Team:Washington/Protocols/test

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Latest revision as of 23:09, 28 September 2011

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-'''Restriction Digest''' (10 uL DNA)
+</a>
-uL buffer ( 2 for most, check NEB)
-.5 uL BSA
-uL enzyme 1
-uL enzyme 2
-water to 50 uL(32.5 uL, add first)
-oligo assembly by PCR
-resuspend oligos with water, amount of water= concentration(in nm)*10 in uL
-make oligo mix with 5uL of each primer
-PCR reaction: 1uL phusion
-.5uL oligo mix
-uL first oligo
-uL last oligo
-uL buffer
-uL dnTP
-dH20 to 50uL
-Ligation
-uL insert
-uL vector
-uL T4 ligase buffer
-uL T4 ligase
-incubate at 37C no. **Note that NEB website recommends 16C - room temp for ligations, we do ours at RT and it works well. 1 hour.
-Colony PCR with Green tag
-Master mix(7ul):
-ul 10uM forword primer
-ul 10uM reverse Primer
-ul 2x Green tag
-Cell water(3ul): Pick one colony from the plate and mix with 10ul of ddH2O to make 10ul of cell water
-Reaction = Master mix(7ul) + Cell water(3ul) = 10ul per tube
-Use program "Colony" & change the extention time (1min per kb)
-Heat Shock Transformation
-ul ligation
-ul cells
-Ice 20 minutes
-Heat shock at 42C for 1 minute
-Ice 2 minutes
-Prepare 200 ul of TB (no anti) and transformed cells in culture tube
-Incubate at 37C for 1 hour
-Plate cells