The MRTF-A/B function as oncogenes in pancreatic cancer
- Authors:
- Published online on: October 15, 2015 https://doi.org/10.3892/or.2015.4329
- Pages: 127-138
Abstract
Introduction
Pancreatic adenocarcinoma is a highly lethal disease and it is currently the fourth leading cause for cancer-related mortality (1,2). The overall 5-year survival rate among patients with pancreatic cancer is <5% (2,3). The mortality rate approaches 100% due to the propensity for early metastatic spread and because the disease is highly resistant to radiation and chemotherapy (2). Increasing evidence indicates that human pancreatic cancer is driven by 'cancer-initiating cells (CICs)' popularly also known as 'cancer stem cells' (CSCs) that may contribute to tumor metastasis and therapeutic resistance (4–7). The molecular basis for these characteristics of CICs or CSCs is incompletely understood.
The transcription factor, serum response factor (SRF) is an important regulator of cytoskeletal and muscle-specific gene expression (8,9). The myocardin family members MRTF-A/B (also known as megakaryocytic acute leukemia and megakaryoblastic leukemia-1/2) are well-established co-activators of SRF (10,11). Although myocardin expression is restricted to smooth and cardiac muscle lineages, MRTF-A/B are expressed ubiquitously. The activity of MRTF-A/B is regulated by their translocation from the cytosol to the nucleus, which is triggered by the activation of Rho family proteins (11). Similar to myocardin, MRTF-A/B are reported to contribute to skeletal, cardiac and smooth muscle differentiation (12). For example, Wnt2 signaling activates the airway smooth muscle program in the lung by regulating myocardin/MRTF-B expression (13). Although their importance in mammary myoepithelial differentiation (14,15) and the epithelial-mesenchymal transition (EMT) (16) has been established, their functions in cancer are completely different between myocardin and MRTF-A/B. Myocardin as an effective inducer of growth arrest and differentiation of certain tumors and is frequently repressed during human malignant transformation (12,17). Yet, MRTF-A/B promotes tumor cell invasion and metastasis (18). Up to now, the roles of MRTF-A and MRTF-B have not been reported in pancreatic cancer.
Herein, to clarify involvement of MRTF-A/B expression in pancreatic cancer, we used quantitative reverse transcription-polymerase chain reaction and western blot analysis to detect MRTF-A/B in pancreatic cancer, intraductal papillary mucinous neoplasm (IPMN) and non-neoplastic pancreata. MRTF-A/B expression differed significantly between cancer and non-neoplastic tissues as well as also differed between non-neoplastic tissues and IPMN bulk tissues. Next, we studied the roles of MRTF-A/B in vitro. Overexpression of MRTF-A/B promoted EMT and generated stem cell-like cells in normal pancreatic cells. We performed quantitative reverse transcription-polymerase chain reaction to detect the level of MRTF-A/B in 19 pancreatic cancer cell lines. We found that their expression was associated with gemcitabine resistance. Like in normal pancreatic cells, MRTF-A/B also promoted EMT and generated stem cell-like cells in pancreatic cancer cells and they could regulate microRNA expression associated with EMT and CICs. Finally, to further demonstrate the roles of MRTF-A/B in vivo, we performed a nude mouse model of s.c. xenografts and found that overexpression of MRTF-A and MRTF-B promoted pancreatic cancer growth. Elucidating the roles of MRTF-A/B will help us to further understand molecular basis of the disease and offer new gene targets for effective therapies.
Materials and methods
Pancreatic tissues
Tissues were obtained from the primary tumor of each resected pancreas for a total of 37 IDC and 48 IPMN samples as well as 32 non-neoplastic pancreata at the time of surgery at the Department of Hepatobiliary and Pancreatic Surgery, Jinan Central Hospital and Hubei Cancer Hospital. All tissues were examined histologically, and pathologists confirmed the diagnosis. The University Medical Ethics Committee approved the experiments undertaken. The use of human tissue samples follows internationally recognised guidelines as well as local and national regulations. Informed consent was obtained from each individual.
