Passaging A1 cell: Difference between revisions

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Prepare plates and flasks
Prepare plates and flasks
# 1 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)
# 2 --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
  --transfer the gelatin from the first flask into the second and coat, then the same procedure for the third 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  
--then coat the 10 cm plates  
Passage the cells
Passage the cells
# 3 aspirate  media off of the flask containing the cells
# aspirate  media off of the flask containing the cells
# 4 Rinse  each black cap flask with 7 mls APBS
# 4 Rinse  each black cap flask with 7 mls APBS
# 5 aspirate off the APBS
# 5 aspirate off the APBS
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# 7 wait until almost all cells come off
# 7 wait until almost all cells come off
# 8 stop with 3 mls HS AMEM in each flask
# 8 stop with 3 mls HS AMEM in each flask
# 9 mix with a pipette using the flow from pipette to detach
# 9 mix with a pipette using the flow from pipette to detach any adherent cells
any adherent cells
# 10 put the cells into the 15 ml conical tube
# 10 put the cells into the 15 ml conical tube
# 11 centrifuge ( spin 1000 rpm for 3 minutes )
# 11 centrifuge ( spin 1000 rpm for 3 minutes )
# 12 while you are waiting put 25 mls HS AMEM into each new flask  
# 12 while you are waiting put 25 mls HS AMEM into each new flask and 10 mls into each 10 cm plate
and 10 mls into each 10 cm plate
# 13 aspirate off the liquid in each conical tube
# 13 aspirate off the liquid in each conical tube
# 14 flasks. use a pipette and resuspend cells in 6 mls HS MEM and put 2 mls of resuspension into each new flask!
# 14 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
 
10 cm plates: resuspend 2 flasks in 4 mls HS MEM and put 2 mls of resuspension into each 10 cm dish
# 15 check cells  in the microscope
# 15 check cells  in the microscope
# 16 label with cell type, passage number , date and name
# 16 label with cell type, passage number , date and name
put cells in 25 °c and 2 % CO2 incubator
put cells in 25 °c and 2 % CO2 incubator

Revision as of 09:07, 2 July 2014

For passaging 3 flasks of A1 cells:

  • 1 flask into 3 flasks and
  • 2 flasks into 2 x 10 cm plates (for making myotubes)

    Materials :

  • 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

    Execution:

    Prepare plates and flasks

    1. 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)
    2. --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

    1. aspirate media off of the flask containing the cells
    2. 4 Rinse each black cap flask with 7 mls APBS
    3. 5 aspirate off the APBS
    4. 6 take 6 ml TE and put in flask
    5. 7 wait until almost all cells come off
    6. 8 stop with 3 mls HS AMEM in each flask
    7. 9 mix with a pipette using the flow from pipette to detach any adherent cells
    8. 10 put the cells into the 15 ml conical tube
    9. 11 centrifuge ( spin 1000 rpm for 3 minutes )
    10. 12 while you are waiting put 25 mls HS AMEM into each new flask and 10 mls into each 10 cm plate
    11. 13 aspirate off the liquid in each conical tube
    12. 14 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
    13. 15 check cells in the microscope
    14. 16 label with cell type, passage number , date and name

    put cells in 25 °c and 2 % CO2 incubator