Overview
This protocol describes the technique of isolating fluorescently labeled T-cell acute lymphoblastic leukemia (T-ALL) tumor cells from an adult zebrafish and quantifying them using trypan blue dye.
Protocol
1. Collection of fluorescently labeled T-ALL cells from the primary tumor fish
- Prepare at least 20 mL of 10% heat-inactivated fetal bovine serum in 0.9x phosphate buffered saline (FBS/PBS).
- Add 1 mL of FBS/PBS to one vial of heparin sodium salt (300 units).
- Select fish bearing tumors in more than 50% of the body, or those fish having difficulty eating or swimming. Sacrifice the fish by overdosing them with tricaine or by ice water immersion. Confirm death by lack of gill movement and heartbeat.
- Use a razor blade to remove the head of the fish.
- Wash the cavity of the fish with the heparin solution to remove excess red blood cells.
- Using a pipette, inject 100 µL of heparin solution (Add 1 mL of FBS/PBS to one vial of heparin sodium salt) into the body cavity of the fish. Remove all liquid that spills out (it will contain blood cells) and pipette it into a 1.5 mL microcentrifuge tube.
- Use a fresh pipette tip to wash the body again. Perform at least three washes, or until the liquid that spills out appears free of blood.
- Discard all liquid from the washes in these steps, as it will not be used in further analyses.
- Collect the leukemia cells.
- Inject 100 µL of FBS/PBS into the body cavity of the fish.
- Apply gentle pressure to the outside of the body of the fish with the pipette tip to squeeze/push out the tumor cells.
NOTE: If this step is performed using a dissecting microscope, the tumor cells spilling out of the body cavity will be evident. - Collect the liquid and cells from each wash into a 1.5 mL microcentrifuge tube.
- Repeat steps 1.6.1-1.6.3 until most of the tumor cells are collected (usually 5-10 times). Collect all tumor cells into the same 1.5-mL microcentrifuge tube. Keep the cells at room temperature.
- Mix the collected tumor cells from previous step by gently pipetting them to dissociate the clumps of cells. Filter the cell suspension through a 40-µm mesh filter. Wash the filter 1-2 times with 100 µL of FBS/PBS. Keep the cells at room temperature.
- Mix 2 µL of cell suspension with 18 µL of trypan blue (0.4%, diluted 1:10 and filtered) in a new tube. Load 10 µL on a hemocytometer and count the number of live (non-blue) fluorescent cells to calculate the number of isolated tumor cells.
NOTE: Non-blue GFP-negative cells are likely normal, non-malignant T-cells and should not be counted. At least 2 x 106 cells are required to stain the cells with Hoechst 33342.
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Materials
| Name | Company | Catalog Number | Comments |
| Syngeneic zebrafish (CG2) | See Mizgireuv et al., 2006 | ||
| rag2:c-myc plasmid | Langenau Laboratory | ||
| rag2:GFP plasmid constructed in de Jong Lab | rag2 promoter from Langenau Laboratory | ||
| pCS2-transposase plasmid | Chien Laboratory | ||
| SteREO Discovery V8 Microscope | Carl Zeiss Microscopy | 495015-0008-000 | |
| Tricaine methanesulfonate (MS-222) | Western Chemical, Inc | Fisher Scientific - NC0342409 | 100 g |
| Fetal bovine serum (FBS) | HyClone Laboratories, Inc. | Fisher Scientific - SH3007103 | 500 mL |
| Phosphate-Buffered Saline (PBS) | Gibco by Life Technologies | 1001-023 | pH 7.4 (1x) - 500 mL |
| Heparin sodium salt | Sigma-Aldrich | 2106 | 15 - 300 unit vials |
| 40 µm mesh filter | Falcon Corning Brand | 352340 | Case of 50 |
| Trypan blue | Sigma Life Science | T8154 | 20 mL - Solution (0.4%) |
