Leukocyte traffic into lymph nodes and sites of inflammation is guided by L-selectin. Experiments performed in vitro and with gene-deleted mice suggest that CD34 recognizes L-selectin if decorated by 6-sulfo sialyl Lewis x (sLex) saccharides and the MECA-79 epitope. However, very little is known about glycosylation of human L-selectin ligands. We report here on matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS) profiles of N- and O-linked oligosaccharide fractions from human tonsillar endothelial CD34. All detected O-glycans were sialylated; some were also monosulfated or monosulfated and monofucosylated. If a given CD34-glycan may carry all requirements for L-selectin recognition, that is, both 6-sulfo-sLex and MECA-79 epitopes, only one O-glycan fraction, O-9, SA2Hex3HexNAc3- Fuc1(SO3)1, meets the criteria. A candidate structure is SAα2-3Galβ1-4(Fucα1-3)(6-sulfo)GlcNAcβ1-3Galβ1-3(SAα2-3Galβ1-4GlcNAcβ1-6)GalNAc. However, if sulfo sLex glycans are supplemented with separate sulfated, nonfucosylated O-glycans, saccharides in O-6, O-8, or O-9, putatively carrying MECA-79 epitopes, could form multiglycan binding epitopes for L-selectin.

High-endothelial venules (HEV) are the sites of leukocyte entry into the lymph nodes from the blood circulation. L-selectin on leukocytes recognizes its ligands on HEV, such as CD34 and other members of a heterogenous group of mucin-type glycoproteins forming the peripheral node addressins (PNAd).1,2 In vitro experiments and results derived from gene-deleted mice suggest that the proper recognition of L-selectin requires at least the presence of the following posttranslational decorations: α2,3sialylated galactose as well as α1,3fucosylated and 6-sulfated N-acetylglucosamine in the form of 6-sulfo sLex epitopes in the ligand glycoproteins.2-7 Furthermore, the HEVs express the MECA-79 epitope, which resides in the PNAd complex and has recently been shown to recognize a core 1 O-glycan Galβ1-4(sulfo-6)GlcNAcβ1-3Galβ1-3GalNAc.8-10 The 6-sulfo sLex and MECA-79 epitopes are not commonly expressed in other locations of the vascular endothelium under normal conditions.2 However, these glycans are rapidly induced in the endothelium at sites of inflammation, where they probably participate in recruitment of the inflammatory leukocytes into the inflammed tissue.11-13 

The L-selectin–binding glycans are synthesized by various glycosyltransferases. As the repertoire of these enzymes shows remarkable interspecies variability, the data obtained from murine experiments cannot be directly extrapolated to human settings. So far, very little is known of the human endothelial L-selectin ligands, except that they contain sLex, 6-sulfo sLex, and MECA-79 epitopes.8,14,15 Therefore, we have initiated research on human leukocyte extravasation,16 and report here on the glycosylation of CD34 in human tonsillar HEV.

Purification of CD34

Human tonsils were obtained from tonsillectomies performed at the Department of Otorhinolaryngology, Helsinki University Central Hospital, after the institutional review board had approved the study protocol. The tonsils used for this study were all removed due to hyperplasia, and the patients had no signs of infections or inflammations at the time of their operations. CD34 was isolated from tonsillar lysates by chromatography on immobilized wheat germ agglutinin (WGA) and anti-CD34 mAb581 as described.8 The purity of the sample was verified by sodium dodecyl sulfate–polyacrylamide gel electrophoresis (SDS-PAGE) followed by silver staining and MALDI-TOF MS fingerprinting.

Glycan preparation

N-glycans were liberated on-blot with the Flavobacterium meningosepticum N-glycosidase F from CD34 blotted on polyvinylidenefluoride (PVDF) membrane. The liberated N-glycans were passed through a BondElut C18 column (Varian, Palo Alto, CA) and desalted by gel filtration HPLC. The blot was subjected to reductive β-elimination and liberated O-glycan alditols were isolated by gel filtration high-performance liquid chromatography (HPLC).

Matrix-assisted laser desorption/ionization time-of-flight mass spectrometry

MALDI-TOF MS was performed with a Biflex mass spectrometer (Bruker Daltonics, Bremen, Germany). Analysis was performed in negative- and positive-ion linear delayed-extraction mode, using 2,4,6-trihydroxyacetophenone (THAP; Sigma-Aldrich Finland, Helsinki, Finland) as the matrix.17,18 External calibration was performed with THAP matrix dimer and sialyl Lewis x beta-methylglycoside (Toronto Research Chemicals, Ontario, Canada). (3-sulfo)Galβ1-4(Fucα1-3)GlcNAc (Calbiochem, San Diego, CA), and SAα2-3Galβ1-4(Fucα1-3)GlcNAcβ1-3Galβ1-4GlcNAc17gave equivalent matrix assisted laser desorption ionization-time of light mass spectrometry (MALDI) responses, implying that sialylated and sulfated glycans were analyzed with comparable efficiency (data not shown). In mass spectra of the CD34 glycans, only peaks with signal-to-noise ratios above 2 were taken into account.

