Enrichment for Chemoresistant Ovarian Cancer Stem Cells from Human Cell Lines

Summary

Cancer stem cells (CSCs) are implicated in tumor relapse due to chemoresistance. We have optimized a protocol for selection and expansion of CSCs from ovarian cancer cell lines. By treating cells with the chemotherapeutic cisplatin and culturing in a stem cell promoting media we enrich for non-adherent CSC cultures.

Abstract

Cancer stem cells (CSCs) are defined as a subset of slow cycling and undifferentiated cells that divide asymmetrically to generate highly proliferative, invasive, and chemoresistant tumor cells. Therefore, CSCs are an attractive population of cells to target therapeutically. CSCs are predicted to contribute to a number of types of malignancies including those in the blood, brain, lung, gastrointestinal tract, prostate, and ovary. Isolating and enriching a tumor cell population for CSCs will enable researchers to study the properties, genetics, and therapeutic response of CSCs. We generated a protocol that reproducibly enriches for ovarian cancer CSCs from ovarian cancer cell lines (SKOV3 and OVCA429). Cell lines are treated with 20 µM cisplatin for 3 days. Surviving cells are isolated and cultured in a serum-free stem cell media containing cytokines and growth factors. We demonstrate an enrichment of these purified CSCs by analyzing the isolated cells for known stem cell markers Oct4, Nanog, and Prom1 (CD133) and cell surface expression of CD177 and CD133. The CSCs exhibit increased chemoresistance. This method for isolation of CSCs is a useful tool for studying the role of CSCs in chemoresistance and tumor relapse.

Introduction

Resistance to chemotherapy is a major impediment to the treatment and cure of cancer. Ovarian cancer is the 5^th leading cause of cancer-related deaths among women in the United States (American Cancer Society Facts and Figures 2013). Patients initially respond well to chemotherapy, but most patients relapse¹. After relapse patients are treated with a variety of additional chemotherapy agents with very little benefit². General properties of CSCs include unlimited proliferative capabilities, retention of an undifferentiated state, resistance to drug treatment, efficient DNA repair, and ability to generate malignant tumor cells with different phenotypes³. CSCs frequently exhibit expression of stem cell genes such as Nanog, Oct4, Sox2, Nestin, CD133, and CD117. CSCs often express elevated levels of ABCG2, and ALDH genes that may contribute to drug efflux and metabolism^3,4.

The first definitive evidence for CSCs was demonstrated by isolating acute myeloid leukemia-initiating cells that were capable of self-renewal and tumor generation⁵. These leukemic stem cells expressed surface CD34 and generated leukemia in NOD/SCID (immunocompromised) mice⁵. Since then CSCs have been identified in many cancer types including leukemias/lymphomas, breast, bladder, colorectal, endometrial, sarcomas, hepatocellular carcinoma, melanomas, gliomas, ovarian, pancreatic, prostate, squamous cell carcinoma, and lung⁶. Therefore, being able to study this subtype of cancer cell is advantageous.

The goal of this study is to create a protocol for the selection and isolation of chemoresistant CSCs. Several methods have been reported for the isolation of CSCs from ovarian cancer cell lines. Non-adherent spheroids isolated from OVCAR-3, SKOV3, or HO8910 cultures demonstrate stem-like properties^7,8. Isolation of CD133+ cells from OVCAR-3 cultures also yields CSCs. CSCs have also been selected in culture by treatment with chemotherapeutic agents. Treating tumor cell lines (OVCA433, Hey, and SKOV3 cells) with cisplatin and paclitaxel allows for the expansion and isolation of CSCs^4,9. While culture of some cell types in CSC media leads to isolation of CSCs, SKOV3 cells did not survive culture in serum-free media or form sphere cells⁴. Therefore, treatment of cells with cisplatin and paclitaxel aided the expansion or isolation of this population⁴.

