Team:BCCS-Bristol/Notebook/Week 4

From 2009.igem.org

Revision as of 11:38, 9 October 2009

• Home
• VESECURE
  • Wet lab
    • BioBricks
    • Notebook
    • Lab photos
    • Safety
  • Modelling
• BSim
  • Features
  • Tutorials
  • Download
  • Case studies
    • VESECURE
    • Magnetotaxis
    • Repressilators
• Bioscaffold
  • Fusion Problem
  • BCCS Bioscaffold
• Team
  • Calendar
  • Brainstorm
  • Preliminary meetings

Week 4

• One more try to get Fiu protein on pSB1A3 backbone. NovaBlue transformed with ligation products of pSB1A3 and Fiu.

• Grew colonies for FhuA and OsmE midi preps.

• Carried out midi preps for FhuA and OsmE ( [FhuA]=378.9 ng/ul, [OsmE]=113.2 ng/ul).

• Transformed Nova Blue with biobrick part BBa_B0014 (double terminator)

• Culture colonies of BBa_B0014 transformants to get ready for mini prep.

• PCR FhuA and GFP for assembling together a quick and dirty fusion to be ready prior to BioScaffold arrival.

• Carried out colony growth (agar & liquid) for the AraC promoter (2 parts BBa_R0080 (lacking O2 region) and BBa_R0081 (the O2 region).

• Miniprepped DNA from cultures of BBa_R0080 and R0081.

• Attempted a 2-way ligation and of the BBa_R0080 and R0081 parts. The final product should be a 2-component biobrick on a plasmid in 5'-R0081-R0080-3' direction which can be transformed into cells.

• R0081 part was purified by gel extraction after being treated by double digest. R0080 and R0081 were ligated together and used to transform NovaBlue cells.

• First attempt to make the AraC promoter from the two parts failed.

• Fiu still not being ligated on ANY backbone.

Standard 1kb NEB Ladder. Lanes 1-2 FhuA Midipreps, Lanes3-4 OsmE midipreps.

Standard 1kb NEB Ladder. Lanes 1-2 FhuA PCR fragment for Quick and Dirty assembly Method, Lanes3-4 GFP PCR fragments for quick and dirty assembly method.

• Recent changes
• What links here
• Related changes
• Special pages
• My preferences

• Printable version
• Permanent link
• Privacy policy
• Disclaimers