E‑cadherin is downregulated by microenvironmental changes in pancreatic cancer and induces EMT
- Authors:
- Published online on: June 27, 2018 https://doi.org/10.3892/or.2018.6528
- Pages: 1641-1649
Abstract
Introduction
The pathogenesis of pancreatic cancer is opaque, its progress is rapid, its prognosis and therapeutic effects are poor, its incidence is almost equal to its mortality rate, and the vast majority of patients die due to metastases. Pancreatic cancer still has the fourth highest death rate worldwide (1,2). The early metastasis of pancreatic cancer is an extremely complex, dynamic process with multi-factor participation and multi-stage development. The exact molecular mechanism responsible is still not clear. Many studies have shown that many factors, including epithelial-mesenchymal transition (EMT) (3,4), the tumor microenvironment (5,6), inflammatory factors (7,8), stress response (9), and circulating tumor cells (CTCs) (10) play vital roles in the process of pancreatic cancer metastasis.
EMT is the ‘engine’ that leads to the invasion and metastasis of pancreatic cancer (11). The process is accompanied by changes in the expression of multiple genes. The most significant changes are in the epithelial marker E-cadherin and mesenchymal marker vimentin. Microenvironmental changes in pancreatic cancer are the primary causes of EMT. In the present study, we induced changes in the microenvironment of pancreatic cancer cells in vitro, such as making it anaerobic, making it serum-deficient, and adding TGF-β, and then observed the changes of the protein and mRNA expression levels of EMT markers E-cadherin and vimentin. Furthermore, we conducted a survival analysis and Cox regression analysis to investigate the correlation between the expression level of E-cadherin and overall survival.
Materials and methods
Cell lines
Eight human pancreatic cancer cell lines, AsPC-1, BxPC-3, Capan-1, Colo-357, MIA PaCa-2, Panc-1, SU86.86 and T3M4, were kindly donated by Professor Helmut Freiss from the Technical University Munich of Germany. All the cell lines were individually cultured in a humidified incubator with 5% CO2 at 37°C in either RPMI-1640 medium or Dulbecco's modified Eagle's medium (DMEM) containing 10% fetal bovine serum (FBS; Thermo Fisher Scientific Inc., Waltham, MA, USA).
Clinical samples
All 52 pancreatic tissues (Table I), including 25 male cases and 27 female cases, age distribution from 41.4 to 81.1 years (65.59±1.21 years), were obtained from the Department of General Surgery, Peking Union Medical College Hospital (PUMCH), China. The date range of recruitment was from January 2012 to December 2017. The experimental protocol was approved by the Peking Union Medical College Hospital Ethics Committee. Written informed consent was obtained from the patients. Tissue sampling and processing were performed as previously described (12).
Table I.Association between E-cadherin expression and clinicopathological features in PDAC patients. |
RNA extraction and quantitative real-time PCR (qPCR)
Total RNA was extracted from cells and tissues using Invitrogen™ TRIzol reagent (Thermo Fisher Scientific, Inc. Waltham, MA, USA), according to the manufacturer's instructions. cDNA was synthesized using Invitrogen™ M-MLV reverse transcriptase (Thermo Fisher Scientific, Inc.) from 5 µg total RNA. Quantitative RT-PCR was performed on the Bio-Rad CFX96 Real-Time PCR System (Bio-Rad Laboratories, Foster City, CA, USA) using KAPA PROBE FAST qPCR kits (Kapa Biosystems, Inc., Wilmington, MA, USA) and TaqMan probes (Thermo Fisher Scientific, Inc.) with the following cycling conditions: 95°C for 10 min (initial denature) and then 40 cycles of 95°C for 15 sec, 60°C for 60 sec. The expression of genes was calculated using the 2−ΔΔCq method (13). The sequences of E-cadherin primers used were as follows: 5′-CTGAGAACGAGGCTAACG-3′ and 5′-TTCACATCCAGCACATCC-3′; the sequences of vimentin primers used were as follows: 5′-CCAGGCAAAGCAGGAGTC-3′ and 5′-CGAAGGTGACGAGCCATT-3′. Reference gene was GAPDH, the sequences of GAPDH primers used were as follows: 5′-TCAACGACCACTTTGTCAAGCTCA-3′ and 5′-TCATTCTGGGGACCTGGTGGTCG-3′.
