(Received for publication, May 21, 1996, and in revised form, October 30, 1996)
From the Departments of Pharmacology and
Neuroscience, The Johns Hopkins University School of Medicine,
Baltimore, Maryland 21205,
Department of Biological Sciences,
Hunter College, City University of New York,
New York, New York 10021, and ** Department of Applied Bioorganic
Chemistry, Gifu University, Gifu 501-11, Japan
Myelin-associated glycoprotein (MAG), a nervous
system cell adhesion molecule, is an I-type lectin that binds to
sialylated glycoconjugates, including gangliosides bearing
characteristic structural determinants (Yang, L. J.-S., Zeller, C. B.,
Shaper, N. L., Kiso, M., Hasegawa, A., Shapiro, R. E., and Schnaar, R. L. (1996) Proc. Natl. Acad. Sci. U. S. A. 93, 814-818).
Two cell adhesion systems, COS-1 monkey kidney fibroblasts transiently transfected to express MAG and Chinese hamster ovary (CHO) cells stably
transfected to express MAG, were used to probe the structural specificity of MAG-ganglioside binding. Both cell types bound to
the same gangliosides: GQ1b
(IV3NeuAc,III6NeuAc,II3(NeuAc)2-Gg4Cer) > GT1b = GD1a > GM3 > GM1, GD1b, and GQ1b (the latter
do not support adhesion). Binding was enhanced by pretreatment of
MAG-expressing cells with neuraminidase. MAG-expressing Chinese hamster
ovary cells bound directly to gangliosides resolved on thin layer
chromatograms, allowing detection of MAG binding species in a mixture.
The simplest ganglioside ligand for MAG was GM3 bearing
N-acetylneuraminic acid, whereas GM3 bearing
N-glycolylneuraminic acid did not support adhesion.
Chemical modifications of N-acetylneuraminic acid residues
(on GD1a) abrogated MAG binding. Mild periodate oxidation of sialic
acids to their corresponding seven-carbon (or eight-carbon) sialic acid
aldehydes abolished MAG binding, as did further conversion to the
corresponding primary alcohols. Eliminating the anionic charge by ethyl
esterification, amidation, or reduction also abolished MAG-mediated
cell adhesion. These data demonstrate that MAG-ganglioside binding is
highly specific and defines key carbohydrate structural determinants
for MAG-mediated cell adhesion to gangliosides.
Myelin-associated glycoprotein (MAG)1 is a member of the Ig superfamily and is composed of five extracellular Ig-like domains, a single transmembrane domain, and a short cytoplasmic tail (1, 2, 3, 4). It is a minor component of myelin, comprising 1% of central nervous system and 0.1% of peripheral nervous system myelin proteins (5). Based on its periaxonal location (6) and its in vitro adhesion properties (7, 8), MAG has been hypothesized to play a role in myelin-axon interactions. Although transgenic MAG-knockout mice are able to myelinate, they have altered periaxonal architecture (9, 10).
A second function proposed for MAG is in the inhibition of central nervous system neurite outgrowth (axon regeneration). Neurite outgrowth from neurons plated on a substratum of MAG-expressing Chinese hamster ovary (CHO) cells was significantly inhibited compared with neurons plated on control cells (11). Similarly, NG108-15 (neuroblastoma-glioma hybrid) cells did not extend neurites onto a substratum adsorbed with myelin or MAG (12). Myelin from MAG-deficient transgenic mice is less inhibitory to NG108-15 cell neurite outgrowth than is myelin from control mice (13), although the two preparations inhibit neurite outgrowth equally from some peripheral nervous system neurons in vitro. In vivo, transgenic mice lacking the MAG gene demonstrate enhanced axon regeneration in a lesion-induced axon regrowth model (14). Current data are consistent with the presence of multiple myelin inhibitors of neurite outgrowth (15), of which MAG is one. Complementary nerve cell surface ligands for myelin inhibitors of neurite outgrowth have yet to be identified. The discovery that MAG belongs to the family of sialic acid binding lectins termed sialoadhesins (16) or I-type lectins (17) led us to investigate the role of gangliosides, prominent neural cell surface sialoglycoconjugates, as MAG ligands (18).
