Background
Ovarian cancer is a highly lethal disease which represents a great clinical challenge in gynecologic oncology. It is asymptomatic until the disease is in the late stage, causing it to have the highest fatality-to-case ratio of all gynecologic malignancies. There is emerging evidence showing that cancer stem cells are capable of regenerating tumors and they are responsible for the aggressiveness of the disease, metastasis and resistance to therapy [
1]. Cancer stem cells, like somatic stem cells, are thought to be capable of self-renewal or unlimited proliferation. A recent study describes that ovarian cancer cell lines were shown to possess "side population" (SP) cells that have been described as cancer stem cells due to their ability to differentiate into tumors with different histologies, similar to the pluripotent character of stem cells [
1]. It is now believed that cancer often relapses after the treatment due to the stem-like population in some solid tumors [
2]. Although advanced ovarian cancer is generally initially responsive to standard chemotherapies (cisplatin and paclitaxel), it is almost inevitably followed by the drug resistant phenotype. One accepted hypothesis about chemoresistance is that standard therapies fail to target tumor progenitors, which are like normal stem cells, because of the expression of membrane efflux transporters [
1].
The alterations in the mucin expression or glycosylation pattern is often associated with the development of cancer via influencing cellular growth, differentiation, transformation, adhesion, invasion and immunosuppression [
3,
4]. MUC4 frequently displays an altered expression under the pathological conditions of many cancers [
3,
4]. Previously, our study has revealed an aberrant expression of MUC4 mucin in > 90% of different histological subtypes and grades of ovarian tumors with very low or undetectable expression in the normal ovary [
5]. Overexpression of MUC4 mRNA has also been reported in ovarian cancer [
6]. In our previous study, we showed that MUC4 interacts and stabilizes HER2 in both ovarian and pancreatic cancer cells [
7,
8]. We have further shown that MUC4 induces the epithelial to mesenchymal transition (EMT) through the upregulation of N-cadherin, and thereby induces metastasis of human ovarian cancer cells [
9]. A recent study has shown that HER2 amplification regulates the mammary stem/progenitor cell population and promotes carcinogenesis, tumorigenicity and invasive properties [
10]. Recently, Engelmann et al have demonstrated that MUC1 (a membrane bound mucin) is also expressed in the mammary stem/progenitor cells [
11] and is important in the future application of MUC1-based therapies for complete cancer eradication.
The aforementioned observations suggest that MUC4 may have an important role in the pathogenesis of ovarian cancer. In this study, we have investigated increased expression of HER2 and the cancer stem cell population in MUC4 overexpressed ovarian cancer cells. Further, we have analyzed cancer stem cell and self-renewal specific markers in the isolated populations. These studies indicate that MUC4 induces HER2 expression and may enrich the cancer stem cell population in ovarian cancer stem cells.
Methods
Generation of MUC4 construct
We generated a MUC4 minigene construct to overcome the transfection associated problems due to its large size and to investigate the biological function and effect of MUC4 expression in OC cells [
8,
12]. The resultant MUC4 cDNA was sub-cloned into the pSecTag-C vector for further transfection studies.
Cell culture and transfection procedure
SKOV3 cells was procured from ATCC (Manassas, VA, U.S.A.) and cultured in DMEM supplemented with 10% fetal calf serum and antibiotics. The MUC4 gene construct along with the empty vector control pSecTag-C, were transfected in SKOV3 OC cells by Fugene (Invitrogen) following the manufacturer's protocol. Transfected cells were selected in the medium containing 200 μg/ml zeocin (30 Days) and the drug-resistance (zeo+) clones (three from the empty vector, five from the MUC4 gene construct transfected) were selected from different plates and studied after expansion [
8,
9].
Immunoblot assay
SKOV3 derived cell lines were processed for protein extraction and Western blotting using standard procedures. Briefly, the cells were washed twice in PBS and lysate was prepared in RIPA buffer (100 mM Tris, 5 mM EDTA, 5% NP40; pH8.0) containing protease inhibitors (1 mM phenyl-methyl sulphonyl fluoride, 1 μg/ml aprotinin, 1 μg/ml leupeptin). SDS-PAGE (10%) was performed under standard conditions. Resolved proteins were transferred on to the PVDF membrane. After quick washing in PBST (Phosphate buffered saline and 0.1% Tween 20), the membranes were blocked in 5% nonfat dry milk in PBS for at least 2 h and then incubated with primary antibodies MUC4 (mouse), HER2 (rabbit), ALDH1 (rabbit), CD133 (rabbit), Shh (rabbit) and β-actin (mouse) (diluted in 5% non fat dry milk in PBS) overnight at room temperature. Then the membranes were washed (3 × 10 min) in PBST at room temperature and probed with 1:2000 diluted secondary antibodies (anti-mouse and anti-rabbit) for 1 h at room temperature and washed 5 × 10 min with PBST. The signal was detected with an ECL chemiluminescence kit (Amersham Bioscience, UK).
