Transfection of HEK293T cells

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Materials
Plasmid DNA
2x HBS- buffer, pH 7.05 (correct pH is extremely critical !!)
2.5 M CaCl2 (sterile)
25 mM chloroquin (sterile)

Procedure:

  • 1 day before transfection: cells split 1:3 up to 1:5 in 10cm dishes
  • Next day: Set up for each 10cm dish: 500 μl ddH2O (sterile) in 14 ml PP Greiner tube
  • Add 5 μg (or adapted amounts) of plasmid DNA
  • Add 500 μl 2x HBS buffer, mix sample
  • Add drop-wise and during constant mixing on vortex 50 μl sterile CaCl2 to sample
  • Incubate for 5 min at room temperature to allow DNA/Ca2+ precipitate formation
  • During DNA/Ca2+ precipitate formation, add 10 μl of chloroquin to cells in 10 cm dish
  • Add drop-wise 1 ml of DNA/Ca2+ precipitate sample on cells in 10 cm dish (“carpet bombing”), be carefull not to detach cells
  • Incubate cells for 6- 8 h in incubator
  • Remove medium and add 8 ml/dish of fresh medium carefully onto cells
  • Expression of transgenes is usually highest on day 2 after the transfection
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