Using a modification of the procedure presented by Ma and colleagues⁴ we developed a method to isolate CSCs from the ovarian cancer cell lines. Our protocol is advantageous as it yields more viable cells while using less toxic chemotherapeutic agents. Cells are treated with cisplatin and subsequently grown in serum-free media supplemented with growth factors (stem cell media). We isolate the resulting non-adherent sphere cells and assay them for their expression of stem cell markers. This model enables the study of CSC properties and response to drug therapy.

Protocol

1. Cell Culture and Fluorescent Labeling of Ovarian Cancer Cell Lines

1. Prepare SKOV3 media: McCoy media supplemented with 10% fetal bovine serum (FBS), 0.1 mM L-glutamine, 50 U/ml penicillin, and 50 μg/ml streptomycin. Maintain OVCA429 cells in minimal essential media (MEM) supplemented with 10% FBS, 1 mM sodium pyruvate, 0.1 mM L-glutamine, 50 U/ml penicillin, and 50 μg/ml streptomycin.
2. Propagate SKOV3 and OVCA429 cell lines in a humidified incubator at 37 °C with 5% CO₂. Grow cells to 40-50% confluency.
3. Generate cells expressing red fluorescent protein (RFP) in order to monitor viability in vitro and in vivo.
   1. To generate SKOV3 cells expressing RFP, add lentiviral particles expressing RFP and 10 μg/ml polybrene to SKOV3 media in the absence of penicillin and streptomycin for 72 hr.
   2. After 72 hr, select for RFP positive cells by Fluorescence Activated Cell Sorting (FACS) as follows: Trypsinize RFP and non-RFP expressing cells, centrifuge at 125 x g for 5 min, resuspend cells at 10⁷ cells/ml in PBS containing 0.1% BSA. On a cell sorter, use non-RFP cells to determine the sorting parameters. Then collect cells that express high RFP using a 561 nm laser.
   3. Alternatively, if the lentiviral plasmid expresses an antibiotic resistance cassette, select for RFP expressing cells by culturing in the appropriate antibiotic (such as 10 mg/ml blasticidin). NOTE: The amount of lentiviral particles that needs to be used can vary by batch and by cell type. Proper lentiviral titer should be determined for each cell type.

2. Enrichment of Cancer Stem Cells

1. Treat SKOV3, SKOV3-RFP, or OVCA429 cell lines with 20 μM of cisplatin for 72 hr. CAUTION: Cisplatin is toxic. Use protective clothing/gloves and avoid contact with skin and mucus membranes. Do not dispose of cisplatin in wastewater.
2. Prepare CSC media: serum free DMEM/F12 media supplemented with 5 μg/ml insulin, 10 ng/ml human recombinant epidermal growth factor (EGF), 10 ng/ml basic fibroblast growth factor (bFGF), 12 ng/ml leukemia inhibitory factor, and 0.4% bovine serum albumin (BSA).
3. Trypsinize cells. Culture surviving cells in CSC media.
   NOTE: After 2 days in culture non-adherent spheroids will form.
4. Change media every 2 days by collecting media containing cells and centrifuging at 125 x g for 5 min. Then resuspend the pellet in fresh CSC media. Check cells for viability every 2 days by counting cells and performing trypan blue exclusion.
5. Then collect CSCs for further experiments by centrifuging 129 x g for 5 min and resuspending the pellet in phenol containing guanidinium thiocynate (RNA), phosphate buffered saline (PBS: 137 mM NaCl, 2.7 mM KCl, and 11.9 mM phosphate buffer, pH 7.4) with 0.1% BSA (for flow cytometry), or CSC media to continue culturing the cells.
6. Monitor CSC cell morphology using a light microscope at 20X and 40X magnifications.

