Difference between revisions of "Team:Toulouse/Experiments"

 
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<script>
var myurl = "https://2015.igem.org/Team:Toulouse/Descrition";
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var myurl = "https://2015.igem.org/Team:Toulouse/Description";
 
var elementId = "project";
 
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   <div class="title">
 
   <div class="title">
       <a href="#main1"><h3>Protocols for varroa tests</h3></a>
+
       <a href="#main1"><h3>Content</h3></a>
 
     </div>
 
     </div>
 
 
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     <div id="breadcrumb" class="clear" style="float: center;" >
 
     <div id="breadcrumb" class="clear" style="float: center;" >
 
  <ul>
 
  <ul>
         <li><a href="#part1">- Sampling of varroas</a></li>
+
         <li><a href="#varroatest">- Protocols for varroa tests</a></li>
         <li><a href="#part2">- Standardization of varroas and sampling</a></li>
+
         <li><a href="#culturetest">- Protocols for culture tests</a></li>
         <li><a href="#part3">- Attraction test on varroas</a></li>
+
         <li><a href="#PCR">- Protocol for Polymerase Chain Reaction</a></li>
        <li><a href="#part4">- Mortality test on varroas</a></li>
+
 
       </ul>
 
       </ul>
 
     </div>
 
     </div>
 
 
</center>
+
 
+
+
<div class="title">
+
      <a href="#main2"><h3>Protocols for culture tests</h3></a>
+
    </div>
+
+
<center> 
+
 
     <div id="breadcrumb" class="clear" style="float: center;" >
 
     <div id="breadcrumb" class="clear" style="float: center;" >
 
  <ul>
 
  <ul>
        <li><a href="#part5">- Cytotoxicity tests</a></li>
+
     
        <li><a href="#part6">- Growth culture</a></li>
+
  <li><a href="#TPX">- Protocols for TPX permeability tests</a></li>
        <li><a href="#part7">- Enzyme kinetic</a></li>
+
<li><a href="#transfo">- Transformation Protocol: RbCl method</a></li>
        <li><a href="#part8">- Acids production test</a></li>
+
<li><a href="#cloning">- Cloning protocol</a></li>
<li><a href="#part8">- Test of gas concentration</a></li>
+
      </ul>
+
 +
  </ul>
 +
  </div>
 +
<div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
     
 +
  <li><a href="#infusion">- InFusion cloning protocol</a></li>
 +
 +
  </ul>  
 
     </div>
 
     </div>
 
 
</center>
 
</center>
 
 
 
  <div class="title">
 
      <a href="#main1"><h3>Transformation Protocol: RbCl method</h3></a>
 
    </div>
 
 
 
 +
<div class="group center">
 +
<hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;">
 +
</div>
 +
<div class="group center">
 +
<div class="title" id="varroatest">  
 +
<h3>Protocols for varroa tests</h3>
 +
 +
 
<center>   
 
<center>   
 
     <div id="breadcrumb" class="clear" style="float: center;" >
 
     <div id="breadcrumb" class="clear" style="float: center;" >
 
  <ul>
 
  <ul>
         <li><a href="#part1">- Media and solution</a></li>
+
         <li><a href="#samplingV">- Sampling of varroa</a></li>
         <li><a href="#part2">- Competent Cells</a></li>
+
         <li><a href="#standardV">- Standardization of varroas and sampling</a></li>
         <li><a href="#part3">- Miniprep</a></li>
+
         <li><a href="#attractV">- Attraction test on varroas</a></li>
         <li><a href="#part4">- Transformation</a></li>
+
         <li><a href="#mortalV">- Mortality test on varroas</a></li>
 
       </ul>
 
       </ul>
 
     </div>
 
     </div>
 
 
</center>
 
</center>
 
 
  <div class="title">
+
 
      <a href="#main2"><h3>Cloning</h3></a>
+
    </div>
+
<center> 
+
    <div id="breadcrumb" class="clear" style="float: center;" >
+
  <ul>
+
        <li><a href="#part6">- Digestion</a></li>
+
        <li><a href="#part7">- Gel extraction</a></li>
+
        <li><a href="#part8">- Ligation</a></li>
+
<li><a href="#part9">- Transformation</a></li>
+
      </ul>
+
    </div>
+
<hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;">
+
</center>
+
<div class="group center">
+
<div class="title" >  
+
<h3>Protocols for varroa tests</h3>
+
<div id="part1"><!-- ANCHOR 1--></div>
+
 
</div>
 
</div>
 
</div>
 
</div>
 
<div class="group">
 
<div class="group">
<div class="subtitle">    
+
<div class="subtitle" id="samplingV">    
 
<h3>Sampling of varroa</h3>
 
<h3>Sampling of varroa</h3>
 
</div>
 
</div>
 
</div>
 
</div>
 +
 +
 +
<div class="group">
 +
<p align="justify" style="font-size:15px;">To run tests with varroas it is necessary to get them back from beehive directly because they cannot live without bees. </p>
 +
</div>
 +
 +
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
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<li>Small brush</li>
 
<li>Small brush</li>
 
<li>Petri dishes <br> Ø x h = 35 x 15 mm</li>
 
<li>Petri dishes <br> Ø x h = 35 x 15 mm</li>
 +
 
</div>
 
</div>
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>Slip beekeeper suit and gloves on and go to bee hive</li>
+
<li>Slip beekeeper suit and gloves on and go to beehive</li>
 
<li>Fire dry twigs in smoker</li>
 
<li>Fire dry twigs in smoker</li>
 
<li>Open bee hive and activate smoker to get bees inside the hive</li>
 
<li>Open bee hive and activate smoker to get bees inside the hive</li>
 
<li>Take a frame out the hive and remove bees with big brush and smoker</li>
 
<li>Take a frame out the hive and remove bees with big brush and smoker</li>
<li>Close bee hive</li>
+
<li>Close beehive</li>
 
<li>In the lab, put the frame on a table against the wall</li>
 
<li>In the lab, put the frame on a table against the wall</li>
 
<li>With tweezer drill hole into one beehive cell</li>
 
<li>With tweezer drill hole into one beehive cell</li>
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</div>
 
</div>
 
</div>
 
</div>
 +
<br><br><br>
 +
 +
<div class="group center">
 +
 +
<div style="padding-top:50px;">
 +
<img src="https://static.igem.org/mediawiki/2015/c/cd/TLSE_sampling_img2.jpg" style="width:100%" />
 +
</div>
 +
<div>
 +
<img src="https://static.igem.org/mediawiki/2015/7/71/TLSE_sampling_img1.png"  style="width:100%"/>
 +
</div>
 +
<div style="padding-top:50px;">
 +
<img src="https://static.igem.org/mediawiki/2015/f/f5/TLSE_sampling_img3.jpg" style="width:100%" />
 +
</div>
 +
 +
</div>
 +
<center><p class="legend">
 +
Steps 1, 4 & 7: Our teams members gathering varroas on infected larvae
 +
</p>
 +
</center>
 +
 +
 +
  
 
<div class="group">
 
<div class="group">
<div class="subtitle">    
+
<div class="subtitle" id="standardV">    
 
<h3>Standardization of varroas and sampling</h3>
 
<h3>Standardization of varroas and sampling</h3>
 
</div>
 
</div>
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<p align="justify" style="font-size:15px;">When we take varroas directly from frame, as it is described in  
 
<p align="justify" style="font-size:15px;">When we take varroas directly from frame, as it is described in  
 
protocol “Sampling Varroas”, we have varroas in different phases. In order to have varroas  
 
protocol “Sampling Varroas”, we have varroas in different phases. In order to have varroas  
in the same phase it is necessary to add one step and it is important for reproducibility of  
+
in the same phase it is necessary to add one step and it is important for reproducibility of the
 
experiments. With this method we place varroas on adult bees so all varroas will be in phoretic phase.</p>
 
experiments. With this method we place varroas on adult bees so all varroas will be in phoretic phase.</p>
 
</div>
 
</div>
 
<div class="group" style="padding-top:10px">
 
<div class="group" style="padding-top:10px">
 
<div class="one_quarter first">
 
<div class="one_quarter first">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
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<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
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</div>
 
</div>
 
</div>
 
</div>
 +
<br><br>
  
 
<div class="group">
 
<div class="group">
<div class="subtitle" >    
+
<div >
 +
<img src="https://static.igem.org/mediawiki/2015/d/d5/TLSE_Expe77_img4.jpg"  style="width:90%; padding-left:100px; " />
 +
 
 +
</div>
 +
<div >
 +
<img src="https://static.igem.org/mediawiki/2015/2/20/TLSE_Expe_img5.jpg" style="width:80%;" />
 +
 
 +
</div>
 +
 
 +
</div>
 +
<center>
 +
<p class="legend">
 +
Steps 2 & 5: Varroas gathering on infected bees
 +
</p>
 +
</center>
 +
 
 +
 
 +
<div class="group">
 +
<div class="subtitle" id="attractV">    
 
<h3>Attraction test on varroas</h3>
 
<h3>Attraction test on varroas</h3>
 
</div>
 
</div>
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<div class="group center">
 
<div class="group center">
 
<p align="justify" style="font-size:15px;">In order to test the attraction effect of butyric acid  
 
<p align="justify" style="font-size:15px;">In order to test the attraction effect of butyric acid  
on varroas an Y test was used, as it is showed with diagram below. Where we place varroas for the
+
on varroas a Y test tube was built, as it is showed below. A glass pipe was chosen because on plastic varroas could load themselves with electrostatics and die.  
test we choose glass pipe because on plastic they could load themselves with electrostatics and die.  
+
For butyric acid, the concentration chosen 4 % (V/V) because this is the concentration used in the patent quoted (see “Attribution” part). </p>
For butyric acid concentration we choose 4% (V/V) because this is the concentration used in the patent we see, see “Attribution” part. </p>
+
 
</div>
 
</div>
  
 
<div class="group" style="padding-top:10px">
 
<div class="group" style="padding-top:10px">
 
<div class="one_quarter first">
 
<div class="one_quarter first">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
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<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>Put a cotton on Petri dish and add 400µL of one acid formic solution</li>
+
<li>Put a cotton on Petri dish and add 400 µL of one acid formic solution</li>
 
<li>Place three varroas on this Petri dish and close it</li>
 
<li>Place three varroas on this Petri dish and close it</li>
 
<li>Start again step1 and 2 for each formic acid solution and water</li>
 
<li>Start again step1 and 2 for each formic acid solution and water</li>
<li>Each 30 minutes check if varroas are alive. To do that :</li>
+
<li>Each 30 minutes check if varroas are alive. To do that:</li>
 
<li>When varroa heads for one side of Glass T tube and covers more than 2 cm test is over and we write down the side choosen by varroa (Butyric acid or Water)</li>
 
<li>When varroa heads for one side of Glass T tube and covers more than 2 cm test is over and we write down the side choosen by varroa (Butyric acid or Water)</li>
 
<li>Two tests can be made in the same time thanks to the plastic separator</li>
 
<li>Two tests can be made in the same time thanks to the plastic separator</li>
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</div>
 
</div>
 
</div>
 
</div>
 
+
<br>br>
 
+
<center><img src="https://static.igem.org/mediawiki/2015/6/6d/Glass_T-tube.jpg" style="width:70%;" />
 +
<p class="legend">
 +
Glass T-tube: Varroa is going to butyric acid (at left)
 +
</p>
 +
</center>
  
  
 
<div class="group">
 
<div class="group">
<div class="subtitle" >    
+
<div class="subtitle" id="mortalV" >    
 
<h3>Mortality test on varroas</h3>
 
<h3>Mortality test on varroas</h3>
 
</div>
 
</div>
 
</div>
 
</div>
 
<div class="group center">
 
<div class="group center">
<p align="justify" style="font-size:15px;">To test toxicity of formic acid  
+
<p align="justify" style="font-size:15px;">Test the toxicity of formic acid  
on varroas we had to choose which concentrations we use. For that we based
+
on varroas. When beekeepers use formic acid for long  
our thoughts on present treatments. When beekeepers use formic acid for long  
+
 
treatment they place a diffuser at the top of the hive and formic acid concentration  
 
treatment they place a diffuser at the top of the hive and formic acid concentration  
was assessed at 200ppm<a target="_blank" href="http://www.agroscope.admin.ch/imkerei/00316/00329/02079/index.html?lang=en"> <SUP>1</SUP> </a>on average that is equivalent to 7.826 mmol.m<SUP>-3</SUP>.  
+
was assessed at 200 ppm<a target="_blank" href="http://www.agroscope.admin.ch/imkerei/00316/00329/02079/index.html?lang=en"> <SUP>1</SUP> </a>on average which is equivalent to 7.8 mmol.m<SUP>-3</SUP>.  
As gas concentration is difficult to evaluate we calculate the liquid concentration balance   
+
As gas concentration is difficult to evaluate we calculated the liquid concentration balance   
thanks to the ideal gas law and the Henry’s law. To simplify calculation we noted down formic acid A.
+
using the ideal gas law and Henry’s law. To simplify calculation we noted down formic acid A.
 
