Difference between revisions of "Team:BostonU/Experiments"

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<p class="body-type mainwrap">With the desire to create fusion proteins in mind, our second region consisted of 30-nt sourced from within our lab and verified to work in dozens of constructs. This would allow us to tag the recombinases with fluorescent proteins and track their synthesis overtime. At the end of our time working on the iGEM project, we were working on characterizing the effects of adding these linker regions to the pBEST plasmid’s activity in cell free. Once this is verified, we could tag our recombinase proteins and verify that they are being expressed in the cell free system. From here we can better troubleshoot our system and gain functional recombinases in cell free.</p>
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<p class="body-type mainwrap">With the desire to create fusion proteins in mind, our second region consisted of 30-nt sourced from within our lab and verified to work in dozens of constructs. This would allow us to tag the recombinases with fluorescent proteins and track their synthesis overtime. At the end of our time working on the iGEM project, we were working on characterizing the effects of adding these linker regions to the pBEST plasmid’s activity in cell free. Once this is verified, we could tag our recombinase proteins and verify that they are being expressed in the cell free system. From here we can better troubleshoot our system and gain functional recombinases in cell free. <img src="https://static.igem.org/mediawiki/2017/f/f4/T--BostonU--AddLinkerFig1.svg" width=30%></img></p>
 
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Revision as of 06:30, 31 October 2017

EXPERIMENTS