Abstract
The suppressor of cytokine signalling-1 (SOCS-1) gene is frequently silenced in human hepatocellular carcinoma by aberrant methylation. The aim of this study was to determine if SOCS-1 is inactivated in pancreatic ductal neoplasms, and to investigate if aberrant methylation of this gene affected the Janus kinase/signal transducers and activators of transcription (JAK/STAT) pathway. Aberrant methylation in the CpG island of the SOCS-1 gene was detected in six of 19 (31.6%) human pancreatic cancer cell lines using methylation-specific PCR, and was associated with a loss or reduction of gene expression in five of the six methylated cell lines. Thirteen of 60 pancreatic ductal adenocarcinomas (21.7%) and two of 34 intraductal papillary mucinous neoplasms (IPMNs) (5.9%) had methylated SOCS-1. In contrast, SOCS-1 methylation was not seen in pancreatic normal ductal epithelia (zero out of 15), in pancreatic intraepithelial neoplasia (PanINs) (zero out of 49) or in the IPMNs without infiltrating cancer (zero out of 20). 5-Aza-2′-deoxycytidine treatment of the SOCS-1-methylated pancreatic cancer cell lines led to restoration of SOCS-1 gene expression. Interleukin-6, which has been shown to act through the JAK/STAT pathway to increase cell growth, induced modest time and dose-dependent cell proliferation in a SOCS-1-methylated cell line (PL10, P=0.015) but not in two unmethylated cell lines. These results indicate that loss of SOCS-1 gene is associated with transcriptional silencing and may have growth-promoting effects, and that its methylation is a useful marker of pancreatic cancer.
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Main
Pancreatic ductal adenocarcinoma is a highly malignant neoplasm that still carries an extremely poor prognosis. Most patients are diagnosed at an advanced stage of disease, and the incidence and mortality rates for invasive pancreatic cancer are almost identical. The 5-year survival rate is 0–2% (Klöppel, 2000). Characterisation of the genetic and epigenetic changes involved in the pathogenesis of pancreatic cancer should help in the development of sensitive early detection strategies.
Suppressor of cytokine signalling-1 (SOCS-1) is a cytokine-inducible protein that functions to regulate negatively cytokine signal transduction pathways by directly interacting with Janus kinase (JAK) (Endo et al, 1997; Naka et al, 1997; Starr et al, 1997). The SH2 domain of SOCS-1 binds to a JH1 domain of JAK2 and inhibits the phosphorylation of JAK2, thus downregulating the JAK/ signal transducers and activators of transcription (STAT) pathway (Narazaki et al, 1998; Yasukawa et al, 1999). Several studies have shown that constitutive overexpression of SOCS-1 inhibits signalling in response to a range of cytokines, including interferon-γ (Brysha et al, 2001), tumour necrosis factor-α (Morita et al, 2000), interleukin-2 (IL-2) (Sporri et al, 2001), IL-4 and IL-6 (Starr et al, 1997).
Interleukin-6 has been implicated as a mediator of growth control in several human neoplasms including multiple myeloma (Hussein et al, 2002), prostatic cancer (Giri et al, 2001) and colonic cancer (Schneider et al, 2000) and elevation of serum IL-6 level have been reported in some cancers such as renal cell carcinoma (Blay et al, 1992), ovarian cancer (Plante et al, 1994), cholangiocarcinoma (Goydos et al, 1998) and pancreatic cancer (Barber et al, 1999). The binding of IL-6 to its receptor induces homodimerisation of gp130, which leads to cross-phosphorylation and activation of the associated JAK2. Signal transducers and activators of transcriptors 3 is then recruited to the cytoplasmic region of gp130 and phosphorylated by JAK2 (Kishimoto and Kikutani, 2001). Activated STAT3 forms homodimers, moves into the nucleus and activates transcription of various genes, including the antiapoptotic regulatory protein Bcl-xl and SOCS-1 (Kishimoto and Kikutani, 2001).
