1. Preculture for competent Bacillus subtilis
Aim:Preparation for mainculture the next day
5 mL of LB were inoculated with Bacillus WT3610 from an LB plate and incubated at 37°C overnight.
2. Transformation of competent Bacillus subtilis
Aim: transformation of plasmid into Bacillus subtilis WT3610
100 µL of overnight culture were added to 10 mL of MNGE-Medium and incubated till an OD of 1,1-1,3 at 37°C which could take 4-5h.4
After reaching OD of 1,1-1,3 400 µL of the culture were transformed with 1,5 µg plasmid. After 1h incubation at 37°C 100 µL Expression mix were added and incubated for 1h as well.
In the end the 500 µL attempt was plated out on MLS-X-Gal plates and incubated at 30 °C overnight until colonies could be seen.
3. Overnight culture of blue clones
Aim: transformation of plasmid into Bacillus subtilis WT3610
Colonies were grown on the plates with transformed plasmid. The blue/ white screening showed positive transformed blue clones. 3 clones of different morphology per plate were picked and used for inoculation of LB-MLS (4 mL LB, 4 µL Lincomycin, 4 µL Erythromycin). Incubation was carried out overnight at 30°C with the cultures.
4. First temperature shift
Aim: integration of pMAD-Insert into Bacillus chromosome via flanks
The overnight cultures were used to inoculate 10 mL LB MLS until the culture obtained an OD of 0,1. The cultures were incubated at 30°C for 2h.
Then the temperature was shifted to 42°C for 6h.
After the heat shock dilutions from 10-4 to 10-6 of each culture were plated out on MLS-X-Gal so that plates could be incubated overnight at 42°C.
5. Second temperature shift
Aim: flip out of the pMAD backbone
One blue colony per diluted clone was used to inoculate 4 mL LB. The cultures were incubated at 30°C for 6h and afterwards for 3h at 42°C.
Dilutions from 10-4 to 10-6 were plated out on X-Gal plates WITHOUT MLS selection. The positive clones should not contain the resistance inside the backbone as well as the galactosidase. The plates were incubated at 42°C overnight.
6.1 selection of positive clones
Aim: checking the correct flip out of the pMAD backbone
From the dilution plates was one WHITE clone picked and transferred on a Master X-Gal Plate as well as on a MLS plate so that clones were proven for the right integration of the insert although flipping out the pMAD backbone.
The plates were incubated at 42°C overnight.
6.2 selection of positive clones
Aim: checking the correct flip out of the pMAD backbone
The white colonies grew on the X-Gal Master plates but not on MLS plates so the transformation seemed to be successful. The Backbone with the MLS resistance flipped out of the genome.
7. cPCR with checked clones
Aim: checking integration of constructs Hag-Spe and Hag-Spe-DARPin into B. s. genome
No clone was growing on MLS plates so the picked clones seemed to be positive. In order to check the correct integration of the domain constructs a cPCR with the picked clones on the X-Gal plates was done. The picked B.s. clones were cooked in 10 µL PBS for 5 min at 95°C.