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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

This protocol describes the establishment of a three-dimensional (3D) ex vivo model of cancer cell-omentum interaction. The model provides a platform for elucidating pro-tumor mechanisms within the adipose niche and for testing novel therapies.

Abstract

Ovarian cancer is the deadliest gynecologic malignancy. The omentum plays a key role in providing a supportive microenvironment to metastatic ovarian cancer cells as well as immune modulatory signals that allow tumor tolerance. However, we have limited models that closely mimic the interaction between ovarian cancer cells and adipose-rich tissues. To further understand the cellular and molecular mechanisms by which the omentum provides a pro-tumoral microenvironment, we developed a unique 3D ex vivo model of cancer cell-omentum interaction. Using human omentum, we are able to grow ovarian cancer cells within this adipose-rich microenvironment and monitor the factors responsible for tumor growth and immune regulation. In addition to providing a platform for the study of this adipose-rich tumor microenvironment, the model provides an excellent platform for the development and evaluation of novel therapeutic approaches to target metastatic cancer cells in this niche. The proposed model is easy to generate, inexpensive, and applicable to translational investigations.

Introduction

Ovarian cancer is the deadliest gynecologic malignancy worldwide1. The lifetime risk of developing this cancer is approximately 1 in 70, with the median age of diagnosis at 63 years old2. Primary ovarian malignancies are classified histologically as either epithelial or non-epithelial. Epithelial ovarian cancers (EOC) represent over 90% of tumors, and the most common subtype is high-grade serous carcinoma (HGSC), which accounts for approximately 70%-80% of EOCs. Currently, there are no effective screening methods to detect disease early. So most patients are diagnosed at an advanced stage (i.e., FΓ©dΓ©ration Internationale de GynΓ©cologie et d'ObstΓ©trique [FIGO] stage III or IV) after the cancer has spread throughout the peritoneal cavity2.

Standard frontline treatment is cytoreductive surgery to remove all visible macroscopic disease, followed by adjuvant platinum-based chemotherapy to destroy any residual microscopic disease. While there have been many advances in ovarian cancer treatment over the last two decades, approximately 70% of patients with advanced disease will relapse within 3 years of treatment3. Given the overall poor prognosis of these patients, ongoing and future translational research efforts in EOC aim to identify biomarkers for early detection, prevent metastasis, improve current therapies to evade resistance and develop new personalized cancer treatments.

Generalized metastasis within the peritoneal cavity and its associated chemoresistance are two of the major limitations for the improvement of the treatment of patients with ovarian cancer4,5. The omentum, a fatty apron-like structure that hangs down from the stomach over the intestines, is a main site of ovarian cancer metastasis6,7. In addition to its function as a physical barrier, the omentum has been shown to have regenerative and angiogenic capacities and possess immune activities, which together promote vascularization, accelerate wound healing, and limit infection8. It contains a high concentration of stem cells that can differentiate into various cell types and can help repair damaged tissues. The omentum can become inflamed in response to injury or infection, which triggers the migration of immune cells to the site of injury9. These immune cells release growth factors and other molecules that help to promote the repair and regeneration of damaged tissue. Immune cells, such as macrophages, lymphocytes, and plasma cells, localized in the omentum are structures known as "milky spots", which are responsible for detecting and attacking pathogens and regulating peritoneal immunity. The omentum has also been shown to play a role in inducing immune tolerance10, which is the ability of the immune system to tolerate self-antigens and not attack healthy tissues. However, the same immune-related activities are also involved in pathological responses, such as the growth of omental tumors, metastasis, and escape of immune surveillance9,11. Previous studies from our lab and others have demonstrated a unique and active role of the adipose microenvironment in the inhibition of anti-tumoral immune responses and in the acquisition of chemoresistance12,13,14. Unfortunately, we have limited information on the cellular and molecular mechanisms by which the omentum provides a pro-tumoral microenvironment.

To better understand the interactions between cancer cells and the omentum, a 3D culture system consisting of human ovarian cancer cells and patient-derived omentum explants was developed. The protocol described here represents a novel ex vivo model of peritoneal carcinomatosis. This model mimics the natural progression of ovarian cancer tumorigenesis in this adipose-rich tissue. The proposed model is easy to generate, inexpensive, and potentially applicable to translational investigations in ovarian cancer research.

