Transformation of plasmids in E. coli

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Revision as of 08:39, 2 June 2025 by ESO wikiadmin (talk | contribs) (Created page with " == Procedure == * Before transformation, appropriate aliquots of competent bacteria should be thawn on ice. * Add the plasmid DNA to 100 μl competent E. coli in a snap-cap tube and mix well. * Incubate the samples 30 min on ice. * Transfer samples for 75 seconds to a 42°C water bath or heating block and quickly back on ice. * Add 1 ml LB-Medium and incubate the bacteria for 1h at 37°C (220 rpm). * Transfer the bacterial suspension from the snap-cap tube to Eppendorf...")
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Procedure

  • Before transformation, appropriate aliquots of competent bacteria should be thawn on ice.
  • Add the plasmid DNA to 100 μl competent E. coli in a snap-cap tube and mix well.
  • Incubate the samples 30 min on ice.
  • Transfer samples for 75 seconds to a 42°C water bath or heating block and quickly back on ice.
  • Add 1 ml LB-Medium and incubate the bacteria for 1h at 37°C (220 rpm).
  • Transfer the bacterial suspension from the snap-cap tube to Eppendorf-cups, centrifuge at 2500 rpm for 2 min, discard ~900 μl, resuspend the bacterial pellet in the remaining 100 μl, and spread the bacterial suspension with a Drigalski-spatula onto LB agar plates containing appropriate antibiotic for selection.
  • Incubate the plates with the lid down in the incubator o/n at 37°C
  • For E.coli BL-21, there might be only few colonies as transformation efficiency is regularly low.
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