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Latest revision as of 06:56, 19 October 2016
console.js:26
Wednesday June 29, 2016
Wednesday, 6/29
Members Present: Hamed, Kat, Cathy, Dk, Tam
LAB:
Morning:
- Made 2 bottles of 500mL of 2×YTPG (for s30 pellets)
- Cultured 100mL of DH10B as part of RbCl competent cell protocol
- PCR amplification of Short Linear LacZ fragment under the following conditions: Normal (being the conditions run previously yesterday, with a shortened annealing time of 20sec), 2 step (with the annealing temperature raised to the extension temperature 72C), 7sec (wherein the extension time was reduced from 15 sec to 7 sec to account for the smaller size of the fragment), and MgCl2 (where the Mg+ concentration was boosted by 0.2uM to account for the present of EDTA)
Afternoon:
- Made rubidium chloride competent cells, stored in -80 as CCD
- Miniprep and nanodrop of previous E.glowli culture:
- Made 5x glycerol stocks of e.coli DH10B and of RFP containing DH10B. made 3x glycerol stocks of E.glowli containing E.coli.
- Nanodrop of the PCR results.
- Ran a gel along with previous PCRs of the LacZ.
- Appears that running a 2 step PCR might resolve the issue of our PCR insters concatemerizing.
- 5ml Overnight culture of E.glowli and the single colony from L1 plates.
- Made 10% w/w of L-arabinose solution for inducing the PBAD promoter found in E.glowli.
Administrative:
TO DO:
For the next day:
LAB TEAM:
LAB MANAGERS:
Gmail correspondence:
Meetings/Notes:
References: