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+ | For our project this year we successfully designed and characterized an accessible and modular degradation based system for the control of gene expression speed. Utilizing an <i>E. coli</i> orthogonal tmRNA degradation system consisting of a <i>Mesoplasma florum</i> Lon (mf-Lon) protease [1] and highly engineered tmRNA tags [2] with a range of protease affinities, we were able to create a qualitative and quantitative gene expression speed change that was dependent on degradation rate. To do this we first had developed a time course measurement protocol that would allow robust and reproducible single cell measurements. Developing this method was time intensive, and meant that we spent a large portion of the summer without getting high-quality gene expression speed data, but ultimately our final <a href='https://2017.igem.org/Team:William_and_Mary/Protocols' style='text-decoration: underline;'>time course protocol</a> ensured that we got robust, reproducible data that we could feel confident in. | ||
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+ | <div style = 'padding-left: 190px; padding-bottom: 10px;font-size: 25px' ><b>References</b></div> | ||
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+ | [1] Eyal Gur and Robert T Sauer. Evolution of the ssra degradation tag in mycoplasma: specificity switch to a different protease. Proceedings of the National Academy of Sciences, 105(42):16113– 16118, 2008. | ||
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+ | [2] D Ewen Cameron and James J Collins. Tunable protein degradation in bacteria. Nature biotechnology, 32(12):1276–1281, 20 | ||
+ | </div> | ||
Revision as of 19:58, 1 November 2017