From the Imperial Cancer Research Fund, Breast Cancer
Biology Group, 3rd Floor, Thomas Guy House, Guy's Hospital, London SE1
9RT, United Kingdom,
Department of Medicine, Division of
Rheumatology, Queen's University, Etherington Hall, Room 1021, 96 Stuart Street, Kingston K7L 3N6, Ontario, Canada, ** Electron
Microscopy Unit, Imperial Cancer Research Fund, 44 Lincoln's Inn
Fields, London WC2A 3PX, United Kingdom, and
School of Dentistry, Faculty of Health
Sciences, University of Copenhagen, Norre Alle 20, DK 2200 Copenhagen
N, Denmark
Received for publication, July 21, 2000, and in revised form, December 15, 2000
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ABSTRACT |
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In breast cancer, the O-glycans added
to the MUC1 mucin are core 1- rather than core 2-based. We have
analyzed whether competition by the glycosyltransferase, ST3Gal-I,
which transfers sialic acid to galactose in the core 1 substrate, is
key to this switch in MUC1 glycosylation that results in the expression
of the cancer-associated SM3 epitope. Of the three enzymes known to
convert core 1 to core 2, by the addition of GlcNAc to GalNAc in core1
C2GnT1 is the dominant enzyme expressed in normal breast tissue.
Expression of C2GnT1 is low or absent in around 50% of breast cancers,
whereas expression of ST3Gal-I is consistently increased. Mapping of
ST3Gal-I and C2GnT1 within the Golgi pathway showed some overlap. To
examine functional competition, the enzymes were overexpressed in T47D cells, which normally make core 1-based structures, have no detectable C2GnT1 activity and express the SM3 epitope. Overexpression of C2GnT1
resulted in loss of binding of SM3 to MUC1, accompanied by a decrease
in the GalNAc/GlcNAc ratio, indicative of a switch to core 2 structures. Transfection of a C2GnT1 expressing line with ST3Gal-I
restored SM3 binding and reduced GlcNAc incorporation into MUC1
O-glycans. Thus, even when C2GnT1 is expressed, the O-glycans added to MUC1 become core 1-dominated structures,
provided expression of ST3Gal-I is increased as it is in breast cancer.
Interest has been focused on the MUC1 mucin as a target antigen
for immunotherapy of breast and other carcinomas since the cancer-associated mucin is overexpressed and aberrantly glycosylated (1). The MUC1 mucin is a membrane glycoprotein with an extracellular domain made up largely of tandem repeats of 20 amino acids, each of
which contains potential O-glycosylation sites (2, 3). The
aberrant glycosylation has been well documented in breast cancers where
it has been shown (4, 5) that the addition of shorter
O-glycans leads to the exposure of peptide epitopes in the
tandem repeats, which are normally masked, and the appearance of novel
carbohydrate epitopes. Recent data suggest that not only the
composition but the number of O-glycans added to MUC1 is
altered in breast cancer (6). Thus, the cancer-associated glycoprotein is antigenically distinct from the normally processed mucins (7). This
difference in antigenic profile is detected by the antibody SM3 (8, 9),
which recognizes a core protein epitope selectively exposed in the
tandem repeat of the cancer-associated MUC1 mucin (10).
Analysis of the O-glycans attached to the mucin produced by
the normal lactating breast and by breast cancer cell lines has shown
that the oligosaccharides added to the normal mucin are core 2-based
structures (11), whereas in the cancer-associated mucin, shorter core
1-based structures dominate (4, 5, 12). As illustrated in Fig.
1, core 1 (Gal
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
1,3GalNAc-Ser/Thr) can
be a substrate for enzymes adding GlcNAc in the
1,6 linkage to
GalNAc to form core 2 or for sialyltransferases adding sialic acid in
2,3 linkage to galactose. These early steps in O-glycan
synthesis are crucial to the final definition of O-glycan
structure, since the conversion to core 2 promotes chain branching and
elongation, whereas the addition of sialic acid terminates chain
growth.
View larger version (18K):
[in a new window]
Fig. 1.
Pathways of O-glycosylation
of MUC1 in breast tissue and tumors. In normal mammary epithelial
cells, core 1 glycans are converted to core 2 by the action of
6GlcNAc transferases (mainly C2GnT1). In breast carcinomas this
conversion is reduced, resulting in the expression of mainly core
1-based structures, which are largely sialylated by ST3Gal-I.
Sialyl Tn or SialylT,
sialyltransferase.
In considering the potential competition of glycosyltransferases for the core 1 substrate, the level of activity of a specific glycosyltransferase and their relative positions in the Golgi pathway need to be considered. It now appears that glycosyltransferases are not confined exclusively to specific Golgi compartments but show a more diffuse distribution among compartments (13). For example, although the expression of the sialyltransferase ST3Gal-I1 is highest in the medial/trans-Golgi, some expression can be seen in the cis Golgi (14).