Gangliosides, sialic acid-containing glycosphingolipids, are highly enriched in the nervous system (19). Their prominent location on the outer leaflet of the plasma membrane and their structural diversity lead to the hypothesis that gangliosides are involved in neural cell adhesion (20, 21). If this is the case, gangliosides may interact with complementary binding proteins (lectins) to initiate cell-cell recognition. In support of this hypothesis, endogenous ganglioside receptors have been revealed in the nervous system and elsewhere (22, 23). Mammalian ganglioside-binding proteins have distinct structural specificities for their carbohydrate targets. One of the most highly specific ganglioside binding lectins is MAG (18). The current study defines conditions for highly sensitive detection of MAG-ganglioside adhesion and describes fine structural requirements for MAG binding, with special emphasis on sialic acid substructure.
The structures of the
gangliosides used in this article are presented schematically in Fig.
1. GM1, GD1a, and GT1b were from EY Laboratories (San
Mateo, CA) or Matreya (Pleasant Gap, PA), GQ1b was from Accurate
Chemical (Westbury, NY), and GM3 (NeuAc form) was from
Sigma. GM3 (NeuGc form) was purified from bovine spleen (24) and contained 93% NeuGc and 7% NeuAc as measured by
Dionex Carbopac high performance liquid chromatographic analysis (25).
A mixture of disialogangliosides was purified from bovine brain (26,
27). GQ1b
(IV3NeuAc,III6NeuAc,II3(NeuAc)2-Gg4Cer)
was synthesized de novo (28). GM1b (cis-GM1, IV3NeuAc-Gg4Cer) was the generous gift of Dr.
Robert Yu (Medical College of Virginia, Richmond, VA). SLeX
(IV3NeuAc,III3Fuc-nLcCer) was the kind gift of
Dr. Brian Brandley (Glycomed, Inc., Alameda, CA).
2,3-Sialyllactose and
2,6-sialyllactose were from Sigma.
Oligosaccharides from gangliosides GT1b and GM1 were prepared
enzymatically using ceramide glycanase (29), as described previously
(30).
The structures of the sialic acid
derivatives used in this article are presented in Fig.
2. The glycerol chains of GD1a sialic acids were
oxidized to the 7- and 8-aldehyde forms and then reduced to the
corresponding truncated primary alcohols as described (31). Briefly,
GD1a (1 mg) was treated with 1 ml of ice-cold 150 mM NaCl,
50 mM sodium phosphate, pH 7.4, containing 2.5 mM sodium periodate for 90 min. The aldehyde products were
purified by reverse phase chromatography (using a Sep-Pak
C18 cartridge; Millipore Corp., Milford, MA) as described
(26). A portion of the resulting GD1a-aldehyde was dissolved in 1 ml of
50 mM sodium bicarbonate containing 10 mM
sodium borohydride and incubated for 2 h at 37 °C. The
resulting products were purified by reverse phase chromatography (26).
The sialic acids on 1 µmol of GD1a were converted to the corresponding ethyl esters by incubation for 1 h at ambient
temperature in 0.6 ml Me2SO/iodoethane (5:1) (32). The
resulting diester was purified by DEAE-Sepharose (acetate form)
chromatography in methanol. The product in the unretained eluent was
further purified by reverse phase chromatography (26). One portion of
the GD1a diethyl ester was reduced to the corresponding dialcohol in
1% sodium borohydride in methanol for 2 h. The product was
purified by DEAE-Sepharose and reverse phase chromatography. Another
portion of the GD1a ethyl ester was converted to the corresponding
diamide by treatment with 4 M ammonium hydroxide in
methanol/water (5:2) for 12 h at ambient temperature. The product
was purified by reverse phase and DEAE-Sepharose chromatography.
Products were analyzed by TLC and fast atom bombardment-mass
spectrometry (33) at the Middle Atlantic Mass Spectrometry
Laboratory.
