Team:WashU/Week5
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We have also decided to use PCR to amplify our DNA, as we are getting extremely low yields from our gel extractions. Thus, we designed the primers today. | We have also decided to use PCR to amplify our DNA, as we are getting extremely low yields from our gel extractions. Thus, we designed the primers today. | ||
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==Saffron in a Kan== | ==Saffron in a Kan== | ||
- | We finally received our gene from DNA 2.0!! We streaked out some of the gene, still in its plasmid | + | We finally received our gene from DNA 2.0!! We streaked out some of the gene, still in its plasmid onto plates with ampicillin. |
In addition, we transformed <i>Synechocystis</i> with the plasmid PSL2131 obtained from one of our mentors, Burt. | In addition, we transformed <i>Synechocystis</i> with the plasmid PSL2131 obtained from one of our mentors, Burt. | ||
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==YLC== | ==YLC== | ||
- | In the interest of time, we will use existing biobrick constructs with the necessary fluorescent proteins to show to the YLC students, and then we will complete our own constructs at a later date. Thus, today, we plated several biobrick constructs | + | In the interest of time, we will use existing biobrick constructs with the necessary fluorescent proteins to show to the YLC students, and then we will complete our own constructs at a later date. Thus, today, we plated several biobrick constructs (RFP: I13521, |
GFP: I13522, | GFP: I13522, | ||
YFP: 13604, and | YFP: 13604, and | ||
- | CFP: S03475 | + | CFP: S03475) and will pick colonies to prep. |
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Latest revision as of 16:43, 17 August 2012