Targeting of IgMkappa  Antibodies to Oligodendrocytes Promotes CNS Remyelination

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The Journal of Neuroscience, October 1, 1998, 18(19):7700-7708

Targeting of IgM $kappa$ Antibodies to Oligodendrocytes Promotes CNS Remyelination
Kunihiko Asakura¹^,², David J. Miller², Larry R. Pease², and Moses Rodriguez¹^,²
Departments of ¹ Neurology and ² Immunology, Mayo Clinic and Foundation, Rochester, Minnesota 55905

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We previously identified the remyelinating activity of a natural IgM $kappa$ oligodendrocyte-reactive autoantibody (SCH94.03), usinga virus-induced murine model of multiple sclerosis. We now describea second mouse IgM $kappa$ monoclonal antibody (mAb) (SCH79.08) raisedagainst normal mouse spinal cord homogenate, which reacts withmyelin basic protein and also promotes remyelination. Becausethese two mAbs recognize different oligodendrocyte antigens, severalpreviously identified oligodendrocyte-reactive IgM $kappa$ mAbs (O1,O4, A2B5, and HNK-1), each with distinct antigen specificities,were evaluated and found to promote remyelination. In contrast,IgM $kappa$ mAbs that did not bind to oligodendrocytes showed no remyelination.One of these, CH12 IgM $kappa$ mAb, which shares variable region cDNAsequences with SCH94.03 except for amino acid differences in thecomplementarity-determining region 3 in both heavy and light chains,did not bind to oligodendrocytes and did not promote remyelination.The fact that multiple oligodendrocyte-reactive antibodies withdistinct antigen reactivities induce remyelination argues againstdirect activation by a unique cell surface receptor. These findingsare most consistent with the hypothesis that the binding of mAbsto oligodendrocytes in the lesions induces myelin repair via indirectimmune effector mechanisms initiated by the µ-chain. Importantly,these studies indicate that oligodendrocyte-reactive natural autoantibodiesmay provide a powerful and novel therapeutic means to induce remyelinationin multiple sclerosis patients.

Key words: Theiler's virus; oligodendrocytes; demyelination; natural autoantibody; remyelination; multiple sclerosis; immunoglobulin

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Demyelination in association with inflammation is the primary structural abnormality in multiple sclerosis (MS). Spontaneousremyelination is limited in the CNS, in part because oligodendrocytesare considered to be postmitotic cells. However, spontaneous remyelinationis observed at the edge of MS plaques (Prineas and Connell, 1979).Studies have shown that oligodendrocyte/type-2 astrocyte (O-2A)progenitor cells persist in the adult CNS and proliferate (Wolswijkand Noble, 1989; Armstrong et al., 1992). Alternatively, it hasbeen shown that mature oligodendrocytes can be induced to generatenew myelin under the influence of neurons (Wood and Bunge, 1991).Basic fibroblast growth factor induces mature oligodendrocytesto reenter the cell cycle (Fressinaud et al., 1993; Grinspan etal., 1993) and converts the cells to a novel phenotype (Bansaland Pfeiffer, 1997), providing another cellular mechanism forremyelination.

One of the major goals for the treatment of MS is to develop strategies to promote remyelination. One strategy shown in vivoto enhance endogenous myelination has been the use of naturalgermline antibodies that react to CNS antigens (Miller et al.,1994). This approach is particularly attractive because it rapidlycan be translated from the bench to the bedside as a therapy forhuman MS (Noseworthy et al., 1994; Fazekas et al., 1997).

We demonstrated that a mouse monoclonal antibody (mAb) raised against normal mouse spinal cord homogenate (SCH), designatedSCH94.03, enhanced CNS remyelination in the Theiler's murine encephalomyelitisvirus (TMEV) model of MS (Miller et al., 1994). SCH94.03 belongsto the IgM $kappa$ subclass, is highly polyreactive against known andunknown protein antigens including cytoskeletal proteins, andis encoded by unmutated Ig germline genes, confirming that SCH94.03is a natural autoantibody (Miller and Rodriguez, 1995a; Asakuraet al., 1996a). Of unique importance, SCH94.03 recognizes an unidentifiedsurface antigen on oligodendrocytes (Asakura et al., 1996b), providinga potential target for the mechanism of action of this antibody.

