Protoplast Transformation

From ActinoBase
The printable version is no longer supported and may have rendering errors. Please update your browser bookmarks and please use the default browser print function instead.

Materials

Instructions

  1. Follow the instruction in Protoplasts Formation, Regeneration and Transformation
  2. Add 3.85 ml P buffer to 1 g PEG sterilised.
  3. Add 200 µl PEG-P buffer mixture and a DNA solution to 50 µl of the protoplast suspension.
  4. Plate it onto R5 or R2YE.
  5. Incubate the plate at 28-30ºC overnight (typically 12-18 hours).
  6. Overlay 1 ml sterilised water containing nalidixic acid and an appropriate antibiotic.
Retrieved from ‘https://actinobase.org/index.php?title=Protoplast_Transformation&oldid=1623