From the
Mayo Clinic Cancer Center and Divisions of Gastroenterology and Hepatology,
Experimental Pathology, ¶Nephrology, and ||Oncology Research, Mayo Clinic and Foundation, Rochester, Minnesota 55905
Received for publication, March 3, 2003 , and in revised form, April 8, 2003.
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ABSTRACT |
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INTRODUCTION |
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The sulfation state of HSPGs is classically thought to reflect the activity of sulfotransferases that are active during HSPG biosynthesis. Dhoot et al. (7), however, previously identified the quail sulfatase QSulf-1 as a developmentally regulated protein that modulates Wnt signaling by altering HSPG sulfation. Unlike many other sulfatases, which are lysosomal enzymes, QSulf-1 was localized on the cell surface (7). These observations raise the possibility that signaling by other HB-GFs might be modulated by cell surface sulfatase expression.
Morimoto-Tomita et al. (8) recently utilized the EST KIAA1077 to identify HSulf-1 as a human homolog of QSulf-1. Upon expression in Chinese hamster ovary cells, HSulf-1 reportedly is released into the medium, where it catalyzes endo-glucosamine-6-sulfatase activity (8). Further analysis by PCR demonstrated that HSulf-1 mRNA was expressed in a variety of tissues, including ovary, although the size of the transcripts and the possibility of alternative splice forms was not investigated (8).
In a recent study, we performed suppression subtraction hybridization analyses of two early and late stage tumors subtracted against normal ovarian epithelial brushings, and we demonstrated that the mRNA corresponding to KIAA1077 is down-regulated (9). In view of the report of Dhoot et al. (7) identifying Qsulf-1 as a modulator of Wnt signaling, this observation raised the possibility that KIAA1077 down-regulation might alter growth factor signaling in ovarian cancer. Current understanding suggests that generation of the neo-plastic phenotype requires multiple genetic or epigenetic changes that increase proliferation, inhibit apoptosis, and enhance cell invasiveness (10). Of interest in the present context is the observation that enhanced signaling by certain "growth factors" can simultaneously stimulate proliferation and inhibit apoptosis (1113). Elevated expression of and signaling by growth factors that activate the mitogen-activated kinase pathway, including FGF and HB-EGF, have been seen frequently in ovarian cancers and other solid tumors (1420). Moreover, activation of the ERK pathway has been implicated in enhanced proliferation as well as resistance to apoptosis (21, 22). As a result, there is considerable interest in understanding the factors that contribute to activation of this pathway as well as mechanisms that can reverse this activation.
In this report, we describe the widespread down-regulation of HSulf-1 in cancer cell lines and ovarian cancer specimens. To examine the functional consequences of this down-regulation, we re-expressed HSulf-1 in two ovarian cancer cell lines that lack this message. Results of this analysis suggest that HSulf-1 is a cell surface sulfatase that diminishes HSPG sulfation, thereby modulating signaling by HB-GFs. Consistent with this conclusion, we demonstrate diminished ERK pathway activation after treatment with FGF-2 and HB-EGF, diminished proliferation, and enhanced drug-induced apoptosis in ovarian cancer cell lines in which HSulf-1 is re-expressed. These observations not only provide new insight into the function of HSufl-1, but also suggest that its down-regulation is a previously unidentified mechanism by which cancer cells enhance growth factor signaling.
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MATERIALS AND METHODS |
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Drugs and ReagentsStaurosporine (Sigma) and UCN-01 (Drug Synthesis Branch, NCI, National Institutes of Health) were dissolved in Me2SO at a concentration of 1 mM, stored at 20 °C, and subsequently diluted with serum-free medium before use. In all experiments the concentration of Me2SO did not exceed 0.1%. Cisplatin (Sigma) was prepared immediately before use as a 1000-fold concentrated solution in Me2SO. Fibroblast growth factor, heparin-stabilized FGF, and heparin-binding epidermal growth factors (Sigma) were dissolved in water.
Cloning of HSulf-1 cDNA and GeneBLAST search of the isolated sequence from SSH libraries of early and late stage tumors identified ESTs homologous to KIAA1077 in the dbEST. The homologous ESTs were assembled into a contig with the use of Sequencher 3 software (Gene Codes Corp, Ann Arbor, MI). Additional 5' sequences not present in KIAA1077 were obtained with electronic walking by assembling overlapping EST sequences in the genome BLAST server. The integrity of the full-length cDNA obtained by this electronic walking was confirmed by PCR analysis using PCR primers flanking each junction between EST clones.