Two major hypotheses have been proposed by which SCH94.03 promotes remyelination. (1) The mAb may bind to a unique receptoron the surface of oligodendrocytes to induce myelination. Thishypothesis would predict that only a limited repertoire of Abswith unique specificity would function for myelin repair. (2)The mAb may work by binding to damaged oligodendrocytes and/ormyelin, which triggers a cascade of events by other resident CNScells (i.e., astrocytes, microglia, or neurons) and in turn enhancesmyelin repair. An attractive hypothesis is that binding to damagedoligodendrocytes and myelin may enhance the opsonization and clearingof CNS debris by macrophages, thus allowing for the normal processof remyelination to ensue. This hypothesis would predict thatmany polyreactive autoantibodies with specificity to oligodendrocytesand/or myelin would be effective. To address these hypothesesand the mechanism for Ab-mediated CNS remyelination, we set outto identify additional mAbs that promote CNS remyelination inTMEV model and compared their specificities with SCH94.03. Inaddition, we tested the remyelination-promoting activity of wellrecognized oligodendrocyte-reactive mAbs O1, O4, A2B5, and HNK-1,which previously were shown to have genotypic or phenotypic featuresof natural autoantibodies (Asakura et al., 1995).

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

mAb production and screening. Hybridomas were generated and screened as described (Miller et al., 1994). SJL/J mice were immunizedwith normal mouse SCH in incomplete Freund's adjuvant, and theirsplenocytes were fused with NS-1 myeloma cell. Hybridoma supernatantsthat showed high binding to SCH by ELISA were screened furtherfor their ability to promote remyelination in the TMEV model.Therefore, the Abs were screened on the basis of their abilityto promote CNS remyelination rather than for a unique antigenspecificity. IgM $kappa$ Abs were purified from hybridoma culture supernatantsby ammonium sulfate precipitation and dialysis against PBS pluslow-ionic-strength precipitation or by affinity chromatography,using goat anti-mouse IgM Ab (µ-chain-specific; Jackson ImmunoResearch,West Grove, PA) bound to carbonyldiimidazole-activated cross-linkedagarose (Reacti-Gel 6× matrix, Pierce, Rockford, IL).

Hybridomas and mAb preparation. Hybridomas A2B5, HNK-1, and R24 were purchased from American Type Culture Collection (ATCC,Rockville, MD). Hybridomas O1 and O4 were a gift from Dr. S. E.Pfeiffer (University of Connecticut, Farmington, CT). These hybridomaswere cultured in RPMI 1640 supplemented with 10% fetal calf serum(HyClone, Logan, UT) and 2 × 10² mM $beta$ -mercaptoethanol. B-cell lymphoma CH12 (CH12.Lx) was providedby Dr. G. Haughton (University of North Carolina, Chapel Hill,NC). To obtain secreted IgM from CH12 lymphoma, we stimulatedCH12.Lx cells with 50 µg/ml of lipopolysaccharide (Sigma, St.Louis, MO). mAbs O1, O4, and HNK-1 were purified from hybridomaculture supernatant by ammonium sulfate precipitation and dialysisagainst PBS plus low-ionic-strength precipitation. mAbs A2B5 andCH12 were purified by affinity chromatography. R24 was purifiedby protein A column. The purity of these mAbs was examined bySDS-polyacrylamide gel electrophoresis, and the immunoreactivityof these mAbs was examined by the immunostaining of rat oligodendrocytes.Control hybridoma XMMEN-OE5 producing anti-bacterial lipopolysaccharideIgM $kappa$ Ab was purchased from ATCC. Clarified ascites of controlABPC22 IgM $kappa$ mAb were purchased from Sigma. Both IgM $kappa$ mAbs werepurified by affinity chromatography, using goat anti-mouse IgMAb. The purity of the mAbs was confirmed by SDS-polyacrylamidegel electrophoresis.

