Team:EPF-Lausanne/Notebook/August2011

From 2011.igem.org

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(Saturday, 27 August 2011)
(Monday, 29 August 2011)
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== Monday, 29 August 2011 ==
== Monday, 29 August 2011 ==
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Some brainstorming with Henrike on the topic of the failed IPTG platereader experiment made it clear to Vincent that he had been using the wrong colony plate to make his T7-lysis liquid cultures. Having cast light on a potentially crucial mistake, we then thought it would be a good idea to do another platereader experiment, this time with the BL21 cells and not DH5 alpha.
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Before getting to work on those new liquid cultures, Vincent made the premixed tubes for Microsynth sequencing of Nadine's colonies. Results should be coming in on Tuesday by email. Lilia and Vincent then had an interview with Stéphane of the BioSafety committee at the EPFL. His comments and insights will soon be finding their way to the wiki safety page.
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Henrike, Clara, and Matt helped Vincent mini-prep the 16 T7-RFP and T7-Lysis variants and measure the DNA concentration. They transformed and plated these and the T7-const-LYS, T7-lac-LYS, and T7-lac2-LYS into BL21 cells and also transformed and plated the pSB3K1 plasmid from Gibson assembly (negative control) into DH5 alpha. Vincent had not realized that the plasmid he Gibson-assembled did not have extensions and that there was no need to put this into DH5 alpha. Since Vincent made pSB3K1 extended for the next day's Gibson assemblies (of the remaining RFP and Lysis variants), this only put us behind by one day.
== Tuesday, 30 August 2011 ==
== Tuesday, 30 August 2011 ==

Revision as of 08:41, 30 August 2011