Cell culture
HPDE6c7 normal pancreatic cells and pancreatic cancer cell lines KP-2, CFPAC-1, KP-3, H48N, Suit-2, Capan-1, SW1990, Kp-1N, L3.6pl, Colo357, BxPC-3, HPAC, CFPAC, Capan-2, MiaPaCa-2, NOR-P1, ASPC-1, PANC-1 and HS766T were obtained from the American Type Culture Collection (ATCC). HPDE6c7 normal pancreas cells as well as pancreatic cancer cell lines BxPC-3 and Colo357 were chosen to establish stable cell lines overexpressing MRTF-A and MRTF-B for this study. HPDE6c7, BxPC-3 and Colo357 cells were transfected with the corresponding empty vector pcDNA3 Neo or pcDNA3-MRTF-A or pcDNA3-MRTF-B by using ExGen-500 transfection reagent (Fermentas, Germany) following the manufacturer's instructions, as previously described (1,19,20) and referred to as HPDE6c7-control or HPDE6c7-MRTF-A or HPDE6c7-MRTF-B, BxPC-3-control or BxPC-3-MRTF-A or BxPC-3-MRTF-B cells, Colo357-control or Colo357-MRTF-A or Colo357-MRTF-B, respectively. Stable cell lines overexpressing MRTF-A or MRTF-B were selected by antibiotics, gentamycin, and the level of expression was confirmed by western blot analysis. The stably transfected cell lines were cultured in Dulbecco's modified Eagle's medium (DMEM; Invitrogen, Carlsbad, CA, USA), supplemented with 10% fetal bovine serum (FBS), 2 mmol/l glutamine, 50 U/ml penicillin, and 50 µg/ml streptomycin. All cells were maintained in a 5% CO2-humidified atmosphere at 37°C.
Quantitative real-time RT-PCR (qRT-PCR)
Quantitative real-time RT-PCR was described before (21). The specific primer sets for PCR were as follows: GAPDH forward, 5′-GAAGGTGAAGGTCGGAGTCA-3′ and reverse, 5′-GAAG ATGGTGATGGGATTTC-3′; MRTF-A forward, 5′-ATGGA GCTGGTGGAGAAGAATATC-3′ and reverse, 5′-GAAGGA GGAACTGTCTGCTACC-3′; MRTF-B, forward, 5′-CCAGA CCGCTCTGAGCTTG-3′ and reverse, 5′-TCCTTGACACTC GAATCCAC3′; E-cadherin forward, 5′-TCAACGATCCTGA CCAGCAGTTCG-3′ and reverse, 5′-GGTGAACCATCATC TGTGGCGATG-3′; N-cadherin forward, 5′-CATCCCTCCA ATCAACTTGC-3′ and reverse, 5′-ATGTGCCCTCAAATG AAACC-3′; vimentin forward, 5′-GACAATGCGTCTCTGG CACGTCTT-3′ and reverse, 5′-TCCTCCGCCTCCTGCAGG TTCTT-3′; ZEB1 forward, 5′-TTAGTTGCTCCCTGTGCA GTT-3′ and reverse, 5′-TAGGAGCCAGAATGGGAAAAG-3′; FOXC2 forward, 5′-TCTCTCGCGCTCTCTCGCTC-3′ and reverse, 5′-TGCAGCCCCTTAATTGTCTGG-3′; Slug, forward, 5′-TGATGAAGAGGAAAGACTACAG-3′ and reverse, 5′-GCTCACATATTCCTTGTCACAG-3′; SIP1 forward, 5′-GTCCATGCGAACTGCCATCTGATCCGC TCT-3′ and reverse, 5′-GGCTTGCAGAATCTCGCCAC-3′; TWIST, forward, 5′-GGAGTCCGCAGTCTTACGAG-3′ and reverse, 5′-TCTGGAGGACCTGGTAGAGG-3′; and Snail forward, 5′-TCAGAATTCATGCCGCGCTCTTTCCTCGTC AGGAAGCC-3′ and reverse, 5′-ACTGGATCCTCAGCGGG GACATCCTGAGCAGCCGGAC-3′.
