder was denatured by boiling. The light,medium, and heavy membrane fractions correspond to the 12/22%interface, the 22/27% interface, and the 27/35% interface,respectively.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We used immunofluorescence microscopy with specific antibodies to examine the disposition of NG2 in longitudinal sectionsof adult rat sciatic nerve. As shown in Figure 1A, NG2-like immunoreactivitywas associated with several different structures within the nerve.First, immunoreactivity was found at the lateral margins of thenerve, most likely associated with the basal lamina of the epineurialand perineurial sheaths (Fig. 1A, small-headed arrow). Second,thin linear elements within the nerve bound the anti-NG2 antibodies.Some of these elements were intensely stained, whereas othersappeared to bind the antibodies less robustly (Fig. 1A, wide-headedarrows). Third, NG2 immunoreactivity was found on small punctaand short, dash-like structures that often were oriented perpendicularto the longitudinal axis of the nerve (Fig. 1A, narrow arrows).Fourth, NG2 was found on the blood vessel-like structures lyingwithin the central regions of the nerve (Fig. 1A, wide arrowhead).At higher magnification (Fig. 1B,D), individual NG2-positive profilesappeared as long, thin cells, a characteristic of perineurialfibroblasts in peripheral nerve (Peltonen et al., 1987). Eachof these thin, elongated NG2-positive profiles contained a Hoechst33258-positive nucleus, demonstrating that they are cells ratherthan aggregates of NG2-containing extracellular matrix (Fig. 1D,E).These elongated cellular profiles were stained also with an anti-vimentinantibody, as were most of the NG2-negative Schwann cells (datanot shown).

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Figure 1. Localization of NG2 in adult sciatic nerve. NG2 was localized in cryostat sections of adult sciatic nerve prepared as described in Materials and Methods. A, Low-power overview of NG2 immunoreactivity in adult nerve. NG2 is associated with the extracellular matrix surrounding the nerve (small-headed arrow), linear cellular elements within the nerve (wide-headed arrow), large blood vessels (large arrowhead), and numerous small puncta (small thin arrows). Scale bar, 100 µm. B, C, High-power views of NG2-positive cells from adult sciatic nerve. These cells, which are stained at their plasma membrane with the anti-NG2 antibodies, have elongated, thin processes that lie between the nerve fibers. D, E, Hoechst 33258-stained nuclei of the cells shown in B and C. Scale bar (E), 50 µm.

To further characterize the NG2-positive cellular profiles, we compared the distribution of NG2 with that of marker antigensspecific for Schwann cells using double-label immunofluorescenceof the same tissue sections. Figure 2 shows that there was verylittle overlap in the distribution of NG2 and of myelin-associatedglycoprotein (MAG) (Fig. 2A-C) and myelin basic protein (MBP)(Fig. 2D-F), two markers for myelinating Schwann cells. When theimages of the two different fluorochromes were colorized and digitallymerged, the NG2-positive profiles (Fig. 2, arrows) appeared tofill the space between the myelinating Schwann cells. Althoughthe myelin sheath did not bind the anti-NG2 antibodies, a thinrim of light staining was observed along the external surfaceof the Schwann cell. This rim of anti-NG2 immunoreactivity isassociated with either the Schwann cell membrane or the basallamina that surrounds the Schwann cell-axon unit. We also useda monoclonal antibody against the S100 $beta$ protein as a general markerfor Schwann cells (Jessen and Mirsky, 1991). As shown in Figure2, E-G, there was again little or no overlap between the distributionof NG2 and that of S100 $beta$ in adult sciatic nerve. Last, we comparedthe distribution of NG2 with that of the low-affinity neurotrophinreceptor p75 (Fig. 2J-L). The anti-p75 antibody only lightly stainedthe Schwann cell cytoplasm and myelin but was enriched in theSchwann cell microvilli that abut the node of Ranvier (also seeFig. 5). None of these structures expressed high levels of NG2.Nevertheless, there was a low level of anti-p75 staining associatedwith the NG2-positive cells. This low level of double stainingwas not unexpected, because perineurial fibroblasts and numerousother cell types are reported to express p75 (Bothwell, 1991;Bradley et al., 1998). Because neither Schwann cells nor the myelinthey make contains the NG2 proteoglycan, these data suggest thatthe major source of NG2 in adult peripheral nerve is the perineurialfibroblasts. Because these single- and double-label studies onlyused adult nerve, we cannot rule out the possibility that othercell types produce NG2 at earlier developmental stages (Schneideret al., 2001).

