| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
|
|
|
|||||||
|
|||||||||
J. Biol. Chem., Vol. 277, Issue 17, 14996-15001, April 26, 2002
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
1,3Gal and
Gal1,3Gal
1,4GlcNAc Porcine Xenotransplantation Epitopes with High
Affinity*
, and
From the Department of Biological Chemistry, University of
Michigan, Medical School, Ann Arbor, Michigan 48109-0606 and the
Department of Natural Sciences, University of Michigan,
Dearborn, Michigan 48128-1491
Received for publication, January 7, 2002, and in revised form, February 6, 2002
 |
ABSTRACT |
|---|
 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
A blood group B-specific lectin from the mushroom
Marasmius oreades (MOA) was investigated with respect to
its molecular structure and carbohydrate binding properties. SDS-PAGE
mass spectrometric analysis showed it to consist of an intact
(H; 33 kDa) and truncated (L; 23 kDa) subunit in addition to a
small polypeptide (P; 10 kDa). Isolation in the presence of EDTA
produced only the H subunits, indicating that the latter two are formed
by metalloprotease cleavage of the intact H subunit. Tryptic digestion
of the H, L, and P polypeptide chains followed by mass spectral
analysis supports this view. The lectin strongly precipitated blood
group type B substance, was nonreactive with type A substance, and
reacted weakly with type H substance. Carbohydrate binding studies
reveal a high affinity for Gal Blood group-specific lectins have served as serological reagents
for typing blood for over 65 years (1-3). Among the useful reagents
are Dolichos biflorus lectin for human type A1
erythrocytes (4, 5), the B4 Griffonia
simplicifolia isolectin for type B erythrocytes (6), and the
Ulex europeus I (7, 8) and eel (Anguilla
anguilla) serum agglutinins for type O(H) erythrocytes (1, 2). Of
all the blood group-specific lectins studied, group B-specific lectins
are probably fewest in number.
Presently, the fruiting bodies of mushrooms are being studied as
sources for lectins with novel carbohydrate binding activity. Several
surveys have been published that classify these proteins based on their
ability to agglutinate human (and rabbit) erythrocytes according to
blood type (9-12).
Crude extracts of the mushroom Marasmius oreades
(Tricholomataceae) were first reported to exhibit human type B
erythrocyte agglutinating activity in 1951 (9, 13). A lectin from this source was isolated by affinity chromatography on a matrix of We have undertaken a more detailed investigation of this potentially
important B-specific lectin with interesting results. Quantitative
precipitation studies using a highly purified preparation with A, B,
and O(H) blood group substances show absolute specificity for B
versus A substance, with slight O-binding activity. Binding studies by the techniques of hapten inhibition of agglutination and
precipitation, and hapten binding in solution by isothermal titration
calorimetry established that the lectin possesses an extended binding
site specific for the Gal Most sugars were available from previous studies. Gal Electrophoresis--
SDS-PAGE was carried out in 12.5% gels
(0.8% cross-linked) in Tris/glycine buffer, pH 8.8, by the method of
Laemmli (16). Unless otherwise indicated, samples were denatured by
boiling in buffer containing 1% SDS and 1% 2-mercaptoethanol.
HPLC1--
Size
exclusion chromatography was performed using a Beckman System Gold
equipped with a column (30 × 0.78 cm) of ProGel-TSK G2000-SWXL
(Supelco, Bellefonte, PA) in PBS (10 mM sodium phosphate, pH 7.2, 0.15 M NaCl, 0.04% NaN3, and 0.2 mM Ca2+ (unless otherwise indicated)) with or
without added haptenic sugars, at a flow rate of 0.5 ml/min. Samples of
0.1-0.4 mg of protein in 0.1 ml were injected, and effluent was
monitored at 280 nm.
Quantitative Precipitation and Hapten Inhibition
Assay--
Quantitative microprecipitation assays and inhibition of
precipitation by sugar haptens were performed as described previously (17). For quantitative precipitation assays, 20 µg of MOA and increasing amounts of glycoprotein or polysaccharide were used in a
total volume of 120 or 200 µl, all in PBS plus 0.15 M
NaCl. Quantitative carbohydrate hapten inhibition assays were conducted by adding increasing amounts of haptens to a mixture of MOA (20 µg)
and type B blood group substance (5.0 µg). The reactions were incubated at 37 °C for 1 h and then at 4°C for 48 h
followed by centrifugation of the precipitates, washing, and
determination of protein by the Lowry method (18).