Western blot analysis
Western blot analysis was performed as described before (22). Mainly, after incubation with primary antibody anti-MRTF-A (1:250); anti-MRTF-B (1:250); anti-CD44 (1:250); anti-Tspan8 (1:250); anti-c-Met (1:250); anti-CD151 (1:250); anti-ZEB1 (1:250); anti-Slug (1:250); anti-E-cad (1:250); anti-vimentin (1:250) and anti-β-actin (1:500) (all from Abcam, Cambridge, MA, USA) overnight at 4°C. IRDye™-800 conjugated anti-rabbit secondary antibodies (Li-COR Biosciences, Lincoln, NE, USA) were used for 30 min at room temperature. The specific proteins were visualized by Odyssey™ Infrared Imaging system (Gene Company, Lincoln, NE, USA).
Sphere growth
Cells (103/ml) in serum-free RPMI-1640/1 mM Na-pyruvate were seeded on 0.5% agar precoated 6-well plates. After 1 week, half the medium was changed every third day. Single spheres were picked and counted.
Immunofluorescence analyses
For cell immunofluorescence analyses, cells were plated on glass coverslips in 6-well plates and transfected as indicated. At 48 h after transfection, coverslips were stained with the mentioned anti-fibronectin, anti-vimentin, anti-E-cadherin, and anti-EpCAM antibody. Alexa Fluor 488 goat anti-rabbit IgG antibody was used as secondary antibody (Invitrogen). Coverslips were counter-stained with DAPI (Invitrogen-Molecular Probes, Eugene, Oregon, USA) for visualization of nuclei. Microscopic analysis was performed with a confocal laser-scanning microscope (Leica Microsystems, Bensheim, Germany). Fluorescence intensities were measured in a few viewing areas for 300 cells/coverslip and analyzed using ImageJ 1.37v software (http://rsb.info.nih.gov/ij/index.html).
Clonogenic assay
Cells were collected after trypsinization, and re-suspended in the complete medium. Single-cell suspensions were plated in regular 10 cm in diameter Petri dishes at the clonal density of 1,000 cells/dish. After 3 weeks of culture, colonies were fixed with 4% paraformaldehyde for 10 min, stained with crystal violet for additional 15 min, and washed with 1X PBS. The colonies were photographed. The colony numbers were counted using software image analysis program Scion Image downloaded from NIH website (http://www.scioncorp.com). Particle Analysis program was used for counting the colony numbers. Data are presented as relative colony number.
Soft agar assay
Cells were harvested and suspended in culture medium. To make the bottom layer, 1 ml of 0.5% agarose (Invitrogen) was added to 6-well plates, and allowed to gel at room temperature. To prepare the top layer (0.25% agarose), 500 µl of 0.5% agarose was mixed with 500 µl cell suspension containing the 5,000 cells. This mixture was laid above the bottom layer and allowed to solidify at room temperature. An additional 2 ml of culture medium was added after solidification to the top layer, and cells were incubated for 4 weeks at 37°C. After three weeks of growth, the colonies were photographed (×40). The colony numbers were counted under a phase contrast microscope (×40). Data are presented as colony numbers per field.
