Team:EPF-Lausanne/Our Project/Assembly/Ptet
From 2011.igem.org
Ptet promoter characterization
Back to Reporter systems || Ptet | Plac | Plasmid detailsSince we are using the Ptet promoter in combination with TetR in our reporter systems, it was useful for us to characterize the Ptet promoter only. This characterization was done with the J61002 Ptet-RFP plasmid.
We added increasing concentrations of ATC in order to see if the DH5alpha cells that we used for the transformations expressed a lot of TetR; we also wanted to know the highest RFP expression we can get when Ptet is fully induced.
ATC induction
The DH5alphas cells, even if the plasmid we transform doesn't contain TetR, can still have a basal expression of the transcription factor. By adding ATC, we are able to inhibit this TetR basal expression, revealing the full power of Ptet as a promoter sequence.
Experimental results:
There is a clear difference between cells untreated or treated with high doses of ATC. Still, this difference is not enormous, showing that our DH5alpha cells don't normally express much TetR. The basal expression of RFP is about 23'000 normalized RFUs, whereas with ATC we go up to 28'000 normalized RFUs.
Dose-response curve
The dose-response curve doesn't seem to saturate at the highest values of ATC added, indicating that some TetR proteins were perhaps still acting on the Ptet promoter. However, it is nice to see that TetR does have a quantifiable action on the promoter; it means that we can use it in our first readout system.