Team:Lyon-INSA/notebook

From 2012.igem.org

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<titre>For all purposes</titre>
<titre>For all purposes</titre>
<date> Monday, July 2nd 2012</date>
<date> Monday, July 2nd 2012</date>
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<description>Liquid culture (5 mL LB media) of NM 522 cells and overnight incubation under agitation at 37°C for later transformation.</description>
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<description>Liquid culture (5 mL LB medium) of NM 522 cells and overnight incubation under agitation at 37°C for later transformation.</description>
</jour>
</jour>
                 <jour nb="3">
                 <jour nb="3">
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<ul>
<ul>
     <li>pBBa_I742123 was put in storage (under the reference pBK1).</li>
     <li>pBBa_I742123 was put in storage (under the reference pBK1).</li>
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     <li>A liquid culture of NM522/pBK1 transformed cells was made so we could extract more plasmid DNA (50 mL LB media + 500 µL Chloramphenicol + 500 µL liquid culture of transformed bacteria ).</li>
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     <li>A liquid culture of NM522/pBK1 transformed cells was made so we could extract more plasmid DNA (50 mL LB medium + 500 µL Chloramphenicol + 500 µL liquid culture of transformed bacteria ).</li>
     <li>The 3 genes coding for lysostaphin, dispersin and <i>lacI</i> repressor in pUC57 Ampicillin resistant plasmids were delivered.</li>
     <li>The 3 genes coding for lysostaphin, dispersin and <i>lacI</i> repressor in pUC57 Ampicillin resistant plasmids were delivered.</li>
     <li>Transformation of NM522 strain with pUC57-Lysostaphin, pUC57-Dispersin and pUC57-<i>sfp</i>.</li>
     <li>Transformation of NM522 strain with pUC57-Lysostaphin, pUC57-Dispersin and pUC57-<i>sfp</i>.</li>
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     <li>Extractions with a miniprep kit are made :
     <li>Extractions with a miniprep kit are made :
     <ul>
     <ul>
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             <li>4 clones containing the pLac promoter (1,2,3,4);</li>
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             <li>4 clones containing the P<sub>lac</sub> promoter (1,2,3,4);</li>
             <li>4 clones containing the <i>Bacillus subtilis</i> RBS (1,2,3,4);</li>
             <li>4 clones containing the <i>Bacillus subtilis</i> RBS (1,2,3,4);</li>
             <li>3 clones containing theTerminator (1,2,3);</li>
             <li>3 clones containing theTerminator (1,2,3);</li>
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     <li>Plasmid extraction from Bacillus strain (BT407 GFP). We tested 2 methods in parallel. However, only the one using the extraction kit seems to work.</li>
     <li>Plasmid extraction from Bacillus strain (BT407 GFP). We tested 2 methods in parallel. However, only the one using the extraction kit seems to work.</li>
     <li>Extraction of <i>gfp</i>, <i>cfp</i>, <i>yfp</i> ;  test → OK : put in storage.</li>
     <li>Extraction of <i>gfp</i>, <i>cfp</i>, <i>yfp</i> ;  test → OK : put in storage.</li>
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     <li>Extraction of the pHT315 GFP plasmid of <i>B. thuringiensis</i> 407 GFP to build a shuttle vector <i>B. subtilis</i> ↔ <i>E. coli</i>. Transformation in NM522 strain and selection on Ampicillin media : ok.</li>
+
     <li>Extraction of the pHT315 GFP plasmid of <i>B. thuringiensis</i> 407 GFP to build a shuttle vector <i>B. subtilis</i> ↔ <i>E. coli</i>. Transformation in NM522 strain and selection on LB+Ampicillin medium : ok.</li>
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     <li><i>S. epidermidis</i> is put in storage in TSB media under the reference BK15.</li>
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     <li><i>S. epidermidis</i> is put in storage in TSB medium under the reference BK15.</li>
</ul>
</ul>
</description>
</description>
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<ul>
<ul>
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<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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<li>Multiple tubes containing LB medium 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>
</ul>
</ul>
</description>
</description>
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<titre>Surfactant</titre>
<titre>Surfactant</titre>
<description>
<description>
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<li> 24 clones transformed with the construction [pXyl-<i>sfp</i>-<i>abrB</i>-<i>lacI</i>] are screened;  
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<li> 24 clones transformed with the construction [P<sub>xyl</sub>-<i>sfp</i>-<i>abrB</i>-<i>lacI</i>] are screened;  
</li>
</li>
</description>
</description>
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<ul>
<ul>
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<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>
+
<li>Multiple tubes containing  2 mL liquid LB medium 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>
</ul>
</ul>
</description>
</description>

Revision as of 00:42, 27 September 2012



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