In the present study, endothelial CD34 was isolated from human tonsils, the N- and O-linked glycans were released separately from the protein, and the oligosaccharides were analyzed and quantified with gel filtration HPLC and MALDI-TOF MS. N-glycans were mostly complex-type and contained 1-4 sialic acid residues (Table1). No signs of neutral N-glycans were detected in positive-ion mode MALDI-TOF MS. No functions in leukocyte traffic are currently known for N-glycans of CD34.

Table 1.

Analyses of the human tonsillar CD34

No.m/z%Proposed composition
N-linked glycans 
  N-1 1713.1 1.5 SA1Hex1HexNAc1+ Man3GlcNAc2Fuc1 
 N-2 1875.3 1.5 SA1Hex2HexNAc1+ Man3GlcNAc2Fuc1 
 N-3 2076.9 36 SA1Hex2HexNAc2+ Man3GlcNAc2Fuc1 
 N-4 2222.9 3.5 SA2Hex2HexNAc2+ Man3GlcNAc2Fuc1 
 N-5 2281.7 SA1Hex2HexNAc3+ Man3GlcNAc2Fuc1 
 N-6 2368.0 30 SA2Hex2HexNAc2+ Man3GlcNAc2Fuc1 
 N-7 2442.0 SA1Hex3HexNAc3+ Man3GlcNAc2Fuc1 
 N-8 2571.3 1.5 SA2Hex2HexNAc3+ Man3GlcNAc2Fuc1 
 N-9 2733.2 SA2Hex3HexNAc3+ Man3GlcNAc2Fuc1 
 N-10 3025.1 10 SA3Hex3HexNAc3+ Man3GlcNAc2Fuc1 
 N-11 3100.2 1.5 SA2Hex4HexNAc4+ Man3GlcNAc2Fuc1 
 N-12 3391.2 SA3Hex4HexNAc4+ Man3GlcNAc2Fuc1 
 N-13 3682.5 1.5 SA4Hex4HexNAc4+ Man3GlcNAc2Fuc1 
 N-14 3758.1 0.5 SA3Hex5HexNAc5+ Man3GlcNAc2Fuc1 
 N-15 4049.0 0.5 SA4Hex5HexNAc5+ Man3GlcNAc2Fuc1 
O-linked glycan alditols 
  O-1 674.8 53 SA1Hex1HexNAc1 
 O-2 966.4 10 SA2Hex1HexNAc1 
 O-3 1040.6 SA1Hex2HexNAc2 
 O-4 1186.3 0.5 SA1Hex2HexNAc2Fuc1 
 O-5 1333.0 21 SA2Hex2HexNAc2 
 O-6 1413.8 SA2Hex2HexNAc2(SO3)1 
 O-7 1698.4 SA2Hex3HexNAc3 
 O-8 1778.7 SA2Hex3HexNAc3(SO3)1 
 O-9 1925.9 SA2Hex3HexNAc3(SO3)1Fuc1 
 O-10 2062.1 SA2Hex4HexNAc4 
No.m/z%Proposed composition
N-linked glycans 
  N-1 1713.1 1.5 SA1Hex1HexNAc1+ Man3GlcNAc2Fuc1 
 N-2 1875.3 1.5 SA1Hex2HexNAc1+ Man3GlcNAc2Fuc1 
 N-3 2076.9 36 SA1Hex2HexNAc2+ Man3GlcNAc2Fuc1 
 N-4 2222.9 3.5 SA2Hex2HexNAc2+ Man3GlcNAc2Fuc1 
 N-5 2281.7 SA1Hex2HexNAc3+ Man3GlcNAc2Fuc1 
 N-6 2368.0 30 SA2Hex2HexNAc2+ Man3GlcNAc2Fuc1 
 N-7 2442.0 SA1Hex3HexNAc3+ Man3GlcNAc2Fuc1 
 N-8 2571.3 1.5 SA2Hex2HexNAc3+ Man3GlcNAc2Fuc1 
 N-9 2733.2 SA2Hex3HexNAc3+ Man3GlcNAc2Fuc1 
 N-10 3025.1 10 SA3Hex3HexNAc3+ Man3GlcNAc2Fuc1 
 N-11 3100.2 1.5 SA2Hex4HexNAc4+ Man3GlcNAc2Fuc1 
 N-12 3391.2 SA3Hex4HexNAc4+ Man3GlcNAc2Fuc1 
 N-13 3682.5 1.5 SA4Hex4HexNAc4+ Man3GlcNAc2Fuc1 
 N-14 3758.1 0.5 SA3Hex5HexNAc5+ Man3GlcNAc2Fuc1 
 N-15 4049.0 0.5 SA4Hex5HexNAc5+ Man3GlcNAc2Fuc1 
O-linked glycan alditols 
  O-1 674.8 53 SA1Hex1HexNAc1 
 O-2 966.4 10 SA2Hex1HexNAc1 
 O-3 1040.6 SA1Hex2HexNAc2 
 O-4 1186.3 0.5 SA1Hex2HexNAc2Fuc1 
 O-5 1333.0 21 SA2Hex2HexNAc2 
 O-6 1413.8 SA2Hex2HexNAc2(SO3)1 
 O-7 1698.4 SA2Hex3HexNAc3 
 O-8 1778.7 SA2Hex3HexNAc3(SO3)1 
 O-9 1925.9 SA2Hex3HexNAc3(SO3)1Fuc1 
 O-10 2062.1 SA2Hex4HexNAc4 

