BeNa Culture Collection
info@bncc.com
| Subculture procedure | 1. Dissolution: Upon receiving the plasmid Freeze dried pellet, add 20 μl sterile water to the bottom of the tube to dissolve the plasmid. Incubate at Room temperature for 1 min; 2. Mixing (Plasmid Adsorption): Mix 200 μl competent cells + 5–10 μl plasmid DNA thoroughly. Incubate on ice for 30 min; 3. Heat shock transformation: Incubate at 42°C for 90 seconds; 4. Shrink membrane wells: Ice bath for 2 minutes; 5. Repair culture: Add 800μl LB liquid medium to each tube; incubate at 37°C for 1 hour at 150 rpm; 6. Screening culture: Spread an appropriate volume (100 µl) of the revived cells onto LB plates with the corresponding antibiotic. Incubate plates upright for 30 min (ensure agar surface is dry), then invert and incubate for 12–16 hours until colonies appear. 7. Extraction: Transfer a single colony to LB liquid medium with the corresponding antibiotic, shake-incubate for 12-16 hours, and extract the plasmid as required for the experiment. |
| Growth conditions | LB + Ampicillin, 37°C, Cloning Strain BL21(DE3) |
| Storage conditions | 2-8°C |
| Safety level | 1 |
| Sharing mode | Public welfare sharing |
Quantitative strains of candida albicans
BNCC359899
Quantitative strains of pseudomonas aeruginosa
BNCC365156
Biochemical ldentification Kit for Escherichia coli
BNCC361455
Quality control samples of salmonella from sewage of medical institutions
BNCC362178
Biochemical ldentification Kit for Escherichia coli EHEC O157
BNCC364763
Standard quality control samples of enterococcus faecalis in drinking water
BNCC362540
- English
- Japanese