Plasmid-Miniprep (Birnboim – Dooley protocol)

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Materials
Buffer P1: Solve 6.055 g Tris Base and 3.722g EDTA x 2H2O in 800 ml H20.

Adjust pH to 8.0 with 1M HCl, fill up to 1L. Per 1 ml buffer P1, add 100 µg RNase A. Store at 4°C.

Buffer P2: Solve 8.0 g NaOH in 950 ml H20. Add 50 ml 20% SDS. Store at RT.
Puffer P3: 294.45g KAc in 500 ml H2O. Adjust pH to 5.5 with glacial acetic acid (about 110 ml acid needed), fill up to 1L with H2O. Store at 4°C.
TE-Puffer 10 mM Tris/HCl pH 8.0; 1mM EDTA
Isopropanol
sterile dd H2O 70% Ethanol
For each clone Klon 2 x 1,5ml Eppendorf cups

Procedure

  • Resuspend completely bacterial pellet in 300µl P1 solution
  • Add 300 µl P2 and invert tube 10x
  • Add 300 µl P3 solution and invert tube 10x
  • Centrifuge 10 min at 4°C (12.000rpm)
  • Transfer 800 µl supernatant in a new tube and add 0.7 Vol. (560 µl) Isopropanol, invert 3x
  • Centrifuge 15 min at 4°C (12.000rpm)
  • Remove carefully supernatant and wash pellet with 0.5 ml 70% Ethanol
  • Centrifuge 5 min (14,000rpm), remove supernatant
  • Centrifuge pellet for additional 2 min at 14,000rpm
  • Dry the pellet at 37°C (~ 15 min)
  • Solve the pellet in 40 µl TE Puffer/ddH2O for at least 5 min
  • Analyse quantity of plasmid DNA preparation
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