"
Team:Grenoble/Biology/Protocols/Double
From 2012.igem.org
Revision as of 02:37, 27 September 2012 by Adeline millet (Talk | contribs)
Double mutant construction
Goal
Obtain double gene knockout mutant strains of E. coli from single mutant strains. (Keio collection)Protocol
From the single mutant strains ΔcyaA, the first step was to remove the Kan cassette in order to create the recipient strain. [1]The second step is using the P1 bacteriophage to transfer a Kan cassette from another bacteria to this recipient strain [2], in order to replace the second gene. The phage is grown on a strain containing the Kan cassette (ΔaraC or ΔenvZ), and the resulting phage lysate, wich contains phage DNA and bacterial DNA, is used to infect the recipient strain. Genetic recombination, catalyzed by enzymes of the recipient strain, incorporates the Kan cassette into the recipient chromosome.