Cell Culture and Transfection
COS-1 cells were maintained in 10% fetal calf serum in Dulbecco's modified Eagle's medium (DMEM) at 37 °C in a humidified atmosphere of 90% air/10% CO2. Transient COS-1 transfections with an expression plasmid containing cDNA for the long form of MAG (pCDM8-MAG; Ref. 18) and control plasmid (MAG in the reverse orientation) were performed using DEAE-dextran (40 µg/ml) as described (34). Cells were harvested for adhesion experiments (see below) 48 h after transfection.
CHO cells were stably transfected using the plasmid pSJL into which cDNA for the long form of MAG was subcloned in the forward (subclone MAG1) or reverse (control) direction as described previously (11). CHO cells were maintained in DMEM supplemented with 10% dialyzed fetal bovine serum, 2 mM glutamine, 347 µM proline, 3 µM thymidine, and 100 µM glycine. Twelve hours before harvesting for adhesion experiments (see below), 100 nM CdCl2 was added to the CHO growth medium to stimulate expression via an upstream metallothionein promoter.
Microplate Cell Adhesion to Adsorbed GlycolipidsAdhesion was performed as reported previously (18, 35). Briefly, a 50-µl aliquot of ethanol/water (1:1) containing gangliosides (concentrations as indicated), phosphatidylcholine (0.5 µM), and cholesterol (2.0 µM) was added to microwells (96-well Serocluster; Costar, Cambridge, MA). Plates were incubated 90 min uncovered at ambient temperature to allow evaporation and lipid adsorption (36, 37), after which the wells were washed with water. Wells were preblocked by addition of 100 µl/well Hepes-buffered DMEM containing 1.5 mg/ml bovine serum albumin (BSA) when using COS cells or 5 mg/ml BSA when using CHO cells. Plates were covered and incubated 10 min at 37 °C prior to cell addition (see below).
Transfected COS cells were harvested using hypertonic Ca2+- and Mg2+-free phosphate-buffered saline (PBS) containing 1 mM EDTA as described (18), collected by centrifugation, and resuspended at 107 cells/ml in Dulbecco's PBS containing 2 mg/ml BSA. Transfected CHO cells were harvested using 0.53 mM EDTA in Ca2+- and Mg2+-free Dulbecco's PBS, collected by centrifugation, and resuspended at 4 × 106 cells/ml in PBS containing 2 mg/ml BSA. Aliquots of cells (500 µl) were placed in 1.5-ml microfuge tubes, and Vibrio cholerae neuraminidase (Calbiochem) was added (10 milliunits/500 µl or as indicated). Suspensions were incubated for 2 h at 37 °C with end-over-end mixing. Cells were collected by centrifugation and resuspended at 250,000 cells/ml (for COS cells) or 500,000 cells/ml (for CHO cells) in Hepes-buffered DMEM containing 1.5 mg/ml BSA (for COS cells) or 5 mg/ml BSA (for CHO cells). Aliquots of cell suspension (200 µl) were added to preblocked, lipid-adsorbed microwells and incubated at 37 °C for 45 min. To remove nonadherent cells after the incubation, the plate was immersed upright in a vat of PBS, inverted, and placed in an immersed custom-designed Plexiglas box, which was sealed with a gasket to exclude air (35). The inverted plate in its fluid-filled chamber was placed in a centrifuge carrier and centrifuged at 110 × g to gently remove nonadherent cells. The box was again immersed in a vat of PBS, and the plate was removed and righted (while immersed), and surface fluid was removed by aspiration. Adherent cells were lysed by addition of 20 µl of 10% Triton X-100, and 80 µl/well was removed to a fresh 96-well plate for quantitation. Cell adhesion was quantitated by measuring lactate dehydrogenase activity in the cell lysate after addition of 120 µl of 0.1 M potassium phosphate buffer, pH 7.0, containing 0.7 mM NADH and 4.7 mM pyruvate. The decrease in absorbance at 340 nm as a function of time was measured simultaneously in each well using a Molecular Devices UV multiwell kinetic plate reader. Details of the adhesion assay have been described (35).
