Team:Toulouse/Notebook/Calendar

From 2014.igem.org

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   <p style="color:#696969; padding-top:20px; font-size:16px; float:left;"> Notebook&nbsp;&nbsp;&nbsp;>&nbsp;&nbsp;&nbsp;Calendar</p>  
   <p style="color:#696969; padding-top:20px; font-size:16px; float:left;"> Notebook&nbsp;&nbsp;&nbsp;>&nbsp;&nbsp;&nbsp;Calendar</p>  
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       <div class="centering" style="padding-top: 85px; padding-bottom:40px;">
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<p style="font-size:1.3em; margin: 0 0 30px 0;"><a href="#" onClick="ddaccordion.expandall('technology'); return false">Expand all</a> | <a href="#" onClick="ddaccordion.collapseall('technology'); return false">Collapse all</a></p>
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<p class="texte">
<p class="texte">
- iGEM competition presentation and explanations<br/>
- iGEM competition presentation and explanations<br/>
-
- Constitution of the team by interviewing different students from Université Paul Sabatier and INSA<br/>
+
- Constitution of the team by interviewing different students from Université Paul Sabatier and INSA
</p>
</p>
<p class="texte" style="text-align:center"><B> The adventure begins for the 2014 Toulouse iGEM Team ! </B>
<p class="texte" style="text-align:center"><B> The adventure begins for the 2014 Toulouse iGEM Team ! </B>
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<div class="technology">January – June 2014: Projects brainstorming</div>
<div class="technology">January – June 2014: Projects brainstorming</div>
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<br/>
<br/>
- Reduction of ruminants’ methane production: the goal is to reduce the production of methane by ingesting a microorganism in the animals' rumen. This bacterium would be able to reduce the quantity of metabolic hydrogen and eliminate the methanogenic Archaes population.
- Reduction of ruminants’ methane production: the goal is to reduce the production of methane by ingesting a microorganism in the animals' rumen. This bacterium would be able to reduce the quantity of metabolic hydrogen and eliminate the methanogenic Archaes population.
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<br/>
 
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<div class="technology">June 2014: Choice of SubtiTree project</div>
<div class="technology">June 2014: Choice of SubtiTree project</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="texte">The discussion has been long to estimate the practicability of our final project. By the end of June, most of the ideas were eliminated but two of them remained: controlling the cancer or saving the trees. It became easily clear that SubtiTree was successfully completed whether regarding the scientific part or the ethical aspect. Indeed, our knowledge in medicine was not sufficient enough to evaluate the consequences of a bacterium injection in the human body for <i>E. coli</i> cancer.</br>
<p class="texte">The discussion has been long to estimate the practicability of our final project. By the end of June, most of the ideas were eliminated but two of them remained: controlling the cancer or saving the trees. It became easily clear that SubtiTree was successfully completed whether regarding the scientific part or the ethical aspect. Indeed, our knowledge in medicine was not sufficient enough to evaluate the consequences of a bacterium injection in the human body for <i>E. coli</i> cancer.</br>
Therefore, the whole team agreed on focusing on a local issue as the preservation of the Canal du Midi plane trees. However, the final goal was based on the idea to allow our optimized bacteria to be efficient for all fungi infections in the environment.</br>
Therefore, the whole team agreed on focusing on a local issue as the preservation of the Canal du Midi plane trees. However, the final goal was based on the idea to allow our optimized bacteria to be efficient for all fungi infections in the environment.</br>
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<div class="technology2">Week 1(16-22 June)</div>
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<div class="technology">Week 1(16-22 June)</div>
