Difference between revisions of "Team:Tuebingen/Lab/Notebook"

Revision as of 16:47, 1 November 2017

iGem Tübingen 2017

Team Inspiration Results Human Practice Lab Attribution

Begin of 3-(((1-carboxypropan-2-yl)amino)methyl)-4-hydroxybenzoic acid synthesis in a small batch.

Duff- reaction and reductive amination occurred without problems.
Synthesis of 3-(((1-carboxypropan-2-yl)amino)methyl)-4-hydroxybenzoic acid in a large batch succeeded without problems. Various cleanup methods were tried but failed.

Various clean-up methods (extraction, recrystallization, chromatography) of chemical synthesis were tried, but failed. The product was stored in methanol at room temperature during this time, which might have reduced yield significantly.
Preparation for work in molecular biology lab (competent cells, media, agar-plates). Begin of cloning β-lactam-synthetases wild type (WT) and double mutant (DM) into pUWL.

No success in purification of 3-(((1-carboxypropan-2-yl)amino)methyl)-4-hydroxybenzoic acid.
Begin of cloning NovL, SimL, CouL and CloL into pUWL and pSB1C3.
The cloning of GyrB (S.aureus) plus Terminator BamHI/HindIII in pSB1C3 was started and finished successfully. Furthermore the GyrB (E.coli) was cloned into pSB4C5 under control of a arac-pBad promoter.
Additionally the Interlabstudy was carried out.
The work with S. coelicolor was started. Collection of spores from S.coelicolor M1146/Clo BG1 and Clo SA02 and inoculation of S. coelicolor M1146 / Clo BG1 for Clorobiocin production.

Extraction of Clorobiocin from S. coelicolor M1146 / Clo BG1. HPLC analysis showed very low yield which made further purification not feasible.
Cloning of CouL and CloL in pUWL was finished and conjugated into S. coelicolor M1146/SA02.
Cloning of SimL and NovL did not work and was stopped to focus on more important projects.
Cloning of BLS-WT in pSB1C3 was finished and confirmed by sequencing.
First feeding experiments of S.coelicolor M1156/Clo BG1, with unpurified 3-(((1-carboxypropan-2-yl)amino)methyl)-4-hydroxybenzoic acid was started. LC-MS showed neither product nor intermediate.

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                 <li>The work with S. coelicolor was started. Collection of spores from S.coelicolor M1146/Clo BG1 and Clo SA02 and inoculation of S. coelicolor M1146 / Clo BG1 for Clorobiocin production.</li>
           </ul>
+     <h2 id="September 2017">September 2017</h2>
+               <ul>
+               <li>Extraction of Clorobiocin from S. coelicolor M1146 / Clo BG1. HPLC analysis showed very low yield which made further purification not feasible. </li>
+               <li>Cloning of CouL and CloL in pUWL was finished and conjugated into S. coelicolor M1146/SA02.  </li>
+               <li>Cloning of SimL and NovL did not work and was stopped to focus on more important projects. </li>
+               <li>Cloning of BLS-WT in pSB1C3 was finished and confirmed by sequencing.
+</li>
+               <li>First feeding experiments of S.coelicolor M1156/Clo BG1, with unpurified 3-(((1-carboxypropan-2-yl)amino)methyl)-4-hydroxybenzoic acid was started. LC-MS showed neither product nor intermediate. </li>
+         </ul>
+ <h2 id="October 2017">October 2017</h2>
+               <ul>
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+               <li></li>
+               <li></li>
+               <li></li>
+               <li></li>
+               <li></li>
+               <li></li>