Team:Lyon-INSA/notebook

From 2012.igem.org

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                       <titre>Surfactant</titre>
                       <titre>Surfactant</titre>
<description>
<description>
 +
<ul>
 +
<li>One of the 12 screened clones transformed with the ligation of pBK22 and pBK39 has the expected fragments. Unfortunately, the plasmid is mixed with another one. To separate the two plasmids we decided to transform 1 µL of the miniprep into the NM522 <i>E. coli</i> strain.</li>
 +
<li>Another 6 clones with the transformed 3A ligation (done on August 29th) are screened.</li>
 +
<li>Standard ligation of the abrB gene and the plasmid containing lacI in pSB1C3 backbone (pBK37) and transformation. In parallel, another ligation is attempted : [pBK37 + pBK29].</li>
 +
</ul>
 +
</description>
 +
                      </jour>
 +
<jour nb="2">
 +
                      <date>Sunday, September 2nd 2012</date>
 +
                      <titre>For all purposes</titre>
 +
<description>
 +
Liquid cultures containing the modified shuttle vectors with the iGEM linker are inoculated and incubated over night.
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</description>
 +
                      <titre>Kill</titre>
 +
<description>
 +
Shuttle vector containing the lysostaphin is treated with an alcaline phosphatase, then a ligation with the dispersin is realised followed by transformation in NM522 <i>E. coli</i> strain.
 +
</description>
 +
                      <titre>Surfactant</titre>
 +
<description>
 +
<ul>
 +
<li>Plasmids from the 6 clones containing the 3A ligation are extracted and digested. Gel electrophoresis showed that one of the clones has the expected fragments. However, it was mixed with another plasmid. In order to separate them, we decided to transform the NM522 strain with 1µL of the miniprep.</li>
 +
<li>12 clones for each ligation (done the day before) are screened.</li>
 +
</ul>
</description>
</description>
                       </jour>
                       </jour>
 +
 +
<jour nb="3">
 +
                      <date>Monday, September 3rd 2012</date>
 +
                      <titre>For all purposes</titre>
 +
<description>
 +
Midiprep of the cloned shuttle vectors (containing the iGEM linker).
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</description>
 +
                      <titre>Kill</titre>
 +
<description>
 +
Transformations of BS 168 :
 +
<ul>
 +
      <li>Trial n°1 : negative control with H<sub>2</sub>O, positive control with pHT315 GFP (pBK18), transformation with Lysostaphin in pBK25 (=pBK28).</li>
 +
      <li>Trial n°2 : negative control with H<sub>2</sub>O, positive control with pHT315 GFP (pBK18), transformation with Lysostaphin in pBK26 (=pBK38).</li>
 +
</ul>
 +
The bacteria are spread on GL+Ery plates ([ERY]=1 µg/mL and [ERY]=10 µg/mL).
 +
</description>
 +
                      <titre>Surfactant</titre>
 +
<description>
 +
<ul>
 +
<li>abrB gene obtained by PCR was cloned in pSB1T3 backbone.</li>
 +
<li>6 clones transformed with the mixture of two plasmids are screened.</li>
 +
<li>Miniprep of 12 clones per transformed ligation : only one had the expected fragments (ligation of the lacI and abrB genes). The clone is put in storage under the reference pBK39.</li>
 +
</ul>
 +
</description>
 +
                      </jour>
 +
</month>
</month>

Revision as of 00:16, 18 September 2012


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