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Team:Groningen/protocols/Transformation
From 2013.igem.org
B. subtilis transformation
Losick protocol
-1 Day: Streak out strain and incubate 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 (more if culture is not really turbid).
3. Mix 400 µl of culture with DNA* in fresh tube (i.e. 15 ml tubes loosely closed – aeration)
(*usually 1 µl. Then 10 µl of Quiagen plasmid miniprep or <1 µl of chromosal prep)
4. Grow for an additional 2 hours at 37 °C.
5. Plate all on selective antibiotic plates, and incubates at 37°C o/n.
Sub1: Copmpetence medium (MC completed)
| H20 | 1,8 ml | |
| 10x MC (sub2) | 200 ul | filter sterilize |
| MgSO4 | 6,7 ul | autoclave sterilize |
| Tryptophan 1% | 10 ul | filter steralize, wrap in Al |
Sub2: MC 10x
| for | 100 ml | 10 ml |
| K2H PO4 | 14,036g | 1,4036g |
| KH2 PO4 | 5,239g | 0,5239g |
| Glucose | 20g | 2g |
| Tri-Na Citrate 300mM(Sub3) | 10ml | 1ml |
| Ferric NH4 citrate(Sub4) | 1ml | 0,1ml |
| Casein Hydrolysate | 1g | 0,1g |
| Potassium Glutamate | 2g | 0,2g |
Sub3: Tri-Na Citrate 300mM
| Tri-Na Citrate | 0,8823g |
| H2O | 10ml |
Sub4: Ferric NH4 citrate
| Ferric NH4 citrate | 0,22g |
| H2O | 10ml |
iGEM 2013 Groningen
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