Team:Groningen/protocols/Transformation
From 2013.igem.org
B. subtilis transformation
The Losick protocol is used
Day 0: Streak out the Bacillus strain of use and plate this on an LB agar plate o/n at 37°C.Transformation (D-Day):
1. Pick up a nice big colony and drop it in 2 ml of completed MC (1x) (see sub1).
2. Grow at 37°C for 5 hours (longer if the culture is not really turbid).
3. Mix 400 µl of culture with DNA* in a fresh tube (i.e. 15 ml tubes loosely closed – aeration)
4. Grow the cells at 37°C for an additional 2 hours .
5. Spread the complete 400 µl reaction mix on selective antibiotic plates, and incubate at 37°C overnight.
(*usually 1 µl. Then 10 µl of Qiagen plasmid miniprep or <1 µl of chromosomal prep)
Sub1: Competence medium (MC completed)
compound | amount | treatment |
---|---|---|
MQ water | 1.8 ml | |
10x MC (Sub2) | 200 µl | filter sterilized |
MgSO4 | 6.7 µl | autoclaved |
Tryptophan 1% | 10 µl | filter sterilized (stored in aluminium foil) |
Sub2: MC 10x
compound | amount 10 ml | amount 100 ml |
---|---|---|
K2HPO4 | 1.40 g | 14.04 g |
KH2PO4 | 0.52 g | 5.24 g |
Glucose | 2 g | 20 g |
Tri-Na Citrate 300 mM (Sub3) |
1 ml | 10 ml |
Ferric NH4 citrate (Sub4) |
0.1 ml | 1 ml |
Casein Hydrolysate |
0.1 g | 1 g |
Potassium Glutamate | 0.2 g | 2 g |
Sub3: Tri-Na Citrate 300 mM
compound | amount |
---|---|
Tri-Na Citrate | 0.88 g |
MQ water | 10 ml |
Sub4: Ferric NH4 citrate
compound | amount |
---|---|
Ferric NH4 | 0.22 g |
MQ water | 10 ml |