Another important finding is that most glycosidic linkages are in fact
formed by multiple glycosyltransferase isoenzymes that have different
kinetic properties and expression patterns and possibly different
subcellular distributions. Thus there are several transferases that are
able to add sialic acid in 2,3 linkage to the galactose moiety in
core 1 (15). However, of the cloned
2,3-sialyltransferases enzymes,
ST3Gal-I appears to play the major role in the sialylation of core 1 structures on MUC1 in breast, as deduced from enzyme specificity and
tissue distribution (16-18). Significantly, the ST3Gal-I enzyme has
been found to be elevated in breast cancer cell lines and primary
breast cancers (14, 19).
Similarly, formation of the branched complex type O-glycans
(core 2) may be controlled by at least three
6GlcNAcTs,2 which show
different patterns of expression in tissues. The enzymes C2GnT1 and
C2GnT3 (20, 21) act only on core 1 to produce core 2. On the other
hand, C2GnT2 or C2/4GnT (22, 23) is able to catalyze the formation of
core 4 from core 3 as well as core 2 from core 1. Of the C2GnTs
identified to date by cloning, it appears that C2GnT1 is the enzyme
most commonly expressed in breast tissue and tumors, although C2GnT3
can occasionally be expressed (this manuscript).
Although the expression of the C2GnT1 enzyme has been found to be
decreased or absent in most breast cancer cell lines (24, 14),
reasonable levels of the mRNA coding for this enzyme can be found
in a high proportion of primary breast cancers (19). This is in
contrast to the level of expression of ST3Gal-I mRNA, which is
consistently elevated in primary breast cancers (19). Moreover, the
level of expression of the mRNA coding for ST3Gal-I correlates with
the level of expression of the SM3 epitope and with tumor grade (19).
Since core 2 branching by 6GlcNAc-transferases is inhibited by
2,3 sialylation of core 1 in vitro (25, 26, 27), it
follows that ST3Gal-I could be a key controlling enzyme leading to
simple mucin type core 1 glycosylation pattern in cancer cells. The
question, however, is whether ST3Gal-I can effectively compete with
C2GnT1 in vivo, leading to an inhibition in the formation of
core 2 structures on MUC1 and whether this relates to exposure of the
cancer-associated SM3 epitope.
For competition to be effective, the enzymes must overlap in the
compartments of the Golgi apparatus. We have therefore examined in
detail the level of expression of C2GnT1 throughout the Golgi pathway
and compared this profile with the profile of expression of ST3Gal-I in
the same Golgi compartments. We find that although the peak expression
of C2GnT1 is in the cis and ST3Gal-I peaks in the medial/trans, the
enzymes did show partial overlap. To directly examine if this degree of
overlap is sufficient to allow competition between the two enzymes, we
transfected the cDNAs encoding C2GnT1 and ST3Gal-I into the breast
cancer cell line T47D (28). Our data clearly show that despite the
later peak of localization in the Golgi, the ST3Gal-I enzyme is able to
compete effectively with C2GnT1 for the core 1 substrate in
vivo, when the sialyltransferase is highly expressed. The results
show that the relative levels of the competing enzymes affect both the
structure of the O-glycans attached to MUC1 and the exposure
of the SM3 epitope. Thus, the SM3 epitope was exposed in breast cancer
cells expressing C2GnT1, providing the ST3Gal-I enzyme was elevated as
it is in breast cancer.
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EXPERIMENTAL PROCEDURES |
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Materials--
Biotinylated Arachis hypogaea Peanut
agglutinin (PNA) was from Vector laboratories Ltd. (Peterborough, UK).
Streptavidin-horseradish peroxidase,
D-[6-3H]glucosamine hydrochloride (26 Ci/mmol), MegaPrime kit and enhanced chemiluminescence (ECL) reagents
were from Amersham Pharmacia Biotech. pcDNA3 vector was from
Invitrogen. PBabe-puro retroviral vector was from Promega.
Clostridium perfringens and Vibrio cholerae sialidases were from Oxford Glycosciences (Abingdon, UK).
[-32P]dCTP (3,000 Ci/mmol) was from ICN.
Antibodies-- Supernatants of the mouse monoclonal antibodies HMFG-1, HMFG-2, and SM-3, reactive with MUC1, (29, 8) were used for FACS analysis. CT-1 polyclonal rabbit antibody was raised against the cytoplasmic tail of MUC1 (30).
Cell Culture-- The human mammary epithelial cell line MTSV1-7 was derived by SV40 immortalization of normal mammary epithelial cells isolated from human milk (31) and grown in E4, 10% FCS with 10 µg/ml insulin, 5 µg/ml hydrocortisone, and 0.3 µg/ml glutamine. The cell line T47D was derived from breast carcinoma cells isolated from a pleural effusion (28) and was cultured in E4, 10% FCS. HPAF, a human pancreatic carcinoma line, was grown in E4, 10%FCS.