Confocal immunofluorescence microscopy
MUC4 and vector transfected SKOV3 cells were grown on sterilized cover slips for 20 h. Cells were washed with Hanks buffer containing 0.1 M HEPES, and fixed in ice-cold methanol at 20°C for two minutes and blocked with 10% goat serum (Jackson Immunoresearch Labs, Inc., West Grove, PA, U.S.A.) containing 0.05% Tween-20 for at least 30 minutes. For Phalloidin staining, cells were fixed with 3.6% formaldehyde-PBS solution and followed by permeabilization with 0.1% TritonX-100 in PBS for 20 min at room temperature. After the blocking step and a quick wash in PBS, cells were incubated with the MUC4, HER2 and CD133 for 60 minutes at room temperature. Then cells were washed (4 × 5 minutes each washing) with PBS containing 0.05% Tween-20 (PBS-T) and then incubated with FITC-conjugated anti-mouse (green) and Texas red conjugated anti-rabbit (red) secondary antibodies (Jackson Immunoresearch labs, Inc., West Grove, PA) for 30 minutes at room temperature in the dark. Propidium iodide was used for nuclear staining. Cells were washed (5 × 5 minutes) again and mounted on glass slides in anti-fade Vectashield mounting medium (Vector Laboratories, Burlingame, CA). Laser confocal microscopy was performed by using a LSM 510 microscope (Carl Zeiss GmbH, Germany). Microphotographs of different stainings were taken in different channels separately.
Hoechst 33342 dye and CD133 staining for Flowcytometry analysis
Hoechst 33342 dye based FACS analysis have been used to determine the SP and NSP population in MUC4 overexpressed and control SKOV3 cells. Cells were stained with Hoechst 33342 (Sigma) as previously described [
13]. SP cells actively pump-out the dye (Hoechst 33342) and hence exhibit low fluorescence as compared to the NSP cells. Briefly, single cell suspension of OC cells was prepared at a density of 2 × 10
6/ml in pre-warmed DMEM mixed with Hoechst 33342 dye (5 μg/ml). The cells were incubated in water bath at 37°C for 60 minutes and subsequently spun and re-suspended in cold HBSS+ (Hanks Balanced Salt Solution) containing 2 μg/ml propidium iodide (PI) for dead cell discrimination. Finally, the samples were run directly on the FACS and counted according to the strength of staining. The Hoechst dye was excited with the UV laser at 350 nm and its fluorescence measured with a 450/20 BP filter (Hoechst blue) and a 675 EFLP optical filter (Hoechst red). For the CD133-FITC and FACS analysis, 2 × 10
7 cells were incubated with FcR blocking reagent (MACS, Miltenyi Biotech) for 30 minutes. Then it was incubated with surface marker antibody CD133-FITC (MACS, Miltenyi Biotech) for 10 minutes. Finally, FACS analysis was carried out to count CD133-positive populations in MUC4-transfected and control SKOV3 cells.
Discussion
Ovarian cancer is the fourth leading cause of cancer deaths among all women and has the highest mortality among the gynecologic cancers. It is one of the most challenging of all cancers to fight as it often goes undiagnosed until it has already advanced and metastasized. Furthermore, current therapeutic strategies have been inefficient and tumor recurrence is observed in up to 70% of patients with advanced stage ovarian cancer, even after treatment [
18‐
20]. Numerous evidences have revealed that a small population of cells behaving like stem-cells are responsible for the tumor recurrence and disease aggressiveness [
1]. These populations of cells known as cancer stem cells have been demonstrated to have roles in many cancers, such as cancers of the hematopoietic system, ovarian, breast, brain, prostate, pancreas, colon and liver [
1,
2,
11,
13,
16,
21‐
25]. To date, very few specific tumor antigens have been identified to target the cancer stem cell population to prevent tumor recurrence. Hence, the present study showed that MUC4 overexpression is enriching the cancer stem cell population and it is expressed in stem/progenitor cells in ovarian cancer cells.
MUC4 is known to be overexpressed in many types of carcinomas, including ovarian carcinoma [
3,
5,
26]. The primary role of MUC4 is to protect the epithelial surface from injuries under normal physiological conditions, but overexpression is often correlated with the malignant phenotype. Our previous study reveals that MUC4 is aberrantly expressed in ovarian tumors [
5] and in pancreatic tumors [
3]. Another study from our laboratory shows that down-regulation of MUC4 is involved in the suppression of pancreatic tumor cell growth and metastasis [
27]. In our recent study, we have shown a direct association of the MUC4 mucin with the metastatic human ovarian cancer phenotype and also provided experimental evidence for a functional role of MUC4 in altered growth behavioral properties of the tumor cell [
8]. The ectopic expressed MUC4 gene has all the basic elements of the MUC4 gene but its tandem repeat region is only 10% of the wild-type MUC4 allele [
8,
12]. As predicted, MUC4 overexpressed cells expressed an approximately 322 kDa protein. The localization of the MUC4 protein was observed in both the membrane and cytoplasm of SKOV3 ovarian cancer cells.
