Knockout1

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Revision as of 09:07, 21 October 2010

Target gene
- yfaL
  - an AmpR and CmR plasmid that shows temperature-sensitive replication and thermal induction of FLP synthesis (Datsenko and Wanner paper [1])

Transformation of pKD46 to target strain
- Preparation of competent cells
  - Using the protocol of TSS method - TSS method.
  - Target strain - BW25113, Top10

Generation of cassette flanked by homologous arms
- Design of primers
  - Primers have overhangs which were homologous to surrounding region of target gene.
  - Sequences from cassette region have about 60℃ Tm-value.
- PCR condition
  - Anneling temparature and extension time depends on the target sequence.
  - Anneling temparature is tested at 55℃ at first.
  - Extension time is depend on the length of the target sequence. (1kb = about 1 min.)
- PCR program
  - 94°C 1min → 30*[98°C 11s → 55°C 30s → 72°C 2min] → 72°C 5min

Pick the single colony containg pKD46.
Inoculate it to 5㎖ LB broth with ampicilline and L-arabinose.
- L-arabinose final concentration is 1mM.
Incubate at 27℃, 180rpm until the culture OD reaches 0.6.
Centrifuge 3600rpm, for 5min at 4℃.
Wash with ice-cold 10% glycerol 3 times.
Concetrate 100-fold.

Primers
- For pKD 13 kanamycin cassette
  - Foward: ATGCGGATTATCTTTCTACGCAAGGAGTATTTATCTTTACaATTCCGGGGATCCGTCGACC
  - Reverse: gcgcccctgccagcacgtagtgtgtaggctggagctgcttcggccggttagcgccatcggct
- For confirmation of Knockout
  - Foward: GTTTCATGCAGACTACCTGTAGTACG
  - Reverse: ctgcctcgtcctgcagttcattca

@@ Line 48: / Line 48: @@
 | reverse primer||10 pmol||2㎕
 |-
-| 10x EX buffer||-||5㎕
+| 10x EX buffer||   ||5㎕
 |-
 | dNTP||2 mM||2㎕
 |-
-| EX-Tag polymerase||-||0.5㎕
+| EX-Tag polymerase||    ||0.5㎕
 |-
-| D.W.||-||50㎕
+| D.W.||   ||50㎕
 |}