3. CSC Characterization via Gene Expression Analysis for Stem Cell Markers

1. Collect 3 preparations of CSCs by collecting media containing cells, centrifuging at 129 x g for 5 min, and resuspending the pellet in a solution of phenol containing guanidinium thiocynate (other methods for RNA extraction may be used).
2. Prepare total RNA using TRIzol according to the manufacturer’s protocol. Synthesize complementary DNA (cDNA) from 0.1-1 µg of RNA using a commercially available cDNA Reverse Transcription kit.
3. Perform quantitative reverse transcribed polymerase chain reaction (QRT-PCR).
   1. Make up master mix for each set of primers containing QRT-PCR mix, primers, and water to total 8 µl per sample (primers with different fluorophores can be amplified in the same well). For example, generate one master mix for Oct4-FAM, Nanog-Hex, and GAPDH-CY5. Generate separate master mixes for Nestin and Prom1. Add 2 µl of cDNA template per sample.
      NOTE: For this study, QRT-PCR was performed using the primers listed in Table 1.
   2. Perform all QRT-PCR in duplicate for each sample using a real time PCR thermocycler capable of detecting multiple fluorophores. Include no template controls.
   3. Normalize stem cell gene expression to GAPDH expression for each sample using the ΔΔC_T method.

Oct-4-FAM	Primer 1: 5′-CCCAAGGAATAGTCTGTAGAAGTG-3′
	Primer 2: 5′-TGCATGAGTCAGTGAACAGG-3′
	FAM probe: 5′-CTTCCAAGC/ZEN/TGCCCACCTAACTTCT/3IABkFQ -3′
Nanog-HEX	Primer 1: 5′-CCTTCTGCGTCACACCATT-3′
	Primer 2: 5′-AACTCTCCAACATCCTGAACC-3′
	HEX probe: 5′-CTGCCACCT/ZEN.CTTAGATTTCATTCTCTGGT/3IABkFQ-3′
GAPDH-CY5	Primer 1: 5′-TGTAGTTGAGGTCAATGAAGGG-3′
	Primer 2: 5′-ACATCGCTCAGACACCATG-3′
	CY5 probe: 5′-AAGGTCGGAGTCAACGGATTTGGTC/3IABRQSP-3′
NESTIN-FAM	Primer 1: 5′-AGGACCTGAGCGATCTGG-3′
	Primer 2: 5′-CGTTGGAACAGAGGTTGGAG-3′
	FAM probe: 5′-AACTTTTCA/ZEN/GTAGCCCGCAGCC/3IABkFQ -3′
CD133-HEX	Primer 1: 5′-ACTCTCTCCAACAATCCATTCC-3′
	Primer 2: 5′-AAACAATTCACCAGCAACGAG-3′
	HEX probe: 5′-ACAATCACT/ZEN/GAGCACTCTATACCAAAGCG/3IABkFQ-3

Table 1. Primers used for CSC characterization by QRT-PCR.

4. Analyzing CSCs for Cell Surface Markers CD117 and CD133

1. Harvest CSCs by collecting media containing cells and centrifuging at 125 x g for 5 min. Add 500 µl of a non-proteolytic cell detachment solution to break-up cells. Centrifuge cells at 125 x g for 5 min to remove cell detachment solution. Then wash cells twice with cold PBS.
2. Incubate in normal growth media for 1 hr prior to labeling cells. Spin down cells for 5 min at 129 x g. Resuspend cells in PBS with 0.1% BSA with anti-CD133-PE and anti-CD117-FITC.
3. Fix cells overnight in 1% paraformaldehyde. Caution: Paraformaldehyde is toxic (suspected carcinogen). Make in fume hood and use within a week.
4. Perform flow cytometry to analyze CD117 (with an anti-CD117 conjugated to FITC) and CD133 (with anti-CD133 conjugated to PE) cell surface expression on a flow cytometer. Collect data on cells in the FL1 (for FITC) and FL3 (for PE) channels. Generate gates for cells expressing both FITC and PE. Generate a dot plot with 4 quadrants (FITC- and PE-, FITC+ PE-, FITC- PE+, and FITC+ and PE+) and determine the number of cells in each quadrant.