For comparison with neuraminidase-pretreated cells, some MAG-transfected COS cells were pretreated with sodium periodate under mild conditions, which destroy MAG ligands (see below) but do not result in a loss of cell viability (38). Cells were suspended at 1 × 106 cells/ml in 2.5 mM sodium periodate in PBS. After 45 min on ice with intermittent mild agitation, the cells were collected by centrifugation, washed three times with PBS, and finally resuspended at 250,000 cells/ml in Hepes-buffered DMEM containing 1.5 mg/ml BSA (as above). More than 75% of the cells were recovered intact (as measured by cellular lactate dehydrogenase activity) after periodate pretreatment and washing.
Neuraminidase InhibitorV. cholerae neuraminidase (0.1 milliunit) in 500 µl of Dulbecco's PBS containing 2 mg/ml BSA was incubated with or without 100 µM N-acetyl-2,3-dehydro-2-deoxyneuraminic acid (Toronto Research Chemicals, Downsview, Ontario, Canada) for 30 min at 37 °C. COS cells transfected with pCDM8-MAG (5 × 106 cells) were resuspended in the above solutions and incubated for 2 h at 37 °C with end-over-end mixing, collected by centrifugation, and used in adhesion experiments as described above.
Cell Adhesion Directly to Gangliosides Resolved by TLCCell adhesion to TLC-resolved glycolipids was performed as described (39). MAG-transfected CHO cells were radiolabeled by addition of 20 µCi of 32Pi to their medium for 16 h. Cells were harvested, neuraminidase-pretreated (see above), and resuspended at 7 × 105 cells/ml in Hepes-buffered DMEM containing 5 mg/ml BSA. Gangliosides were applied to duplicate Silica Gel 60 high performance TLC plates (5635; EM Separations, Gibbstown, NJ), and the chromatogram was developed with isopropyl alcohol/0.25% aqueous KCl (3:1). One plate was stained for gangliosides using resorcinol-hydrochloric acid (40). The other was dried, dipped in 100 µg/ml polyisobutylmethacrylate (Polysciences, Warrington, PA) in hexanes, blocked in Hepes-buffered DMEM containing 5 mg/ml BSA for 15 min at 37 °C, and placed in a Plexiglas TLC adhesion chamber (GlycoTech, Rockville, MD). The cell suspension (14 ml, see above) was pipetted into the chamber, which was incubated at 37 °C for 45 min to allow adhesion to occur. The chamber was then inverted, and nonadherent cells were removed by centrifugation at 110 × g for 10 min. The chamber was immersed, the plate was removed while immersed and transferred to a Petri dish without exposing to an air-liquid interface, and cells were fixed in place by addition of 2% glutaraldehyde in Dulbecco's PBS for 30 min at ambient temperature. The fixed plate was washed with PBS, dried, and subjected to PhosphorImager analysis (Fujix BAS 1000, Fuji Photo Film Co., Tokyo, Japan).
Binding of transiently
transfected COS cells and stably transfected CHO cells to control and
ganglioside-adsorbed microwells was compared (Fig. 3).
Consistent with our previous report (18), surfaces adsorbed with GT1b
supported specific adhesion of MAG-transfected cells, whereas those
adsorbed with GM1 did not. Adhesion of both transfected cell lines was
greatly enhanced by pretreatment with V. cholera
neuraminidase, indicating the presence of inhibitory structures on the
transfected cells. COS and CHO cells transfected with control plasmids,
with or without pretreatment with neuraminidase, did not specifically
adhere to any ganglioside-adsorbed surface (data not shown). Adhesion
of neuraminidase-treated, MAG-transfected COS cells to surfaces
adsorbed with GT1b was resistant to higher detachment forces than
adhesion of untreated cells (data not shown), suggesting that more MAG
binding sites were available to support adhesion. Incubation of
neuraminidase-pretreated, MAG-transfected COS cells with
conformationally specific monoclonal antibody 513 (7, 41) blocked
adhesion to GT1b-adsorbed surfaces (data not shown). This is consistent
with previous observations (18) and demonstrates that neuraminidase
pretreatment unmasks the same MAG binding sites that are apparent on
untreated cells.
The relationship between the concentration of neuraminidase used and
enhancement of MAG-mediated carbohydrate adhesion is shown in Fig.