Amino acid analysis, automated amino acid sequencing, and MALDI-TOF
mass spectrometric analyses of the native lectin, gel-isolated subunits, and tryptic peptides thereof were performed at the University of Michigan Biomedical Core Facilities.
Isothermal Titration Calorimetry--
Isothermal titration
calorimetry was carried out as previously described (19) except that
1.0 ml of lectin solutions containing 0.08-0.12 mM
subunits were used. Since this volume underfills the titration cell,
variable volume calculations were applied, using the Bindworks software
installed in the instrument.
Hemagglutination Assays--
Hemagglutination assays were
performed using formaldehyde-treated erythrocytes in V-well microtiter
plates as previously described (17). Titers were recorded as the
greatest dilution of the lectin solution yielding visible
agglutination. Agglutination of Ehrlich ascites tumor cells (grown in
in vitro culture, kindly supplied by Dr. D. K. MacCallum, University of Michigan) was observed microscopically.
Fluorescein-labeled MOA Staining--
MOA was fluorescently
labeled using fluorescein isothiocyanate (Sigma) at pH 9.5 in the
presence of 0.2 M lactose, followed by exhaustive dialysis.
A solution of fluorescein-labeled MOA (8 µg/ml) in PBS containing 2%
goat serum and 0.2% Triton X-100, in the absence or presence of 20 mM linear B6 trisaccharide, was applied to a cryostat
section (10 µm, fixed in paraformaldehyde) of porcine skeletal
muscle. After standing at room temperature for 2 h, the staining
solution was removed, and the section was washed with PBS and examined
under a fluorescent microscope.
Preparation of Lectin--
Fruiting bodies of M. oreades mushrooms were harvested in June and from August to
October 2000 from grassy plots in Ann Arbor, Michigan, or were
purchased from American Mushroom Hunter Corp. (Middle Town, NJ). Caps
and undamaged stems were cleaned of soil and debris and chopped into
small pieces. Initially, fresh tissue (45 g) was homogenized at 4 °C
in 250 ml of PBS containing 10 mM thiourea, 1 g/liter
ascorbate, 50 mg/liter phenylmethylsulfonyl fluoride, and 1-2 g of
insoluble polyvinylpolypyrrolidone (Sigma) in a Waring Blendor at high
speed. The homogenate was stirred 3-4 h in the cold, strained through
four layers of cheesecloth, and centrifuged at 13,000 × g for 20 min. The supernatant solution was made 20%
saturated with (NH4)2SO4, and the
resulting solution was centrifuged to remove a small amount of
precipitate. This supernatant solution was adjusted to 80% saturation
with solid (NH4)2SO4 and stirred
overnight, and the precipitate was collected by centrifugation,
redissolved in 20 ml of PBS, and dialyzed. An affinity column (2.5 × 15 cm) of melibiose-Sepharose gel, prepared using divinyl sulfone
coupling, was loaded with the dialyzed fraction and washed with PBS
until the absorbance of the effluent at 280 nm became <0.1. Lactose
(0.1 M) in PBS was then used to displace bound protein. The
protein solution so eluted was dialyzed against PBS and passed through
a second affinity column, Synsorb-B, consisting of type B trisaccharide
(Gal
It was later found (see below) that proteolysis and possibly oxidation
was taking place during the isolation and purification steps.
Subsequently, the extraction procedure was modified by including a
protease inhibitor mixture (product P8215; Sigma) at the level of 1 ml/liter of extract buffer in place of phenylmethylsulfonyl fluoride,
eliminating Ca2+ and including 1.25 mM EDTA in
all buffers, and carrying out the extraction and ammonium sulfate
precipitations under an atmosphere of argon.
By employing a series of chromatographic affinity columns, we have
isolated a lectin that strongly agglutinates human B erythrocytes with
a concomitant low activity against O cells. Successive passage through
Synsorb B and Synsorb A columns removed a slight activity against type
A erythrocytes that was present in some preparations. The
hemagglutinating activity against types A, B, and O cells and several
other cell types is presented in Table I.
Hemagglutination activity was unchanged by extensive dialysis of the
lectin and assay in metal-free buffer containing EDTA, indicating the
absence of a divalent metal ion requirement (data not shown).