For expression of truncation mutants of HSulf-1, the N-terminal portion of HSulf-1 (N-Sulf) containing only the sulfatase domain was amplified using primers NF (5'-ATTGGACCAAATACAATGAAG-3') and NRFlg (ttaagccttgtcatcgtccttgtagtcGAATGTATCACGCCAAAT), where the lowercase letters encode the FLAG epitope. The C-terminal portion of HSulf-1 (C-Sulf) was amplified using primers CF (5'-CGTGATACATTCCTAGTGG) and CRFlg (ttaagccttgtcatcgtccttgtagtcACCTTCCCATCCATCCCA) with a stop codon introduced after the epitope tag. The full-length HSulf-1 was amplified using primers NF and CRFlg using ExpandTM Long Template PCR system (Roche Applied Science). All three products were cloned into GFP Fusion TOPO® TA Expression plasmid (Invitrogen). For generating a full-length HSulf-1/GFP fusion construct, the stop codon of CRFlg was not included. cDNAs generated from short term cultures of normal ovarian surface epithelial cells were used as a template for generating PCR products for cloning. The products of each PCR were resolved on a 1.6% agarose gel and purified using a gel extraction kit (Qiagen, Valencia, CA) for cloning into expression vectors.
Establishment of Stable TransfectantsExponentially growing SKOV3 cells in 100-mm dishes were washed with serum-free medium and treated with a mixture containing 4 µg of plasmid, 30 µl of LipofectAMINE, and 20 µl of Plus reagent. After 3 h of incubation, complete medium with serum was added. G418 (400 µg/ml) was added 24 h later to select transfectants. Individual colonies were subsequently cloned using cloning cylinders. For controls, cells were similarly transfected with vector (pcDNA3.1 GFP-CT); and stable clones were selected.
Semi-quantitative RT-PCRTotal RNA was extracted from 7 ovarian cancer cell lines and 30 primary ovarian tumors using the RNeasy mini kit (Qiagen). cDNA synthesis was performed as described (9). 50100 ng of reverse-transcribed cDNA was used in a multiplex reaction with three different primer pairs Sulf-1F (5'-CCACCTTCATCAATGCCTT-3') and Sulf-1R (5'-CCTTGACCAGTCCAAACCTGC-3'), Sulf-2F (5'-CATCATTTACACCGCCGACC) and Sulf-2R (5'-CTGCCGTCTCTTCTCCTTC-3'), Sulf-3F (5'-GAGCCATCTTCACCCATTCAA-3') and Sulf-3R (5'-TTCCCAACCTTATGCCTTGGGT-3'), and GAPDH-F (5'-ACCACAGTCCATGCCATCAC-3') and GAPDH-R (5'-TCCACCACCCTGTTGCTTGTA-3') in separate reactions to yield 760-, 1260-, and 825-bp products, respectively. The PCR mixes contained 50 mM KCl, 10 mM Tris-HCl (pH 8.3), 1.5 mM MgCl2, 400 µM concentration of each primer for HSulf-1 and 50 µM for the GAPDH primers, and 0.5 units of Taq polymerase (Promega) in a 12.5-µl reaction volume. The conditions for amplification are as follows: 94 °C for 3 min followed by 29 cycles of 94 °C for 30 s, 58 °C for 30 s, and 72 °C for 30 s in a PerkinElmer Life Sciences 9600 Gene-Amp PCR system. The products of the reaction were resolved on a 1.6% agarose gel and photographed using the Gel Doc 1000 photo documentation system.
LOH AnalysisThe 5 pairs of microsatellite markers within the HSulf-1 gene used in this study are listed in Table I along with their locations within the HSulf-1 gene. Amplifications were performed as described (9) except that annealing was performed at 5257 °C, and reactions were run in a 96-well plate. After denaturation, PCR products were run on 6% polyacrylamide sequencing gels containing 8 M urea. Gels were dried, subjected to autoradiography using multiple exposure times, and scored for LOH. Allelic imbalance indicative of LOH was scored, and a >50% loss of intensity of one allele in the tumor sample with respect to the matched allele from normal tissue was observed.
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Northern BlotTotal RNA (15 µg) was fractionated on 1.2% formaldehyde agarose gels and blotted in 1x SPC buffer (20 mM Na2HPO4, 2 mM CDTA (pH 6.8)) onto Hybond-N membranes (Amersham Biosciences). The probes were labeled using the random primer labeling system (Invitrogen) and purified using spin columns (100 TE) from Clontech. Filters were hybridized at 68 °C with radioactive probes in a hybridization incubator and washed according to the manufacturer's guidelines.
Analysis of ApoptosisApoptosis was quantitated by assessing the number of cells containing nuclear changes indicative of apoptosis (chromatin condensation and nuclear fragmentation) after staining with DAPI. HSulf-1-transfected SKOV3 cells were seeded in 35-mm plates at a density of 2 x 105 cells/well. After incubation at 37 °C for 24 h, the plates were washed and changed to serum-free medium. Staurosporine was added to a final concentration of 1 µM for 5 h. DAPI was then added to each well at a final concentration of 5 µg/ml. After a 20-min incubation in the dark at 20 °C, cells were examined by fluorescence microscopy (Nikon Eclipse TE200; Nikon Corp., Tokyo, Japan) using excitation and emission filters of 380 and 430 nm. An individual blinded to the experimental conditions counted at least 300 cells in six different high power fields for each treatment. Each treatment was repeated at least three times, performed in triplicate each time. To inhibit apoptosis, the cells were pretreated with 40 µM N-(N-benzyl-oxycarbonylvalinylalanyl) aspartic acid (O-methyl ester) fluoromethyl ketone for 1 h before the addition of staurosporine. The significance of differences between experimental variables was determined using the Student's t test.