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Figure 2. Comparison of the localization of NG2, MBP, MAG, S100 $beta$ , and p75 in adult sciatic nerve. Tissue sections were stained as described in Materials and Methods. Each horizontal row shows staining with the individual antibodies and a colorized and digitally merged image showing both fluorochromes. A, Monoclonal anti-NG2; B, rabbit anti-MAG; C, A and B colorized and merged. D, Rabbit anti-NG2; E, mouse anti-MBP; F, D and E colorized and merged. G, Rabbit anti-NG2; H, mouse anti S100 $beta$ ; I, G and H colorized and merged. J, Mouse anti-NG2; K, rabbit anti-p75; L, J and K colorized and merged. Neither the Schwann cells nor the myelin they make are stained with the anti-NG2 antibodies. Scale bar, 20 µm.

Because cellular identification is often difficult in intact tissue, we prepared cultures of adult sciatic nerve and stainedthe cells with cell type-specific marker antibodies after 48 hrin dissociated cell culture. As shown in Figure 3, A and D, theanti-NG2 antibodies bound to a population of large cells thatwere well spread on the substrate. In contrast, anti-p75 antibodiesrecognized thin cells with a spindle-shaped appearance (Fig. 3B,G).There was no overlap in the staining obtained with these two antibodies.The NG2-positive cells also bound antibodies against the thy1.1antigen, a marker for fibroblasts and thymocytes, as well as othercell types (Brockes et al., 1979). The p75-positive Schwann cellsdid not bind the anti-thy1.1 antibodies. In additional experiments,the large NG2-positive cells were not stained with monoclonalantibody 04, which did stain the spindle-shaped Schwann cells(data not shown). Similar results were obtained when we stainedcultures of newborn rat dorsal root ganglia that were grown for8 d under conditions that foster the proliferation of non-neuronalcells. The anti-NG2 antibodies stained large, well spread cellsthat were not labeled with the anti-p75 antibodies (data not shown).Highly purified Schwann cells maintained in continuous culturein the presence of neuregulin and forskolin also did not bindthe anti-NG2 antibodies (data not shown). Together these double-labelfluorescence in vivo and in vitro studies show that NG2 is notexpressed by myelinating or nonmyelinating Schwann cells, butit is present on fibroblastic cells within the adult peripheralnerve.

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Figure 3. Lack of colocalization of NG2 and p75 in dissociated cultures of adult rat sciatic nerve. Dissociated cell cultures of rat sciatic nerve were prepared and immunofluorescently stained as described in Materials and Methods. A, Anti-NG2 stain; B, anti-p75 stain. The large, flat NG2-positive cells are p75-negative, whereas the spindle-shaped cells are p75-positive. C, Phase-contrast view of the cultures. D, Anti-NG2 stain; E, anti-thy1.1 stain; F, phase contrast view. The NG2-positive cells are also stained with the anti-Thy1.1 antibodies. G, Anti-p75 stain; H, anti-thy1.1 stain; I, phase contrast view of the culture. The p75-positive Schwann cells do not bind the anti-thy1.1 antibodies. The arrows in C, F, and I point to spindle-shaped Schwann cells. Scale bar, 20 µm.

Most cellular elements within the mature peripheral nerve are surrounded by a basal lamina (Rutka et al., 1988). IndividualSchwann cell-axon units are surrounded by an endoneurial basallamina that contains laminin B1 and B2 chains, whereas nerve bundlesand the entire nerve itself are surrounded by a perineurial basallamina that contains S-laminin (Sanes et al., 1990). Given theapparent association of NG2 with some of these basal laminae (Fig.1), we compared the distribution of NG2 with that of the lamininB2 chain to identify those basal laminae that are enriched inNG2. As shown in Figure 4B, high levels of anti-laminin B2 immunoreactivitywere found in the endoneurial basal lamina tubes surrounding theSchwann cell-axon units. These structures contain only very lowlevels of anti-NG2 immunoreactivity, which was often observedas punctate aggregates of immunoreactivity (Fig. 4, A,C). Theendoneural basal lamina extends into the nodal gap, which wasmore heavily stained with the anti-NG2 antibodies (see below).The NG2-positive cellular profiles were costained with the anti-lamininB2 chain antibodies, most likely a reflection of their fibroblasticnature (Fig. 4, arrows). NG2 immunoreactivity also was found onthe perineurial basal lamina (Fig. 1, small-headed arrow), a structurethat was also stained with the anti-S-laminin antibodies (datanot shown). The epineurial and perineurial basal laminae constitutethe nerve-blood barrier, and the specific association of NG2 withthese structures suggests that it may participate in these barrierfunctions.