5. Analyzing CSCs for Therapeutic Response

1. Plate 5,000 cells per well (SKOV3, SKOV3-RFP, SKOV3 CSC and SKOV3-RFP CSCs) on 96-well plates overnight.
2. Treat with cisplatin (0, 1, 10, 100, and 1,000 µM) or paclitaxel (0, 0.01, 0.1, 1, 10, and 100 µM) for 96 hr.
3. Perform MTT (3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide) cell viability assay.
   1. Plate 5,000 cells per 100 µl per well on a 96-well plate (plate cells in duplicate and include media only control wells).
   2. After 24 hr, add 10 µl of 10 mg/ml MTT. Incubate at 37 °C for 2-4 hr (until precipitate forms).
   3. Add 100 µl of MTT solvent 4 mM HCl, 0.1% NP-40 in isopropanol. Incubate for 15 min in dark.
   4. Read plates at 570 nm on a plate reader.

Results

To demonstrate that we isolated CSCs from epithelial ovarian cancer cell lines using cisplatin treatment, we first acquired images of the cell lines prior to treatment and after selection. We used light microscopy to capture images of adherent (untreated) SKOV3 and OVCA429 cells and SKOV3 and OVCA429 CSCs (Figure 1). CSCs appear round and not attached to the tissue culture plates (Figures 1 and 2). We further show that SKOV3 cells transduced with RFP retain their fluores...

Discussion

CSCs that are resistant to therapy may be accountable for relapse after treatment of primary tumor. Characterization of CSCs may lead to improved therapies for ovarian cancer. The critical parameters in the establishment of chemoresistant CSCs using the above protocol are timing the length of treatment with chemotherapy and the concentration of chemotherapy. When using the protocol in Ma et al. it was found that after 7 days of treatment with cisplatin and paclitaxel, no viable cells remained⁴. By red...

Materials

Name	Company	Catalog Number	Comments
McCoy	Life Technologies	16600-108	Warm to 37 °C prior to use
DMEM / F12 serum free	Life Technologies	11320-033	Warm to 37 °C prior to use
Minimal Essential Media	Life Technologies	42360032	Warm to 37 °C prior to use
Sodium pyruvate	Life Technologies	11360070
Polybrene	Millipore	TR-1003-G
Blasticidin	Life Technologies	R21001
Fetal Bovine Serum	Atlas Biologicals	F-0500-A
Penicillin-streptomycin	Life Technologies	15070-063
Cisplatin	Sigma-Aldrich	T7402-5MG	Caution: Toxic. Use precautions
pLenti-suCMV-Rsv	Gentarget	LVP023	BSL2 approval needed
Insulin	Sigma-Aldrich	I-1882
Human Recombinant EGF	Cell Signaling Technology	8916LC
bFGF	BD biosciences	354060
LIF	Santa Cruz	sc-4988A
Bovine Serum Albumin	Roche	03 116 956 001
TRIzol	Life Technologies	15596-018
High Capacity cDNA Reverse Transcription Kit	Applied Biosystems	4368813
IQ Multiplex Powermix	BioRad	1725849
Accumax	Millipore
Primers	Integrated DNA Technology	individually designed and ordered (see protocol for sequnces)
Anti-CD133 PE	Milenyl	130-098-826	Primer/probe sets are light sensitive
CD117-Biotin	Miltenly	130-098-570
AntiBiotin-FITC	Miltenly	130-098-796
Paraformaldehyde	Sigma-Aldrich	P6148-1KG	Caution: Toxic. Always prepare in hood and make fresh.
Trypsin	Life Technologies	25300062
MTT (3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide)	Sigma-Aldrich	25200-072
EVOS Fl Epifluorescence and Transmitted Light Microscope	Advanced Microscopy Group
Biorad CFX96 C1000 System	Biorad
Beckman Coulter FC500 Flow Cytometer	Beckman Coulter
Spectramax 340PC384	Molecular Devices