Team:EPF-Lausanne/Notebook/August2011

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The Gibson-transformed cells yielded a lot of mutants, with significantly more on the Gibson plates than on the negative controls ones. One strange thing with the J61002 Plac-RFP: the negative control  cells were weakly red fluorescent, while for the Gibson assembly some of the cells were expressing RFP. We'll see the results of the colony PCR tomorrow, but it's possible that the cells are autofluorescent...
The Gibson-transformed cells yielded a lot of mutants, with significantly more on the Gibson plates than on the negative controls ones. One strange thing with the J61002 Plac-RFP: the negative control  cells were weakly red fluorescent, while for the Gibson assembly some of the cells were expressing RFP. We'll see the results of the colony PCR tomorrow, but it's possible that the cells are autofluorescent...
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== Wednesday, 24 August 2011 ==
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Nadine ran the colony PCRs on a gel and got strange results.
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* For J61002 Plac-RFP, the negative control cells are definitely red - although they should not contain RFP -  and the colony PCR that includes a primer on RFP is positive. The colonies 8-10 were still white on the plate, but here again the colony PCR is positive. Perhaps this comes from the template plasmid used for the PCR (J61002 Ptet_EFP); since the miniprep failed we have to wait before sending the samples for sequencing.
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* For pSB3K1 Pconst-TetR Ptet-LacI, we also have positive results for the negative control. Here it's unlikely that it can be because of the template plasmid for the PCR, because be used the repressilator that has ampicillin resistance when the plates contained kanamycin. We'll see tomorrow the results of the sequencing of colony 7.
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Preparing for the next Gibson assemblies, Nadine also ran two PCRs:
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* One for amplifying the lysis cassette and putting it into J61002 backbone (with a new primer)
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* One for amplifying LacI and put it into J61002 Plac-RFP or Plac-lysis, once we'll have them.
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Revision as of 14:48, 24 August 2011