IGEM:MIT/2006/Notebook/2006-6-30: Difference between revisions

Stationary Phase Promoter Stuff To Get Done

Two plates carrying the control to compare with the stationary phase promoter are in the 30 degree room. Remove them at the beginning of the day (really early if you don't want to come in on Saturday) and inoculate them in LB AMP liquid culture. Please remember to take them out. There is also a liquid culture labelled "control promoter" in the 37 degree room. I don't think it was growing yesterday, but you may want to check if it grew. If it grew, you still may want to make the LB AMP liquid culture from the fresh plates. If it didn't, I guess we have to make the liquid cultures from the 30 degree plates. If you guys feel ambitious and the liquid culture grew, you could start the fluorescent experiments (you can ask Barry to show you how it's done). Anyways, good luck, and have a great weekend!

Number of Transformants from 6/29 BSMT-BB Ligation/Transformation

We can make a few conclusions from these data:

• The old Top 10 cells are probably not suitable for use (despite colonies appearing at the 200μ plating volume).
• Barry's E0040 positive control worked.
• Our ligation was "succcessful", as colonies did appear on our plates.

SAMT PCR Product Eco/Pst Digest

1. We are cutting the SAMT pcr product (using EcoRI and PstI)--Began at 11AM
2. Total reaction volume is 50μL
3. the amount of dna desired is about 800 nanograms (it was 400ng last time, but Samantha said 1microg so we doubled.)
   • SAMT pcr product at 75.5 ng/μL -----add 11 μL
4. we are also going to use Dpn1 only in SAMT cut reaction to destroy dna that is not a pcr product (i.e. get rid of extra template)
5. SAMT pcr cleanup product cut reaction:
   • 31.5 μL water
   • 5 μL NEB buffer 2
   • .5 μL BSA
   • 11 μL BSMT pcr cleanup product (concentration = 50 ng/μL)
   • .75 μL Pst1
   • .75 μL EcoR1
   • .5 μL Dpn 1
6. Incubate tube in 37c room for 1-6 hours, then 20 mins at 80deg C to heat inactivate the enzyme, then 4deg forever. ---- and run a gel before moving on to ligation !!

Biosynthesis (meeting at 2 pm)

1. BAMT
   • Seems to be working in a few strains of bacteria (esp. Streptomyces maritimus)

• 1. Piel J, Hertweck C, Shipley PR, Hunt DM, Newman MS, and Moore BS. Cloning, sequencing and analysis of the enterocin biosynthesis gene cluster from the marine isolate 'Streptomyces maritimus': evidence for the derailment of an aromatic polyketide synthase. Chem Biol. 2000 Dec;7(12):943-55. DOI:10.1016/s1074-5521(00)00044-2 | PubMed ID:11137817 | HubMed [Piel00]

• 2. Moore BS, Hertweck C, Hopke JN, Izumikawa M, Kalaitzis JA, Nilsen G, O'Hare T, Piel J, Shipley PR, Xiang L, Austin MB, and Noel JP. Plant-like biosynthetic pathways in bacteria: from benzoic acid to chalcone. J Nat Prod. 2002 Dec;65(12):1956-62. DOI:10.1021/np020230m | PubMed ID:12502351 | HubMed [Moore02]

New BAMT PCR

• Total reaction volume of 50μL -- Began at 11:35AM
  • 1μL 1ng/μL BAMT template
  • 0.6μL of BAMTfor2 and BAMTrev primers (.6 μL of the 25μM primer yields roughly 300 nM final concentration of that primer, which is the goal)
  • 49 μL of Tom's PCR mix.
• Run the tubes on the thermocycler at: 95deg for 3:00, then cycle through: (a) 94deg for :30 (b) 55deg for :30 (c)68deg for 2:15, then 72deg for 10:00

Email requests to be done (kate)

1. Indole negative E. coli mutant strain 3714 (Di Martino) --- Kate ---- COMPLETE
2. Plasmid with pchA and pchB from Mauch (pmid #11169183)
3. Plasmid with pmsA, pmsB, pmsC, pmsE from Mercado-Blanco lab (in Switzerland).
4. Methylobacterium shuttle vector