Culture and Passage Cells

Culture and Passage Cells

From Powers Wiki

Culture and passage cells

ready to passage when cell confluence to 80% or 90% or when the cell density reaches an average of 2 X 105 cells/cm2

remove medium by aspiration

wash cells with PBS to remove the residual medium

add Trypsin-EDTA (enough to cover the flask surface)

incubate at 37oC for 5 minutes

observe by microscope to see cell death

add 2ml of medium trypsinization

pipet to detach all cells

transfer cell suspension to 15 ml tube

add cell culture medium to new flask

dilute as appropriate into the flask and mix well

a seeding density of 4.0 X 104 to 5.0 X 104 viable cells/cm2 is used when subculturing capan-1 cells

for T-75 use 3 x 106 cells, 100 mm Petri plate (57 cm2 surface area) use 2.3 X106 cells , 60 mm Petri plate (22.1 cm 2 surface area) use 8.8 X 10 5 cells.

incubate at 37oC

replace media 2-3 days

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Cell Culturing