S.C. tumor models
BxPC-control and BxPC-MRTF-A and BxPC-MRTF-B cells were harvested by trypsinization, and resuspended in RPMI-1640. Only single-cell suspensions with >95% viability were used. The cells (5×106) were inoculated into the right flank (s.c. tumor model) of 5 to 6-week-old male nude mice (NCI/Charles River Breeding Labs, Wilmington, MA, USA). All mice were cared for in accordance with the Office for Protection from Research Risks and Animal Welfare Act guidelines under an animal protocol approved by the Jinan Central Hospital of Medicine Institutional Animal Care and Use Committee. For the s.c. tumor model, the tumor size was measured weekly using a digital caliper (VWR International, Leuven, Belgium), and the tumor volume was calculated using the following formula: tumor volume (mm3) = 0.52 × [width (mm)]2 × [length (mm)] (23). After week 5, all surviving mice were euthanized with an overdose of CO2 exposure and evaluated for the presence of tumors and the metastases in their abdominal cavity. For both s.c. experiments, the animals were euthanized when their tumor size reached 2 cm in diameter or the animals became moribund during the observation period, and the time of euthanization was recorded as the time of mortality.
miRNA microarray
Total RNA from cultured cells, with efficient recovery of small RNAs, was isolated using the mirVana miRNA Isolation kit (Ambion, Austin, TX, USA). cRNA for each sample was synthesized by using 3′ IVT Express kit (Affymetrix, Santa Clara, CA, USA) according to the manufacturer's instructions. The purified cRNA was fragmented by incubation in fragmentation buffer (provided in the 3′ IVT Express kit) at 95°C for 35 min and chilled on ice. The fragmented labeled cRNA was applied to MicroRNA 2.0 array and hybridized in Genechip hybridization oven 640 (both from Affymetrix) at 45°C for 18 h. After washing and staining in Genechip fluidics station 450, the arrays were scanned by using Genechip scanner 3000 (both from Affymetrix). The gene expression levels of the samples were normalized and compared by using Partek GS 6.5 (Partek, Inc., St. Louis, MO, USA). Average-linkage hierarchical clustering of the data was applied by using the Cluster; http://rana.lbl.gov) and the results were displayed by using TreeView (both: Eisen et al, Stanford, Stanford University, CA, USA; http://rana.lbl.gov).
Results
Analysis of MRTF-A and MRTF-B expression in pancreatic cancer, IPMN, and non-neoplastic bulk tissues
We measured the levels of MRTF-A and MRTF-B in bulk tissues from 37 pancreatic cancers (conventional IDC), 48 IPMNs and 32 non-neoplastic pancreata. To normalize MRTF-A and MRTF-B expression, we used U6 as a reference gene. Pancreatic cancer bulk tissues expressed higher levels of MRTF-A (Fig. 1A) and MRTF-B (Fig. 1B) than did IPMN bulk tissues (pancreatic cancer vs. IPMN, p<0.05), there was a significant difference between pancreatic cancer and non-neoplastic pancreata (p<0.01). We also observed that IPMN bulk tissues expressed higher levels of MRTF-A and MRTF-B than non-neoplastic pancreata (IPMN bulk tissues vs. non-neoplastic pancreata, p<0.05). Representative results of electrophoresis of RT-PCR products are shown in the bottom of Fig. 1A and B. Next, we performed western blot analysis to detect MRTF-A and MRTF-B level among non-neoplastic pancreas, IPMN and pancreatic cancer. Consistent with the results of RT-PCR, the results of western blot analysis showed that MRTF-A (Fig. 1C) and MRTF-B (Fig. 1D) were upregulated in pancreatic cancer, compared with IPMN and non-neoplastic pancreas. We also found that IPMN bulk tissues expressed higher levels of MRTF-A (Fig. 1C) and MRTF-B (Fig. 1D) than did non-neoplastic pancreas (IPMN bulk tissues vs. non-neoplastic pancreata, p<0.05). Representative results of western blot analysis are shown (Fig. 1C and D). The results implied that upregulation of MRTF-A and MRTF-B are associated with the development of pancreatic cancer and IPMN.
