Axo-Glial Interactions Regulate the Localization of Axonal Paranodal Proteins

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© The Rockefeller University Press, 0021-9525/1999//1145 $5.00
The Journal of Cell Biology, Volume 147, Number 6, , 1999 1145-1152

Brief Report

Axo-Glial Interactions Regulate the Localization of Axonal Paranodal Proteins

Jeffrey L. Dupree^a, Jean-Antoine Girault^d, and Brian Popko^a^,b^,c

^a Neuroscience Center, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599
^b Department of Biochemistry and Biophysics, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599
^c Program in Molecular Biology and Biotechnology, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599
^d Institut National de la Santé et la Recherche Médicale, Unit 114, Collège de France, Paris 75231, France
Neuroscience Center, CB#7250, University of North Carolina at Chapel Hill, Chapel Hill, NC 27599-7250.(919) 966-9605(919) 966-1449

popko{at}css.unc.edu

Mice incapable of synthesizing the abundant galactolipids ofmyelin exhibit disrupted paranodal axo-glial interactions inthe central and peripheral nervous systems. Using these mutants,we have analyzed the role that axo-glial interactions play inthe establishment of axonal protein distribution in the regionof the node of Ranvier. Whereas the clustering of the nodalproteins, sodium channels, ankyrin_G, and neurofascin was onlyslightly affected, the distribution of potassium channels andparanodin, proteins that are normally concentrated in the regionsjuxtaposed to the node, was dramatically altered. The potassiumchannels, which are normally concentrated in the paranode/juxtaparanode,were not restricted to this region but were detected throughoutthe internode in the galactolipid-defi- cient mice. Paranodin/contactin-associatedprotein (Caspr), a paranodal protein that is a potential neuronalmediator of axon-myelin binding, was not concentrated in theparanodal regions but was diffusely distributed along the internodalregions. Collectively, these findings suggest that the myelingalactolipids are essential for the proper formation of axo-glialinteractions and demonstrate that a disruption in these interactionsresults in profound abnormalities in the molecular organizationof the paranodal axolemma.

Key Words: paranodin • potassium channels • sodium channels • galactolipids • axo-glial interactions

MYELINATED axons contain regularly spaced unmyelinated gapsknown as nodes of Ranvier, which are critical for the properfunction of the central nervous system (CNS) and the peripheralnervous system (PNS) (Morell et al. 1994). Both the structureand molecular organization of the nodal region are dependenton the formation of the appropriate axo-glial interactions.Structurally, these interactions establish the spacing of adjacentmyelin segments and ultimately determine the position and lengthof the nodal gaps. In addition, septate-like junctions are formedat the interface between the myelin sheath and axon in the paranode(for review see Salzer 1997). Based on the location of theseaxo-glial junctions, Rosenbluth 1990 proposed that they functionin the establishment and maintenance of axolemmal protein domainsof the nodal and paranodal regions.

The most recognized domains of the nodal/paranodal region arethose of the sodium and potassium channels. The positioningand segregation of these channels along the axonal membraneof myelinated fibers is crucial for the rapid conduction ofnerve impulses in both the CNS and PNS (Black et al. 1990).Voltage-gated sodium channels, which are concentrated at thenode of Ranvier are mainly responsible for the axonal depolarizationthat is required for action potential induction (for reviewsee Ritchie 1995). In the paranodal and adjacent juxtaparanodalregions, Shaker-type Kv1.1 potassium channels cluster (Wang et al. 1993).The function of these channels is not completely understood,but they appear to prevent aberrant neuronal firing during development(Vabnick et al. 1999) and may modulate action potential durationand frequency (Hille 1992; Smart et al. 1998).