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<div class="thelanguage">
<div class="thelanguage">
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<p class="texte">
<p class="texte">
- Bibliography researches about our subject<br/>
- Bibliography researches about our subject<br/>
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- Increase in our communication strategy to find more sponsors specialized in environment and ecological matters <br/>
- Increase in our communication strategy to find more sponsors specialized in environment and ecological matters <br/>
- Support of Adisseo, Toulouse White Biotechnology, LISBP, INSA Toulouse<br/>
- Support of Adisseo, Toulouse White Biotechnology, LISBP, INSA Toulouse<br/>
-
- Organization of a weekly meeting each Friday with our supervisors to tackle any problem encountered<br/>
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- Organization of a weekly meeting each Friday with our supervisors to tackle any problem encountered
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<div class="technology">Week 2 (23-29 June)</div>
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<div class="technology2">Week 2 (23-29 June)</div>
<div class="thelanguage">
<div class="thelanguage">
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-
 
<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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<p class="title3">Lab work:</p>
<p class="title3">Lab work:</p>
<p class="texte">
<p class="texte">
-
- E. coli transformation with BBA_J004450 (pSB1C3)<br/>
+
- E. coli transformation with BBA_J004450 (pSB1C3)
</p>
</p>
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- Check the mechanism of action of each fungicide to complete the ethical part
- Check the mechanism of action of each fungicide to complete the ethical part
</p>
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<p class="title1" id="select4">July 2014</p>
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 +
<div class="technology">July 2014</div>
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<div class="thelanguage">
<p class="title2">Main activities</p>
<p class="title2">Main activities</p>
<p class="texte">
<p class="texte">
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<div class="technology">Week 3 (30 June -6 July) and Week 4 (7-13 July)</div>
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<div class="technology2">Week 3 (30 June -6 July) and Week 4 (7-13 July)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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<div class="technology">Week 5 (14-20 July)</div>
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<div class="technology2">Week 5 (14-20 July)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="texte">
<p class="texte">
- Our team was interviewed by many local newspapers such as 20minutes, Metronews, La Voix du Midi, La Dépêche but also by the local television channel France3 Midi-Pyrénées to present our draft to the community. Moreover, SubtiTree was approached in some radio programs like Virgin Radio Toulouse and France info.</br>
- Our team was interviewed by many local newspapers such as 20minutes, Metronews, La Voix du Midi, La Dépêche but also by the local television channel France3 Midi-Pyrénées to present our draft to the community. Moreover, SubtiTree was approached in some radio programs like Virgin Radio Toulouse and France info.</br>
-
- Support of ThermoFisher, New Englands BioLabs, Qiagen, Eurofins but also GenoToul, Labex Tulip, L’Université Paul Sabatier, CROUS.
+
- Support of ThermoFisher, New Englands BioLabs, Qiagen, Eurofins but also GenoToul, Labex Tulip, L’Université Paul Sabatier, CROUS.</p>
<p class="title3">Lab work:</p>
<p class="title3">Lab work:</p>
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- Transformation and cryopreservation of biobricks BBa_K823002 (PlepA), BBa_K823003 (Pveg), BBa_K606061 (RBS SpoVG) and BBa_B0015 (double terminator), BBa_K823023 (pSBBS1C), BBa_K733013 (Pveg+ RBS) in <i>E. coli</i>.<br/>
- Transformation and cryopreservation of biobricks BBa_K823002 (PlepA), BBa_K823003 (Pveg), BBa_K606061 (RBS SpoVG) and BBa_B0015 (double terminator), BBa_K823023 (pSBBS1C), BBa_K733013 (Pveg+ RBS) in <i>E. coli</i>.<br/>
- Transformation of the Munich B. subtilis backbones<br/>