Subsequently, metal-free buffer containing EDTA was used routinely to
prevent matalloprotease degradation of the lectin.
1,3Gal (but not for the isomeric
1,2-, 1,4-, and 1,6-disaccharides); Gal1,3Gal
1,4GlcNAc;
and the type B branched trisaccharide. MOA also reacts strongly with
murine laminin from the Engelbreth-Holm-Swarm sarcoma and bovine
thyroglobulin, both of which contain multiple Gal1,3Gal1,4GlcNAc
end groups. This linear B trisaccharide is a component of porcine
tissues and organs, preventing their transplantation into humans. MOA also shares carbohydrate recognition of this trisaccharide with toxin A
elaborated by Clostridium difficile.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-galactosyl-polyacrylamide gel by Horejsi and Kocourek (14). It was
reported to agglutinate type B erythrocytes six times more avidly than
type A erythrocytes and was stated to be a heterodimeric protein of 50 kDa, with subunits of 33 and 23 kDa. No mono- or oligosaccharides (25 mM) tested were found to inhibit
agglutination of human type B erythrocytes.
1,3Gal structure, in contrast to other
B-specific lectins having more general affinity toward
-galactosides. A companion paper (15) reports the cloning, sequencing, expression, and characterization of the recombinant lectin
and indications of its homology to other important carbohydrate-binding proteins.
MATERIALS AND METHODS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
1,3Gal,
Gal1,3(L-Fuc1,2)Gal, and
L-Fuc1,2Gal1,4Glc were purchased from Dextra
Laboratories (Reading, United Kingdom). Gal1,6Gal was from Sigma,
and Gal1,3Gal1,4GlcNAc (linear B-2 trisaccharide) was from
Calbiochem. Gal1,2Gal was from Toronto Research Chemicals, Inc. (New
York, Ontario, Canada). Soluble GalNAc1,3Gal-polyacrylamide conjugate was purchased from Glycotech Corp. (Rockville, MD). Gal1,6Gal was a gift of Dr. Paul Kovac (Laboratory of Medicinal Chemistry, Section on Carbohydrates, National Institutes of Health). Blood group types A (368 PI/WS), B (hnmad BGS 531 PI/WS, pepsin treated), and H (BGS PI/WS) substances were the gift of Dr. Ronald Poretz (Rutgers University). Pigeon ovalbumin was a gift from Dr.
Y. C. Lee (Department of Biology, Johns Hopkins University). Synsorbs A and B were purchased from Chembiomed Ltd. (Edmonton, Alberta, Canada).
1,3(L-Fuc1,2)GalO(CH2)8CONH)
linked to diatomaceous earth. The bound lectin was eluted with 20 mM diaminopropane containing 0.15 M NaCl, pH
~11. The "pass-through" and displaced protein fractions were
combined separately and assayed against a panel of human erythrocytes.
Finally, the protein fraction displaced from the Synsorb B column was
passed through a column of Synsorb A, which contains covalently bound
type A trisaccharide. A very small amount of material was bound
(<5%); it was eluted with 20 mM diaminopropane, 0.15 M NaCl. Both fractions were assayed against types A, B, and
O erythrocytes.
RESULTS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
Agglutination of cells by M. oreades lectin
SDS-PAGE analysis of the lectin revealed the presence of two major
bands at 33 and 23 kDa (designated H and L, respectively), as was
previously reported (14). A significant band, not noted previously, was
also observed at ~10 kDa, designated P (Fig.
1). Upon heavy loading of the gel,
several minor bands migrating between the L and P bands were also
observed. The absence of 2-mercaptoethanol in the sample preparation
buffer did not alter the pattern of bands, indicating the absence of
interchain disulfide links. Samples prepared without heating also
showed a band at ~55 kDa, streaking between the bands, and lesser
amounts of the other bands, suggesting that bands H, L, and P are
associated into a heteromeric structure that is dissociated slowly by
SDS at room temperature.
|
The native protein was subjected to size exclusion chromatography by
HPLC, wherein it migrated as a single, symmetric peak having the same
mobility as Pisum sativum and Xanthosoma
sagittifolium lectins, both known to be of ~50 kDa (20, 21). In
the absence of a haptenic sugar, all three lectins appeared to be of
much lower molecular mass based on calibration of the column with
cytochrome c, ovalbumin, and bovine serum albumin. In the
presence of 0.1 M lactose, but not methyl -mannoside,
MOA migrated slightly faster than ovalbumin (Fig.
