Difference between revisions of "Team:Pasteur Paris/Microbiology week11"

 
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</div>
 
</div>
  
 
+
  <div id="week11">
 +
                  <p><h5><B>Week 11</B></h5></p>
 +
   
 
     <p><h3><B>August 17, 2016:</B></h3></p>
 
     <p><h3><B>August 17, 2016:</B></h3></p>
 
     <p>
 
     <p>
         <a href="#exp1"><h4> Extraction of plasmid DNA </h4></a></br>  
+
         <a href="#exp1"><h4> 188. Miniprep of precultures B1col1/B1col2 and C2col1 </h4></a></br>  
         <a href="#exp2"><h4> Digestion of the plasmid pET43.1a(+) with A1 and D1 </h4></a></br>  
+
         <a href="#exp2"><h4> 189. Digestion of the plasmid pET43.1a(+) with A1/A2/D1/D2 </h4></a></br>  
<a href="#exp3"><h4> Electrophoresis on agarose gel </h4></a></br>  
+
<a href="#exp3"><h4> 190. Electrophoresis on agarose gel of digestion products A1/A2/D1/D2/B1 col1/B1 col2/C2</h4></a></br>  
         <a href="#exp4"><h4> Harvest the culture with Midiprep </h4></a></br>  
+
         <a href="#exp4"><h4> 191. Harvest the culture with Midiprep A1/A2/D1/D2 </h4></a></br>  
 +
 
     </p>
 
     </p>
 
     <p><h3><B>August 18, 2016:</B></h3></p>
 
     <p><h3><B>August 18, 2016:</B></h3></p>
 
     <p>
 
     <p>
         <a href="#exp5"><h4> Extraction of plasmid DNA </h4></a></br>  
+
         <a href="#exp5"><h4> 192. Miniprep of A1/A2/D1/D2</h4></a></br>
        <a href="#exp6"><h4> Purification of the protein </h4></a></br>  
+
                <a href="#exp6"><h4> 193. Purification of the protein </h4></a></br>
         <a href="#exp7"><h4> Protein gel on SDS-Page </h4></a></br>  
+
         <a href="#exp7"><h4> 194. Protein gel on SDS-Page </h4></a></br>
         <a href="#exp8"><h4> Harvest the culture with Miniprep </h4></a></br>  
+
         <a href="#exp8"><h4> 195. Harvest the culture with Miniprep 4 colonies from A1, A2, D1 and D2, 2 colonies of B1 and 1 colony of C2</h4></a></br>
  
 
     </p>
 
     </p>
 
     <p><h3><B>August 19, 2016:</B></h3></p>
 
     <p><h3><B>August 19, 2016:</B></h3></p>
 
     <p>
 
     <p>
         <a href="#exp9"><h4> Extraction of plasmid DNA </h4></a></br>  
+
         <a href="#exp9"><h4> 196. Miniprep of cultures made on the 18/08 </h4></a></br>
         <a href="#exp10"><h4> Measure the amount of DNA extracted from the miniprep </h4></a></br>  
+
         <a href="#exp10"><h4> 197. Measure the amount of DNA extracted from the miniprep of B1 and C2 </h4></a></br>  
         <a href="#exp11"><h4> Digestion of the plasmid pET43.1a(+) with A1/D1/D2 </h4></a></br>  
+
         <a href="#exp11"><h4> 198. Digestion of the plasmid pET43.1a(+) with A1(0)/A1(1)/A1(3)/A1(4)/D1(3)/D1(4)/D2(2) </h4></a></br>  
         <a href="#exp12"><h4> Electrophoresis on agarose gel </h4></a></br>  
+
         <a href="#exp12"><h4> 199. Electrophoresis on agarose gel of digestion products </h4></a></br>
 
+
                <a href="#exp13"><h4> 200. Harvest preculture for miniprep of C2 and B1</h4></a></br>
    </p>
+
     <p><h3><B>August 20, 2016:</B></h3></p>
     <p><B><h3>August 21, 2016:</B></h3></p>
+
               
    <p>
+
                <a href="#exp14"><h4> 201. Miniprep of C2 and B1</h4></a></br>
        <a href="#exp13"><h4> Harvest the culture with Miniprep </h4></a></br>  
+
                <a href="#exp15"><h4> 202. Measure the amount of DNA extracted from the miniprep of B1 and C2</h4></a></br>
 
+
                <a href="#exp16"><h4> 203. Digestion of E1(4 tubes)/E2(12tubes) and B2(14 tubes)</h4></a></br>
    </p>
+
                <a href="#exp17"><h4> 204. Electrophoresis on agarose gel of digestion products </h4></a></br>
    <p> <h3><B>August 22, 2016:</B></h3></p>
+
 