Immunoblot analysis
For immunoblot analysis, cells were grown in 6-well plates and processed as previously described (1). The primary antibodies were applied overnight at 4°C, and the secondary antibodies were added and incubated for 1 h at room temperature. The E-cadherin antibody (cat. no. sc-21791), HIF-1α antibody (cat. no. sc-71247) and vimentin antibody (cat. no. sc-66002) (all from Santa Cruz Biotechnology, Inc., Dallas, TX, USA) were diluted at 1:1,000. The GAPDH antibody was diluted at 1:5,000 and used to verify equal loading.
Serum starvation, hypoxia and TGF-β induction
For serum starvation, Colo-357 and BxPC-3 cells were seeded in 6-well plates; after the cells reached 70% confluency, the medium was changed to either 0.5 or 10% FCS containing medium that was kept on the cells for the indicated periods of time. For hypoxia, sister clones of Colo-357 cells were incubated under normoxic and hypoxic conditions (89.25% N2 + 10% CO2 + 0.75% O2) for 24 and 48 h at 37°C in medium supplemented with 10% FCS, as previously described (13,19,21). For TGF-β induction, sister clones of Colo-357 and BxPC-3 cells were incubated with TGF-β (ab50036, terminal concentration 10 ng/ml; Abcam, Cambridge, UK) or not. All experiments were performed in triplicate and repeated three times.
Immunohistochemical analysis
Semi-quantitative immunohistochemistry (IHC) was performed to determine E-cadherin expression in 10 normal pancreas and 52 pancreatic cancer samples according to a previously published standard protocol (2). The E-cadherin antibody was diluted at 1:200. Two pathologists who specialized in pancreatic cancer independently rated the staining intensity and percentage of stained cells for each sample. Briefly, scores were applied to rate staining intensity in the cancer cells (no staining, 0; weak, 1; moderate, 2; strong, 3) and to determine the percentage of stained cells (<5%, 0; 5–25%, 1; >25–50%, 2; >50–75%, 3; >75%, 4). The final intensity score was equal to the staining intensity multiplied by the cell percentage. The staining was stratified accordingly to low levels of expression (scores 1–3) or high levels of expression (score ≥4).
Statistical analysis
Statistical analyses were performed using SPSS 23.0 software (IBM Corp., Armonk, NY, USA). Median values were used as cut-off limits for group comparisons. Survival analyses were performed using the Kaplan-Meier method and log-rank tests. Multivariable analysis was performed using a Cox proportional hazards model. The median survival and estimations of hazard ratios were reported with 95% confidence intervals. Comparisons of demographic and clinicopathological data between groups were made using a Chi-square test. The data are presented as the mean ± standard deviation (SD) and were compared using either Student's t test, the Mann-Whitney U test and the one-way analysis of variance (ANOVA) followed by Fisher's Least Significant Difference post hoc test. Statistical significance was set at a P-value of <0.05. Graph-Pad Prism 5 (GraphPad Software, Inc., San Diego, CA, USA) software was used to create graphs.
Results
E-cadherin protein and mRNA are expressed in several of 8 pancreatic cancer cell lines, and the expression was decreased by hypoxia, inversely to vimentin
We first detected the expression of E-cadherin in 8 pancreatic cancer cell lines with western blotting and real-time PCR. The results showed that E-cadherin mRNA and protein were distinctly detectable in some of these cell lines, with high expression in T3M4, BxPC-3 and Colo-357 cells and low expression in MIA PaCa-2, Panc-1 and SU86.86 cells (Fig. 1A and B). In order to further research this topic using siRNA and overexpression plasmid, the cell lines with relatively high expression, BxPC-3 and Colo-357 were chosen for further functional experiments.
