DH5α (containing pBiT1.1-N [TK-LgBiT] plasmid) E. coli|359211 |BNCC

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Escherichia coli DH5α(pBiT1.1-N [TK-LgBiT])

Subculture procedure	① Prepare 1 vial of sterile water and 2 90mm resistant plates; ② Disinfect ampoule surface, open in safety cabinet, cauterize top with alcohol lamp, then immediately add sterile water to rupture; break ampoule with forceps; ③ Pipette 0.5 mL sterile water into lyophilized tube, dissolve completely, then spread solution onto antibiotic plates (200 μL/Agar plate); ④ Incubate the resistance plates under specified conditions for 18-24 hours before observation (do not seal or wrap plates); ⑤ Pick a single colony and inoculate into 50 mL LB resistance liquid medium; incubate overnight at 37°C on a shaking incubator; ⑥ Extract plasmids from an appropriate volume of the bacterial culture as required by the experiment;
Growth conditions	37°C; 18-24h; aerobic;
Storage conditions	2-8°C
Safety level	1
Sharing mode	Public welfare sharing

DH5α(containing pBiT1.1-N [TK-LgBiT] plasmid) Escherichia coli

Storage conditions : 2~8 ℃

No. :359209

Product format :freeze dried, 200ul

Validity : 6 years

Biosafety level : 1 , handle in ultra-clean table or safety cabinet

Receiving notice: if any abnormality is found on the day of receipt, please contact the customer service within 24 hours. If it is overdue, it is deemed that the bacteria are well. The freeze dried culture shall be used up once and shall not be retained. The bacterial viability will resume after 1-2 generation of recovery and can be used normally. Handling instructions of agar plate is enclosed. Please operate in strict accordance with this instruction, otherwise the replacement of bacteria are not be available in case of aberrant growth and loss of viability.

Host bacteria:BNCC353719 DH5α;.

Plasmid:BNCC357528 pBiT1.1-N [TK-LgBiT](containing chloramphenicol resistance gene).

Medium:resistant agar medium, yeast extract 5.0g, peptone 10.0g,NaCl 10.0g, agar 15.0g (not included in liquid medium), distilled water 1.0 L,pH 7.0. Sterilization at 121 ℃ for 15min. After sterilization, cooling and cooling, chloramphenicol was added to make the final content of chloramphenicol in the culture medium 50μg/mL。

Growth conditions: 37 ℃ aerobic 18-24h.

Recovery steps:

1. Prepare 1 sterile liquid test tube (including 5~10mL of culture medium) and 2 pieces of 90mm plate;

2. After disinfecting the surface of the ampoule tube, open it in the safety cabinet, burn the top with an alcohol lamp, quickly drop sterile water to break it, and then break it with tweezers;

3. suck 0.5mL of liquid culture medium and put it into the freeze-drying tube, fully dissolve it and return it to the liquid test tube again and mix well.

4. Draw the mixed solution from the test tube liquid to apply the flat plate, 200μL/piece;

5. Put all the test tubes and plates under the above specified conditions for cultivation. It is forbidden to seal and wind the plates. After 18-24 hours, observe the obvious turbidity of the culture medium and the growth of plate colonies or moss.

6. if the strain has not grown, it should continue to be cultured for 72h until a single colony or moss grows.

Plasmid purification:

1. pick a single colony and inoculate it into 50mL liquid LB resistance medium, and culture at 37 ℃ overnight;

2. according to the experimental requirements, absorb appropriate amount of bacterial liquid for plasmid extraction.

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