Protocol

The following research protocol was reviewed and approved by the Wayne State University Institutional Review Board (IRB). Informed consent was obtained from all patients prior to surgery. Figure 1 illustrates the three general steps in this protocol.

1. Preparation of human omentum tissue

  1. Prepare omentum culture media (DMEM/F12 + 10% fetal bovine serum + 1% penicillin-streptomycin) and store at 4 Β°C. Aliquot 30-40 mL of this media into a sterile 50 mL conical tube or surgical specimen container.
  2. Obtain surgical specimens from omental biopsy or omentectomy surgery. Immerse the sterile specimen in omentum culture media immediately after removal in the operating room. If the workflow does not allow this, place the specimen in omentum culture media as soon as possible. Transfer the sample by placing it on ice and store at 4 Β°C until processing.
    NOTE: The size of the omentum specimen removed will determine the amount of workable tissue.
  3. Process the omentum specimen within 1-2 h of collection using a laminar flow hood. Ensure that all materials and tools are sterile or sterilized.
  4. Remove the omentum from the collection container and transfer it into a 100 mm culture dish. Immerse the specimen in 1x phosphate-buffered saline (1x PBS) and gently wash the specimen to remove any blood clots or debris.
  5. Cut the tissue into pieces (0.5 cm x 0.5 cm or 100-200 mg; Figure 2A) using either small surgical scissors or a 10-15 mm scalpel. Use small surgical forceps to help manipulate the tissue and avoid crushing the omentum. If an energy device was used to surgically remove the omentum specimen, then avoid using the distorted tissue at the sealed edge.
  6. Place each piece of cut omentum into individual wells of a 24-well culture plate and fill the wells with 500 ΞΌL of omentum culture media or to a volume that is enough to cover the omentum without allowing the omentum piece to float above the well floor (Figure 2B).
  7. Store omentum pieces in fresh culture media at 4 Β°C until ready for injection.

2. Preparation of ovarian cancer cells

  1. Culture human ovarian cancer cells in a 75 cm2 culture flask at 37 Β°C and 5% CO2 to at least 75% confluency by the day of omentum collection.
    NOTE: This protocol utilizes mCherry-positive OCSC1-F2 human ovarian cancer cells previously described15,16,17,18. It can be modified to any cancer cell line tagged with a fluorescence signal.
  2. Prepare cells inside a laminar flow hood immediately after collection of the omentum specimen. Ensure that all materials and tools are sterile or sterilized.
  3. Add 10 mL of sterile 1x PBS to the culture flask and wash the cells by gently rocking the flask. Remove the 1x PBS and then add 3 mL of 0.05% Trypsin-EDTA.
  4. Gently rock the culture flask to coat all cells, and then place the flask in an incubator (37 Β°C and 5% CO2) for no more than 5 min. Tap the culture flask to completely detach the cells, and then neutralize trypsin by adding 3 mL of omentum culture media.
  5. Mix the cell suspension by pipetting, and then transfer the suspension into a 15 mL conical tube. Centrifuge the suspension for 5 min at 1,200 x g at 24 Β°C. Remove the supernatant and resuspend the cell pellet in 6 mL of fresh omentum culture media.
  6. Count the cells using a hemacytometer. Dilute the cell suspension to at least 100,000 cells per 100-200 ΞΌL of suspension. This is the volume of injection into each cut piece of omentum.
  7. Transfer an appropriate number of cells into a new culture flask to continue cell passage.