To analyze whether hypoxia decreases the expression of E-cadherin, cancer cells were exposed to a hypoxic environment. Cellular hypoxia was verified by increased HIF-1α protein expression. When compared with the normoxic controls, E-cadherin protein in Colo-357 cells was decreased 1.7- and 2.6-fold (P<0.01) due to hypoxia at 24 and 48 h, respectively (Fig. 1C), and in BxPC-3 cells, E-cadherin protein was decreased 1.2- and 2.1-fold (P<0.01) due to hypoxia at 24 and 48 h, respectively (Fig. 1F). Similarly, in Colo-357 cells, there were 4.7 and 7.8-fold (P<0.01) decreases at the mRNA level due to hypoxia at 24 and 48 h, respectively (Fig. 1D), and in BxPC-3 cells, there were 1.2- and 4.6-fold (P<0.01) decreases at the mRNA level of E-cadherin due to hypoxia at 24 and 48 h, respectively (Fig. 1G). In contrast, in Colo357 cells, vimentin protein was increased 1.9- and 3.1-fold (P<0.01) due to hypoxia at 24 and 48 h, respectively (Fig. 1C), and in BxPC-3 cells, vimentin protein was increased 1.8- and 1.9-fold (P<0.05) due to hypoxia at 24 and 48 h, respectively (Fig. 1F). Similarly, there were 1.3- and 2.1-fold (P<0.01) increases at the vimentin mRNA level due to hypoxia at 24 and 48 h, respectively (Fig. 1E), and in BxPC-3 cells, the vimentin mRNA level was increased 1.7- and 1.9-fold (P<0.05) due to hypoxia at 24 and 48 h, respectively (Fig. 1H).
Under serum starvation, E-cadherin protein and mRNA expression were significantly decreased, while vimentin was increased
In the next experiment, we tested the effect of serum starvation on E-cadherin and vimentin protein and mRNA expression in pancreatic cancer cells. For serum starvation, Colo-357 and BxPC-3 cells were cultured with 0.5% FCS; this was the second model of pancreatic cell microenviroment change. Due to serum starvation, in Colo-357 cells, E-cadherin protein was decreased 1.5-fold (P<0.05) and 4.3-fold (P<0.01) at 24 and 48 h, respectively (Fig. 2A), and in BxPC-3 cells, E-cadherin protein was decreased 1.6-fold (P<0.05) and 2.1-fold (P<0.01) at 24 and 48 h, respectively (Fig. 2E). Meanwhile, in Colo-357 cells, E-cadherin mRNA was decreased 1.4-fold (P<0.01) and 5.9-fold (P<0.01) at 24 and 48 h, respectively (Fig. 2B), and in BxPC-3 cells, E-cadherin mRNA was decreased 2.2-fold (P<0.01) and 6.8-fold (P<0.01) at 24 and 48 h, respectively (Fig. 2F). Conversely, in Colo-357 cells, vimentin protein was increased 2.4-fold (P<0.05) and 2.8-fold (P<0.05) at 24 and 48 h, respectively (Fig. 2C), and in BxPC-3 cells, vimentin protein was increased 1.2- and 1.7-fold (P<0.05) at 24 and 48 h, respectively (Fig. 2E). In accordance, in Colo-357 cells, vimentin mRNA was increased 1.4-fold (P<0.05) and 1.6-fold (P<0.05) at 24 and 48 h, respectively (Fig. 2D), and in BxPC-3 cells, vimentin mRNA was increased 1.3- and 3.9-fold (P<0.01) at 24 and 48 h, respectively (Fig. 2G).