In addition to the sodium and potassium channels, other axolemmalproteins are also clustered in the region of the node of Ranvierof mature, myelinated axons (for review see Scherer 1996). Severalof these proteins are initially distributed along the entireaxon of unmyelinated fibers. Although these proteins becomerelocated to the nodal region, the mechanisms that mediate theseevents are poorly understood. Nodal clustering of neurofascin,an L1-associated protein that is tightly coupled to the cytoskeleton(Tuvia et al. 1997), precedes the elaboration of compact myelinand may play an important role in defining the site of nodeformation (Lambert et al. 1997). In contrast, the clusteringof ankyrin_G, a nodal protein that is associated with sodiumchannel distribution (Kordeli et al. 1990), appears to be dependenton the presence of the myelin sheath (Lambert et al. 1997).Similarly, paranodin, a 180–190-kD neuronal glycoproteinthat is a potential cell adhesion molecule, accumulates in theparanodal axolemma after myelination (Einheber et al. 1997;Menegoz et al. 1997) and is a component of the paranodal septate-likejunctions that may be involved in establishment and maintenanceof the protein domains of the nodal and paranodal axolemma (Rosenbluth 1990).This protein was also identified as a partner of contactin,a glycosyl-phosphatidyl-inositol–anchored adhesion molecule,and termed contactin-associated protein (Caspr) (Peles et al. 1997).Nevertheless, the neuronal and/or glial molecules that are responsiblefor its localization in the paranodal junctions are not known.

To further explore the role that axo-glial interactions playin the organization of axolemmal nodal proteins, we have analyzedthe distribution of these proteins in mice that contain a disruptionin the gene that encodes UDP-galactose–ceramide galactosyltransferase(CGT), an enzyme that is essential for the production of galactocerebroside(GalC) and sulfatide (Morell and Radin 1969). The galactolipid-deficientmice display several CNS nodal and paranodal abnormalities,including increased heminode formation, altered node length,and terminal loops that frequently face away from the axon (Dupree et al. 1998;Popko 2000). Moreover, the complete absence of CNS and PNS transversebands, which are prominent components of the paranodal septate-likejunctions, indicates that axo-glial interactions are severelydisrupted in the galactolipid-deficient animals (Dupree et al. 1998;Dupree and Popko 1999). These studies described here shouldenhance our understanding of the role that axo-glial interactionsplay in the organization of axolemmal proteins.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
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Immunocytochemical Analysis
Spinal cords (C3) and sciatic nerves were harvested from 30-d-oldCGT^+/+ and CGT^–/– mice that were perfused throughthe heart with either 4 or 1% paraformaldehyde in 0.1 M phosphatebuffer (PB), pH 7.3. Spinal cords were postfixed for 1 h inthe same fixative, cryopreserved in 30% sucrose in PB for 48h at 4°C and sectioned at 10 µm. Sciatic nerves wereteased apart to yield single fiber preparations. Spinal cordsections and sciatic teased fibers were blocked for 1 h in PBcontaining 10% normal goat serum, 5% fish gelatin, and 0.1%Triton X-100 and incubated in the primary antibody overnightat 4°C. The primary antibodies used in this study were directedagainst ankyrin_G (mouse monoclonal, Zymed and gift from Dr.Van Bennett, Duke University, Durham, NC) (Kordeli et al. 1990),neurofascin (rabbit polyclonal, gift from Dr. Van Bennett) (Lambert et al. 1997),paranodin (rabbit polyclonal) (Menegoz et al. 1997), potassiumchannel Kv1.1 (rabbit polyclonal, gift from Dr. Bruce Tempel,University of Washington School of Medicine, Seattle, WA; mousemonoclonal, Upstate Biotechnology) (Wang et al. 1995), sodiumchannels (rabbit polyclonal, gift from Dr. Rock Levinson, HealthSciences Center, Denver, CO) (Dugandzija-Novakovic et al. 1995),and myelin basic protein (mouse monoclonal, Sternberger Monoclonal,Inc.; rabbit polyclonal, Dako, Inc.). After primary antibodyincubation, the tissue was thoroughly rinsed in PB, blockedfor 1 h as described previously, and incubated in the appropriatesecondary antibody conjugated to biotin or Texas red for 2 h.After rinsing the tissue four times for 5 min, the tissue incubatedin the secondary antibody conjugated to biotin was incubatedin streptavidin fluorescein (diluted 1:200) for 30 min and thoroughlyrinsed. The tissue was coverslipped using Vectashield (VectorLabs, Inc.). For double-labeling, the above procedure was repeatedusing a different species-specific antibody and the appropriatesecondary antibody conjugated to the proper fluorochrome. Whenmyelin basic protein was the second antigen to be labeled, thetissue was postfixed in 4% paraformaldehyde in PB for 10 minat –20°C, rinsed, and permeabilized in –20°Cacetone for 10 min. All labeled slides were analyzed by bothconventional fluorescent and scanning confocal microscopy. Imageswere generated on a Leica TCS-NT Laser Scanning microscope usinga 40x oil objective and a pinhole size of 1.0 Airy disk units.

