Antibody Cross-Linking of Myelin Oligodendrocyte Glycoprotein Leads to Its Rapid Repartitioning into Detergent-Insoluble Fractions, and Altered Protein Phosphorylation and Cell Morphology

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

The Journal of Neuroscience, July 2, 2003, 23(13):5461-5471

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (24)

Citing Articles via Google Scholar

Google Scholar

Articles by Marta, C. B.

Articles by Pfeiffer, S. E.

Search for Related Content

PubMed

PubMed Citation

Articles by Marta, C. B.

Articles by Pfeiffer, S. E.

Previous Article  |  Next Article
Antibody Cross-Linking of Myelin Oligodendrocyte Glycoprotein Leads to Its Rapid Repartitioning into Detergent-Insoluble Fractions, and Altered Protein Phosphorylation and Cell Morphology
C. B. Marta, C. M. Taylor, T. Coetzee, T. Kim, S. Winkler, R. Bansal, and S. E. Pfeiffer
Department of Neuroscience, University of Connecticut Medical School, Farmington, Connecticut 06030-3401

   Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Myelin oligodendrocyte glycoprotein (MOG) is, quantitatively,a relatively minor component of the myelin membrane. Nevertheless,peritoneal administration of MOG evokes potent cellular andhumoral immunoreactivity, resulting in an experimental allergicencephalitis with immunopathology similar to multiple sclerosis.Moreover, antibodies against MOG cause myelin destruction insitu. Therefore, it appears that MOG-related demyelinationis dependent on anti-MOG antibody, but the mechanism(s) by which it occurs is unclear. Of potential significance are observationsthat some proteins are selectively partitioned into specializedplasma membrane microdomains rich in glycosphingolipids andcholesterol ("lipid rafts"). In particular, during ligand orantibody cross-linking, various plasma membrane receptors undergoenhanced partitioning into rafts as an obligatory first steptoward participation in early signal transduction events. Incontrast to mature myelin, in oligodendrocytes (OLs) in cultureMOG is not raft associated [Triton X-100 (TX-100) soluble,4°C]. However, in this study we show that antibody cross-linking(anti-MOG plus secondary antibody) of MOG on the surface ofOLs results in the repartitioning of $~$ 95% of MOG into the TX-100-insolublefraction. This repartitioning of MOG is rapid ( $<=$ 1 min), antibodydose dependent, requires an intact cytoskeleton, leads to phosphorylationor dephosphorylation of tyrosine, serine, and threonine residuesin specific proteins (e.g., ${beta}$ -tubulin, G ${beta}$ _1–2), and invokesa rapid retraction of OL processes. After removal of the cross-linkingantibodies, these events are reversed. We hypothesize thatantibody-mediated repartitioning of MOG into TX-100-insoluble glycosphingolipid–cholesterol-rich microdomains initiatesspecific cellular signaling that could be related to initialsteps of MOG-mediated demyelination.

Key words: myelin oligodendrocyte glycoprotein; oligodendrocytes; multiple sclerosis; lipid rafts; cytoskeleton; signaling

   Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Myelin is a unique, lipid-rich biological membrane producedin the CNS by oligodendrocytes (OLs) (Pfeiffer et al., 1993;Madison et al., 1999). Loss or damage of this functionallyactive membrane results in neurological deficits such as occurin multiple sclerosis (MS). Myelin oligodendrocyte glycoprotein(MOG) is an integral myelin membrane protein present primarilyin the outer lamella of the myelin sheath. Despite its relativelylow abundance (0.01–0.05% of the total myelin protein),it has been implicated as a potentially major player in demyelinatingdiseases (Linington et al., 1984).
Besides inflammatory mediators derived from T cells, there isincreasing evidence that anti-MOG effector mechanisms playan important role in the pathogenesis of demyelination (Reindlet al., 1999; Iglesias et al., 2001; Von Büdingen et al., 2001). Anti-MOG antibodies are found in the CSF and in disintegrating myelin around axons in lesions of acute MS patients (Linington and Lassmann, 1987; Xiao et al., 1991; Genain etal., 1995; Reindl et al., 1999). Presentation of purifiedMOG induces severe demyelinating experimental allergic encephalomyelitis(EAE) in both rodents and primates (Johns and Bernard, 1999; Iglesias et al., 2001). When a monoclonal antibody (mAb) againstMOG is injected into rodents, there is extensive demyelination(Schluesener et al., 1987; Linington et al., 1988). In addition,demyelination was produced in aggregating brain cell culturesby anti-MOG, whereas antibodies against other myelin proteinshad no effect (Kerlero de Kosbo et al., 1990). Despite thegrowing conviction that MOG/anti-MOG interactions are mediatorsof demyelination in rat EAE and MS, a mechanism has not beenestablished. The demyelinating capacity of the MOG/anti-MOGcomplex may be related to its ability to activate complement (Piddlesden et al., 1993); however, MOG-related demyelinationalso occurs independently of complement (Dyer and Matthieu,1994; Menon et al., 1997).
Glycosphingolipids and cholesterol form lateral assemblies ("rafts") in the plasma membrane of cells, into which certain proteins can partition whereas others are excluded (Simonsand Ikonen, 1997; Brown and London, 1998; Friedrichson andKurzchalia, 1998; Varma and Mayor, 1998). Lipid rafts havean important role as platforms for the initiation of signaltransduction by favoring specific protein–protein interactionsnecessary for signal transduction. Ligand or antibody cross-linkingof some proteins results in their enhanced partitioning into rafts and their participation in early signal transduction events (Simons and Toomre, 2000). We have proposed that the high contentof glycosphingolipids and cholesterol in myelin sheaths maycontribute functionally to OL–myelin physiology (Bansaland Pfeiffer, 1989; Pfeiffer et al., 1993; Kim et al., 1995; Bansal et al., 1999). Consistent with this hypothesis, myelinproteins are differentially partitioned into rafts, includingthe glycosylphosphatidylinositol-anchored proteins NCAM (neuralcell adhesion molecule)-120 and contactin, doubly acylatedproteins Fyn and Lyn kinases, and 2',3'-cyclic nucleotide 3'-phosphodiesterase(CNP) and MOG (Kim et al., 1995; Kramer et al., 1997, 1999; Kim and Pfeiffer, 1999; Simons et al., 2000; Taylor et al.,2002).
In this study we show that antibody-induced cross-linking ofMOG in OLs in a complement-independent manner (1) results inthe partitioning of MOG into the detergent-insoluble fractionproduced by Triton X-100 (TX-100) extraction at 4°C, (2)concomitantly activates dephosphorylation of ${beta}$ -tubulin and theG ${beta}$ subunit of the trimeric G-protein complex, as well as the phosphorylation of other yet unidentified proteins, and (3)triggers OL process retraction. We propose that similar eventsmay contribute to a molecular mechanism leading to the initialsteps of MOG-related demyelination.

   Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Materials. Antibodies were obtained from the following sources: monoclonal anti-MOG antibody (8–18C5) (Dr. C. Linington,Max-Planck Institute, Germany); anti-proteolipid protein (PLP)antibody (AA3) (Dr. M. Lees, Shriver Center, Waltham, MA);anti-CNP (Bansal and Pfeiffer, 1985); anti-phosphoserine (Calbiochem,San Diego, CA); anti-phosphothreonine (Zymed, San Francisco,CA); anti-phosphotyrosine (4G10), polyclonal anti-caveolin antibody, and goat anti-mouse IgG (Transduction Laboratories,San Diego, CA); anti-G ${beta}$ 1–4 (Santa Cruz Biotechnology,Santa Cruz, CA); horse radish peroxidase-conjugated goat anti-mouseIgG (Chemicon, Temecula, CA); and anti- ${beta}$ -actin and anti- ${beta}$ -tubulinantibodies (Sigma, St. Louis, MO). Saponin, methyl- ${beta}$ -cyclodextrin(MCD), filipin complex, peroxidase-conjugated cholera toxinB subunit, cytochalasin D, nocodazol, okadaic acid, vanadate, 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS),and Hoechst 33342 were obtained from Sigma. The general tyrosinekinase inhibitor PD166285 was a gift from Parke Davis (AnnArbor, MI). All solutions were prepared with MilliQ H₂O. Proteinconcentrations were determined by DC protein assay kit (Bio-Rad,Richmond, CA).
Cell culture. Mixed primary cultures and highly enriched populationsof maturing OLs were prepared and maintained as described previously(Pfeiffer et al., 1993; Bansal et al., 1996). OL populationswere grown in defined medium [modified N2 (mN2)] (Bottensteinand Sato, 1979; Gard and Pfeiffer, 1989) for 7 d to obtainMOG-expressing OLs.
Immunofluorescence microscopy. Cells were incubated with HEPES-bufferedEarle's balanced salt solution (EBSS-HEPES) containing 3% normalgoat serum (NGS) (also used for diluting antibodies) to block nonspecific absorption, and live cells were stained (20 min,4°C) with O4 mAb (1:25), in some cases double-immunolabeledfor the surface antigens galactocerebroside (GalC) (O1 mAb,1:25) (Sommer and Schachner, 1981; Bansal et al., 1989) orMOG (8–18C5 mAb) (1:100). Cells were then incubated withthe appropriate secondary antibodies for 20 min: FITC-conjugatedgoat anti-mouse IgM (1:50; µ-chain specific, for O1 orO4; Chemicon) plus Cy3-conjugated goat anti-mouse IgG (1:500; ${gamma}$ -chain specific, for MOG; Jackson ImmunoResearch, West Grove,PA). Cells were mounted in 50% glycerol, pH 8.6, and 2.5% diazobicyclo-(2,2,2)octane to suppress fading and examined by epifluorescence microscopy.Total cell number was determined by counting cells labeledwith a nuclear counterstain (1 µg/ml Hoechst dye 33342)included with the secondary antibodies. Washing between stepswas performed with three 5 min changes of 1% NGS and EBSS-HEPES.Data of cell counting from at least 10 fields were used foreach preparation. To assess the integrity of microtubules andmicrofilaments after nocodazol (10 µM; 0, 30, 60, 90,and 120 min) or cytochalasin D (20 µM; 0, 30, 60, 90,and 120 min) treatments, insoluble tubulin and actin, respectively,were stained as described by Pigino et al. (2001). Briefly,cells were fixed with 4% paraformaldehyde (15 min, 4°C),washed with 0.13 M HEPES, pH 6.9, 2 mM MgCl₂, 10 mM EGTA,and extracted in the same buffer plus 0.2% TX-100 for 5 minat 37°C before tubulin staining, or with 0.02% saponinfor 2 min at 37°C before actin staining.
Estimation of OL morphology after MOG cross-linking. OLs grownin mN2 medium were washed with 1% bovine serum albumin (BSA)in DMEM and incubated at 37°C with monoclonal anti-MOGantibody [8–18C5; 1:100 (156 µg/ml IgG dilutedin freshly prepared mN2; antibody concentration was determinedby QuantiType Radial Immunodiffusion kit, QED Bioscience, San Diego, CA)] for various time intervals (5–15 min). Antibodywas washed out by two changes of DMEM. Goat anti-mouse IgG(1:500, diluted in DMEM) was added for 5–15 min at 37°C.In some experiments, plates were incubated with 0.1 µMPD166285 (3 hr, 37°C) or 10 nM okadaic acid (3 hr, 37°C)before MOG cross-linking. In some other experiments, the antibody-containingmedia was removed, and the cells were grown further in freshmedium for 2, 4, or 14 hr. Controls were subjected to the sameschedule of washes and incubations. Plates were put on an ice tray, and antibody was washed out by two changes of EBSS-HEPES.Live cells were stained (20 min, 4°C) with O4 mAb (1:25)as described before and analyzed by epifluorescence microscopy.The areas occupied by mature OLs in randomly selected fieldswere compared, using Adobe Photoshop 5.0 (number of pixelsper cell). Averages and SEM were calculated (n = 20–35), and evaluation of statistics significance between conditionswas made using Student's two-tail t test.
Antibody perturbation and preparation of cell lysate. OLs grownin mN2 medium were washed with 1% BSA in DMEM and incubatedat 37°C with monoclonal anti-MOG antibody [8–18C5;1:25–1:500 (624–31 µg/ml IgG, diluted infresh mN2)] for various time intervals (1–60 min). Antibodywas washed out by two changes of DMEM. Goat anti-mouse IgG (1:25–1:10,000, diluted in DMEM) was added for 1–30min at 37°C to cross-link MOG/anti-MOG complexes. Controls,including no additions or treatment with only primary or secondaryantibody, were subjected to the same schedule of washes andincubations. Some plates were treated with monoclonal antibodyO10 (recognizing an extracellular epitope of PLP, diluted 1:10)(Jung et al., 1996) and secondary antibody in the same wayas anti-MOG treatment. In some experiments, plates were incubatedwith 5 mM MCD (15 min, 37°C; see below), 10 µM nocodazol(2 hr, 37°C), 20 µM cytochalasin D (2 hr, 37°C),10 nM okadaic acid (3 hr, 37°C), or 0.1 µM PD166285(3 hr, 37°C) before MOG cross-linking. In some cases, thecontrol and antibody-containing media were removed, and thecells were grown further in fresh medium for 15 or 30 min. After cross-linking, plates were put on an ice-tray and washedtwice with ice-cold PBS or with mN2 and then incubated at 37°Cfor 15 or 30 min. Cells were scraped into 0.5 ml of 150 mMNaCl, 5 mM EDTA, 25 mM Tris-Cl buffer, pH 7.5, containing 1mM PMSF, 10 µg/ml leupeptin–aprotinin, 50 mM NaF,10 mM NaP₂O₇, and 1 mM Na o-vanadate (scraping buffer) andpassed 10 times (on ice) through a 30 ga needle.
Detergent extraction and sucrose gradient ultracentrifugation. Triton X-100 (1% final concentration) was added to cell lysatesand incubated for 30 min at either 4 or 37°C (Kim andPfeiffer, 1999; Taylor et al., 2002) (see Results). The TX-100extracts were centrifuged (13,000 x g, 4°C, 10 min) toseparate them into detergent-insoluble pellet and detergent-solublesupernatant fractions.
The supernatant fraction was precipitated with 2 vol of ethanolat –20°C overnight and centrifuged (13,000 x g, 4°C, 10 min), and the new supernatant was discarded. Finally, boththe original detergent-insoluble pellet and the ethanol-precipitatedsoluble fraction pellets were solubilized in equal volumes(to allow comparison of the relative amount of each proteinin the two fractions) of sample buffer for analysis by SDS-PAGE.
For sucrose gradient ultracentrifugation, TX-100-insoluble pelletfractions were resuspended in 0.5 ml of scraping buffer plus1% TX-100, mixed with 2 M sucrose (1 ml), overlaid with 1 M(2 ml) and 0.2 M (1.5 ml) sucrose, and centrifuged for 16 hrat 45,000 rpm (SW 55 Ti, $~$ 200,000 x g; Beckman) at 4°C.After centrifugation, 0.5 ml fractions were collected at 4°Cfrom the top to the bottom of the gradient.
Cholesterol extraction. To disrupt cholesterol in OL membranes before TX-100 extraction, cell lysates were treated with saponin(final 0.2%) on ice for 30 min and centrifuged (13,000 x g,10 min) (Kim and Pfeiffer, 1999). The supernatant (S1) wascollected. The pellet was extracted with 0.5 ml of 1% TX-100in scraping buffer for 30 min (see above) and centrifuged (13,000 x g, 10 min), and the TX-100-soluble fraction (S2) and pellet were separated. Supernatants S1 and S2 were precipitated withethanol at –20°C overnight and centrifuged (13,000x g, 10 min). Pellets and ethanol-precipitated supernatantfractions were resuspended in equal volumes (to allow a comparisonof the relative amount of each protein in the two fractions)of sample buffer for analysis by SDS-PAGE. To remove cholesterolfrom live cells, OLs in culture were treated with 5 mM MCDfor 15 min at 37°C (Ledesma et al., 1998), before MOG cross-linking.Cholesterol levels were evaluated by filipin staining (50 µg/ml,30 min, 4°C).
SDS-PAGE and Western blotting analysis. Equal volumes of the soluble and insoluble fractions (see above) of the various TX-100extracts were solubilized in sample buffer [50 mM Tris-HCl,pH 6.8, 2.5% glycerol, 5% SDS, 4 M urea, 0.01% bromophenolblue, with or without 10 mM DTT (see Results)], loaded ontoacrylamide gels (Protean II mini-cell apparatus, Bio-Rad),and run at constant voltage (120 V, 1–2 hr). The proteinswere transferred to polyvinylidene difluoride (PVDF) membranes(Hybond-P, Amersham Biosciences, Piscataway, NJ) at 4°Cwith a constant voltage (100 V, 1 hr). The blots were blockedwith 5% nonfat milk or 5% BSA (Sigma) depending on the antibody(1 hr, room temperature) before immunostaining and detection[enhanced chemiluminescence (ECL Plus), Amersham Biosciences].
Two-dimensional PAGE. Mature OL cells were scraped into 25 mM Tris-Cl buffer, pH 7.5, containing 2% CHAPS, 1 mM PMSF,10 µg/ml leupeptin–aprotinin, 50 mM NaF, 10 mMNaP₂O₇, and 1 mM Na o-vanadate. Proteins were precipitatedovernight with 2 vol of ethanol at –20°C. Cell extracts(300 µg of protein) were solubilized in rehydration buffer:7 M urea, 2 M thiourea, 2% CHAPS, 0.5% immobilized pH gradient(IPG) buffer 4–7 (Amersham Biosciences), 100 mM DTT,0.001% bromophenol blue. All samples were left in rehydrationbuffer for 1 hr at room temperature with occasional mixingbefore centrifugation (10,000 x g, 10 min) to clear particulatematter. Sample supernatant was added to IPGphor coffins (AmershamBiosciences), and an Immobiline Dry Strip, pH 4–7, isoelectric focusing gel (Amersham Biosciences) was placed over the solution.The IPG strips were allowed to rehydrate overnight. Proteinswere separated in the first dimension (200 V, 1 hr; 500 V,1 hr; 1000 V, 1 hr; ramped to 8000 V, 30 min; held at 8000V for 30,000 Vh) at 20°C using an IPGphor electrophoresisunit (Amersham Biosciences). After isoelectric focusing, the gel was equilibrated first for 15 min with 130 mM DTT in an equilibration buffer containing 6 M urea, 50 mM Tris, pH 6.8,30% glycerol, 2% SDS, and second for 15 min with 135 mM iodoacetamidein the same equilibration buffer. SDS-PAGE was performed in10% acrylamide running gels at a constant current (15 mA, 14hr), using a Hoefer DALT vertical system (Amersham Biosciences).The proteins were transferred to PVDF membranes (Hybond-P,Amersham Biosciences) at constant current (400 mA, 14 hr).In some cases, gels were stained with ammoniacal silver nitrateor Colloidal Blue (Invitrogen, Carlsbad, CA).

   Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Antibody-induced cross-linking of MOG on the surface of differentiated OLs in culture induces its partitioning into a detergent insoluble fraction
Glycosphingolipid–cholesterol microdomains are often studied biochemically by taking advantage of their insolubility in nonionic detergents. We have shown previously that in myelin membrane $~$ 40% of MOG is present in TX-100 (4°C)-insoluble, low-density, glycosphingolipid–cholesterol-rich microdomains (lipidrafts) (Kim and Pfeiffer, 1999; Taylor et al., 2002). In contrast, when cultures enriched for OLs were extracted withTX-100 at 4°C, nearly all of MOG was detected in the solublefraction at all ages studied (Fig. 1). We conclude that theassociation of MOG in the relatively immature, myelin-like membranes of OLs in culture (Singh and Pfeiffer, 1985) differs in thisimportant characteristic from that in mature myelin in associationwith axons.

View larger version (24K):
[in this window]
[in a new window]
Figure 1. Developmental association of MOG with detergent-insoluble microdomains in OLs. Western blot analysis of MOG in pellet (P, insoluble) and supernatant (S, soluble) fractions during TX-100 extraction at 4°C from OLs (3–8 d in culture). Cell lysate (20 µg of protein) was extracted, and the entire yield in each fraction was loaded in the gels for each condition. The percentage of O1 + /total cells and MOG +/O1+ cells in each preparation is indicated (estimated by immunofluorescence microscopy as described in Materials and Methods). This figure represents a typical result of three independent experiments.

Noting that cross-linking of a number of membrane receptorswith antibodies leads to their repartitioning into lipid rafts (Simons and Toomre, 2000), we treated MOG-positive OLs at 37°Cwith anti-MOG antibody (1:100) for 15 min before detergentextraction; again, nearly all of the MOG was found in the solublefraction (Fig. 2A). However, when OLs were first treated withanti-MOG (primary antibody) and then were further treated witha cross-linking secondary antibody (1:100; anti-IgG) for anadditional 15 min at 37°C, MOG was recovered nearly entirelyin the detergent-insoluble fraction (Fig. 2A). Several controlstudies were performed (Fig. 2): (1) secondary antibody alonehad no effect on MOG partitioning; (2) immunoblot analysisconfirmed that the signal observed was not attributable tothe detection of 25 kDa anti-MOG antibody light chains (which,were they present, could potentially be confused with 28 kDa MOG/anti-MOG signals in reducing gel Western blots); (3) thedetergent solubilities of two other major myelin proteins,CNP and PLP (both mostly soluble during extraction of OLs inculture with TX-100 at 4°C), were unaltered by the anti-MOG/anti-IgGcross-linking (data not shown); (4) similar cross-linking ofPLP with a monoclonal antibody against an extracellular domain(010, Jung et al., 1996) did not alter the detergent solubilityof either PLP or MOG (Fig. 2B).

View larger version (29K):
[in this window]
[in a new window]
Figure 2. MOG repartitioning after antibody-induced cross-linking. A, B, Western blot analyses of MOG (A, B), anti-IgG (to control for residual antibody light-chain reaction in the $~$ 25 kDa region of blots; 2° Ab) (A) and PLP (B) in pellet (P, insoluble) and supernatant (S, soluble) fractions during TX-100 extraction at 4°C of mature OLs. Cells were incubated for 15 min with anti-MOG mAb 8–18C5 (1:100, MOG Ab), anti-mouse IgG (1:100, 2° Ab), subsequently with MOG Ab and 2° Ab (A), subsequently with O10 (1:10) and anti-mouse IgM (1:100) (B) or media alone (control, no Ab). After scraping, cell lysates (20µg of protein) were extracted with TX-100 at 4°C and separated into pellets and supernatants by centrifugation, and the entire yield in each fraction was loaded in the gels for each condition. The figure represents a typical result of three independent experiments.