Following exposure to TGF-β induction, E-cadherin protein and mRNA expression are obviously upregulated, while vimentin is downregulated
Subsequently, we detected the effect of TGF-β induction on E-cadherin and vimentin protein and mRNA expression in pancreatic cancer cells. This was the third model of pancreatic cancer cell microenviroment, and TGF-β was used as an inducer of EMT. Due to TGF-β induction, in Colo-357 cells, E-cadherin protein was decreased 2.1-fold (P<0.05) and 3.2-fold (P<0.01) at 24 and 48 h, respectively (Fig. 3A), and in BxPC-3 cells, E-cadherin protein was decreased 1.6-fold (P<0.05) and 1.7-fold (P<0.05) at 24 and 48 h, respectively (Fig. 3C). In Colo-357 cells, E-cadherin mRNA was decreased 1.7-fold (P<0.05) and 2.8-fold (P<0.01) at 24 and 48 h, respectively (Fig. 3B), and in BxPC-3 cells, E-cadherin mRNA was decreased 2.9-fold (P<0.01) and 3.8-fold (P<0.01) at 24 and 48 h, respectively (Fig. 3D). On the contrary, in Colo-357 cells, vimentin protein was increased 1.8-fold (P<0.05) and 1.7-fold (P<0.05) at 24 and 48 h, respectively (Fig. 3E), and in BxpPC-3 cells, vimentin protein was increased 1.2- and 1.5-fold (P<0.05) at 24 and 48 h, respectively (Fig. 3G). Similarly, in Colo-357 cells, vimentin mRNA was increased 1.5-fold (P<0.05) and 1.6-fold (P<0.05), respectively (Fig. 3F), and in BxPC-3 cells, vimentin mRNA was increased 1.4-fold (P<0.05) and 2.3-fold (P<0.05), respectively (Fig. 3H).
Location and varying expression intensity of E-cadherin in pancreatic cancer tissues
In order to investigate the expression of E-cadherin in pancreatic tissues, immunohistochemistry was performed in consecutive sections of 52 pancreatic ductal adenocarcinoma (PDAC) tissues. E-cadherin immunoreactivity showed varying intensity in different pancreatic cancer tissues, and was clearly found in cell membrane staining. For E-cadherin, some cancer cells had weak and moderate expression in 30 cases (57.7%, Fig. 4A and B), while some cancer cells were strongly positive in 22 cases (42.3%, Fig. 4C). In pancreatic PanIN lesions, E-cadherin was strongly expressed (Fig. 4D). In addition, E-cadherin was also strongly expressed in pancreatic islet cells (Fig. 4E), whereas there was no E-cadherin staining in pancreatic nerves (Fig. 4F).
Correlation of E-cadherin expression in pancreatic cancer with patient survival
Based on differential E-cadherin expression levels in PDAC tissues, we further divided the PDAC patients into E-cadherin-weak and E-cadherin-strong expression groups. The demographics and the association between E-cadherin expression and clinicopathological features are displayed in Table I. The correlation analysis results indicated that the expression level of E-cadherin was not related to patient sex, age, tumor-node-metastasis (TNM) staging or histological grade. Consistently, patients with higher levels of E-cadherin expression [n=22, median survival=22.9 (18.9–26.8) months] had significantly longer survival times compared to those with lower E-cadherin expression [n=30, median survival=14.1 (9.1–19.1) months, P<0.01] (Fig. 5A). The prognostic value of E-cadherin expression was assessed by multivariable analysis using a Cox proportional hazards model (Table II). Based on the factors analyzed, the results revealed that the expression of E-cadherin [HR=6.810, 95% confidence interval (CI), 0.149–0.763, P<0.01] and the occurrence of lymph node metastasis [hazard ratio (HR)=9.445, 95% CI, 0.077–0.567, P<0.01] were independent prognostic factors (Fig. 5C). The other related prognostic factors (age, T-status, grade), did not appear to impact the prognosis independently (Table II and Fig. 5B, D and E).
Discussion
It is well known that a hypoxic environment is a common feature of several solid tumors. While normal tissues generally receive an oxygen (O2) pressure of 30–50 mmHg, the pressure drops to below 2.5 mmHg in up to 50–60% of locally advanced solid tumors (14). When O2 levels were measured in patients with various solid tumors using pO2 histography, pancreatic cancer was found to be the most hypoxic, and intraoperative pO2 measurements of seven resectable pancreatic tumors further showed the hypoxic microenvironment (15,16). Several mechanisms contribute to the hypoxic milieu of PDAC. The major mechanism underlying reduced tumor oxygenation is the insufficient and aberrant vasculature that cannot deliver the necessary blood supply to all parts of the tumor tissue. In addition, stromal cells in PDAC may contribute to this hypoxia both by amplifying the production of antiangiogenic substances or by physically compressing the capillaries through extracellular matrix deposition in the periacinar spaces. Importantly, hypoxia is an important activator of pancreatic stellate cells (PSCs), the major fibroblastic cells of the pancreas, which perpetuate the vicious cycle of hypoxia and fibrosis (17,18). It is likely that the already fibrotic and hypovascular microenvironment of pancreatic cancer is one of the reasons for the failure of antiangiogenic therapies in pancreatic cancer in the clinical setting. Overall, reduced microvessel density, nutrient deprivation and extracellular matrix deposition create a hypoxic setting for pancreatic cancer cells.