Western Blot Analysis
Spinal cord and sciatic nerve tissues were harvested from 30-d-oldgalactolipid-deficient and wild-type mice, diced into smallpieces, homogenized in 1% SDS in PB, and placed in a boilingwater bath for 10 min. Insoluble material was removed by centrifugationat 5,000 g for 10 min. Protein concentrations were determinedusing a modified Lowry assay (Bio-Rad, Inc.). 100 µg ofprotein was separated using a precast 4–15% gradient polyacrylamidegel (Jule, Inc.), transferred to nitrocellulose, and stainedwith Ponceau S. The nitrocellulose was blocked for 1 h in 5%milk solids, 5% normal goat serum, and 0.1% Triton X-100 inPB, incubated in antiparanodin (1:3,000) for 1 h at room temperature,rinsed in PB, blocked, incubated in goat anti–rabbit secondaryantibody conjugated to HRP, rinsed in PB, and visualized usingECL^TM according to the manufacturer's instructions (AmershamPharmacia Biotech).

Results

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Abstract
Materials and Methods
Results
Discussion
References

Distribution of Ion Channels
To better understand the consequences that altered axo-glialinteractions of the CNS (Dupree et al. 1998) and PNS (Dupree and Popko 1999)have on the establishment of ion channel domains, we analyzedthe distribution of the nodally clustered voltage-gated sodiumchannels and the paranodal/juxtaparanodal Kv1.1 potassium channelsin the CGT-deficient mice. In both the mutant and wild-typemice, CNS and PNS sodium channels were concentrated in smallregions that were presumptive nodes of Ranvier (Fig. 1). Similarresults have been reported previously regarding sodium channeldistribution in the PNS of galactolipid-deficient mice (Bosio et al. 1998).Since we reported previously that CNS nodal length is increasedin the galactolipid-deficient mice (Dupree et al. 1998), wemeasured the length and the width of the sodium channel domainand report node length as a function of axon caliber. In theCNS, the length to width ratio was significantly greater inthe mutant (1.17 ± 0.05; n = 3 mice and 36 nodes; P <0.02 by t test) compared with littermate wild-type (0.75 ±0.13; n = 3 mice and 35 nodes) mice, indicating that the sodiumchannel domains, which likely corresponds to nodal length, wereincreased in the galactolipid-deficient animals.

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Figure 1 (a) In the spinal cord of wild-type mice, potassium channels (red) are concentrated in the juxtaparanodes, and to a lesser extent, in the paranode, whereas the sodium channels (green) are restricted to the nodes of Ranvier. (b) In contrast, the potassium channels rarely accumulate in the juxtaparanodes of spinal cord tissue from the galactolipid-deficient mice. However, similar to the wild-type, the sodium channels cluster in the nodes but the sodium channel domains are slightly longer in the mutant as compared with the wild-type. The distribution of the potassium and sodium channels in the PNS is similar to the CNS for both the wild-type (c) and the mutant (d) mice. Note that in the CNS and the PNS of the galactolipid-deficient mice the channel domains occasionally overlap (yellow). a and b were generated as the compilation of eight consecutive images each 0.4 µm apart. c and d were generated as the compilation of 10 images each 0.26 µm apart. Bar, 5 µm.

In contrast, potassium channel distribution was dramaticallyaltered in the CNS of the CGT-deficient mice. In the CNS andPNS of wild-type mice, intense labeling was commonly observedin the juxtaparanodal region (Fig. 1, a and c; Table ). Thejuxtaparanode was easily distinguished from the paranodal andnodal regions, since its diameter was conspicuously larger.Potassium channel antibody reactivity was occasionally observedin the paranodal region; however, the labeling intensity wasgreatly reduced. In the CNS of the mutant animals, fewer juxtaparanodalregions were immunolabeled with the Kv1.1 antibody (Fig. 1 b),whereas diffuse labeling over long stretches of axons was occasionallyobserved (see Fig. 3 b). When paranodal/juxtaparanodal potassiumchannel accumulations were present, the width of the labelingpattern did not change, indicating that the diameter of theseaxons does not change at the interface between the paranodeand juxtaparanode in the galactolipid-deficient mice. In thePNS, paranodal/juxtaparanodal regions were typically labeled,although the labeling was frequently less intense and more diffuseas compared with the wild-type sciatic nerve fibers (Fig. 1cand Fig. d).