2), at an apparent mass of 49.5 kDa,
suggesting that the lectin interacted weakly with the column matrix,
despite its being a silica-based noncarbohydrate matrix. Lectins
frequently are observed to migrate through size exclusion matrices at
slower rates than expected by their molecular masses, either because of
weak interaction with the matrix (generally polysaccharide-based matrices) or because of their compact structures, usually with a high
amount of -structure.2
Interestingly, neither sugar used altered the migration of the other
two lectins, both of which bind mannose. These results do not rule out
the possibility that native MOA is somewhat larger than 49.5 kDa, but
it is clear from the HPLC results it exists in solution as a single
molecular weight species composed of at least three different sized
subunits.
|
The native lectin was subjected to MALDI-TOF mass spectrometric analysis, wherein mass ions corresponding to the three bands were detected (data not shown). Pairs of masses corresponding to the 23- and 32-kDa subunits, separated by ~180 and 260 Da, respectively, were observed (probably due to binding of the matrix), whereas the 10-kDa subunit exhibited a single molecular mass of ~9800 Da. Within the limits of the mass calibration, the sum of the two smaller molecular masses (corresponding to L and P subunits) approximates the larger molecular mass of band H. Mass spectrometric analysis of tryptic peptides from the various bands and total amino acid analysis (data not shown) also support the conclusion that the two lighter bands, L and P, are fragments of the intact band H.
No significant amounts of any amino acids were obtained during several cycles of automated amino acid sequencing of the native protein or of the H and L bands, indicating that they possess blocked N-termini. The P band released small amounts of several amino acid derivatives at some of the cycles (similar to traces seen in the native protein also), but no single sequence was detected, suggesting that it is also largely blocked and may be heterogeneous.
Proceeding from the observation that recombinant MOA is a homodimer consisting of two identical subunits of 32 kDa (15) whose solutions are completely colorless (no absorbance above 320 nm), we set out to attempt to isolate a similar protein from the mushroom, taking care to inhibit any protease activity that could give rise to the "clipped" lectin (the 23- and 10-kDa polypeptide chains) as well as prevent possible oxidation of aromatic side chains. The modified procedure described above indeed led to the isolation of a homodimer similar to the recombinant lectin in lacking any 23- and 10-kDa subunits and having no absorbance above 320 nm (data not shown).
To further study the blood group specificity of the M. oreades lectin, we conducted quantitative precipitation assays of
the lectin with soluble cyst blood group substances. Fig.
3 shows that MOA reacts strongly with
human blood type B substance, not at all with type A substance, and
rather weakly with type H substance. The explanation for these
reactions will be discussed in terms of the specificity studies
described below.
|
Sugar ligand binding to MOA was conducted using three approaches:
inhibition of type B hemagglutination, hapten inhibition of MOA-type B
substance precipitation, and isothermal titration calorimetry. All
three techniques gave approximately the same results, with the
calorimetric data being the most precise. Being a blood type B
agglutinin, MOA was assayed primarily against
D-galactosyl-terminated sugars and oligosaccharides. As
shown in Fig. 4 and Table
II, lactose,
N-acetyllactosamine, and melibiose (Gal1,6Glc) were very
poor ligands. Methyl -galactopyranoside was similarly very poor. The
blood group B disaccharide, Gal1,3Gal, was an excellent ligand, with
Ka = 6.0 × 103
M
1, whereas the isomeric disaccharides
Gal1,2Gal, Gal1,4Gal, and Gal1,6Gal bound poorly or not at
all. The addition of a GlcNAc group to the reducing end of Gal1,3Gal
to give Gal1,3Gal1,4GlcNAc increased the binding by ~50% to
Ka = 9.7 × 103
M1. Similarly, adding an
L-fucosyl group to the disaccharide to afford the blood
group B branched trisaccharide
(Gal1,3(L-Fuc1,2)Gal) enhanced its affinity to
MOA 4-fold (Ka 3.6 × 104
M1). Finally, we assayed the trisaccharide
L-Fuc1,2Gal1,4Glc (fucosyllactose), related to
the blood group H trisaccharide; it had a Ka of 548 M1 by isothermal titration calorimetry. It is
apparent that the L-fucosyl residue makes a significant
contribution to the binding affinity of the essentially inactive
lactose (Ka = 185 M1).