  </p>
 
  </p>
 
</div>
 
</div>
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$$ P\cdot V = n\cdot R\cdot T, \textrm{ideal gaz law} $$
 
$$ P\cdot V = n\cdot R\cdot T, \textrm{ideal gaz law} $$
 
<!-- P. V = n.R.T, ideal gaz law-->
 
<!-- P. V = n.R.T, ideal gaz law-->
$$ P_A = C_A\cdot R\cdot T = 7,826\cdot10^{-3}\times8.314\times293=19,964 Pa $$
+
$$ P_A = C_A\cdot R\cdot T = 7.826\cdot10^{-3}\times8.314\times293=19.96 Pa $$
 
</p>
 
</p>
 
</div>
 
</div>
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<!-- P_A = C_A.R.T = 7,826.10^3 x 8.314 x 293 = 19,964 Pa -->
 
<!-- P_A = C_A.R.T = 7,826.10^3 x 8.314 x 293 = 19,964 Pa -->
 
$$ P_A = H_A\cdot C_{A,eq}, \textrm{Henry's law} $$
 
$$ P_A = H_A\cdot C_{A,eq}, \textrm{Henry's law} $$
<!-- P_A = H_A . C_{A,eq}, Henry's law -->
+
<!-- P_A = H_A . C_{A,eq} (Henry's law) -->
$$ C_{A,eq} = \frac{19,964}{0,019} = 1,019mol.L^{-1}$$
+
$$ C_{A,eq} = \frac{19.964}{0.019} = 1.019 mol.L^{-1}$$
 
</p>
 
</p>
 
</div>
 
</div>
 
<ul style="font-size:15px;">
 
<ul style="font-size:15px;">
 
<li>C<SUB>A,eq</SUB>: equivalent concentration in liquid in mol.L<SUP>-1</SUP></li>
 
<li>C<SUB>A,eq</SUB>: equivalent concentration in liquid in mol.L<SUP>-1</SUP></li>
<li>H<SUB>A</SUB>: Henry's constant = 0,019 Pa.m<SUP>3</SUP>mol<SUP>-1</SUP></li>
+
<li>H<SUB>A</SUB>: Henry's constant = 0.019 Pa.m<SUP>3</SUP>mol<SUP>-1</SUP></li>
 
</ul>
 
</ul>
 +
 +
<div class="group center">
 +
<p align="justify" style="font-size:15px;">We chose a positive control with a higher concentration, 2 mol.L<SUP>-1</SUP>, and then decreasing concentration in order to identify which minimum concentration could kill varroa. We used water as a negative control.
 +
For this test we use varroas directly from frames because we did not have enough standardized varroas.
 +
</p>
 +
</div>
  
 
<div class="group" style="padding-top:10px">
 
<div class="group" style="padding-top:10px">
 
<div class="one_quarter first">
 
<div class="one_quarter first">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
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<li>Varroas form “Sampling varroas”</li>
 
<li>Varroas form “Sampling varroas”</li>
 
<li>Cotton</li>
 
<li>Cotton</li>
<li>Acid formic solutions : </li>
+
<li>Acid formic solutions: </li>
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
 
<li>2 mol.L<SUP>-1</SUP></li>
 
<li>2 mol.L<SUP>-1</SUP></li>
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<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>Put a cotton on Petri dish and add 400µL of one acid formic solution</li>
+
<li>Put a cotton on Petri dish and add 400 µL of one acid formic solution</li>
<li>Place three varroas on this Petri dish and close it</li>
+
<li>Place three varroas in this Petri dish and close it</li>
 
<li>Start again step1 and 2 for each formic acid solution and water</li>
 
<li>Start again step1 and 2 for each formic acid solution and water</li>
<li>Each 30 minutes check if varroas are alive. To do that : </li>
+
<li>Every 30 minutes check if varroas are alive. To do that: </li>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li value="5">Tap on Petri dish and see if varroa move. If yes varroa is alive, if not see below</li>
+
<li>Tap on Petri dish and see if varroa moves. If it does varroa is still alive, if not see below</li>
<li>Look at binocular magnifier if varroas move their feets. If yes varroa is alive, if not varroa is dead <br>  
+
<li>Observe through a binocular magnifier if varroa move. If it does, it is still alive. <br>  
<u>Remark:</u> A varroa stop moving approximately one or two hours before it dies <div id="main2"></div></li>
+
</li>
</li>
+
 
</ol>
 
</ol>
 
</ol>
 
</ol>
 
</div>
 
</div>
 
</div>
 
</div>
 +
<br><br>
 +
<center><img src="https://static.igem.org/mediawiki/2015/2/23/Mortality_test.jpg" style="width:70%;" />
 +
<p class="legend">
 +
Varroa mortality experiment
 +
</p>
 +
</center>
  
  
  
 
 
<br>
 
 
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
 
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
  
 
<center>
 
<center>
<div class="title" >    
+
<div class="title" id="culturetest">    
 
<h3>Protocols for culture tests</h3>
 
<h3>Protocols for culture tests</h3>
 
</div>
 
</div>
 
</center>
 
</center>
  
 +
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
        <li><a href="#CytotoxicityTests">- Cytotoxicity tests</a></li>
 +
        <li><a href="#erlencult">- Culture on erlenmeyers and TubeSpin<SUP>®</SUP> Bioreactors</a></li>
 +
        <li><a href="#NMR">- NMR analysis</a></li>
 +
        <li><a href="#platecult">- Culture on 48 wells plates</a></li>
 +
      </ul>
 +
    </div>
 +
</center>
 +
 +
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
        <li><a href="#enzymekinetic">- Enzyme kinetic</a></li>
 +
        <li><a href="#acidsprod">- Acids production test</a></li>
 +
        <li><a href="#gasconcentration">- Test of gas concentration</a></li>
 +
     
 +
      </ul>
 +
    </div>
 +
</center>
  
<div class="subtitle">
+
<div class="subtitle" id="CytotoxicityTests">
     <h3>Cytotoxicity tests<br>&nbsp;&nbsp;&nbsp;&nbsp;Choice of concentrations</h3>   
+
     <h3>Cytotoxicity tests</h3>
 +
</div>
 +
 +
<div class="subsubsubtitle">
 +
<h3>Choice of concentrations</h3>   
 
</div>
 
</div>
 
   
 
   
Line 365: Line 435:
 
<div class="group">
 
<div class="group">
 
<p align="justify" style="font-size:15px;">
 
<p align="justify" style="font-size:15px;">
In the begining we tested high and low concentrations and in function of results we adapted concentrations. In the end we worked with these concentrations:
+
In the beginning we tested high and low concentrations and we further adapted the concentrations. In the end we worked with these concentrations:
 
</p>
 
</p>
 
</div>
 
</div>
Line 378: Line 448:
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
Line 390: Line 460:
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
Line 399: Line 469:
 
<li>Place the 48 well plate in the optical reader</li>
 
<li>Place the 48 well plate in the optical reader</li>
 
<li>Adjust parameters on computer. <br>  
 
<li>Adjust parameters on computer. <br>  
Usually we set 250 cycles around 24 hours so we have an OD measure every six minutes</li>
+
Usually we set 250 cycles around 24 hours so we have an OD measurement every six minutes</li>
 
</ol>
 
</ol>
 
</div>
 
</div>
Line 405: Line 475:
  
 
<p align="justify" style="font-size:15px;">
 
<p align="justify" style="font-size:15px;">
<u>Remark:</u> Each condition is tested in three replicates
+
<u>Note:</u> Each condition is tested in three replicates
 
</p>
 
</p>
  
  
<div class="subtitle">
+
<div class="subtitle" id="erlencult">
     <h3>Growth culture</h3>
+
      
<h3 style="font-size:18px;"> &nbsp; Culture on erlenmeyers and TubeSpin<SUP>®</SUP> Bioreactors</h3>
+
<h3>Culture on erlenmeyers and TubeSpin<SUP>®</SUP> Bioreactors</h3>
<h3 style="font-size:16px;">&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;Inoculation and sampling</h3>   
+
<h3>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp; - Inoculation and sampling</h3>   
 
     </div>
 
     </div>
  
Line 418: Line 488:
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
<li>Pre-culture of <i>E.Coli</i> BW 25113 in LB</li>
+
<li>Pre-culture of <i>E. coli</i> BW 25113 in LB</li>
 
<li>Spectrophotometer</li>
 
<li>Spectrophotometer</li>
 
<li>1mL Spectrophotometer cuvettes</li>
 
<li>1mL Spectrophotometer cuvettes</li>
Line 435: Line 505:
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>Add 50 mL of medium on erlenmyer and TubeSpin<SUP>®</SUP> Bioreactor</li>
+
<li>Add 50 mL of medium on erlenmeyer and TubeSpin<SUP>®</SUP> Bioreactor</li>
 
<li>Inoculate from pre-culture to have OD<SUB>600nm</SUB>=0.1. <br>
 
<li>Inoculate from pre-culture to have OD<SUB>600nm</SUB>=0.1. <br>
 
To do that centrifuge the appropriate volume of pre-culture, then remove LB medium and resuspend sediment with M9 medium to inoculate.<br>
 
To do that centrifuge the appropriate volume of pre-culture, then remove LB medium and resuspend sediment with M9 medium to inoculate.<br>
<u>Remark:</u> This step permits to eliminate substrates from LB medium which could interfere during NMR analysis.</li>
+
<u>Note:</u> This step permits to eliminate substrates from LB medium which could interfere during NMR analysis.</li>
<li>Place erlenmeyers in incubator 37°C 130rpm and TubeSpin<SUP>®</SUP> Bioreactor in incubator 37°C without agitation</li>
+
<li>Place erlenmeyers in incubator 37 °C 130 rpm and TubeSpin<SUP>®</SUP> Bioreactor in incubator 37 °C without agitation</li>
 
<li>Sampling every two hours the first day:</li>
 
<li>Sampling every two hours the first day:</li>
 
<ul>
 
<ul>
<li>Take 1mL of culture in 1.5 mL Eppendorf. <br>
+
<li>Take 1 mL of culture in 1.5 mL Eppendorf. <br>
Attention: for TubeSpin<SUP>®</SUP> Bioreactor use needle and syringe in order not to let air enter, as possible.
+
For TubeSpin<SUP>®</SUP> Bioreactor use needle and syringe in order not to let air enter.
 