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Table 1 Quantitation of Potassium Channel Distribution

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Figure 3 Western blot analysis revealed no difference in the expression of paranodin between the wild-type (+/+) and the mutant (–/–) mice in either the spinal cord (S.C.) or the sciatic nerve (S.N.).

To verify the location of the sodium and potassium channel accumulations,we double-labeled CNS and PNS tissues with antibodies directedagainst the ion channels (Fig. 1). The findings from these double-labelingexperiments supported the single immunolabeling experimentalobservations that the sodium channel distribution was not alteredin the mutants, since these channels maintained a nodal localizationin both the CNS and PNS. Using the sodium channel clusteringas an indicator of node position, we have quantitatively demonstratedthat the distribution of potassium channels is dramaticallyaltered in both the CNS and PNS (Table ). In wild-type mice,potassium channels were primarily restricted to the juxtaparanodalregions with a minority of axons exhibiting paranodal distribution.In the galactolipid-deficient mice, the channels were rarelylimited to the juxtaparanode. Instead, the potassium channelsin the CNS were frequently clustered in the paranodal region,diffusely distributed along the internode, or were not detected,whereas in the PNS they were primarily observed only in theparanodes. In addition to facilitating the potassium channelquantitative analysis, the double-labeling approach also revealedthat the prominent separation between the ion channel domainsin the wild-type tissue is frequently absent in the mutant.In the mutant mice the potassium and sodium channel domainsoccasionally overlapped (Fig. 1).

Distribution of Cell Adhesion and Cell Adhesion–associated Molecules
The structural abnormalities at the node of the galactolipid-deficientmice appear to be related to compromised axo-glial interactions,such that we have analyzed the distribution of two potentialneuronal adhesion molecules: paranodin and neurofascin. In addition,we have determined the distribution of the cytoskeleton-associatedmolecule ankyrin_G. Using a combination of immunocytochemicaltechniques and confocal microscopy, we demonstrated the completeabsence of paranodin accumulation in the paranodal regions ofthe myelinated fibers of the spinal cord in the CGT^–/–mouse (Fig. 2, a and b). In the galactolipid mutants, paranodinappeared to be diffusely distributed along the axon (Fig. 2cand Fig. d), resembling the expression pattern of unmyelinatedfibers (Einheber et al. 1997). In the sciatic nerve, paranodinwas localized to the paranodal region; however, the stainingintensity was reduced and the border between the paranode andthe juxtaparanode was not as clearly defined as in the wild-typesciatic nerve (Fig. 2c and Fig. d). Paranodin was not detectedin the paranode of any of the CNS fibers examined and reducedaccumulations of paranodin were always observed in the paranodeof the PNS fibers observed. Western blot analysis revealed nodifference in the level of paranodin expression between thegalactolipid mutant and wild-type animals for either the spinalcord or the sciatic nerve (Fig. 3), indicating that the diminishedimmunoreactivity was a result of abnormal paranodal accumulations.In contrast, the distribution of the nodal proteins neurofascin(Fig. 4) and ankyrin_G (data not shown) did not appear alteredin either the spinal cord or the sciatic nerve of the mutant.

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Figure 2 In the wild-type mice paranodin (green) is highly concentrated in the paranodal regions of spinal cord (a) and sciatic nerve (c) axons. In contrast, the galactolipid-deficient mice exhibit a more diffuse labeling pattern. In the mutant spinal cord (b) paranodin is evenly distributed in the axolemma throughout the internode. In the sciatic nerve (d) of these mice, paranodin is concentrated in the paranode but the interface between the paranode and the juxtaparanode is not clearly demarcated. a and b, eight images 0.26 µm apart; double-labeled for paranodin in green and phosphorylated neurofilament in red. c and d, eight images 0.4 µm apart; double-labeled for paranodin in green and myelin basic protein in red. Bar, 5 µm.

