Team:EPF-Lausanne/Our Project/Reporter Systems

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Our overall strategy to develop new transcription factors includes an ''in vivo'' characterization of the affinity and specificity of our TetR mutants. To that end, we set up two reporter systems based on RFP fluorescence.
Our overall strategy to develop new transcription factors includes an ''in vivo'' characterization of the affinity and specificity of our TetR mutants. To that end, we set up two reporter systems based on RFP fluorescence.
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The first reporter system consists of a TetR-RFP cascade. It has been successfully used to characterize some TetR mutants. Our second reporter system is a longer cascade, comprising TetR, LacI and RFP. Whereas in the first system RFP is expressed in the '''absence''' of a TetR-Ptet interaction, in the second one, the TetR-Ptet interaction directly induces RFP expression.
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The first reporter system consists of a TetR-RFP cascade. It has been successfully used to characterize some TetR mutants. Our second reporter system is a longer cascade, made up of TetR, LacI and RFP. Whereas in the first system RFP is expressed in the '''absence''' of a TetR-Ptet interaction, in the second one, the TetR-Ptet interaction directly induces RFP expression.
The affinity of each mutant can be deduced from the RFP expression profiles it induces in our reporter system. The specificity can be assessed by coupling each mutant to different Ptet sequences.
The affinity of each mutant can be deduced from the RFP expression profiles it induces in our reporter system. The specificity can be assessed by coupling each mutant to different Ptet sequences.

Revision as of 03:11, 22 September 2011