Cultivation of HEK293T cells

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Materials

Medium: DMEM + 10 % calf serum (CS), PBS, Trypsin / EDTA

Procedure:

  • Remove growth medium with sterile pasteur pipette from dishes
  • Wash 1x carefully with PBS, remove PBS
  • 1 ml Trypsin/EDTA on cells, short incubation (max 2 min)
  • If cells are detached, stop activity of trypsin with addition of 4 ml medium
  • Transfer cell solution in falcon tube, centrifugation 800rpm, 3 min, room temperature
  • Remove medium/ trypsin mixture, add new medium and mix
  • Optional - For assays with specific cell numbers:
    • count cells in Neubauer counting chamber or use CasyTT: add 25 μl of cell solution in Casy tube
    • add 5 ml of Casy Ton
    • measure cell number
  • For normal cultivation (two days) or transfection at next day: divide cells 1:5 in new dishes; for cultivation over weekend (three days): divide cells 1:10 in new dishes


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