Team:Bielefeld-Germany/Labjournal/Molecular

From 2013.igem.org

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Revision as of 22:01, 27 September 2013



Protocols



Genetic Engineering

Whole Genome Isolation

  • For the isolation following kit has been used: Fermentas GeneJET™ Plasmid Miniprep Kit
    • Centrifuge 10 mL of over-night liquid culture
    • Resuspend pellet in 800 µL of resuspension solution
    • Ribolyse three times for 60 s with 6500 rpm (30 s break between every run, 400 mg beads)
    • Centrifuge 3 min at 10,000 rpm
    • Transfer 500 µL of supernatant into new 2 mL tube
    • Add 500 µL of lysis buffer, invert 4 - 6 times
    • Add 700 µL of neutralisation buffer, invert 4 - 6 times
    • Centrifuge 10 min at 12,000 rpm
    • Transfer 2 x 600 µL of supernatant into spin column (centrifuge down each time for 30 s at 12,000 rpm)
    • Two wash steps with 750 µL of washing buffer
    • Dry column
    • Elute in 75 µL of elution buffer


Generating electrocompetent cells

  • Material:
    • 550 mL LB-Medium
    • 1 L cooled bidest. H2O
    • 150 mL cooled 10 % glycerine
    • 10 pre-cooled 50 mL Falcons


  • Protocol:
    • Inoculate 2x3 mL LB with bacterial stock; incubate over night at 37 °C and 200 rpm
    • Inoculate 2x250 mL LB with the over night cultures in 1-litre-flask at 37 °C and 140 rpm
    • Incubate until OD600 0,4-0,6
    • Cool the culture 15-30 minutes on ice
    • Onwards all steps at 4°C
    • Divide the cultures into cooled 50 mL Falcons and centrifugate at 4000 rpm, 4 °C for 15 minutes, make sure to slowly accelerate and deccelerate
    • Discard supernatant
    • Resuspend pellet in 5 mL cooled bidest H2O (and don't get frustrated while doing it, keep shaking gently)
    • Pool two suspensions each, add bidest H2O up to 50 mL and centrifugate again (see centrifugation above)
    • Discard supernatant
    • Resuspend pellet in 5 mL cooled bidest H2O
    • Add bidest H2O up to 50 mL and centrifugate again (see centrifugation above)
    • Discard supernatant
    • Resuspend pellet in 5 mL cooled 10 % glycerine
    • Transfer suspensions in two 50 mL Falcons and centrifugate again (see centrifugation above)
    • Discard supernatant
    • Add volume of 10 % glycerine that is approximately equal to the volume of the pellet and resuspend
    • Divide cells in 100 μL aliquots and freeze in liquid N2 immediately
    • Store at -80 °C


Transformation via electroporation

  • Thaw 50 µL competent E.coli cells on ice, dilute with icecold 50 µL glycerine (10 %) if necessary
  • Add 0.5-5 µL plasmid to 50 µl electrocompetent cells
  • Store cells on ice for 1 minute
  • Electroporate at U = 2.5 kV, C = 25 µF, R = 400 Ώ
  • Transfer transformation reaction to 450 µL SOC-Medium and shake 1 h at 37 °C
  • Centrifuge 2 min at 2000 rpm and plate on selective LB-Medium
  • Incubate over night at 37 °C





Contents

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