3. Injection of ovarian cancer cells

  1. Use a 1 mL syringe to draw up the cell suspension, then attach a 26-G needle. Do not draw up the cell suspension using the needle, as this can fragment the cells.
  2. Use small surgical forceps to pick up a piece of cut omentum. Transfer the omentum to a separate working sterile dish to facilitate injection. Gently pierce the omentum with the needle tip and inject a small volume of cell suspension into the tissue (Figure 2C).
  3. Repeat injection over several areas of omentum to a total volume of at least 100 ΞΌL or 100,000 cells. Note that much of the cell suspension may appear to pool around the specimen. If there is concern regarding the quality of the injection, then repeat the injection or inject a larger volume of cell suspension into the specimen.
  4. Return the injected omentum samples into each well of a 24-well culture plate. Take note that the volume of omentum culture media is to a level that covers the omentum without allowing it to float. Carefully handle the plate and place it inside an incubator (37 Β°C and 5% CO2).
  5. OPTIONAL: Use Matrigel (basement membrane matrix) to suspend omentum tissue in a solid matrix to allow easier injection and more concentrated cell suspension delivery.
    1. Thaw the basement membrane matrix at 4 Β°C and mix in 1:1 ratio with omentum culture media immediately prior to use. Store the basement membrane matrix mixture on ice or at 4 Β°C until injection. Fill empty wells with enough basement membrane matrix mixture to immerse a cut piece of omentum.
    2. Place specimens into the basement membrane matrix mixture and then place the 24 well culture plate in an incubator (37 Β°C and 5% CO2) for 20 min. Once the mixture has solidified, continue with injection as described above.
  6. Confirm successful injection using fluorescent imaging. Ensure a streak of fluorescent signal is visualized at the injection sites (Figure 2D). Note that the actual number of cells attached to the omentum after injection is unpredictable.

4. Co-culture of human omentum and ovarian cancer cells

  1. Change media every 48-72 h by adding 500-2000 ΞΌL of fresh omentum culture media. Do not pipet media directly on top of omentum tissue, as this may displace cancer cells. Note that if the media color turns to yellow, then change the media.
    NOTE: The frequency of media change will depend on the volume of media used and the trajectory of cancer cell growth. Once the cancer cells have seeded the omentum, whether or not the omentum piece is floating is no longer important.
  2. OPTIONAL: If a basement membrane matrix was used, the matrix would typically be dissolved by the time of the first media change.
  3. Monitor the growth of ovarian cancer tumors using fluorescent imaging. Frequency of imaging is at the discretion of the investigator. Anticipate evidence of small tumors by about 14 days (Figure 3A-C). Results may vary depending on the quality of the injection.
  4. Terminate the experiment based on the experiment endpoint.
    NOTE: Tumor growth and integrity of omentum tissue have been observed past 50 days.

Results

Successful establishment of ovarian cancer cells into omentum specimens was evident by about day 14 (Figure 3A-C). At least 24 replicates were prepared and injected per collected specimen to allow for further experimentation. Tumor growth was monitored by taking fluorescent images (Figure 3D,E). Images had to be carefully interpreted as a monolayer of cancer cells also grew at the bottom of each well that was no...

Discussion

Using this protocol, a preclinical model of peritoneal carcinomatosis for ovarian cancer was developed using a combination of basic in vitro and ex vivo techniques. A progressive tumor growth was observed across 50 days of co-culture after seeding omentum specimens with mCherry+ OCSC1-F2 human ovarian cancer cells. This method was developed and optimized across several experimental trials using different omentum specimens. Successful tumor growth depended on the quality of omentum, viability of cancer c...

Disclosures

The authors have nothing to disclose.

Acknowledgements

This study is funded in part by The Janet Burros Memorial Foundation. We acknowledge the patients and the Karmanos Cancer Institute Gynecologic Oncology Department for the collection of omentum samples. We also acknowledge the Biobank and Correlative Sciences Core at Karmanos Cancer Institute for coordination of patient recruitment and preparation of pathology slides. The Biobank and Correlative Sciences Core is supported in part by NIH Center grant P30 CA22453 to the Karmanos Cancer Institute at Wayne State University.

Materials

NameCompanyCatalog NumberComments
0.05% Trypsin-EDTA (1x)Gibco25300054
1 mL Insulin Syringe with 26 G detachable needleBD329652
10 mL Serological PipetsCELLTREAT229010B
100 mm Tissue Culture DishFisherbrandFB012924
15 mL Centrifuge TubeCELLTREAT229411
24 Well Cell Culture PlateCostar3524
50 mL Centrifuge TubeCELLTREAT229421
75 cm2 Tissue Culture FlaskCELLTREAT229341
Corning Cell CounterCorning9819000
Cytation 5 imagerBiotek
DMEM/F12 (1:1) (1x), +L-Glutamine, +2.438 g/L Sodium BicarbonateGibco11320033
Fetal Bovine Serum, QualifiedGibco1043028
MatrigelCorning356230Basement membrane matrix
No. 10 Stainless Steel Disposable ScalpelIntegra-Miltex4410
Penicillin StreptomycinGibco15140122
Phosphate Buffered Saline, pH 7.4 (1x)Gibco10010023
Revolve microscopeEcho

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