Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Thursday, 25 August 2011)
(Thursday, 25 August 2011)
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The sequencing results of the pSB3K1 TetR-LacI plasmid came. It seems that LacI got insterted correctly, but that TetR got lost... We'll try to send this plasmid again for sequencing with another primer to be sure. Also, a new Gibson assembly has been done.
The sequencing results of the pSB3K1 TetR-LacI plasmid came. It seems that LacI got insterted correctly, but that TetR got lost... We'll try to send this plasmid again for sequencing with another primer to be sure. Also, a new Gibson assembly has been done.
For the J61002 Plac-RFP plasmid, Nadine  forgot the cell cultures on the bench so the sequencing will have to wait over the week-end. Here again, a new Gibson assembly has been done, along with J61002-lysis.
For the J61002 Plac-RFP plasmid, Nadine  forgot the cell cultures on the bench so the sequencing will have to wait over the week-end. Here again, a new Gibson assembly has been done, along with J61002-lysis.
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Vincent made liquid cultures from the successful transformation of the K1-T7-Lysis into BL21 cells. Nadine was kind enough to purify all 18 of Vincent's T7-RFP variants, as well as the 4 T7-Lysis variants. In the same spirit, the C5-T7-Lysis plasmids were miniprepped and then transformed into the BL21 cells and plated.
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In order to continue with the production of T7 promoter variants, Vincent had to make more gene-specific Lysis (i.e. T4 Lysis with RBS upstream). For this, Vincent used the new Hifi+ enzyme that had been ordered the previous day. Since we were also running out of PCR primer mix, Vincent went ahead and made some more.
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Revision as of 15:21, 25 August 2011