This also is probably the reason that MOA recognizes and agglutinates human O erythrocytes to a limited extent and gives a weak precipitin curve with blood group H substance.
|
|
On the basis of MOA's recognition of blood type B disaccharides and
linear trisaccharides, we believed that the lectin should precipitate
both with laminin from the Engelbreth-Holm-Swarm murine sarcoma and
with bovine thyroglobulin. Indeed, as shown in Fig. 5, MOA reacted strongly with laminin,
which we have shown contains Gal1,3Gal1,4GlcNAc end groups (22,
23), as well as with bovine thyroglobulin, which has the same
determinants (24). Significantly, the lectin did not give a precipitin
reaction with pigeon ovalbumin, which contains multiple Gal1,4Gal
end groups (25), thus demonstrating its specificity for Gal1,3Gal
groups. Also of significance, MOA did not recognize the blood group
type A disaccharide (GalNAc1,3Gal), as shown by its failure to
precipitate with this disaccharide-polyacrylamide glycoconjugate. MOA
readily agglutinated Ehrlich ascites tumor cells, which contain the
same epitopic end groups in their cell membranes (26).
|
Fluorescein-labeled MOA stained porcine striated skeletal muscle (Fig.
6), endothelial cells lining the
capillaries being the significant structures stained by the lectin.
Incubation of the staining solution in the presence of 20 mM linear B6 trisaccharide essentially abolished staining
(data not shown), indicating specific binding of the
fluorescein-labeled lectin to the porcine tissue.
|
| |
DISCUSSION |
|---|
|
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
Results presented in this paper indicate that the M. oreades lectin, as isolated previously and in the initial stages of this work, was a dimer composed of an intact and a truncated subunit in addition to a small polypeptide presumably generated by proteolytic cleavage of the intact H subunit. Both the intact H and truncated L subunits are blocked at their N termini. Subsequently, we isolated an intact form of the lectin and an intact recombinant lectin (15), which have very similar binding properties, indicating that cleavage is due to the presence of contaminating metalloprotease activity and is not relevant to protein function.
The most interesting aspect of this study concerns the high specificity
of the lectin for Gal1,3Gal end groups; the 1,2-, 1,4-, and
1,6-linked disaccharides do not bind to the lectin. These data
indicate that MOA has an extended binding site that accommodates the
Gal1,3Gal disaccharide. To the best of our knowledge, this is the
first lectin shown to exhibit this exclusive specificity. Additional
contributions to the binding energy are made by the addition of
1,4GlcNAc and 1,2-L-fucosyl groups to the
reducing Gal unit of Gal1,3Gal. These additions account
for the blood group B activity of the lectin. The structures of these
oligosaccharides, related to human blood group B substance and assayed
for their activity in this study, are presented in Fig.
7.
|
It is instructive to compare MOA with the Griffonia
simplicifolia I-B4 isolectin (GS I-B4), a
highly specific -D-galactosyl-binding lectin, with
respect to the size of their combining sites. A great deal of binding
data indicate that the GS I-B4 isolectin has a very
restricted binding site that does not appear to extend significantly beyond the monosaccharide unit (i.e. the
-D-galactosyl group) (27, 28). This concept of a
restricted site was substantially verified by the recently completed
x-ray crystallographic structure of the B4 isolectin
complexed with Gal1,3Gal in which it is shown that only the
nonreducing -galactosyl group makes contact with the lectin (29).
Moreover, Kirkeby and Moe (30), using an enzyme-linked lectin assay,
showed that the -galactosyl group and the 1,2-, 1,3-,
and 1,4-galactobiosyl groups as well as the linear B-trisaccharide
(Gal1,3Gal1,4GlcNAc) linked to human serum albumin were very
similar in their binding affinity to GS I-B4. On the
contrary, MOA, which binds only very weakly or not at all to methyl
-D-galactopyranoside or to the 1,2-, 1,4-, and
1,6-linked galactobioses, has an extended binding site, which accommodates the blood type B disaccharide and linear trisaccharide (Gal1,3Gal and Gal1,3Gal1,4GlcNAc, respectively) and the
branched chain blood group B trisaccharide determinant with high affinity.