The human SOCS-1 gene on chromosome 16p13.3 is a single-exon gene encoding 211 amino acids (Endo et al, 1997; Naka et al, 1997; Starr et al, 1997). The gene lies within a large CpG island spanning 2.5 kb. Recently, frequent aberrant methylation of the CpG island of SOCS-1 gene in hepatocellular carcinoma (HCC) and in multiple myeloma, and it was also demonstrated that the aberrant methylation had growth suppression activity (Yoshikawa et al, 2001; Galm et al, 2002). These results implicate the JAK/STAT pathway as having growth-promoting properties and suggest that SOCS-1 may normally suppress growth (Bromberg et al, 1999; Rottapel et al, 2002).
DNA methylation is a major mechanism for the inactivation of tumour-suppressor genes in cancer (Jones and Baylin, 2002). We have previously reported that many benign and malignant pancreatic neoplasms harbour aberrant methylation at multiple genes including p16, preproenkephalin, TSLC1, and others (Fukushima et al, 1997; Ueki et al, 2000; Ueki et al, 2001; Jansen et al, 2002). In this study, we determined the prevalence and significance of SOCS-1 methylation in pancreatic neoplasms.
Materials and methods
Cell lines and lymphocytes
Human pancreatic cancer cell lines AsPC1, BxPC3, Capan1, Capan2, CFPAC1, Mia PaCa2 and Panc-1 were obtained from the American Type Culture Collection (Rockville, MD, USA) and Colo357 was purchased from the EACC (Salisbury, UK). Twelve pancreatic carcinoma cell lines (PL1, 3, 4–6, 8–14) were generously provided by Dr Elizabeth Jaffee (Johns Hopkins University). An immortal human pancreatic duct epithelial cell line, HPDE, was kindly provided by Dr Ming-Sound Tsao (University of Toronto, Ontario, Canada). All cell lines, except for HPDE, were cultured in RPMI 1640 medium (Life Technologies, Inc., Gaithersburg, MD, USA) supplemented with 10% fetal bovine serum and antibiotics (100 U/ml penicillin and 100 μg ml−1 streptomycin), and incubated at 37°C in a humidified atmosphere of 5% CO2 in air. HPDE cells were cultured in keratinocyte serum-free (KSF) medium supplemented by bovine pituitary extract and epidermal growth factor (Gibco-BRL, Grand Island, NY, USA). Lymphocyte DNA was collected from 11 healthy individuals after informed consent as part of an IRB-approved clinical trial that aims to investigate candidate markers of pancreatic cancer.
Surgically resected pancreatic ductal adenocarcinoma and intraductal papillary mucinous neoplasms
Sixty primary pancreatic adenocarcinomas and 34 intraductal papillary mucinous neoplasms (IPMNs) were obtained from resected surgical specimens at the Johns Hopkins Hospital. The patients with pancreatic ductal adenocarcinoma included 33 men and 27 women; mean age was 65.6 years (range, 38–85 years), and those with IPMN included 17 men and 17 women; mean age was 66.1 years (range, 36–83 years). The IPMNs were histologically divided into three adenomas, 12 borderline neoplasms, five non-invasive and 14 invasive adenocarcinomas according to the WHO classification. Frozen tissues or formalin-fixed paraffin-embedded tissues were microdissected manually by blade and needle to obtain greater than 40% neoplastic cellularity in these primary pancreatic neoplasms. Microdissected tissues were transferred to tube containing 50–100 μl of 1 × TK buffer (200 μg ml−1 proteinase K and 0.5% Tween-20), and incubated at 56°C overnight. The tubes were placed in a 100°C block for 10 min for inactivation of the proteinase K.
