Difference between revisions of "Team:Alverno CA/Experiment"
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<br>After constructing these plasmids, we grew transformed <i>E. coli</i> as overnight liquid cultures. </h5> | <br>After constructing these plasmids, we grew transformed <i>E. coli</i> as overnight liquid cultures. </h5> | ||
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| − | < | + | <h3>Testing spacers <i>in vivo</i></h3> |
<h5>Cultures that contained strains with plasmids with a 500bp spacer or 1000bp spacer, were diluted to normalize their OD absorbance. RFP expression (in AFU), GFP expression (in AFU), and OD was measured in a plate reader (<a href="http://www.perkinelmer.com/product/victor-x5-for-fl-lum-uv-trf-fp-2030-0050">VICTOR-X3</a>). For strains using a 1000bp spacer we the effects of using inducer (ATc and IPTG) were tested as well. (See our <a href="https://2016.igem.org/Team:Alverno_CA/Protocols">Plate Reading (for Fluorescence, Absorbance, Induction, etc.) Protocol</a> for more information) </h5> | <h5>Cultures that contained strains with plasmids with a 500bp spacer or 1000bp spacer, were diluted to normalize their OD absorbance. RFP expression (in AFU), GFP expression (in AFU), and OD was measured in a plate reader (<a href="http://www.perkinelmer.com/product/victor-x5-for-fl-lum-uv-trf-fp-2030-0050">VICTOR-X3</a>). For strains using a 1000bp spacer we the effects of using inducer (ATc and IPTG) were tested as well. (See our <a href="https://2016.igem.org/Team:Alverno_CA/Protocols">Plate Reading (for Fluorescence, Absorbance, Induction, etc.) Protocol</a> for more information) </h5> | ||
Revision as of 23:03, 19 October 2016
Experiment
Introduction
It has been reported in the synthetic biology literature that the relative orientations and positions of genes physically placed near each other in multigene circuits may affect their expression. Specifically, it has been postulated that the issue of supercoiling may be responsible for this interference. Considering this, our intent was to demonstrate these effects on a series of plasmids containing both a RFP coding device, and a GFP coding device on a pSB1C3 pSB1C3 or DVK_AE (derived from pSB1K3). In between the two genes on each plasmid, we placed one of several insulators to separate the genes. These included a 500bp spacer, a 1000 bp spacer, and a dCas9 clamp; each was designed to isolate and eliminate interference. Constructed plasmids were inserted into E. coli (DH5α). Ultimately, the goal of the experiment was to accurately demonstrate interference between two genes (RFP/GFP) on the same plasmid and, in addition, find an insulating mechanism to restrain the effects of possible supercoiling. (For more details, see Design)
After constructing these plasmids, we grew transformed E. coli as overnight liquid cultures.
Methods
Testing spacers in vivo
Cultures that contained strains with plasmids with a 500bp spacer or 1000bp spacer, were diluted to normalize their OD absorbance. RFP expression (in AFU), GFP expression (in AFU), and OD was measured in a plate reader (VICTOR-X3). For strains using a 1000bp spacer we the effects of using inducer (ATc and IPTG) were tested as well. (See our Plate Reading (for Fluorescence, Absorbance, Induction, etc.) Protocol for more information)
