Team:Lyon-INSA/notebook

From 2012.igem.org

(Difference between revisions)
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                       <titre>Kill</titre>
                       <titre>Kill</titre>
<description>
<description>
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Miniprep of the clones BS 168 transformed by pBK26, pBK28 : we use the same protocol as DNA extraction for <i>E.coli</i> with addition of Lysozyme to the buffer A1. Electrophoresis to analyze extracted DNA : there is nothing on the gel → Maybe the DNA isn’t concentrated enough ?<br />
+
Miniprep of the clones Bs 168 transformed by pBK26, pBK28 : we use the same protocol as DNA extraction for <i>E.coli</i> with addition of Lysozyme to the buffer A1. Electrophoresis to analyze extracted DNA : there is nothing on the gel → Maybe the DNA isn’t concentrated enough ?<br />
New clones are put in liquid cultures in order to make other minipreps.  
New clones are put in liquid cultures in order to make other minipreps.  
</description>
</description>
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</ul>
</ul>
</description>
</description>
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<titre>P<sub>lac</sub> and P<sub>xyl</sub> kinetics</titre>
+
<titre>Plac and Pxyl kinetics</titre>
<description>
<description>
<ul>
<ul>
-
<li>Measurement of the NM522 + P<sub>lac</sub> kinetics (with Cm) during 12h in a 96 wells plate with and without different IPTG concentration addition. (1 mM; 0.5mM and 0.1mM)</li>
+
<li>Measurement of the NM522 + P<sub>lac</sub> kinetics (with Cm) during 12h in a 96 well plate with and without different IPTG concentration addition. (1 mM; 0.5mM and 0.1mM)</li>
-
<li>In the same 96 wells plate NM522 + P<sub>xyl</sub> kinetics is also measured during 12h with and without different xylose concentration. (2%; 0.5% and 0.2%)</li>
+
<li>In the same 96 well plate NM522 + P<sub>xyl</sub> kinetics is also measured during 12h with and without different xylose concentration. (2%; 0.5% and 0.2%)</li>
<li>Results : kinetics decreases so there is a problem. But it can be explained by the fact that the promoters need to be activated by a sigma factor which is active in the exponential phase and 12h is not enough. So this experiment has to be done during 24h.</li>
<li>Results : kinetics decreases so there is a problem. But it can be explained by the fact that the promoters need to be activated by a sigma factor which is active in the exponential phase and 12h is not enough. So this experiment has to be done during 24h.</li>
</ul>
</ul>
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<description>
<description>
<ul>
<ul>
-
<li>Seeding a 96 wells plate with <i>S. aureus</i> to produce a biofilm. Addition of supernatant of Bs168+pBK25 or Bs168+pBK26 or Bs168+pBK28 or Bs168+disp in pBK26 and Romain Briandet’s strains (Bs168+pWG200) with different dilutions (straight, 1/10, 1/100).(plate 1)</li>
+
<li>Seeding a 96 well plate with <i>S. aureus</i> to produce a biofilm. Addition of supernatant of Bs168+pBK25 or Bs168+pBK26 or Bs168+pBK28 or Bs168+disp in pBK26 and Romain Briandet’s strains (Bs168+pWG200) with different dilutions (straight, 1/10, 1/100).(plate 1)</li>
-
<li>Seeding a 96 wells plate with <i>S. aureus</i> to produce a biofilm (plate 2).</li>
+
<li>Seeding a 96 well plate with <i>S. aureus</i> to produce a biofilm (plate 2).</li>
</ul>
</ul>
</description>
</description>
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<description>
<description>
<ul>
<ul>
-
<li>Seeding of 2 96 wells plate with <i>S. aureus</i> to produce a biofilm. Addition of supernatant of Bs168+pBK25 or Bs168+pBK26 or Bs168+pBK28 or Bs168+dispersin in pBK26 and Romain Briandet's strain (Bs168+pWG200) with different dilutions (straight, 1/10, 1/100).(plate 1)</li>
+
<li>Seeding of 2 96 well plate with <i>S. aureus</i> to produce a biofilm. Addition of supernatant of Bs168+pBK25 or Bs168+pBK26 or Bs168+pBK28 or Bs168+dispersin in pBK26 and Romain Briandet's strain (Bs168+pWG200) with different dilutions (straight, 1/10, 1/100).(plate 1)</li>
<li>OD<sub>600</sub> measurements with filtered supernatants.</li>
<li>OD<sub>600</sub> measurements with filtered supernatants.</li>
<li>Mobility test of Bs168  on agar 0.25% plate.</li>
<li>Mobility test of Bs168  on agar 0.25% plate.</li>
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<jour nb="21">
<jour nb="21">
<date>Friday, September 21st 2012</date>
<date>Friday, September 21st 2012</date>
-
<titre>P<sub>lac</sub> and P<sub>xyl</sub> kinetics</titre>
+
<titre>Plac and Pxyl kinetics</titre>
<description>
<description>
A 7-hour-long kinetics is made with P<sub>lac</sub> and P<sub>xyl</sub> to be sure to have measurement in the exponential phase. Only one IPTG and xylose concentration is used.
A 7-hour-long kinetics is made with P<sub>lac</sub> and P<sub>xyl</sub> to be sure to have measurement in the exponential phase. Only one IPTG and xylose concentration is used.

Revision as of 19:25, 25 September 2012


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