- Transformation of the Munich B. subtilis backbones<br/>
-
- Cloning of BBa_K606061 (RBS SpoVG) with BBa_K823003 (PvEG) and BBa_K823002 (PlepA)<br/>
+
- Cloning of BBa_K606061 (RBS SpoVG) with BBa_K823003 (PvEG) and BBa_K823002 (PlepA)
</p>
</p>
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<div class="technology">Week 6 (21 July-27 July)</div>
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<div class="technology2">Week 6 (21 July-27 July)</div>
<div class="thelanguage">
<div class="thelanguage">
<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
-
- Description of SubtiTree project and determination of the goodies for a crowdfunding campaign on Ulule website
+
- Description of SubtiTree project and determination of the goodies for a crowdfunding campaign on Ulule website</p>
<p class="title3">Lab work:</p>
<p class="title3">Lab work:</p>
<p class="texte">
<p class="texte">
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- PCR and migration on electrophoresis gel<br/>
- PCR and migration on electrophoresis gel<br/>
- Transformation BBA_1364003 (D4E1)  on pSB1C3 and BBA_1364002 (GAFP1) on pSB1C3<br/>
- Transformation BBA_1364003 (D4E1)  on pSB1C3 and BBA_1364002 (GAFP1) on pSB1C3<br/>
-
- Cloning BBA_1364002 (GAFP1) with BBa_B0015 (double terminator) and BBA_1364003 (D4E1) with BBa_K823003 (Pveg)<br/>
+
- Cloning BBA_1364002 (GAFP1) with BBa_B0015 (double terminator) and BBA_1364003 (D4E1) with BBa_K823003 (Pveg)
</p>
</p>
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<p class="texte">
<p class="texte">
- Research for plane tickets and hotels in Boston for the Giant Jamboree<br/>
- Research for plane tickets and hotels in Boston for the Giant Jamboree<br/>
-
- New idea: analyze the plane tree sap to determine its composition<br/>
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- New idea: analyze the plane tree sap to determine its composition
</p>
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<div class="technology">August 2014 </div>
<div class="technology">August 2014 </div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title2">Main activities</p>
<p class="title2">Main activities</p>
<p class="texte">
<p class="texte">
- Finishing the cloning for the different parts of the bacterium<br/>
- Finishing the cloning for the different parts of the bacterium<br/>
-
- Putting in place the fungicides, binding and chemotaxis tests<br/>
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- Putting in place the fungicides, binding and chemotaxis tests
</p>  
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<div class="technology">Week 7 (28 July-3 August)</div>
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<div class="technology2">Week 7 (28 July-3 August)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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- Cloning of BBa_K823002 (PlepA) + RFP (BBa_K1364016)  in pSBBs4S (BBa_K823022), subculture and minipreps<br/>
- Cloning of BBa_K823002 (PlepA) + RFP (BBa_K1364016)  in pSBBs4S (BBa_K823022), subculture and minipreps<br/>
- Cloning of BBa_1364018 (Strong Promotor + RFP)<br/>
- Cloning of BBa_1364018 (Strong Promotor + RFP)<br/>
-
- Cloning of BBA_1364003 (D4E1) + BBA_1364002 (GAFP1) + Promotor BBa_K823003 (Pveg) biobirck BBa_K1364012 with gel extraction for BBA_1364003 (D4E1) + BBA_1364002 (GAFP1)  and a PCR cleanup for BBa_K823003 (Pveg), subculture<br/>
+
- Cloning of BBA_1364003 (D4E1) + BBA_1364002 (GAFP1) + Promotor BBa_K823003 (Pveg) biobrick BBa_K1364012 with gel extraction for BBA_1364003 (D4E1) + BBA_1364002 (GAFP1)  and a PCR cleanup for BBa_K823003 (Pveg), subculture<br/>
- Cloning BBa_K823003 (Pveg) + BBA_1364002 (GAFP1) + BBa_B0015 (double terminator) on pSBBS4S in <i>E. coli</i><br/>
- Cloning BBa_K823003 (Pveg) + BBA_1364002 (GAFP1) + BBa_B0015 (double terminator) on pSBBS4S in <i>E. coli</i><br/>
- Transformation of binding gene with <i>E. coli</i> competent cells<br/>
- Transformation of binding gene with <i>E. coli</i> competent cells<br/>
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- Spreading of BBa_K1162001 (EcAMP), miniprep and digestion<br/>
- Spreading of BBa_K1162001 (EcAMP), miniprep and digestion<br/>
Problem: the digestion did not work => Issue with the quantity of DNA in the miniprep is assumed<br/>