Breast Tumors-- 20 frozen breast cancer tumor tissues were provided by Dr. Andrew Hanby, Imperial Cancer Research Fund Breast Pathology Group. All samples were classified as invasive ductal carcinoma grade 3 showing positive staining with the SM3 antibody. Before RNA extraction (which was done as described for the cell lines; see below), samples were kept in liquid nitrogen and then subject to mechanical dis-aggregation using a dis-membranator.
cDNA-- The cDNA encoding the human C2GnT1 was obtained from Dr. R. McEver (W. K. Warren Medical Research Institute, University of Oklahoma). A 950-base pair PstI fragment containing the open reading frame from +710 to +1,660 was used a probe for Northern analysis. The cDNA encoding the human ST3Gal-I (32) was obtained from Dr. J. Lau (Roswell Park Cancer Institute, Buffalo, NY). A 1,121-base pair open reading frame fragment released from a pCR2.1 vector (Invitrogen) by EcoRI digestion was used as a Northern probe. C2GnT2 (22) probe was a 1,227-base pair EcoRI digest of the expression vector pAcGP67-C2/4GnT-sol spanning the open reading frame from +91 to +1,318. The C2GnT3 (21) probe was a 1,254-base pair EcoRI/BamHI digest containing the open reading frame from +114 to + 1,368.
cDNA Constructs--
The full-length C2GnT1 cDNA-coding
region was ligated into the EcoRI site of pcDNA3
expressing the neomycin-selectable marker (Invitrogen). For Golgi
localization experiments, C2GnT1 cDNA was tagged with six 9E10 Myc
epitopes and cloned into the retroviral vector, pBabepuro. The
production of amphotrophic ST3Gal-I- and C2GnT1-expressing retroviruses
was essentially as previously described (14). Briefly, ST3Gal-I DNA
(tagged with an Myc epitope at the C terminus) and C2GnT cDNA,
subcloned into the pBabe puro vector, was transfected into the
amphotrophic packaging cell line AM12. 48 h after transfection,
cells were split 1:10 into growth medium containing 2 µg/ml puromycin
for selection. Medium was changed every 3 to 4 days for 4 weeks until
selection was complete. The retrovirus producer cell lines were grown
to 70% confluency, and the spent medium was replaced with a
half-volume of fresh medium. 3 days later, the virus-containing medium
was removed, filtered, quick frozen in dry ice, and stored at
70 °C.
Transfection of T47D Cells with C2GnT1-- T47D cells were transfected with pcDNA3neo-expressing C2GnT1 or with the empty vector to give the T47 E2B and T47D E2J cell lines expressing C2GnT and the T47D neo cell line expressing only the selectable marker. To ensure efficient transfection of cells and the isolation of stable clones, a modified method of electroporation in the presence of Me2SO was used, which improves the efficiency of transfection of epithelial cell lines (33). 1.25% Me2SO was included in both the electroporation cuvette and also after the pulse in the culture medium. Three days post-transfection T47D cells were split 1:10 into growth medium containing 500 µg/ml G418. Media were changed every 3 days until selection was complete and stable clones were expanded.
Transduction of T47D C2GnT1 Clones and the MTSV1-7 Cell Line-- For transduction of T47D-E2B, T47D-E2J, and MTSV1-7 cell lines with the ST3Gal-I and C2GnT1 retroviruses, cells were seeded at ~1 × 105 cells/well on a 6-well plate overnight, then 2 ml of retroviral supernatant (derived from transfection of packaging cell line above) was added along with sterile Polybrene at 8 µg/ml and incubated for 7 h. Medium was then changed to E4, 10% FCS for T47D and E4, 10% FCS + 10 µg/ml insulin and 5 µg/ml hydrocortisone for MTSV1-7, and cells were left for 24 h. At this time the medium was changed to contain the appropriate antibiotic for selection. Selection was continued for 7 days, after which individual clones were isolated and expanded.
Localization of C2GnT1 within the Golgi Apparatus--
MTSV1-7
cells (31) were transduced with the Myc-tagged C2GnT1 retrovirus (34),
and clones were isolated. Cells were fixed for 1 h at room
temperature in 0.1% glutaraldehyde, 4% paraformaldehyde before being
scraped, spun, and stored overnight at 4 °C. Pellets were then
stained with the 9E10 monoclonal antibody followed by goat anti mouse
Ig coupled to 10-nm gold particles and processed for electron
microscopy as described by Whitehouse et al. (14). The
orientation of the Golgi was determined by reference to the position of
1-4 galactosyltransferase (GalT1) using rabbit antibody to GalT1 (a
generous gift from Dr. Eric Berger) and followed by protein A coupled
to 5-nm gold particles. Quantitation was performed as described by
Whitehouse et al. (14).
Assays of Glycosyltransferase Activities--
Cells were
harvested and washed three times in phosphate-buffered saline. 1 ml of
0.25 M sucrose was added to 108 cells, and the
cells were hand-homogenized and stored at 80 °C. The activities of
6GlcNAc transferase and ST3Gal(O) transferase in cell homogenates
were measured using Gal
1,3GalNAc-nitrophenol as substrate, and the
product was estimated by high performance liquid chromatography, as
described by Brockhausen et al. (24). Activities were
expressed as nmol/h/mg.