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Figure 4 In the spinal cord, neurofascin (green) was restricted to the nodes of Ranvier in both the wild-type (a) and the mutant (b) mice. a and b are also labeled for the potassium channels (red) in an effort to assist with the recognition of nodal/paranodal regions. In the sciatic nerve (c and d), neurofascin also is concentrated in the node; however, some protein is also located in the paranodal regions of the wild-type (c) and mutant (d) mice. a and b, six images 0.31 µm apart; double-labeled for neurofascin in green and potassium in red. c and d, four images 0.26 µm apart; double-labeled for neurofascin in green and myelin basic protein in red. Bar, 5 µm.

	Discussion

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We reported previously that mice incapable of synthesizing themyelin galactolipids GalC and sulfatide exhibit structural abnormalitiesof the nodal and paranodal regions that are likely due to compromisedaxo-glial interactions (Dupree et al. 1998; Dupree and Popko 1999).In this study, we demonstrate that in the CNS, the distributionof the Shaker-type Kv1.1 potassium channels is altered, whereasthe clustering of the voltage-gated sodium channels is onlymildly affected. Furthermore, we show a complete disruptionin the axolemmal organization of the potential axo-glial adhesionmolecule paranodin. In the PNS, we demonstrate similar trendswith regard to ion channel organization and paranodin distribution;however, the abnormalities are less dramatic. The regional differencescorrelate well with the structural data, since the morphologicalabnormalities in the PNS are less severe. Taken together, wepropose that the disruption in the distribution of paranodinis further evidence that axo-glial interactions are disruptedin the galactolipid-deficient mice, and that these aberrantinteractions impair appropriate ion channel segregation.

Compromised Axo-glial Interactions Result in Abnormal Ion Channel Distribution
The pattern of potassium channel distribution that we reportfor the galactolipid-deficient mice is consistent with a previousreport of shiverer mice (Wang et al. 1995), which also displaycompromised axo-glial interactions in the CNS (Rosenbluth 1980a).In both shiverer and galactolipid-deficient mice, potassiumchannels frequently do not cluster in the paranodal/juxtaparanodalregion but are diffusely distributed throughout the internodalregions. Furthermore, the sciatic nerve of shiverer mice displayelongated paranodal/juxtaparanodal potassium channel labeling(Wang et al. 1995). This alteration in ion channel distributioncorrelates well with the mild disruption in paranodal Schwanncell–axon interactions (Rosenbluth 1980b). Likewise, potassiumchannel distribution is altered in the PNS of the CGT^–/–mice coinciding with compromised axo-glial interactions andreduced paranodal accumulation of paranodin.

Consistent with abnormal potassium channel distribution, particularlyin conjunction with aberrant paranode structure, action potentialduration is increased in the CNS of the galactolipid-deficientmice (Coetzee et al. 1996). In addition, action potential amplitudeis decreased in the CNS (Coetzee et al. 1996), and to a lesserdegree in the PNS (Dupree et al. 1998). Furthermore, the additionof 4-aminopyridine, an inhibitor of potassium channels, resultsin little or no change in PNS amplitude, whereas CNS amplitudeincreased 25%. This difference likely reflects the greater alterationof potassium channel distribution in the CNS compared with thePNS in these mutants.

Axo-glial interactions do not only influence potassium channeldistribution. Clustering of sodium channels in the PNS alsoappears dependent upon the appropriate association of the Schwanncell with the axon (Dugandzija-Novakovic et al. 1995). In theCNS, Kaplan et al. 1997 reported that oligodendrocyte contactis not required for initial sodium channel clustering in vitro,but a recent report demonstrates that axo-glial contact, asindicated by paranodin and myelin-associated glycoprotein labeling,is required for the sodium channel accumulation in vivo (Rasband et al. 1999).In the galactolipid-deficient mice, sodium channels are concentratedin nodal regions. This finding demonstrates that normal paranodalaxo-glial contacts are not essential for nodal clustering ofsodium channels. Although gross clustering of sodium channelsto the nodal gap is not dependent upon the formation of theparanodal septate-like junctions, these axo-glial junctionsmay be important in establishing and maintaining the interfacebetween the sodium and potassium domains, since these domainsoccasionally overlap in both the CNS and the PNS of the galactolipid-deficientmutant.

