Team:EPF-Lausanne/Notebook/September2011

From 2011.igem.org

(Difference between revisions)
(Wednesday, 7 September 2011)
(Wednesday, 7 September 2011)
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[[File:EPFL_Igem_ligations1_0709.jpg|thumb|200px|first part of the colony PCR on T7 promoter variants biobricks]]
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[[File:EPFL_Igem_ligations2_0709.jpg|thumb|200px|second part of the colony PCR on T7 promoter variants biobricks]]
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Nadine made colony PCRs for the T7 promoter variants that Henrike cloned into the biobrick vector. The right insert should be ~450 bp long, but all the colonies show a fragment at 300 bp. Nevertheless, we have 5 colonies with the 450 insert. The low number of positive colonies correlates with the observation that the ligation negative control plate had about half as much colonies as the different ligations.
Nadine made colony PCRs for the T7 promoter variants that Henrike cloned into the biobrick vector. The right insert should be ~450 bp long, but all the colonies show a fragment at 300 bp. Nevertheless, we have 5 colonies with the 450 insert. The low number of positive colonies correlates with the observation that the ligation negative control plate had about half as much colonies as the different ligations.
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She also prepared some liquid cultures for tomorrow's platereader experiment.
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She also prepared some liquid cultures for tomorrow's platereader experiment, and miniprepped the pSB TetR-LacI plasmid before sending it for 2 new sequencing reactions.
Vdog made glycerol stocks and minipreps of the non-randomer RFP variants 6, 13, and 14 as well as Alina's T7-const-C2/C11, T7 lac 1, and T7 lac2 3.  
Vdog made glycerol stocks and minipreps of the non-randomer RFP variants 6, 13, and 14 as well as Alina's T7-const-C2/C11, T7 lac 1, and T7 lac2 3.  

Revision as of 11:32, 8 September 2011