     <p>
 
     <p>
        <a href="#exp14"><h4> Extraction of plasmid DNA </h4></a></br>
 
        <a href="#exp15"><h4> Measure the amount of DNA extracted from the miniprep </h4></a></br>
 
        <a href="#exp16"><h4> Digestion of the plasmid pET43.1a(+) with A1/D1/D2 </h4></a></br>
 
        <a href="#exp17"><h4> Electrophoresis on agarose gel </h4></a></br>
 
        <a href="#exp18"><h4> Harvest the culture with Miniprep gel </h4></a></br>
 
        <a href="#exp19"><h4> Harvest the culture with Miniprep gel </h4></a></br>
 
  
 
     </p>
 
     </p>
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             <figcaption>
 
             <figcaption>
 
               <p>
 
               <p>
               <U> Aim:</U> To perform a Miniprep to isolate plasmid DNA of pET43.1a(+) with the inserts A1 and D1. The amplification method to increase the amount of plasmid is called Miniprep. </br> </br>
+
               <U> Aim:</U> To perform a Miniprep to isolate plasmid DNA of pET43.1a(+) with the inserts B1 col1, B1 col2 and C2 col1. The amplification method to increase the amount of plasmid is called Miniprep. </br> </br>
               <U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a></br></br>
+
               <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a></br></br>
 
               <U>What we did in the lab:</U></br>
 
               <U>What we did in the lab:</U></br>
 
               <U>Materials:</U></br>
 
               <U>Materials:</U></br>
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           <a href="#" class="closemsg"></a>
 
           <a href="#" class="closemsg"></a>
 
               <figcaption>
 
               <figcaption>
                   <p><U> Aim:</U> To get back our insert from the Miniprep with appropriate enzymes. </br>
+
                   <p><U> Aim:</U> To get back our insert from the Miniprep of our inserts with appropriate enzymes. </br>
 
We perform restriction enzyme digestion in order to recover our inserts. We choose appropriate restriction sites based on the host plasmid. </br> </br>  
 
We perform restriction enzyme digestion in order to recover our inserts. We choose appropriate restriction sites based on the host plasmid. </br> </br>  
                   <U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a></br></br>
+
                   <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a></br></br>
 
                   <U>What we did in the lab:</U></br>
 
                   <U>What we did in the lab:</U></br>
 
                   <U>Materials:</U></br>
 
                   <U>Materials:</U></br>
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                       1. Mix all the reagents and let digest during 2 hr at 37°C. </br> Big volumes must be added first!</br>Beginning of digestion 12h10.</br>
 
                       1. Mix all the reagents and let digest during 2 hr at 37°C. </br> Big volumes must be added first!</br>Beginning of digestion 12h10.</br>
 
                   <table>
 
                   <table>
 +
<caption align="bottom" align="center"><i><p> <U>Table 125</U></p></i></caption>
 
                     <thead>
 
                     <thead>
 
                         <tr>
 
                         <tr>
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             <figcaption>
 
             <figcaption>
 
                 <p><U> Aim:</U> This step check the digestion efficiency. Moreover, the inserts will be purified during this step because they will be extracted from the gel.</br> </br>
 
                 <p><U> Aim:</U> This step check the digestion efficiency. Moreover, the inserts will be purified during this step because they will be extracted from the gel.</br> </br>
                     <U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a></br></br>
+
                     <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/6/60/T--Pasteur_Paris--Gel_electrophoresis_protocol.pdf">link</a></br></br>
 
                     <U>What we did in the lab:</U></br>
 
                     <U>What we did in the lab:</U></br>
 
                     <U>Materials:</U></br>
 
                     <U>Materials:</U></br>
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                           &bull; Restriction enzyme buffers </br>
 
                           &bull; Restriction enzyme buffers </br>
 
                           &bull; 37°C water bath</br>
 
                           &bull; 37°C water bath</br>
                           &bull; UV spectrophotometer</br>
+
                           &bull; UV spectrophotometer</br></br>
 
                     <U>Method:</U></br>
 
                     <U>Method:</U></br>
 
                           &bull; Electrophoresis cuve </br>
 
                           &bull; Electrophoresis cuve </br>
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                           &bull; UV table </br>
 
                           &bull; UV table </br>
 
                           &bull; BET </br></br></br>
 
                           &bull; BET </br></br></br>
                     <U>Method:</U></br>Beginning of the electrophoresis at 14h30 at 100V. </br></br></br>
+
                     Beginning of the electrophoresis at 14h30 at 100V. </br></br></br>
 