Fluorescence-activated Cell-scanning Analysis (FACScan)-- Cells were trypsinized and washed once in growth medium, and a minimum of 5 × 105 cells were resuspended in 100 µl of the appropriate specific antibody diluted in growth medium, neat tissue culture supernatant, or in 100 µl of growth medium alone as a negative control. All incubations were carried out in the presence of 0.02% sodium azide and on wet ice. After a 30-min incubation, cells were washed three times in growth medium containing 0.02% sodium azide. Cells were resuspended in 100 µl of fluorescein isothiocyanate-conjugated rabbit anti-mouse immunoglobulins, diluted 1:40 in growth medium, and incubated for 30 min in the dark. After washing three times in growth medium containing 0.02% sodium azide, cells were resuspended in 300 µl of phosphate-buffered saline, and 10,000 cells were analyzed by a Becton Dickinson FACScan. For FACS analysis of PNA binding, cells were incubated with or without sialidase (V. cholerae), 0.06 units/ml, and analyzed for the binding of fluorescein isothiocyanate-conjugated PNA as described previously (7).
Northern Analysis of RNA--
Total RNA was extracted from cell
lines or breast tumors using TRIZOL as per the manufacturer's
instructions. Placental poly(A)+ RNA was obtained from
CLONTECH. RNA was run on 1% agarose, 2.2 M formaldehyde-diethyl pyrocarbonate gel in running buffer
(0.02 M MOPS, 8 mM sodium acetate, 1 mM EDTA, pH 7.0, in diethyl pyrocarbonate water). After
denaturing, the RNA was transferred and immobilized onto Hybond-N
membrane and incubated with -32P-labeled probe (labeled
using MegaPrime kit with [
-32P]dCTP) and hybridized
overnight at 65 °C. Filters were then washed for 1 h in buffer
A (0.08 M sodium phosphate, 2 mM EDTA, 5%
bovine serum albumin, 10% SDS) at 65 °C, then twice in buffer B
(0.16 M sodium phosphate, 4 mM EDTA, 4%SDS)
for 1 h at 65 °C and then exposed to a Kodak phosphor screen
overnight and visualized using a STORM scanner system.
Cell Lysis-- Cells grown to around 80% confluence in a T75 flask were washed twice in 10 ml of ice-cold phosphate-buffered saline and lysed in 0.4 ml of radioimmune precipitation buffer (20 mM sodium phosphate, pH 7.2, 50 mM sodium fluoride, 5 mM EDTA, 1% Triton X-100, 1% deoxycholate, 109 µg/ml phenylmethylsulfonyl fluoride, 25 µg/ml leupeptin, 10 µg/ml aprotinin). Cells were scraped off, the flask was washed with an additional 0.2 ml of radioimmune precipitation buffer, and the lysates were spun at 14,000 × g for 10 min at 4 °C. Supernatant was used for Western blotting or MUC1 immunoprecipitation.
Analysis of Hexosamine Content of MUC1-- Changes in the hexosamines in the side chains of MUC1 were analyzed by high performance anion exchange chromatography (HPAEC) after metabolically labeling the glycoprotein with [3H]glucosamine hydrochoride and precipitating with the CT-1 antibody as previously described (4). Briefly, cells in 75-cm2 flasks at 70-80% confluence were incubated for 2 h with medium containing reduced glucose (0.45 g/liter) before changing to low glucose medium (3 ml) containing 100 µCi/ml [3H]glucosamine hydrochoride. After overnight incubation, cells were lysed, and 500 µl of the lysate was pre-cleared with pre-immune rabbit serum and protein A-Sepharose beads. The radioactively labeled MUC1 was immunoprecipitated with 10 µl of CT-1 polyclonal antibody (30), which was directed to the cytoplasmic tail and precipitated all glycoforms of the mucin. Protein A-Sepharose was then added, and the complex was removed by centrifugation and washed thoroughly. The immunoprecipitate was eluted in 2% SDS and hydrolyzed in 2 N trifluoroacetic acid at 100 °C for 3 h and then analyzed by HPAEC on a CarboPak PA1 column by isocratic elution with 0.01 M NaOH.
Western Blotting--
300 µg of cell lysate were incubated
with or without 1.0 unit of C. perfringens sialidase in 50 mM sodium acetate buffer, pH 5.0, in a 37 °C water bath
overnight. 50 µg of lysate was separated on a 12% SDS-polyacrylamide
gel and then blotted onto nitrocellulose in Towbin buffer using a
Bio-Rad semi-dry electroblotter. The blot was blocked overnight at
4 °C in 1× phosphate-buffered saline, pH 7.4, 0.2% Tween 20, 1.0%
bovine serum albumin (PTB solution) and then incubated with
biotinylated PNA (5 µg/ml in 20 ml PTB solution) for 1 h at room
temperature with gentle agitation. After 3 washes in PTB solution, the
blot was incubated for 1 h at room temperature with
streptavidin-horseradish peroxidase (1/2000 dilution in 20 ml of PTB
solution). After 3 additional washes, the bound lectin-streptavidin-horseradish peroxidase was detected using enhanced
chemiluminescence (ECL) and light-sensitive film.
