Team:Lyon-INSA/notebook

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</description>
                       </jour>
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<jour nb="16">
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                        <date>Thursday, August 16th 2012</date>
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                        <titre>For all purposes</titre>
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<description>
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The electrophoresis after digestion with EcoRI and SpeI showed that the SpeI site was eliminated. 4 clones were chosen for further tests. However, the DNA concentration was too low so the enzymes did not digest the plasmids.
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</description>
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                      <titre>Kill</titre>
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<description>
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<ul>
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<li>Ligation of the Constitutive promoter (pVeg) produced by PCR in an iGEM plasmid.</li>
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<li>Result of the lysostaphin tests : didn’t work again. The Bs 168 pWG100 supernatant doesn’t contain any lysostaphin : the lysostaphin is probably degraded in one way or another (sensitivity to the defrosting ?).</li>
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<li>Result of the transformation with [pSB1C3 + promoter] : a lot of red clones, some white clones (20 - 30). Isolation of 6 white clones and plasmid extractions by miniprep.</li>
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</ul>
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</description>
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                      <titre>Surfactant</titre>
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<description>
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<ul>
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<li>Two of the 6 [sfp+abrB] clones had the expected fragments.</li>
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<li>Ligation of pXyl produced by PCR in an iGEM plasmid.</li>
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</ul>
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</description>
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                      <titre>Stick</titre>
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<description>
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<ul>
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<li>Ligation of XylR produced by PCR in an iGEM plasmid (pSB1K3).</li>
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<li>Results of the transformation of NM522 by [pBK7 + XylR] (for the second ligation) : the plate with bacteria transformed by [pBK7 + XylR] contains a lot of clones and the controls are standard. 14 clones are selected to do liquid culture and extract their DNA.</li>
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<li>Plasmid extractions from the 8 clones transformed by [pBK7 + XylR]. The electrophoresis of the digested plasmids showed that the clones do not have the right plasmid : they have just the vector without XylR.</li>
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</ul>
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</description>
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                      </jour>
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___________________________________________________________________________________
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Friday, 17th August :
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For all :
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- The plasmids (pBK19 and pBK20) from 2 clones were re-extracted using columns. This time the digestion was successful. The tests showed that there was no SpeI site. However, the pHT315 plasmid also had no XbaI site.
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Stick :
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- Plasmid extractions from the 14 clones transformed by PBK7+XylR (with the second ligation). Like for the first transformation, the electrophoresis of the digested plasmids showed that the clones have not the right plasmid : they have just the vector without XylR.

Revision as of 16:52, 10 September 2012


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