Galactolipids Are Essential for Proper Formation of Axo-glial Interactions
Using ultrastructural analysis, we have shown previously thataxo-glial interactions are disrupted in the galactolipid-deficientmice (Dupree et al. 1998; Dupree and Popko 1999). Here we provideevidence that these interactions are also disrupted at the molecularlevel, since paranodin, a known component of the septate-likejunctions that form between the myelin sheath and the axolemma(Einheber et al. 1997), does not appropriately accumulate inthe paranodal region. Presently, the mechanism responsible forproper axolemmal distribution of paranodin is not known. Sinceparanodin has multiple potential cell adhesion domains includingan extracellular lectin-binding domain (Menegoz et al. 1997;Peles et al. 1997), an attractive model is that GalC and/orsulfatide directly bind paranodin and facilitate its accumulationin the paranodal axolemma. Nevertheless, there is no evidenceto suggest that the galactolipids accumulate in the paranodalregion. Another possibility centers on the role that the galactolipidsplay in detergent-insoluble-complex (DIGs) formation and trafficking.In oligodendrocytes, DIGs, which are raft-like microdomainscomposed of the myelin galactolipids and proteins, are thoughtto be responsible for the molecular organization of the myelinsheath (Kramer et al. 1997, Kramer et al. 1999). Therefore,in mice that lack GalC and sulfatide, an as yet unidentifiedparanodin ligand may be abnormally distributed in the oligodendrocyteof CGT^–/– mice, resulting in the disruption of paranodinintracellular targeting.

The rearrangement of axolemmal proteins in the CGT^–/–mice appears to be specific to the paranodal region, since themembrane arrangement of ankyrin_G and neurofascin is not grosslyaffected. The clustering of neurofascin precedes myelination(Lambert et al. 1997), therefore it is not surprising that itsdistribution is not affected by a myelin gene mutation. In contrast,the clustering of ankyrin_G and voltage-dependent sodium channelsis temporally associated with the elaboration of myelin-associatedglycoprotein-positive myelin-forming processes (Lambert et al. 1997).Therefore, if the distribution of sodium channels and ankyrin_Gis dependent on myelin, the mechanism by which these proteinsare spatially organized apparently does not require the myelingalactolipids and is distinct from the process that regulatespotassium channel and paranodin distribution.

In summary, mice that are incapable of producing the myelingalactolipids have compromised axo-glial interactions as evidencedby CNS and PNS structural abnormalities (Dupree et al. 1998;Dupree and Popko, in press). Furthermore, the distribution ofparanodin, a prominent component of the paranodal septate-likejunctions (Menegoz et al. 1997; Einheber et al. 1997), is dramaticallyaltered with no paranodal accumulation in the CNS. The disruptionin axo-glial interactions leads to the abnormal distributionof the Shaker-type Kv1.1 potassium channels in both the CNSand the PNS. Therefore, our data indicate that axo-glial interactionsare essential not only for the proper myelin formation but alsoaxolemmal organization.

Acknowledgments

The authors thank Dr. Jim Salzer for his insightful suggestionsand his advice with the preparation of the sciatic teased fibers.We also thank Drs. Rock Levinson, Vann Bennett, and Bruce Tempelfor kindly supplying us with antibodies. In addition, we wishto thank Dr. Michael Chua for his assistance with preparingthe confocal microscopy images, and Ms. Jill Marcus for hercritical reviews of the manuscript.

This work was supported by the National Institutes of Health(NS27336 to B. Popko). J.L. Dupree is supported by an AdvancedPost-doctoral Fellowship Award from the National Multiple SclerosisSociety.

Submitted: 12 October 1999

Revised: 2 November 1999

Accepted: 3 November 1999

Abbreviations used in this paper: Caspr, contactin-associatedprotein; CGT, ceramide galactosyltransferase; CNS, central nervoussystem; GalC, galactocerebroside; PB, phosphate buffer; PNS,peripheral nervous system.

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