4A. As little as 0.02 milliunits/ml
neuraminidase significantly increased MAG-mediated cell adhesion,
whereas adhesion was maximally enhanced by pretreatment with 2 milliunits/ml enzyme. When
N-acetyl-2,3-dehydro-2-deoxyneuraminic acid (42) was used to
block neuraminidase prior to incubation with cells, MAG-mediated adhesion to GT1b-adsorbed surfaces was reduced to the level of untreated cells (Fig. 4B). These data indicate that removal
of endogenous sialic acid residues from the transfected cells is responsible for the enhanced adhesion of MAG-transfected cells to
gangliosides.
Carbohydrate Specificity of MAG-mediated Adhesion
A
restricted family of structurally related glycolipids supports
MAG-mediated cell adhesion (18), the order of potency being (in part)
GQ1b > GT1b = GD1a
GM1, GD1b, and GQ1b (the latter do
not support adhesion). MAG-transfected COS and CHO cells, pretreated with neuraminidase to enhance MAG binding, adhered to the same set of
gangliosides (Fig. 5). GQ1b
was the most potent
ganglioside supporting MAG-mediated cell adhesion, whereas GT1b and
GD1a supported specific adhesion when adsorbed at higher
concentrations. Although GQ1b at high concentrations appeared to
support MAG-mediated adhesion of transfected COS and CHO cells, this
was due to contaminating GT1b in the commercially obtained sample, as
indicated by TLC (see below). All other purified or synthetic
gangliosides were single species by TLC (data not shown). These data
confirm the requirement for a single terminal 2,3-linked sialic acid to
support MAG binding (16, 18). This led us to reassess the ganglioside GM3 for binding, using two forms, one carrying only NeuAc
(N-acetylneuraminic acid) and the other carrying
predominantly NeuGc (N-glycolylneuraminic acid; see Fig. 2).
Using neuraminidase-pretreated COS cells, adhesion to GM3 (NeuAc) was
detected (Fig. 6A), although the potency of GM3 in supporting adhesion was much less than that of GD1a under identical conditions. GM3 (NeuGc), in contrast, did not support MAG-mediated adhesion, demonstrating that the presence of a single additional hydroxyl group on sialic acid can abrogate recognition.
To distinguish whether the enhanced potency of GD1a compared with GM3
was due to steric factors (its longer neutral core) or to additional
structural components, two gangliosides bearing an 2,3-linked sialic
acid moiety on the terminal galactose of a tetraosyl core (GM1b and
SLeX) were tested. Using neuraminidase-pretreated COS cells, adhesion
to GM1b was relatively poor, and adhesion to SLeX was undetectable
(Fig. 6B).
To further test the carbohydrate binding specificity of MAG, a series
of soluble oligosaccharides were used in an attempt to inhibit adhesion
of neuraminidase-pretreated, MAG-transfected COS cells to gangliosides.
Cells were preincubated with various concentrations of potential
soluble saccharide inhibitors for 60 min at 37 °C with constant
end-over-end agitation prior to addition to GT1b-adsorbed microwells.
Even at the maximum concentrations tested (25 mM sialic
acid, 1.5 mM 2,3- or
2,6-sialyllactose, and 50 µM GT1b or GM1 oligosaccharides), none of the soluble
saccharides significantly inhibited MAG-transfected COS adhesion (data
not shown). In contrast, micellar (intact) GT1b ganglioside (but not GM1 ganglioside) inhibited adhesion ~50% at 50 µM
(data not shown).
Because purified gangliosides may harbor minor
species as contaminants, direct adhesion of MAG-transfected cells to
TLC-resolved gangliosides (39, 43) was used to determine whether the
major species were the active MAG ligands. A partially purified mixture of disialylated gangliosides from bovine brain, purified bovine brain
gangliosides GT1b and GQ1b, and synthetic GQ1b were resolved by TLC.