Virus and animals. The Daniel's strain of TMEV was used for these experiments. Female SJL/J mice from the Jackson Laboratories(Bar Harbor, ME) were used after 1 week of rest. Mice from 4 to6 weeks of age were injected intracerebrally with 2 × 10⁵ plaque-forming units (pfu) of TMEV in a 10 µl volume. The handlingof all animals was in accordance with the institutional guidelinesprescribed by National Institutes of Health and Mayo Clinic.

mAb treatment and quantitative morphometry of remyelination. Chronically infected mice (5-6 months after infection) were givenintraperitoneal injections of mAb twice weekly for 5 weeks (50µg/injection). The total dose of each Ab was 0.5 mg. The micewere killed 2 weeks after the completion of mAb treatment. Lightmicroscopic sections were prepared as described (Miller et al.,1994). Mice were anesthetized with pentobarbital, exsanguinatedby cardiac puncture, and fixed by intracardiac perfusion withTrump's fixative (phosphate-buffered 4% formaldehyde containing1.5% glutaraldehyde, pH 7.2). The entire spinal cord was removedand sectioned into 1 mm transverse blocks. Every third block waspost-fixed in 1% osmium tetroxide and embedded in Araldite (Polysciences,Warrington, PA). One micrometer sections were cut and stainedwith p-phenylenediamine. Ten spinal cord sections of each mousewere examined. The total areas of white matter, demyelination,and remyelination on each section were quantitated by a Zeiss(Oberkochen, Germany) interactive digital analysis system. Thearea of demyelination was characterized by cellular infiltrates,macrophages engulfing myelin debris, and naked axons. Abnormallythin myelin sheaths relative to axon diameter were used as thecriterion for remyelination by oligodendrocytes. Those remyelinatedfibers were identified readily (as shown in Fig. 1). Remyelinatedareas were defined as a cluster of at least 10 remyelinated fibers.Spontaneous remyelination by Schwann cells also was present rarelyin the spinal cord lesions (Miller and Rodriguez, 1995b). Remyelinationby Schwann cell was characterized by abnormally thick myelin sheathsrelative to axon diameter, with a one-to-one relationship betweenaxons and Schwann cells. These peripheral-type remyelinated areaswere excluded from the quantitation. The quantitation was doneon coded sections without previous knowledge of the treatmentto avoid bias. Statistical comparison between groups in the extentof demyelination and remyelination was performed with an unpairedStudent's t test.

Cell culture and immunocytochemistry. Oligodendrocytes, astrocytes, and microglia were isolated from telencephalon of newbornSprague Dawley rats as described (Asakura et al., 1996b). Abswere diluted in PBS. Surface staining was performed at 4°C for15 min on unfixed cells after they were blocked with PBS containing3% normal goat serum (NGS). Cytoplasmic antigen staining was performedon cells fixed for 10 min at 4°C with 2% paraformaldehyde andtreated for 5 min at room temperature with 0.1% Triton X-100 inPBS, followed by blocking with 3% NGS in PBS. After incubationwith the primary Abs and the secondary FITC-conjugated anti-mouseIgM (µ-chain-specific) Ab (Jackson ImmunoResearch), the slideswere mounted in MOWIOL (Aldrich Chemical, Milwaukee, WI) containing2.5% 1,4-diazobicyclo-[2.2.2]-octane (DABCO; Sigma) and were viewedwith an epifluorescent microscope.

Immunohistochemistry. Fresh-frozen sections (10 µm) were prepared from various organs of neonatal (postnatal days 7 and 14)rats. Fresh-frozen sections were immunostained with primary Absand then were fixed with 4% paraformaldehyde or were lightly fixedwith acetone and then were immunostained with primary Abs. BoundAbs were detected by fluorochrome-conjugated secondary Ab or bythe avidin-biotin immunoperoxidase technique, using the VectastainABC kit (Vector Laboratories, Burlingame, CA). MOPC104E (Sigma)mouse IgM mAb was used as an isotype control.