Analysis of MRTF-A and MRTF-B expression in a normal pancreas cell line and pancreatic cancer cell lines and their expression associated with gemcitabine resistance
We also performed real-time PCR to detect the expression of MRTF-A and MRTF-B in the HPDE6C7 normal pancreatic cell line and 19 pancreatic cancer cell lines. Except for KP2 cells, we detected MRTF-A and MRTF-B mRNA in 18 pancreatic cancer cell lines (Table I). It has been reported that L3.6pl, Colo357, BxPC-3, HPAC and CFPAC cells are gemcitabine-sensitive and MiaPaCa-2, ASPC-1, PANC-1 and HS766T cells are gemcitabine-resistant (24,25). We found that expression of MRTF-A and MRTF-B was significantly increased in gemcitabine-resistant cells (Table I). To confirm that MRTF-A and MRTF-B were increased in gemcitabine-resistant cells, we performed western blot analysis to detect their protein. The results showed that MRTF-A and MRTF-B protein were evidently upregulated in gemcitabine-resistant cells (Fig. 2).
MRTF-A and MRTF-B promote EMT and generate stem cell-like cells in normal pancreatic cells
To determine whether MRTF-A and MRTF-B could promote EMT, HPDE6C7 cell line was chosen to establish a stable cell line overexpressing MRTF-A and MRTF-B for this study. HPDE6C7 cells were transfected with the corresponding empty vector pcDNA3 NEO or pcDNA3-MRTF-A or pcDNA3-MRTF-B. We performed real-time PCR and western blot analysis to detect MRTF-A in HPDE6C7-MRTF-A cells. Compared with HPDE6C7-control cells, we found that MRTF-A mRNA (Fig. 3A) and its protein (Fig. 3B) were significantly upregulated in HPDE6C7-MRTF-A cells. Similar to HPDE6C7-MRTF-A cells, MRTF-B mRNA (Fig. 3C) and its protein (Fig. 3D) were significantly upregulated in HPDE6C7-MRTF-B cells.
We observed phase-contrast images of HPDE6C7 cells expressing the control vector, MRTF-A and MRTF-B, as well as HPDE6C7 cells treated with TGFβ1 for 12 days, a standard treatment that induces EMT (26). The results showed that MRTF-A, MRTF-B and TGFβ1 induced EMT phenotype from a cobblestone-like to a spindle-like morphology (Fig. 3E), accompanied by increase of invasion and migration in the cells (data not shown). We also performed real-time PCR to detect epithelial and mesenchymal markers. As anticipated, HPDE6c7-MRTF-A and HPDE6c7-MRTF-B cells as well as HPDE6C7 cells treated with TGFβ1, epithelial markers (E-cadherin) was downregulated and mesenchymal markers (such as N-cadherin, vimentin, and Snail) were upregulated in HPDE6c7-MRTF-A and HPDE6c7-MRTF-B cells (Fig. 3F), compared with HPDE6c7-control cells. CD44, Tspan8, c-Met and CD151 are markers for CICs in pancreatic cancer (5,27–30). We performed western blot analysis to detect the expression of CD44, Tspan8, c-Met and CD151 in MRTF-A and MRTF-B overexpressing pancreatic cancer cells. We found that the overexpression of MRTF-A and MRTF-B significantly upregulated CD44, Tspan8 and CD151 expression (Fig. 3G).
Following induction of EMT in HPDE6c7 cells by exposing them to TGFb1, the cells formed at least 40-fold more spheres than the untreated control cells (Fig. 3H). With these findings in mind, we examined the sphere forming ability of the HPDE6C7 cells forced to undergo EMT by ectopic expression of MRTF-A or MRTF-B. Significantly, we found that the HPDE6c7-MRTF-A and HPDE6c7-MRTF-B cells that underwent EMT formed >60-fold more spheres than the cells infected with the corresponding control vector (Fig. 3I). Based on this functional assay, we concluded that overexpression of MRTF-A and MRTF-B was able to promote EMT and generate stem cell-like cells in normal pancreatic cells.
MRTF-A and MRTF-B promote EMT in pancreatic cancer
Having demonstrated that MRTF-A and MRTF-B promoted EMT and generated stem cell-like cells in normal pancreatic cells and MRTF-A and MRTF-B could promote metastasis in tumor cell and xenografts (18), we reasoned that MRTF-A and MRTF-B also could promote EMT in pancreatic cancer cells.