Taking advantage of these carbohydrate binding properties of MOA, we
demonstrated that it gave a very strong precipitation reaction with
laminin from the Engelbreth-Holm-Swarm murine sarcoma. This highly
glycosylated glycoprotein contains the linear type B blood group
trisaccharide at many of its chain ends (22, 23). It also recognizes
and precipitates bovine thyroglobulin, which also contains the linear B
trisaccharide (24). Interestingly, this lectin will not precipitate the
galactomannan from Cassia alata that contains multiple
-galactosyl end groups, illustrating its lack of reactivity with
single such sugar residues (Fig. 5). Nor did MOA bind to
cross-linked guaran, also a galactomannan. Conversely, both the
galactomannan (not shown) and pigeon ovalbumin precipitated strongly
with GS I isolectins (Fig. 5). MOA does not recognize the blood group
type A disaccharide (GalNAc1,3Gal), as shown by its failure to
precipitate with this disaccharide-polyacrylamide glycoconjugate,
whereas the GS I-A4 isolectin, which is specific for
GalNAc end groups (27), reacted strongly with it (Fig. 5).
MOA should be a valuable reagent for the glycobiologist for
the detection and preliminary characterization of glycoconjugates containing Gal1,3Gal disaccharide and Gal1,3Gal1,4GlcNAc
trisaccharide on cell surfaces and in solution, since these epitopes
occur in many biologic sources. They have been found, for example, in
the basement membranes of mice, rats, and rabbits (31); the surface of
3T3 cells (32); calf thyroid plasma membranes (33); and the plasma
membranes of Ehrlich ascites tumor cells (26, 34). It also has been
known for many years that porcine tissues and organs contain the
Gal1,3Gal1,4GlcNAc epitope, the so-called Galili trisaccharide
(35), which prevents their use for transplantation into humans. Indeed,
fluorescein-labeled MOA does stain porcine striated skeletal muscle as
shown in Fig. 6, in which endothelial cells lining the capillaries bind
the lectin. This epitope is present in most cells of nonprimate mammals
and New World monkeys but not in humans, apes, or Old World monkeys. It
is also possible that this carbohydrate antigen is present on the
surface of the malaria parasite, Plasmodium
falciparum (36). Another interesting application of this
lectin could be its use in the possible competition with toxin A
elaborated by Clostridium difficile, which is responsible for antibiotic-induced diarrhea (37). Both MOA and toxin A recognize the Gal1,3Gal1,4GlcNAc trisaccharide epitope.
| |
ACKNOWLEDGEMENTS |
|---|
We thank the following for gifts of reagents:
Dr. Ronald Poretz for blood group A, B, and H substances; Dr. Donald
MacCallum for Ehrlich ascites tumor cells; Dr. Paul Kovac (National
Institutes of Health) for a sample of Gal1,6Gal, Dr. Y. C. Lee
for a sample of pigeon ovalbumin; Dr. Peng G. Wang for linear B-6
trisaccharide; and Dr. Phillip Andrews for helpful discussions. We also
thank Dr. Stephen Ernst and Julie A. S. Edwards for staining a
specimen of porcine striated muscle with fluorescein-labeled MOA.
| |
FOOTNOTES |
|---|
* This work was supported by National Institutes of Health Grant GM29470-35.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
§ To whom correspondence should be addressed: Dept. of Biological Chemistry, University of Michigan, 1301 Catherine St., Ann Arbor, MI 48109-0606. Tel.: 734-763-3511; Fax: 734-763-4581; E-mail: igoldste@umich.edu.
Published, JBC Papers in Press, February 8, 2002, DOI 10.1074/jbc.M200161200
2 W. J. Peumans, personal communication.
| |
ABBREVIATIONS |
|---|
The abbreviations used are: HPLC, high performance liquid chromatography; GS I-B4 and -A4 G. simpicifolia I-B4 and A4 isolectin, respectively; MOA, M. oreades agglutinin; PBS, phosphate-buffered saline; MALDI-TOF, matrix-assisted laser desorption ionization time-of-flight.
| |
REFERENCES |
|---|
|
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
| 1. | Sugishita, S. (1935) Juzenkwai-Zasshi 40, 1938 |
| 2. |
Jonsson, B.
(1944)
Acta Pathol. Microbiol. Scand. Suppl.
54,
456-464 |
| 3. |
Boyd, W. C.,
and Reguera, R. M.