Direct ELISA. Protein antigens, including human red blood cell (RBC) spectrin, bovine myosin (heavy chain), mouse albumin,mouse hemoglobin, mouse transferrin, hen egg lysozyme (HEL), rabbitactin, rabbit myelin basic protein (MBP), and keyhole limpet hemocyanin(KLH), were purchased from Sigma. Proteins were tested for purityby SDS-polyacrylamide gel electrophoresis. All chemical haptenswere purchased from Sigma and coupled to bovine serum albumin(BSA) (Miller and Rodriguez, 1995a). Protein antigens were usedat 5 µg/ml and haptens at 2 µM. The proteins and hapten-BSA antigenswere coated onto polystyrene or polyvinyl chloride microtiterplates in 0.1 M carbonate buffer, pH 9.5, for 18 hr at 4°C. Coatedplates were blocked with PBS containing 5% nonfat dry milk and0.05% Tween 20 for 2 hr at room temperature and were incubatedwith mAbs diluted in blocking buffer for 4 hr at room temperature.TEPC183 (Sigma) and XMMEN-OE5 IgM $kappa$ mAbs were used as isotype controlAbs. Bound IgM was detected with biotinylated goat anti-mouseIgM (µ-chain-specific; Jackson ImmunoResearch), followed by alkalinephosphatase conjugated to streptavidin, with p-nitrophenylphosphateas the chromogenic substrate. Absorbance was determined at 405nm.

Immunoblotting. Purified TMEV (Njenga et al., 1996) and rabbit MBP (Sigma) were separated by SDS-polyacrylamide gel electrophoresison 15% acrylamide gels. Proteins were transferred to a nitrocellulosemembrane by electroblotting. The membrane was blocked with Tris-bufferedsaline containing 5% nonfat dry milk and 0.03% Tween 20 for 2hr at room temperature. The membrane was incubated with SCH79.08,SCH94.03, O1, O4, A2B5, HNK-1, CH12, R24, control IgM (MOPC104E),rabbit polyclonal anti-TMEV (1:2000; Njenga et al., 1996), andrabbit polyclonal anti-MBP (1:200; Dako, Carpinteria, CA) Absfor 4 hr at room temperature. SCH79.08, SCH94.03, O1, O4, A2B5,HNK-1, CH12, R24, and control IgM were used at the same concentration(10 µg/ml). Bound Abs were detected with biotinylated secondaryAbs (Jackson ImmunoResearch) and alkaline phosphatase-conjugatedstreptavidin, using 5-bromo-4-chloro-3-indolyl phosphate and nitrobluetetrazolium (BCIP/NBT).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

IgM $kappa$ mAb SCH79.08 promotes CNS remyelination

After cell fusion and cloning, a large panel of mAbs (~100) was screened by ELISA. One mAb, designated SCH79.08 and belongingto the IgM $kappa$ subclass, showed significant binding to SCH by ELISA.SJL/J mice chronically infected with TMEV and treated with SCH79.08showed significantly greater CNS remyelination than animals treatedwith PBS or isotype-matched control mAb (Table 1). On average,~20% of the total demyelinated area showed CNS remyelination inmice treated with SCH79.08 (p < 0.05), as compared with 2-5% inanimals treated with PBS or isotype-matched mAb, respectively.Treatment with SCH79.08 had no effect on the extent of demyelination(Table 1). Remyelinated lesions were characterized by hundredsof axons with thin myelin sheaths and a relative absence of inflammatorycells or macrophages (Fig. 1). In contrast, most lesions in micetreated with the control IgM $kappa$ mAb ABPC22 or PBS had few, if any,remyelinated axons, and the lesions contained intense inflammationand macrophage infiltration (Fig. 1).