Because expression of MRTF-A and MRTF-B was low in BxPC-3 and Colo357 cells, these cells were chosen to establish the stable cell lines overexpressing MRTF-A and MRTF-B. BxPC-3 and Colo357 cells were transfected with the corresponding empty vector pcDNA3 NEO or pcDNA3-MRTF-A or pcDNA3-MRTF-B. We performed real-time PCR and western blot analysis to detect MRTF-A in BxPC-3-MRTF-A cells. Compared with BxPC-3-control cells, we found that MRTF-A mRNA (Fig. 4A) and its protein (Fig. 4B) were significantly upregulated in BxPC-3-MRTF-A cells. Real-time PCR and western blot analysis were also performed to detect MRTF-B mRNA and protein expression. The result showed that MRTF-B mRNA (Fig. 4C) and its protein (Fig. 4D) were significantly upregulated in BxPC-3-MRTF-B cells. Similar to BxPC-3 cells, MRTF-A (Fig. 4E and F) and MRTF-B (Fig. 4G and H) were significantly increased in Colo357-MRTF-A and Colo357-MRTF-B cells, respectively.
In order to assess the role of MRTF-A and MRTF-B in pancreatic cancer, we observed phase-contrast images of pancreatic cancer BxPC-3 cells expressing the control vector, MRTF-A and MRTF-B. The results showed that MRTF-A and MRTF-B induced EMT phenotype from a cobblestone-like to a spindle-like morphology (Fig. 5A), accompanied by the decrease of E-cadherin expression and the increase of fibronectin and vimentin in the cells (Fig. 5B). We performed real-time PCR to detect epithelial marker (E-cadherin) and mesenchymal markers (N-cadherin, vimentin, ZEB1, FOXC2, Slug, SIP1, Twist and Snail). The results showed that epithelial marker (E-cadherin) was downregulated and all the mesenchymal markers were upregulated in MRTF-A or MRTF-B overexpressing BxPC-3 cells, compared with BxPC-3-control cells (Fig. 5C). Relative to the expression in BxPC-3-control cells, the level of the E-cadherin mRNA in BxPC-3-MRTF-A and BxPC-3-MRTF-B cells was strongly reduced (>100-fold), while expression of mRNAs encoding mesenchymal markers was markedly increased, specifically N-cadherin (145- and 150-fold, respectively), vimentin (138- and 129-fold, respectively). There was also a considerable increase in the expression of EMT-inducing transcription factors, specifically FOXC2 (62- and 129-fold), SIP1 (75- and 70-fold, respectively), Snail (49- and 74-fold, respectively), and Twist (140- and 220-fold); Slug expression was only marginally increased (5-fold) in MRTF-A overexpressing BxPC-3 cells, but it was significantly upregulated in BxPC-MRTF-B cells. To further confirm that the markers associated with EMT were affected by MRTF-A and MRTF-B, we performed western blot analysis to detect E-cadherin, ZEB1, vimentin and Slug protein. The result showed that MRTF-A and MRTF-B downregulated E-cadherin expression and upregulate ZEB1, vimentin and Slug expression in BxPC-3 cells (Fig. 5D). These measurements provided further indication that MRTF-A and MRTF-B promote EMT in pancreatic cancer.
In addition, real-time PCR was performed to detect whether MRTF-A and MRTF-B overexpression could affect E-cadherin, N-cadherin, vimentin, Slug and Twist expression in Colo357 cells. The results showed that MRTF-A and MRTF-B downregulated E-cadherin and upregulated N-cadherin, vimentin, Slug and Twist expression in the cells (Fig. 5E and F).