The plate was treated with a polymer coating and then incubated with
32P-labeled, MAG-transfected CHO cells. Nonadherent cells
were removed without subjecting adherent cells to an air-liquid
interface using a Plexiglas adhesion chamber (GlycoTech; Refs. 39 and
43). Adherent cells were detected with a PhosphorImager, and positions of adhesion were compared with the migration of gangliosides detected on a sister plate by chemical staining (Fig. 7). In the
disialoganglioside mixture, cells adhered at the migration position of
GD1a, but not to GD1b, even though the sample had more GD1b. Cells
adhered at the migration positions of purified GT1b and synthetic
GQ1b
, with the latter supporting avid adhesion, even though it was
present at less than (null)/1;10 of the concentration of GT1b. The
cells did not adhere at the migration position of GQ1b. Although cell adhesion was detected in this GQ1b sample (see Fig. 5), adhesion on TLC
was at the migration position of GT1b. This particular commercial
sample of GQ1b was contaminated with GT1b, as indicated by chemical
staining on TLC (Fig. 7). Quantitation by scanning densitometry (27)
established that the GQ1b sample contained 27% GT1b (data not shown).
Essentially all of the adhesion to microwell-adsorbed GQ1b (Fig. 5) can
be accounted for by the presence of GT1b. These data demonstrate the
power of combined microwell and TLC binding to confirm the identity of
MAG ligands.
Sialic Acid Structural Requirements for MAG Binding
MAG-mediated adhesion to GM3 was absent when the sialic acid was NeuGc rather than NeuAc (Fig. 6). To further assess the fine structural specificity of binding, sialic acids on GD1a (di-NeuAc form) were chemically modified (see Fig. 2). Treatment of GD1a with 2 mM aqueous sodium periodate at 0 °C selectively cleaved the sialic acid glycerol side chains to the corresponding 7- or 8-aldehydes (31). Further treatment of the aldehyde products with sodium borohydride reduced the sialic acid aldehydes to their corresponding 7- or 8-position alcohols. GD1a sialic acid carboxylic acids were ethyl-esterified by treatment with iodoethane, followed by either conversion to the corresponding 1-position amides with ammonia or reduction to the 1-position alcohols with sodium borohydride.
Periodate treatment under these conditions resulted in approximately equal conversion of each sialic acid to either its 7-aldehyde or 8-aldehyde forms, as evidenced by appropriate molecular ions detected by fast atom bombardment-mass spectrometry. Resolution by TLC in isopropyl alcohol/0.25% aqueous KCl (3:1) resulted in two major bands. Reduction of the aldehydes generated the expected mixture of sialic acid 7-alcohol and 8-alcohol forms, confirmed by fast atom bombardment-mass spectrometry and TLC as above. Conversion of GD1a to its diethyl ester resulted in a single species by TLC with the appropriate mass ions by fast atom bombardment-mass spectrometry. Further conversion to the corresponding sialic acid 1-amide or 1-alcohol forms resulted in new single species with appropriate changes in TLC migration.
GD1a and its derivatives were adsorbed to microwells and tested for
their ability to support specific adhesion of MAG-transfected COS
cells. Neither the truncated glycerol side chain derivatives nor any of
the uncharged species (carboxylic acid ethyl esters, 1-position amides,
or 1-position alcohols) supported MAG binding (Figs. 8 and
9). All derivatives adsorbed equally to
the microwells and remained adsorbed equally during incubation with
cells (data not shown). Control transfected COS cells did not adhere to
any of the GD1a derivatives (data not shown).
Periodate Treatment of MAG-transfected Cells
The discovery
that mild periodate treatment of gangliosides abrogated MAG binding
(Fig. 8) provided an experimental method to investigate the mechanism
by which neuraminidase treatment of transfected cells enhanced
MAG-mediated cell adhesion (Fig. 3). If neuraminidase enhanced
MAG-mediated adhesion by destroying endogenous MAG ligands on the
transfected cells, periodate would be expected to do the same. In
contrast, if neuraminidase enhanced MAG binding by an alternative
mechanism, such as reducing the surface anionic charge on transfected
cells, periodate would not be expected to enhance binding. The results
demonstrate the latter to be the case. Using periodate incubation
conditions that destroyed the ability of adsorbed GD1a to support
MAG-mediated cell adhesion (Fig. 10A),
periodate pretreatment of intact cells failed to enhance binding (Fig.