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RESULTS |
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Expression of 6GlcNAc T Activity in Normal and Malignant Breast
Tissue and Epithelial Cell Lines--
Genes coding for three enzymes
able to synthesize core 2 (C2GnT1, C2GnT2, and C2GnT3) from core 1 have
been isolated (20-22). Expression of these enzymes in the T47D breast
cancer cell line and in the nonmalignant MTSV1-7 cells was examined by
Northern analysis. Fig. 2 shows that none
of these enzymes were expressed in T47D cells, whereas C2GnT1 and
C2GnT3, but not C2GnT2, were expressed in MTSV1-7 cells (Fig.
2B, lane 1). When RNA from normal breast tissue
was examined, only C2GnT1 could be detected, mRNA for the other two
enzymes being undetectable (Fig.
3A). A positive control for
the C2GnT2 mRNA is shown in lane 3 of Fig.
2B, containing RNA from the pancreatic carcinoma cell line
HPAF (Fig. 2B, lane 3).
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In situ hybridization analysis of primary breast cancers has shown that C2GnT1 levels vary widely among breast carcinomas, whereas levels of ST3Gal I mRNA are consistently increased (19). At the time of this analysis, cDNAs coding for the C2GnT2 and C2GnT3 enzymes were not available. To document expression of all three enzymes in malignancy, we performed Northern analysis on RNA from 20 primary breast cancers. All tumors were classified as invasive ductal carcinomas Grade III, and all stained positively with the SM3 antibody. The analysis showed that C2GnT2 was not expressed in any of the tumors. On the other hand, C2GnT1 was found to be expressed at reasonable levels in 10 of the 20 cancers, the others showing weak or undetectable expression. Clearly detectable levels of C2GnT3 mRNA were seen in only one of the 20 tumors, with one other giving a weak signal. Fig. 3B shows Northern blots of four of the tumors with the three relevant probes. In Fig. 3B, I, lane 4 shows an example of the bands seen in 1 of the 10 tumors expressing reasonable levels of C2GnT1, whereas the other tumors (lanes 1-3) show very low expression. Fig. 3B, III, lane 1 shows the band detected in the only tumor showing a clearly detectable level of C2GnT3. This enzyme appeared to be completely absent from 18 of the 20 tumors, with one other showing a very weak band.
Thus, the key enzyme capable of synthesizing the core 2 structure in normal and malignant breast epithelial cells appears to be C2GnT1. Whereas expression of C2GnT3 is a rare event in breast cancer, the MTSV1-7 cell line was found to express this enzyme. Although retaining many features of the normal luminal epithelial cell, this line was derived by immortalizing cultured milk epithelial cells with SV40 T antigen, which may have modified gene expression. Since the T47D cell line does not express any of the core 2-synthesizing enzymes but has elevated levels of ST3Gal-I (24), it represents an appropriate cell for following the effect of overexpressing C2GnT1 on O-glycan structure.
Localization of C2GnT1 within the Golgi Apparatus--
For the
C2GnT1 transferase to compete with the ST3Gal-I enzyme for the core 1 substrate in breast epithelial cells, there must be some overlap in
their positions in the Golgi pathway. We have previously shown that
although the ST3Gal-I transferase is located mainly in the medial/trans
compartments of the Golgi apparatus (14), a detectable level of
expression can also be seen in the cis-Golgi. The nonmalignant mammary
epithelial cell line MTSV1-7 transfected with the Myc-tagged ST3Gal-I
cDNA was used for the detailed mapping of this enzyme because the
structure of the Golgi apparatus is well defined in these cells.
Moreover, the use of tagged constructs to localize glycosyltransferases in transfected cells has been shown to give similar results for Golgi
localization to that seen with direct detection of endogenous enzymes
(13). To determine whether C2GnT1 localization overlapped with
ST3Gal-I, C2GnT1 cDNA was tagged with 9E10 Myc epitopes and transduced into MTSV1-7. To orient the Golgi apparatus, an antibody to
1-4 galactosyltransferase (GalT1) operative in N-linked
glycosylation and that has been previously mapped to the trans
cisternae and the TGN (35) was used in double-labeling experiments
(data not shown). The distribution of C2GnT1 across the Golgi apparatus was determined by counting the gold particles across the Golgi stack
using a method described in Whitehouse et al. (14). This method provides a more detailed analysis of the distribution of C2GnT1
across the Golgi stack rather than dividing the Golgi into each
cisternae, as the stack often consist of more than three cisternae and,
therefore cannot be simplified into cis, medial, and trans. Fig.
4 shows the distribution of C2GnT1 in
comparison with ST3Gal-I. The peak of C2GnT1 localization appears in
the early part of the Golgi, probably corresponding to the cis. There is, however, some expression in the medial compartment and low but
detectable levels in the trans-Golgi. Thus, as can be seen from Fig. 4,
although on the whole C2GnT1 is localized earlier than ST3Gal-1, there
is a degree of overlap between the two enzymes that could allow for
competition for the core 1 substrate.