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Figure 4. Comparison of the localization of NG2 with that of the endoneurial extracellular matrix. Sections of adult sciatic nerve were immunofluorescently stained as described in Materials and Methods. A, Anti-NG2 stain; B, anti-laminin B2 stain; C, colorized and digitally merged image of A and B. The endoneurial matrix is heavily stained with the anti-laminin B2 antibodies but only contains discontinuous and punctate deposits of anti-NG2 immunoreactivity. Scale bar, 10 µm.

The small puncta and dash-like structures within the sciatic nerve that were stained with anti-NG2 antibodies strongly resemblenodes of Ranvier. We therefore compared the distribution of NG2with that of several different proteins known to be specificallyassociated with nodes of Ranvier. As shown in Figure 5, A andB, NG2 immunoreactivity is coincident with the staining obtainedwith a monoclonal antibody that recognizes the cytoplasmic domainsof all known mammalian sodium channel isoforms (Rasband et al.,1999). In Figure 5, A and B, it appears that NG2 is slightly outof alignment with the anti-sodium channel staining. Because NG2is likely extracellular, and the epitope recognized on the sodiumchannel is intracellular, such misalignment would be expectedif the plane of section were not exactly parallel to the longitudinalaxis of the nerve. A similar close opposition and misalignmentwere observed (Fig. 5C,D) when sections were stained with antibodiesagainst NG2 and ankyrin G 480/270, an isoform of ankyrin specificallyfound on the cytoplasmic surface of the nodal axolemma (Kordeliet al., 1995). NG2 immunoreactivity colocalized closely with stainingfor NrCaM (Fig. 5E,F), a member of the immunoglobulin superfamilyof cell adhesion molecules that is specifically found at nodesof Ranvier in the PNS (Davis et al., 1996). In contrast to thecolocalization of NG2 with these three nodal proteins, NG2 wasnot coincident with caspr, a marker for the paranodal region (Einheberet al., 1997). Rather, NG2 immunoreactivity appeared to fill thegap between the two closely opposed bands of caspr staining (Fig.5G,H). This filling of the nodal gap by NG2 was more apparentwhen sections were stained with the anti-p75 antibodies, whichheavily stain the Schwann cell microvilli (Fig. 5I,J). The anti-NG2staining of the node of Ranvier persisted in teased sciatic nervepreparations (Fig. 6), demonstrating that NG2 is bound to thenode, either directly or indirectly, and that the staining patternobserved in intact nerve preparations is not simply a consequenceof the three-dimensional structure of the nerve. Figure 6 alsoshows again that the p75-positive Schwann cells do not bind theanti-NG2 antibodies (Fig. 6E,F, arrows). Thus, NG2 is presentat the node of Ranvier, where it colocalizes with other knowncomponents of the node.

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Figure 5. NG2 is found at nodes of Ranvier. Sections of adult sciatic nerve were stained with the indicated antibodies and digitally merged as described in Materials and Methods. A, B, Rabbit anti-NG2 (green) and mouse anti-sodium channel (red). C, D, Rabbit anti-NG2 (green) and mouse anti-ankyrin G (red). E, F, Mouse anti-NG2 (red) and rabbit anti-NrCaM (green). G, H, Mouse anti-NG2 (red) and rabbit anti-caspr (green). I, J, Mouse anti-NG2 (red) and rabbit anti-p75 (green). NG2 immunoreactivity colocalizes with that of the sodium channel, ankyrin G, and NrCaM but is not found in the paranodal and juxtaparanodal regions that contain caspr. NG2 is also not associated with the Schwann cell microvilli that stain heavily for p75. Scale bar, 5 µm.