Proliferation AssaysSKOV3 parental cells and cells stably transfected with empty vector were plated at 100,000 cells/10-cm disk in triplicate in complete medium. After trypsinization, the total number of trypan blue-excluding cells was determined daily for 5 days.
Treatment with FGF-2, HB-EGF, and EGFTo assess the role of HSulf-1 in HB-GF-mediated signaling, vector-transfected and HSulf-1 clones 7 and 8 were serum-starved for 812 h, treated with diluent, 10 ng/ml FGF-2, 100 ng/ml HB-EGF (Sigma), or 10 ng/ml EGF for the times indicated in individual figures. Following treatment, cells were rinsed with ice-cold PBS, scraped from the dishes, and lysed at 4 °C in SDS sample buffer without bromphenol blue. Protein concentrations were determined with bicinchoninic acid (Pierce).
ImmunoblottingEqual amounts of protein (20 µg/lane) were separated by electrophoresis on an SDS gel containing a 412% acrylamide gradient and electrophoretically transferred to nitrocellulose. Blots were washed once with TBS, 0.2% Tween 20 (TBST) and blocked with TBST containing 5% non-fat dry milk for 1 h at 20 °C. The blocking solution was replaced with a fresh solution containing a 1:500 dilution of rabbit anti-phospho-ERK (Cell Signaling Inc., Beverly, MA). After overnight incubation at 4 °C, the blots were washed three times for 10 min each in TBS, 0.1% (w/v) Tween 20 and incubated with horseradish peroxidase-conjugated secondary antibody in 5% milk/TBST at 20 °C for 1 h. After washing 3 times in TBST, the proteins were visualized using enhanced chemiluminescence (Amersham Biosciences). The blots were stripped and reprobed with antisera that recognize total ERK, EGFR phosphorylated on Tyr1068 and/or Tyr992, total EGFR (all from Cell Signaling Inc., Beverly, MA), or mouse monoclonal anti-actin (Sigma).
Sulfatase AssayConfluent flasks of stable transfectants were washed in ice-cold PBS and lysed in SIE buffer (250 mM sucrose, 3 mM imidazole (pH 7.4), 1% ethanol) containing 1% (w/v) Nonidet P-40 and protease inhibitor mixture (Roche Applied Science). After cells were sheared by passage through a 20-gauge needle, protein concentration was determined using the Bradford assay. 100 µg of total cellular protein was preincubated with 10 µM estrone 3-O-sulfamate (Sigma) at 37 °C for 1 h to inhibit steroid sulfatases. 4-MUS was then added to a final concentration of 10 mM in the presence of 10 mM lead acetate in a total volume of 200 µl. After incubation for 24 h at 37 °C, the reaction was terminated by addition of 1 ml of 0.5 M Na2CO3/NaHCO3 (pH 10.7). The fluorescence of the liberated 4-methylumbelliferone was measured using excitation and emission wavelengths of 360 and 460 nm, respectively. To assess the effects of transient transfection, SKOV3 cell lysates prepared 48 h after transfection with empty vector, full-length HSulf-1 cDNA, or mutant N-Sulf were assayed as described above except that the incubation was shortened to 3.5 h.
HSulf-1 LocalizationSKOV3 cells seeded on glass coverslips were allowed to adhere overnight and then transfected with empty vector or cDNA encoding full-length HSulf-1 fused at its C terminus to GFP. 24 h after transfection, cells were fixed in 4% paraformaldehyde, permeabilized with 0.2% Triton X-100, and mounted with Vectorshield® mounting medium containing DAPI. The GFP fusion protein was visualized using a Zeiss LS510 laser scanning confocal microscope. Alternatively, SKOV3 cells were transfected with 4 µg of plasmid encoding FLAG-tagged HSulf-1, incubated for 24 h, washed with PBS, fixed for 10 min in PBS containing 3.7% formaldehyde and 1% sucrose, washed with 0.1 M glycine in PBS, permeabilized with PBS containing 0.4% Triton X-100 and 2% bovine serum albumin for 20 min, and washed three times in washing buffer (PBS containing 0.2% bovine serum albumin and 0.1% Triton X-100). After incubation for 1 h at 20 °C with anti-EGFR antibody, cells were washed four times with washing buffer, incubated with 1:200 TRITC-conjugated anti-rabbit IgG and 1:200 FITC-conjugated anti-FLAG monoclonal antibody (Sigma) in the dark, washed twice in washing buffer, stained with 0.5 µg/ml DAPI for 5 min, washed twice in PBS, and viewed with an Axiovert 35 epifluorescence microscope (Carl Zeiss, Thornwood, NY) equipped with a 100-watt mercury lamp or a Zeiss LSM510 confocal microscope.
HSulf-1 Distribution48 h after transfection of cDNA encoding GFP-tagged HSulf-1 into SKOV3 parental cells, cells and medium were collected separately. The cells were washed in ice-cold PBS, scraped, and lysed at 4 °C in SDS buffer without bromphenol blue. Protein concentrations were determined with bicinchoninic acid (Pierce). Conditioned medium was concentrated in a Centricon 10 microconcentrator (Millipore Corp). The cell lysate and 50x concentrated medium were resolved on 7.5% SDS-polyacrylamide gels under reducing conditions. Immunoblotting was performed as described above using anti-GFP antibody (Santa Cruz Biotechnology).
