Cell Freezing
Reagents / Solutions
- Cells! (at least 5 x 106).
- Foetal calf serum (FCS), heat inactivated at 65 癈 for 1 hr.
- Dimethylsulfoxide (DMSO).
- Freezing vials.
- Hi - Tech Cell freezer (polystyrene box wadded with cotton wool [!]).
- Liquid nitrogen bank.
Protocol
- Spin down cells, remove and discard the supernatant.
- Resuspend the cells at 5 x 106 per ml in FCS.
- Add DMSO to 10% (by volume) dropwise, agitating gently after each drop. Do this slowly.
- Place 1ml aliquots into the vials. Remember to label the vials precisely.
- Put vials into central positions of a polystyrene rack (from e.g. Boehringer Enzyme Storage box), and place that rack into an expanded polystyrene box (e.g. 'Eprack' as supplied by Scotlab) which is wadded with cotton wool.
- Place lid on box and seal in place with tape.
- Place box in the vapour phase of the liquid nitrogen bank. It must not be placed in the liquid phase. Leave for more than 4 hrs to freeze.
- Remove vials from box and place in liquid phase in the cell bank.
- Test the efficiency of the freezing procedure by thawing (method) and growing on one vial.
If the cells were healthy (> 95% viable) at the start of this procedure, then we obtain a culture 80-90% viable 24 hours after thawing and growing on (method) the test vial from point 9.
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