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Expression of C2GnT1 in T47D Cells Modifies the Structure of the
MUC1-O-glycans--
To directly examine the competition between
ST3Gal-I and C2GnT1, the cDNA coding for the human C2GnT1 enzyme
was transfected into T47D cells (which do not normally express this
enzyme), and several clones were isolated. Two cell clones were
expanded for analysis, T47D- E2B and T47D-E2J. T47D-E2B was selected
because it had a 6GlcNAc transferase activity similar to that of
MTSV1-7, a nonmalignant cell line, and T47D-E2J was selected because
it had an activity considerably higher (3-fold). Both lines
demonstrated significant elevation in C2GnT1 mRNA by Northern
hybridization (data not shown). Table I
shows the expression of C2GnT1 as measured by the activity of
6GlcNAc transferase in these two clones.
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To look for changes in the structure of the O-glycans added
to MUC1, the parental cell line and transfectants were labeled with
[3H]glucosamine, and the radioactively labeled MUC1 was
precipitated using the polyclonal antibody CT-1, which reacts with
epitopes in the cytoplasmic tail and precipitates all glycoforms (see
"Experimental Procedures"). The hexosamine content of the
O-glycans carried on the mucin was then determined as
previously described (4, 14), and the results are shown in Fig.
5 and Table I. As compared with the
parental T47D cell line and the mock transfectant T47D-Neo, the
O-glycans carried on MUC1 in the C2GnT1 transfectants showed a higher content of GlcNAc. This would be explained by the branching and chain extension that is initiated by the addition of GlcNAc by
C2GnT1, which is absent in parental cells.
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The Addition of the Extended O-Glycans in T47D Cells Expressing
High Levels of C2GnT1 Leads to the Masking of the SM3 and HMFG2
Epitopes in the MUC1 Mucin--
A correlation between the structure of
MUC1 O-glycans and the reactivity of MUC1 with the SM3
antibody, recognizing a cancer-associated epitope in the tandem repeat
sequence of MUC1 (8, 9), has been previously demonstrated (7, 36).
Thus, MUC1 from T47D, which carries core 1 structures, reacts with SM3,
whereas MUC1 expressed by MTSV1-7, which carries mainly core 2-based
structures, does not. Fig. 6 shows that
when C2GnT1 is highly over expressed in T47D, as it is in the T47D E2J
cell line, the cancer-specific epitope recognized by SM3 becomes barely
detectable.
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The reactivity of MUC1 from T47D E2J with two other antibodies (HMFG1 and HMFG2) that recognize core protein epitopes in the tandem repeat (10) was also examined. The reactivity of the antibody HMFG2 has been shown to be reduced but not abolished when the O-glycans added to MUC1 are core 2-based (7). On the other hand, the antibody HMFG1 reacts well with MUC1 carrying core 2-based O-glycans (7). Fig. 6 shows that, as expected, the reactivity of HMFG2 with MUC1 produced by the E2J cell line is reduced, whereas HMFG1 reactivity is largely unaffected. Fig. 6 shows the staining for the high expressing clone T47D-E2J, but a 4-fold reduction in the binding of SM3 and HMFG2 is also seen with clone E2B (see below, Fig. 8). Binding of HMFG1, however, remains constant in all the cell lines, indicating that the level of MUC1 expression is similar.
Increasing the Level of the ST3Gal-I Transferase in T47D Cells Expressing C2GnT1 Induces Re-expression of the SM3 and HMFG2 Epitopes-- The data of Figs. 5 and 6 demonstrate that the C2GnT1 enzyme can override the glycosylation pattern of T47D cells, leading to chain extension and masking of the SM3 epitope and a reduction in the expression of the HMFG2 epitope. This effect might be predictable from the fact that the C2GnT1 enzyme (when present) has earlier access to the core 1 substrate and, therefore, makes it unavailable to the ST3Gal-I. On the other hand, we have observed that some breast cancers and breast cancer cell lines (e.g. MCF-7) express the C2GnT1 enzyme, but the SM3 epitope is not completely masked (14, 19). Analysis by in situ hybridization, however, showed that most of the breast cancers express increased levels of the ST3Gal-I enzyme. Indeed the level of expression of ST3Gal-I appears to correlate with tumor grade (19). Moreover, the increase in expression of the mRNA coding for ST3Gal-1 has now been shown to be accompanied by an increase in the level of protein using immunohistochemical analysis with a recently developed monoclonal antibody to this enzyme.3
To test whether increased expression of ST3Gal-I can compete
effectively with C2GnT1 for the core 1 substrate in breast cancer cells, cDNA coding for ST3Gal-I (tagged with the 9E10 Myc epitope) was introduced into the core 2-expressing cell lines T47D-E2B and
T47D-E2J. The transfected cells were then analyzed for ST3(O) and
6GlcNAc transferase activities, for hexosamine content of O-glycans attached to MUC1, and for expression of the SM3 epitope.
