Team:Evry/Interlab Study/Results
From 2014.igem.org
Interlab study - Aim & Results
There were two sub-parts in this study:
To test the expression of promoters, they are cloned into the PSB1C3 vector followed by the
BBa_E0240, a GFP generator. Constructions are inserted in E. coli DH5 alpha that grown on LB medium added with the selection agent, chloramphenicol. Our team decided to test the fluorescence with a
TECAN infiniteM200 in 96 well plates.
Fluorescence data were analyzed via following formula that come from 2010 De Jong et al Experimental and computational validation of models of fluorescent and luminescent reporter genes in bacteria .
Equation B: B(t) is the absorbance of the strain carrying the promoterless vector, Iu(t) the uncorrected fluorescence intensity of DH5 alpha with the functional reporter system and Ib(t) the background fluorescence intensity of LB chloramphenicol medium with the DH5 alpha carrying the promoterless vector.
Required Devices
The three required constructions shown various fluorescence intensity at OD 600 nm = 0.5, as shown on bar chart on the right. The same trend was observed between OD 600 nm = 0.1 to 0.8(Data shown on
Interlab study notebook). Fluorescence intensity curve profile according to OD 600 nm corresponded to the expected profile for a constitutive promoter (Data shown on
Interlab study notebook).
Entire Anderson library of constitutive promoters (J23100-J23119)