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

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(Introduction)
(Results)
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[[Image:dose_response.png|500px|center]]
[[Image:dose_response.png|500px|center]]
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The dose-response graph above was also made using triplicate data. This time, the functional T7-lysis plasmid (C2) was tested against two negative controls: a T7-RFP plasmid (which should only fluoresce, not lyse) and a plasmid containing a non-functional lysis cassette driven by a T7 promoter (C11). The points of each curve are the unaveraged fluorescence responses (normalized by OD) over the last hour of the experiment, which we take to be a good estimate of the steady-state saturation. The C2 lysis plasmid shows strong lysing, since the fluorescence drops significantly as the IPTG dose increases.  
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The dose-response graph above was also made using triplicate data. This time, the functional T7-lysis plasmid (C2) was tested against two negative controls: a T7-RFP plasmid (which should only fluoresce, not lyse) and a plasmid containing a non-functional lysis cassette driven by a T7 promoter (C11). The points of each curve are the OD values of each replicate averaged over the last hour of the experiment. For the lysis plasmid we observed a strong lysis response with increasing IPTG concentrations. Both controls show no significant change in endpoint OD in respect to IPTG concentration.
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Revision as of 16:30, 21 September 2011