Team:Calgary/23 July 2010
From 2010.igem.org
Friday July 23, 2010
Raida
The first thing I did this morning was run a Gel Electrophoresis of my Mal-E Gene Specific Primer Testing PCR products. I ran it on a 1% gel at 100 V for an hour. Please refer to the image to the side. As it can be seen, the PCR results are positive. All the bands are near the 1200 bp band size, which indicates that it is the Mal-E gene. Furthermore, Lane 7 and Lane 13 show no band because this was the DNA that had the deleted sequence. So the fact that there is no band there is an indication of the fact that the MalE primer is functional and only amplified the MalE gene as it was supposed to. Further testing will be done to assure that the band shows the MalE Gene.
Himika
Today I ran a colony PCR of 11 of the colonies from the plates last night which was I0500-B0034 plasmid switched into pSB1AC3. Most of the colony PCRs seem to work, although the bands are faint. Primers used:
- Bbk_CP_F
- Bbk_CP_R
These two primers anneal 100 bp upstream and downstream of the biobrick prefix and suffix. The expected size of the bands was 1400 bp which was exactly what was seen in the gel. I have decided to forward with B1,C1 which are lanes 2 and 3 respectively.
I also restreaked the two colonies on AC plates and left it in the incubator at 20 C. I also made overnight cultures of the same colonies which will be taken out of the shaker on saturday 24 July, 2010.
Dev This week I worked on the t-shirt designs in Inkscape. The designs are almost finalized. I also helped miniprep the construction of K239000+I13507 today.
Emily
Today I diluted the malE-BBK primers as well as the pRFP-M primers for the site-directed mutagenesis of pRFP. I ran a PCR of malE and malE31 in order to try to Biobrick it. I also ran a PCR of my old construct of I0500-B0034 with the new BBK-CP-F and BBK-CP-R primers. If Himika's I0500-B0034 construct does not give positive reuslts after sequencing, then we may try this one out as a back-up. Raida's PCR of malE and malE31 with gene specific primers as well as the primers that add XbaI and SpeI restriction sites looked really good, so I went ahead and PCR purified the PCR product from the reactions set up with the XbaI/ SpeI primers. Raida also diluted the PCR product that had been run with the gene specific primers and we ran this as a template in two reactions of the malE-BBK PCR.
Chris
Today, I ran an agarose gel electrophoresis of the gradient PCR that was run overnight last night. The bands came up as shown on the right. The bands that appeared were in the range of approximately 400 bp for several of the lanes. This is the projected size of the part of the CpxP promoter as well as the plasmid it was inserted into. After this, I set up a restriction digest with XbaI and PstI which would then be run on an agarose gel electrophoresis to verify the size. Finally, a regular plasmid PCR was set up to determine the size of the part. This will be left to run overnight. Contact was also made with several different companies for funding and possible sponsorships for our project. Several companies that we are contacting have different time zones and thus the times must be coordinated so they are open and we are here. Packages to mail to companies were started but will be finished for next week to mail.
No notebook page exists for this date. Sorry!