Team:Toulouse/Notebook/project-monitoring

From 2014.igem.org

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<p class="title2">EcAMP</p>
<p class="title2">EcAMP</p>
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<p class="texte">The EcAMP part was sent by the Utah iGEM team. It was on a pUC plasmid (ampicilin resistance) with biobrick suffix and prefix.</p>
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<p class="texte">The EcAMP part was sent by the Utah iGEM team. It was on a pUC plasmid (ampicilin resistance) with BioBrick suffix and prefix.</p>
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<p class="title2">1. Transformation of EcAMP in Escherichia coli MC 1061</p>
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<p class="title2">1. Transformation of EcAMP in <i>Escherichia coli</i> MC 1061</p>
<p class="texte"><b>Date:</b> 07/25/2014</p>
<p class="texte"><b>Date:</b> 07/25/2014</p>
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<p class="title2">2. Spreading of coli cells transformed with pUC + Utah </p>
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<p class="title2">2. Spreading of coli cells transformed with EcAMP (plasmid pUC) </p>
<p class="texte"><b>Date:</b> 07/28/2014</p>
<p class="texte"><b>Date:</b> 07/28/2014</p>
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<p class="title2">3. Liquid culture + Miniprep + Test of the miniprep</p>
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<p class="title2">3. Liquid culture, Miniprep and Test of the miniprep</p>
<p class="texte"><b>Date:</b> 07/30/2014</p>
<p class="texte"><b>Date:</b> 07/30/2014</p>
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<p class="title2">4. Cloning 1: EcAMP + Pveg + RBS</p>
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<p class="title2">4. Cloning 1: EcAMP + P<sub>veg</sub> + RBS</p>
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<p class="title3">Digestion of EcAMP (INSERT) by XbaI and PstI</p>
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<p class="title3">Digestion of EcAMP (insert) by XbaI and PstI</p>
<p class="texte"><b>Date:</b> 07/31/2014</p>
<p class="texte"><b>Date:</b> 07/31/2014</p>
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<p class="title3">Digestion of Pveg + RBS (VECTOR)</p>
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<p class="title3">Digestion of P<sup>veg</sup> + RBS (VECTOR)</p>
<p class="texte"><b>Date:</b> 07/31/2014</p>
<p class="texte"><b>Date:</b> 07/31/2014</p>
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<p class="texte"><b>Date:</b> 08/05/2014
<p class="texte"><b>Date:</b> 08/05/2014
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<br>The first cloning show a lack of DNA in the Miniprep EcAMP. The bands are hardly visible on the gel for the linearization of EcAMP + Pveg + RBS. The problem came from the PCR cleanup step: the fragment size of EcAMP is lower than 200bp.</p>
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<br><b>Result:</b> The first cloning show a lack of DNA in the Miniprep EcAMP. The bands are hardly visible on the gel for the linearization of EcAMP + Pveg + RBS. The problem came from the PCR cleanup step: the fragment size of EcAMP is lower than 200bp.</p>
<p class="title2">5. Cloning 2: EcAMP + Pveg + RBS </p>
<p class="title2">5. Cloning 2: EcAMP + Pveg + RBS </p>
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<p class="texte"><b>Date:</b> 06/08/2014</p>
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<p class="texte"><b>Date:</b> 08/06/2014</p>
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<p class="title3">Digestion of EcAMP (INSERT) by XbaI and PstI</p>
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<p class="title3">Digestion of EcAMP (insert) by XbaI and PstI</p>
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<p class="title3">Digestion of Pveg + RBS (VECTOR)</p>
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<p class="texte"><b>Date:</b> 08/06/2014</p>
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<p class="title3">Digestion of P<sub>veg</sub> + RBS (vector)</p>
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<p class="texte"><b>Date:</b> 08/06/2014</p>
<p class="title3">Heat inactivation of the enzymes</p>
