Team:EPF-Lausanne/Notebook/August2011

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(Tuesday, 09 August 2011)
(Monday, 08 August 2011)
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A lot of colonies grew on the co-transformation plate; Alessandro will start a liquid culture the following day to test them in the plate-reader.
A lot of colonies grew on the co-transformation plate; Alessandro will start a liquid culture the following day to test them in the plate-reader.
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Vincent used the QuikChange Site-Directed Mutagenesis (SDM) Kit to try to produce TetR mutants. The pWhitescript 4.5-kb control plasmid provided by the Kit was used. The plasmid contains a stop codon (TAA) rather than a glutamine codon (CAA) in the beta-galactosidase gene of the pBluescript II SK(-) phagemid. When we transform the plasmid into XL10-gold ultracompetent cells, the resulting cells should look white on LB-ampicillin plates that have been treated with IPTG and X-gal, since the beta-galactosidase is no longer functional. However, if the mutagenesis works, there should be a point mutation that reverts the T into a C (TAA into CAA), meaning that the cells should appear blue on plates that contain IPTG and X-gal.
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The protocol for Mutant Strand Synthesis (provided with the Kit) was followed meticulously. Vincent made a master mix for 5 mutants and made a separate control mixture. The DNA template concentration was 130 ng/uL so we used .5 uL to get around 65 ngThe mutants were the following:
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* Y42F
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* V36F
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* P29Q-Y42M
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* P39Q-LV41
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* P39K
== Tuesday, 09 August 2011 ==
== Tuesday, 09 August 2011 ==

Revision as of 07:47, 10 August 2011