Sulfation State of Cell Surface HS-GAGsCells growing on coverslips for 24 h were fixed in methanol for 10 min at 20 °C, washed with PBS, and incubated for 1 h at 20 °C with 1:30 dilution of mouse 10E4 antibody, which recognizes an epitope that includes the N-sulfated glucosamine residue (Seikagaku America, Falmouth, MA). After washing, cells were stained with FITC-conjugated anti-mouse IgG and examined by laser scanning confocal microscopy as described above. As a control, cells were stained with antibody 3G10, which recognizes nonglycosylated glycosaminoglycans. In brief, cells grown on coverslips for 24 h were fixed in 4% paraformaldehyde at 37 °C for 20 min, washed, preincubated in buffer containing 50 mM sodium acetate (pH 7.0), 100 mM NaCl, and 3.3 mM CaCl2 at 37 °C for 1 h, and followed by incubation with 20 milliunits/ml of heparitinase I (Sigma) for 1.5 h at 37 °C. After thorough washing, cells were incubated with a 1:250 dilution of 3G10 monoclonal antibody (Seikagaku America) for 2 h at 37 °C followed by FITC-conjugated anti-mouse IgG and examined as described above.
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RESULTS |
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After HSulf-1 was assembled into a contig using Sequencher 3 software, a 5696-bp cDNA containing a single open reading frame encoding an 871-amino acid polypeptide was isolated (GenBankTM accession number AF545571
[GenBank]
). The predicted amino acid sequence is identical to that recently reported for HSulf-1 (8). Based on the computer algorithm Signal P version 1.1 at the Centre for Biological Sequence Analysis website (24), a 22-amino acid signal peptide (MKYSCCALVLAVLGTELLGSLCST) is found at the N terminus, with the most likely cleavage site indicated by
. The transmembrane prediction program TMPRED (25) predicts two additional membrane-spanning domains at amino acids 6988 and 754779. The cDNA contains five potential polyadenylation signals AATAAA at positions 4170, 4679, 4820, 4824, 5052, and 5678.
The HSulf-1 gene spans 211-kb genomic fragment on chromosome 8q13.3. Our analysis of the cDNA and gene agree with that reported by Morimoto-Tomita et al. (8) with one notable exception. Morimoto-Tomita et al. (8) reported the presence of a 280-bp noncoding exon in the 5'-UTR that they called exon 1 (8), and we will denote exon 1A. In addition to this sequence, we have identified two other noncoding exons, one 5' to this exon (314 bases, which we call exon 1) and another 3' to this sequence (165 bases, which we call exon 2). To determine which of these exons, 1, 1A, or 2, are present in transcribed message, primers in exons 1 and 5 were utilized to amplify a 950-bp 5'-UTR from normal ovarian epithelial cells, HMEC, and normal kidney. All of the cDNAs amplified lacked exon 1A. Instead, two different splice variants were amplified, a less abundant one lacking exon 1A but containing exons 1 and 2, and a more abundant one lacking both exon 1A and exon 2 (data not shown).
HSulf-1 Is Widely Expressed in Normal TissueNorthern blot analysis using full-length HSulf-1 cDNA as a probe (Fig. 1D) revealed a 6.0-kb and a smaller 5.0-kb transcript. Expression was observed in all nonlymphoid tissues but was highest in small intestine, pancreas, and colon. Importantly, the blot shown in Fig. 1D contains message from total ovary. Further analysis (Fig. 2, A and B) demonstrated that HSulf-1 message was readily detected in purified human ovarian surface epithelial cells. Testis appears to express tissue-specific splice variants that have not been characterized further.
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Decreased HSulf-1 Expression in Primary Ovarian CancersBecause KIAA1077 was initially identified as a down-regulated transcript in SSH libraries of ovarian cancer, we next evaluated HSulf-1 expression ovarian cancer cell lines and primary tumor specimens. Although semi-quantitative PCR (Fig. 2, A, C, and E, lane 1) and Northern blotting (Fig. 2B) readily detected HSulf-1 mRNA in all normal ovarian surface epithelial samples examined, the message was undetectable in 5 of 7 ovarian cancer cell lines (Fig. 2, A and B). Moreover, semi-quantitative RT-PCR with overlapping primers spanning the entire HSulf-1 open reading frame (illustrated in Fig. 2C and summarized in Table II) demonstrated that HSulf-1 down-regulation is common in primary ovarian cancer specimens. In particular, HSulf-1 mRNA was undetectable in 40% of samples and extremely weak in another 37%. Among the histological subtypes of ovarian cancer, clear cell cancers have a particularly poor prognosis (26) and uniformly lack detectable HSulf-1 expression (Fig. 2C and Table II).