We conclude that cross-linking MOG on the surface of differentiatedOLs in culture results in a major change in its detergent solubilityproperties. We therefore initiated a series of experimentsto assess the time course, dose–response, biochemicalcharacteristics, and potential functional significance of theMOG cross-linking-mediated detergent insolubility of MOG.
MOG partitioning occurs during treatment with low doses and short durations of anti-MOG
The detergent insolubility of MOG in response to antibody cross-linkingwas studied as a function of dose and duration of treatmentof both the primary and secondary antibodies.
At a constant dilution of secondary antibody (1:100), the partitioningof MOG into the detergent-insoluble fraction was essentiallycomplete at dilutions of primary antibody ranging from 1:25(624 µg/ml IgG) to 1:500 (31 µg/ml IgG) (Fig. 3A). Treatment of OLs with anti-MOG (1:100) followed by 15min of cross-linking with secondary antibody (1:100, 23 µg/ml)as a function of time (Fig. 3B) resulted in the partitioninginto the insoluble fraction of $~$ 80% of MOG within 1 min andnearly all MOG within 5 min [with longer exposures (e.g., 1hr), a minor amount of MOG reappeared in the soluble fractionin some experiments].

View larger version (38K):
[in this window]
[in a new window]
Figure 3. MOG repartitioning as a function of antibody dose and incubation time. Western blot analysis of MOG in the insoluble pellet (P) and soluble (S) fractions during TX-100 extraction at 4°C of mature OLs after various treatments. A, 1° Ab dose–response: cells were incubated for 15 min with varying concentrations of anti-MOG mAb 8–18C5 (1:25–1:500), and then for 15 min with anti-mouse IgG (1:100); B, 1° Ab time course: cells were incubated for 1–60 min with anti-MOG mAb 8–18C5 (1:100), and then for 15 min with anti-mouse IgG (1:100); C, 2° Ab time course: cells were incubated for 15 min with anti-MOG mAb 8–18C5 (1:100), and then for 1–30 min with anti-mouse IgG (1:100); D, OLs incubated under the following conditions for 1° and 2° Ab doses and incubation times: control, no Ab (a); 1° Ab 1:100 15 min, 2° Ab 1:100 15 min (b); 1° Ab 1:100 5 min, 2° Ab 1:100 5 min (c); 1° Ab 1:100 5 min, 2° Ab 1:500 5 min; (d) 1° Ab 1:100 1 min, 2° Ab 1:500 1 min (e). Controls were similarly incubated with media alone. After scraping, cell lysates (20µg of protein) were extracted with TX-100 at 4°C and separated into pellets and supernatants by centrifugation, and the entire yield in each fraction was loaded in the gels for each condition. The figure represents a typical result of three independent experiments.

With primary antibody at a constant dilution (1:100) and durationof treatment (15 min), >90% of MOG partitioned into thedetergent-insoluble fraction during cross-linking with secondaryantibody dilutions up to 1:500 (data not shown). Under theseconditions, significant partitioning was observed within 1min and was nearly complete within 5 min (Fig. 3C).
On the basis of these results, the following conditions werechosen for subsequent analyses: anti-MOG, 1:100 for 5 min;cross-linking secondary antibody, 1:500 for 5 min. Nevertheless,at these antibody concentrations (anti-MOG 1:100; secondaryantibody 1:500) even 1 min incubations with each antibody resultedin $~$ 50% partitioning of MOG (Fig. 3D, e). We conclude thatthe cross-linking-induced partitioning of MOG into a detergent-insolublefraction occurs rapidly and at low concentrations of antibody.
Detergent-insoluble MOG from differentiated OLs in culture has both low- and high-density components
Insolubility of a protein in TX-100 at 4°C by itself isnot sufficient to conclude that these proteins are associatedwith lipid rafts; insolubility can also be derived from protein–proteininteractions with, for example, cytoskeletal elements (Pfeifferet al., 1993; De Angelis and Braun, 1996; Kim and Pfeiffer, 1999; Taylor et al., 2002). We therefore applied three additional,well established biochemical criteria. During TX-100 extractionat 4°C, raft-associated proteins float to a characteristic,low-bouyant density in density (e.g., sucrose) gradients (Brownand Rose, 1992; Simons and Ikonen, 1997); raft-associatedproteins insoluble in TX-100 at 4°C generally become solubilizedwhen the extraction is performed either at 37°C (Brownand Rose, 1992) or at 4°C after previous treatment withthe cholesterol-binding agent saponin (Rothberg et al., 1990; Cerneus et al., 1993; Hanada et al., 1995; Stulnig et al.,1997; Ledesma et al., 1998). These three criteria are fulfilledby MOG present in the detergent-insoluble fraction obtainedduring treatment of purified myelin with TX-100 at 4°C (Kim and Pfeiffer, 1999; Taylor et al., 2002) (Fig. 4A).

View larger version (59K):
[in this window]
[in a new window]
Figure 4. Further analyses of the TX-100-insoluble fractions. Western blot analyses of MOG were performed on either purified myelin (extraction at 4°C) (A) or treated OLs (B) [anti-MOG mouse mAb 18–18C5 (1:100, 5 min) followed by anti-mouse IgG (1:500, 5 min)]. OLs were extracted with TX-100 at 4°C, 37°C, and 4°C after pretreatment of the cell lysate with saponin (Saponin 4°C) or MCD 4°C after pretreatment of the cells in culture with 5 mM methyl ${beta}$ -cyclodextrin for 15 min at 37°C. The insoluble fractions (myelin, 50 µg; OLs, 300 µg of protein) were then further fractionated by centrifugation on sucrose gradients as described in Materials and Methods (fraction 1, top of gradient; i.e., lowest density). C, D, Western blot analysis of GM1 detected by reaction with cholera toxin B subunit (C) or caveolin after various treatments (D) as described above in B. OLs were untreated (Control 4°C) or first antibody-treated (above) and extracted with TX-100 at 4°C (Treated 4°C) or 37°C (Treated 37°C) or at 4°C after pretreatment with saponin (Treated Saponin 4°C). P and S are the insoluble and soluble fractions, respectively, after extraction with TX-100 at the indicated temperatures. S1, Soluble fraction after pretreatment of the cell lysate with saponin; S2, soluble fraction after pretreatment with saponin followed by extraction with TX-100 at 4°C. Cell lysate (5 µg of protein in A; 20 µg of protein in B) was extracted, and the entire yield in each fraction was loaded in the gels for each condition (A, B, right panel). Typical results of four independent experiments are shown.

In contrast to myelin, the detergent-insoluble MOG from antibody cross-linked OLs (Fig. 2A) was distributed in both light andheavy fractions during floating on sucrose gradients, bothof which were poorly solubilized by extraction with TX-100at 37°C (Fig. 4B). On the other hand, pretreatment of thecell lysate with saponin, or depletion of cholesterol by previoustreatment of the OLs with methyl ${beta}$ -cyclodextrin (see Fig. 6A,B),did result in efficient solubilization of the light fractions(but much less efficiently for the heavy fractions) during extraction with TX-100 at 4°C (Fig. 4B). The small amountof detergent-insoluble material obtained from untreated controlcells had similar characteristics as that from cross-linkedcells (data not shown). The light fraction was further analyzed for the presence of GM1 ganglioside (a widely used marker forlipid rafts) and caveolin (a marker of caveolae, a subgroupof lipid rafts) (Abrami et al., 2001) (Fig. 4C,D). Both of these markers were enriched in the light fractions during TX-100extraction at 4°C, were completely solubilized during extractionat 37°C or pretreatment with saponin, and were similarlydistributed in control and MOG cross-linked cells. We concludethat during antibody cross-linking, MOG becomes repartitionedinto a preexisting TX-100-insoluble (4°C) fraction withkey characteristics of lipid rafts (low density, solubilizationby saponin pretreatment, GM1, caveolin) and a higher densityfraction that is likely to be based on protein–proteininteractions.