(1949)
J. Immunol.
26,
333-339 |
| 4. |
Bird, G. W. G.
(1951)
Curr. Sci.
20,
298-299 |
| 5. |
Etzler, M. E.,
and Kabat, E. A.
(1970)
Biochemistry
9,
869-877[CrossRef][Medline]
[Order article via Infotrieve] |
| 6. |
Murphy, L. A.,
and Goldstein, I. J.
(1977)
J. Biol. Chem.
252,
4739-4742 |
| 7. |
Cazal, P.,
and Lalaurie, M.
(1952)
Acta Haematol.
8,
73-80[CrossRef][Medline]
[Order article via Infotrieve] |
| 8. |
Boyd, W. C.,
and Shapleigh, E.
(1954)
Science
119,
419 |
| 9. |
Elo, J.,
Estola, E.,
and Malmstrom, N.
(1951)
Ann. Med. Exp. Biol. Fenn.
29,
297-308 |
| 10. |
Pemberton, R. T.
(1994)
Mycol. Res.
98,
277-290 |
| 11. |
Wang, H., Ng, T. B.,
and Ooi, V. E. C.
(1998)
Mycol. Res.
102,
897-906[CrossRef] |
| 12. |
Yagi, F.,
Sakai, T.,
Shiraishi, N.,
Yotsumoto, M.,
and Mukoyoshi, R.
(2000)
Mycoscience
41,
323-330[CrossRef] |
| 13. |
Elo, J.,
and Estola, E.
(1952)
Ann. Med. Exp. Biol. Fenn.
30,
165-167[Medline]
[Order article via Infotrieve] |
| 14. |
Horejsi, V.,
and Kocourek, J.
(1978)
Biochim. Biophys. Acta
538,
299-315[Medline]
[Order article via Infotrieve] |
| 15. |
Kruger, R. P.,
Winter, H. C.,
Goldstein, I. J.,
Simonson-Leff, N.,
and Dixon, J. E.
(2002)
J. Biol. Chem.
277,
15002-15005 |
| 16. |
Laemmli, U. K.
(1970)
Nature
227,
680-685[CrossRef][Medline]
[Order article via Infotrieve] |
| 17. |
Mo, H.,
Winter, H. C.,
and Goldstein, I. J.
(2000)
J. Biol. Chem.
275,
10623-10629 |
| 18. |
Lowry, O. H.,
Rosebrough, N. J.,
Farr, A. L.,
and Randall, R. J.
(1951)
J. Biol. Chem.
193,
265-275 |
| 19. |
Mo, H.,
Winter, H. C.,
Van Damme, E. J. M.,
Peumans, W. J.,
Misaki, A.,
and Goldstein, I. J.
(2001)
Eur. J. Biochem.
268,
2609-2615[Medline]
[Order article via Infotrieve] |
| 20. |
Entlicher, G.,
Kostir, J. V.,
and Kocourek, J.
(1970)
Biochim. Biophys. Acta
221,
272-281[Medline]
[Order article via Infotrieve] |
| 21. |
Mo, H.,
Rice, K. G.,
Evers, D. L.,
Winter, H. C.,
Peumans, W.,
Van Damme, E. J. M.,
and Goldstein, I. J.
(1999)
J. Biol. Chem.
274,
33300-33305 |
| 22. |
Shibata, S.,
Peters, B. P.,
Roberts, D. D.,
Goldstein, I. J.,
and Liotta, L. A.
(1982)
FEBS Lett.
214,
194-198 |
| 23. |
Knibbs, R. N.,
Perini, F.,
and Goldstein, I. J.
(1989)
Biochemistry
28,
6379-6392[CrossRef][Medline]
[Order article via Infotrieve] |
| 24. |
Spiro, R. G.,
and Bhoyroo, V. D.
(1984)
J. Biol. Chem.
259,
9858-9866 |
| 25. |
Suzuki, N.,
Khoo, K.-H.,
Chen, H.-C.,
Johnson, J., R.,
and Lee, Y. C.
(2001)
J. Biol. Chem.
276,
23230-23239 |
| 26. |
Eckhardt, A. E.,
and Goldstein, I. J.
(1983)
Biochemistry
22,
5290-5297[CrossRef][Medline]
[Order article via Infotrieve] |
| 27. |
Murphy, L. A.,
and Goldstein, I. J.