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Figure 6. NG2 is localized at nodes of Ranvier in teased sciatic nerve fibers. Teased sciatic nerve fibers were stained with the indicated antibodies. A, Rabbit anti-NG2; B, mouse anti-sodium channel; C, phase contrast; D, mouse anti-NG2; E, rabbit anti-p75; F, phase contrast. NG2 (arrowhead) is concentrated at nodes of Ranvier, which also stain with the anti-sodium channel and anti-p75 antibodies. The arrows in E and F point to a p75-positive spindle-shaped cell that is NG2-negative. Scale bar, 10 µm.

The primary structure of NG2 predicts a transmembrane glycoprotein with covalently attached glycosaminoglycan (GAG) chains(Nishiyama et al., 1991). Previous studies of NG2 in the CNS haveindicated that most of the NG2 present is localized to membranes(Levine and Card, 1987; Butt et al., 1999; Ong and Levine, 1999).In contrast, the data above show that NG2 can be a component ofextracellular structures such as the epineurial and perineurialbasal lamina. This extracellular compartmentalization is consistentwith the ability of some transfected cell lines to secrete orshed a truncated form of NG2 into the medium and with the abilityof NG2 to bind to extracellular matrix molecules (Nishiyama etal., 1995; Burg et al., 1996). To assess whether some of the NG2in peripheral nerve is in a nonmembranous subcellular compartment,we divided homogenates of sciatic nerve and brainstem white matterinto total soluble and particulate fractions and then assayedthese fractions for NG2 using immunoblotting. Figure 7A, top panel,shows that considerable amounts of NG2 from sciatic nerve canbe extracted into aqueous buffers, whereas lesser amounts of NG2from CNS white mater partition into the soluble fraction. Whengels such as those shown were analyzed by densitometry, the ratioof soluble to particulate NG2 in sciatic nerve was 0.91 (n = 3);in brainstem white matter, the ratio was 0.26 (n = 2). In theseimmunoblots, NG2 appears as single polypeptide with a molecularweight of 240,000; a high molecular weight smear that is moretypical of the electrophoretic mobility of proteoglycans was notdetected in extracts of sciatic nerve, although such a smear couldbe seen in extracts of brainstem white matter after overexposureof the x-ray film (data not shown). Although this suggests thatNG2 may exist in a nonproteoglycan form, it is possible that intactproteoglycans either transfer poorly to nitrocellulose membranesor are not well detected with our antibodies. Therefore, to determinewhether peripheral nerve NG2 contains chondroitin sulfate GAGchains, we prepared total nonionic detergent extracts of sciaticnerve and brainstem white matter and treated the extracts withprotease-free chondroitinase ABC before electrophoresis and immunoblotting.This procedure removes most of the GAG chains, causing increasedintensity of the core protein band on immunoblots (Stallcup etal., 1983). Figure 7A, bottom panel, shows that when a total extractof sciatic nerve was treated with chondroitinase ABC, there wasa 165% increase in the intensity of the core protein bands. Similartreatment of a nonionic detergent extract of brainstem white matter,however, resulted in a 335% increase in the intensity of the coreprotein band. These data suggest that in peripheral nerve, approximatelyhalf of the NG2 present is in a soluble as opposed to a membrane-boundcompartment, and NG2 is not as heavily decorated with chondroitinsulfate GAG chains as are the forms of NG2 found in the CNS.