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To begin to assess the mechanism by which HSulf-1 expression might be decreased in ovarian cancer, LOH analysis was performed. Genomic sequence analysis revealed microsatellite markers in the 5'-UTR, introns 1 and 2, and two within intron 3. The primers flanking these repeats are shown in Table I. Analysis in 30 primary ovarian tumor samples revealed that LOH of these markers ranged from 44 to 53% (Fig. 2D).
Decreased HSulf-1 Expression in Other Tumor TypesTo assess the possibility that loss of HSulf-1 expression might be unique to ovarian cancer cells (Fig. 2, AC), semi-quantitative RT-PCR was performed using cancer cell lines of breast, pancreas, kidney, and liver origin. For these studies, normal HMEC and normal kidney (Fig. 2E, lanes 1 and 16) served as positive controls. Results of this analysis revealed that the majority of cancer cell lines had either a complete loss or markedly diminished expression of HSulf-1 (Fig. 2E), raising the possibility that down-regulation of this transcript might be relatively widespread among epithelial malignancies. However, MCF10A cells derived from fibrocystic breast generally regarded as relatively normal (27) also had a complete loss of HSulf-1 expression, possibly implicating HSulf-1 loss as an early event in mammary carcinogenesis.
HSulf-1 Encodes an Active SulfataseTo begin to analyze the function of HSulf-1, full-length cDNA was stably transfected into two lines lacking detectable message, SKOV3 and OV207, and multiple clones were isolated. Analysis by RT-PCR demonstrated varying levels of message within the clones (Fig. 3A). Both sets of lines were utilized in the analyses presented below.
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To determine whether the stable transfectants exhibited sulfatase activity, cell lysates from clones displaying abundant HSulf-1 message were incubated with the fluorogenic substrate 4-MUS in the presence of estrone 3-O-sulfamate to specifically inhibit endogenous steroid sulfatase activity (Fig. 3, B and C). By using this nonspecific sulfatase substrate, an increase in activity comparable with that reported by Morimoto-Tomita et al. (8) was observed in HSulf-1-expressing clones compared with parental cells or clones transfected with empty vector. A comparable increase in sulfatase activity was also observed 48 h following transient transfection of full-length H-Sulf-1 cDNA into SKOV3 cells (data not shown).
HSulf-1 Is Localized to the Cell SurfaceThe avian ortholog of HSulf-1, QSulf1, was shown to localize to the cell surface (7). In contrast, Morimoto-Tomita et al. (8) reported that HSulf-1 is secreted to the medium after transfection into Chinese hamster ovary cells. To being to address this apparent inconsistency, cDNA encoding HSulf-1 fused to GFP was transiently transfected into SKOV3 cells. Blotting with anti-GFP antibody readily detected the fusion protein in whole cell lysates but not in medium that was concentrated 50-fold (Fig. 4A). This is similar to observations made previously with the HSulf-1 homologs QSulf-1 and RsulfFP1 (7, 28).
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Confocal microscopy of cells expressing the HSulf-1/GFP fusion protein demonstrated that HSulf-1 localized to the plasma membrane (Fig. 4B). Further analysis demonstrated co-localization with growth factor receptors such as EGFR at the cell surface (Fig. 4C).
HSulf-1 Expression Is Associated with Decreased HSPG SulfationTo assess the possibility that HSulf-1 affects HSPG sulfation, clones transfected with empty vector or HSulf-1 were stained with 10E4 antibody, which specifically recognizes sulfated glucosamine in HSPGs (29). Intense staining was observed in parental and vector transfected cells (Fig. 5A). In contrast, HSulf-1-expressing clones showed reduced staining. Staining with anti-stub antibody 3G10 revealed that both HSulf-1-negative and HSulf-1-transfected cells express HSPGs equally (Fig. 5B).
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To assess further the ability of HSulf-1 to modulate cell surface sulfation, OV202 cells, which endogenously express HSulf-1 (Fig. 2, A and B), were transiently transfected with HSulf-1 antisense cDNA. Cell surface staining for sulfated glucosamine in HSPGs was markedly increased (Fig. 5C). Collectively, these results provide preliminary evidence that HSulf-1 down-regulation increases HSPG sulfation and HSulf-1 re-expression decreases HSPG sulfation.
HSulf-1 Modulates Signaling by HB-EGF but Not EGFTo determine whether HSulf-1 modulates HB-GF signaling, we examined the action of HB-EGF in parental and HSulf-1-transfected ovarian cells. This growth factor was chosen because of its dependence on heparin binding for its action and because of its postulated role in ovarian carcinogenesis (30). Overexpression of HER2 and HER4, which mediate the effects of heparin-independent EGF and HB-EGF, respectively, is well documented in ovarian cancer cells (30, 31).
HB-EGF treatment of serum-starved parental and vector-transfected cells resulted in sustained phosphorylation of the EGFR on Tyr1068 (Fig. 6A, upper panels). Identical results were obtained with anti-Tyr992 antiserum (data not shown). Both Tyr1068 and Tyr992 have been implicated in EGFR-induced ERK pathway activation (32, 33). Consistent with the enhanced phosphorylation of these sites, ERK phosphorylation was demonstrated in these cells after HB-EGF treatment (Fig. 6A, lower panels). In contrast, HSulf-1-expressing clones demonstrated diminished EGFR phosphorylation and diminished ERK phosphorylation after HB-EGF treatment (Fig. 6A). These results suggest that HSulf-1 can modulate signaling by HB-EGF.