Problem: the digestion did not work => Issue with the quantity of DNA in the miniprep is assumed<br/>
-
- First experience of chemotaxis with a glucose chemo-attractant<br/>
+
- First experience of chemotaxis with a glucose chemo-attractant
</p>
</p>
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- Discussion about EcAMP cloning which presents some issues
- Discussion about EcAMP cloning which presents some issues
<br/>
<br/>
-
- Discussion about the transfer of pSB1C3 from <i>E. coli</i> to <i>Bacillus</i> strain
+
- Discussion about the transfer of pSB1C3 from <i>E. coli</i> to <i>B. subtilis</i> strain
</p>  
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<div class="technology">Week 8 (04-10 August)</div>
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<div class="technology2">Week 8 (04-10 August)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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- Elaboration of an efficient fungicide test protocol  
- Elaboration of an efficient fungicide test protocol  
<br/>
<br/>
-
- Test of the fungus growth on PDA medium + test of growth for <i>Bacillus subtilis</i> liquid culture on PDA
+
- Test of the fungus growth on PDA medium + test of growth for <i>B. subtilis</i> liquid culture on PDA
</p>
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- Ask iGEM headquarters if all the biobricks must be on pSB1C3 plasmid
- Ask iGEM headquarters if all the biobricks must be on pSB1C3 plasmid
<br/>
<br/>
-
- Use another strain of i>E. coli</i> (DH5-1 instead of DH5 alpha) to have a faster growth
+
- Use another strain of <i>E. coli</i> (DH5-1 instead of DH5 alpha) to have a faster growth
<br/>
<br/>
-
- Check which quantity of <i>Bacillus subtilis</i> is necessary to naturally destroy the fungus
+
- Check which quantity of <i>B. subtilis</i> is necessary to naturally destroy the fungus
</p>
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<div class="technology">Week 9 (11-17 August)</div>
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<div class="technology2">Week 9 (11-17 August)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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<p class="title2">Lab work:</p>
<p class="title2">Lab work:</p>
<p class="texte">
<p class="texte">
-
- Evaluation of the bacterial decrease rate from 10°C to 4°C with a sporuling strain of <i>Bacillus subtilis</i>.
+
- Evaluation of the bacterial decrease rate from 10°C to 4°C with a sporuling strain of <i>B. subtilis</i>.
<br/>
<br/>
- Chemotaxis test with different concentrations of glucose on a 0.3% agar.
- Chemotaxis test with different concentrations of glucose on a 0.3% agar.
<br/>
<br/>
-
- Miniprep of pSBBs4S with binding gene and transformation in <i>Bacillus subtilis</i>.
+
- Miniprep of pSBBs4S with binding gene and transformation in <i>B. subtilis</i>.
<br/>
<br/>
Problem: no digestion was visible on the gel => the cloning failed
Problem: no digestion was visible on the gel => the cloning failed
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- Transformation of BBa_K1374010 (Pveg + RBS SpoVG + EcAMP) + BBa_K1364012 (RBS + Gafp1 + D4E1 + double terminator), subculture
- Transformation of BBa_K1374010 (Pveg + RBS SpoVG + EcAMP) + BBa_K1364012 (RBS + Gafp1 + D4E1 + double terminator), subculture
<br/>
<br/>
-
- Subculture of Bacillus subtilis clones transformed by BBa_K823003 (Pveg) + BBA_1364002 (GAFP1)  + BBa_B0015 (double terminator) in pSBBs4S, cryopreservation
+
- Subculture of <i>B. subtilis</i> clones transformed by BBa_K823003 (Pveg) + BBA_1364002 (GAFP1)  + BBa_B0015 (double terminator) in pSBBs4S, cryopreservation
<br/>
<br/>
- Fungicide test
- Fungicide test
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<div class="technology">Week 10 (18-24 August)</div>
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<div class="technology2">Week 10 (18-24 August)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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<p class="title3">Lab work:</p>
<p class="title3">Lab work:</p>
<p class="texte">
<p class="texte">
-
- Subculture and transformation in <i> Bacillus sutbilis </i> of BBa_K1364011 in pSBBS4S (BBa_K823022) and cloning of BBa_K1364011 on pSBBS1C (BBa_K823023).
