User:University of Washington/30 July 2008

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Since I expect poor transformation, innoculated ON culture of DY331 for next transformation experiment.  DY331 will be rendered electrocompetent and immediately transformed to eliminate any problems that may be due to using a glycerol stock.
Since I expect poor transformation, innoculated ON culture of DY331 for next transformation experiment.  DY331 will be rendered electrocompetent and immediately transformed to eliminate any problems that may be due to using a glycerol stock.
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==AHL Expression in Yeast (Bryan)==
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X & S double restriction digest on yeast expression plasmids and C0161.  Ran on gel.  Analysis pending.
==LuxR from AraC and TetR==
==LuxR from AraC and TetR==

Revision as of 00:39, 1 August 2008

Lambda Red Recombineering of RP4 (Bryan)

Co-transformed DY331 with pUC307 (RP1) and recombinant vector containing Cm resistance cassette. Time constants 1.0 and 1.2 for two trials. Suspect glycerol stocks may contribute to poor time constant. Plated on selective media.

Since I expect poor transformation, innoculated ON culture of DY331 for next transformation experiment. DY331 will be rendered electrocompetent and immediately transformed to eliminate any problems that may be due to using a glycerol stock.

AHL Expression in Yeast (Bryan)

X & S double restriction digest on yeast expression plasmids and C0161. Ran on gel. Analysis pending.

LuxR from AraC and TetR

- Did restriction digestion on Elowitz's plasmid with HindIII. (30 ul of DNA for digestion reaction, 15 ul for control with no enzyme). Incubated the reaction for about 4.5 hours, then ran the gel. Saw bands: 4-5 kb, 2 kb, 0.5-1 kb as expected. However, the 4-5 kb fraction wasn't clear enough to tell whether it was only 4.7kb of pCD26 or 4.2kb of pACYC184. Will have to select another enzyme to confirm the nonexistence of pACYC184(this produces LuxR which we don't want).

- Overnighted Elowitz's plasmid in Tsy+Kan, E0240 in Tsy+Amp.

- Streaked out Elowitz's E.coli in Tsy plate.



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