                     <U>Results:</U></br>The gel reveals that A1 contains the insert but the amount of DNA is too low so we will redo the experiment.</br>
 
                     <U>Results:</U></br>The gel reveals that A1 contains the insert but the amount of DNA is too low so we will redo the experiment.</br>
 
                 </p>
 
                 </p>
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         <p>
 
         <p>
 
             <U> Aim:</U>  To start a culture for Midiprep. </br>In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
 
             <U> Aim:</U>  To start a culture for Midiprep. </br>In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
             <U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a></br></br>
+
             <U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a></br></br>
 
             <U>What we did in the lab:</U></br>
 
             <U>What we did in the lab:</U></br>
 
             <U>Materials:</U></br>
 
             <U>Materials:</U></br>
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       <figcaption>
 
       <figcaption>
 
         <p>
 
         <p>
 +
 
             <U> Aim:</U> To perform a Midiprep to isolate plasmid DNA of pET43.1a(+) with A1/A2/D1/D2 and B1/B2 for sequencing.</br>
 
             <U> Aim:</U> To perform a Midiprep to isolate plasmid DNA of pET43.1a(+) with A1/A2/D1/D2 and B1/B2 for sequencing.</br>
  
  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>:
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a>:
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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</div>
 
</div>
  
<div class="lightbox" id="exp7">
+
 
 +
 
 +
<div class="lightbox" id="exp6">
 
   <figure>
 
   <figure>
 
     <a href="#" class="closemsg"></a>
 
     <a href="#" class="closemsg"></a>
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  </br>
 
  </br>
  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/0/07/T--Pasteur_Paris--FPLC_Protein_purification_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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<p ><U> Aim:</U> Get the size of the protein purified thanks to FPLC in order to know if it is our protein  </br></br>
 
<p ><U> Aim:</U> Get the size of the protein purified thanks to FPLC in order to know if it is our protein  </br></br>
  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
 
</br></br>
 
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
 
</br>
 
</br>
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</div>
 
</div>
 
 
 +
 +
 
<div class="lightbox" id="exp8">
 
<div class="lightbox" id="exp8">
 
   <figure>
 
   <figure>
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In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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   </figure>
 
   </figure>
 
</div>
 
</div>
 +
 +
  
 
<div class="lightbox" id="exp9">
 
<div class="lightbox" id="exp9">
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The amplification method to increase the amount of plasmid is called Miniprep. </br> </br>
 
The amplification method to increase the amount of plasmid is called Miniprep. </br> </br>
  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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   </figure>
 
   </figure>
 
</div>
 
</div>
 +
 +
  
 
<div class="lightbox" id="exp10">
 
<div class="lightbox" id="exp10">
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<p><U> Aim:</U> Measure the quantity of plasmid using a Nanodrop (Thermofisher) before sending for sequencing (inserts B1 and C2)</br></br>
 
<p><U> Aim:</U> Measure the quantity of plasmid using a Nanodrop (Thermofisher) before sending for sequencing (inserts B1 and C2)</br></br>
  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
 
</br></br>
 
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
 
</br>
 
</br>
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<U>Results:</U></br>
 
<U>Results:</U></br>
 
<table>
 
<table>
 +
<caption align="bottom" align="center"><i><p> <U>Table 126</U></p></i></caption>
 
   <thead>
 
   <thead>
 
     <tr>
 
     <tr>
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<p><U> Aim:</U> To get back our insert from the miniprep with appropriate enzymes.</br>
 
<p><U> Aim:</U> To get back our insert from the miniprep with appropriate enzymes.</br>
 
We perform restriction enzyme digestion in order to recover our inserts. We choose appropriate restriction sites based on the host plasmid.</br> </br>
 
We perform restriction enzyme digestion in order to recover our inserts. We choose appropriate restriction sites based on the host plasmid.</br> </br>
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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<table>
 
<table>
 +
<caption align="bottom" align="center"><i><p> <U>Table 127</U></p></i></caption>
 
   <thead>
 
   <thead>
 
     <tr>
 
     <tr>
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<p><U> Aim:</U> This step check the digestion efficiency of A1 (4 tubes)/D1 (2 tubes)/ D2 (1 tube). Moreover, the inserts will be purified during this step because they will be extracted from the gel.</br>
 