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Table 1. Enhancement of CNS remyelination by SCH79.08

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Figure 1. Light micrograph demonstrating extensive CNS remyelination after treatment with SCH79.08, O1, O4, A2B5, and HNK-1. Sections are from the spinal cords of SJL/J mice chronically infected with TMEV. Note the CNS remyelination, characterized by abnormally thin myelin sheath as compared with axon diameter, in demyelinated lesions of mice treated with SCH79.08 (A), O1 (B), O4 (C), A2B5 (D), and HNK-1 (E). Note the demyelination without significant remyelination in mice treated with R24 (F), CH12 (G), and control IgM $kappa$ ABPC22 (H). Araldite-embedded sections were stained with 1% p-phenylenediamine (magnification, 875×).

mAb SCH79.08 is polyreactive and reacts with MBP

To characterize the antigens recognized by SCH79.08, we performed immunochemistry, ELISA, and Western blotting. By immunocytochemicalstudy, SCH79.08 strongly stained the cytoplasmic structure ofmost of the cultured cells (Fig. 2D). The pattern of reactivityresembled the staining with SCH94.03 (Fig. 2B), presumably toa cytoskeletal protein. In contrast to the live surface stainingof oligodendrocytes, oligodendrocytes at specific stages of differentiationdid not react on the surface with SCH79.08 (Fig. 2C). Immunohistochemicalstaining of fresh-frozen rat tissue sections showed that SCH79.08is reactive to multiple organs, including brain (predominantlywhite matter glial cell population), small intestine (lamina propria),and kidney (mesangial cells). These results are consistent withthe conclusion that SCH79.08 is polyreactive.

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Figure 2. Indirect immunofluorescence of cultured glial cells. Note the live surface staining of oligodendrocytes with SCH94.03 (A) and R24 (E) but the absence of surface staining with SCH79.08 (C). Also note intracellular staining of the cytoplasm of astrocytes with SCH94.03 (B) and SCH79.08 (D) but the absence of staining with R24 (F). Scale bar, 20 µm. Oligodendrocytes and astrocytes were isolated from telencephalon of newborn Sprague Dawley rats.

To assess further the polyreactivity of SCH79.08, we performed ELISA, using a panel of protein antigens and chemical haptens.SCH79.08 showed prominent reactivity toward RBC spectrin, butit also reacted with rabbit actin, rabbit MBP, KLH, and mousehemoglobin (Fig. 3A). SCH79.08 also showed reactivity toward multiplechemical haptens, including phenyloxazolone (PhoX), (4-hydroxy-3-nitrophenyl)acetyl(NP), and azophenyltrimethyl ammonium (TMA) (Fig. 3B). No reactivitywas detected with the carrier protein BSA. Control IgM mAb didnot react with any of the protein antigens and chemical haptensthat were tested (Fig. 3C,D). By Western blotting, SCH79.08 showedreactivity against the 21.5 and 18.5 kDa isoforms of rabbit MBP,confirming the ELISA result (Fig. 4B).

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Figure 3. Protein antigen reactivity (A) and chemical hapten reactivity (C) of SCH79.08 are assessed by direct ELISA. Also shown are protein antigen reactivity (B) and chemical hapten reactivity (D) of control IgM (XMMEN-OE5). Abbreviations used in these panels: Ars, azophenylarsonate; BSA, bovine serum albumin; FL, fluorescein; HEL, hen egg lysozyme; KLH, keyhole limpet hemocyanin; MBP, myelin basic protein; NP, (4-hydroxy-3-nitrophenyl)acetyl; PC, azophenylphosphoryl-choline; PhoX, phenyloxazolone; RBC, red blood cells; TMA, azophenyltrimethyl ammonium; TNP, trinytrophenyl acetyl. No reactivity to these protein antigens or chemical haptens was detected with another control IgM mAb (TEPC 183) (data not shown).

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Figure 4. Western blotting of TMEV proteins (A) and MBP (B). Proteins from purified TMEV and rabbit MBP (obtained from Sigma) were separated on 15% SDS polyacrylamide gels. Bound Ig was detected with alkaline phosphatase-conjugated secondary antibodies by using BCIP/NBT. Molecular weight markers are indicated in kDa at the right or left margin. A, Lane 1, Polyclonal rabbit anti-TMEV Ab; lane 2, SCH79.08; lane 3, O1; lane 4, O4; lane 5, A2B5; lane 6, HNK-1; lane 7, CH12; lane 8, R24; lane 9, control mouse IgM (MOPC 104E). Arrows indicate TMEV capsid proteins. B, Lane 1, Control mouse IgM (MOPC 104E); lane 2, SCH94.03; lane 3, polyclonal rabbit anti-MBP Ab (obtained from Dako); lane 4, SCH79.08. Arrows indicate two MBP isoforms (21.5 and 18.5 kDa) recognized by SCH79.08.

