Team:Lyon-INSA/notebook

From 2012.igem.org

(Difference between revisions)
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<jour nb="15">
<jour nb="15">
<date>Saturday, September 15th 2012</date>
<date>Saturday, September 15th 2012</date>
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<titre>For all purposes</titre>
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<description>
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<ul>
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<li>Bacillus subtilis transformation with the 2 shuttle vectors pBK35 and pBK36.</li>
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</ul>
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</description>
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<titre>Kill</titre>
<titre>Kill</titre>
<description>
<description>
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LB plates containing a 0.3% agarose gel are inoculated with 5 μL of a 5 hour liquid culture of <i>B. subtilis</i> containing the plasmids used in transformations.
LB plates containing a 0.3% agarose gel are inoculated with 5 μL of a 5 hour liquid culture of <i>B. subtilis</i> containing the plasmids used in transformations.
</description>
</description>
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<titre>Surfactant</titre>
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<description>
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Transformation of the ligations between the plasmid pBK42 containing the construction [pXyl-sfp-abrB-lacI] and the shuttle vectors pBK35 and pBK36 into the NM522 strain .
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</description>
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</jour>
</jour>
<jour nb="16">
<jour nb="16">
<date>Sunday, September 16th 2012</date>
<date>Sunday, September 16th 2012</date>
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<titre>For all purposes</titre>
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<description>
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<ul>
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<li>Screening of 12 clones per Bacillus transformation;</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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Screening of 15 clones transformed with the liagtion pBK42+pBK35 and pBK42+pBK36
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</description>
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<titre>Physiological tests : Mobility of B. subtilis</titre>
<titre>Physiological tests : Mobility of B. subtilis</titre>
<description>
<description>
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<date>Monday, September 17th 2012</date>
<date>Monday, September 17th 2012</date>
 +
<titre>For all purposes</titre>
 +
<description>
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<ul>
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<li>LB plates were spread  with Erythromycin at different concentration in order to test the Erythromycin resistance of the <i>B. Subtilis</i> strain transformed with the shuttle vectors</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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<li>Unfortunately the screened clones (containing the ligations pBK42+pBK35 and pBK42+pBK36) did not have the right plasmid. Another ligation of the construction [pXyl-sfp-abrB-lacI] is attempted, this time after gel extraction and purification of the digested pBK42 plasmid with EcoRI and PstI. This way, the backbone is eliminated and the chances of ligating the construction instead of the plasmid are higher.</li>
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</description>
</jour>
</jour>
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<jour nb="18">
<jour nb="18">
<date>Tuesday, September 18th 2012</date>
<date>Tuesday, September 18th 2012</date>
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titre>For all purposes</titre>
 +
<description>
 +
<ul>
 +
 +
<li>Multiple tubes containing LB media supplemented with Erythromycin at different concentrations are inoculated with the <i>B. subtilis</i> strains containing the shuttle vectors pBK35 and pBK36 in order to test the antibiotic resistance. For the same purpose LB + Ery plates are spotted with the same cultures at different dilution ratios.</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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<li>30 clones containing the construction [pXyl-sfp-abrB-lacI]  in the shuttle vector are screened
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</li>
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</description>
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<jour nb="19">
<jour nb="19">
<date>Wednesday, September 19th 2012</date>
<date>Wednesday, September 19th 2012</date>
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<titre>For all purposes</titre>
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<description>
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<ul>
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<li>The strains that were supposed to contain the shuttle vectors did not grow, so we suspect that the clones  are in fact mutants</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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<li> Miniprep of the transformed clones with the construction [pXyl-sfp-abrB-lacI]. The gel electrophoresis shows that only  two of them have the expected fragments.
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</li>
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</description>
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</jour>
</jour>
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<jour nb="20">
<jour nb="20">
<date>Thursday, September 20th 2012</date>
<date>Thursday, September 20th 2012</date>
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 +
<titre>For all purposes</titre>
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<description>
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<ul>
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<li><i>Bacillus subtilis</i> transformation with the shuttle vectors pBK35 and pBK36</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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<li> Transformation of <i>B. subtilis 168</i> and <B. subtilis abrB> strains with the construction [pXyl-sfp-abrB-lacI] in the pBK35 shuttle vector.
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</li>
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</description>
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</jour>
</jour>
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<jour nb="22">
<jour nb="22">
<date>Saturday, September 22th 2012</date>
<date>Saturday, September 22th 2012</date>
 +
<titre>For all purposes</titre>
 +
<description>
 +
<ul>
 +
 +
<li>12 clones transformed with the shuttle vectors are screened</li>
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</ul>
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</description>
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<titre>Kill</titre>
<titre>Kill</titre>
<description>
<description>
A new SDS-PAGE is done for dispersin. A migration problem persists, due to ammonium persulfate.  
A new SDS-PAGE is done for dispersin. A migration problem persists, due to ammonium persulfate.  
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</description>
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<titre>Surfactant</titre>
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<description>
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<li> 24 clones transformed with the construction [pXyl-sfp-abrB-lacI] are screened;
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</li>
</description>
</description>
</jour>
</jour>
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<jour nb="23">
<jour nb="23">
<date>Sunday, September 23th 2012</date>
<date>Sunday, September 23th 2012</date>
 +
<titre>For all purposes</titre>
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<description>
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<ul>
 +
 +
<li>Multiple tubes containing  2 mL liquid LB media are supplemented with Erythromycin at various concentrations in order to test the antibiotic resistance of the two shuttle vectors. Also, LB+Ery plates are spotted with liquid cultures with the <i>B. subtilis </i> strains containing the shuttle vectors</li>
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</ul>
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</description>
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<titre>Kill</titre>
<titre>Kill</titre>
<description>
<description>
A last SDS-PAGE is run. This time the problems were succesfully solved. But the gels were not conclusive due to a low dispersin concentration.
A last SDS-PAGE is run. This time the problems were succesfully solved. But the gels were not conclusive due to a low dispersin concentration.
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</description>
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<titre>Surfactant</titre>
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<description>
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<li> 6 of the 24 clones are put in liquid culture for further testing in LB media supplemented with xylose at a concentration of 2%;
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</li>
</description>
</description>
</jour>
</jour>
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<jour nb="24">
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<date>Monday, September 24th 2012</date>
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<titre>For all purposes</titre>
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<description>
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<ul>
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<li> Both strains grew in all tubes. However, there is a difference concerning the OD between the two strains. The test is repeated (with antibiotic concentrations ranging from 0 to 1,5 mg/mL) in order to make sure there is a notable difference between the two strains. </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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<li> In order to characterize the construction [pXyl –sfo-abrB-lacI] two tests are made. To confirm the presence of the <i>sfp</i> gene, we made emulsions with the filtered supernatant of the transformed strains and sunflower oil. Concerning the <i>abrB</i>  gene, a biofilm formation test was made in a 24-well microplate in order to compare the transformed strain to the wild-type strain.
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</li>
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</description>
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</jour>
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<jour nb="25">
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<date>Tuesday, September 25th 2012</date>
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 +
<titre>For all purposes</titre>
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<description>
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<ul>
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<li>The results of the antibiotic resistance in liquid culture show that the <i>B. subtilis</i> strain containing pBK35 is less resistant than the one containing pBK36.</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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<li> The emulsion test and the biofilm formation test confirm the presence of <i>sfp</i> and <i>abrB</i> genes;
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</li>
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</description>
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</jour>
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</month>
</month>

Revision as of 23:40, 26 September 2012



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