Team:EPF-Lausanne/Our Project/T7 promoter variants/selection

From 2011.igem.org

(Difference between revisions)
(Experimental Setup)
(Experimental Setup)
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To that end, we again set up an experiment involving two flasks but this time each flask contains two types of cells. For one flask, one culture is a co-transformation of a lysis plasmid and a RFP-containing plasmid and the other is a co-transformation of a negative control plasmid with a GFP-containing plasmid. In the other flask, the reverse is true: lysis is with GFP and negative control is with RFP. This co-culture experiment was prepared by mixing equal amounts of cells from an overnight culture in one big flask. After a 1h culture, we induced lysis with 500 µM IPTG.
To that end, we again set up an experiment involving two flasks but this time each flask contains two types of cells. For one flask, one culture is a co-transformation of a lysis plasmid and a RFP-containing plasmid and the other is a co-transformation of a negative control plasmid with a GFP-containing plasmid. In the other flask, the reverse is true: lysis is with GFP and negative control is with RFP. This co-culture experiment was prepared by mixing equal amounts of cells from an overnight culture in one big flask. After a 1h culture, we induced lysis with 500 µM IPTG.
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[[File:multiple_lysis_setup.png|300px|left]]
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[[File:multiple_lysis_setup.png|330px|left]]
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[[File:double_cultured_induced_iptg.png|300px|right]]
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[[File:double_culture_induced_iptg.png|330px|right]]
=== Results ===
=== Results ===

Revision as of 15:38, 21 September 2011