From 2007.igem.org

What to do ?

• Remove the plate of the transduction experiment and the transformation ones from the 37°C incubator (Upper-left shelf): If it has worked and if someones comes on Sunday:
  • isolation of the clones from the transduction on petri-dishes (LB+DAP+Erm+Citrate)
  • LB + antibio culture of the transformants (to make a glycerol stock and to do MiniPreps)

• Make a gel (0.8%) and migrate the PCR products
• Purify them
• Do the assembly PCR

If enough time (we can also wait to have the plasmids to do everything at the same time):

• Digestion of the purifications products with appropriate enzymes
• Purification