Difference between revisions of "Team:Uppsala/Results"

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       <div class="header"> Summary </div>
 
       <div class="header"> Summary </div>
 
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       <div class="text">We successfully integrated all five steps of the FPP to zeaxanthin pathway into the <i>E. coli</i> chromosome. The result is an <i>E. coli</i> strain expressing zeaxanthin. We have created six BioBricks in two versions. One version which is sequence verified, producing our enzymes CaCCD2, CsADH2946 and UGTCs2 respectively with inducible promoters. The other version include the three respective enzymes with a consecutive promoter. We have also modeled all our enzymes. Above all, <b>we are the first</b> to purify and confirm activity of CsADH2946 as well as estimating the kinetic parameters.</div>
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       <div class="text">We successfully integrated all five steps of the FPP to zeaxanthin pathway into the E. coli chromosome. The result is a E. coli strain expressing zeaxanthin. We have created six BioBricks in two versions. One version which is sequence verified, producing our enzymes CaCCD2, CsADH2946 and UGTCs2 respectively with inducible promoters. The other version include the three respective enzymes with a consecutive promoter. We have also modelled all our enzymes. In addition to this <b>we are the first</b> to purify and confirm activity of CsADH2946 as well as estimating the kinetic parameters.</div>
       <div class="text">We created and combined the zeaxanthin producing strain with a plasmid containing the extended crocin pathway which gave us an <i>E. coli</i> strain including the entire production pathway from FPP to crocin. <b>In the end, we were able to identify, create and extensively characterize the pathway for <a href="https://2017.igem.org/Team:Uppsala/Demonstrate">crafting crocin.</a></b></div>
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       <div class="text">We created and combined the zeaxanthin producing strain with a plasmid containing the extended crocin pathway which gave us an E. coli strain including the entire production pathway from FPP to crocin. <b>In the end, we were able to identify, create and extensively characterize the pathway for crafting crocin</b>.
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Revision as of 20:31, 31 October 2017

<!DOCTYPE html> Results

Summary
We successfully integrated all five steps of the FPP to zeaxanthin pathway into the E. coli chromosome. The result is a E. coli strain expressing zeaxanthin. We have created six BioBricks in two versions. One version which is sequence verified, producing our enzymes CaCCD2, CsADH2946 and UGTCs2 respectively with inducible promoters. The other version include the three respective enzymes with a consecutive promoter. We have also modelled all our enzymes. In addition to this we are the first to purify and confirm activity of CsADH2946 as well as estimating the kinetic parameters.
We created and combined the zeaxanthin producing strain with a plasmid containing the extended crocin pathway which gave us an E. coli strain including the entire production pathway from FPP to crocin. In the end, we were able to identify, create and extensively characterize the pathway for crafting crocin.
Chromosomal integration:
Farnesyl Pyrophosphate (FPP) → Zeaxanthin
Step 1: CaCCD2
Zeaxanthin → Crocetin dialdehyde
  • Biobrick - Coding for the enzyme CaCCD2 with His-tag and Lac-inducible promoter, characterised with correct sequencing!
  • Homology model
  • Molecular dynamics - the model was stable!
  • Successfully combined with pathway and transformed into zeaxanthin strain!
Step 2: CsADH2946
Crocetin dialdehyde → Crocetin
Step 3: UGTCs2
Crocetin → Crocin