</li>
 
</li>
<li>Add 100 µL of sample in spectrophotometer cuvette, complete with 900µL water and measure OD<SUB>600nm</SUB> with spectrophotometer</li>
+
<li>Add 100 µL of sample in spectrophotometer cuvette, complete with 900 µL water and measure OD<SUB>600 nm</SUB> with spectrophotometer</li>
<li>Centrifuge the rest of samples at 13000 rpm during 3 minutes</li>
+
<li>Centrifuge the rest of samples at 13,000 rpm during 3 minutes</li>
<li>Filter the supernatant through a 0.2 µm filter and conserve it at -20°C
+
<li>Filter the supernatant through a 0.2 µm filter and conserve it at -20 °C
 
</li>
 
</li>
 
</ul>
 
</ul>
Line 461: Line 531:
 
 
  
<div class="subtitle">
+
<div class="subtitle" id="NMR">
     <h3 style="font-size:18px;">&nbsp;NMR analysis</h3>   
+
     <h3>&nbsp;&nbsp;&nbsp;&nbsp;&nbsp; - NMR analysis</h3>   
 
     </div>
 
     </div>
 +
 +
 +
 +
 +
 +
 
 
 
 
Line 469: Line 545:
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
Line 477: Line 553:
 
</li>
 
</li>
 
<li>0.5 mm NMR tubes</li>
 
<li>0.5 mm NMR tubes</li>
<li>1.5mL Eppendorf</li>
+
<li>1.5 mL Eppendorf</li>
 
<li>Spinners (5mm)</li>
 
<li>Spinners (5mm)</li>
<li>500MHz Bruker Avance Spectrometer</li>
+
<li>500 MHz Bruker Avance Spectrometer</li>
 
</div>
 
</div>
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>Add 400 µL of culture supernatant in 1.5mL Eppendorf
+
<li>Add 400 µL of culture supernatant in 1.5 mL Eppendorf
 
</li>
 
</li>
 
<li>Add 100 µL of TSP solution</li>
 
<li>Add 100 µL of TSP solution</li>
Line 496: Line 572:
 
</div>
 
</div>
 
</div>
 
</div>
+
<br><br>
+
<center>
+
<div class="group center">
+
<div>
 +
<img src="https://static.igem.org/mediawiki/2015/1/18/TLSE_Protocols_Culture_2b.jpg" style="width:73%;" />
  
<div class="subtitle">
+
</div>
 +
 
 +
<div style="width:45%;padding-bottom:10px;padding-top:35px;">
 +
<img src="https://static.igem.org/mediawiki/2015/4/43/TLSE_Protocols_Culture_1b.png"/>
 +
 
 +
</div>
 +
 
 +
<div style="width:22%;padding-bottom:10px;padding-left:25px">
 +
<img src="https://static.igem.org/mediawiki/2015/f/fa/TLSE_Protocols_Culture_3b.png" " />
 +
</div>
 +
</div>
 +
<p class="legend">
 +
Micro-aerobic culture, filtration and NMR samples
 +
</p>
 +
</center>
 +
<br><br>
 +
<center><img src="https://static.igem.org/mediawiki/2015/1/13/TLSE_Protocols_Culture_4b.png" style="width:30%;" />
 +
<p class="legend">
 +
500MHz NMR Spectrometer used for culture supernatant analysis
 +
</p>
 +
</center>
 +
 +
 
 +
<div class="subtitle" id="platecult">
 
     <h3>Culture on 48 wells plates</h3>   
 
     <h3>Culture on 48 wells plates</h3>   
 
     </div>
 
     </div>
Line 510: Line 610:
 
In order to determine the right concentration of polysaccharide and enzyme of  
 
In order to determine the right concentration of polysaccharide and enzyme of  
 
BioSilta kit we have to do several cultures at the same time. So, we use an optical  
 
BioSilta kit we have to do several cultures at the same time. So, we use an optical  
reader and 48 wells plates in order to have lots of test in the same time.  
+
reader and 48 wells plates.  
 
</p>
 
</p>
 
</div>
 
</div>
Line 516: Line 616:
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
Line 531: Line 631:
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>Add 450µL of medium in each well
+
<li>Add 450 µL of medium in each well
 
</li>
 
</li>
<li>Add 50µL of pre-culture</li>
+
<li>Add 50 µL of pre-culture</li>
 
<li>Place the 48 well plate in the optical reader
 
<li>Place the 48 well plate in the optical reader
 
</li>
 
</li>
Line 547: Line 647:
 
<div class="group center">
 
<div class="group center">
 
<p align="justify" style="font-size:15px">
 
<p align="justify" style="font-size:15px">
<u>Remark:</u> Each condition is tested almost in two replicates.  
+
<u>Note:</u> Each condition is tested in two replicates.  
 
According to our results we adapt concentrations of Biosilta medium and enzyme,  
 
According to our results we adapt concentrations of Biosilta medium and enzyme,  
results are exposed in Device part.
+
results are exposed in device part.
 
</p>
 
</p>
 
</div>
 
</div>
  
 
 
<div class="subtitle">
+
<div class="subtitle" id="enzymekinetic">
 
<h3>Enzyme kinetic</h3>
 
<h3>Enzyme kinetic</h3>
 
     </div>
 
     </div>
Line 560: Line 660:
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
Line 571: Line 671:
 
</li>
 
</li>
 
<li>Bradford’s reagent</li>
 
<li>Bradford’s reagent</li>
<li>1.5mL Eppendorf</li>
+
<li>1.5 mL Eppendorf</li>
 
<li>Standard solutions of glucose</li>
 
<li>Standard solutions of glucose</li>
 
</div>
 
</div>
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
<li>For each standard solutions : in a 1.5 mL Eppendorf sample 10 µL and add 1mL Bradford’s Reagent, wait 20 minutes and measure OD<SUB>505nm</SUB>
+
<li>For each standard solutions : in a 1.5 mL Eppendorf sample 10 µL and add 1 mL Bradford’s Reagent, wait 20 minutes and measure OD<SUB>505 nm</SUB>
 
</li>
 
</li>
 
<li>Plot glucose concentration in function of OD<SUB>505nm</SUB> and determine the linear region
 
<li>Plot glucose concentration in function of OD<SUB>505nm</SUB> and determine the linear region
Line 592: Line 692:
 
<li>Wait 20 minutes
 
<li>Wait 20 minutes
 
</li>
 
</li>
<li>Measure OD<SUB>505nm</SUB>
+
<li>Measure OD<SUB>505 nm</SUB>
 
</li>
 
</li>
<li>If OD<SUB>505nm</SUB> is over linear region dilute sample and measure OD<SUB>505nm</SUB> again
+
<li>If OD<SUB>505 nm</SUB> is over linear region dilute sample and measure OD<SUB>505 nm</SUB> again
 
</li>
 
</li>
 
</ol>
 
</ol>
Line 602: Line 702:
 
</div>
 
</div>
 
 
<div class="subtitle">
+
<div class="subtitle" id="acidsprod">
 
<h3>Acids production test</h3>
 
<h3>Acids production test</h3>
 
</div>
 
</div>
  
 
<div class="group center">
 
<div class="group center">
<p align="justify" style="font-size:15px;"> In order to test if E.coli produce formic acid and butyric acid with genes we add we made culture test with modified bacteria. We used the same protocol as “Culture on Erlenmeyers and TubeSpin® Bioreactors” with some changes: </p>
+
<p align="justify" style="font-size:15px;"> In order to test if <i>E. coli</i> produces formic acid and butyric acid with genes added, we made culture test with modified bacteria. We used the same protocol as “Culture on Erlenmeyers and TubeSpin® Bioreactors” with some changes: </p>
 
</div>
 
</div>
  
<div class="group center">
+
<div class="group">
 
<div class="one_quarter">
 
<div class="one_quarter">
 
</div>
 
</div>
 
<div class="one_half">
 
<div class="one_half">
 
<ul style="font-size:15px;" align="left">
 
<ul style="font-size:15px;" align="left">
<li>Volume of culture : 30mL
+
<li>Volume of culture : 30 mL
 
</li>
 
</li>
<li>Add Ampicillin at 25µg/mL to have selection pressure</li>
+
<li>Add Ampicillin at 25 µg/mL to have selection pressure</li>
 
<li>The number of samples:  
 
<li>The number of samples:  
 
</li>
 
</li>
Line 624: Line 724:
 
<li>Sample at the end of the first day
 
<li>Sample at the end of the first day
 
</li>
 
</li>
<li>Sample after 24h culture and 48h culture</li>
+
<li>Sample after 24 hours culture and 48 hours culture</li>
 
</ul>
 
</ul>
 
</ul>
 
</ul>
Line 632: Line 732:
  
 
 
<div class="subtitle">
+
<div class="subtitle" id="gasconcentration">
 
<h3>Test of gas concentration</h3>
 
<h3>Test of gas concentration</h3>
 
     </div>
 
     </div>
Line 638: Line 738:
 
<div class="group center">
 
<div class="group center">
 
<p style="font-size:15px;" align="justify">
 
<p style="font-size:15px;" align="justify">
The objective of our device is to produce gas, so we would like to know gas composition of our culture.  
+
The objective of our device is to produce gas, so we would like to know the gas composition of our culture.  
 
So, we developed a system in order to recover acids gas.
 
So, we developed a system in order to recover acids gas.
 
