Team:Paris Saclay/Notebook/July/9

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Notebook : July 9

Summary :

For regulation system :

  • extraction of BioBrick BBa_K1155000 in concentrated medium for further DNA sequencing.
  • the terminator BBa_B0010 in PSB1A2 plasmidwas extracted form iGEM plate kit 2013 and was transformed into competent cells and then was cultured on solid medium
  • the plasmid PSB3K3 was extracted form iGEM plate kit 2013 and transformed into competent cells and then was cultured on solid medium for confirmation

For sensor system:

  • A series of digestion, ligation were performed for BioBrick BphR2, BphR1, BphA1

Lab work

DNA purification

See protocol DNA purification Briobrick promoter BphR1, BphR2, BphA1 were purified.

Restriction digestion

We had 5 samples for digestion: 3 extracts, plasmid PSB1C3 and Plasmid PSB1K3(extracted from plate kit 2013 6F ).

For the plasmid (PSB1C3 and PSB1K3):

  • Plasmid : 4µl
  • (orange): 0.8µl
  • EcoR I: 0.5µl
  • PST I:0.5µl
  • H2O:2.2µl
  • Total:8µl

For the DNA extract:

  • DNA: 15µl
  • Buffer(orange): 3µl
  • EcoR I: 0.75µl
  • PST I:0.75µl
  • H2O:10.5µl
  • Total:30µl

After the digestion, superfluous enzyme was removed by Ethanol precipitation method. Then we suspended them with 10µl H2O.

Quantification

DNA concentration(ng/µl) 260/280
BphR2 24.2 1.97
BphA1 108.3 1.85
BphR1 97.9 1.82
PSB1C3 36.1 1.77
PSB3K3 19.4 1.77

Ligation

Common way for ligation.

  • Plasmid : 2µl
  • Bph : 2µl
  • Buffer : 2µl
  • T4 ligase : 12µl
  • H2O : about 7µl
  • Total : 20µl


Transformation

See protocol transformation terminator BBa_B0010 in PSB1A2 plasmid and plasmid PSB3K3was transformed into competent cells and then was cultured on solid medium.



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