Team:Lyon-INSA/notebook

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<li>6 clones transformed with the mixture of two plasmids are screened.</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>
<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>
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</ul>
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</description>
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                      </jour>
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<jour nb="4">
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                      <date>Tuesday, September 4th 2012</date>
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                      <titre>For all purposes</titre>
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<description>
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Multiple tubes containing LB media and Ampicillin at different concentrations ranging from 0 to 1,3 mg/mL are inoculated with bacteria containing the shuttle vectors (pBK35 and pBK36).
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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>Results of the transformations of BS 168 : not coherent. However, the problem seems to be identified : it is the erythromycin solution. Indeed, the erythromycin must be diluted in ethanol and not in water and must be kept refrigerated at -20°C.</li>
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<li>Standard ligations between :
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      <ul>
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            <li>pLac in pSB1C3 (pBK9) digested by SpeI and PstI and [RBS-GFP] in pSB1T3 digested by XbaI and PstI;</li>
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            <li>pXyl (amplified by PCR) digested by SpeI and EcoRI and [RBS-GFP] in pSB1T3 digested by XbaI and EcoRI.</li>
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    </ul>
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These two ligation products are transformed in NM522 strain.</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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Gel electrophoresis showed that 5 clones out of 6 clones screened after the transformation with the miniprep containing two plasmids had the expected fragments. However, we had doubts and we decided to search for restriction sites in the sequences that the plasmid was supposed to contain to make sure we had the right construction. We found out that a digestion with EcoRV would give 5 fragments of different sizes, enough to confirm the presence of the expected genes. Unfortunately, the electrophoresis was disappointing.
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</description>
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                      <titre>Biofilm</titre>
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<description>
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<ul>
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<li>One plate with <i>S. epidermidis</i> to evaluate the adhesion.</li>
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<li>One plate with <i>S. epidermidis</i> + supernatant of different cultures (lysostaphin, dispersin...).</li>
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<li>Same plate as the one above one + crystal violet.</li>
</ul>
</ul>
</description>
</description>

Revision as of 00:30, 18 September 2012


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