10B). Neuraminidase pretreatment, in contrast, sharply enhanced MAG-mediated adhesion.
MAG is a lectin with highly specific binding to terminal sialic acids attached in particular arrays on glycoconjugates (16, 18). Optimal conditions for detecting MAG-carbohydrate binding were determined using both transiently and stably transfected cell lines, each expressing full-length MAG as a plasma membrane protein (11, 18). Adhesion of the transfected cells to ganglioside-containing phosphatidylcholine and cholesterol monolayers was quantitated in a high throughput microwell adhesion format (35). In these assays, MAG, which is polyvalent on the transfected cell surface, interacts with carbohydrate targets presented as multivalent arrays in an apposing membrane. This system models the potential interaction of natural MAG-expressing cells (oligodendroglia and Schwann cells) with glycoconjugates on neurons or other cells in their environment.
Neuraminidase pretreatment markedly increased MAG-ganglioside adhesion without changing its carbohydrate specificity or anti-MAG monoclonal antibody susceptibility. These data are consistent with at least two possible interpretations. Endogenous sialoglycoconjugates on the transfected cells may bind, in cis configuration, to a significant proportion of the expressed MAG, reducing its availability for interaction with exogenous targets. This mechanism apparently regulates carbohydrate binding by two other I-type lectins, CD22 and CD33 (44, 45, 46). Alternatively, the anionic nature of the cell surface may limit interactions of transfected cells with anionic ganglioside-adsorbed surfaces. In either case, neuraminidase treatment would reverse the inhibition. Periodate pretreatment, in contrast, would be expected to destroy endogenous ligands but not to reduce surface anionic charge. Because periodate pretreatment failed to enhance MAG-mediated cell adhesion, neuraminidase is likely to enhance binding by reducing the cell surface anionic charge. This finding may have a physiological correlate. Attenuating charge repulsion to facilitate membrane-membrane interactions is a possible function of a membrane-bound myelin-associated neuraminidase, which is active against myelin glycoproteins and glycolipids (47) and which is involved in the ganglioside "simplification" of mature myelin (48). Whether or not an endogenous myelin neuraminidase facilitates cell-cell interactions, our data indicate that pretreatment of MAG-expressing cells with neuraminidase may reveal more pronounced effects of MAG on neuronal behaviors in vitro (11).
Under optimal binding conditions, using either MAG-transfected COS or
CHO cells, MAG binds to a discrete family of gangliosides with the
relative potencies: GQ1b > GT1b = GD1a > GM3
GD1b, GM1, and GQ1b (the latter do not detectably bind MAG). Although an
2,3-NeuAc bound to the terminal Gal on a neutral sugar core appears
to be required for binding (16, 18), other moieties enhance or diminish
that binding. For example, gangliosides GM3 and GM1b are comparable and
much weaker binding ligands for MAG than is GD1a. These data indicate
that the internal sialic acid (II3NeuAc) on GD1a enhances
its interaction with MAG. In addition to the IV3NeuAc, the
ganglioside GQ1b
has additional II3NeuAc and
III6NeuAc residues, which sharply increase binding
affinity. Other moieties diminish MAG binding. Whereas MAG binds
(albeit weakly) to GM3, it does not bind at all to GM1, which is
equivalent to GM3 with a disaccharide constituent on the 4-position of
Gal(II). The failure of SLeX, which also has the terminal
NeuAc
2,3Gal group, to support MAG adhesion may be due to steric
hindrance by the nearby fucose or to structural differences in the
neutral core (neolacto versus ganglio structure).
Monovalent soluble sialo-oligosaccharides, including the oligosaccharide released from GT1b (up to 50 µM), failed to inhibit binding of MAG-transfected COS cells to adsorbed gangliosides. This may reflect cooperativity when polyvalent MAG in the transfected cell membrane contacts polyvalent gangliosides on an apposing planar surface (49). Similar polyvalent interactions may take place at the interface between the periaxonal myelin membrane and the axolemma (6). Alternatively, the ceramide moiety of gangliosides may impart conformational restraints on ganglioside oligosaccharides, which enhance binding affinity (50).