+
- Subculture and transformation in <i> B. subtilis </i> of BBa_K1364011 in pSBBS4S (BBa_K823022) and cloning of BBa_K1364011 on pSBBS1C (BBa_K823023).
<br/>
<br/>
Problem: no clone had the insert on pSBBS1C => the cloning had to be done again
Problem: no clone had the insert on pSBBS1C => the cloning had to be done again
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<div class="technology">Week 11 (25- 31 August)</div>
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<div class="technology2">Week 11 (25- 31 August)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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- Cloning of BBa_K1364014 in BBa_K823022 and in BBa_K823023  
- Cloning of BBa_K1364014 in BBa_K823022 and in BBa_K823023  
<br/>
<br/>
-
- Cloning GAFP1 + BBa_K823023 (pSBBS1C) in <i>Bacillus subtilis</i> with a change in the protocol: pre-induction of the culture with 0.125 µg/ml of chloramphenicol one hour after the addition of DNA, and let grow for another hour.
+
- Cloning GAFP1 + BBa_K823023 (pSBBS1C) in <i>B. subtilis</i> with a change in the protocol: pre-induction of the culture with 0.125 µg/ml of chloramphenicol one hour after the addition of DNA, and let grow for another hour.
<br/>
<br/>
Problem: no colony  
Problem: no colony  
<br/>
<br/>
-
- Liquid culture of Bacillus + BBA_1364002 (GAFP1) ; Bacillus + BBA_1364003 (D4E1) + BBA_1364002 (GAFP1) ; Bacillus + BBA_1364003 (D4E1) for future fungicide tests
+
- Liquid culture of Bacillus + BBA_1364002 (GAFP1); Bacillus + BBA_1364003 (D4E1) + BBA_1364002 (GAFP1) ; Bacillus + BBA_1364003 (D4E1) for future fungicide tests
<br/>
<br/>
- Miniprep of BBa_ K1364011 in BBa_ K823023 (pSBBs1C) and transformation in <i>Bacillus subtilis</i> strain.  
- Miniprep of BBa_ K1364011 in BBa_ K823023 (pSBBs1C) and transformation in <i>Bacillus subtilis</i> strain.  
<br/>
<br/>
-
- Fungicide test of BBa_K1364011 in pSBBs4S, Promotor + BBA_1364002 (GAFP1) + Terminator (biobrick BBa_K1364008) in pSBBS4S, Promotor + BBA_1364003 (D4E1) + Terminator (biobrick BBa_K1364009) in pSBBS4S, Promotor + BBA_1364002 (GAFP1) + BA_1364003 (D4E1)  + Terminator ( biobrick BBa_K1364013) in pSBBS4S
+
- Fungicide test of BBa_K1364011 in pSBBs4S, Promotor + BBA_1364002 (GAFP1) + Terminator (biobrick BBa_K1364008) in pSBBS4S, Promotor + BBA_1364003 (D4E1) + Terminator (biobrick BBa_K1364009) in pSBBS4S, Promotor + BBA_1364002 (GAFP1) + BA_1364003 (D4E1)  + Terminator ( biobrick BBa_K1364013) in pSBBS4S
<br/>
<br/>
- Transformation of a new vector PKL 190 (threonine integrative) in <i>Bacillus</i> strain  
- Transformation of a new vector PKL 190 (threonine integrative) in <i>Bacillus</i> strain  
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- Objectives : chemotaxis, binding and fungicides tests have to be performed again
- Objectives : chemotaxis, binding and fungicides tests have to be performed again
</p>  
</p>  
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<p class="title1" id="select6"> September 2014</p>
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-
<p class="title2">Main activities</p>
+
<div class="technology">September 2014</div>
 +
<div class ="thelanguage">Main activities
<p class="texte">
<p class="texte">
- Finish the tests of the different modules
- Finish the tests of the different modules
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</p>  
</p>  
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<div class="technology2">Week 12 (1-7 September)</div>
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<div class="technology">Week 12 (1-7 September)</div>
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<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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</p>
</p>
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<div class="technology">Week 13 (8- 14 September)</div>