To exclude the possibility that remyelination was the consequence of SCH79.08 reacting with TMEV, we performed Western blotting,using purified TMEV. SCH79.08 did not react with any of the knownTMEV capsid proteins (Fig. 4A).

Variable region cDNA sequences of SCH79.08 are different from those of the prototypic remyelination-promoting Ab SCH94.03

Despite binding similarities, variable region cDNA sequences of SCH79.08 were completely different from those of SCH94.03(Miller and Rodriguez, 1995a) (cDNA sequences of SCH79.08 areavailable from the GenBank database under accession numbers U91317and U92070). SCH79.08 VH belonged to the VH558 family. TheD segment was derived from the germline DQ52 gene. The JH regionwas identical to the JH2 germline gene. The V $kappa$ segment for thelight chain belonged to the V $kappa$ 24 family, whereas the J $kappa$ segmentwas identical to the J $kappa$ 5 germline gene.

Multiple oligodendrocyte-reactive IgM $kappa$ mAbs with unique antigen specificities promote CNS remyelination

Of interest, SCH94.03 and SCH79.08 have important similarities with a number of well characterized oligodendrocyte-reactivemAbs. Mouse IgM $kappa$ mAbs O1, O4 (Sommer and Schachner, 1981), A2B5(Eisenbarth et al., 1979), and HNK-1 (Abo and Balch, 1981) recognizeunique differentiation stage-specific surface antigens on oligodendrocytes.O1 recognizes multiple lipid antigens, including galactocerebroside,monogalactosyl-diglyceride, and psychosine (Bansal et al., 1989);O4 recognizes proligodendroblast antigen and sulfatide (Bansalet al., 1989, 1992); and A2B5 recognizes ganglioside GQ1c andother gangliosides (Kasai and Yu, 1983; Fredman et al., 1984).The carbohydrate epitope on myelin-associated glycoprotein (MAG)appears to be the principal antigen recognized by HNK-1 (McGarryet al., 1983). This carbohydrate epitope recognized by HNK-1 isalso present in other cell adhesion molecules in the nervous system.Similar to SCH94.03 and SCH79.08, these mAbs all belong to theIgM $kappa$ subclass, are polyreactive, recognize distinct antigens onoligodendrocytes, and recognize intracellular structures of manycell types. In addition, variable region cDNA sequences of thesemAbs have indicated minimal mutations from the germline Ig genes,a characteristic feature of natural autoantibodies (Asakura etal., 1995).

On the basis of these striking similarities, we tested the therapeutic efficacy of oligodendrocyte-reactive mAbs O1, O4, A2B5,and HNK-1 in the TMEV model. A mouse IgG3 mAb R24, which recognizesganglioside GD3 expressed on O-2A progenitor cells, and an irrelevantmouse IgM $kappa$ mAb (XMMEN-OE5) without reactivity to oligodendrocytesalso were tested to determine whether Ig isotype and specificityto a unique oligodendrocyte differentiation stage were criticalfor function. SJL/J mice treated with oligodendrocyte-reactivemAbs O1, O4, A2B5, and HNK-1 showed significantly enhanced CNSremyelination as compared with SJL/J mice treated with controlIgM $kappa$ or PBS (Table 2). Approximately 20-24% of the area of demyelinationwas remyelinated in mice treated with O1, O4, A2B5, and HNK-1.Remyelinated lesions in mice treated with O1, O4, A2B5, and HNK-1were characterized by axons with thin myelin sheaths relativeto axon diameter and a relative absence of inflammation (see Fig.1). In contrast, mice treated with R24 did not show significantlyenhanced remyelination (Table 2; Fig. 1). Of interest, thesemAbs had no effect on the extent of demyelination and were notpathogenic (Table 2).