m/z values refer to [M-H] ions in negative-ion linear mode matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. The percentages of N- and O-linked glycans have been presented separately. There are 7 times more O- than N-linked glycans on the human endothelial CD34.

Western blot shows that human tonsillar endothelial CD34 reacts with MECA-79 (Figure 1A). The molar amounts of O-glycans were 7-fold higher compared with N-glycans (Table 1). The procedures for isolating CD34, releasing glycans from it, and the purification of glycans for analysis leaves open that some structures may be lost during this processing. However, currently we cannot make any valid statements of such putative glycans.

Fig. 1.

Isolation and characterization of CD34 and its glycans.

(A) Western blot shows that human tonsillar endothelial CD34 reacts with MECA-79. Lanes 1 and 4 are after the WGA column, lanes 2 and 5 after the CD34 mAB 581 column, and lanes 3 and 6 after desalting and concentration. The arrow indicates the CD34 at 105 kd. (B) Proposal for structures of human tosillar high endothelial CD34 O-glycans of the sLex containing fraction O-4 and sulfated sLex containing fraction O-9. The latter putatively bears both 6-sulfo-sLex and MECA-79 epitopes.

Fig. 1.

Isolation and characterization of CD34 and its glycans.

(A) Western blot shows that human tonsillar endothelial CD34 reacts with MECA-79. Lanes 1 and 4 are after the WGA column, lanes 2 and 5 after the CD34 mAB 581 column, and lanes 3 and 6 after desalting and concentration. The arrow indicates the CD34 at 105 kd. (B) Proposal for structures of human tosillar high endothelial CD34 O-glycans of the sLex containing fraction O-4 and sulfated sLex containing fraction O-9. The latter putatively bears both 6-sulfo-sLex and MECA-79 epitopes.

Close modal

The recovered glycans represented core 1 and core 2 structures, but most likely not core 3-7 branches as the number of hexoses (Hex) was equal to the number of N-acetylhexosamines (HexNAc). Acidic but not neutral O-glycans were detected in human tonsillar endothelial CD34. Monosialylated, disialylated, monosialylated-monofucosylated, disialylated-monosulfated, and disialylated-monosulfated-monofucosylated O-glycans were observed (Table 1). It remains to be explained why the relatively large fractions, O-5 and O-7, representing 21% and 5% respectively, do not undergo sulfate-independent fucosylation to generate sLex epitopes on human endothelial CD34, although in vitro fucosylation with endothelial α1,3fucosyltransferases prefer nonsulfated over sulfated N-acetyllactosamine acceptors.6 

Recombinant soluble CD34 expressed in Chinese hamster ovary (CHO) cells has been decorated with bivalent 6-sulfo sLex glycans10 and was shown to be several-fold more effective in mediating L-selectin–dependent lymphocyte rolling than the 2 variants lacking one or the other sulfo sLex branch.10However, none of the human CD34 glycans revealed 2 sulfates or 2 fucoses in the present experiments, suggesting that in the tonsillar repertoire of human CD34 only one sulfo sLex epitope may be present in one glycan. Previously, the glycans from a murine endothelial L-selectin ligand, GlyCAM-1, have been shown to carry 6 or 6′-sulfo sLex in the core 2 branch,2 19 but similar sulfated heptasaccharides were not present among the O-glycans of human high endothelial CD34.

