Competent cells

Principle

Bacteria can integrate DNA fragments from the environment. Escherichia coli, contrary to Bacillus subtillis, another bacteria frequently used in molecular and synthetic biology, is not naturally in a state of competence (able to integrate DNA fragments during transformation), that is why we have to prepare them.
Two methods can be used:
-Electrocompetent cells
-Chimiocompetent cells
We choose to use chimiocompetent cells

Preparation

Solutions preparation

Solution for 1M Cacl2:
Add 14,30g of CaCl2 into 100 ml desalted water

Solution for 0,1M Cacl2:
Add 50 mL of CaCl2 1M solution into 450 ml of desalted water

Solution for 0,1M Cacl2 + 15% glycerol:
Add 50 mL of CaCl2 1M solution and 75 mL of glycerol 100% into 450 ml of desalted water

Competent cells preparation

For 200 ml LB medium, add 400 µL of strain sample.
Let the bacteria grow until it reaches an OD between 0,3 and 0,35. Bacteria are more able to transform when they are in exponential phase
Once it reached the right OD, put the medium on ice for 30 minutes to slow down growth.
Split the 200 mL into 4x50 mL tubes then centrifuge at 3000 rpm for 5 minutes at 4°C and suppress supernatant afterwards.
Resuspend the pellet cells with 5 mL of Cacl2 at 0,1M for each 50 mL tube.
Again, put the medium on ice for 30 minutes.
Centrifuge at 3000 rpm for 5 minutes at 4°C then suppress supernatant.
Resuspend the cells with 1 mL of Cacl2 at 0,1M + 15% glycerol for each 50 mL tube.
Split the total 4 mL into 40 tubes containing each 100 µL of concentrated cell solution. This step should be executed fast enough and on ice.

Contamination and competence tests

Plate each strain on LB medium with Ampicillin, Kanamycin or Chloramphenicol in order to evaluate if it contaminated or not.
Plate each strain with a pSB1A3 plasmid (red colonies) and plated them on LB medium with Ampicillin only to evaluate wether our strains are competent or not.