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Figure 7. Biochemical identification of NG2 in sciatic nerve. A, Sciatic nerves and brainstem white matter were homogenized and differentially extracted as described in Materials and Methods. Fifty micrograms of total protein were separated on 6% SDS-polyacrylamide gels, transferred to nitrocellulose, and immunoblotted using rabbit anti-NG2. Top panel, NG2 is a major component present in total soluble extracts of sciatic nerve but only a minor component in soluble extracts of brainstem white matter. S, Soluble extract; P, particulate extract. Bottom panel, Effects of chondroitinase ABC digestion on the electrophoretic behavior of NG2 in total nonionic detergent extracts of either sciatic nerve or brainstem white matter. Chondroitinase digestion increases the apparent amount of the NG2 core protein of 300,000. $-$ , No treatment; +, digestion with chondroitinase ABC. B, NG2 cofractionates with sodium channels. Sciatic nerves were subjected to subcellular fractionation as described in Materials and Methods, and the proteins present in each fraction were identified by Western blotting. The relevant regions of each Western blot are shown, aligned with the other gels. NG2 is detected as a broad band with a molecular weight of 240,000. Voltage-dependent sodium channels also appear heterogeneous, with a molecular weight of 215,000. Two isoforms of NrCam are detected in sciatic nerve, with molecular weights of 135,000 and 100,000. Caspr has an apparent molecular weight of 192,000. For NG2 and NrCaM, 20 µg of total protein was loaded per lane; for caspr, 40 µg of protein was loaded; and for the sodium channel, 35 µg of total protein was loaded. My, Myelin membranes; L, light membranes, i.e., those membranes collected at the 12/22% sucrose interface; M, medium-density membranes, the 22/27% sucrose interface; H, heavy membranes collected at the 27/35% sucrose interface; P, material sedimenting through 35% sucrose; St, protein standards used as positive controls for the Western blots. For NG2, the standard was a total nonionic detergent extract of sciatic nerve; all other St lanes were adult rat brain membranes (5-10 µg total protein).

The data given above suggest that in peripheral nerve, perineurial fibroblasts synthesize and secrete NG2, which then becomeslocalized to nodes of Ranvier and other structures. This modelpredicts that some of NG2 might be in a subcellular compartmentthat also contains other proteins associated with the nodal region.To isolate such a subcellular compartment, we subjected isotonichomogenates of sciatic nerve to subcellular fractionation on sucrosegradients and obtained three membrane fractions, termed light,medium, and heavy membranes on the basis of their migration indiscontinuous sucrose gradients. As shown in Figure 7B, NG2 isenriched in the medium (M) and heavy (H) membrane fractions andis not present in either peripheral nerve myelin (My) or the lightmembrane fraction (L). Trace amounts of NG2 were detected in thematerial that sediments through 35% sucrose (P). These mediumand heavy membrane fractions also contained NrCaM and caspr, althoughsmaller amounts of these proteins are also found in the otherfractions analyzed (Fig. 7). In sciatic nerve, NrCam is presentas two polypeptides with molecular weights of 135,000 and 100,000.These variant forms may arise from alternate mRNA splicing (Wanget al., 1998). Voltage-dependent sodium channels, on the otherhand, were found almost exclusively in the medium membrane fraction.Although this medium-density membrane fraction represented onlybetween 6 and 8% of the total membrane protein in sciatic nervehomogenates, it contains significant amounts of nodal membranes,together with the axolemma of unmyelinated axons. These data alsoestablish that the NG2 proteoglycan remains associated with nodalstructures after tissuedisruption.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
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DISCUSSION
REFERENCES

Schwann cells, perineurial fibroblasts, and blood vessels constitute the non-neuronal cellular elements of a peripheral nerve.The Schwann cells and perineurial fibroblasts cooperate to elaboratethe extracellular matrices and basal laminae that surround theentire nerve, individual nerve fascicles, and each Schwann cell-axonunit (Bunge, 1993; Obremski and Bunge, 1993). The epineurial andperineurial linings form barriers whose integrity is essentialin keeping pathogens out of the nerve (for review, see Olsson,1990). The data presented here add NG2, a structurally unique,highly conserved, integral membrane protein that is most oftenfound as a CSPG, to the growing list of cell surface and extracellularmolecules found in peripheral nerve (Nishiyama et al., 1991; Arroyoand Scherer, 2000; Peles and Salzer, 2000). NG2 is likely synthesizedby the perineurial fibroblasts and, when secreted or shed fromthe cell surface, associates with the node of Ranvier and theepineurial and perineurial basal lamina. By virtue of its anti-adhesiveand growth-inhibitory properties (Dou and Levine, 1994; Fidleret al., 1999), NG2 may contribute to the barrier functions ofthese basal laminae and to the organization and stabilizationof the node ofRanvier.

