Difference between revisions of "Team:Marburg/Results"

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                   Fig.1: Overview over the expansion of the Marburg Collection
 
                   Fig.1: Overview over the expansion of the Marburg Collection
 
                 </figcaption>
 
                 </figcaption>
               </figure><br>
+
               </figure><br> <br>
  
  
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     </section>
 
     </section>
  
               </p><br>
+
               </p><br><br>
               <p><u>Sequencing results of the LVL 0 parts</u></p>
+
               <p><u>Sequencing results of the lvl0 parts</u></p>
 
               <p>We built and validated 55 new BioBricks this year. They are all listed in the Registry of Standard
 
               <p>We built and validated 55 new BioBricks this year. They are all listed in the Registry of Standard
 
                 Biological Parts
 
                 Biological Parts
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                 </figure><br>
 
                 </figure><br>
  
               </p><br>
+
               </p><br><br>
 
               <p><u>Building constructs to test the lethality of origin of transfer</u></p>
 
               <p><u>Building constructs to test the lethality of origin of transfer</u></p>
 
               <p>If plasmids reach a certain size normal transformation protocols are not feasible anymore to bring
 
               <p>If plasmids reach a certain size normal transformation protocols are not feasible anymore to bring
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                 sequences) we built
 
                 sequences) we built
 
                 it into an integration vector. For sequencing results see the dropdown menu below.
 
                 it into an integration vector. For sequencing results see the dropdown menu below.
               </p><br>
+
               </p><br><br>
               <p><u>Sequencing results of the LVL 1 parts for modularized genome integrations</u></p>
+
               <p><u>Sequencing results of the lvl1 parts for modularized genome integrations</u></p>
 
               <p>We successfully build two integration cassettes from our rationally designed artificial neutral
 
               <p>We successfully build two integration cassettes from our rationally designed artificial neutral
 
                 integration sites
 
                 integration sites
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                   </figcaption>
 
                   </figcaption>
 
                 </figure><br>
 
                 </figure><br>
               </p><br>
+
               </p><br> <br>
 
               <p><u>Workflow to integrate a modularized integration cassette</u></p>
 
               <p><u>Workflow to integrate a modularized integration cassette</u></p>
 
               <p>We established a workflow on how to integrate a cassette - from LVL 0 Parts to a finished change in
 
               <p>We established a workflow on how to integrate a cassette - from LVL 0 Parts to a finished change in
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                   Fig.11: Workflow of integration
 
                   Fig.11: Workflow of integration
 
                 </figcaption>
 
                 </figcaption>
               </figure><br>
+
               </figure><br><br>
  
  
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                 </div>
 
                 </div>
 
               </div>
 
               </div>
               <br>
+
               <br><br>
 
               <p><u>Construction of a promoter library with standard measuring vectors</u></p>
 
               <p><u>Construction of a promoter library with standard measuring vectors</u></p>
 
               <p>We built a promoter library using our standard promoter measurement vector and 25 BioBricks.
 
               <p>We built a promoter library using our standard promoter measurement vector and 25 BioBricks.
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                 </figure><br>
 
                 </figure><br>
  
               </p><br>
+
               </p><br><br>
 
               <p><u>Workflow for the screen of a BioBrick library</u></p>
 
               <p><u>Workflow for the screen of a BioBrick library</u></p>
 
               <p>We designed a workflow to build a library, introduce it into UTEX2973 and measure its
 
               <p>We designed a workflow to build a library, introduce it into UTEX2973 and measure its
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                 </figure><br>
 
                 </figure><br>
  
               </p><br>
+
               </p><br><br>
  
 
               <p><u>Testing the reproducibility and standard deviation of the screening workflow</u></p>
 
               <p><u>Testing the reproducibility and standard deviation of the screening workflow</u></p>
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                   </figcaption>
 
                   </figcaption>
 
                 </figure><br>
 
                 </figure><br>
               </p><br>
+
               </p><br><br>
 
               <p><u>Application note for the characterization of BioBricks in our chassis</u></p>
 
               <p><u>Application note for the characterization of BioBricks in our chassis</u></p>
 
               <p>After calibrating our screening procedure, we decided to share our practical knowledge with other end
 
               <p>After calibrating our screening procedure, we decided to share our practical knowledge with other end

Revision as of 18:16, 8 December 2019

R E S U L T S


The way to the results we demonstrate here was full of success and failure. Therefore, it was necessary to compare and revise our theoretical plans with the practical work and the associated results. After trying our best to implement our plans, we would like to show you on this page that we have managed to realize some of our goals and are able to show some achievements for every sub-group.


S T R A I N
E N G I N E E R I N G


By genetic modification of S. elongatus UTEX 2973 we succeeded the transformation of plasmids in UTEX 2973.

M A R B U R G
C O L L E C T I O N  2.0


We expanded the Marburg Collection by adding the Green expansion and the first MoClo compatible shuttle vector for Cyanobacteria.