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ColiGuard
PY Promoter - Preparation of electrocompetent cells
Protocol 4.
Fabi and Léo
Testing the new device
We confirmed our device yesterday, but we continued working with it. We proved that our device really works. To fulfill this aim, we transformed competent E. Coli C43. This E. coli strain can be producing the T7 polimeraze by IPTG induction. Thus, when we put IPTG into the culture medium, we will have expression of T7 polimeraze which will induce the T7 promoter of our device and so, the endolysin will be expressed. Our test consists in overexpress the endolysin in order to break it's own peptidoglycan wall. We transformed cells with our device BBa_K284022 plasmid and with the BBa_K112806 plasmid (without promoter).
So, after get the transformed cell, we put them to growth in 5 erlenmeyers (ampicilim LB medium) until half log phase(OD-0.6 to 1). Then, we induced with IPTG (1mM) and we measured the optical density for 4 hours after induction. We plated the 5 cultures in ampicilin LB medium plates in order to confirm the diminished cellular growth. To have a definitive confirmation, we also performed SDS-PAGE to notice the protein overexpression. We show the result in ColiGuard results.
Luige, Ane & Marcos
YeastGuard
We sent 4 biobricks to iGEM today: pJEN1, pDLD, Lysozyme, and the devices Adh1+YFP and Adh1+Lysozyme. =)
Yeast experiments
We did miniprep of YEP+Adh1-YFP and the following devices: b) pJEN1+YFP, c) pJEN1+Lys, d) pDLD+YFP, e) pDLD+Lys.
Raíssa and Taís
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