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To determine whether this modulation was specific for HB-EGF, the same cells were treated with heparin-independent EGF. As indicated in Fig. 6B, there was no difference in either EGF-stimulated EGFR phosphorylation at Tyr1068 or ERK phosphorylation in HSulf-1-expressing clones compared with parental and vector-transfected controls.
HSulf-1 Also Modulates FGF-2 SignalingPrevious studies (46, 3436) have shown that N-sulfation and 2-O-sulfation are critical for the interaction between HS-GAGs and FGF-2, whereas 6-O-sulfation is required for the interaction between HS-GAGs and FGFR1 in the formation of the FGF-2·HS-GAG·FGFR1 ternary complex. Conversely, it has been reported that cells containing GAG chains with reduced sulfation lose their proliferative response to FGF-2 (34, 35, 37). These observations, coupled with the demonstration of elevated FGF-2 and FGFR1 in ovarian cancer cells (38, 39), prompted us to examine the effect of HSulf-1 on FGF signaling.
As a read out for FGF signaling, we again measured mitogen-activated protein kinase pathway activation. Formation of the FGF-2·HS-GAG·FGFR1 ternary complex induces receptor dimerization, activation of the FGFR1 tyrosine kinase (36, 40), receptor autophosphorylation, and binding of the adaptor SNT/FRS, which then activates intracellular signaling pathways, including the ERK pathway (41).
When serum-starved vector-transfected cells were treated with FGF-2, sustained phosphorylation of ERK1 and ERK2 lasting >60 min in parental (not shown) and vector-transfected cells (Fig. 7A) was observed. In contrast, HSulf-1-expressing clones demonstrated lower basal levels of ERK phosphorylation and only transient elevation after FGF-2 treatment (Fig. 7A). Collectively, these results suggest that HSulf-1 not only down-regulates the basal activation of ERK pathway activation, but also inhibits a sustained activation of this pathway that may be required for cell survival and proliferation.
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Several controls pointed to sulfation of HSPGs as a critical factor in this HB-GF signaling modulation. First, replacement of FGF-2 with heparinated FGF (heparin-stabilized FGF) abrogated the ability of HSulf-1 to modulate FGF-initiated signaling (Fig. 7B). In addition, transient transfection of SKOV3 cells with the sulfatase domain N-Sulf also dampened FGF signaling, whereas mutation of two conserved cysteines at the active site of this domain abrogated the modulation (Fig. 7C). Collectively, the results in Figs. 6 and 7 demonstrate the ability of HSulf-1 to modulate signaling by two different HB-GFs and the dependence of this modulation on an intact sulfatase domain.
HSulf-1 Modulates Proliferation and ApoptosisPrevious studies have demonstrated that stimulation of the Mek/ERK pathway leads to enhanced proliferation and inhibition of apoptosis (reviewed in Refs. 21 and 22). Based on the ability of HSulf-1 to modulate signaling through this pathway, we predicted that HSulf-1 re-expression in HSulf-1-deficient cells would lead to inhibition of proliferation and enhancement of apoptosis.
To test the first of these predictions, parental or HSulf-1-transfected clones were plated at 100,000 cells/dish and counted at various times. As predicted HSulf-1-expressing clones proliferated more slowly than parental or empty vector-transfected clones (Fig. 8A).
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To examine the effects of HSulf-1 re-expression on apoptosis, stable transfectants were treated for 24 h with 5 µM cisplatin, an agent that is widely used to treat ovarian cancer (42), or diluent. Cells were then stained with DAPI under conditions where this agent preferentially enters apoptotic cells and examined for apoptotic morphological changes (nuclear fragmentation) by fluorescence microscopy (schematic, Fig. 8B). Results of this analysis indicated that cisplatin induced little apoptosis in parental or vector-transfected cells under these conditions. In contrast, cisplatin induced apoptosis in 2540% of HSulf-1-transfected cells (Fig. 8B). HSulf-1 re-expression likewise sensitized OV207 clones to cisplatin (Fig. 8C). To rule out the possibility that these results were unique to cisplatin, the same cell lines were treated for 5 h with 1 µM staurosporine, a broad spectrum kinase inhibitor (43) that is widely used as a proto-typic pro-apoptotic stimulus because it induces apoptosis in a wide variety of cells (44), or with UCN-01, a staurosporine analog currently in phase I clinical trials (45). Once again, HSulf-1-transfected clones were sensitized to the induction of apoptosis (Fig. 8D). Similar results were observed in the OV207 clones and in a second set of independently derived HSulf-1-expressing SKOV3 clones (data not shown). Further experiments revealed the typical biochemical hallmarks of apoptosis, including cytochrome c release from mitochondria and DNA fragmentation, when HSulf-1-transfected clones were drug-treated (data not shown). Two aspects of these results deserve particular emphasis. First, HSulf-1 by itself did not induce apoptosis but instead modulated the sensitivity of cells to other stimuli (Fig. 8, BD). Second, higher expression of HSulf-1 correlated with somewhat higher induction of apoptosis (Fig. 8, BD).