Our previous study demonstrates an altered expression of the human epidermal growth factor receptor 2 (HER2), also known as ErbB2, in MUC4 overexpressing cells [
8]. HER2 belongs to the epidermal growth factor receptor (EGFR) family. Most membrane-bound mucins have juxtamembrane domains with homology to the members of the EGF family [
4]. MUC4 has been shown to act as an unorthodox ligand for ErBB2/HER2 [
28], potentiating its responsiveness in cancer signaling [
7,
8]. Our recent finding showed that an overexpression of MUC4 increases the expression of HER2 in ovarian cancer cells [
8] and stabilizes the HER2 oncoprotein in pancreatic cancer cells [
7]. In the present study, we analyzed the expression of the HER2 protein in MUC4-transfected ovarian cancer cells. The exogenous MUC4 expression in ovarian cancer cells showed an increase in HER2 expression and colocalization, suggesting that MUC4 is involved in the stabilization of HER2 protein.
There is emerging evidence that small subpopulations that behave like stem cells are present in many types of cancer. These subpopulations are responsible for the initiation, drug resistance and tumor recurrence [
1]. Korkaya and colleagues showed that HER2-overexpression in breast cancer cells enriched the cancer stem cell population, evidenced by an increased number of tumor sphere formation and cancer stem cell marker aldehyde dehydrogenase expression [
10]. They have further shown an increased expression of stem cell regulatory genes, increased invasion
in vitro and increased tumorigenesis in NOD/SCID mice [
10]. This suggests that, in addition to genetic alterations such as amplification, the expression of the HER2 level is important for the maintenance of CSCs. Recently, a minor population of cells was isolated by flow cytometry based on their capacity to efflux the fluorescent DNA-binding dye Hoechst 33342 to identify cancer stem cells. This is one of the important properties for cancer stem/progenitor cells [
14,
15] because of the expression of ABCG2 drug resistance protein. In our study, we have observed enriched population of CSCs in MUC4-transfected ovarian cancer cells using Hoechst33342 dye and CD133-positive population analysis. Further, an interesting observation of tumor sphere like circular colony formation was observed predominantly in MUC4-transfected ovarian cancer cells and these colonies were isolated from the cells and analyzed with cancer stem cell markers. There was a slight change in the molecular weight of MUC4 protein in the isolated colonies suggesting that there may be some variation in glycosylation pattern, which will be explored in future studies (Figure
4B). The enriched cancer stem cell population in MUC4 overexpressed cells may be due to the increased expression of HER2 expression. Furthermore, isolated circular colonies showed significant expression of cancer stem cell specific markers CD133 and ALDH1 and the self-renewal maintenance marker Shh, which concludes that MUC4 is enriching the cancer stem cell population in ovarian cancer cells. Similarly, a recent study showed that a membrane-bound mucin MUC1 maintains a small population of stem/progenitor cells in the breast cancer (MCF7) cell line [
11]. The fact that the vast majority of MCF7 stem cell enriched SP cells express MUC1 suggests that epithelial cancer stem cells would also be the targets of various immunotherapy approaches based on the MUC1 tumor antigen that has been designed with mature tumor cells in mind [
11].
In conclusion, overexpression of MUC4 induces the HER2 level and enrichment of cancer stem cells in MUC4-transfected ovarian cancer cells. Circular colonies isolated from MUC4 overexpressed ovarian cancer cells show an increased expression of cancer stem cell specific markers (ALDH1and CD133) and the self-renewal maker (Shh). This suggests that MUC4 stabilizes HER2 and enriches the cancer stem cell population, by either a direct or indirect mechanism which is yet to be explored. Our study proves that MUC4 is not only expressed on mature cancer cells, but also on tumor cells that have multiple characteristics of stem/progenitor cells (Figure
5). This will help for the future application of a specific therapeutic target for cancer stem cells.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
All the authors in this manuscript have read and approve the final manuscript. PPM: Conception and design, collection and/or assembly of data, data analysis and interpretation, manuscript writing. PS.: Experimental help and data analysis. AV: Data analysis and manuscript writing. PD.: Experimental help and manuscript writing. SKB: Conception and design, financial support, data analysis and interpretation, manuscript writing, and final approval of manuscript.