Haynes Lab:Notebook/Engineering PC-TFs/2014/05/15: Difference between revisions

Summary

Digest PcTF1 (BL01)

Restriction Digest Table

Gel Purification: BL01/V0120

• Using Prior Digest
  
• Placed 15μL 1kB Ladder in well one and 30μL of BL01 digest in well two.
• Ran gel at 110V for 55 minutes.
• Placed gel on UV transilluminator and cut out desired band.

0.8% agarose; cut the brightest band furthest down at ~ 2500bp; Ladder

• Used Zymo gel purification kit.
• Assumed 200mg gel, added 600μL ADB to the 1.5mL tube.
• Put on heat block at 55°C for 5 minutes, vortexed and then placed back on the heat block for an additional 5 minutes, vortexed again.
• Put ~750μL gel/ADB into spin column, centrifuged at max rpm for 30 seconds.
• Pipetted 200μL wash buffer to the tube, centrifuged at max rpm for 30 seconds. Repeated once.
• Transferred column to new labeled 1.5mL tube.
• Pipetted 15μL elution buffer to the column.
• Spun at max rpm for 30 seconds.
• Put marked (GelP BL01 5/15/2014) BL01 in -20°C fridge in box labeled Cameron.

Ligation

• Added 10μL dH₂O to two 0.5mL tubes marked 1 and 2.
• Pipetted 0.5μL BL01 into tube 1. Put both tubes on ice.
• Let DH5a-T cells thaw in ice.
• Transferred 50μL cells into each tube. Incubated for 5 minutes on ice.
• Spread sample 1 onto labeled plate 1 using sterile beads. Repeated for tube two and plate two.
• Placed in incubator for overnight growth.