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pDR244 Cre Ts枯草芽孢杆菌无痕敲除(cre-lox敲除)载体质粒
Order ID | Name | Description |
Biovector-pDR244Cre | pDR244Cre-Ts | pDR244Cre-Ts, 15uL DNA. AmpR.Storage:-20℃ |
cre/lox-Mediated Loop-outProtocol for pDR244
(1)Transform pDR224 into one of the Bacillus subtilis BKE collection or any otherstrain harboring a
loxP-ankedantibiotic resistance cassette with selection for spectinomycin resistance at30°C
(2)Transfer several transformant colonies to plain LB plates and incubateovernight at 42°C
(3)Screen resulting colonies for plasmid curing (spectinomycin sensitivity) andthe antibiotic
resitancecassette (erythromycin sensitivity).
(4)Streak for fresh single colonies and then confirm loss of the cassette by PCR
Transformation of plasmid DNAto competent E. Coli cells
Thaw competent cells on ice. 20–200µL per tube
Add max. 1-3µL of plasmid
Mix very gently!
Incubate the tubes on ice for 30 min
Heat shock the cells for 45 sec to 2 min at 42°C
Place the tubes immediately on ice for at least 2 min
Add 800µL of SOC medium to each tube
Incubate for 1 hour at 37°C and shake vigorously
Spin down briefly and remove most supernatants
Resuspend cell pellet with the rest SOC medium in the tube by pipetting
Plate out the suspension on a LB agar plate containing the appropriate antibiotic. Incubate the plates overnight at 37°C
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