Microdissection of normal pancreatic duct epithelia and PanINs
PanINs was classified into four categories of PanIN-1A, -1B, -2 and -3 according to the standardised nomenclature and classification of pancreatic intraepithelial neoplasia (Hruban et al, 2001). Serial sections (8 μm) of formalin-fixed and paraffin-embedded tissue were stained with haematoxylin & eosin. Microdissection of normal pancreatic duct epithelium and PanINs including approximately total 200–1500 cells on three slides each was performed with a small blade and needle as previously described and subjected cells to DNA extraction (Fukushima et al, 2002). Forty-nine PanINs (eight PanIN-1A, 21 PanIN-1B, 10 PanIN-2 and 10 PanIN-3) were collected from 13 pancreata with ductal adenocarcinoma (mean age of the patients, 64.4 years; range, 50–79 years) and as were 15 samples of normal pancreatic ductal epithelia (mean age of the patients, 60.9 years; range, 36–79 years).
Methylation-specific PCR
Bisulphite modification of genomic DNA was performed as previously described (Fukushima et al, 2002). The bisulphite-treated DNA was amplified with either a methylation-specific or unmethylation-specific primer set at 40 cycles: 95°C for 20 s, 57°C for 30 s and 72°C for 30 s. A final extension step was included for 3 min at 72°C. The methylation-specific primer sequences in exon 1, which lies within the SOCS-1 CpG island, were 5′-TCGTTCGTACGTCGATTATC-3′ (sense) and 5′-AAAAAAATACCCACGAACTCG-3′ (antisense). The unmethylation-specific primer sequences were 5′-TATTTTGTTTGTATGTTGATTATTG-3′ (sense) and 5′-AAACTCAACACACAACCACTC-3′ (antisense). The unmethylated reaction was predicted to yield a product of 122 bp and the methylated reaction a product of 132 bp. PCR products were resolved in 3% agarose gels, stained with ethidium bromide and visualised under UV illumination. DNA extracted from normal pancreatic tissue treated in vitro by Sss1 methyltransferase (New England Biolabs, Beverly, MA, USA) was used as a positive control for methylated alleles.
Reverse-transcription–PCR
RNA from pancreatic cancer cell lines was isolated using Trizol Reagent (Life Technologies, Rockville, MD, USA). One microgram of each total RNA was reverse transcribed (RT) using the Superscript II kit (Life Technologies, Rockville, MD, USA). RT–PCR primers for exon 1 were 5′-GACGCCTGCGGATTCTAC-3′ (sense) and 5′-AGCGGCCGGCCTGAAAG-3′ (antisense). A 181 bp was amplified according to the following conditions; an initial denaturation at 95°C for 3 min, then 35 cycles of 95°C for 15 s, 65°C for 30 s and 72°C for 30 s, followed by a final extension step at 72°C for 3 min. PCR mixture contained 5% dimethyl sulphoxide. A glyceraldehyde-3-phosphate dehydrogenase (GAPDH) primer set was run in duplex PCR with the SOCS-1 primer to provide an internal control for RNA quantity and quality. PCR products were separated in 3% agarose gels.
5-aza-2′-deoxycytidine treatment
To confirm that transcriptional repression related to the methylation status of the SOCS-1 CpG island, SOCS-1-methylated cells (PL10 and PL12) were treated with the demethylating agent 5-aza-2′-deoxycytidine (5Aza-dC) at a final concentration of 1.0 μ M for 96 h. After treatment, total RNA was extracted from the cells again and compared the SOCS-1 gene expression to that of untreated cells.
Western blotting analysis
Western blotting analysis was performed using antibodies specific for phosphorylated JAK2 (anti-JAK2 pYpY1007/1008 rabbit polyclonal antibody, BioSource International, CA, USA) or phosphorylated STAT3 (anti-pStat3, B-7, mouse monoclonal antibody, Santa Cruz Biotechnology, CA, USA) to investigate the JAK2 and STAT3 phosphorylation status after IL-6 treatment (20 ng ml−1 recombinant human IL-6 , BD Biosciences, San Diego, CA, USA). After 96 h treatment of IL-6, culture cells (HPDE, Panc1, PL10 and PL12) were lysed in cell lysis buffer (50 μ M Tris-HCl, pH 8.0; 50 μ M ethylenediamine tetraacetic acid (EDTA); 150 μ M NaCl; 50 μl Triton X-100; 5 μl Protease Inhibitor Cocktail) and boiled for 4 min. After 50 μl of each sample was subjected to SDS–polyacrylamide gel electrophoresis, proteins were transferred to nitrocellulose membranes (Amersham Pharmacia Biotech UK Limited, England) and probed with each antibody. After 2 h treatment with the secondary antibody, specific binding was detected by the enhanced chemiluminescence system (SuperSignal®West Pico Luminol/Enhancer Solution and Stable Peroxide Solution, PIERCE, Rockford, IL, USA).
Examination of cell proliferation in response to exogenous IL-6
To investigate the effect of methylation of SOCS-1 gene and its silencing on the JAK/STAT pathway, cells were grown with or without adding human IL-6 and the cell proliferation was observed. SOCS-1-methylated (PL10 and PL12) or unmethylated (HPDE and Panc1) cells were seeded at equal densities (1 × 104 cells ml−1) in six-well plates. After 72 h, cells were incubated in the presence or absence of 20 ng ml−1 recombinant human IL-6 (BD Biosciences, San Diego, CA, USA) for 48, 72 or 96 h. To examine the dose-dependent effect on cell proliferation of IL-6, cells were incubated in the existence or absence of 4, 20 or 100 ng ml−1 IL-6 for 96 h in the same way. Cells were counted using a haemacytometer (Hausser Scientific, Horsham, PA, USA).
Statistical analysis
Statistical analysis was performed using the StatView 5.0 statistical software package (SAS Institute Inc., Cary, NC, USA). The unpaired t-test was used to determine statistical differences of cell proliferation in between IL-6 treated and untreated cells. A P-value of less than 0.05 was considered to indicate statistical significance.
Results
Methylation of SOCS-1 in pancreatic tissues
MSP analysis revealed aberrant methylation of SOCS-1 in six of 19 (31.6%) pancreatic cancer cell lines (Table 1). The cell lines harbouring methylated SOCS-1 were PL9, PL10, PL12, Capan1, Capan2 and MiaPaCa2. Complete or almost complete methylation was seen in the cell lines PL9, PL10 and PL12. An example of an MSP analysis is shown in Figure 1A.
Thirteen of 60 (21.7%) resected primary pancreatic ductal adenocarcinomas showed SOCS-1 CpG island methylation (Table 1). There was no significant difference in the age of patients with unmethylated SOCS-1 (65.8 years; range, 38–85 years) and methylated SOCS-1 (65.1 years; range, 46–83 years) in their primary pancreatic cancers. DNA from normal pancreatic ducts (n=16) and from 49 PanINs obtained from the resection specimens of patients with pancreatic adenocarcinoma did not show methylation of CpG island of SOCS-1 gene (Table 1). Lymphocyte DNA from healthy individuals also only contained unmethylated SOCS-1 DNA (n=11).
Aberrant methylation of the SOCS-1 CpG islands was detected in two (5.9%) of 34 IPMNs (Table 1). Both of them were IPMNs with associated invasive carcinoma. One of these two patients with methylated SOCS-1 in their cancer was a patient with Peutz-Jeghers syndrome.
Relation between aberrant methylation and gene expression of SOCS-1
SOCS-1 gene expression was silenced or markedly reduced in seven of 19 cell lines relative to GAPDH by RT–PCR (Figure 1B). Five of the six methylated SOCS-1 cell lines had markedly reduced or absent SOCS-1 gene expression. To investigate whether the suppression of SOCS-1 gene expression was mediated by methylation of CpG islands in human pancreatic cancer cells, we treated the pancreatic cancer cell lines PL10 and PL12 cells with 5-Aza-dC. Both cell lines showed loss of SOCS-1 gene expression and both harboured methylated SOCS-1 prior to treatment with 5-Aza-dC. 5-Aza-2′-deoxycytidine restored SOCS-1 gene expression (Figure 2). Despite 5-Aza-dC induction of SOCS-1 gene expression, 5-Aza-dC treatment did not lead to induction of JAK2 or pSTAT3, perhaps because of the relatively modest induction of SOCS-1 gene expression by 5-Aza-dC.
