Team:Braunschweig/Notebook

From 2013.igem.org

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   <div id="Week5" class="menuSection">
   <div id="Week5" class="menuSection">
     <h2><a href="#Week5">Week 5: June 16 - June 22, 2013</a></h2>
     <h2><a href="#Week5">Week 5: June 16 - June 22, 2013</a></h2>
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     <p style=" margin-left:5px; margin-right:5px;">This week was dominated by a lot of cloning. We equipped our constitutive and inducible promoters with ribosome binding sites, terminators, an ampicillin resistance gene and a lactonase (not all of them got each of these elements). Additionally, we separated the ampicillin resistance gene from its native promoter in order to make its expression inducible. Although cloning was mostly successful, we were struggling to amplify and purify the luxR brick (C0062), which cost us a lot of time and effort. Unfortunately, it also wasn’t rewarded with success in the end.</p>
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     <p style=" margin-left:5px; margin-right:5px;">This week was dominated by a lot of cloning. We equipped our constitutive and inducible promoters with ribosome binding sites, terminators, an ampicillin resistance gene and a lactonase (not all of them got each of these elements). Additionally, we separated the ampicillin resistance gene from its native promoter in order to make its expression inducible. Although cloning was mostly successful, we were struggling to amplify and purify the <i>luxR</i> brick (C0062), which cost us a lot of time and effort. Unfortunately, it also wasn’t rewarded with success in the end.</p>
<p style=" margin-left:5px; margin-right:5px;">Another important step was to adapt our cloning strategy towards new chromoproteins which we received from iGEM team Uppsala. These allow us to evaluate our cultuvation experiments solely with own equipment, rather than having to find a cell sorter with suitable excitement lasers for all fluorescent proteins.</p>
<p style=" margin-left:5px; margin-right:5px;">Another important step was to adapt our cloning strategy towards new chromoproteins which we received from iGEM team Uppsala. These allow us to evaluate our cultuvation experiments solely with own equipment, rather than having to find a cell sorter with suitable excitement lasers for all fluorescent proteins.</p>
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<b>Investigators: Laura, Oliver, Jan </b><br>
<b>Investigators: Laura, Oliver, Jan </b><br>
Today, we first digested the inducible promoters, followed by purification and clean-up. Then we equipped the inducible and previously digested constitutive promoters with a RBS (B0032) by ligating respective parts. Subsequently, these ligated constructs were used to transform competent bacteria.
Today, we first digested the inducible promoters, followed by purification and clean-up. Then we equipped the inducible and previously digested constitutive promoters with a RBS (B0032) by ligating respective parts. Subsequently, these ligated constructs were used to transform competent bacteria.
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We also inoculated overnight suspension cultures with B0015- and B0032-transformed e.coli cells from cryo stocks for DNA preparation.</p>
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We also inoculated overnight suspension cultures with B0015- and B0032-transformed <i>E. coli</i> cells from cryo stocks for DNA preparation.</p>
   
