Difference between revisions of "Part:BBa K4046902"

 
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<b><font size="+1">Overview</font></b>
 
<b><font size="+1">Overview</font></b>
This is a binding site for the <i>DhdR</i> gene, as identified in the literature by Xiao et al. The <i>DhdR</i> protein was originally identified in <i>Achromobactor denitrificans</i>, and the  <i>dhdO</i> sequences were designed and optimized for binding to the  DhdR protein. In this composite part, we added a Kozak sequence and [insert <i>cLuc</i> or <i>tdTomato</i> or <i>mCherry </i>] gene downstream of the binding site and promoter, which allow the part to be used in a DhdR-based biosensor for oncometabolite D-2-HG.  
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This is a binding site for the <i>DhdR</i> gene, as identified in the literature by Xiao et al. The <i>DhdR</i> protein was originally identified in <i>Achromobactor denitrificans</i>, and the  <i>dhdO</i> sequences were designed and optimized for binding to the  DhdR protein. In this composite part, we added a Kozak sequence and <i>mCherry</i> gene downstream of the binding site and promoter, which allow the part to be used in a DhdR-based biosensor for oncometabolite D-2-HG.  
  
 
This composite part is one of several that the Duke iGEM intends to test for use in a biosensor for the oncometabolite D-2-HG. A schematic for the operation of our system is shown below.
 
This composite part is one of several that the Duke iGEM intends to test for use in a biosensor for the oncometabolite D-2-HG. A schematic for the operation of our system is shown below.

Latest revision as of 03:17, 22 October 2021

hUBC - BS #1 with spacer - BS #1 - Kozak - mCherry - bghA

Overview This is a binding site for the DhdR gene, as identified in the literature by Xiao et al. The DhdR protein was originally identified in Achromobactor denitrificans, and the dhdO sequences were designed and optimized for binding to the DhdR protein. In this composite part, we added a Kozak sequence and mCherry gene downstream of the binding site and promoter, which allow the part to be used in a DhdR-based biosensor for oncometabolite D-2-HG.

This composite part is one of several that the Duke iGEM intends to test for use in a biosensor for the oncometabolite D-2-HG. A schematic for the operation of our system is shown below.

T--Duke--DhdrSchematic.png

Figure 1: This figure outlines the mechanism of the interaction between the DhdR allosteric transcription factor and the dhdO binding site.

This plasmid will be tested together with another construct expressing the protein DhdR, which is a transcriptional repression factor isolated from the bacteria Achromobacter denitrificans. In a wild-type environment, without the presence of DhdR, we expect normal expression of the reporter protein. However, when DhdR is present, it will bind to the dhdO binding site, allosterically blocking the transcription of our reporter gene. When D-2-HG is elevated, particularly in IDH1 mutant cells, it binds to DhdR, releasing it from the binding site.

T--Duke--T--Duke--DhdO0 curve.png

Figure 2: This figure outlines the energetics of the interaction between the DhdR allosteric transcription factor and the dhdO binding site. This allows for transcription of the downstream reporter protein sequence, resulting in brighter expression that is visible in our in vivo droplet system. Since D-2-HG levels are elevated due to the IDH1 mutation, we expect that there will be an increase in fluorescence or luminescence due to the release of the allosteric transcription factor caused by the binding of the upregulated oncometabolite. When we perform drug screening assays on our completed co-culture system, we will associate decreased fluorescence or luminescence with lower levels of D-2-HG, which is associated with a variety of downstream metabolic impacts.

Literature sources indicate that repressor binding can be affected by variables like the number of repeats of the binding site present, as well as the presence of spacer sequences in between repeats of the binding sequence. Because of these variations, we intend to test several different combinations to see which functions the best. By optimizing the binding site and promoter combination, we hope to establish a reporter system that allows for precise quantification of D-2-HG levels over a large dynamic range.

Sequence and Features


Assembly Compatibility:
  • 10
    INCOMPATIBLE WITH RFC[10]
    Illegal PstI site found at 820
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal PstI site found at 820
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    INCOMPATIBLE WITH RFC[23]
    Illegal PstI site found at 820
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal PstI site found at 820
  • 1000
    COMPATIBLE WITH RFC[1000]