Schwann cells in vitro, grown acutely in dissociated cultures of adult sciatic nerve or for long periods in continuous culture,do not bind the anti-NG2 antibodies, and NG2 could not be detectedby immunoblotting using either lysates of Schwann cell culturesor medium conditioned by Schwann cells (Morganstern et al., 1999).In contrast, abundant NG2 was detected in both perineurial fibroblastcultures and in the medium conditioned by these cells. In tissuesections, a low level of anti-NG2 immunoreactivity was associatedwith the outer membrane of myelinating Schwann cells. Whetherthis represents a low level of synthesis of NG2 by Schwann cellsor the binding of secreted NG2 to sites on either the Schwanncell surface or the endoneurial basal lamina remains to bedetermined.

Our conclusion that the major site of NG2 expression in adult peripheral nerve is the perineurial fibroblast differs fromthat of Schneider et al. (2001), who suggested that in the adultmouse, AN2, the mouse homolog of NG2, is associated with a subpopulationof nonmyelinating Schwann cells. In the adult mouse, AN2 is foundon blood vessels, perineurial cells, and long, thin cells thatlie between myelinated axons, a distribution remarkably similarto that reported here for NG2 in the adult rat. The identificationof the elongated murine cells as nonmyelinating Schwann cellsis based, at least in part, on the colocalization of AN2 and p75.However, p75 can be expressed by many different cell types, includingfibroblasts of peripheral nerve (Thomson et al., 1988; Bothwell,1991; Bradley et al., 1998). In addition, after nerve crush, whenSchwann cells revert to an immature and nonmyelinating phenotype,there is no increase in levels of either AN2 or NG2 (Morgansternet al., 1999; Schneider et al., 2001). Such an increase mightbe expected if nonmyelinating Schwann cells expressed these twohighly related antigens. Thus, although Schwann cell precursorscan express NG2 and AN2 (Schneider et al., 2001), the morphologicaldata presented here and elsewhere (Morganstern et al., 1999) suggestthat perineurial fibroblasts are the major but not necessarilythe only source of these molecules in normal adultnerve.

Biochemical studies of transfected cells have shown that the NG2 core protein, an integral membrane protein with a molecularweight of 300,000, can be proteolytically cleaved from the cellsurface to generate truncated molecules (Nishiyama et al., 1995).Our data show that in the sciatic nerve a significant fractionof NG2 can be extracted into aqueous buffers and that only ~50-60%of the total NG2 present is tightly bound to or associated withmembranes. This soluble form of NG2 may be generated by proteolyticcleavage of intact, full-length NG2. Once secreted or shed, solubleNG2 then associates with distinct structures within the nerve,including basal laminae and nodes ofRanvier.

At present, we can only speculate about how these associations occur. NG2 binds to several different extracellular matrixmolecules, and these molecules could be NG2 binding sites in peripheralnerve (Burg et al., 1996; Tillet et al., 1997). Binding to typeV and VI collagen is mediated by the central extended domain ofthe core protein (domain 2), which is present in both membrane-boundand secreted NG2 (Nishiyama et al., 1995; Tillet et al., 1997).However, the disposition of NG2 in sciatic nerve is not directlycorrelated with the localization of these collagens. Type V collagensare synthesized by neonatal Schwann cells, and these chains aremost prominent in young rather than adult rats such as those studiedhere (Chernousov et al., 2000). In human nerve, type VI collagenis associated with the epineurium, perineurium, and endoneurium(Peltonen et al., 1990). Because NG2 is associated with the perineurialand epineurial linings but is not a major component of the endoneurium,potential interactions between extracellular NG2 and type VI collagencannot fully account for the specific anatomical localizationof NG2 in the nerve. Moreover, proteolytically processed NG2 interactswith type VI collagen poorly, if at all (Nishiyama et al., 1995).Cell adhesion molecules such as neural cell adhesion molecule,neuron-glia cell adhesion molecule, and NrCam, which are concentratedat nodes of Ranvier, as well as tenascin C, are all potentialbinding partners for NG2 (Rieger et al., 1986; Martini et al.,1990; Davis et al., 1996; Burg et al., 1996).

