Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Tuesday, 30 August 2011)
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Vincent received the sequences for Nadine's 3 colonies (J6 1 & 4 Plac-RFP, K1-TetR-LacI 9) but did not have time to analyze them.
Vincent received the sequences for Nadine's 3 colonies (J6 1 & 4 Plac-RFP, K1-TetR-LacI 9) but did not have time to analyze them.
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== Wednesday, August 31 2011 ==
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Vincent made new Gibson master mixes using TAQ ligase (there are now 12 tubes that can do 2 Gibsons each).
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Vincent ran a plateread er experiment with thoe three T7-lysis constructs (const / lac / lac2) and the various T7-RFP variants. It looks as though lysis was induced in at least one T7 system. Vincent made more liquid cultures of the T7-lysis systems and their variants for another platereader experiment on Thursday.
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Vdog also made a Gibson of J6 Plac-Lys and transformed it into BL21 cells (plated all 300 uL). He made another Gibson attempt at the elusive K1-Tet-Lac and transformed that into the DH5 alpha cells (plated 150 uL). He did not forget that one of the plates had ampicillin resistance and the other had kanamycin.
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Vincent also made a colony PCR of the remaining 5 (out of the 18) RFP variants in DH5 alpha. He chose different colonies from the plates to see if those would fare better.
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He also tried to clone the version of the psB3K1 backbone that does not have TetR (we think it's the one that's labelled 1:10 on the eppendorf top but we're not sure). He used the K1-extensino primers. Hopefully, these will be good for Gibsoning the remaining T7-Lysis variants into K1. It will also be used to make the negative control (co-transformed with RFP, eventually).

Revision as of 21:12, 31 August 2011