<p class="title3">Heat inactivation of the enzymes</p>
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<p class="texte"><b>Date:</b> 08/06/2014</p>
<p class="title3">Ligation and transformation</p>
<p class="title3">Ligation and transformation</p>
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<p class="texte"><b>Date:</b> 08/06/2014</p>
<p class="title3">PCR test</p>
<p class="title3">PCR test</p>
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<p class="texte"><b>Date:</b> 07/08/2014</p>
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<p class="texte"><b>Date:</b> 08/07/2014</p>
<p class="title3">Striation on a petri dish to purify the clone</p>
<p class="title3">Striation on a petri dish to purify the clone</p>
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<p class="texte">Purpose: to isolate a clone with vector+insert
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<p class="texte"><b>Purpose:</b> to isolate a clone with vector+insert
<br><b>Date:</b> 08/072014</p>
<br><b>Date:</b> 08/072014</p>
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<p class="title3">Miniprep of Pveg+SpoVG+EcAMP and analytic digestion</p>
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<p class="title3">Miniprep of P<sub>veg</sub> + SpoVG + EcAMP and analytic digestion</p>
<p class="texte"><b>Date:</b> 08/08/2014</p>
<p class="texte"><b>Date:</b> 08/08/2014</p>
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<p class="title3">Ligation of Pveg SpoVG EcAMP with double terminateur B0015 +Transformation and liquid culture</p>
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<p class="title3">Ligation of Pveg SpoVG EcAMP with double terminateur B0015 + transformation and liquid culture</p>
<p class="texte"><b>Date:</b> 08/11/2014</p>
<p class="texte"><b>Date:</b> 08/11/2014</p>
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<p class="title3">Miniprep of Pveg SpoVG EcAMP + analytic digestion</p>
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<p class="title3">Miniprep of P<sub>veg</sub> SpoVG EcAMP + analytic digestion</p>
<p class="texte"><b>Date:</b> 08/13/2014</p>
<p class="texte"><b>Date:</b> 08/13/2014</p>
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<p class="title3">Cloning K1364011 (EcAMP+Pveg +SpoVG + B0015) + K823022 (psBbs4S) : Digestion, ligation, transformation</p>
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<p class="title3">Cloning K1364011 (EcAMP + P<sub>veg</sub> +SpoVG + B0015) + K823022 (pSB<sub>BS</sub>4S): Digestion, ligation, transformation</p>
<p class="texte"><b>Date:</b> 08/19/2014</p>
<p class="texte"><b>Date:</b> 08/19/2014</p>
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<p class="title3">Cloning K1364011 + K823023 (pSBBS1C) : Digestion, ligation, transformation</p>
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<p class="title3">Cloning K1364011 + K823023 (pSB<sub>BS</sub>1C) : Digestion, ligation, transformation</p>
<p class="texte"><b>Date:</b> 08/18/2014</p>
<p class="texte"><b>Date:</b> 08/18/2014</p>
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<p class="title3">Verification of the insertion of K1364011 + K823022 (pSBBS4S) into the subtilis genome by threonine test </p>
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<p class="title3">Verification of the insertion of K1364011 + K823022 (pSB<sub>BS</sub>4S) into the subtilis genome by threonine test </p>
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<p class="texte"><b>Date:</b> 08/21/2014
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<p class="texte"><b>Date:</b> 08/21/2014</p>
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<br>
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<p class="title2">Assembling the fungicides module: D4E1 + GAFP1 </p>
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<br>Assembling the fungicides module : </p>
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<p class="title2">D4E1 + GAFP1 </p>
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<p class="title2">1.  Cloning GAFP1+D4E1 on pSB1C3: <a href="http://parts.igem.org/Part:BBa_K1364012">BBa_K1364012</a></p>
<p class="title2">1.  Cloning GAFP1+D4E1 on pSB1C3: <a href="http://parts.igem.org/Part:BBa_K1364012">BBa_K1364012</a></p>

Revision as of 19:30, 17 October 2014