 
</p>
 
</p>
</div>  
+
</div>
 +
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
<li>4 h culture in 50 mL Falcon in M9 medium with 15 mM of glucose</li>
+
<li>4 hours culture in 50 mL Falcon in M9 medium with 15 mM of glucose</li>
<li>Silicon plugs adapted to 50mL Falcon</li>
+
<li>Silicon plugs adapted to 50 mL Falcon</li>
 
<li>Needles
 
<li>Needles
 
</li>
 
</li>
Line 659: Line 759:
 
</li>
 
</li>
 
<li>10 mM NaHCO<SUB>3</SUB></li>
 
<li>10 mM NaHCO<SUB>3</SUB></li>
<li>1.5mL Eppendorf</li>
+
<li>1.5 mL Eppendorf</li>
<li>1mL Sterile cone</li>
+
<li>1 mL Sterile cone</li>
<li>Incubator 3°C without agitation</li>
+
<li>Incubator 3 °C without agitation</li>
 
 
 
</div>
 
</div>
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
Line 672: Line 772:
 
<li>Replace Falcon plug with silicon plug
 
<li>Replace Falcon plug with silicon plug
 
</li>
 
</li>
<li>Adjust fliter on needle and peg it into silicon plug. Do it twice</li>
+
<li>Adjust filter on needle and peg it into silicon plug. Do it twice</li>
 
<li>Adjust neoprene pipe into each filter</li>
 
<li>Adjust neoprene pipe into each filter</li>
<li>Add 700µL of NaHCO<SUB>3</SUB> in an Eppendorf</li>
+
<li>Add 700 µL of NaHCO<SUB>3</SUB> in an Eppendorf</li>
 
<li>At the end of first pipe put a sterile cone and immerse it into Eppendorf with NaHCO<SUB>3</SUB></li>
 
<li>At the end of first pipe put a sterile cone and immerse it into Eppendorf with NaHCO<SUB>3</SUB></li>
<li>At the end of second pipe put a 10mL syringe</li>
+
<li>At the end of second pipe put a 10 mL syringe</li>
<li>After 24h culture, press 10mL syringe in order to expel gas in NaHCO<SUB>3</SUB> solution</li>
+
<li>After 24 hours culture, press 10 mL syringe in order to expel gas in NaHCO<SUB>3</SUB> solution</li>
<li>Conserve samples at -20°C before NMR analysis (see protocol foregoing) </li>
+
<li>Conserve samples at -20 °C before NMR analysis (see protocol foregoing) </li>
  
 
</div>
 
</div>
Line 685: Line 785:
 
<div class="group">
 
<div class="group">
 
<p style="font-size:15px;" align="justify">
 
<p style="font-size:15px;" align="justify">
<u>Remark 1:</u> We used culture in M9 because with the “Acids production tests” we had data on this medium.<br>
+
<u>Note 1:</u> We used culture in M9 because with the “Acids production tests” we had data on this medium.<br>
<u>Remark 2:</u> 10 mM NaHCO<SUB>3</SUB> solution was used because pH was 8.3 so it would permit acid gas solubilisation.
+
<u>Note 2:</u> 10 mM NaHCO<SUB>3</SUB> solution was used because pH was 8.3 so it would permit acid gas solubilisation.
 
</p>
 
</p>
 
</div>  
 
</div>  
 +
<br>
 +
<center>
 +
 +
<img src="https://static.igem.org/mediawiki/2015/b/b7/TLSE_expe_1b.png" style="width:80%"/>
 +
<p class="legend">
 +
Photo 8: Gas concentration test with falcons
 +
</center>
 +
  
  
<img src="https://static.igem.org/mediawiki/2015/d/d5/TLSE_expe_1.png" />
 
 
<br>
 
<br>
 
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
 
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
 +
 +
<center>
 +
<div class="title" id="PCR">
 +
<h3>Protocol for Polymerase Chain Reaction (PCR), From Thermo Scientific™ DreamTaq™ Green PCR Master Mix </h3>
 +
</div>
 +
</center>
 +
 +
 +
 +
<div class="group">
 +
<div class="one_quarter first" >
 +
<div class="subsubsubtitle">  
 +
<h3>Materials</h3>
 +
</div>
 +
<ul align="justify" style="font-size:15px;">
 +
<li>MilliQ water nuclease free
 +
(QSP)</li>
 +
<li>PCR Mix 2X</li>
 +
<li>Forward primer
 +
</li>
 +
<li>Reverse primer</li>
 +
<li>Template DNA
 +
</li>
 +
<li>Thin walled PCR tube</li>
 +
<li>Ice</li>
 +
 +
 +
 +
</div>
 +
 +
<div class="three_quarter">
 +
<div class="subsubsubtitle">  
 +
<h3>Methods</h3>
 +
</div>
 +
<ol align="justify" style="font-size:15px;">
 +
<li>Gently vortex and briefly centrifuge the PCR mix after thawing</li>
 +
<li>Place a thin-walled PCR tube on ice and add the different components for a 50 μL PCR reaction</li>
 +
<li>Gently vortex the samples</li>
 +
<li>Perform PCR using the recommended thermal cycling conditions</li>
 +
</div>
 +
</div>
 +
 +
<div class="group center">
 +
 +
<p class="text">
 +
The PCR Mix from Thermo Scientific contains Taq DNA polymerase, Green Buffer, MgCl2, dNTPs but also two tracking dyes and a density reagent that allows for direct loading of the PCR product on a migration gel.
 +
<br>
 +
The template DNA concentration has to be adapted in order to be between 10 pg and 1 μg in the final volume of 50 μL. The template DNA can come from a miniprep solution or from a single colony. The primer concentrations have to be between 0.1 μM and 1 μM.
 +
<br>
 +
Each PCR reaction has to be adapted to the length of the PCR products, and to the melting temperature Tm of the primers. The extension step lasts 1 min for PCR products up to 2 kb. For longer products, the extension time has to be prolonged by 1 min/kb.
 +
</p>
 +
</div>
 +
 +
 +
<div class="group center">
 +
<table class="df" style="font-size:15px;">
 +
        <thead>
 +
          <tr>
 +
            <th>Step</th>
 +
<th>Temperature (°C)</th>
 +
<th>Time</th>
 +
<th>Number of cycles</th>
 +
          </tr>
 +
        </thead>
 +
        <tbody>
 +
          <tr>
 +
            <td><p>Initial denaturation</p></td>
 +
            <td><p>95</p></td>
 +
<td><p>1-3 min</p></td>
 +
<td><p>1</p></td>
 +
          </tr>
 +
          <tr>
 +
            <td><p>Denaturation</p></td>
 +
            <td><p>95</p></td>
 +
<td><p>30s</p></td>
 +
<td rowspan=3><p>25-40</p></td>
 +
          </tr>
 +
          <tr>
 +
            <td><p>Annealing</p></td>
 +
            <td><p>Tm – 5°C</p></td>
 +
            <td><p>30s</p></td>
 +
 +
          </tr>
 +
          <tr>
 +
            <td><p>Extension</p></td>
 +
            <td><p>72</p></td>
 +
<td><p>Adapt to the length</p></td>
 +
          </tr>
 +
 
 +
  <tr>
 +
            <td><p>Final extension</p></td>
 +
            <td><p>72</p></td>
 +
<td><p>5-15 min</p></td>
 +
<td><p>1</p></td>
 +
          </tr>
 +
        </tbody>
 +
      </table>
 +
  </div>
 +
 +
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
 +
 
 
 
<center>
 
<center>
<div class="title">
+
<div class="title" id="TPX">
<h3>Protocols for TPX permeability tests</h3>
+
<h3>Protocols for TPX® permeability tests</h3>
 
     </div> </center>
 
     </div> </center>
 
 
<div class="subtitle">
+
<h3>Preparation of TPX bag</h3>
+
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
        <li><a href="#prepTPX">- Preparation of TPX® bag</a></li>
 +
        <li><a href="#permeabTPX">- Permeability test</a></li>
 +
        <li><a href="#sterilTPX1">- Sterility test of TPX® bag</a></li>
 +
 
 +
      </ul>
 +
    </div>
 +
</center>
 +
 +
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
     
 +
        <li><a href="#cultTPX">- Culture test of <i>E. coli</i> in TPX® bag</a></li>
 +
      </ul>
 +
    </div>
 +
</center>
 +
 +
<div class="subtitle" id="prepTPX">
 +
<h3>Preparation of TPX® bag</h3>
 
     </div>
 
     </div>
  
 
<div class="group">
 
<div class="group">
 
<div class="one_quarter first" >
 
<div class="one_quarter first" >
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Materials</h3>
 
<h3>Materials</h3>
 
</div>
 
</div>
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
<li>TPX, gas permeable plastic</li>
+
<li>TPX®, gas permeable plastic</li>
 
<li>Fusing machine</li>
 
<li>Fusing machine</li>
 
<li>2 mM Formic acid solution</li>
 
<li>2 mM Formic acid solution</li>
Line 717: Line 946:
  
 
<div class="three_quarter">
 
<div class="three_quarter">
<div class="subsubtitle">    
+
<div class="subsubsubtitle">    
 
<h3>Methods</h3>
 
<h3>Methods</h3>
 
</div>
 
</div>
 
<ol align="justify" style="font-size:15px;">
 
<ol align="justify" style="font-size:15px;">
 
<li>Prepare plastic bag in sticking on 3 sides over 4 with fusing machine</li>
 
<li>Prepare plastic bag in sticking on 3 sides over 4 with fusing machine</li>
<li>Add 7mL of appropriate solution in plastic bag</li>
+
<li>Add 7 mL of appropriate solution in plastic bag</li>
 
<li>Stick on the last side with fusing machine</li>
 
<li>Stick on the last side with fusing machine</li>
 
</div>
 
</div>
Line 729: Line 958:
  
 
 
<div class="subtitle">
+
<div class="subtitle" id="permeabTPX">
 
<h3>Permeability test</h3>
 
<h3>Permeability test</h3>
 
     </div>
 
     </div>
Line 735: Line 964:
 
<div class="group center">
 
<div class="group center">
 
<p style="font-size:15px;" align="justify">
 
<p style="font-size:15px;" align="justify">
To test gas permeability of TPX plastic, we use the same protocol as “Test of gas concentration”.  
+
To test gas permeability of TPX® plastic, we use the same protocol as “Test of gas concentration”.  
 
The only change is that no filters were used because the sterility is not necessary.
 
The only change is that no filters were used because the sterility is not necessary.
 
</p>
 
</p>
 
</div>  
 
</div>  
 +
  
 
<center>
 
<center>
<img src="https://static.igem.org/mediawiki/2015/3/37/TLSE_expe_2.png"/>
+
 
<p class="legend">The device used for the permeability test </p></center>
+
<img src="https://static.igem.org/mediawiki/2015/3/3c/TLSE_expe_2b.png" style="width:60%"/>
 +
<p class="legend">
 +
Photo 9: The device used for the permeability test
 +
</p></center>
 
<br>
 
<br>
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
+
 
 
<div class="group center">
+
 
<div class="title" >    
+
<div class="subtitle" id="sterilTPX2">
<h3>Transformation Protocol: RbCl method</h3>
+
<h3>Sterility test of TPX® bag</h3>
 +
<h3 style="font-size:18px">&nbsp;&nbsp;&nbsp;&nbsp;Demonstrate that the TPX® bag is impermeable to bacteria</h3>
 +
</div>
 +
 
 +
 
 +
<div class="group">
 +
<div class="one_quarter first" >
 +
<div class="subsubsubtitle">    
 +
<h3>Materials</h3>
 
</div>
 
</div>
 +
<ul align="justify" style="font-size:15px;">
 +
<li>TPX bags</li>
 +
<li>M9 defined Medium</li>
 +
<li><i>E. coli</i> BW 25113</li>
 +
<li>Steril laboratory glass bottle</li>
 
</div>
 
</div>
  
  <div class="subtitle">
+
<div class="three_quarter">
 +
<div class="subsubsubtitle">  
 +
<h3>Methods</h3>
 +
</div>
 +
<ol align="justify" style="font-size:15px;">
 +
<li>Overnight culture of <i>E. coli</i> BW 25113 at 37 °C</li>
 +
<li>Inoculate a small TPX® bag at OD<SUB>600 nm</SUB> = 0.1 in LB medium (Final Volume = 8 mL)
 +
</li>
 +
<li>Negative Control: Fill a small TPX® bag with M9 medium (Final Volume=8 mL)
 +
</li>
 +
<li>Dispose each small bag in a Steril glass measuring cylinder containing M9 medium</li>
 +
<li> Incubate at 37 °C</li>
 +
<li>Measure OD<SUB>600 nm</SUB> twice a day</li>
 +
</div>
 +
</div>
 +
 +
 +
<div class="subtitle" id="cultTPX">
 +
<h3>Culture test of <i>E. coli</i> in TPX® bag</h3>
 +
</div>
 +
 