View larger version (78K):
[in this window]
[in a new window]
Figure 6. Removal of cholesterol, or depolymerization of microfilaments or microtubules, in OLs in culture. Treatment with MCD, nocodazol, or cytochalasin D resulted in the removal of nearly all of the cholesterol (A, B) or depolymerization of microtubules (C, D) or actin microfilaments (E, F), respectively. A, B, Mature OLs in culture were either not treated (A) or treated with 5 mM MCD for 15 min (B) before staining with filipin to assess the efficiency of removal of cholesterol by the drug.C, D, Mature OLs in culture were either not treated (C) or treated with 10 µM nocodazol for 2 hr (D) to assess the efficiency of depolymerization of microtubules by the drug, as analyzed by immunostaining with anti-tubulin antibodies. E, F, Mature OLs in culture were either not treated (E) or treated with 20 µM cytochalasin D for 2 hr (F) to assess the efficiency of depolymerization of actin microfilaments by the drug, as analyzed by immunostaining with anti-actin antibodies. See Materials and Methods for details. Scale bar, 5 µ.

Role of the cytoskeleton in MOG cross-linking
Dyer and Matthieu (1994) reported that MOG becomes associatedwith microtubules after long exposures of OLs to high dosesof anti-MOG antibodies. Because cytoskeletal elements can be insoluble in TX-100 at 4°C (Pereyra et al., 1988), thedistributions on sucrose gradients of tubulin and actin inthe TX-100-insoluble material (4°C) were analyzed (Fig.5A). As for MOG, both proteins were present in both the lightand heavy fractions. However, in contrast to MOG, both tubulinand actin in the light fractions were solubilized during TX-100extraction at 37°C, as well as at 4°C after saponinpretreatment (Fig. 5A). When OLs were first treated with eithernocodazol or cytochalasin D to depolymerize microtubules ormicrofilaments, respectively (Fig. 6C–F), the redistributionof MOG into the insoluble fraction (TX-100, 4°C) was nearlyentirely eliminated, and the small amount of remaining insolublematerial was present in the heavy fractions (Fig. 5B,C). However,further analysis on sucrose gradients showed that under these conditions caveolin, tubulin, and actin were also present inthe heavy fractions (Fig. 5C), suggesting that cytoskeletaldisruption affected raft integrity in general rather than theredistribution of MOG in particular.

View larger version (43K):
[in this window]
[in a new window]
Figure 5. Role of cytoskeletal proteins in lipid raft formation and MOG repartitioning. Control and antibody-treated [anti-MOG mAb 8–15C5 (1:100, 5 min), anti-mouse IgG (1:500, 5 min)] OLs in culture were detergent extracted. The soluble (S) and insoluble pellet (P) fractions during TX-100 extraction (4°C or 37°C, or pretreatment with saponin followed by TX-100 extraction at 4°C) were analyzed by Western blot. A typical result from three independent experiments is shown. A, Analysis of phospho- ${beta}$ -tubulin (P-Tub), ${beta}$ -tubulin (Tub), and actin (Actin). Insoluble fractions (300 µg of protein) were loaded on sucrose gradients, and fractions were collected from the top (1) to the bottom (10) of the gradient. S, Soluble fraction after TX-100 extraction at 4 or 37°C; S1, soluble fraction after pretreatment with saponin; S2, soluble fraction after pretreatment with saponin followed by extraction with TX-100 at 4°C. Note that essentially all of the tubulin becomes dephosphorylated during cross-linking of MOG; tubulin and actin that are present in the low-density fractions (3–5) when cells are extracted at 4°C become soluble when extractions are performed at 37 or 4°C after pretreatment with saponin. B, Western blot analysis of MOG after a 2 hr pretreatment with either 20 µM cytochalasin D or 10 µM nocodazol. Soluble and insoluble fractions from control and antibody-treated cells after extraction with TX-100 at 4°C are Sc, Pc, St, and Pt, respectively. Cell lysate (20 µg of protein) was extracted, and the entire yield in each fraction was loaded in the gels for each condition. Note that the repartitioning of MOG into lipid rafts during cross-linking is virtually eliminated during dissociation of the actin (cytochalasin D) or tubulin (nocodazol) cytoskeleton. C, The TX-100 (4°C)-insoluble fractions from drug-and antibody-treated cells (B, Pt) were analyzed on sucrose gradients (300 µg of protein). Note that not only MOG but also caveolin, tubulin, and actin are absent from the low-density DIG fractions (3–5) during pretreatment of the cells with cytoskeleton-disrupting agents.

Specific proteins are phosphorylated in response to MOG antibody cross-linking
In a number of systems, ligand- or antibody-mediated partitioningof proteins into lipid rafts results in the initiation of signaltransduction cascades (Simons and Toomre, 2000). Because phosphorylationof proteins is an integral part of signal transduction mechanisms,we examined by Western blotting the phosphorylation state oftyrosine, serine, and threonine residues in proteins from untreatedand cross-linked OLs.
After cross-linking, two proteins present in the detergent-insoluble material became either tyrosine phosphorylated ( $~$ 160 kDa) (Fig.7A) or dephosphorylated (50 kDa) [(Fig. 7A) nonreducing gel];these changes in phosphorylation were not found in the detergent-solublematerial (data not shown). The $~$ 160 kDa phosphotyrosine bandwas present in both the light and heavy fractions during floatingon sucrose gradients; in contrast, the $~$ 50 kDa dephosphorylated protein was exclusively in the light fraction (Fig. 5A) (anddata not shown). These changes in phosphorylation were notfound when cells were treated with anti-MOG without secondaryAb (data not shown), and they were prevented if cells werepretreated with either a general tyrosine kinase (PD166285)(Fig. 7A) or phosphatase (vanadate) inhibitor (data not shown).

View larger version (68K):
[in this window]
[in a new window]
Figure 7. Altered protein phosphorylation mediated by MOG cross-linking. The soluble and insoluble fractions from TX-100 extractions (4°C; 20 µg of total cell protein was extracted and the entire protein yield in each fraction was loaded) of untreated control and antibody-treated [anti-MOG mAb 8–15C5 (1:100, 5 min), anti-mouse IgG (1:500, 5 min)] OLs in culture were analyzed by Western blot for protein phosphorylation. P, Insoluble pellet fraction; S, soluble fraction; c, control; t, treated to achieve cross-linking. The positions on the gels of proteins for which the phosphorylation pattern was altered by cross-linking are indicated by closed circles attached to short lines. Typical results from three independent experiments are shown. A, Western blots for proteins containing phosphotyrosine were analyzed by either reducing or nonreducing gel electrophoresis. The nonreducing gels were performed to demonstrate that the $~$ 50 kDa protein (weakly present in reducing gels, but not shown in A) was not residual antibody heavy chain. In some cases the cells were pretreated for 3 hr with 0.1 µM PD166285, a general tyrosine kinase inhibitor (A). A protein of $~$ 160 kDa was detected that became phosphorylated during MOG cross-linking. A second phosphoprotein of $~$ 50 kDa was identified that became dephosphorylated during cross-linking. B, Western blot for proteins containing phosphothreonine. A protein of $~$ 35 kDa was detected that became partially dephosphorylated during MOG cross-linking. C, Western blot for proteins containing phosphoserine. Two proteins ( $~$ 70 and 100 kDa) that became phosphorylated during MOG cross-linking were detected. The phosphorylation of the $~$ 70 kDa protein(s) was strongly upregulated in both the soluble and insoluble fractions. The phosphorylation of the $~$ 100 kDa protein(s) was strongly upregulated in the insoluble fraction and significantly so in the soluble fraction. Examples of potentially altered phosphorylation states in other proteins were tentatively identified but are not indicated.