Hypoxia induces EMT and plays a major role in the metastatic phenotype of PDAC cells (19–22). In EMT, cancer cells acquire mesenchymal features, such as dissolution of adhesion to the extracellular matrix and loss of cell polarity, which result in their transition into invasive cells. Moreover, EMT promotes the survival of cancer cells in the blood and metastatic sites by endowing them with stem-cell-like features and inhibiting their apoptosis. Furthermore, cells that have already undergone EMT migrate at the forefront of the invading cancer, creating tracks that other cancer cells can exploit. EMT is one important molecular mechanism underlying early invasion and metastasis in PDAC (23,24).
E-cadherin is a classic cadherin (calcium-dependent adhesion molecule) family member, with key roles in cell growth and differentiation, apoptosis and morphological changes in normal tissues and cells. E-cadherin protein promotes the formation of stable intercellular connections between adjacent cells, promotes epithelial cell adhesion, and maintains the integrity of tissue structure and function (25–27). In addition, E-cadherin can inhibit tumor cell secretion of matrix metalloproteinases (MMPs). Therefore, the loss of E-cadherin protein expression decreases the mutual adhesion force between tumor cells, which can then break through the extracellular matrix and basement membrane, detach from the primary tumor and invade and metastasize (28,29). As a very sensitive EMT marker, the expression of E-cadherin is often related to the infiltration and undifferentiated phenotype of tumor cells, and it is closely related to invasion and metastasis of early tumor cells (30,31).
Throughout cancer development, the expression of the mesenchymal marker vimentin is increased. Cancer cells often have altered cell surface molecules, and vimentin is an important molecular marker of mesenchymal cells. Although mature epithelial cells show no vimentin expression, during epithelial cell migration, vimentin can be re-expressed (32). Our experimental results showed that the expression of E-cadherin was decreased gradually over time with microenvironmental changes (including lack of serum and anaerobic environment), suggesting that microenvironmental changes can downregulate E-cadherin to inhibit the epithelial phenotype of pancreatic cancer cells. Decreases in E-cadherin induced by changes to the tumor microenvironment may be involved in the invasion and metastasis of pancreatic cancer cells. In contrast, alterations in the microenvironment can significantly promote the expression of vimentin in pancreatic cancer cells, further demonstrating that changes in the microenvironment of pancreatic cancer cells lead to EMT. In addition, HIF-1α was used as a marker for the successful creation of an anaerobic environment, and its protein expression was upregulated, suggesting that the anaerobic state was achieved in the microenvironment surrounding the pancreatic cancer cells.
Transforming growth factor-β (TGF-β) is a multifunctional cytokine that participates in the autocrine and paracrine regulation of a variety of biological functions in cells, including the inhibition of epithelial cell, immune cell and hematopoietic cell proliferation, the promotion of angiogenesis, and the induction of fibroblast differentiation from normal epithelial cells, a process of transformation that is closely related to E-cadherin expression (33,34). Our study applied TGF-β as an EMT-inducing factor. The results showed that TGF-β addition induced changes to the levels of E-cadherin and vimentin mRNA in pancreatic cancer cells that were consistent with those that occurred under serum starvation and in a hypoxic environment, which further confirmed the interactions of TGF-β, E-cadherin and vimentin in EMT in pancreatic cancer cells.
