Team:Lethbridge/Notebook/Planning

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Revision as of 01:43, 15 June 2010

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Work to be done:

Week of June 14/2010

Justin et al

Finish mms6-dT work

• Heat kill ligase
• take small sample for gel
• take another sample for restriction (cut out entire biobrick)
• Run gel of above
• Transform into DH5α

Test T4 DNA Ligase:

• Restrict rbs-xylE with EcoRI and SpeI (take sample for analysis on gel)
• Heat kill EcoRI and SpeI
• Ligate with T4 DNA Ligase
• Run unrestricted, restricted and ligated samples on a gel.

Prepare plasmid DNA for sequencing

Adam to upload guidelines for preparation.

Test PCR conditions for confirmation of ligation via PCR:

• Run a PCR of lumazine synthase gene that was sent for sequencing (and subsequently confirmed)
  • using VF2 and VR primers
• Run this PCR on a 2% agarose gel

PCR Confirm previous ligations

If (AND ONLY IF) PCR conditions amplified our known lumazine synthase gene, set up PCR of our previous ligation reactions to see if there is any ligated product.

Adam

• Finish VWR order (1000µL tips); test tubes; test tube racks; 96 well plates for sequencing, petri dishes
• Get RMA for VWR order (ie wrong test tube and test tube racks)
• Get guidelines for sequencing.
• Make primers for inserting mms6, xylE, lumazine, (C and N terminal labelled CFP/YFP-maybe) into pET28a expression vectors.No longer required.
• Order polymerase, SpeI, NotI, and (maybe, depending on results) T4 DNA ligase from Fermentas.
  • Check with HJ's lab to see which polymerase they use and from whom.
• Restrict lumazine, mms6, and xylE from BioBrick plasmid, and ligate into pET28a plasmid.
  • Check ligation and gel extract bands of proper size (Check for double insertion, plasmid self-ligation)
  • Transform into DH5α and purify plasmid DNA
  • Perform restriction analysis (using EcoRI and EcoRV) to check orientation of insert
  • Perform overexpression tests
  • Send for sequencing