CTC Isolation from a Whole Blood Sample: A Method to Obtain CTCs from Murine Colorectal Cancer Model
Abstract
Source: Kochall, S., et al. Isolation of Circulating Tumor Cells in an Orthotopic Mouse Model of Colorectal Cancer. J. Vis. Exp. (2017).
This video describes a detailed protocol for isolating circulating tumor cells from the whole blood sample of a euthanized colorectal tumor mouse model. These isolated CTCs can be cultured and used for intended downstream analysis.
Protocol
All procedures involving animals have been reviewed by the local institutional animal care committee and the JoVE veterinary review board.
1. Isolation of Circulating Tumor Cells from Whole Blood Samples
NOTE: Obtain blood by transcutaneous cardiac puncture on anesthetized mice, followed by euthanasia. Ideally, 1,000 µL of blood are drawn into a syringe prefilled with 100 µL of an anticoagulant (Ethylenediaminetetraacetic acid (EDTA) or heparin). Use an anti-human-EpCAM (epithelial cell adhesion molecule) antibody to identify the CTCs. This works very well if human epithelial cell lines are used in the mouse model. For other applications, different antibodies may be required.
- CTC enrichment:
- Prefill 15 mL tubes with 5 mL density gradient medium and carefully transfer the blood into the 15 mL tube.
- Centrifuge (30 min at 300 x g without brake) and carefully remove the upper supernatant.
- Pour the rest into a new 15 mL tube and centrifuge (15 min, 300 x g with brake).
- Recover the interphase containing the mononuclear cells (discard the rest) and wash the cells twice with PBS.
- Resuspend the pellet in 200 µL PBS/1% EDTA and add 4 µL of EpCAM antibody. Incubate 20 min on ice in the dark.
- Screening and picking
- Prepare the following buffer (in the following referred to as picking buffer): PBS + 10% fetal calf serum (FCS) + 1% Penicillin/Streptomycin (1%) + 0.8% EDTA.
- Use a PAP pen to draw a ~1 cm circle in a 6 cm sterile Petri dish (prevents the fluid from dispersing in the dish), and pipet 700 µL of picking buffer into this circle.
- Add 50 µL of cell suspension to the 700 µL picking buffer within the circle. Check the density of cells with the microscope. Split the sample into different dishes if it is too dense.
- Wait for the cells to settle down (~5 min).
- Screen the drop of cell suspension for stained (= EpCAM-positive) cells.
- Once a cell is found, pick the cell with the micromanipulator and put it in a 50 µL buffer depending on the intended downstream analysis (e.g., RNA extraction buffer or culturing medium).
- Depending on the intended downstream analyses, isolate EpCAM-negative cells and/or medium as negative controls.
- Proceed with downstream analyses (e.g., cell culture, PCR).
Offenlegungen
The authors have nothing to disclose.
Materials
| Density gradient medium – Ficoll | StemCell – Lymphoprep | 7801 | |
| Alexa Fluor 488 anti-human CD326 (EpCAM) Antibody clone 9C4 | BioLegend | 324210 | |
| Alexa Fluor 488 anti-mouse CD326 (EpCAM) Antibody clone G8.8 | BioLegend | 118210 | |
| Petri Dish, ø 60 x 15 mm, 21 cm², Vent | Greiner bio-one | 628102 | |
| Fluorescence Cell Culture Microscope | Leica | ||
| Transferman 4r Micromanipulator | Eppendorf | ||
| CellTram Air | Eppendorf | aspiration pump connected to the micromanipulator | |
| Dmz Universal Microelectrode Puller | Dagan Corporation | required for the manufacturing of micro capillaries for single cell aspiration | |
| Prism Glass Capillaries | Dagan Corporation | ||
| PAP pen | Abcam | ||
| Dulbecco's Phosphate Buffered Saline | Life Technologies GmbH | 14190169 | picking buffer |
| Fetal Calf Serum (FCS) | BIOCHROM AG | S 0115 | picking buffer |
| Penicillin/Streptomycin (PenStrep) | Life Technologies GmbH | 15140122 | picking buffer |
| EDTA | Roth | 8040.1 | picking buffer |
| Immunohistochemistry | |||
| Purified anti-human CD326 (EpCAM) antibody clone 9C4 | BioLegend | 324201 | EpCAM immunohistochemistry |
| HRP rabbit anti-mouse IgG | Abcam | ab97046 | EpCAM immunohistochemistry |
