Yesterday we started the process of cloning the GAPC gene from
Arabidopsis, which we amplified via nested PCR in lab 5. The lab was divided in three main steps
- Ligation (of GAPC gene on to the pJet1.2 plasmid)
- Preparation of competent cells
- Genetic transformation of E. coli
We spent most of the lab manipulating bacteria to make them competent (
i.e. get them ready to uptake extracellular naked DNA). Once this was achieved, the
GAPC gene from
Arabidopsis, obtained via nested PCR, was ligated to the
pJet1.2 plasmid.
The plasmid was then used to genetically transform
E. coli, which were spread on
LB agar/Amp/IPTG plates and incubated.
----------------------
No comments:
Post a Comment