Team:EPF-Lausanne/Our Project

From 2011.igem.org

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(Strategy)
(Strategy)
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During the summer, we worked on 3 main sections needed to complete the whole project:
During the summer, we worked on 3 main sections needed to complete the whole project:
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'''1) TetR mutants:''' Building mutations of TetR, both random ones and defined, already characterized in the litterature, ones. This part also comprised ''in vitro'' characterization, using MITOMI setup.
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'''1) TetR mutants:''' Building mutations of TetR, either random or defined (i.e. already characterized in the litterature). This part also comprised ''in vitro'' characterization, using MITOMI setup.
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'''2) Reporter plasmids:''' Assembling different plasmids allowing an ''in vivo'' characterization of TetR binding. Here we focused on RFP as a readout.
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'''2) Reporter plasmids:''' Assembling different plasmids allowing an ''in vivo'' characterization of TetR binding to its recognition sequence. We used RFP and a lysis cassette as a readout - either for characterization or for recovering DNA
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'''3) T7 promoter variants:''' Coupling T7 promoters of different strength with a lysis cassette. This part includes both T7 characterization with RFP and a proof-of-concept that we can efficiently lyse cells and recover their DNA.
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'''3) T7 promoter variants:''' Coupling T7 promoters of different strength with our 2 reporter genes, to have a better regulation of our Reporter plasmids system. This part includes both T7 characterization with RFP and a proof-of-concept that we can efficiently lyse cells and recover their DNA.
Section 1 presents the different TetR mutants and characterizes them ''in vitro''; sections 2 and 3 demonstrate '' in vivo'' TetR-Ptet interaction as well as recovery of DNA from the successful interactions.
Section 1 presents the different TetR mutants and characterizes them ''in vitro''; sections 2 and 3 demonstrate '' in vivo'' TetR-Ptet interaction as well as recovery of DNA from the successful interactions.

Revision as of 21:17, 15 September 2011