To confirm that this modulation of apoptosis reflected the sulfatase activity of HSulf-1, SKOV3 cells were transiently transfected with two truncation constructs and an active site mutant. Transfection with the C-terminal half of HSulf-1 (C-Sulf) had little effect on the ability of staurosporine and UNC-01 to induce apoptosis (Fig. 8E). In contrast, an N-terminal fragment containing the entire sulfatase domain (N-Sulf) enhanced the ability of staurosporine to induce apoptosis. Importantly, site-directed mutagenesis of the putative catalytic cysteines Cys87 and Cys88 in N-Sulf (Mut-N-Sulf) abolished the ability of HSulf-1 to modulate apoptosis (Fig. 8E), providing evidence that sulfatase activity is required for this modulation.
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DISCUSSION |
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While these studies were in progress, Morimoto-Tomita et al. (8) reported cloning of the HSulf-1 cDNA and gene. Our analysis has extended this previous report by demonstrating the presence of two previously unrecognized upstream exons (Table III), both of which appear to be included in transcripts from a variety of human cell lines and cells.
Further studies by Morimoto-Tomita et al. (8) indicated that HSulf-1 exhibits sulfatase activity with a preference for glucosamine 6-sulfate substrates. Interestingly, transfection of Myc-tagged HSulf-1 into Chinese hamster ovary cells resulted in secretion of the protein into the culture medium rather than retention in or on the cells (8). In our experiments, HSulf-1 fused to GFP or tagged with the FLAG epitope was transfected into ovarian cancer cell lines that express undetectable amounts of endogenous HSulf-1 message. These experiments not only confirmed the induction of sulfatase activity (Fig. 3) but demonstrated desulfation of cell surface HSPGs upon HSulf-1 re-expression (Fig. 5). As was the case with QSulf-1 (7), however, our localization studies suggested that a substantial fraction of HSulf-1 remains associated with the cell surface. In particular, HSulf-1/EGFP was detected by immunoblotting in whole cell lysates but not 50-fold concentrated conditioned medium (Fig. 4). Moreover, both HSulf-1/EGFP and FLAG-tabbed HSulf-1 were localized to the cell surface by confocal microscopy (Fig. 4). Why these results differ from those of Morimoto-Tomita et al. (8) is at present unclear but might reflect the transfection of different cell lines or the use of different epitope tags.
Previous SSH analysis of two early and late stage tumors subtracted against normal ovarian epithelial brushings identified HSulf-1 as an mRNA that was diminished in several ovarian cancers compared with the cell of origin of these neoplasms (9). We have extended these studies by showing that HSulf-1 mRNA is markedly diminished or absent from 5 of 7 ovarian cancer cell lines and 23 of 30 epithelial ovarian cancers (Fig. 2). Further analysis has demonstrated that the HSulf-1 locus is subject to allelic loss in 5060% of ovarian cancers (Fig. 2D). As indicated in Table II, the lack of detectable HSulf-1 expression was particularly common in clear cell ovarian cancers. This variant accounts for 10% of all epithelial ovarian cancers, but these tumors have a worse prognosis and are resistant to platinum-based chemotherapy (26, 46, 47). Interestingly, HSulf-1 expression was undetectable in the clear cell cancers even though all four of the tumors analyzed were early stage tumors. Equally important, analysis of a series of cancer cell lines demonstrated that HSulf-1 down-regulation is common in hepatocellular, renal, pancreatic, and breast carcinomas (Fig. 2E). This early and apparent widespread occurrence of HSulf-1 down-regulation raises the possibility that HSulf-1 down-regulation might be important in the carcinogenic process.
In order to examine the functional consequences of HSulf-1 down-regulation, we re-expressed HSulf-1 in two ovarian cancer cell lines lacking detectable message. Studies of Dhoot et al. (7) previously implicated QSulf-1 in the regulation of Wnt signaling and alluded to the possibility that QSulf-1 might also potentially regulate FGF signaling, which is controlled by 6-O-sulfation of N-acetylglucosamine in HSPGs (4). Based on the similarity of HSulf-1 to QSulf-1, we hypothesized that HSulf-1 down-regulation might modulate HB-GF signaling. Consistent with this possibility, we observed altered signaling by HB-EGF in cells after HSulf-1 re-expression (Fig. 6). In particular, we observed diminished HB-EGF-induced phosphorylation of at least two important sites on the EGFR, Tyr1068, a binding site for Grb2 (32), and Tyr992, a binding site for phospholipase C- (33). In previous studies (48), the interaction of HB-EGF with cell surface HSPGs was indirectly demonstrated by showing that sodium chlorate, which inhibits HS-GAG sulfation, and heparinase abrogate HB-EGF signaling. A subsequent report (49) indicated that 125I-HB-EGF binding is diminished in Chinese hamster ovary cells deficient in HSPG. The present studies extend these earlier results by demonstrating that HSulf-1 re-expression, which diminishes cell surface HS-GAG sulfation (Fig. 5), interferes with HB-EGF signaling through the EGFR (Fig. 6). Consistent with these results, we observed diminished HB-EGF-induced activation of the ERK pathway (Fig. 6A). Importantly, these results were not seen with EGF (Fig. 6B), which lacks an HSPG binding domain and is thought to signal independent of the HS-GAGs.
