Team:WashU/Week11

From 2012.igem.org

(Difference between revisions)
Line 9: Line 9:
</html>
</html>
 +
Colony PCR of U construct using four new colonies and the same positive Z control has once again resulted in no successful colonies. However, the PCR has reaffirmed that the control works, which is a good sign.
 +
We also did a PCR of the color constructs in order to form our BioPaint set. [PICTURE BELOW]
 +
 +
Since our T plasmid and Z construct ligations have not been going well, we started over by preparing new cultures of Z and T, running them on a gel, and then gel purifying the results. [SEE PICTURE]
 +
 +
We began 5 ml cultures for the good Z construct with TOPO and for one of the U ligation colonies. We will use the Z culture for a glycerol stock, and digest the U culture to see if our ligations actually succeded.
<br>
<br>

Revision as of 20:54, 6 August 2012



Monday, August 6

Colony PCR of U construct using four new colonies and the same positive Z control has once again resulted in no successful colonies. However, the PCR has reaffirmed that the control works, which is a good sign.

We also did a PCR of the color constructs in order to form our BioPaint set. [PICTURE BELOW]

Since our T plasmid and Z construct ligations have not been going well, we started over by preparing new cultures of Z and T, running them on a gel, and then gel purifying the results. [SEE PICTURE]

We began 5 ml cultures for the good Z construct with TOPO and for one of the U ligation colonies. We will use the Z culture for a glycerol stock, and digest the U culture to see if our ligations actually succeded.


Tuesday, August 7



Wednesday, August 8



Thursday, August 9



Friday, August 10
Retrieved from "http://2012.igem.org/Team:WashU/Week11"