   
<p style="font-size:14px; font-weight:bold; text-decoration:none; border:none; color:#be1e3c; margin-left:5px; margin-right:5px; margin-top:0px; margin-bottom:0px">Tuesday, June 18, 2013</p>
<p style="font-size:14px; font-weight:bold; text-decoration:none; border:none; color:#be1e3c; margin-left:5px; margin-right:5px; margin-top:0px; margin-bottom:0px">Tuesday, June 18, 2013</p>
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<div id="Week7" class="menuSection">
<div id="Week7" class="menuSection">
     <h2><a href="#Week7">Week 7: June 30 - July 6, 2013</a></h2>
     <h2><a href="#Week7">Week 7: June 30 - July 6, 2013</a></h2>
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     <p style=" margin-left:5px; margin-right:5px;">
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In week 7 we started our first experiments with our inducible promotors. Unfortunatly we had trouble caused by the leakyness of two of our three promotors. We did further experiments but could not find a solution yet.  
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In week 7 we started our first experiments with our inducible promotors. Unfortunately we had trouble caused by the leakyness of two of our three promotors. We did further experiments but could not find a solution yet.  
Good news is that we received the chromoproteins from Uppsala! So we started working on our new cloning strategy by combining the chromoprotein DNA with our constitutive promotor-RBS construct. We hope to see nice and colorful colonies next week!  
Good news is that we received the chromoproteins from Uppsala! So we started working on our new cloning strategy by combining the chromoprotein DNA with our constitutive promotor-RBS construct. We hope to see nice and colorful colonies next week!  
</p>
</p>
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<p style="font-size:14px; font-weight:bold; text-decoration:none; border:none; color:#be1e3c; margin-left:5px; margin-right:5px; margin-top:0px; margin-bottom:0px">Tuesday, July 2, 2013</p>><p style="margin-left:5px; margin-right:5px; margin-bottom:0px; margin-top:0px">
<p style="font-size:14px; font-weight:bold; text-decoration:none; border:none; color:#be1e3c; margin-left:5px; margin-right:5px; margin-top:0px; margin-bottom:0px">Tuesday, July 2, 2013</p>><p style="margin-left:5px; margin-right:5px; margin-bottom:0px; margin-top:0px">
<b>Investigators: Kerstin, Laura </b><br>
<b>Investigators: Kerstin, Laura </b><br>
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The ligations from yesterday were transformed into E. coli XL1 by heatshock and plated on 2xYT agar containing glucose and chloramphenicol.<br>  
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The ligations from yesterday were transformed into <i>E. coli</i> XL1 by heatshock and plated on 2xYT agar containing glucose and chloramphenicol.<br>  
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Since the chromoprotein DNA from Uppsala iGEM Team 2011 arrived today we now switch to our new cloning strategy starting with resuspending and transforming the newly arrived DNA into E. coli EL1 by heatshock. Cells were as well plated on 2xYT agar containing glucose and chloramphenicol.<br>
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Since the chromoprotein DNA from Uppsala iGEM Team 2011 arrived today we now switch to our new cloning strategy starting with resuspending and transforming the newly arrived DNA into <i>E. coli</i> XL1 by heatshock. Cells were as well plated on 2xYT agar containing glucose and chloramphenicol.<br>
Even if we switched to our new strategy we still keep working on the other fluorescent markers. Therefore we digested the bricks E0420 (eCFP), E0430 (YFP) and J06702 (mCherry) as well as our promotor-RBS-LasR and promotor-RBS-RhlR-constructs. Still lacking the construct containing LuxR we decided to proceed with the promotor-RBS-construct instead to ligate it to the YFP-Brick. Gelextraction was performed for the inserts and DNA purification for the vector parts. Inserts and bricks were ligated overnight using T4 DNA ligase (NEB) at 16°C.<br><br>
Even if we switched to our new strategy we still keep working on the other fluorescent markers. Therefore we digested the bricks E0420 (eCFP), E0430 (YFP) and J06702 (mCherry) as well as our promotor-RBS-LasR and promotor-RBS-RhlR-constructs. Still lacking the construct containing LuxR we decided to proceed with the promotor-RBS-construct instead to ligate it to the YFP-Brick. Gelextraction was performed for the inserts and DNA purification for the vector parts. Inserts and bricks were ligated overnight using T4 DNA ligase (NEB) at 16°C.<br><br>
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Since we now have our first constructs containing the inducible promotors as well as the the ampicillin resistence gen we started our first leakyness experiments. All constructs (Plas, Prhl, Plux in combination with the RBS and ampR) were cultivated overnight in 2xYT medium containing various ampicillin concentrations.</p>
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Since we now have our first constructs containing the inducible promotors as well as the the ampicillin resistence gen we started our first leakyness experiments. All constructs (P<sub>las</sub>, P<sub>rhl</sub>, P<sub>lux</sub> in combination with the RBS and <i>ampR</i>) were cultivated overnight in 2xYT medium containing various ampicillin concentrations.</p>
    
    
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The evaluation of the experiment for the inducible promotors showed that only the Prhl is not leaky. Plux as well as Plas were leaky and showed growth of E. coli XL1 at all tested ampicillin concentrations. Therefore we repeated the experiment using higher ampicillin conentrations.<br><br>
The evaluation of the experiment for the inducible promotors showed that only the Prhl is not leaky. Plux as well as Plas were leaky and showed growth of E. coli XL1 at all tested ampicillin concentrations. Therefore we repeated the experiment using higher ampicillin conentrations.<br><br>
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The bricks containing the fluorescent markers ligated yesterday were transformed in E. coli XL1 by heatshock.<br><br>
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The bricks containing the fluorescent markers ligated yesterday were transformed in <i>E. coli</i> XL1 by heatshock.<br><br>
<img alt="July3" src="https://static.igem.org/mediawiki/2013/f/fa/Braunschweig_Lab_Journal_July_3.png" width="200" align="right" vspace="0" hspace="10"/>Colony PCR of the constructs containing lactonase and LuxI which were transformed yesterday was performed. Since all screened colonies showed religated vectors we decided to try an alternativ restriction strategy to combine the bricks by using the endonuclease NcoI.<br>   
<img alt="July3" src="https://static.igem.org/mediawiki/2013/f/fa/Braunschweig_Lab_Journal_July_3.png" width="200" align="right" vspace="0" hspace="10"/>Colony PCR of the constructs containing lactonase and LuxI which were transformed yesterday was performed. Since all screened colonies showed religated vectors we decided to try an alternativ restriction strategy to combine the bricks by using the endonuclease NcoI.<br>   
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<div id="Week8" class="menuSection">
<div id="Week8" class="menuSection">
     <h2><a href="#Week8">Week 8: July 7 - July 13, 2013</a></h2>
     <h2><a href="#Week8">Week 8: July 7 - July 13, 2013</a></h2>
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     <p><p style=" margin-left:5px; margin-right:5px;">
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     <p style=" margin-left:5px; margin-right:5px;">Week 8</p>
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Week 8</p>
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   </div>
   </div>

Revision as of 20:38, 1 October 2013

Labjournal

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This is the documentation of our lab work. An overview on how we approached this project can be found under Approach. For detailed protocols of certain procedures please refer to Protocols. Attributions are given for each day, however please check our Attributions section for efforts beyond the lab work.

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