 +
 
 +
<div class="group">
 +
<div class="one_quarter first" >
 +
<div class="subsubsubtitle">  
 +
<h3>Materials</h3>
 +
</div>
 +
<ul align="justify" style="font-size:15px;">
 +
<li>TPX bags</li>
 +
<li>LB Medium</li>
 +
<li>Steril clips</li>
 +
<li><i>E. coli</i> BW 25113</li>
 +
<li>Steril laboratory flask</li>
 +
</div>
 +
 
 +
<div class="three_quarter">
 +
<div class="subsubsubtitle">  
 +
<h3>Methods</h3>
 +
</div>
 +
<ol align="justify" style="font-size:15px;">
 +
<li>Overnight culture of E. coli BW 25113 at 37 °C</li>
 +
<li>Inoculate a small TPX® bag at OD<SUB>600 nm</SUB> = 0.1 in LB medium (Final Volume = 8 mL)
 +
</li>
 +
<li>Close the small bag via fusing machine and Put the closed small bag in a Steril laboratory flask
 +
 
 +
</li>
 +
<li>Positive Control: Inoculate a culture tube at OD<SUB>600 nm</SUB> = 0.1 in LB medium (Final Volume = 20 mL)
 +
</li>
 +
<li> Incubate at 37 °C</li>
 +
<li>Measure OD<SUB>600 nm</SUB> twice a day</li>
 +
</div>
 +
</div>
 +
 +
<center><hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
 +
 
 +
<center><div class="title" id="transfo">  
 +
<h3>Transformation Protocol: RbCl method</h3>
 +
</div>
 +
</center>
 +
 
 +
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
        <li><a href="#mediaAndSol">- Media and solution</a></li>
 +
        <li><a href="#competentCell">- Preparation of Competent Cells</a></li>
 +
        <li><a href="#transfoCell">- Transformation of Competent Cells </a></li>
 +
        <li><a href="#minipreps">- Minipreps</a></li>
 +
      </ul>
 +
    </div>
 +
</center>
 +
 
 +
  <div class="subtitle" id="mediaAndSol">
 
     <h3> Media and solution</h3>  <!-- MEDIA AND SOLUTION -->
 
     <h3> Media and solution</h3>  <!-- MEDIA AND SOLUTION -->
 
     </div>
 
     </div>
Line 767: Line 1,084:
 
         <tbody>
 
         <tbody>
 
           <tr>
 
           <tr>
             <td><!-- YETM 500mL -->
+
             <td><!-- YETM 500 mL -->
 
<ul style="font-size:15px;"align="left">
 
<ul style="font-size:15px;"align="left">
 
<li> 2.5 g Yeast Extract </li>
 
<li> 2.5 g Yeast Extract </li>
Line 775: Line 1,092:
 
<li> <b>For Plates</b>: add 7.5 g of Agar </li>
 
<li> <b>For Plates</b>: add 7.5 g of Agar </li>
 
</ul>
 
</ul>
</td><!-- YETM 500mL END -->
+
</td><!-- YETM 500 mL END -->
 
 
 
<td><!-- TFB1 200 mL -->
 
<td><!-- TFB1 200 mL -->
Line 808: Line 1,125:
  
  
<div class="subtitle">
+
<div class="subtitle" id="competentCell">
 
     <h3> Preparation of Competent Cells </h3>  <!-- COMPETENT CELLS -->
 
     <h3> Preparation of Competent Cells </h3>  <!-- COMPETENT CELLS -->
 
     </div>
 
     </div>
 
<div class="group">
 
<div class="group">
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
<li>1. Streak cells froms frozen stock onto YETM plate. Incubate overnight at 37 °C </li>
+
<li>1. Streak cells from frozen stock onto YETM plate. Incubate overnight at 37°C </li>
<li>2. Pick a single fresh colony to inoculate 5 mL of YETM medium. Grow over night at 37 °C.</li>
+
<li>2. Pick a single fresh colony to inoculate 5 mL of YETM medium. Grow over night at 37°C.</li>
 
<li><b>Do not vortex cells at any time after this point in the procedure</b></li>
 
<li><b>Do not vortex cells at any time after this point in the procedure</b></li>
 
<li>3. Dilute 1 mL of culture into 50 mL YETM medium prewarmed to 37 °C</li>
 
<li>3. Dilute 1 mL of culture into 50 mL YETM medium prewarmed to 37 °C</li>
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
 
<li> Grow at 37 °C for 2 hours with agitation </li>
 
<li> Grow at 37 °C for 2 hours with agitation </li>
<li> Volumes can be scaled up 5X and all of the 5mL overnight culture can be used </li>
+
<li> Volumes can be scaled up 5X and all of the 5 mL overnight culture can be used </li>
 
</ul>
 
</ul>
 
<li> 4. Transfer culture to sterile 50 mL tube. Chill on ice/water 10-15 minutes </li>
 
<li> 4. Transfer culture to sterile 50 mL tube. Chill on ice/water 10-15 minutes </li>
Line 838: Line 1,155:
 
</div> <!-- COMPETENT CELLS END-->
 
</div> <!-- COMPETENT CELLS END-->
 
 
<div class="subtitle">
+
<div class="subtitle" id="transfoCell">
 
     <h3> Transformation of Competent Cells </h3>  <!-- COMPETENT CELLS -->
 
     <h3> Transformation of Competent Cells </h3>  <!-- COMPETENT CELLS -->
 
</div>
 
</div>
Line 845: Line 1,162:
  
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
<li>1. If starting with frozen competent cells, warm tube/cells by gently twirling between your fingers until just thawed. <br>Immedately place on ice for about 5 minutes </li>
+
<li>1. If starting with frozen competent cells, warm tube/cells by gently twirling between your fingers until just thawed. <br>Immediately place on ice for about 5 minutes </li>
<li>2. Add to 1,5 mL eppendorff on ice: 2-3 μL iGEM plate or 1 μL plasmid or 10 μL ligation.</li>
+
<li>2. Add to 1,5 mL eppendorf on ice: 2-3 μL iGEM plate or 1 μL plasmid or 10 μL ligation.</li>
 
<li>3. Add 100 μL of competent cells and mix by gentle re-pipetting</li>
 
<li>3. Add 100 μL of competent cells and mix by gentle re-pipetting</li>
 
<li> 4. Incubate cells on ice for 20-30 minutes </li>
 
<li> 4. Incubate cells on ice for 20-30 minutes </li>
 
<li> 5. Heat shock the cells exactly 90 seconds at 42 °C </li>
 
<li> 5. Heat shock the cells exactly 90 seconds at 42 °C </li>
 
<li> 6. Return cells on ice for 2 minutes </li>
 
<li> 6. Return cells on ice for 2 minutes </li>
<li> 7. Add 1mL of YETM medium. Incubate at 37 °C for 45-60 minutes with slow gentle shaking </li>
+
<li> 7. Add 1 mL of YETM medium. Incubate at 37 °C for 45-60 minutes with slow gentle shaking </li>
 
<li> 8. Plate 0.1-0.2 mL of transformed cells on LB-plate containing the appropriate antibiotic. Incubate  overnight at 37°C</li>
 
<li> 8. Plate 0.1-0.2 mL of transformed cells on LB-plate containing the appropriate antibiotic. Incubate  overnight at 37°C</li>
 
  </ul>
 
  </ul>
Line 857: Line 1,174:
  
  
<div class="subtitle">
+
<div class="subtitle" id="minipreps">
 
     <h3> Minipreps </h3>  <!-- MINIPREPS -->
 
     <h3> Minipreps </h3>  <!-- MINIPREPS -->
 
</div>
 
</div>
Line 874: Line 1,191:
 
<div class="group center">
 
<div class="group center">
 
 
<center><div class="title" >    
+
<center><div class="title" id="cloning">    
 
<h3 >Cloning</h3><!-- CLONING -->
 
<h3 >Cloning</h3><!-- CLONING -->
 
</div></center>
 
</div></center>
 
</div>
 
</div>
 +
 +
 +
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
        <li><a href="#sameAntibio">- Digestion: both parts have the same antibiotic resistance</a></li>
 +
        <li><a href="#diffAntibio">- Digestion: The two parts have a different antibiotic resistance</a></li>
 +
       
 +
      </ul>
 +
    </div>
 +
</center>
 +
 +
<center> 
 +
    <div id="breadcrumb" class="clear" style="float: center;" >
 +
  <ul>
 +
  <li><a href="#migration">- Migration and gel extraction</a></li>
 +
        <li><a href="#ligation">- Ligation</a></li>
 +
        <li><a href="#cloningtransfo">- Transformation</a></li>
 +
       
 +
      </ul>
 +
    </div>
 +
</center>
 +
 +
 
<div class="subtitle" >    
 
<div class="subtitle" >    
 
<h3>First step: Digestion</h3>
 
<h3>First step: Digestion</h3>
 
</div>
 
</div>
  
<div class="group center">
+
 
<div class="subsubtitle" >    
+
<div class="subsubsubtitle" id="sameAntibio">    
 
<h3>Both parts have the same antibiotic resistance</h3>
 
<h3>Both parts have the same antibiotic resistance</h3>
 
</div>
 
</div>
</div>
+
 
  
 
<div class="group center">
 
<div class="group center">
Line 894: Line 1,235:
 
             <th>Vector</th>
 
             <th>Vector</th>
 
<th>Insert</th>
 
<th>Insert</th>
 +
<th>Digestion control first enzyme</th>
 +
<th>Digestion control second enzyme</th>
 
           </tr>
 
           </tr>
 
         </thead>
 
         </thead>
 
         <tbody>
 
         <tbody>
 
 
           <tr>
 
           <tr>
             <td><p>5 µL of miniprep plasmid</p></td>
+
             <td><p>Volume equivalent to 1 µg of vector miniprep </p></td>
             <td><p>10 µL of miniprep plasmid</p></td>
+
             <td><p>Volume equivalent to 1 µg of insert miniprep </p></td>
          
+
         <td><p>Volume equivalent to 1 µg of vector miniprep </p></td>
 +
<td><p>Volume equivalent to 1 µg of vector miniprep </p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
 
             <td><p>1 µL of each restriction enzymes</p></td>
 
             <td><p>1 µL of each restriction enzymes</p></td>
 
             <td><p>1 µL of each restriction enzymes</p></td>
 
             <td><p>1 µL of each restriction enzymes</p></td>
            
+
           <td><p>1 µL of the first restriction enzyme</p></td>
 +
<td><p>1 µL of the second restriction enzyme</p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
             <td><p>2 µL of Green Buffer</p></td>
+
             <td><p>2 µL of Fast Digest Green Buffer (Thermo Scientific™)</p></td>
             <td><p>2 µL of Green Buffer</p></td>
+
             <td><p>2 µL of Fast Digest Green Buffer (Thermo Scientific™)</p></td>
           
+
            <td><p>2 µL of Fast Digest Green Buffer (Thermo Scientific™)</p></td>
 +
<td><p>2 µL of Fast Digest Green Buffer (Thermo Scientific™)</p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
             <td><p>10 µL of Milli-Q water</p></td>
+
             <td><p>Up to 20 µL of Milli-Q water</p></td>
             <td><p>5 µL of Milli-Q water</p></td>
+
             <td><p>Up to 20 µL of Milli-Q water</p></td>
 +
<td><p>Up to 20 µL of Milli-Q water</p></td>
 +
<td><p>Up to 20 µL of Milli-Q water</p></td>
 
