Revision as of 13:58, 6 July 2011

Todo

All the parts are verified, we can now assemble them!

~~Research plasmid backbones. Is there one that already contains Tet-repressed LacI or GFP?~~
~~Design Gibson primers to assemble the three different plasmids.~~
~~Receive said primers~~
Determine which sequence on LacI-plasmid and Lysis-plasmid should be used to create the "mega-plasmid".
Think of new assemblies we want to make (pTet with RFP, for example)

Specifically:

For wtTetR

~~repeat MITOMI with wtTetR His-tagged (linear template) and wtTetR GFP-tagged (plasmid), for consensus and negative control sequence. DNA spotted in different concentrations~~
experiment with de Brujin library spotted on His-wtTetR or/and wtTetR-GFP (this will yield PWM)

experiment planned on July 6

Further, check the ordered muTetRs (determine position weight matrix)

Repeat experiments to check design
Grow E. Coli from spotted arrays
~~[No microfluidics] Setup a plate and test tween concentrations~~
~~Determine growth rate as function of tween concentration (say 0.075% +- 0.7, as many increments as will fit on the chip)~~
Adapt design of "chemostat" chip for e-coli

@@ Line 47: / Line 47: @@
 * Grow E. Coli from spotted arrays
 * <s>[No microfluidics] Setup a plate and test tween concentrations</s>
-* Determine growth rate as function of tween concentration (say 0.075% +- 0.7, as many increments as will fit on the chip)
+* <s>Determine growth rate as function of tween concentration (say 0.075% +- 0.7, as many increments as will fit on the chip)</s>
 * Adapt design of "chemostat" chip for e-coli