Based on the results of immunohistochemistry, E-cadherin expression levels were significantly reduced in most pancreatic cancer samples. In our study, we analyzed 30 pancreatic cancer tissues from 50 patients with lower E-cadherin expression (58%), and the Kaplan-Meier and log-rank analyses showed that the expression level of E-cadherin and the survival time of patients with pancreatic cancer were positively correlated. It is worth noting that precancerous lesions such as PanINs and tubular complexes have abundant E-cadherin expression. This result also indirectly shows that the changes in expression of E-cadherin, which occur throughout the transformation of benign pancreatic diseases to pancreatic cancer, occur simultaneously with EMT. Therefore, research into the mechanism of this occurrence and the development of pancreatic cancer is important.
Results from the multivariable analysis of the Cox proportional hazards model showed that the expression of E-cadherin and the occurrence of lymph node metastasis both were independent prognostic factors of pancreatic cancer. G staging showed a trend towards correlation with patient overall survival, but there was no statistical significance, and an increased sample size would be needed to confirm these findings. In summary, the characteristics of the pancreatic cancer microenvironment can induce pancreatic cancer cell EMT, furthering the cell invasion and metastasis capacities.
Further research efforts should focus on how to effectively address the microenvironmental conditions (i.e., the lack of serum and occurrence of a hypoxic environment) of pancreatic cancer cells to inhibit their malignancy. It is well known; the tumor cell microenvironment is essential for the generation of EMT in pancreatic cancer. The pancreatic cancer cells, extracellular matrix cells and related cytokines are the most important components of the pancreatic cancer microenvironment (24). In order to investigate the relationship in vivo between the microenvironment and EMT, we can conduct primary cultures of pancreatic cancer cells in vitro from the surgical resection of pancreatic cancer tissues. We can also extract the extracellular matrix cells (the activated stellate cells) in vitro, and then combine pancreatic cancer cells and stellate cells and transplantate into the pancreas of mice. By successfully establishing a patient-derived xenograft model (PDX), we can continually develop a series of studies concerning the microenvironment and EMT in vivo.
Acknowledgements
The authors thank Professor Yu Jia and Professor Ma Yanni for their technical support.
Funding
The present study was supported by grants from the 2016 PUMCH Science Found for Junior Faculty (no. pumch-2016-2.6) and the National Natural Science Foundation of China (no. 81773215).
Availability of data and materials
The datasets used during the present study are available from the corresponding author upon reasonable request.
Authors' contributions
YZ conceived and designed the study. WW, LD, BZ and JL performed the experiments. WW and LD wrote the paper. WW and LD reviewed and edited the manuscript. All authors have read and approved the final manuscript and agree to be accountable for all aspects of the research in ensuring that the accuracy or integrity of any part of the work are appropriately investigated and resolved.
Ethics approval and consent to participate
All experimental protocols were approved by the Peking Union Medical College Hospital Ethics Committee (Beijing, China).
Patient consent for publication
Not applicable.
Competing interests
The authors state that they have no competing interests.
References
