Freezing of mouse embryonic fibroblasts (MEFs) for hPSC cultures

Wash the plates twice with DPBS

Add Trypsin (5 ml for 15-cm plate) and incubate for 0h 5m 0s (37°C; 5% CO2)

Add 10 ml MEF medium to neutralize the Trypsin and collect the solution into a conical tube.

MEF medium

A	B
DMEM	435 ml
FB Essence/FBS*	75 ml
200mM L-Glutamine	5 ml
Penicillin & Streptomycin (100x)	5 ml
MEM Non-Essential Amino Acids	5 ml

*We have successfully used either FB Essence or FBS and have not observed an obvious difference. Final volume: 500ml

Centrifuge the cell suspension at 250x g

Discard supernatant, and re-suspend the cells in MEF Freezing Medium I at a concentration 2X the desired final freezing concentration (Freezing concentration will vary with MEF usage.)

MEF Freezing Medium I

A	B
FB Essence/FBS*	5 ml
MEF medium	5 ml

*We have successfully used either FB Essence or FBS and have not observed an obvious difference. Final volume: 10ml

While swirling, slowly and drop-wise, add an equal volume of MEF Freezing Medium II to the cell suspension.

MEF Freezing Medium II

A	B
FB Essence/FBS*	8 ml
DMSO	2 ml

*We have successfully used either FB Essence or FBS and have not observed an obvious difference. Final volume: 10ml

Dispense cell mixture into pre-labeled cryovials (10x10⁶) including type of cells, passage number, date frozen, and who handled cells.

Place cryovials into Styrofoam microtube freezer box or NALGENE™ Cryo 1°C Freezing Container pre-filled with 250 ml room temperature isopropanol.(This ensures that a -1°C/min rate of cooling is achieved, which is critical to cell viability.)

Freeze at -80°C

For long term storage, store cryovials in liquid nitrogen (-196ºC).