Table II shows the ratio of activities of
ST3(O) transferase and 6GlcNAc transferase for several
ST3Gal-I-transfected clones derived from the E2B cell line together
with the level of staining with SM3. The core 1 sialyltransferase
activity in cell extracts could include other ST3(O) enzymes besides
ST3Gal-I. Similarly, the core 2-synthesizing activity could formally
include other enzymes catalyzing this reaction. However, because the
respective activities increase with the transfection of ST3Gal-I and
C2GnT1, it is highly probable that the activities being measured are
ST3Gal-I and C2GnT1. Moreover, the clone T47D-E2B-ST4 showing the
highest level of expression of ST3Gal-I also showed a high level of
expression of mRNA coding for this enzyme (data not shown). That
the ST3Gal-I transferase is functional in vivo in fully
sialylating core 1 structures is shown by the complete loss of
reactivity of the transfectants with peanut lectin (shown for
T47D-E2B-ST4 in Fig. 7).
|
|
It can be seen from Table II that re-expression of the SM3 epitope
correlates with the highest expression of ST3(O) activity in clone
T47D-E2B-ST4. The detailed FACS analysis of antibody reactivity is
shown in Fig. 8 for T47D-E2B-ST4 compared
with the E2B and parental T47D cell lines. Clearly, whereas expression of the MUC1 epitopes recognized by SM3 and HMFG2 are significantly decreased in the E2B cells expressing moderate levels of C2GnT1, their
expression is increased in ST4 cells, where the ratio of ST3Gal-I
activity to C2GnT1 activity is high. In contrast to the results with
the E2B cell line, none of the ST3Gal-I transfectants of the high
C2GnT1 line, E2J, showed re-expression of the SM3 epitope by FACS
analysis (data not shown).
|
The appearance of the SM3 epitope was accompanied by changes in the
composition of the O-glycans attached to MUC1. Thus,
analysis of the hexosamines in O-glycans attached to MUC1
from T47D-E2B-ST4 cells demonstrated a decrease in the ratio of GlcNAc
to GalNAc (compared with T47D-E2B) as indicated in Fig.
9. Since in T47D-E2B cells the only
pathway leading to chain branching/extension from core 1 is via core 2, thus incorporating GlcNAc, the results demonstrate unequivocally that
ST3Gal-I can compete effectively with C2GnT1 for the core 1 substrate.
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DISCUSSION |
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The O-glycans added in mucin-type O-glycosylation are constructed by adding sugars individually and sequentially as the protein/glycoprotein passes through the Golgi apparatus. This means that, providing the relevant glycosyltransferases overlap in the Golgi, enzymes that use the same substrate but add different sugars can compete for the common substrate. Two enzymes, C2GnT1 and ST3Gal-I, both of which can use core 1 as a substrate, appear to be important players in defining the final structure of the O-glycans added to MUC1 in breast cancer, since they control chain branching/extension and chain termination, respectively. Although it should be noted that C2GnT3 mRNA was detected in a small number of breast carcinomas (1/20), nevertheless C2GnT1 appears to be the dominant and, hence, influential, core 2 synthesizing glycosyltransferase in both normal and malignant tissue from the mammary gland Our previous data showed that ST3Gal-I is localized mainly in the medial/trans-Golgi, with detectable levels in the cis-Golgi (14). We now show that in mammary epithelial cells, C2GnT1 is located mainly in the cis-Golgi but with some expression in the medial cisternae and low but detectable levels in the trans-Golgi (Fig. 4). This is in agreement with other investigators who have found, using confocal microscopy, C2GnT1 to be mainly in the cis/medial-Golgi of Chinese hamster ovary cells (38).
To determine whether the level of overlap is sufficient to allow
competition between the two enzymes, we have developed transfectants of
a breast cancer cell line T47D that show different ratios of expression
of C2GnT1 and ST3Gal-I. To demonstrate competition between the enzymes
in vivo, changes in O-glycan composition were studied by determining the relative levels of the hexosamines GalNAc
and GlcNAc in MUC1 O-glycans. It should be noted that we have previously shown a decrease in the ratio of GlcNAc to GalNAc in
MUC1 O-glycans in MTSV1-7 cells transfected with ST3Gal-I
(14). However, this cell line shows activity not only of two core
2-synthesizing enzymes but also of the 3GlcNAc transferase, which
adds GlcNAc to the Gal moiety in core 1 (24). Thus the ST3Gal-I enzyme
could theoretically be competing with this activity or with C2GnT3. T47D cells, however, do not express either of these enzymes (Ref. 24
and this paper); therefore the reduction in the GlcNAc to GalNAc ratio
seen in the ST3Gal-I-transfected T47D E2B cells can be unequivocally
attributed to competition between the ST3Gal-I and C2GnT1 transferases.
