Team:EPF-Lausanne/Notebook/July2011

From 2011.igem.org

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(Tuesday, 26 July 2011)
(Tuesday, 26 July 2011)
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Alessandro made PCR to amplify pSB3K1 backbone to use for a gibson assembly to make the Pconst-TetR plasmid. We can't do the assembly now since we are waiting for primers for TetR.
Alessandro made PCR to amplify pSB3K1 backbone to use for a gibson assembly to make the Pconst-TetR plasmid. We can't do the assembly now since we are waiting for primers for TetR.
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All the mutagenesis primers have been delivered, so Douglas diluted them. They are now all at 1 ug/ul concentrations, and need a further 1:10 or sodilution before being used for mutagenesis. He then ran a first mutagenesis on Alina's pF3A-tetR-GFP plasmid, introducing the following five mutations:
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All the mutagenesis primers have been delivered, so Douglas diluted them. They are now all at 1 ug/ul concentrations, and need a further 1:10 or sodilution before being used for mutagenesis. He then ran a first mutagenesis on Alina's pF3A-tetR-GFP plasmid, introducing the following five mutations, in addition to a control reaction:
# V36F
# V36F
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# P39Q_Y42M
# P39Q_Y42M
# P39Q_L41V
# P39Q_L41V
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The mutagenesis kit (remains from last year) was almost empty, so he made 10 ul instead of 50 ul reactions. There should be enough remaining reagents for one more batch, possibly with control, but hardly any more.
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A gel was run for the gradient PCR, that used HiFi enzyme. It gave no product! In conclusion, we shall wait for the Hifi+ Enzyme.
A gel was run for the gradient PCR, that used HiFi enzyme. It gave no product! In conclusion, we shall wait for the Hifi+ Enzyme.
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Revision as of 13:35, 26 July 2011