Rensselaer/30 July 2008

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Promoter Group - 7.30.08

Transformation of Fe Promoter (Plate 1007 Well 7C) Into TOP10 E. coli

Set up petri dishes with bleach, dH2O, ethanol for wash of punch tool.

Aliquot 10 uL H20 to PCR tube. Incubate 10 uL H2O @ 50C for 5 minutes.

Punch out two DNA disks into 10 uL H2O making sure to wash punch tool in between.

Incubate PCR tube w/ H20 and DNA @ 42C for 20 minutes.

During incubation, thaw TOP10 supercompetent cells on ice.

Transfer all liquid to TOP10 cells. Incubate on ice 30 minutes.

Heat shock cells @ 42C 45 s. Incubate on ice for 2 minutes.

Transfer sample (cells + DNA) to 900 uL 2XYT. Incubate 1h @ 37C w/ shaking.

Plate 100 uL undiluted and 100 uL 50% concentrated on LB + 100 ug/ml amp plate.

Incubate @ 37C ON.

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