Team:Carnegie Mellon/Met-Challenges

From 2012.igem.org

(Difference between revisions)
Line 124: Line 124:
<p> Our cloning procedures did not work initially due to confounding factors of contamination in media and competent cells, inappropriate design of digestion sites, and non-optimal PCR reactions. However, these issues were eventually ironed out and we managed to get the FAP and Spinach into a single construct. <br \><br \>
<p> Our cloning procedures did not work initially due to confounding factors of contamination in media and competent cells, inappropriate design of digestion sites, and non-optimal PCR reactions. However, these issues were eventually ironed out and we managed to get the FAP and Spinach into a single construct. <br \><br \>
-
We have attempted to clone our constructs into pSB1C3 and another plasmid vector that has both EcoR1 and Pst1 digestion sites. The cloning using the plasmid vector worked in the first trial. However, the cloning using pSB1C3 was more difficult than we expected and only worked after four trials and extensive optimization of our protocols. We have not been able to pinpoint the problems. </p>
+
We have attempted to clone our constructs into pSB1C3 and another plasmid vector that has both EcoR1 and Pst1 digestion sites. The cloning using the plasmid vector worked in the first trial. However, the cloning using pSB1C3 was more difficult than we expected and only worked after four trials and extensive optimization of our protocols. We have not been able to pinpoint the cause for this. </p>
</html>
</html>
{{:Team:Carnegie_Mellon/Templates/Footer}}
{{:Team:Carnegie_Mellon/Templates/Footer}}

Revision as of 05:48, 3 October 2012

Image:CMU_image6.jpeg




Challenges with Molecular Cloning

Our cloning procedures did not work initially due to confounding factors of contamination in media and competent cells, inappropriate design of digestion sites, and non-optimal PCR reactions. However, these issues were eventually ironed out and we managed to get the FAP and Spinach into a single construct.

We have attempted to clone our constructs into pSB1C3 and another plasmid vector that has both EcoR1 and Pst1 digestion sites. The cloning using the plasmid vector worked in the first trial. However, the cloning using pSB1C3 was more difficult than we expected and only worked after four trials and extensive optimization of our protocols. We have not been able to pinpoint the cause for this.

Image:TartanFooter.jpeg