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Table 2. In vivo effects of oligodendrocyte-reactive mAbs and CH12 IgM $kappa$ mAb

O1, O4, A2B5, HNK-1, and R24 did not react with any of the capsid proteins of TMEV, as confirmed by Western blotting (Fig.4A). Immunocytochemical study showed that, although R24 reactedwith the surface of O-2A progenitor cells, it did not stain intracellularstructures of glial cells (see Fig. 2). By ELISA, R24 did notreact with any of the protein antigens and chemical haptens thatwere examined (data not shown), indicating that R24 is not polyreactivein contrast to O1, O4, A2B5, and HNK-1 (Asakura et al., 1995).

Complementarity-determining region 3 of Ig is crucial for enhanced remyelination

Having established that a unique family of oligodendrocyte-reactive Abs, each with distinct surface antigen reactivities,would induce remyelination, it was critically important to determinewhether the complementarity-determining regions (CDR), which formthe Ab-binding site, are essential. Mouse B-cell lymphoma CH12(CH12.Lx cell) secretes IgM $kappa$ mAb under stimulation with lipopolysaccharide.This secreted IgM $kappa$ mAb CH12 is encoded by exactly the same germlineIg genes as the genes of SCH94.03; the nucleotide and amino aciddifferences between SCH94.03 and CH12 exist only in the CDR3 ofheavy and light chains (Miller and Rodriguez, 1995a). Despitethis structural similarity, CH12 did not stain the surface ofoligodendrocytes, did not stain intracellular structure of glialcells (data not shown), and was not polyreactive by ELISA (Millerand Rodriguez, 1995a). TMEV-infected SJL/J mice treated with CH12IgM $kappa$ mAb did not show significant CNS remyelination when comparedwith control groups (Table 2; Fig. 1).

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In this study we demonstrated that a panel of oligodendrocyte-reactive IgM $kappa$ mAbs promotes remyelination in a virus model ofMS. An IgM $kappa$ mAb SCH79.08, isolated from mice immunized with emulsionsof homogenized normal mouse spinal cord, is polyreactive, bindsto MBP, and enhances myelin repair. In addition, other well recognizedoligodendrocyte-reactive IgM $kappa$ mAbs (O1, O4, A2B5, and HNK-1) alsopromote CNS remyelination. The results support the hypothesisthat the targeting of polyreactive Abs to oligodendrocytes hasthe potential to promote CNS remyelination.

Although cDNA sequence analysis revealed that variable regions of SCH79.08 are completely different from those of the prototypicremyelination-promoting mAb SCH94.03 in both heavy and light chainsand that these mAbs were selected exclusively for their abilityto promote remyelination and not on the basis of antigen specificity,this characterization showed that SCH79.08 has remarkable similaritieswith SCH94.03. Both mAbs (1) belong to the IgM $kappa$ subclass (Milleret al., 1994); (2) are multi-organ reactive (Miller et al., 1996)and polyreactive toward multiple protein antigens and chemicalhaptens by ELISA (Miller and Rodriguez, 1995a); (3) strongly staincytoplasmic structures of most cells by immunofluorescence ina similar staining pattern of cytoskeletal proteins (Asakura etal., 1996b); and (4) recognize oligodendrocyte-specific autoantigens:SCH79.08 reacting with MBP and SCH94.03 binding to an uncharacterizedsurface antigen on oligodendrocytes (Asakura et al., 1996b). Theseresults indicate that SCH79.08 has the characteristic featuresof a natural autoantibody, which is produced by autoreactive B-cellsand is known to exist in healthy humans and rodents (Avrameasand Ternynck, 1993). The fact that both SCH79.08 and SCH94.03bind to oligodendrocytes, but react to different antigens on thesecells, supports the indirect hypothesis of Ab-mediated CNS remyelination.