MRTF-A and MRTF-B promotes CSC in pancreatic cancer cells
To determine whether cells with EMT phenotype could have stem-like cell characteristics. Sphere forming assay was conducted to assess the capacity of CSC or CSC-like cell self renewal in this study. We found that BxPC-MRTF-A and BxPC-MRTF-B cells showed increased formation of spheres (Fig. 6A) consistent with increased expression of CSC surface marker, EpCAM in spheres of BxPC-MRTF-A and BxPC-MRTF-B cells compared to BxPC-control cells (Fig. 6B), suggesting that overexpression of MRTF-A and MRTF-B could increase the formation of pancreatospheres associated with increased expression of EpCAM, which further suggest that MRTF-A and MRTF-B is involved in the regulation of the CSC phenotype.
Next, we performed clonogenic assays. We found that clonogenic ability was significantly increased in BxPC-3-MRTF-A and BxPC-3-MRTF-B cells compared with BxPC-3-control cells (Fig. 6C, upper panel). Fig. 6C, bottom panel, further indicated that BxPC-3-MRTF-A and BxPC-3-MRTF-B cells showed ~10-fold increase in colony numbers relative to BxPC-3-control cells.
Soft agar assay, also known as anchorage-independent growth assay, was also performed. BxPC-3-MRTF-A and BxPC-3-MRTF-B cells showed dramatic increase in clonogenic potential compared to BxPC-3-control cells (Fig. 6D, upper panel). Fig. 6D, bottom panel, clearly shows the colony numbers generated from BxPC-3-control cells, BxPC-3-MRTF-A and BxPC-3-MRTF-B cells per microscopic field. These results demonstrated an increase in clonogenic ability of EMT cells. Colo357-MRTF-A and Colo357-MRTF-B cells also displayed an increased clonogenic capacity, compared with Colo357-control cells, respectively (data not shown).
The effect of MRTF-A and MRTF-B on miRNA expression was identified by miRNA profiling in BxPC-3 cells
We next examined the ability of MRTF-A and MRTF-B to regulate miRNA expression by microarray analysis of miRNAs expression profiles in BxPC-3 cells. RNAs isolated from BxPC-3-control, BxPC-3-MRTF-A and BxPC-3-MRTF-B were hybridized to a custom miRNA microarray platform. After 3 times hybridization, quantification, and normalization in each cell line, we identified 25 consistently altered miRNAs, of which especially 16 miRNAs were upregulated and 9 miRNAs were downregulated, with >2-fold changes in BxPC-3-MRTF-A cells compared to BxPC-3-control cells (Table II).
Table IImiRNA expression was significantly regulated by MRTF-A in human pancreatic cancer BxPC-3 cells. |
Like in BxPC-3-MRTF-A cells, we identified 29 consistently altered miRNAs, of which especially 20 miRNAs were upregulated and 9 miRNAs were downregulated, with >2-fold changes in BxPC-3-MRTF-B compared to BxPC-3-control cells (Table III).
Table IIImiRNA expression was significantly regulated by MRTF-B in human pancreatic cancer BxPC-3 cells. |
Overexpression of MRTF-A and MRTF-B promotes pancreatic cancer growth in a nude mouse model of s.c. xenografts
We further analyzed the role of MRTF-A and MRTF-B on tumor growth in vivo using an immunodeficient nude mouse model. BxPC-3-MRTF-A and BxPC-3-MRTF-B cells showed increased tumor growth and a dramatic increase in tumor volume after 4 weeks compared with the BxPC-3-control cells in the s.c. tumor model (p<0.01; n=10; Fig. 6A and B). BxPC-3-MRTF-A and BxPC-3-MRTF-B cells also significantly increased s.c. tumor weight after 4 weeks compared with BxPC-3-control cells (p<0.05; n=10; Fig. 7C and D). Mice given injections of BxPC-3-MRTF-A and BxPC-3-MRTF-B cells had severe skin ulcer (90%) and gain of body weight (50%), whereas only 30% of BxPC-3-control mice showed mild skin ulcering, but no other symptoms.