A prerequisite for L-selectin binding is the presence of fucose on the ligand.2-7 As the fraction O-4 contains fucose, 2 putative glycans containing the sLex structure have been depicted in Figure 1B. The most interesting O-glycan fraction in human tonsillar CD34 is O-9 as it is the only one that is both sulfated and fucosylated. It may contain the nonasaccharideSAα2-3Galβ1-4(Fucα1-3)(6-sulfo)GlcNAcβ1-3Galβ1-3(SAα2-3Galβ1-4GlcNAcβ1-6)GalNAc(Table 1, Figure 1B), which represents both a 6-sulfo-sLex–reactive (underlined) and a MECA-79–reactive saccharide10 (italics) in a partially overlapping form. Another version is also possible, where the sialylated N-acetyllactosamine is linked to the 6-position of the proximal galactose on the core 1 chain (Figure 1B). If the MECA-79 and 6-sulfo-sLex epitopes were not present in a single glycan, they could be organized in clusters.20 The 6-sulfo-sLex saccharides from O-9, representing several structures isomeric to the nonasaccharides of Figure 1B would be supplemented in these clusters by separate MECA-79 glycans (containing the Galβ1-4(6-sulfo)GlcNAcβ1-3Galβ1-3GalNAc10) from O-6 and/or O-8 and/or O-9, forming multiglycan binding determinants for lymphocyte L-selectin.

The sulfated O-glycans O-6, O-8, and O-9 of Table 1 represented together about 4% of the total O-glycans. It has been estimated that the HEV-derived CD34 represents one fourth of the total tonsillar CD34.8 This implies that as much as 16% of the O-glycans in HEV-derived CD34 may be sulfated. The mucin-rich areas of the CD34 glycoprotein might contain O-glycans in such a high density that 2 or several copies of the L-selectin recognizing sulfated O-glycans, belonging to fractions O-6, O-8, and O-9, could be properly spaced to act in a functionally multivalent manner to ligate advantageously with the clustered L-selectin molecules at the tips of lymphocyte microvilli.21 Our previous ex vivo work in the rat allograft rejection model, showing that lymphocyte L-selectin adheres much more efficiently to multivalent sLex epitopes than to monovalent ones,22-24 is in agreement with this suggestion.

We thank Gunilla Rönnholm and Leena Penttilä for technical assistance.

Supported by grants from the Academy of Finland, Technology Development Center of Finland, Emil Aaltonen Foundation, Tampere; Finnish Heart Association, Sigrid Juselius Foundation, Helsinki; Roche Organ Transplant Research Fund (ROTRF), and the HUCH Research Fund.

The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked “advertisement” in accordance with 18 U.S.C. section 1734.

1
Baumheter
 
S
Singer
 
MS
Henzel
 
W
et al
Binding of L-selectin to the vascular sialomucin CD34.
Science.
262
1993
436
438
2
Rosen
 
SD
Endothelial ligands for L-selectin: from lymphocyte recirculation to allograft rejection.
Am J Pathol.
155
1999
1013
1020
3
Maly
 
P
Thall
 
AD
Petryniak
 
B
et al
The α(1,3)fucosyltransferase Fuc-TVII controls leukocyte trafficking through an essential role in L-, E-, and P-selectin ligand biosynthesis.
Cell.
86
1996
643
653
4
Hemmerich
 
S
Bistrup
 
A
Singer
 
M
et al
Sulfation of L-selectin ligands by an HEV-restricted sulfotransferase regulates lymphocyte homing to lymph nodes.
Immunity.
15
2001
237
247
5
Ellies
 
LG
Tsuboi
 
S
Petryniak
 
B
Lowe
 
JB
Fukuda
 
M
Marth
 
JD
Core2 oligosaccharide biosynthesis distinguishes between selectin ligands essential for leukocyte homing and inflammation.
Immunity.
9
1998
881
890
6
Homeister
 
JW
Thall
 
A
Petryniak
 
B
et al
The α(1,3)fucosyltransferase FucT-IV and FucT-VII exert collaborative control over selectin-dependent leukocyte recruitment and lymphocyte homing.
Immunity.
15
2001
115
126
7
Lowe
 
JB
Glycosylation, immunity, and autoimmunity.
Cell.
104
2001
809
812
8
Puri
 
KD
Finger
 
EB
Gaudernack
 
G
Springer
 
TA
Sialomucin CD34 is the major L-selectin ligand in human tonsil high endothelial venules.
J Cell Biol.
131
1995
261
270
9
Hiraoka
 