           </tr>
 
           </tr>
 
  <tr>
 
  <tr>
  <td colspan=2><p>Incubate 15 minutes at 37°C</p></td>
+
  <td colspan=4><p>Incubate 15 minutes at 37 °C</p></td>
 
  </tr>
 
  </tr>
 
         </tbody>
 
         </tbody>
Line 925: Line 1,272:
 
   
 
   
 
   
 
   
  <div class="group center">
+
 
<center><div class="subsubtitle">    
+
<div class="subsubsubtitle" id="diffAntibio">    
 
<h3>The two parts have a different antibiotic resistance</h3>
 
<h3>The two parts have a different antibiotic resistance</h3>
</div></center>
 
 
</div>
 
</div>
 +
  
 
<div class="group center">
 
<div class="group center">
Line 940: Line 1,287:
 
         <tbody>
 
         <tbody>
 
           <tr>
 
           <tr>
             <td><p>5 µL of miniprep plasmid</p></td>
+
             <td><p>Volume equivalent to 1 µg of DNA miniprep </p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
Line 946: Line 1,293:
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
             <td><p>2 µL of Green Buffer</p></td>
+
             <td><p>2 µL of Fast Digest Green Buffer (Thermo Scientific™)</p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
             <td><p>9 µL of Milli-Q water</p></td>
+
             <td><p>Up to 20 µL of Milli-Q water</p></td>
 
           </tr>
 
           </tr>
 
  <tr>
 
  <tr>
Line 958: Line 1,305:
 
  </div>
 
  </div>
 
   
 
   
<center><div class="subsubtitle" >    
+
<div class="subsubsubtitle" id="migration">    
 
<h3>Migration and gel extraction</h3>
 
<h3>Migration and gel extraction</h3>
</div></center>   
+
</div>   
  
 
<div class="group">
 
<div class="group">
Line 967: Line 1,314:
 
<li>2. Put 20 µL of sample + 6 µL of marker (1 kb for 1 % gel and 100 pb for 2 %) into the well</li>
 
<li>2. Put 20 µL of sample + 6 µL of marker (1 kb for 1 % gel and 100 pb for 2 %) into the well</li>
 
<li>3. Migration for 30 min at 100 V or 1 hour at 50 V</li>
 
<li>3. Migration for 30 min at 100 V or 1 hour at 50 V</li>
<li> 4. Bathe 10 minutes in BET</li>
+
<li> 4. Bath 10 minutes in BET</li>
 
<li> 5. Wash in water for 5 minutes </li>
 
<li> 5. Wash in water for 5 minutes </li>
 
<li> 6. The gel extraction is realized thanks to the QIAGEN Gel Extraction Kit</li>
 
<li> 6. The gel extraction is realized thanks to the QIAGEN Gel Extraction Kit</li>
Line 981: Line 1,328:
 
   
 
   
 
   
 
   
<div class="subtitle" >    
+
<div class="subtitle" id="ligation" >    
 
<h3>Second step: Ligation</h3>
 
<h3>Second step: Ligation</h3>
 
</div>   
 
</div>   
Line 990: Line 1,337:
 
           <tr>
 
           <tr>
 
             <th>Mix</th>
 
             <th>Mix</th>
<th>Control</th>
+
<th>Negative Control</th>
 +
<th>Positive Control</th>
 
           </tr>
 
           </tr>
 
         </thead>
 
         </thead>
 
         <tbody>
 
         <tbody>
 
           <tr>
 
           <tr>
             <td><p>10 µL of insert</p></td>
+
             <td><p>Volume equivalent to 3 molecules of insert (for one molecule of vector)</p></td>
 
<td><p>no insert</p></td>
 
<td><p>no insert</p></td>
 +
<td><p>Volume equivalent to 3 molecules of insert (for one molecule of vector)</p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
             <td><p>4 µL of vector</p></td>
+
             <td><p>Volume equivalent to 50 ng of digested vector</p></td>
<td><p>4 µL of vector</p></td>
+
<td><p>Volume equivalent to 50 ng of digested vector</p></td>
 +
<td><p>Volume equivalent to 50 ng of undigested vector</p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
             <td><p>2 µL of 10x T4 buffer</p></td>
+
             <td><p>2 µL of 10X T4 buffer</p></td>
<td><p>2 µL of 10x T4 buffer</p></td>
+
<td><p>2 µL of 10X T4 buffer</p></td>
 +
<td><p>2 µL of 10X T4 buffer</p></td>
 
           </tr>
 
           </tr>
 
           <tr>
 
           <tr>
 
             <td><p>0.5 µL of T4 ligase</p></td>
 
             <td><p>0.5 µL of T4 ligase</p></td>
 
<td><p>0.5 µL of T4 ligase</p></td>
 
<td><p>0.5 µL of T4 ligase</p></td>
 +
<td><p>0.5 µL of T4 ligase</p></td>
 
           </tr>
 
           </tr>
 
  <tr>
 
  <tr>
  <td><p>3.5 µL of Milli-Q water</p></td>
+
  <td><p>Up to 20 µL of Milli-Q water</p></td>
  <td><p>13.5 µL of Milli-Q water</p></td>
+
  <td><p>Up to 20 µL of Milli-Q water</p></td>
 +
<td><p>Up to 20 µL of Milli-Q water</p></td>
 
  </tr>
 
  </tr>
 
  <tr>
 
  <tr>
  <td colspan=2><p>&nbsp;Incubate the ligation mix 15 minutes at room temperature (22°C)</p></td>
+
  <td colspan=3><p>&nbsp;Incubate the ligation mix 15 minutes at room temperature (22°C)</p></td>
 
  </tr>
 
  </tr>
 
  <tr>
 
  <tr>
  <td colspan=2><p>&nbsp;Keep the tubes in ice or at -20 °C to prepare the transformation</p></td>
+
  <td colspan=3><p>&nbsp;Keep the tubes in ice or at -20 °C to prepare the transformation</p></td>
 
  </tr>
 
  </tr>
 
         </tbody>
 
         </tbody>
Line 1,024: Line 1,377:
 
  </div>
 
  </div>
 
   
 
   
<div class="subtitle" >    
+
<div class="subtitle" id="cloningtransfo">    
<h3>Third step: Ligation</h3>
+
<h3>Third step: Transformation</h3>
 
</div>   
 
</div>   
  
 
<div class="group">
 
<div class="group">
 
<ul align="justify" style="font-size:15px;">
 
<ul align="justify" style="font-size:15px;">
<li>1. Take 10 µL of the ligation mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol </li>
+
<li>1a. Take 10 µL of the ligation mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol </li>
 +
<li>1b. Positive control: take 10 µL of the ligation mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol </li>
 +
<li>1c. First restriction enzyme digestion control: take 10 µL of the corresponding digestion mix (First step) for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol </li>
 +
<li>1d. Second restriction enzyme digestion control: take 10 µL of the corresponding digestion mix (First step) for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol </li>
 +
<li>1e. Negative control: take 10 µL of the corresponding mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol </li>
 
<li>2. Plate the solution on selective medium overnight at 37 °C</li>
 
<li>2. Plate the solution on selective medium overnight at 37 °C</li>
 
</ul>
 
</ul>
</div>
+
</div><br><br>
 +
<center>
 +
<hr style="width:66%;height:1px;border:none;color:rgba(29, 5, 79, 1);background-color:rgba(29, 5, 79, 1); z-index:50; position:relative;"></center>
 +
<div class="group center">
 +
 +
<center><div class="title" id="infusion">  
 +
<h3 >InFusion cloning protocol</h3>
 +
</div></center>
 +
 
 +
</div> <br><br>
 +
<center><img src="https://static.igem.org/mediawiki/2015/5/52/TLSE_Protocols_infusion_1.png" style="width:25%;">
 +
<p class"legend">
 +
Principle of In Fusion cloning
 +
</p></center>
 +
<div class="group">
 +
<ul align="justify" style="font-size:15px;">
 +
<li>1. Design the tailed-oligonucleotides for the vector and the inserts. The tail of the 5’oligonucleotide must be the 20 last nucleotides of the previous fragment and the tail of the 3’oligonucleotide must be the 20 first nucleotides of the next fragment. </li>
 +
 +
<li>2. Amplify the different fragments with the <a href="#PCR">previously designed oligonucleotides</a> </li>
 +
<li>3. Clean the PCR products either using a spin column purification kit or by digesting with DpnI. For NEB DpnI, mix the different PCR products together, add 10X CutSmart Buffer and DpnI (1 µL in a 20 µL mix); incubate at 37°C for 20 minutes and inactive at 80 °C during 30 minutes.</li>
 +
<li>4. Set up the In Fusion cloning reaction :</li>
 +
<center><br>
 +
<table class="result" style="padding-left:50px;">
 +
<tbody>
 +
<tr>
 +
<th></th>
 +
<th>Ligation</th>
 +
<th>Control</th>
 +
</tr>
 +
<tr>
 +
<td>5X In-Fusion HD Enzyme Premix</td>
 +
<td>2 µL</td>
 +
<td>-</td>
 +
</tr>
 +
<tr>
 +
<td>Clean PCR mix</td>
 +
<td>4 µL</td>
 +
<td>4 µL</td>
 +
</tr>
 +
<tr>
 +
<td>MilliQ water nuclease free</td>
 +
<td>4 µL</td>
 +
<td>6 µL</td>
 +
</tr>
 +
 +
<tr>
 +
<td>Total</td>
 +
<td>10 µL</td>
 +
<td>10 µL</td>
 +
</tr>
 +
</tbody>
 +
</table></center>
 +
<br>
 +
 +
<li>5. Incubate at 50 °C during 15 min and then cool on ice</li>
 +
<li>6. Transform commercial ultra-competent cells (10<sup>8</sup> to 10<sup>9</sup> cfu/µg DNA) with 2.5 µL of the ligation using provided with the competent cells. Plate several 10-fold dilutions of the transformation mix.</li>
 +
 +
</ul>
 +
</ul>
 +
</div>
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 +
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<center><p class="maintitle">  
 
References
 
</p></center>
 
<br>
 
<div class="clear">
 
 
</div>
 
<br>
 
</div>
 
 
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Latest revision as of 22:16, 18 September 2015

iGEM Toulouse 2015

Experiments & Protocols


Content

Sampling of varroa

To run tests with varroas it is necessary to get them back from beehive directly because they cannot live without bees.

Materials

  • Bee hive
  • Beekeeper suit
  • Gloves
  • Smoker
  • Dry twigs
  • Tweezers
  • Big brush
  • Small brush
  • Petri dishes
    Ø x h = 35 x 15 mm

Methods

  1. Slip beekeeper suit and gloves on and go to beehive
  2. Fire dry twigs in smoker
  3. Open bee hive and activate smoker to get bees inside the hive
  4. Take a frame out the hive and remove bees with big brush and smoker
  5. Close beehive
  6. In the lab, put the frame on a table against the wall
  7. With tweezer drill hole into one beehive cell
  8. Remove larvae and look for varroas on larvae and on beehive cell
  9. If there are varroas, take them with a small brush and put them on Petri dishes
  10. Make sure there are two or three larvae on Petri dishes in order to allow survival of varroas
  11. Start again step 7 to 9 until you have enough varroas



Steps 1, 4 & 7: Our teams members gathering varroas on infected larvae

Standardization of varroas and sampling

When we take varroas directly from frame, as it is described in protocol “Sampling Varroas”, we have varroas in different phases. In order to have varroas in the same phase it is necessary to add one step and it is important for reproducibility of the experiments. With this method we place varroas on adult bees so all varroas will be in phoretic phase.