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<div class="technology2">Week 13 (8- 14 September)</div>
<div class="thelanguage">
<div class="thelanguage">
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<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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<br/>- Culture and miniprep of EcAMP to get more DNA + analytic digestion  
<br/>- Culture and miniprep of EcAMP to get more DNA + analytic digestion  
<br/>- Transformation of K1364014+K1364006 in E. coli  
<br/>- Transformation of K1364014+K1364006 in E. coli  
-
<br/>- Transformation of GAFP1 + D4E1, GAFP1 and  EcAMP+GAFP1+D4E1 on Bacillus subtilis + colony PCR + threonine test
+
<br/>- Transformation of GAFP1 + D4E1, GAFP1 and  EcAMP+GAFP1+D4E1 on <i>B. subtilis</i> + colony PCR + threonine test
<br/>NB: good results for the maxi operon and GAFP1 but not for GAFP1 + D4E1 CA  
<br/>NB: good results for the maxi operon and GAFP1 but not for GAFP1 + D4E1 CA  
<br/>- Cloning of K606013+pEX_K4, 823022+PlepA_RFP, 823022+ Pveg_RFP
<br/>- Cloning of K606013+pEX_K4, 823022+PlepA_RFP, 823022+ Pveg_RFP
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</p>
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<div class="technology">Week 14 (15 - 21 September)</div>
+
<div class="technology2">Week 14 (15 - 21 September)</div>
<div class="thelanguage">
<div class="thelanguage">
-
 
<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
Line 646: Line 632:
<br/>- Colony PCR on the mini operon BBa_K1364013 (GAFP1 - D4E1)
<br/>- Colony PCR on the mini operon BBa_K1364013 (GAFP1 - D4E1)
<br/>- Colony PCR on BBa_K1364011 on BBa_K823022 (pSBBS4S)
<br/>- Colony PCR on BBa_K1364011 on BBa_K823022 (pSBBS4S)
-
<br/>- Chemotaxis test with wild type <i>Bacillus subtilis</i> strain using Imperial College protocol
+
<br/>- Chemotaxis test with wild type <i>B. subtilis</i> strain using Imperial College protocol
-
<br/>- Tansformation of BBa_K1364011 + BBa_K823022 (pSBBS4S) in Bacillus subtilis
+
<br/>- Tansformation of BBa_K1364011 + BBa_K823022 (pSBBS4S) in <i>B. subtilis</i>
<br/>- Culture of fungi with fungicides
<br/>- Culture of fungi with fungicides
<br/>- Sequencing of plasmids containing the fungicides
<br/>- Sequencing of plasmids containing the fungicides
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<div class="technology">Week 15 (22 - 28 September)</div>
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<div class="technology2">Week 15 (22 - 28 September)</div>
<div class="thelanguage">
<div class="thelanguage">
-
 
<p class="title3">Communication and financial support:</p>
<p class="title3">Communication and financial support:</p>
<p class="texte">
<p class="texte">
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- Last experiments regarding chemotaxis tests.
- Last experiments regarding chemotaxis tests.
</p>
</p>
-
 
<p class="title3">Weekly meeting with the instructors(09/26/2014)</p>  
<p class="title3">Weekly meeting with the instructors(09/26/2014)</p>  
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</p>
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</div>
<div class="technology">October 2014</div>
<div class="technology">October 2014</div>
<div class="thelanguage">
<div class="thelanguage">
-
 
<p class="title2">Main activites</p>
<p class="title2">Main activites</p>
<p class="texte">
<p class="texte">
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- Daily presentations in front of the laboratory teachers to repeat again and again and again… let’s get ready for the Jamboree!
- Daily presentations in front of the laboratory teachers to repeat again and again and again… let’s get ready for the Jamboree!
</p>  
</p>  
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Revision as of 14:17, 17 October 2014