Effect of exogenously added IL-6 on proliferation of pancreatic cancer cells
Treatment of SOCS-1-methylated pancreatic cancer cells (PL10 and PL12) and the unmethylated cell line Panc-1 and a non-neoplastic pancreatic ductal epithelial cell line (HPDE) with IL-6 (20 ng ml−1) for 48, 72 or 96 h, led to modest but significant increases in PL10 cell growth over control in a time (data not shown) and in a dose-dependent fashion (Figure 3). After 96 h, IL-6 treatment of PL10 resulted in significant increases in cell number (120.5±21.9%, P=0.015) compared to untreated cells, whereas two other pancreatic cancer cell lines, Panc1 and PL12, and the non-neoplastic HPDE cells did not change their growth patterns in response to IL-6 (Panc1: 111±20.8% (P=0.146), PL12: 116±7.41% (P=0.109), HPDE: 98.7±16.4% (P=0.807)) (Figure 3A). Stimulation by IL-6 would be expected to lead to an induction of phosphorylated JAK2 and STAT3. Despite this prediction, Western blotting analysis revealed that phosphorylated JAK2 was only minimally induced after IL-6 treatment in PL12 but not in PL10 (Figure 4). Phosphorylated STAT3 was present in all cell lines and IL-6 treatment resulted in an increase in pSTAT3 in the SOCS-1-methylated cell lines, PL10 and PL12, but not in the unmethylated cell line Panc-1 (Figure 4). IL-6 treatment also increased pSTAT3 in the pancreatic epithelial non-neoplastic cell line, HPDE (Figure 4).
Discussion
In this study, we demonstrate that SOCS-1 is a frequent target for aberrant methylation in pancreatic cancer. We also demonstrate that silencing of SOCS-1 gene expression occurs in pancreatic cancer cell lines harbouring methylated SOCS-1 and such silencing could be restored after 5-Aza-dC treatment, indicating that methylation was the likely mechanism by which the SOCS-1 gene expression was suppressed. Furthermore, we demonstrated that IL-6 induced modest increases in cell proliferation only in pancreatic cancer cells (PL10) harbouring methylated SOCS-1 gene.
Since SOCS-1 suppresses the JAK/STAT pathway by inhibiting JAK2 activity (Kishimoto and Kikutani, 2001), and since STAT3 is downstream of JAK2 in the JAK/STAT pathway, SOCS-1 methylation status may affect the level of phosphorylation of STAT3. We observed a moderate induction of phosphorylated STAT3 in PL10 and PL12 after IL-6 treatment with little or no induction in an unmethylated cell line (Panc-1). This is consistent with our hypothesis that pSTAT3 induction by IL-6 would be more likely to occur if SOCS-1 is methylated than if it is unmethylated. We did not observe induction of pSTAT3 or JAK2 by 5-Aza-dC treatment despite induction of SOCS-1, but we suspect that the level of induction of SOCS-1 expression by 5-Aza-dC was insufficient to result in a change in pSTAT3. There was not a clear-cut relation between pSTAT3 levels and SOCS-1 expression and we suspect that this observation reflects the fact that STAT3 is regulated not only by JAK2 but also by other factors including the insulin-like growth factor-1 receptor (IGF-R) and Src (Yu et al, 1995).
Methylation of CpG island of SOCS-1 gene appears to occur late in the development of pancreatic ductal adenocarcinoma. PanINs are preinvasive intraductal lesions (Hruban et al, 2001), and PanINs harbour many of the same genetic and epigenetic abnormalities seen in invasive ductal adenocarcinomas such as mutations of the K-ras (Moskaluk et al, 1997), p16 (Moskaluk et al, 1997; Wilentz et al, 1998), SMAD4 (Wilentz et al, 2000), p53 and BRCA2 genes (Goggins et al, 2000), and aberrant methylation of the ppENK, p16 and TSLC1genes albeit at lower frequencies than those seen in invasive pancreatic cancers (Fukushima et al, 2002; Jansen et al, 2002). In contrast, in this study we found that PanINs lacked methylation of SOCS-1 suggesting that if loss of SOCS-1 is a selected event, it does not provide a selective advantage to a pancreatic neoplasm until the neoplasm has evolved into an invasive adenocarcinoma.