The ganglioside binding specificity of MAG may reflect its role in
intracellular interactions in vivo. Central nervous system myelin is enriched in the non-MAG binding ganglioside GM1, which comprises up to 90% of adult rat myelin gangliosides (48, 51). In
contrast, axolemma, which is directly apposed to MAG in
vivo, is enriched in the strong MAG-binding gangliosides GT1b and
GD1a (52). Gangliosides bearing these structures, as well as GQ1b and related structures, are expressed preferentially on neurons and
axons (51, 52, 53) and may act as endogenous MAG ligands. The observations
that monoclonal antibody 513 inhibits binding of MAG to both neurons
and gangliosides (8, 18) and inhibits oligodendrocyte-neuron adhesion
in vitro (7) further support the hypothesis that MAG
expressed on oligodendrocytes binds to neuronal sialoglycoconjugates,
the precise nature of which are unknown. Prior studies suggest that
sialoglycoproteins may be relevant ligands for MAG, at least for some
neuronal cell types (54). Whether neuronal gangliosides,
sialoglycoproteins, or both serve as functional MAG ligands remains to
be determined.
As common termini of mammalian glycoconjugates, sialic acids bear a
special role in recognition (55). The five I-type lectins (16, 17) and
three selectins (56) all bind sialic acids, although their precise
carbohydrate determinant specificities vary. The sialic acid linkage
(2,3 or
2,6) appears critical for recognition, with CD22
requiring
2,6-linked sialic acid and all others requiring
2,3
linkages (16). Selectin-mediated adhesion is maintained when critical
sialic acid residues are replaced by other anionic functional groups
(56, 57), a scenario that has not been thoroughly tested with any of
the I-type lectins. However, the relatively high specificity of I-type
lectins for sialic acid substructure suggests that such replacements
would not be fruitful.
Sialic acids are the most complex saccharides in vertebrate glycoconjugates. They constitute a family of structures based on N-acetylneuraminic acid, the most abundant sialic acid and precursor to diverse structures bearing modifications on the glycerol side chain, N-acyl group, and/or hydroxyl at carbon 4 (55). Sialic acid binding lectins vary in their preference or acceptance of alterations in sialic acid substructure. For example, all three selectins tolerate periodate truncation of the glycerol side chain (58, 59, 60), whereas the I-type lectins CD22 (61) and MAG (this study) do not.
Enzymatic hydroxylation of the N-acetyl group of NeuAc forms N-glycolylneuraminic acid (NeuGc), which is rare in humans but common in some tissues of other vertebrates, including rodents. Notably, human CD22 binds NeuAc and NeuGc residues equally (61), whereas mouse CD22 has a marked preference for NeuGc-terminated glycoconjugates (62), which are abundant on murine CD22 targets (lymphocytes and monocytes). In contrast, we report that rodent MAG (95% amino acid identical to human MAG; Ref. 63) binds NeuAc-terminated GM3 but not the corresponding NeuGc form. Since brain gangliosides bear predominantly NeuAc residues in both rodents and humans (51), our findings are consistent with a MAG binding preference for its neuronal target glycoconjugates. Murine sialoadhesin, another I-type lectin, has a similar preference for NeuAc-bearing glycoconjugates (62).
Ethyl esterification of the carboxylic acid on NeuAc abrogated MAG binding, and conversion of the ester to the corresponding amide or primary alcohol did not restore binding. All three derivatives were uncharged (did not bind DEAE-Sepharose) and stable during the experimental incubations. Thus, MAG is among the most specific NeuAc-directed lectins, since it does not tolerate changes in either the NeuAc glycerol side chain, its N-acyl group, or its carboxylic acid. Having demonstrated the high specificity of MAG-glycoconjugate binding using naturally occurring, synthetic, and chemically modified gangliosides, the nature of the endogenous neuronal glycoligands for MAG, and their functions in neural cell-cell interactions, await future investigations.
We thank Drs. Yoshitaka Ichikawa and Yoshitomo Suhara for helpful chemical advice.