Mutagenesis

From Bridges Lab Protocols
Revision as of 13:06, 27 May 2009 by Davebrid (talk | contribs) (Protocol: added link to checking clones)
Jump to navigation Jump to search
The printable version is no longer supported and may have rendering errors. Please update your browser bookmarks and please use the default browser print function instead.

Materials

  • Template (dilute to ~ 0.1 mg/mL
  • Primers (prepare by adding 2 uL of each sense and antisense primer + 196 uL water and label as 1 uM primer mix). Design using Stratagene Primer Design Program
  • PFU Turbo
  • DpnI
  • Supercompetent XL1-Blue Cells (Stratagene)

Protocol

  1. Mix:
    1. 5 uL 10X Reaction Buffer
    2. ~20 ng Template (1 uL of minprep)
    3. 10 uL of Primer Mix
    4. 5 uL of dNTP mix
    5. 28 uL of water
  2. Add 1 uL of Pfu Ultra HF Polymerase
  3. Run PCR Program (DAVE-MUT)
    1. 95C for 30s
    2. Repeat 18 cycles:
    3. 95C for 30s
    4. 55C for 1 min
    5. 68C for 1 min/kb plasmid length (8 min default)
  4. Place on ice for 2 min
  5. Add 1 uL DpnI, mix and spin down. Digest 1h or overnight at 37C.
  6. Thaw XL1-Blue cells on ice and make 50 uL aliquots (round tube)
    1. Add 1 uL of digest to cells and mix.
    2. Incubate 30 min on ice.
    3. Heat at 42 C for 45 s, then place on ice for 2 min.
    4. Add 450 uL SOC preheated at 42C and grow 1h at 37C shaking
  7. Spread out entire transformation on appropriate antibiotic
  8. Grow O/N at 37C
  9. Pick a colony, miniprep and sequence to verify mutation
  10. Check Clones for Correct Mutation
Retrieved from "http://bridgeslab.sph.umich.edu/protocols/index.php?title=Mutagenesis&oldid=142"