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From 2008.igem.org

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The protocols we used

• LB medium preparation
• Plasmid resuspension from IGEM paper spots
• Transformation
• Plasmid extraction
• BioBrick digestion with restriction enzymes
• DNA gel extraction
• DNA precipitation with sodium acetate
• Antarctic Phosphatase
• Ligation
• PCR

LB medium preparation

(Estimated time: 10 min + 4 hours of autoclavation and cooling)

Materials needed:

• NaCl
• BactoTryptone
• Yeast extract
• ddH2O
• Agar
• Clean bottle or E-flask

• For a final volume of 1 l, put:
  • 10 g NaCl
  • 10 g BactoTryptone
  • 5 g Yeast extract
  • 15 g Agar (only for LB plates)
• into 1 l of ddH2O.
• Autoclave the solution.
• Let it cool to ~40-45°C
• Add the proper antibiotic if needed.
• ONLY FOR PLATES:
  • Pour an homogenous layer of agar LB into Petri plates under the hood.
  • Let agar LB polymerase.
• Cover and store at +4°C.
• Always check for contaminations before using!

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