Materials

  • Bees in box with aeration and glucose
  • Varroas from protocol “Sampling varroas”
  • Gas cylinder of CO2
  • Small brush
  • Tweezers
  • Petri dishes
    Ø x h = 35 x 15 mm

Methods

  1. With small brush take varroas from Petri dish and put them on bees in box through aeration holes
  2. Place the box in a 35 °C incubator overnight. Make sure you have a bowl with water in order to have enough humidity in incubator
  3. Take the box out of incubator
  4. Add CO2 from gas cylinder into the box until all bees fall down
  5. Open the box, take a bee with tweezer and look for varroas
  6. When you find a varroa take him with small brush and replace bee in the box
  7. Start again step 5 and 6 until you have enough varroas


Steps 2 & 5: Varroas gathering on infected bees

Attraction test on varroas

In order to test the attraction effect of butyric acid on varroas a Y test tube was built, as it is showed below. A glass pipe was chosen because on plastic varroas could load themselves with electrostatics and die. For butyric acid, the concentration chosen 4 % (V/V) because this is the concentration used in the patent quoted (see “Attribution” part).

Materials

  • Pump wich expels air
  • 15 mL Flacon tube
  • Plastic pipe
    Ø = 10 mm
  • Glass T pipe
    Ø = 10 mm, made by a glassworker
  • Plastic separator
  • Carded cotton
  • Absorbent cotton
  • 5mL 4% (V/V) Butyric acid
  • 5mL Water
  • Standardized varroas

Methods

  1. Put a cotton on Petri dish and add 400 µL of one acid formic solution
  2. Place three varroas on this Petri dish and close it
  3. Start again step1 and 2 for each formic acid solution and water
  4. Each 30 minutes check if varroas are alive. To do that:
  5. When varroa heads for one side of Glass T tube and covers more than 2 cm test is over and we write down the side choosen by varroa (Butyric acid or Water)
  6. Two tests can be made in the same time thanks to the plastic separator

br>

Glass T-tube: Varroa is going to butyric acid (at left)

Mortality test on varroas

Test the toxicity of formic acid on varroas. When beekeepers use formic acid for long treatment they place a diffuser at the top of the hive and formic acid concentration was assessed at 200 ppm 1 on average which is equivalent to 7.8 mmol.m-3. As gas concentration is difficult to evaluate we calculated the liquid concentration balance using the ideal gas law and Henry’s law. To simplify calculation we noted down formic acid A.

$$ P\cdot V = n\cdot R\cdot T, \textrm{ideal gaz law} $$ $$ P_A = C_A\cdot R\cdot T = 7.826\cdot10^{-3}\times8.314\times293=19.96 Pa $$

  • PA: partial pressure of A in Pa
  • CA: Concentration of A in air in mol.m-3
  • R: perfect gaz constant = 8.314 J.mol-1.K-1
  • T: temperature in °K

$$ P_A = H_A\cdot C_{A,eq}, \textrm{Henry's law} $$ $$ C_{A,eq} = \frac{19.964}{0.019} = 1.019 mol.L^{-1}$$

  • CA,eq: equivalent concentration in liquid in mol.L-1
  • HA: Henry's constant = 0.019 Pa.m3mol-1

We chose a positive control with a higher concentration, 2 mol.L-1, and then decreasing concentration in order to identify which minimum concentration could kill varroa. We used water as a negative control. For this test we use varroas directly from frames because we did not have enough standardized varroas.

Materials

  • Petri dishes
    Ø x h = 35 x 15 mm
  • Varroas form “Sampling varroas”
  • Cotton
  • Acid formic solutions:
    • 2 mol.L-1
    • 10 mmol.L-1
    • 1 mmol.L-1
    • 500 µmol.L-1
    • 50 µmol.L-1
  • Water

Methods

  1. Put a cotton on Petri dish and add 400 µL of one acid formic solution
  2. Place three varroas in this Petri dish and close it
  3. Start again step1 and 2 for each formic acid solution and water
  4. Every 30 minutes check if varroas are alive. To do that:
    1. Tap on Petri dish and see if varroa moves. If it does varroa is still alive, if not see below
    2. Observe through a binocular magnifier if varroa move. If it does, it is still alive.


Varroa mortality experiment

Protocols for culture tests

Cytotoxicity tests

Choice of concentrations

In the beginning we tested high and low concentrations and we further adapted the concentrations. In the end we worked with these concentrations:

  • Butyric acid : 218 mM, 109 mM, 10.9 mM, 5.45 mM and 1.09 mM
  • Formic acid : 100 mM, 10 mM, 1 mM 500 µM, 100 µM, 50 µM and 25 µM

Materials

  • Optical reader, OPTIMA MARS Analysis
  • 48 wells plates
  • Pre-culture of E. coli BW 25113
  • Acid solutions
  • Medium : LB, M9 15 mM of glucose or 30 mM of glucose

Methods

  1. Add 400 µL of medium in each well
  2. Add 50 µL of pre-culture
  3. Add 50 µL of acid solution
  4. Place the 48 well plate in the optical reader
  5. Adjust parameters on computer.
    Usually we set 250 cycles around 24 hours so we have an OD measurement every six minutes

Note: Each condition is tested in three replicates

Culture on erlenmeyers and TubeSpin® Bioreactors

      - Inoculation and sampling

Materials

  • Pre-culture of E. coli BW 25113 in LB
  • Spectrophotometer
  • 1mL Spectrophotometer cuvettes
  • Centrifuge
  • Erlenmeyers
  • TubeSpin® Bioreactors from TPP brand
  • Medium : M9 15 mM of glucose or 30 mM of glucose
  • Incubators at 37 °C, 130 rpm and without agitation
  • 1.5 mL Eppendorf
  • 0.2 µm filters

Methods

  1. Add 50 mL of medium on erlenmeyer and TubeSpin® Bioreactor
  2. Inoculate from pre-culture to have OD600nm=0.1.
    To do that centrifuge the appropriate volume of pre-culture, then remove LB medium and resuspend sediment with M9 medium to inoculate.
    Note: This step permits to eliminate substrates from LB medium which could interfere during NMR analysis.
  3. Place erlenmeyers in incubator 37 °C 130 rpm and TubeSpin® Bioreactor in incubator 37 °C without agitation
  4. Sampling every two hours the first day:
    • Take 1 mL of culture in 1.5 mL Eppendorf.
      For TubeSpin® Bioreactor use needle and syringe in order not to let air enter.
    • Add 100 µL of sample in spectrophotometer cuvette, complete with 900 µL water and measure OD600 nm with spectrophotometer
    • Centrifuge the rest of samples at 13,000 rpm during 3 minutes
    • Filter the supernatant through a 0.2 µm filter and conserve it at -20 °C
  5. Days follow sample once a day with method below and plate on Petri dish an appropriate dilution in order to know if bacteria are alive

      - NMR analysis

Materials

  • Culture supernatants from -20°C
  • 2.5 mM TSP (Trimethylsilyl propanoic acid) diluted in D2O
  • 0.5 mm NMR tubes
  • 1.5 mL Eppendorf
  • Spinners (5mm)
  • 500 MHz Bruker Avance Spectrometer

Methods

  1. Add 400 µL of culture supernatant in 1.5 mL Eppendorf
  2. Add 100 µL of TSP solution
  3. Place the mix in 0.5 mm NMR tubes
  4. Place NMR tube into spinner, sample is ready to analyse


Micro-aerobic culture, filtration and NMR samples



500MHz NMR Spectrometer used for culture supernatant analysis

Culture on 48 wells plates

In order to determine the right concentration of polysaccharide and enzyme of BioSilta kit we have to do several cultures at the same time. So, we use an optical reader and 48 wells plates.

Materials

  • Optical reader, OPTIMA MARS Analysis
  • 48 wells plates
  • Pre-culture of E. coli BW 25113
  • Different concentrations of BioSilta medium
  • For one concentration of BioSilta medium different concentrations of enzyme

Methods

  1. Add 450 µL of medium in each well
  2. Add 50 µL of pre-culture
  3. Place the 48 well plate in the optical reader
  4. Adjust parameters on computer. We tested culture between one day and ten days

Note: Each condition is tested in two replicates. According to our results we adapt concentrations of Biosilta medium and enzyme, results are exposed in device part.

Enzyme kinetic

Materials

  • Spectrophotometer
  • BioSilta medium
  • BioSilta enzyme solution named Reagent A (3000U/L)
  • Bradford’s reagent
  • 1.5 mL Eppendorf
  • Standard solutions of glucose

Methods

  1. For each standard solutions : in a 1.5 mL Eppendorf sample 10 µL and add 1 mL Bradford’s Reagent, wait 20 minutes and measure OD505 nm
  2. Plot glucose concentration in function of OD505nm and determine the linear region
  3. Add 1.5 mL of BioSilta medium and 45 µL of reagent A (50 U/L) in an Eppendorf
  4. Sampling every 30 minutes:
    1. Take 10 µL and add 1 mL of Bradford’s reagent in an Eppendorf
    2. Wait 20 minutes
    3. Measure OD505 nm
    4. If OD505 nm is over linear region dilute sample and measure OD505 nm again
  5. Stop sampling when glucose concentration no longer change

Acids production test

In order to test if E. coli produces formic acid and butyric acid with genes added, we made culture test with modified bacteria. We used the same protocol as “Culture on Erlenmeyers and TubeSpin® Bioreactors” with some changes:

  • Volume of culture : 30 mL
  • Add Ampicillin at 25 µg/mL to have selection pressure
  • The number of samples:
    • Sample at the beginning
    • Sample at the end of the first day
    • Sample after 24 hours culture and 48 hours culture

Test of gas concentration

The objective of our device is to produce gas, so we would like to know the gas composition of our culture. So, we developed a system in order to recover acids gas.

Materials

  • 4 hours culture in 50 mL Falcon in M9 medium with 15 mM of glucose
  • Silicon plugs adapted to 50 mL Falcon
  • Needles
  • 0.2 µm filters
  • 10 mL Syringes
  • Neoprene pipes Ø=0.8 mm
  • 10 mM NaHCO3
  • 1.5 mL Eppendorf
  • 1 mL Sterile cone
  • Incubator 3 °C without agitation

Methods

  1. Replace Falcon plug with silicon plug
  2. Adjust filter on needle and peg it into silicon plug. Do it twice
  3. Adjust neoprene pipe into each filter
  4. Add 700 µL of NaHCO3 in an Eppendorf
  5. At the end of first pipe put a sterile cone and immerse it into Eppendorf with NaHCO3
  6. At the end of second pipe put a 10 mL syringe
  7. After 24 hours culture, press 10 mL syringe in order to expel gas in NaHCO3 solution
  8. Conserve samples at -20 °C before NMR analysis (see protocol foregoing)

Note 1: We used culture in M9 because with the “Acids production tests” we had data on this medium.
Note 2: 10 mM NaHCO3 solution was used because pH was 8.3 so it would permit acid gas solubilisation.


