Difference between revisions of "PhiX:Transformation"

Revision as of 18:20, 18 August 2009

With credit to Art Poon for base protocol and Maniartis.

pre-chill centrifuge to 4^oC and get ice
freeze two 20ml, two 10ml serological pipettes and 1ml, 200ul tip boxes - use these for all transfers
chill two 50ml centrifuge tubes
prepare 50ml LB + 1ml O/N C122 (or chosen strain; Art Poon says inoculate with colony)
follow until OD_600nm = 0.250 (must catch in exponential phase)
using 20ml pipette, divide culture into two ~25ml aliquots into chilled centrifuge tubes
cool for 5 minutes on ice
centrifuge @ 4000rpm (CHECK rotor) for XX minutes at 4^oC
discard supernatent - pellets should be thumb-nail size
using 10ml pipette, dispense 5ml ice-cold 0.1M (CHECK) CaCl₂ to each tube
resuspend pellet (Art Poon says do not disrupt pellet)
chill cells on ice for 30 mins
centrifuge @ 4000rpm for XX minutes at 4^oC - pellets should be ring-shaped
discard supernatent
using frosty 1ml tip, resuspend each pellet with 500ul ice-cold 0.1M CaCl₂ (do not vortex)
using frosty 200ul tip, transfer 100ul aliquots to (thin-walled) PCR tubes
add DNA (e.g., 5ul mutagenesis PCR) to each 100ul aliquot
chill on ice for 1 hour (meanwhile heat waterbath to 42^oC)
transfer tubes to waterbath, incubate for 1 minute and return tubes to ice
recovery in SOC is optional
transfer aliquots to soft agar with 100ul O/N C122 and MgCl/CaCl solution for infection and plate
incubate plates for four hours at 37^oC (Art Poon: 33^oC)

Revision as of 18:20, 18 August 2009 (view source) Ben (talk) m ← Older edit		Revision as of 18:20, 18 August 2009 (view source) Ben (talk) m Newer edit →
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−	With credit to Art Poon for base protocol and Maniartis.	+	''With credit to Art Poon for base protocol and Maniartis.''

	* pre-chill centrifuge to 4<sup>o</sup>C and get ice		* pre-chill centrifuge to 4<sup>o</sup>C and get ice