Team:Lyon-INSA/notebook

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                       </jour>
                       </jour>
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<jour nb="28">
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Tuesday, 28th August
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                        <date>Tuesday, August 28th 2012</date>
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For all :
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                        <titre>For all purposes</titre>
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- Meeting at 1:30 pm
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<description>
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Kill:
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Meeting at 1:30 pm.
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- Ligation of Constitutive promoter-disp in the shuttle vector pBK25.
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</description>
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- Results of the transformation of BS 168 strain with the pBK28 (1) in the shuttle vector : the negative control is full of bacteria ⇒ Is the BS 168 strain resistant to erythromycin ? Or is the erythromycin concentration too low ?  
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                      <titre>Kill</titre>
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We make an other transformation and we spread the transformed bacteria on GL+Ery plates with different erythromycin concentration (from 5 µg/mL to 10 µg/mL).
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<description>
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Surfactant :
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<ul>
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<li>Ligation of [Constitutive promoter + Dispersin] in the shuttle vector pBK25.</li>
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<li>Results of the transformation of BS 168 strain with the pBK28 (1) in the shuttle vector : the negative control is full of bacteria ⇒ Is the BS 168 strain resistant to erythromycin ? Or is the erythromycin concentration too low ? <br />
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We made another transformation and we spread the transformed bacteria on GL+Ery plates with different erythromycin concentration (from 5 µg/mL to 10 µg/mL).</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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The transformations with the two ligations (3A ligation of pBK24, pBK4, pBK29, with two different insert/vector ratios ) was successful. 12 clones per transformation are put in liquid culture and then streaked on LB+Cm plates and LB+Amp plates.
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</description>
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                      </jour>
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the transformations with the two ligations (3A ligation of pBK24, pBK4, pBK29, with two different insert/vector ratios ) was successful. 12 clones per transformation are put in liquid culture and  then streaked on LB+Cm plates and LB+Amp plates.
 
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Stick :
 
   
   
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Revision as of 15:00, 11 September 2012


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