IPMN is clinicopathologically distinct neoplasm from ductal adenocarcinoma (Fukushima et al, 1997; Longnecker et al, 2000). Intraductal papillary mucinous neoplasms show duct ectasia with a papillary growth of neoplastic mucin producing epithelial cells. Patients with IPMNs generally have better prognosis than the patients with usual pancreatic ductal adenocarcinoma; however, some IPMNs evolve into invasive carcinoma and those patients have a poorer outcome. Intraductal papillary mucinous neoplasms have been shown to have similar methylation patterns to PanINs and usual pancreatic adenocarcinomas. For example, ppENK and p16 methylation occurs at a higher frequency in high-grade IPMNs (carcinomas) than it does in low-grade IPMNs (adenoma or borderline neoplasms) (Sato et al, 2002). In this study, we detected aberrant methylation of SOCS-1 gene in only two of 14 IPMNs that had an associated infiltrating carcinoma. None of the 20 benign or borderline IPMNs without an associated invasive carcinoma harboured SOCS-1 methylation. This suggests that, just as is true for usual ductal pancreatic adenocarcinoma, aberrant methylation of SOCS-1 gene may occur late in the development of IPMNs.
Suppressor of cytokine signalling-1 gene can be added to the increasing list of genes that are aberrantly methylated in pancreatic adenocarcinomas. This list includes ppENK, p16, hMLH1, RAR beta (Ueki et al, 2000, 2001), cyclin D2 (Matsubayashi et al, 2003) and TSLC1 (Jansen et al, 2002). In addition to understanding the biological significance of aberrant methylation in pancreatic adenocarcinoma, the detection of aberrantly methylated DNA in secondary fluids such as the pancreatic juice of patients with pancreatic disease may aid in the early diagnosis of pancreatic cancer (Fukushima et al, 2003). Since SOCS-1 methylation is only found in a subset of pancreatic adenocarcinomas, its utility as a diagnostic marker would only be as part of a panel of other aberrantly methylated genes that are specifically methylated in pancreatic cancer but not in normal pancreas.
In conclusion, SOCS-1 is commonly methylated in pancreatic adenocarcinoma and loss of SOCS-1 in pancreatic cancer is moderately associated with increased IL-6-mediated growth. Since SOCS-1 methylation becomes manifest only at the invasive carcinoma stage, detection of methylated SOCS-1 may aid in the early detection of invasive pancreatic adenocarcinoma.
Change history
16 November 2011
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Acknowledgements
This work was supported by the SPORE grant in Gastrointestinal Cancer (CA62924), and Grant CA91968 from the National Cancer Institute, and the Michael Rolfe Foundation.
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Fukushima, N., Sato, N., Sahin, F. et al. Aberrant methylation of suppressor of cytokine signalling-1 (SOCS-1) gene in pancreatic ductal neoplasms. Br J Cancer 89, 338–343 (2003). https://doi.org/10.1038/sj.bjc.6601039
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DOI: https://doi.org/10.1038/sj.bjc.6601039
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Digestive Diseases and Sciences (2022)
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Deciphering DNA methylation signatures of pancreatic cancer and pancreatitis
Clinical Epigenetics (2019)
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Expression of SOCS1 and the downstream targets of its putative tumor suppressor functions in prostate cancer
BMC Cancer (2017)
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SOCS1 inhibits migration and invasion of prostate cancer cells, attenuates tumor growth and modulates the tumor stroma
Prostate Cancer and Prostatic Diseases (2017)