The effect of HSulf-1 re-expression was not limited to HB-EGF. A variety of previous studies has demonstrated that FGF-2 binds to its receptor and to HSPGs, which act as co-receptors and promote formation of a ternary complex that is essential for cell proliferation and angiogenesis (50, 51). As indicated in the Introduction, previous reports have also demonstrated that sulfation of specific sites on the HS-GAGs is critical for this interaction. This interaction of FGF-2 with FGFR and HS-GAGs leads to receptor dimerization, activation, and autophosphorylation followed by activation of downstream signaling pathways, including the mitogen-activated protein kinase pathway (4, 37). Our experiments demonstrated that HSulf-1 also modulated FGF-2 signaling. In particular, FGF-2 induced sustained ERK phosphorylation in cells lacking detectable HSulf-1 expression but only transient ERK phosphorylation at 15 min in the HSulf-1 transfected clones (Fig. 7A). These observations are consistent with a recent report that chlorate treatment, which inhibits GAG sulfation, results in cells that exhibit a transient early (15 min) phosphorylation of ERK in response to FGF-2 but no sustained ERK phosphorylation (37). Once again the modulation of signaling by HSulf-1 was not observed when cells were treated with heparinated FGF-2 (Fig. 7B), which would be expected to signal independent of HS-GAGs. In summary, our results indicate that HSulf-1 transfection abrogates the sustained activation of ERK1 and ERK2 required for cell survival and proliferation.
Because sustained ERK phosphorylation has been implicated in proliferation (52) as well as resistance to apoptosis (22, 53, 54), we next examined the effect of HSulf-1 re-expression on these processes. Results of this analysis demonstrated that HSulf-1 re-expression diminished proliferation of SKOV3 and OV207 clones (Fig. 8A and data not shown). Moreover, HSulf-1 re-expression enhanced the sensitivity of these cells to a number of pro-apoptotic stimuli, including cisplatin, which is widely used to treat ovarian cancer (55), and staurosporine, a broadly active kinase inhibitor that is widely employed as a stimulus of the mitochondrial apoptotic pathway (44, 56). These results are consistent with previous studies (57, 58) demonstrating ERK phosphorylation and ability of the Mek1/2 inhibitor PD98059 to modulate cisplatin sensitivity in ovarian cancer cells. Further analysis demonstrated that an N-terminal fragment containing an intact sulfatase domain is responsible for this HSulf-1-induced modulation of apoptosis (Fig. 8E). Because HSulf-1 modulates sensitivity of cells to induction of apoptosis by cisplatin, which is considered the single most active agent currently available for the treatment of ovarian cancer, future studies to evaluate the relationship between HSulf-1 expression and clinical response in ovarian cancer appear to be warranted.
Although there is ample evidence that differences in the sulfation state of HS-GAGs introduced by altering sulfotransferase activity can modulate growth factor signaling in vitro (35, 5962), there is little precedent for the idea that variations in sulfatase activity can alter survival signaling in human cancer. The functional results described above suggest that HSulf-1 is a cell surface enzyme that desulfates critical sulfated moieties in HS-GAG, thereby inhibiting the action of heparin-dependent growth factors at their receptors and diminishing their ability to activate the ERK pathway. Because expression of HSulf-1 is undetectable or markedly attenuated in >75% of ovarian cancers relative to normal ovarian surface epithelium, these observations appear to outline a novel mechanism by which proliferative and anti-apoptotic signaling by heparin-dependent growth factors can be augmented during the process of carcinogenesis.
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FOOTNOTES |
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** These senior authors contributed equally to this work.
To whom correspondence should be addressed: Division of Experimental Pathology, Mayo Foundation, 200 First St. SW, Rochester, MN 55905. Tel.: 507-266-2775; Fax: 507-266-5193; E-mail: shridv{at}exrch.mayo.edu.
1 The abbreviations used are: HSPGs, heparan sulfate proteoglycans; DAPI, 4',6-diamidino-2-phenylindole dihydrochloride; EGFR, epidermal growth factor receptor; ERK, extracellular signal-regulated kinase; EST, expressed sequence tag; FITC, fluorescein isothiocyanate; GFP, green fluorescent protein; HB-GFs, heparin-binding growth factors; 4-MUS, 4-methylumbelliferyl sulfate; PBS, phosphate-buffered saline; UTR, untranslated region; RT, reverse transcriptase; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; HMEC, human mammary epithelial cells; HS-GAG, heparan sulfate glycosaminoglycan; FGF, fibroblast growth factor; FGFR, FGF receptor; CDTA, 1,2-cyclohexylenedini-trilotetraacetic acid; TRITC, tetramethylrhodamine isothiocyanate; LOH, loss of heterozygosity.
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ACKNOWLEDGMENTS |
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