The N-terminal domain 1 of NG2 contains two laminin G domains, a protein motif found on a variety of different proteins, includingcaspr and agrin (Bellen et al., 1998; Missler and Südhof, 1998).These three proteins (NG2, agrin, and caspr) are found at or closeto nodes of Ranvier (Reist et al., 1987; Einheber et al., 1997;Menegoz et al., 1997). Laminin G domains participate in cell-celland cell-matrix interactions by binding directly to proteins orcarbohydrates (Talts et al., 1999). Thus, it is possible thatthe laminin G domains of NG2 provide a site for interactions withother molecular components of thenode.

The localization of NG2 at nodes of Ranvier in the PNS is particularly intriguing, because oligodendrocyte precursor cells,the major NG2-expressing cell type in the CNS, also contact nodesof Ranvier (Butt et al., 1999). Oligodendrocyte precursor cellprocesses are also closely associated with synapses in the rathippocampus (Ong and Levine, 1999; Bergles et al., 2000). BecauseNG2 is present at both central and peripheral nodes, as well asat other sites of ion movement across membranes, it is likelyto be performing one or more important functionsthere.

Like many other proteoglycans, NG2 is multifunctional. Among its properties, NG2 is anti-adhesive to developing neurons, inhibitsaxonal growth when substrate-bound, and rapidly induces the collapseof newborn dorsal root ganglia neuronal growth cones in vitro(Dou and Levine, 1994; Fidler et al., 1999; Ughrin et al., 1999).These properties suggest several possible functions for NG2 atthe node. The axonal membrane at nodes of Ranvier is capable ofrapidly forming a new growth cone, and new sprouts often formhere after nerve injury (Friede and Bischhausen, 1980; McQuarrie,1985). The inhibitory properties of NG2 suggest that one functionin nerve may be to prevent unregulated sprouting in normal, undamagedanimals. When the nerve is injured, regenerating axons grow ina narrow space between the Schwann cell surface and the endoneurialbasal lamina (the bands of Büngner; Nathaniel and Pease, 1963;Ide et al., 1983; Fawcett and Keynes, 1990). These structurescontain relatively little NG2 but are enriched in growth-promotingmolecules such as laminin (Ide et al., 1983). A second possiblefunction for NG2 on the surface of perineurial cells would beto help direct filopodia into these growth-permissiveconduits.

The anti-adhesive properties of NG2 suggest a third function for NG2 at nodes of Ranvier. Our current understanding of thedevelopment of the node of Ranvier in the PNS emphasizes the essentialrole of the Schwann cell as a determinant of where high-densityclusters of sodium channels form (Vabnick and Shrager, 1998; Pelesand Salzer, 2000). In developing nerves, Schwann cells adhereto axons and elongate as they begin to express myelin-specificproteins such as MAG (Lambert et al., 1997). During this elongationphase, broad clusters of sodium channels are seen at the lateraledges of the Schwann cell. The continued elongation of the Schwanncell results in the formation of compact, high-density clustersof sodium channels, again at the lateral edges of the Schwanncell. These clusters eventually fuse to form nodal clusters. Thismodel raises the question of what causes the elongation of Schwanncells to cease. Secreted NG2 is ideally suited to generate sucha stop signal to the Schwann cell. The central extended domainof NG2 may bind to some as yet unidentified binding protein atthe node exposing the globular N-terminal domain and the juxtamembranedomain (Tillet et al., 1997). Because both of these domains (domains1 and 3) are each sufficient to inhibit axonal extension and toinduce growth cone collapse (Ughrin et al., 1999), it is possiblethat they limit or stop the lateral extension of the Schwann cell.In this way, the deposition of NG2 at nodes of Ranvier, whichoccurs at approximately postnatal day 10 in the rat (J. M. Levineand A. K. Levine, unpublished observation), could function tostabilize the structure of thenode.

  FOOTNOTES

Received Feb. 12, 2001; revised July 2, 2001; accepted Aug. 7, 2001.

This work was supported by National Institutes of Health Grant NS21198 (J.M.L.). S.M. was supported in part by a UniversityRAIRE research fellowship. We thank Dr. M. N. Rasband for hisassistance with the preparation of teased nerve fibers and Dr.J. Trimmer and Dr. M. Grumet for gifts ofantibodies.
Correspondence should be addressed to Dr. Joel Levine, Department of Neurobiology and Behavior, State University of New Yorkat Stony Brook, Stony Brook, NY 11794. E-mail: Joel.Levine{at}sunysb.edu.

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