Photo 8: Gas concentration test with falcons


Protocol for Polymerase Chain Reaction (PCR), From Thermo Scientific™ DreamTaq™ Green PCR Master Mix

Materials

  • MilliQ water nuclease free (QSP)
  • PCR Mix 2X
  • Forward primer
  • Reverse primer
  • Template DNA
  • Thin walled PCR tube
  • Ice

Methods

  1. Gently vortex and briefly centrifuge the PCR mix after thawing
  2. Place a thin-walled PCR tube on ice and add the different components for a 50 μL PCR reaction
  3. Gently vortex the samples
  4. Perform PCR using the recommended thermal cycling conditions

The PCR Mix from Thermo Scientific contains Taq DNA polymerase, Green Buffer, MgCl2, dNTPs but also two tracking dyes and a density reagent that allows for direct loading of the PCR product on a migration gel.
The template DNA concentration has to be adapted in order to be between 10 pg and 1 μg in the final volume of 50 μL. The template DNA can come from a miniprep solution or from a single colony. The primer concentrations have to be between 0.1 μM and 1 μM.
Each PCR reaction has to be adapted to the length of the PCR products, and to the melting temperature Tm of the primers. The extension step lasts 1 min for PCR products up to 2 kb. For longer products, the extension time has to be prolonged by 1 min/kb.

Step Temperature (°C) Time Number of cycles

Initial denaturation

95

1-3 min

1

Denaturation

95

30s

25-40

Annealing

Tm – 5°C

30s

Extension

72

Adapt to the length

Final extension

72

5-15 min

1

Protocols for TPX® permeability tests

Preparation of TPX® bag

Materials

  • TPX®, gas permeable plastic
  • Fusing machine
  • 2 mM Formic acid solution
  • 4 % (V/V) Butyric acid solution

Methods

  1. Prepare plastic bag in sticking on 3 sides over 4 with fusing machine
  2. Add 7 mL of appropriate solution in plastic bag
  3. Stick on the last side with fusing machine

Permeability test

To test gas permeability of TPX® plastic, we use the same protocol as “Test of gas concentration”. The only change is that no filters were used because the sterility is not necessary.

Photo 9: The device used for the permeability test


Sterility test of TPX® bag

    Demonstrate that the TPX® bag is impermeable to bacteria

Materials

  • TPX bags
  • M9 defined Medium
  • E. coli BW 25113
  • Steril laboratory glass bottle

Methods

  1. Overnight culture of E. coli BW 25113 at 37 °C
  2. Inoculate a small TPX® bag at OD600 nm = 0.1 in LB medium (Final Volume = 8 mL)
  3. Negative Control: Fill a small TPX® bag with M9 medium (Final Volume=8 mL)
  4. Dispose each small bag in a Steril glass measuring cylinder containing M9 medium
  5. Incubate at 37 °C
  6. Measure OD600 nm twice a day

Culture test of E. coli in TPX® bag

Materials

  • TPX bags
  • LB Medium
  • Steril clips
  • E. coli BW 25113
  • Steril laboratory flask

Methods

  1. Overnight culture of E. coli BW 25113 at 37 °C
  2. Inoculate a small TPX® bag at OD600 nm = 0.1 in LB medium (Final Volume = 8 mL)
  3. Close the small bag via fusing machine and Put the closed small bag in a Steril laboratory flask
  4. Positive Control: Inoculate a culture tube at OD600 nm = 0.1 in LB medium (Final Volume = 20 mL)
  5. Incubate at 37 °C
  6. Measure OD600 nm twice a day

Transformation Protocol: RbCl method

Media and solution

YETM 500 mL TFB1 200 mL TFB2 200 mL
  • 2.5 g Yeast Extract
  • 10 g Tryptone
  • 5 g MgSO4.7H2O
  • Adjust pH to 7.5 with KOH
  • For Plates: add 7.5 g of Agar
  • 0.59 g KOAc
  • 2.42 g RbCl
  • 0.29 g CaCl2.2H2O
  • 1.98 g MnCl2.4H2O
  • Adjust to pH 5.8 with 0.2 M acetic acid
  • Add dH2O to 200 mL
  • Filter sterilize
  • Store refrigerated at 4°C
  • 0.42 g MOPS
  • 2.21 g CaCl2.2H20
  • 0.24 g RbCl
  • 30 g Glycerol
  • Adjust to pH 6.5 with KOH
  • Add dH2O to 200 mL
  • Filter sterilize
  • Store refrigerated at 4 °C

Preparation of Competent Cells

  • 1. Streak cells from frozen stock onto YETM plate. Incubate overnight at 37°C
  • 2. Pick a single fresh colony to inoculate 5 mL of YETM medium. Grow over night at 37°C.
  • Do not vortex cells at any time after this point in the procedure
  • 3. Dilute 1 mL of culture into 50 mL YETM medium prewarmed to 37 °C
    • Grow at 37 °C for 2 hours with agitation
    • Volumes can be scaled up 5X and all of the 5 mL overnight culture can be used
  • 4. Transfer culture to sterile 50 mL tube. Chill on ice/water 10-15 minutes
  • 5. Centrifuge for 10 minutes at 2,000 rpm at 4 °C. Immediately aspirate off all of the supernatant
  • Do not allow cells to warm above 4 °C at any time in this procedure
  • 6. Resuspend cells in 10 mL of ice-cold TFB1 with gentle re-pipetting. Use chilled glass or plastic pipette
  • 7. Incubate cells on ice for 5 minutes
  • 8. Repeat step 5
  • 9. Resuspend cells in 2 mL of ice-cold TFB2 with gentle re-pipetting. Use micropipet tip (plastic)
  • 10. Incubate cells on ice for 15 minutes
  • Cells may be used for transformation or frozen
    • To freeze: aliquot cell in 200 μL volumes into prechilled 0.5 mL microfuge tube (on ice)
    • Freeze immediately in liquid nitrogen
    • Store cells frozen at -80 °C

Transformation of Competent Cells

  • 1. If starting with frozen competent cells, warm tube/cells by gently twirling between your fingers until just thawed.
    Immediately place on ice for about 5 minutes
  • 2. Add to 1,5 mL eppendorf on ice: 2-3 μL iGEM plate or 1 μL plasmid or 10 μL ligation.
  • 3. Add 100 μL of competent cells and mix by gentle re-pipetting
  • 4. Incubate cells on ice for 20-30 minutes
  • 5. Heat shock the cells exactly 90 seconds at 42 °C
  • 6. Return cells on ice for 2 minutes
  • 7. Add 1 mL of YETM medium. Incubate at 37 °C for 45-60 minutes with slow gentle shaking
  • 8. Plate 0.1-0.2 mL of transformed cells on LB-plate containing the appropriate antibiotic. Incubate overnight at 37°C

Minipreps

  • 1. Resuspend 4 to 12 colonies from the plate and name each colony taken on the tubes and on the plate (A, B, C, …)
  • 2. Resuspend one colony per culture tube in 5 mL of LB medium with antibiotic
  • 3. Let the culture grow overnight at 37 °C in a shaking incubator
  • 4. Use the QIAprep spin Miniprep Kit for each culture tube. The last step consisting in the elution of the DNA is made with elution buffer or water at 55 °C
  • 5. Keep the tubes at -20 °C

Cloning

First step: Digestion

Both parts have the same antibiotic resistance

Vector Insert Digestion control first enzyme Digestion control second enzyme

Volume equivalent to 1 µg of vector miniprep

Volume equivalent to 1 µg of insert miniprep

Volume equivalent to 1 µg of vector miniprep

Volume equivalent to 1 µg of vector miniprep

1 µL of each restriction enzymes

1 µL of each restriction enzymes

1 µL of the first restriction enzyme

1 µL of the second restriction enzyme

2 µL of Fast Digest Green Buffer (Thermo Scientific™)

2 µL of Fast Digest Green Buffer (Thermo Scientific™)

2 µL of Fast Digest Green Buffer (Thermo Scientific™)

2 µL of Fast Digest Green Buffer (Thermo Scientific™)

Up to 20 µL of Milli-Q water

Up to 20 µL of Milli-Q water

Up to 20 µL of Milli-Q water

Up to 20 µL of Milli-Q water

Incubate 15 minutes at 37 °C

The two parts have a different antibiotic resistance

Both parts

Volume equivalent to 1 µg of DNA miniprep

1 µL of each restriction enzymes

2 µL of Fast Digest Green Buffer (Thermo Scientific™)

Up to 20 µL of Milli-Q water

Incubate 15 minutes at 37°C

Migration and gel extraction

  • 1. Prepare a 1 % or 2 % electrophoresis agarose gel with 0.5 X TAE buffer
  • 2. Put 20 µL of sample + 6 µL of marker (1 kb for 1 % gel and 100 pb for 2 %) into the well
  • 3. Migration for 30 min at 100 V or 1 hour at 50 V
  • 4. Bath 10 minutes in BET
  • 5. Wash in water for 5 minutes
  • 6. The gel extraction is realized thanks to the QIAGEN Gel Extraction Kit

  • Two ways to inactivate the enzymes for the vector
    • Use of DNA Clean up kit for the DNA fragment above 200 pb
    • Heat inactivation at 95 °C for 10 minutes

Second step: Ligation

Mix Negative Control Positive Control

Volume equivalent to 3 molecules of insert (for one molecule of vector)

no insert

Volume equivalent to 3 molecules of insert (for one molecule of vector)

Volume equivalent to 50 ng of digested vector

Volume equivalent to 50 ng of digested vector

Volume equivalent to 50 ng of undigested vector

2 µL of 10X T4 buffer

2 µL of 10X T4 buffer

2 µL of 10X T4 buffer

0.5 µL of T4 ligase

0.5 µL of T4 ligase

0.5 µL of T4 ligase

Up to 20 µL of Milli-Q water

Up to 20 µL of Milli-Q water

Up to 20 µL of Milli-Q water

 Incubate the ligation mix 15 minutes at room temperature (22°C)

 Keep the tubes in ice or at -20 °C to prepare the transformation

Third step: Transformation

  • 1a. Take 10 µL of the ligation mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol
  • 1b. Positive control: take 10 µL of the ligation mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol
  • 1c. First restriction enzyme digestion control: take 10 µL of the corresponding digestion mix (First step) for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol
  • 1d. Second restriction enzyme digestion control: take 10 µL of the corresponding digestion mix (First step) for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol
  • 1e. Negative control: take 10 µL of the corresponding mix for 100 µL of competent cells and use the Toulouse iGEM Team 2015 transformation protocol
  • 2. Plate the solution on selective medium overnight at 37 °C


InFusion cloning protocol



Principle of In Fusion cloning

  • 1. Design the tailed-oligonucleotides for the vector and the inserts. The tail of the 5’oligonucleotide must be the 20 last nucleotides of the previous fragment and the tail of the 3’oligonucleotide must be the 20 first nucleotides of the next fragment.
  • 2. Amplify the different fragments with the previously designed oligonucleotides
  • 3. Clean the PCR products either using a spin column purification kit or by digesting with DpnI. For NEB DpnI, mix the different PCR products together, add 10X CutSmart Buffer and DpnI (1 µL in a 20 µL mix); incubate at 37°C for 20 minutes and inactive at 80 °C during 30 minutes.
  • 4. Set up the In Fusion cloning reaction :

    • Ligation Control
    5X In-Fusion HD Enzyme Premix 2 µL -
    Clean PCR mix 4 µL 4 µL
    MilliQ water nuclease free 4 µL 6 µL
    Total 10 µL 10 µL

  • 5. Incubate at 50 °C during 15 min and then cool on ice
  • 6. Transform commercial ultra-competent cells (108 to 109 cfu/µg DNA) with 2.5 µL of the ligation using provided with the competent cells. Plate several 10-fold dilutions of the transformation mix.