Transformation of plasmid

 

Aim: To transform plasmid DNA to competent E. Coli cells

Material and Reagents

• LB medium

Ø  1% peptone

Ø  1% NaCl

Ø  0.5% Yeast Extract

• LB Agar plates with appropriate antibiotic.
• 1.5 mL microfuge tubes
• 42° C water bath
• Ice
• 37° C shaker 

Procedure:

1.      Take out the competent cells from -80⁰C freezer.

2.      Thaw competent cells (20–200µL per vial) on ice.

3.      Add max. 1 to 2µL of a target plasmid (Commercial).

4.      Mix very gently.

5.      Incubate the tubes on ice for 30 min

6.      Heat shocks the cells for 90 sec at 42°C

7.      Place the tubes immediately on ice for at least 2 min

8.      Add 1 mL of LB medium to each tube.

9.      Incubate for 1 hour at 37°C and shake vigorously

10.  Spin down briefly and remove most supernatants

11.  Resuspend cell pellet with the rest LB medium in the tube by pipetting

12.  Plate out the suspension on a LB agar plate containing the appropriate antibiotic.

13.  Incubate the plates overnight at 37°C.

 

 

Theory video: https://youtu.be/7Ul9RVYG5CM

Practical video: https://youtu.be/1PqWnu2uBrY

Reference: https://www.addgene.org/protocols/bacterial-transformation/

 

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