Difference between revisions of "Team:Newcastle/Results"

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           <h2 style="text-align: left; clear: both"> Conclusions and Future Work </h2>
 
           <h2 style="text-align: left; clear: both"> Conclusions and Future Work </h2>
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The aim of the Fim switch part was to make a processor module which can be visually inspected for functionality.  The Fim switch has been shown to expresses the eforRed chromoprotein under normal (uninduced) conditions which allows the user to both determine that the strain is alive and has maintained the Fim switch plasmid.  Following induction, the Fim promoter flips direction and begins expressing RhlI which synthesises the C4-HSL quorum sensing molecule.  This has been shown to successfully induce expression of sfGFP in the reporter strain K2205015.<br/><br/>
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Despite several attempts we were unable to produce a Fim switch testing construct where <i>fimE</i> expression could be controlled using the <i>E. coli</i> arabinose inducible promoter.  Though transformations did yield some colonies when trying to make this part, none were red in colour.  This possibly indicates that the arabinose inducible promoter (even when grown on 0.5% glucose) is still too active.  The design for this construct has been submitted (BBa_K2205006).<br/><br/>
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<u>Future Work:</u>
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Since there is some leaky expression of the <i>fimE</i> gene (even without a promoter) to fine tune the Fim switch the lac operator could be inserted upstream of the <i>fimE</i> RBS to repress unwanted expression.  The part could then be used following the addition of IPTG.  An alternative method would be to clone a transcriptional terminator upstream of the <i>fimE</i> RBS to prevent leaky expression from elsewhere in the plasmid.<br/><br/>
  
 
           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> References </h2>
 
           <h2 style="font-family: Rubik; text-align: left; margin-top: 1%"> References </h2>

Revision as of 19:31, 27 October 2017

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Our Experimental Results

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