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Yeast Transformation

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Yeast Transformation

 

 

  • inoculate 5-10 ml culture with single colony and grow ON
  • measure OD600nm and dilute to OD600nm = 0.3 in 50 ml
  • grow for 2-4 hrs
  • spin, wash cells with 25 ml H2 O
  • spin, resuspend in 2 ml 1 x LiAc/ 0.5 x TE
  • incubate at RT for 10 min
  • combine in tube: 100 µl cells, 10 µl salmon sperm DNA (10 mg/ml), up to 15 µl DNA to be transformed
  • add 700 µl 1 x LiAc / 1 x TE / 40 % PEG mix
  • incubate for 30 min at 30 °C (shaking or not shaking)
  • add 85 µl DMSO
  • heat shock at 42 °C for 7 min
  • spin, resuspend cells in 1 ml 1 x TE
  • spin, resuspend cells in 0.5 ml 1 x TE
  • plate 100 - 200 µl / plate and incubate at 30 °C

 


Buffers:

 10 x TE: 100 mM Tris pH 7.5; 10 mM EDTA.
 10 x LiAc: 1 M LiAc in H2 O; sterile filter.
 50 % PEG 3350: 50 % PEG 3350 in H2 O; sterile filter.

 

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