Haynes Lab:Notebook/Engineering PC-TFs/2013/09/12: Difference between revisions

September 12, 2013

• Follow steps for gel electrophoresis.
• Orient top notch of gel electrophoresis apparatus. Place gel tray into larger tray.
• Fill gel flask with up to 60 ml of TA buffer.
• Create 1% gel by putting .6 grams of agarose into flask.
• Microwave agarose solution for 40 seconds
• Using hot gloves, grab flask out of microwave and swirl flask vigorously. Place back in microwave for 40 more seconds.
• When flask is taken out of microwave, make sure that the agarose is completed dissolved.
• Set up wells on gel electrophoresis apparatus. The mold for the first digest is B-10. Use the thick "teeth" and slip in the notches.
• Add EtBr (ethidium bromide) to the agarose gel. There should be 1 microliter of EtBr per 10ml of agarose gel. Therefore, 6 µL.
• Pour gel into tray.
• Wash the agarose gel flask.
• Run gel for 45 min at 100 V. Check gel under UV light.

Reagent	Volume	30 μL/lane, 1% agarose; Ladder
DNA (plasmid)	20.0 μL
SpeI	1.0 μL
PstI	1.0 μL
Green 10x FastDigest buffer	3.0 μL
dH2O	5 μL
	30 μL --> 37°C/ ~10 min.

Zymoclean^TM Gel DNA Recovery Kit

• Add 3 volumes of ADB Buffer to each volume of gel (600 μL).
• Incubate at 55°C for 10 minutes.
• Centrifuge at ≥ 10,000 x g for 30 seconds. Discard flow-through.
• Add 200 μL of DNA Wash Buffer to the column and centrifuge for 30 seconds. Repeat wash step.
• Place Zymoclean Column into a new 1.5 mL tube. Add 20μL of dH₂O to elute DNA