Generating DMSO Stocks for Cell Culture
From Bridges Lab Protocols
Revision as of 18:34, 1 June 2018 by Elhabbal (Talk | contribs) (clarified some calculations, removed the isopropanol step)
Materials
- Cells in 10cm dishes, at 90-95% confluence.
- Cryopreservation Container (Nalgene 5100-0001)
- Cryopreservation Vials (Corning 430487)
- Sterile DMSO
Protocol
- Pick a low passage number of cells and grow 2-5 10cm dishes.
- At near confluence wash cells twice with PBS -/- and trypsinize normally.
- Collect all the cells in a 15 mL falcon tube. Add media up to 15 ml. (To avoid potentially over-trypsinizing, you can add media to each plate immediately after the cells detach, then add media up tot eh 15 ml mark on the falcon tube.)
- Centrifuge 5 min at 1500RPM to pellet cells.
- Aspirate media.
- Add media (1.8 mL per original plate, so if you started with 5 plates, the added media will be 5*1.8).
- Add sterile DMSO to a final concentration of 10% (0.2 mL per original plate, so if you started with 5 plates, the added DMSO will be 0.2*5).
- Gently resuspend cells and aliquot 1 mL of suspension into cryopreservation vials. (Resuspend with a pipette tip gently.)
- Label vials with name, date, cell type and passage (if known).
- Place container with vials at -80 for 1-3 days.
- Remove cells from container and place in liquid nitrogen storage.