Kamisawa T, Wood LD, Itoi T and Takaori K: Pancreatic cancer. Lancet. 388:73–85. 2016. View Article : Google Scholar : PubMed/NCBI | |
Siegel RL, Miller KD and Jemal A: Cancer statistics, 2016. CA Cancer J Clin. 66:7–30. 2016. View Article : Google Scholar : PubMed/NCBI | |
Rhim AD, Mirek ET, Aiello NM, Maitra A, Bailey JM, McAllister F, Reichert M, Beatty GL, Rustgi AK, Vonderheide RHM, et al: EMT and dissemination precede pancreatic tumor formation. Cell. 148:349–361. 2012. View Article : Google Scholar : PubMed/NCBI | |
De Craene B and Berx G: Regulatory networks defining EMT during cancer initiation and progression. Nat Rev Cancer. 13:97–110. 2013. View Article : Google Scholar : PubMed/NCBI | |
Apte MV, Wilson JS, Lugea A and Pandol SJ: A starring role for stellate cells in the pancreatic cancer microenvironment. Gastroenterology. 144:1210–1219. 2013. View Article : Google Scholar : PubMed/NCBI | |
Feig C, Gopinathan A, Neesse A, Chan DS, Cook N and Tuveson DA: The pancreas cancer microenvironment. Clin Cancer Res. 18:4266–4276. 2012. View Article : Google Scholar : PubMed/NCBI | |
Mantovani A: Cancer: Inflaming metastasis. Nature. 457:36–37. 2009. View Article : Google Scholar : PubMed/NCBI | |
Wen F, Shen A, Choi A, Gerner EW and Shi J: Extracellular DNA in pancreatic cancer promotes cell invasion and metastasis. Cancer Res. 73:4256–4266. 2013. View Article : Google Scholar : PubMed/NCBI | |
Cano CE and Iovanna JL: Stress proteins and pancreatic cancer metastasis. Scientific World Journal. 10:1958–1966. 2010. View Article : Google Scholar : PubMed/NCBI | |
Cen P, Ni X, Yang J, Graham DY and Li M: Circulating tumor cells in the diagnosis and management of pancreatic cancer. Biochim Biophys Acta. 1826:350–356. 2012.PubMed/NCBI | |
Franco-Chuaire ML, Magda Carolina SC and Chuaire-Noack L: Epithelial-mesenchymal transition (EMT): Principles and clinical impact in cancer therapy. Invest Clin. 54:86–205. 2013. | |
Jiang X, Rieder S, Giese NA, Friess H, Michalski CW and Kleeff J: Reduced alpha-dystroglycan expression correlates with shortened patient survival in pancreatic cancer. J Surg Res. 171:120–126. 2011. View Article : Google Scholar : PubMed/NCBI | |
Livak KJ and Schmittgen TD: Analysis of relative gene expression data using real-time quantitative PCR and the 2−ΔΔCT method. Methods. 25:402–408. 2001. View Article : Google Scholar : PubMed/NCBI | |
Vaupel P and Mayer A: Hypoxia in cancer: Significance and impact on clinical outcome. Cancer Metastasis Rev. 26:225–239. 2007. View Article : Google Scholar : PubMed/NCBI | |
Koong AC, Mehta VK, Le QT, Fisher GA, Terris DJ, Brown JM, Bastidas AJ and Vierra M: Pancreatic tumors show high levels of hypoxia. Int J Radiat Oncol Biol Phys. 48:919–922. 2002. View Article : Google Scholar | |
Dhani NC, Serra S, Pintilie M, Schwock J, Xu J, Gallinger S, Hill RP and Hedley DW: Analysis of the intra- and intertumoral heterogeneity of hypoxia in pancreatic cancer patients receiving the nitroimidazole tracer pimonidazole. Br J Cancer. 113:864–871. 2015. View Article : Google Scholar : PubMed/NCBI | |
Erkan M, Reiser-Erkan C, Michalski CW, Deucker S, Sauliunaite D, Streit S, Esposito I, Friess H and Kleeff J: Cancer-stellate cell interactions perpetuate the hypoxia-fibrosis cycle in pancreatic ductal adenocarcinoma. Neoplasia. 11:497–508. 2009. View Article : Google Scholar : PubMed/NCBI | |
Samkharadze T, Erkan M, Reiser-Erkan C, Demir IE, Kong B, Ceyhan GO, Michalski CW, Esposito I, Friess H and Kleeff J: Pigment epithelium-derived factor associates with neuropathy and fibrosis in pancreatic cancer. Am J Gastroenterol. 106:968–980. 2011. View Article : Google Scholar : PubMed/NCBI | |