Discussion
In the present sdufy, we showed that MRTF-A and MRTF-B were upregulated in pancreatic cancer tissues and IPMN bulk tissues, compared with non-neoplastic pancreas. The results supported the hypothesis that MRTF-A and MRTF-B are oncogenes in pancreatic cancer. Leitner et al reported that MRTFs impairs migration of fibroblasts and partial knockdown of MRTFs increases motility (31). However, other studies demonstrated that MRTF double knockout in mouse embryonic fibroblasts (MEFs) impairs cell migration, consistent with an important role for SRF and MRTFs in cytoskeletal organization and actin homeostasis (32) and MRTFs have been implicated in experimental metastasis, where knockdown of MRTFs reduced adhesion, migration and invasion of highly invasive cancer cells (18). Our results demonstrated that overexpression of MRTF-A and MRTF-B can promote EMT and generate stem cell-like cells in normal pancreatic cells and pancreatic cancer cells. EMT is a crucial developmental program in which immotile epithelial cells acquire mesenchymal traits. The term EMT refers to a complex molecular and cellular programme by which epithelial cells shed their differentiated characteristics, including cell-cell adhesion, planar and apical-basal polarity, and lack of motility, and acquire instead mesenchymal features, including motility, invasiveness, metastatic dissemination and an acquisition of therapeutic resistance (33-41). Importantly, expression of the EMT programs has been associated with poor clinical outcome in multiple tumor types (42). Although we showed that MRTF-A and MRTF-B were upregulated in pancreatic cancer tissues and they can promote EMT and generate stem cell-like cells in normal pancreatic cells and pancreatic cancer cells, we did not evaluate whether their expression was associated with poor clinical outcome. In addition, we found that MRTF-A and MRTF-B were upregulated in gemcitabine-resistant pancreatic cancer cells, implying that MRTF-A and MRTF-B could be a key molecule in gemcitabine resistance in human pancreatic cancer. They may have the potential as predictor and modulator of gemcitabine treatment.
MicroRNAs (miRs), the small non-coding RNA molecules that can suppress specific gene expression by interacting with the 3′-untranslated regions (3′-UTRs) of target mRNAs, have also been connected to EMT and cancer (43–46). EMT has been linked to stem cell phenotype (41,47). We found that MRTF-A and MRTF-B could regulate many microRNAs that play an important role in pancreatic cancer. MicroRNA miR-34 inhibits human pancreatic cancer tumor-initiating cells (48); upregulation of miR-200 and let-7 leads to the reversal of EMT in gemcitabine-resistant pancreatic cancer cells (24); miRNA-96 suppresses KRAS and functions as a tumor-suppressor gene in pancreatic cancer (49); hsa-miR-520h downregulates ABCG2 in pancreatic cancer cells to inhibit migration, invasion, and side populations (50); miR-146a suppresses invasion of pancreatic cancer cells (51). Elevated expression of miR-155, miR-203, miR-210 and miR-222 in pancreatic tumors is associated with poorer survival (52); miR-21 is overexpressed in pancreatic cancer (53) and a potential predictor of survival; inhibition of miR-21 or miR-221 arrests the cell cycle, induces apoptosis, and sensitizes the effects of gemcitabine in pancreatic adenocarcinoma (54). We found that MRTF-A overexpression significantly downregulated miR-34, miR-200, let-7, miR-96, miR-520h and miR-146a level and evidently upregulated miR-155, miR-203, miR-210, miR-222, miR-21, miR-221 and miR-224 in pancreatic cancer cells. Similar to MRTF-A, MRTF-B could significantly inhibit miR-34 expression and upregulate miR-155, miR-21, miR-224 and miR-486 expression. Thus, we reasoned that MRTF-A and MRTF-B function as oncogenes through regulating microRNAs that play important roles in pancreatic cancer.
Abbreviations:
CICs |
cancer-initiating cells |
CSCs |
cancer stem cells |
EMT |
epithelial-mesenchymal transition |
IDC |
invasive ductal carcinoma |
IPMN |
intraductal papillary mucinous neoplasm |
MET |
mesenchymal-epithelial transition |
MRTFs |
myocardin-related transcription factors |
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