N
Petryniak
 
B
Nakayama
 
J
et al
A novel, high endothelial venule-specific sulfotransferase expresses 6-sulfo sialyl Lewis(x), an L-selectin ligand displayed by CD34.
Immunity.
11
1999
79
89
10
Yeh
 
J-C
Hiraoka
 
N
Petryniak
 
B
et al
Novel sulfated lymphocyte homing receptors and their control by a core 1 extension β1,3-N-acetylglucosaminyltransferase.
Cell.
105
2001
957
969
11
Toppila
 
S
Paavonen
 
P
Nieminen
 
M
Hayry
 
P
Renkonen
 
R
Endothelial L-selectin ligands are likely to recruit lymphocytes into rejecting human heart transplants.
Am J Pathol.
155
1999
1303
1310
12
Toppila
 
S
Paavonen
 
T
Laitinen
 
A
Laitinen
 
L
Renkonen
 
R
Endothelial L-selectin ligands in bronchial asthma but not in other chronic inflammatory lung diseases.
Am J Resp Cell Mol Biol.
23
2000
492
498
13
Kirveskari
 
J
Paavonen
 
T
Hayry
 
P
Renkonen
 
R
De novo induction of endothelial L-selectin ligands during kidney allograft rejection.
J Am Soc Nephrol.
11
2000
2358
2365
14
Paavonen
 
T
Renkonen
 
R
Selective expression of sialyl-Lewisx and sialyl Lewisa, putative ligands for L-selectin, on peripheral lymph node high endothelial venules.
Am J Pathol.
141
1992
1259
1264
15
Mitsuoka
 
C
Sawada-Kasugai
 
M
Ando-Furui
 
K
et al
Identification of a major carbohydrate capping group of the L-selectin ligand on high endothelial venules in human lymph nodes as 6-sulfo sialyl Lewis X.
J Biol Chem.
273
1998
11225
11233
16
Kirveskari
 
J
Vesaluoma
 
MH
Moilanen
 
JAO
et al
A novel non-invasive, in vivo technique for the quantification of leukocyte rolling and extravasation at sites of inflammation in human patients.
Nat Med.
7
2001
376
379
17
Papac
 
DI
Wong
 
A
Jones
 
AJ
Analysis of acidic oligosaccharides and glycopeptides by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry.
Analyt Chem.
68
1996
3215
3223
18
Toppila
 
S
Renkonen
 
R
Penttilä
 
L
et al
Enzymatic synthesis of α3′sialylated and multiply α3fucosylated biantennary polylactosamines: a bivalent sialyl diLex-saccharide inhibited lymphocyte endothelial adhesion organ selectively.
Eur J Biochemistry.
261
1999
208
215
19
Hemmerich
 
S
Leffler
 
H
Rosen
 
SD
Structure of the O-glycans in GlyCAM-1, an endothelial-derived ligand for L-selectin.
J Biol Chem.
270
1995
12035
12047
20
Varki
 
A
Selectin ligands: will the real ones please stand up?
J Clin Invest.
99
1997
158
162
21
Stein
 
JV
Cheng
 
G
Stockton
 
BM
Fors
 
BP
Butcher
 
EC
von Andrian
 
UH
L-selectin-mediated leukocyte adhesion in vivo: microvillous distribution determines tethering efficiency, but not rolling velocity.
J Exp Med.
189
1999
37
50
22
Turunen
 
J
Majuri
 
M
Seppo
 
A
et al
De novo expression of endothelial sialyl Lewis a and sialyl Lewis x during cardiac transplant rejection: superior capacity of a tetravalent sLex-oligosaccharide in inhibiting L-selectin-dependent lymphocyte adhesion.
J Exp Med.
182
1995
1133
1142
23
Renkonen
 
O
Toppila
 
S
Penttilä
 
L
et al
Enzyme-assisted synthesis of a tetravalent sialyl Lewis x glycan, derived from a linear polylactosamine.
Glycobiology.
7
1997
453
461
24
Toppila
 
S
Lauronen
 
J
Mattila
 
P
et al
L-selectin ligands in rat high endothelium: multivalent sialyl Lewis x glycans are high affinity inhibitors of lymphocyte adhesion.
Eur J Immunol.
27
1997
1360
1365

Author notes

Risto Renkonen, Biomedicum and Haartman Institute, PO Box 63 (Haartmaninkatu 8), SF-00014 University of Helsinki, Helsinki, Finland; e-mail: risto.renkonen@helsinki.fi.

Sign in via your Institution