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<b><div style = 'padding-right: 190px; padding-left: 190px;' >Flow Cytometry</div></b> | <b><div style = 'padding-right: 190px; padding-left: 190px;' >Flow Cytometry</div></b> | ||
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<div class="col-sm-8" style = 'padding-right: 30px; padding-left: 190px; line-height: 25px;' >We used the BioRad S3e Cell Sorter to carry out single-cell fluorescence measurements. We diluted 100µL of cell culture into 400 µL of Phosphate Buffered Saline (PBS). For our induction experiments, we split and induced the cells with IPTG 6 hours after they were inoculated. Four hours after the cells were induced, we diluted the cells in order to obtain an ideal concentration of OD600 0.01. The cells were then grown for another five hours and taken out every 20 minutes to be filtered on ice and FACSed immediately. To acquire data with flow cytometry, we adjust side-scatter (SSC) and | <div class="col-sm-8" style = 'padding-right: 30px; padding-left: 190px; line-height: 25px;' >We used the BioRad S3e Cell Sorter to carry out single-cell fluorescence measurements. We diluted 100µL of cell culture into 400 µL of Phosphate Buffered Saline (PBS). For our induction experiments, we split and induced the cells with IPTG 6 hours after they were inoculated. Four hours after the cells were induced, we diluted the cells in order to obtain an ideal concentration of OD600 0.01. The cells were then grown for another five hours and taken out every 20 minutes to be filtered on ice and FACSed immediately. To acquire data with flow cytometry, we adjust side-scatter (SSC) and | ||
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<div class="col-sm-8" style = 'padding-right: 30px; padding-left: 190px; line-height: 25px;' > <a href="https://static.igem.org/mediawiki/2017/4/4e/T--William_and_Mary--QiagenMiniprep.pdf"> Qiagen Miniprep</a> </div class> | <div class="col-sm-8" style = 'padding-right: 30px; padding-left: 190px; line-height: 25px;' > <a href="https://static.igem.org/mediawiki/2017/4/4e/T--William_and_Mary--QiagenMiniprep.pdf"> Qiagen Miniprep</a> </div class> | ||
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Revision as of 06:14, 1 November 2017