Besides SCH79.08 and SCH94.03, other oligodendrocyte-reactive IgM $kappa$ mAbs O1, O4, A2B5, and HNK-1 also promote CNS remyelinationin the TMEV model of MS. Despite the fact that all of the mAbsthat promote CNS remyelination are IgM $kappa$ , there is no obvious commonpattern in germline Ig gene usage of these mAbs (Asakura et al.,1995). Although R24 binds to oligodendrocyte progenitors, it doesnot promote remyelination possibly because of its IgG isotype,lack of polyreactivity by immunocytochemistry and ELISA, or reactivityto oligodendrocytes of an earlier developmental stage. CH12, whichhas been classified as a natural autoantibody (Dighiero et al.,1987), was not widely polyreactive (Miller and Rodriguez, 1995a),did not bind to oligodendrocytes, and did not promote remyelination.Taken in concert, this indicates that only a unique populationof polyreactive natural autoantibodies with oligodendrocyte reactivity,irrespective of antigen specificity, is effective for treatment.To this point only Igs of the µ-isotypes have induced remyelination,suggesting the possibility that effector functions preferentiallymediated by the µ-heavy chain are central to this process. Additionally,the biological difference between SCH94.03 and CH12 establishesthat the CDR3 of Ig is critical for the remyelination-promotingactivity for this group of Abs and supports the hypothesis thatthe ability of these Abs to bind within the demyelinated lesionsis important to the induction of remyelination.

The mAbs that promote remyelination recognize different differentiation stages of oligodendrocytes from progenitor to mature,suggesting that remyelination-promoting activity may be independentof the developmental stage. The direct binding to surviving oligodendrocytesin the lesion could promote their dedifferentiation. Alternatively,the Abs could block the differentiation of oligodendrocytes tosustain their reactivity with growth factors. There is supportfrom in vitro studies for these possibilities. MAb O4 was reportedto stimulate differentiation of oligodendrocytes (Bansal et al.,1988). Abs to galactocerebroside cause transmembrane signalingin oligodendrocytes (Dyer and Benjamins, 1990). A mAb (R-mAb)that recognizes galactocerebroside, sulfatide, and a developmentallyregulated unidentified antigen on oligodendrocytes reversiblyblocks oligodendrocyte progenitor cell differentiation at thelate progenitor stage (Bansal and Pfeiffer, 1989). In the presenceof R-mAb, mature oligodendrocytes expressing terminally differentiatedmarkers showed a retraction of processes, the formation of swollencells, and a reduction of the levels of terminally differentiatedmarkers (Bansal and Pfeiffer, 1994). MAG, which is recognizedby HNK-1, has been shown to be a major inhibitor of axonal regenerationin vitro (McKerracher et al., 1994; Mukhopadhyay et al., 1994),although its inhibitory activity of axonal regeneration in vivoremains inconclusive (Bartsch et al., 1995; Schäfer et al., 1996).Possibly, HNK-1 may promote CNS remyelination by interfering withMAG expression.

The observation that multiple oligodendrocyte-reactive Abs, each with distinct antigen specificities, promote remyelinationis most consistent with the hypothesis that direct binding ofthe mAbs to injured oligodendrocytes in the lesion induces myelinrepair via an immune effector mechanism initiated by the µ-heavychain. Consistent with this hypothesis, we previously reportedthat affinity-purified polyclonal anti-MBP Abs promote CNS remyelination;therefore, reactivity to an intracellular marker of mature oligodendrocytesis also effective for myelin repair (Rodriguez et al., 1996).In further support of the hypothesis, all mAbs that promoted remyelinationnot only bound to oligodendrocytes but also reacted with intracellularantigens. One possibility is that IgM binding to damaged cellsenhances their removal by scavenger macrophages and microgliaso that healthy oligodendrocytes or O-2A progenitor cells caninitiate their myelination program.

  FOOTNOTES

Received June 4, 1998; revised July 21, 1998; accepted July 21, 1998.

These studies were supported by National Institutes of Health Grant R01 NS24180. We appreciate the generous contributionsof Mr. and Mrs. Eugene Applebaum to this project. We thank DorianMcGavern for a critical review of this manuscript and Kevin Pavelkoand Laurie Zoecklein for technical assistance.
Correspondence should be addressed to Dr. Moses Rodriguez, Department of Immunology, Mayo Clinic, 200 First Street SW, Rochester,MN 55905.

Dr. Miller's present address: University of Wisconsin Hospitals and Clinics, Madison, WI 53792.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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