Thus, even though the evidence for localization suggests that the peak
localization of C2GnT1 is positioned earlier than the peak localization
of the ST3Gal-I enzyme in the Golgi pathway, when ST3Gal-I activity is
increased, this termination pathway dominants over the C2GnT1-branching pathway.
Our interest in the competition between the two enzymes analyzed here
stemmed from the observation that ST3Gal-I activity was found to be
consistently increased, whereas the level of C2GnT1 activity was not
always reduced in breast cancers. Moreover, there was a strong
correlation between the levels of expression of ST3Gal-I and the SM3
epitope (19). In this report, we show that SM3 and HMFG2 reactivity to
MUC1 is dependent on the relative activities of both C2GnT1 and
ST3Gal-I. The results are consistent with the idea that in breast
cancers, where the levels of ST3Gal-I are increased, competition with
C2GnT1 is effective, resulting in a reduced content of GlcNAc in the
O-glycans attached to the cancer mucin and exposure of the
SM3 epitope. It is of interest to note that even in the rare tumors
expressing the C2GnT3 mRNA, the SM3 epitope was detectable,
suggesting that the ST3Gal-I enzyme can also compete effectively with
this core 2-synthesizing enzyme. Competition in vivo between
ST3Gal-I and the 6GlcNAc transferase expressed in T cells, which
could be the C2GnT3 enzyme (21), has also been reported (39). These
studies used mice defective in ST3Gal-I to demonstrate that the
structure of the O-glycans on molecules such as leukosialin
found on peripheral CD8+ T cells has a dramatic effect on the survival
and differentiation of these cells. Whether the increased expression of
ST3Gal-I, which we have identified in breast cancers, affects function,
possibly by affecting cell interactions, is unclear. Certainly core 1 carrying a sialic acid in
2,3 linkage is a major ligand for
sialoadhesin, and MUC1 carrying such glycans interacts well with this
sialic acid binding protein found on macrophages, which can be
found as infiltrates in a proportion of breast cancers (37).
The effect of increasing C2GnT1 activity on MUC1 glycosylation has been studied in a pancreatic carcinoma cell line where again the SM3 epitope was lost (36). The loss of the SM3 binding to MUC1 is apparently due to the core 2 branch masking the polypeptide PDTRP motif recognized by SM3 (10). This steric hindrance by the core 2 branch of access to the VNTR region of the MUC1 polypeptide could also explain the approximate 2-fold reduction in actual number of O-glycans attached to MUC1 in normal cells compared with T47D cells (6). In this case, access for the GalNAc transferases adding the first sugar to serines and threonines would be blocked.
In conclusion, we have presented evidence that ST3Gal-I can compete
with C2GnT1 in directing core structure synthesis on MUC1 in breast
cancer. We therefore argue that it is primarily the elevation of
ST3Gal-I in breast cancer that leads to the dominant expression of core
1 O-glycans on MUC1 in this condition.
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ACKNOWLEDGEMENTS |
---|
We thank Jimmy Yang and Michael Lehotay for
help in performing the 6GlcNAc transferase and ST3(O) enzyme assays
and Dr. Joseph Lau (Roswell Park Cancer Institute, Buffalo, NY) and Dr.
Roger McEver (University of Oklahoma) for generous gifts of human
ST3Gal-I and C2GnT1 cDNA, respectively. We also thank Dr. Eric
Berger for the GalT1 polyclonal antibody.
![]() |
FOOTNOTES |
---|
* This work was supported by European Union Biotech Grant B104 CT96 0139.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.
§ Contributed equally and should be considered joint first authors.
¶ Present address: Div. of Medical and Molecular Genetics, 8th Floor, Guy's Tower, Guy's Hospital, London SE1 9RT, UK.
§§ To whom correspondence should be addressed. Tel.: 44 20 7955 2310/4542; Fax: 44 20 7955 2027; E-mail: papadimi@icrf.icnet.uk.
Published, JBC Papers in Press, December 15, 2000, DOI 10.1074/jbc.M006523200
1
ST3Gal-I (SiaT-4a) refers to a sialyltransferase
with GenBankTM accession number L13972. C2GnT1 (C2GnT,
C2GnT-L), C2GnT2 (C2/C4GnT, C2GnT-M), and C2GnT3 refer to human
6GlcNAc-transferases with GenBankTM accession numbers
M97347, AF038650/AF102542, and AF132035, respectively.
3 U. Mandel, J. M. Burchell, J. Taylor-Papadimitriou, and H. Clausen, manuscript in preparation.
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ABBREVIATIONS |
---|
The abbreviations used are:
6GlcNAc-T, UDP-N-acetyl-
-D-N-acetylglucosamine:
Gal/
GalNAc-1,6-N-acetylglucosaminyltransferase;
ST3(O), CMP-Neu5Ac:Gal
1,3GalNAc-
2,3-sialyltransferase;
PNA, peanut
agglutinin;
FCS, fetal calf serum;
FACScan, fluorescence-activated
cell-scanning analysis;
MOPS, 4-morpholinepropanesulfonic acid;
HPAEC, high performance anion exchange chromatography.
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