Passaging A1 cell: Difference between revisions
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1 flask into 3 flasks and
2 flasks into 2 x 10 cm plates (for making myotubes)
HS AMEM (see additional protocol for recipe)
APBS ( 100 mls PBS + 25 mls water )
50 ml conical tube of 0.75% gelatin ( warmed to 37 degrees C )
0.05% Trypsin/EDTA ( 36 ml APBS + 4 ml 10x TE )
1x unplugged pasteur pipettes
20 ml pipettes
10 ml pipettes
3 large flasks-162 cm2
2 10 cm plates
3 conical tubes, 15 ml
1 scalpel no. 10
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<h3>Execution:</h3> | <h3>Execution:</h3> | ||
Prepare plates and flasks | |||
# score the 10 cm plates using the scalpel making 0.5 x 0.5 cm square grid across the plate. (This limits the size of the myotubes to a reasonable size) | # score the 10 cm plates using the scalpel making 0.5 x 0.5 cm square grid across the plate. (This limits the size of the myotubes to a reasonable size) | ||
# --put 10 mls gelatin into each black cap flask and coat the bottom of the flask | # --put 10 mls gelatin into each black cap flask and coat the bottom of the flask |
Revision as of 10:33, 2 July 2014
For passaging 3 flasks of A1 cells:
Materials :
Execution:
Prepare plates and flasks
- score the 10 cm plates using the scalpel making 0.5 x 0.5 cm square grid across the plate. (This limits the size of the myotubes to a reasonable size)
- --put 10 mls gelatin into each black cap flask and coat the bottom of the flask
--transfer the gelatin from the first flask into the second and coat, then the same procedure for the third flask
--then coat the 10 cm plates
Passage the cells
- aspirate media off of the flask containing the cells
- Rinse each black cap flask with 7 mls APBS
- aspirate off the APBS
- take 6 ml TE and put in flask
- wait until almost all cells come off
- stop with 3 mls HS AMEM in each flask
- mix with a pipette using the flow from pipette to detach any adherent cells
- put the cells into the 15 ml conical tube
- centrifuge ( spin 1000 rpm for 3 minutes )
- while you are waiting put 25 mls HS AMEM into each new flask and 10 mls into each 10 cm plate
- aspirate off the liquid in each conical tube
- flasks. use a pipette and resuspend cells in 6 mls HS MEM and put 2 mls of resuspension into each new flask! 10 cm plates: resuspend 2 flasks in 4 mls HS MEM and put 2 mls of resuspension into each 10 cm dish
- check cells in the microscope
- label with cell type, passage number , date and name
put cells in 25 °c and 2 % CO2 incubator