(1979)
Biochemistry
18,
4999-5005[CrossRef][Medline]
[Order article via Infotrieve] |
| 28. |
Wood, C.,
Kabat, E. A.,
Murphy, L. A.,
and Goldstein, I. J.
(1979)
Arch. Biochem. Biophys.
981,
1-11 |
| 29. |
Tempel, W.,
Tschampel, S.,
and Woods, R. J.
(2002)
J. Biol. Chem.
277,
6615-6621 |
| 30. |
Kirkeby, S.,
and Moe, D.
(2001)
Immunol. Cell Biol.
79,
121-127[CrossRef][Medline]
[Order article via Infotrieve] |
| 31. |
Peters, B. P.,
and Goldstein, I. J.
(1979)
Exp. Cell Res.
120,
321-334[CrossRef][Medline]
[Order article via Infotrieve] |
| 32. |
Stanley, W. S.,
Peters, B. P.,
Blake, D. A.,
Yep, D.,
Chu, E. H. Y.,
and Goldstein, I. J.
(1979)
Proc. Natl. Acad. Sci. U. S. A.
76,
304-307 |
| 33. |
Okada, Y.,
and Spiro, R. G.
(1980)
J. Biol. Chem.
255,
4739-4742 |
| 34. |
Roth, J.,
and Goldstein, I. J.
(1995)
Glycoconj. J.
12,
142-149[CrossRef][Medline]
[Order article via Infotrieve] |
| 35. |
Galili, U.,
Shohet, S. B.,
Kobrin, E,.,
Stults, C. L. M.,
and Macher, B. A.
(1988)
J. Biol. Chem.
263,
17755-17762 |
| 36. |
Ramasamy, R.,
and Rajakaruna, R.
(1997)
Biochim. Biophys. Acta
1360,
241-246[Medline]
[Order article via Infotrieve] |
| 37. |
Teneberg, S.,
Lonnroth, I.,
Torres Lopez, J. F.,
Galili, U.,
Halvarsson, M. O.,
Angstrom, J.,
and Karlsson, K. A.
(1996)
Glycobiology
6,
599-609 |
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati What's this?
This article has been cited by other articles:
|
|
 |
|
  L. Ma, H. Lu, A. Sprinkle, M. R. Parsek, and D. J. Wozniak Pseudomonas aeruginosa Psl Is a Galactose- and Mannose-Rich Exopolysaccharide J. Bacteriol., November 15, 2007; 189(22): 8353 - 8356. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 D. Loganathan, H. C. Winter, W. J. Judd, J. Petryniak, and I. J. Goldstein Immobilized Marasmius oreades agglutinin: use for binding and isolation of glycoproteins containing the xenotransplantation or human type B epitopes Glycobiology, December 1, 2003; 13(12): 955 - 960. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 H. Tateno and I. J. Goldstein Molecular Cloning, Expression, and Characterization of Novel Hemolytic Lectins from the Mushroom Laetiporus sulphureus, Which Show Homology to Bacterial Toxins J. Biol. Chem., October 17, 2003; 278(42): 40455 - 40463. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
S. Teneberg, B. Alsen, J. Angstrom, H. C. Winter, and I. J. Goldstein Studies on Gal{alpha}3-binding proteins: comparison of the glycosphingolipid binding specificities of Marasmius oreades lectin and Euonymus europaeus lectin Glycobiology, June 1, 2003; 13(6): 479 - 486. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
H. Tateno, H. C. Winter, J. Petryniak, and I. J. Goldstein Purification, Characterization, Molecular Cloning, and Expression of Novel Members of Jacalin-related Lectins from Rhizomes of the True Fern Phlebodium aureum (L) J. Smith (Polypodiaceae) J. Biol. Chem., March 21, 2003; 278(13): 10891 - 10899. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
R. P. Kruger, H. C. Winter, N. Simonson-Leff, J. A. Stuckey, I. J. Goldstein, and J. E. Dixon Cloning, Expression, and Characterization of the Galalpha 1,3Gal High Affinity Lectin from the Mushroom Marasmius oreades J. Biol. Chem., April 19, 2002; 277(17): 15002 - 15005. [Abstract] [Full Text] [PDF]
|
|
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
, group A
substance; 
, group B substance; 
, group 
substance.
polyacrylamide; 
, GS I
interaction with pigeon ovalbumin; 
, GS I interaction with
GalNAc
