[Pombelist] Question regarding thawing Bioneer library

Ian

• 25 September 2015 11:02

I am planning to start working with version 5 of the haploid Pombe deletion library from Bioneer and was wondering if anyone could provide a protocol of how to best bring up the strains from frozen glycerol stocks?

The library is a fresh copy from bioneer and I tried pinning directly onto YES agar + G418 using a Singer rotor HDA. Unfortunately, many of the strains did not grow (approximately 10%). I have been suggested to first pin to YES plates without selection before replicating onto YES + G418 for selection, but thought it would be best to ask here first.

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  Ian

  • 25 September 2015 11:02

  This is a common problem. The plates have round bottom wells and cells are mostly sedimented. What helps is:
  1. Set the rotor to 2d source mix without distance clearance between pin and bottom of well. Repeat pinning 3 times. I normally leave plates to dry and re-pin.
  2. Using a plate incubator/shaker gently twirl the plates so cells detach from bottom. Do 3d source mix and do repeated pinning.
  3. In case the results are very poor, work with batches of 3-4 plates, using a multipipette very gently bring the cells in solution. Then do 3d source mix and repeated pinning.
  I always use YES+G418.

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