Lei J, Ma J, Ma Q, Li X, Liu H, Xu Q, Duan W, Sun Q, Xu J, Wu Z and Wu E: Hedgehog signaling regulates hypoxia induced epithelial to mesenchymal transition and invasion in pancreatic cancer cells via a ligand-independent manner. Mol Cancer. 12:662013. View Article : Google Scholar : PubMed/NCBI | |
Cheng ZX, Sun B, Wang SJ, Gao Y, Zhang YM, Zhou HX, Jia G, Wang YW, Kong R, Pan SH, et al: Nuclear factor-kappaB-dependent epithelial to mesenchymal transition induced by HIF-1alpha activation in pancreatic cancer cells under hypoxic conditions. PLoS One. 6:e237522011. View Article : Google Scholar : PubMed/NCBI | |
Zhu H, Wang D, Zhang L, Xie X, Wu Y, Liu Y, Shao G and Su Z: Upregulation of autophagy by hypoxia-inducible factor-1α promotes EMT and metastatic ability of CD133+ pancreatic cancer stem-like cells during intermittent hypoxia. Oncol Rep. 32:935–942. 2014. View Article : Google Scholar : PubMed/NCBI | |
Salnikov AV, Liu L, Platen M, Gladkich J, Salnikova O, Ryschich E, Mattern J, Moldenhauer G, Werner J and Schemmer P: Hypoxia induces EMT in low and highly aggressive pancreatic tumor cells but only cells with cancer stem cell characteristics acquire pronounced migratory potential. PloS One. 7:e463912012. View Article : Google Scholar : PubMed/NCBI | |
Zhang Q, Lou Y, Zhang J, Fu Q, Wei T, Sun X, Chen Q, Yang J, Bai X and Liang T: Hypoxia-inducible factor-2alpha promotes tumor progression and has crosstalk with Wnt/beta-catenin signaling in pancreatic cancer. Mol Cancer. 16:1192017. View Article : Google Scholar : PubMed/NCBI | |
Erkan M, Kurtoglu M and Kleeff J: The role of hypoxia in pancreatic cancer: A potential therapeutic target? Expert Rev Gastroenterol Hepatol. 10:301–316. 2016. View Article : Google Scholar : PubMed/NCBI | |
van Roy F: Beyond E-cadherin: Roles of other cadherin superfamily members in cancer. Nat Rev Cancer. 14:121–134. 2014. View Article : Google Scholar : PubMed/NCBI | |
Hoffman BD and Yap AS: Towards a dynamic understanding of cadherin-based mechanobiology. Trends Cell Biol. 25:803–814. 2015. View Article : Google Scholar : PubMed/NCBI | |
Lecuit T and Yap AS: E-cadherin junctions as active mechanical integrators in tissue dynamics. Nat Cell Biol. 17:533–539. 2015. View Article : Google Scholar : PubMed/NCBI | |
Kotiyal S and Bhattacharya S: Events of molecular changes in epithelial-mesenchymal transition. Crit Rev Eukaryot Gene Expr. 26:163–171. 2016. View Article : Google Scholar : PubMed/NCBI | |
Qian X, Anzovino A, Kim S, Suyama K, Yao J, Hulit J, Agiostratidou G, Chandiramani N, McDaid HM, Nagi C, et al: N-cadherin/FGFR promotes metastasis through epithelial-to-mesenchymal transition and stem/progenitor cell-like properties. Oncogene. 33:3411–3421. 2014. View Article : Google Scholar : PubMed/NCBI | |
Beuran M, Negoi I, Paun S, Ion AD, Bleotu C, Negoi RI and Hostiuc S: The epithelial to mesenchymal transition in pancreatic cancer: A systematic review. Pancreatology. 5:217–225. 2015. View Article : Google Scholar | |
Xie D and Xie K: Pancreatic cancer stromal biology and therapy. Genes Dis. 2:133–143. 2015. View Article : Google Scholar : PubMed/NCBI | |
Kim YR, Park MK, Kang GJ, Kim HJ, Kim EJ, Byun HJ, Lee MY and Lee CH: Leukotriene B4 induces EMT and vimentin expression in PANC-1 pancreatic cancer cells: Involvement of BLT2 via ERK2 activation. Prostaglandins Leukot Essent Fatty Acids. 115:67–76. 2016. View Article : Google Scholar : PubMed/NCBI | |
Hilbig A and Oettle H: Transforming growth factor beta in pancreatic cancer. Curr Pharm Biotechnol. 12:2158–2164. 2011. View Article : Google Scholar : PubMed/NCBI | |
Melzer C, Hass R, von der Ohe J, Lehnert H and Ungefroren H: The role of TGF-beta and its crosstalk with RAC1/RAC1b signaling in breast and pancreas carcinoma. Cell Commn Signal. 15:192017. View Article : Google Scholar |