Analyses with anti-phosphothreonine antibody identified a proteinthat in the insoluble fraction (TX-100, 4°C) became dephosphorylatedduring cross-linking ( $~$ 35 kDa). This protein has characteristicsof a raft-associated protein (insoluble in TX-100 at 4°C,recovered at low density in sucrose gradients, soluble in TX-100at 37°Corat4°C after cholesterol extraction) (Fig. 7B) (and data not shown). Analyses with anti-phosphoserinein Western blots revealed the appearance during cross-linkingof at least two phosphoserine proteins ( $~$ 70 and $~$ 100 kDa) (Fig.7C).
Levels of phospho-fyn, FAK (focal adhesion kinase), and MAPK (mitogen-activated protein kinase) were not changed after MOGcross-linking (data not shown).
We next attempted to identify proteins that change their phosphorylation status during MOG cross-linking by two-dimensional PAGE, analyzedby silver staining and Western blot with anti-phosphotyrosine,anti-phosphoserine, or anti-phosphothreonine antibodies. Asimilar pattern of proteins (silver-stained gels) was observedin control and cross-linked cells, indicating that the overallprotein content and profile were not changed during MOG cross-linking(Fig. 8A). Phosphotyrosine Western blots of MOG cross-linked samples again detected the newly phosphorylated $~$ 160 kDa andthe dephosphorylated $~$ 50 kDa proteins (Fig. 8B). The $~$ 50 kDatyrosine dephosphorylated protein was identified by mass spectrometryand confirmed by Western blot analysis to be ${beta}$ -tubulin (Fig. 8C). The relatively low abundance of the $~$ 160 kDa protein precludedits identification by mass spectrometry. Phosphoserine Westernblots of MOG cross-linked samples resolved the newly phosphorylated ( $~$ 70 kDa) protein observed on one-dimensional PAGE gels (Fig.7C) into three proteins with different isoelectric points (Fig. 8D). Phosphothreonine Western blot analysis (Fig. 8E,F)detected the newly dephosphorylated $~$ 35 kDa protein, identifiedby mass spectrometry and confirmed by Western blot analysisto be the ${beta}$ (1–2) subunit of the heterotrimeric G-proteincomplex.

View larger version (69K):
[in this window]
[in a new window]
Figure 8. Two-dimensional PAGE profiles of OL proteins before and after MOG cross-linking. Cell lysates (300 µg of total cell protein) from untreated and antibody-treated [anti-MOG mAb 8–15C5 (1:100, 5 min), anti-mouse IgG (1:500, 5 min)] OLs in culture were analyzed by two-dimensional electrophoresis. After cross-linking, the cells were harvested by scraping into collection buffer (25 mM Tris-HCl, pH 7.5, 2% CHAPS, 1 mM PMSF, 10 µg/ml leupeptin–aprotinin, 50 mM NaF, 10 mM NaP₂O₇, and 1 mM Na o-vanadate). Proteins were then precipitated with 2 vol of ethanol at –20°C and resolubilized into rehydration buffer (see Materials and Methods). Typical results from three independent experiments are shown. A, Silver staining. No significant differences in the patterns of proteins from control and treated cells were noted. B, Anti-phosphotyrosine. Two proteins of $~$ 160 kDa/pI $~$ 4.5 and $~$ 70 kDa/pI $~$ 6 were identified that became tyrosine phosphorylated, and one phosphotyrosine protein of $~$ 50 kDa/pI $~$ 5 was identified that became dephosphorylated, during MOG cross-linking. C, Anti- ${beta}$ -tubulin. The $~$ 50 kDa/pI $~$ 5 phosphotyrosine protein that became dephosphorylated during MOG cross-linking (A, B) is identified as ${beta}$ -tubulin (confirmed by mass spectroscopy). D, Anti-phosphoserine. A triplet of proteins of $~$ 70 kDa/pI $~$ 6.5 became further serine phosphorylated; their identity is currently unresolved. E, Anti-phosphothreonine. A phosphothreonine protein of $~$ 35 kDa/pI $~$ 6 becomes dephosphorylated during MOG cross-linking. F, Anti-phosphothreonine pretreated with a 50-fold excess of phosphothreonine to control for the specificity of the antibody. G, Anti-G ${beta}$ subunit of the trimeric G-protein. The $~$ 35 kDa/pI $~$ 6 phosphothreonine protein that becomes dephosphorylated during MOG cross-linking (E) is identified as the ${beta}$ -subunit of the heterotrimeric G-protein complex (initially identified by mass spectrometry). Squares indicate proteins for which the tyrosine phosphorylation pattern is altered during MOG cross-linking (A–C). Arrowheads indicate the triplet of serine-phosphorylated proteins (D), and circles indicate threonine-dephosphorylated G ${beta}$ subunit (A, E, F, G) after MOG cross-linking.

We conclude that cross-linking MOG on the surface of differentiatedOLs growing in culture leads to the phosphorylation–dephosphorylationof tyrosine, serine, or threonine residues in specific proteins.
MOG cross-linking in the presence of tyrosine kinase or serine–threonine phosphatase inhibitors
The redistribution of MOG into the pellet (TX-100, 4°C)after MOG cross-linking was not affected by pretreatment ofOLs with the general tyrosine kinase inhibitor PD166285, theserine–threonine phosphatase inhibitor okadaic acid (Fig. 9A), or the general phosphatase inhibitor vanadate (data notshown). This suggests that the observed phosphorylation changeselicited by these activities are a consequence, rather thanthe cause, of MOG redistribution.

View larger version (65K):
[in this window]
[in a new window]
Figure 9. Changes in OL morphology during cross-linking of MOG. OLs in culture were either left untreated as controls (see Materials and Methods) or antibody treated [anti-MOG mAb 8–15C5 (1:100, 5 min), anti-mouse IgG (1:500, 5 min)]. A, Cell lysates were extracted with TX-100 (4°C; 20 µg total cellular protein) and separated into insoluble (P) and soluble (S) fractions by centrifugation, and the entire protein yield of the fractions was analyzed for MOG by Western blotting. c, Control; t, treated to achieve cross-linking. Pretreatment with either a tyrosine kinase (PD166285) or a serine–threonine phosphatase (okadaic acid) inhibitor did not affect the repartitioning of MOG into the insoluble fraction. B, Cells were immunostained with O4 antibody for epifluorescence microscopy. Scale bar, 5 µ. C, The areas occupied by randomly chosen cells were calculated by measuring the number of pixels per cell using Adobe Photoshop 5.0. B, C, Lowercase letters (a, c, e): no anti-MOG cross-linking; (b, d, f): anti-MOG cross-linked; (a, b₀): no further treatment; (b₂, b₄, b₁₄): the antibody-containing medium was removed, and the cells were grown further in fresh medium for 2 (b₂), 4 (b₄), or 14 hr (b₁₄). c, d, Pretreatment for 3 hr with 0.1 µM PD166285, a tyrosine kinase inhibitor; e, f, pretreatment for 3 hr with 10 nM okadaic acid, a serine–threonine phosphatase inhibitor. ***, a/b₀, and b₀/b₁₄ indicate statistically significant differences, p $<=$ 0.0001; the values of a, c–f, and b₀, b₂, and b₄ are not significantly different (p > 0.5). Error bars represent SEM; n = 20–35. Note that inhibition of phosphorylation or dephosphorylation did not alter the antibody-mediated repartitioning of MOG but did block the changes in morphology observed during MOG cross-linking of uninhibited cells. The effect of MOG cross-linking on OL morphology was reversible.

Morphological alterations in OLs after MOG cross-linking
Tubulin dephosphorylation in neurons is associated with growthcone collapse (Atashi et al., 1992). Therefore, the effectof cross-linking MOG and the accompanying tubulin dephosphorylationon the extension and integrity of OL processes (identified by O4 antibody staining, a marker for OLs) was examined (Fig.9B,C). After MOG cross-linking (anti-MOG mAb 1:100, 5 or 15min, and then anti-mouse IgG 1:500, 5 or 15 min), mature OLsunderwent dramatic retraction of cell processes and membranesheets, with a consequent reduction in the area occupied bythe OLs (Fig. 9, compare a, b₀,) (p < 0.0001). These changesin morphology were not observed in OLs treated with anti-MOGantibody alone (no cross-linking with secondary antibody),and they were prevented entirely if OLs were treated with eithera general tyrosine kinase inhibitor (PD166285) (Fig. 9c,d)or a serine–threonine phosphatase inhibitor (okadaicacid) (Fig. 9e,f) before and during MOG cross-linking. Essentiallyidentical results were obtained when the immunocytochemicalanalyses were performed using antiserum against myelin basicprotein (MBP), marker of mature OLs, to estimate the areas occupiedby OLs (data not shown). We conclude that MOG cross-linkingleads to a reversible retraction of myelin-like membranes andprocesses as the result of alterations in phosphorylation ofsignal transduction and cytoskeletal proteins. The potentialsignificance of these changes for demyelinating disease is intriguing.
Reversibility of MOG cross-linking
To assess the reversibility of MOG cross-linking-mediated events,the antibody was removed, and the cells were refed with freshmedium and further incubated at 37°C. Within 15 min boththe amount of MOG that was insoluble in TX-100 at 4°C andthe level of phosphorylation of ${beta}$ -tubulin returned nearly tolevels observed in untreated control cells (Fig. 10A,B) (after 30 min, only a very small amount of MOG was still present inthe detergent-soluble fraction; data not shown). These resultsindicate that MOG repartitioning and ${beta}$ -tubulin dephosphorylationafter MOG cross-linking in OLs is rapidly reversible and that ${beta}$ -tubulin dephosphorylation is observed only when a significantamount of MOG is present in the insoluble fraction. Similarly,reversibility occurred with regard to cross-linking-inducedchanges in morphology. When the antibody-containing mediumwas removed and the cells were further incubated with freshculture medium at 37°C, within 2–4 hr the treatedOLs began to re-extend processes and increase their occupiedarea and underwent substantial recovery of process extension(to >75% of control cultures) within 14 hr of incubation(Fig. 9C, b₀, b₂, b₄, b₁₄). Thus, morphological recovery,albeit substantial, is a slower event than the return to controllevels of MOG partitioning and phosphorylation states.

View larger version (59K):
[in this window]
[in a new window]
Figure 10. Reversibility of MOG repartitioning and tubulin dephosphorylation. OLs in culture were first either left untreated as controls (Pc, Sc) or antibody-treated [Pt, St; anti-MOG mAb 8–15C5 (1:100, 5 min), anti-mouse IgG (1:500, 5 min)]. The control and antibody-containing media were then removed, and the cells were grown further in fresh medium (Pcr, Ptr) for 15 min. Cell lysate (20 µg of protein) was extracted with TX-100 (4°C) and separated into soluble (S) and insoluble (P) fractions by centrifugation, and the entire yield in each fraction was loaded in the gels for each condition and analyzed by Western blot. Typical results from three independent experiments are shown. A, Anti-MOG; B, anti- ${beta}$ -tubulin (phosphotubulin and total tubulin). Immediately after cross-linking followed by removal of the antibody (0; Pt, St), as expected (above), nearly all MOG is recovered in the insoluble (P) fraction (A), and nearly all ${beta}$ -tubulin is dephosphorylated (B). However, within 15 min after removal of the antibody (15; Ptr, Str), nearly all MOG is now recovered once again in the soluble fraction (Str), and ${beta}$ -tubulin has become rephosphorylated to a level nearly equal to that of untreated controls.

   Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Cross-linking of membrane proteins is a physiological phenomenonthat can lead to the repartitioning of these proteins intolipid rafts, resulting in novel protein interactions and initiationof cell signaling (Simons and Toomre, 2000; Ikonen, 2001).Although occurring naturally via multivalent ligands, similarresponses have been observed using antibodies (Simons and Toomre, 2000).
In this report we show that although MOG in OLs in culture ismostly detergent soluble (TX-100, 4°C), it becomes repartitionedinto a detergent-insoluble fraction during antibody-inducedcross-linking (anti-MOG + secondary antibody). Concomitantly,there is an upregulation of the phosphorylation or dephosphorylationof tyrosine, serine, or threonine residues in specific proteins,accompanied by a dramatic retraction of myelin-like membranesheets and cellular processes. These observations are consistentwith a model proposing that during MOG-cross-linking, specific signal transduction pathways are activated, resulting in alterationsin the maintenance of OL cell processes and myelin-like membrane.This repartitioning of MOG is rapid ( $<=$ 1 min) and reversibleand occurs at concentrations of antibody substantially lowerthan previously used to perturb OLs in culture (Dyer and Matthieu,1994). After the detergent-insoluble fraction is floated onsucrose gradients, MOG is distributed between light- and heavy-densityfractions. The low-density fraction has characteristics oflipid rafts; these include, in addition to its low density,sensitivity to pretreatment with cholesterol perturbing agents before detergent extraction (TX-100, 4°C) that renders MOGsoluble. The heavy-density fraction is enriched in the cytoskeletalproteins ${beta}$ -tubulin and ${beta}$ -actin, suggesting that protein–proteininteractions are involved.
After MOG cross-linking there are specific changes in the phosphorylation of tyrosine, serine, and threonine residues of specific detergent-insoluble proteins that are associated with rafts, including ${beta}$ -tubulinand G ${beta}$ 1–2. We propose that there is a causal relationshipbetween partitioning of MOG into the detergent-insoluble fractionsand the induced phosphorylation–dephosphorylation events.Although the partitioning of MOG is independent of cellulartyrosine kinase or serine–threonine phosphatase activities,the retraction of cell processes requires the changes in phosphorylationstate. Therefore, we speculate a sequence of events in whichMOG cross-linking induces repartitioning, implementing novel protein–protein interactions within lipid rafts, followedin turn by specific changes in protein phosphorylation state,resulting in cellular morphological alterations.
Moreover, this study, as well as others (Holowka et al., 2000; Fassett et al., 2001; Nebl et al., 2002), indicates that raftintegrity depends on intact microtubules and microfilaments. Consistent with this, although the bulk of tubulin and actinwere found in the heavy detergent-soluble fraction, significantlevels of these proteins were also identified in the low-densitylipid raft fraction, suggesting a close relationship betweencytoskeletal elements and rafts (Holowka et al., 2000; Maekawaet al., 2001; this study). This is strongly supported by ourobservation that disruption of the cytoskeleton leads to aconcomitant disruption of the OL lipid rafts, as indicatedby the redistribution of raft markers (e.g., caveolin) fromthe detergent-insoluble light fraction to the heavy fraction.
The identification of proteins that change their phosphorylationstatus after MOG cross-linking is a key step toward identifyingmechanisms leading to altered cell physiology. In particular,we identified the dephosphorylation of ${beta}$ -tubulin and G-protein ${beta}$ subunit. ${beta}$ -tubulin dephosphorylation affects microtubule polymerization(Atashi et al., 1992) and is likely to be a factor in the lossof OL membrane reported in this study (acute anti-MOG exposure)and by Dyer and Matthieu (1994) (chronic anti-MOG exposure).The G-protein ${beta}$ ${gamma}$ complex regulates the activity of a diverseset of effectors, including phospholipases, adenyl cyclases,and ion channels (Clapham and Neer, 1997). Phosphorylationof the ${beta}$ subunit activates the dissociated G ${beta}$ ${gamma}$ complex (Sternweis,1994; Nürnberg et al., 1996). The dephosphorylation ofG ${beta}$ ${gamma}$ complex could therefore affect a number of different downstreamsignaling pathways.
MOG is clearly implicated in demyelinating disease. Immunologicalstudies in humans also identified MOG as a prevalent antigenicmolecule among the myelin proteins (Von Büdingen et al., 2001). The encephalitogenic properties of MOG are mainly linkedto the induction of antibody responses, which directly promotedemyelination in CNS disorders such as MS. Although autoimmuneresponses directed against CNS antigens have generally beenconsidered pathogenic, some reports show that both cellularand humoral immune responses can promote tissue repair afterCNS injury and disease. In particular, the exciting observationthat some polyreactive IgM autoantibodies reacting with OLsurface antigens (not well characterized yet) promote myelinrepair (Warrington et al., 2000; Bieber et al., 2001, 2002),as well as the previous finding that the IgM antibody O4 (againstsulfogalactolipids) enhances OL differentiation (Bansal etal., 1988), suggests their possible application as therapeutic agents.
In rat and marmoset models, MOG-induced EAE demyelination isanti-MOG antibody dependent and reproduces the immunopathologyseen in many cases of MS. The demyelinating activity of MOG-specificantibody has often been related to its ability to activatecomplement, which could compromise the metabolic integrityof the cell and/or directly kill OLs and thus disrupt myelin (Piddlesden et al., 1993; for review, see Iglesias et al., 2001; Von Büdingen et al., 2001). The finding that purifiedMOG binds C1q (Johns and Bernard, 1997) strengthens this hypothesis.However, MBP degradation and membrane loss leading to anti-MOG-induceddemyelination was also found in models independent of complementaction (Dyer and Matthieu, 1994; Menon et al., 1997; thisreport).
We propose a new, complement-independent model for MOG/anti-MOG-induced demyelination. According to this model, elevated titers of anti-MOGantibody lead to a sequence of events: (1) cross-linking ofMOG results in the repartitioning of a large fraction of MOGinto DIGs; (2) MOG forms complexes with specific protein partners(e.g., kinases and phosphatases) that are in DIGs; (3) specificsignaling pathways become activated; (4) alterations of OL physiology critical for membrane maintenance are elicited. Wepropose further that similar events may occur in MS. Severalquestions need to be addressed, including whether antibodycross-linking is mimicking or exacerbating, or both, the actionof an endogenous ligand, in which case this signaling could be related not only to anti-MOG-induced demyelination but alsoto normal MOG function within the OLs.

   Footnotes

Received Jan. 10, 2003; revised Mar. 14, 2003; accepted Apr. 11, 2003.
This work was supported by National Institutes of Health GrantsNS10861 and NS41078 and in part by a Post-doctoral Fellowshipfrom the National Multiple Sclerosis Society. We thank Dr.Christopher Linington for providing anti-MOG antibody and forfruitful discussions. We are pleased to acknowledge the excellentadministrative support of Wendy Wolcott, Janice Seagren, and Jennifer Gilman.
Correspondence should be addressed to Cecilia Marta, Departmentof Neuroscience, University of Connecticut Medical School,263 Farmington Avenue, Farmington, CT 06030-3401. E-mail: Marta{at}up.uchc.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235461-11$15.00/0

   References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Abrami l, Fivaz M, Kobayashi T, Kinoshita T, Parton R, Van der Goot FG (2001) Cross-talk between caveolae and glycosylphosphatidylinositol-rich domains. J Biol Chem 276: 30729–30736.[Abstract/Free Full Text]
Atashi JR, Klinz SG, Ingraham CA, Matten WT, Schachner M, Maness S (1992) Neural cell adhesion molecules modulate tyrosine phosphorylation of tubulin in nerve growth cone membranes. Neuron 8: 831–842.[ISI][Medline]
Bansal R, Pfeiffer SE (1985) Developmental expression of 2',3'-cyclic nucleotide 3'-phosphohydrolase in dissociated fetal rat brain cultures and rat brain. J Neurosci Res 14: 21–34.[Medline]
Bansal R, Pfeiffer SE (1989) Reversible inhibition of oligodendrocyte progenitor differentiation by a monoclonal antibody against surface galactolipids. Proc Natl Acad Sci USA 86: 6181–6185.[Abstract/Free Full Text]
Bansal R, Gard AL, Pfeiffer SE (1988) Stimulation of oligodendrocyte differentiation in culture by growth in the presence of a monoclonal antibody to sulfated glycolipid. J Neurosci Res 21: 260–267.[ISI][Medline]
Bansal R, Warrington AE, Gard AL, Ranscht B, Pfeiffer SE (1989) Multiple and novel specificities of monoclonal antibodies O1, O4, and R-mAb used in the analysis of oligodendrocyte development. J Neurosci Res 24: 548–557.[ISI][Medline]
Bansal R, Kumar M, Murray K, Morrison RS, Pfeiffer SE (1996) Regulation of FGF receptors in the oligodendrocyte lineage. Mol Cell Neurosci 7: 263–275.[ISI][Medline]
Bansal R, Winkler S, Bheddah S (1999) Negative regulation of oligodendrocyte differentiation by galactolipids. J Neurosci 19: 7913–7924.[Abstract/Free Full Text]
Bieber AJ, Warrington A, Pease LR, Rodriguez M (2001) Humoral autoimmunity as a mediator of CNS repair. Trends Neurosci [Suppl] 24: S39–44.[Medline]
Bieber AJ, Warrington A, Asakura K, Ciric B, Kaveri SV, Pease L, Rodriguez M (2002) Human antibodies accelerate the rate of remyelination following lysolecithin-induced demyelination in mice. Glia 37: 241–249.[ISI][Medline]
Bottenstein J, Sato G (1979) Growth of a rat neuroblastoma line in serum-free supplemented medium. Proc Natl Acad Sci USA 76: 514–517.[Abstract/Free Full Text]
Brown DA, London E (1998) Structure and origin of ordered lipid domains in biological membranes. J Membr Biol 164: 103–114.[ISI][Medline]
Brown DA, Rose JK (1992) Sorting of GPI-anchored proteins to glycolipid-enriched membrane subdomains during transport to the apical cell surface. Cell 68: 533–544.[ISI][Medline]
Cerneus D, Ueffing E, Posthuma G, Strous G, Van der Ende A (1993) Detergent insolubility of alkaline phosphatase during biosynthetic transport and endocytosis. J Biol Chem 268: 3150–3155.[Abstract/Free Full Text]
Clapham DE, Neer EJ (1997) G protein beta gamma subunits. Annu Rev Pharmacol Toxicol 37: 167–203.[ISI][Medline]
De Angelis DA, Braun PE (1996) 2',3'-cyclic nucleotide 3'-phosphodiesterase binds to actin-based cytoskeletal elements in an isoprenylation-independent manner. J Neurochem 67: 943–951.[ISI]