Team:ETH Zurich/Processing 2
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Revision as of 13:28, 22 October 2013
Creation of a promoter library
Site directed saturation mutagenesis PCR of the BBa_R0062 PluxR
We did site directed saturation mutagenesis of specific sites of the lux box according to the results taken from literature (2) (see Figure 2).
We mutated the promoter directly in the BBa_J09855 construct and cloned it into a eGFP gene as a reporter to be able to screen for differences in the dose response curves. In the end we isolated one mutated promoter which shows a shift in sensitivity (see section below)