Clone Pick-up: We prepared 3ml cultures with ampicillin (100ug/ml) and chloramphenicol (20uq/ml). Colonies transformed with the plasmids pBAD33 and pET16b were picked and placed in the amp and chlor cultures respectively. They were then kept on a shaker overnight at 37C.
Glycerol stocks: for pET and pBAD33, 1.75mL of each culture were added to 0.5ml of LB+50% glycerol.
Minipreps of the pBAD33 and pET16b plasmids were conducted and gels were run to confirm their size.
PCRs were performed on pBAD, araC and lacI to add biobrick sites
3ml cultures of the E coli containing plasmids for GlnAp2, GlnG and the strain 3.3L*G (has lacI/glnG knockout) were prepared. Plates with colonies were obtained from Dr Alex Ninfa (Michigan University).
Glycerol stocks of plasmids from Dr Ninfa were prepared.
Minipreps of the plasmids containing GlnAp2 and glnG were prepared before we did a PCR on glnG to add BioBrick
Gel and purification of araC, lacI, pBAD and glnG. Nanodrop results:
araC = 195 ng/ul
pBAD = 152 ng/ul
glnG = 166.9 ng/ul
Digestion of araC, pBAD and glnG with EcoRI and PstI.