<p><U> Aim:</U> This step check the digestion efficiency of A1 (4 tubes)/D1 (2 tubes)/ D2 (1 tube). Moreover, the inserts will be purified during this step because they will be extracted from the gel.</br>
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/6/60/T--Pasteur_Paris--Gel_electrophoresis_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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<U>Method:</U></br>  
 
<U>Method:</U></br>  
Each well will contain 30 &microL of DNA and 6 &microL of Loading Dye. </br>  
+
Each well will contain 30 &#181;L of DNA and 6 &#181;L of Loading Dye. </br>  
 
Follow the next deposit table :</br>  
 
Follow the next deposit table :</br>  
Ladder (6 &microL) / A1 (1) / A1 (2) / A1 (3) / A1 (4) / D1 (1) / D1 (2) / D2 (2)</br>  
+
Loading dye (6 &#181;L ) / A1 (1) / A1 (2) / A1 (3) / A1 (4) / D1 (1) / D1 (2) / D2 (2)</br>  
 
Beginning of the electrophoresis at 14h20 at 100 V.</br> </br>  
 
Beginning of the electrophoresis at 14h20 at 100 V.</br> </br>  
  
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<p><U> Aim:</U> To start a culture for Midiprep of insert C2 and B1. </br>  
 
<p><U> Aim:</U> To start a culture for Midiprep of insert C2 and B1. </br>  
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight.</br>  
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight.</br>  
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
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<p><U> Aim:</U> To perform a midiprep to isolate plasmid DNA pET43.1a(+) with the inserts C2 and B1.</br>
 
<p><U> Aim:</U> To perform a midiprep to isolate plasmid DNA pET43.1a(+) with the inserts C2 and B1.</br>
 
The amplification method to increase the amount of plasmid is called Mini or Midiprep.</br>
 
The amplification method to increase the amount of plasmid is called Mini or Midiprep.</br>
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/d/d5/T--Pasteur_Paris--Miniprep_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
Line 868: Line 872:
  
 
<p><U> Aim:</U>  Measure the quantity of plasmid using a Nanodrop (Thermofisher) before sending for sequencing (inserts B1 and C2)</br></br>
 
<p><U> Aim:</U>  Measure the quantity of plasmid using a Nanodrop (Thermofisher) before sending for sequencing (inserts B1 and C2)</br></br>
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
 
</br></br>
 
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
 
</br>
 
</br>
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<U>Results:</U></br>
 
<U>Results:</U></br>
 
<table>
 
<table>
 +
<caption align="bottom" align="center"><i><p> <U>Table 128</U></p></i></caption>
 
   <thead>
 
   <thead>
 
     <tr>
 
     <tr>
Line 942: Line 945:
 
<p><U> Aim:</U>To get back our insert from the miniprep with appropriate enzymes.</br>
 
<p><U> Aim:</U>To get back our insert from the miniprep with appropriate enzymes.</br>
 
We perform restriction enzyme digestion in order to recover our inserts. We choose appropriate restriction sites based on the host plasmid.</br></br>
 
We perform restriction enzyme digestion in order to recover our inserts. We choose appropriate restriction sites based on the host plasmid.</br></br>
<U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/a/ab/T--Pasteur_Paris--Restriction_digestion_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
Line 960: Line 963:
  
 
<table>
 
<table>
 +
<caption align="bottom" align="center"><i><p> <U>Table 129</U></p></i></caption>
 
   <thead>
 
   <thead>
 
     <tr>
 
     <tr>
Line 970: Line 974:
 
     <tr>
 
     <tr>
 
       <td><strong><p>Vol<sub>DNA</sub></p></strong></td>
 
       <td><strong><p>Vol<sub>DNA</sub></p></strong></td>
       <td>45 &#181;L </td>
+
       <td>45 &#181;l </td>
       <td>0 &#181;L </td>
+
       <td>0 &#181;l </td>
 
     </tr>
 
     </tr>
 
     <tr>
 
     <tr>
 
       <td><strong><p>Vol<sub>XbaI</sub></p></strong></td>
 
       <td><strong><p>Vol<sub>XbaI</sub></p></strong></td>
       <td>2.25 &#181;L </td>
+
       <td>2.25 &#181;l </td>
       <td>65.25 &#181;L </td>
+
       <td>65.25 &#181;l </td>
 
     </tr>
 
     </tr>
 
     <tr>
 
     <tr>
 
       <td><strong><p>Vol<sub>HindIII</sub></p></strong></td>
 
       <td><strong><p>Vol<sub>HindIII</sub></p></strong></td>
       <td>2.25 &#181;L </td>
+
       <td>2.25 &#181;l </td>
       <td>65.25 &#181;L </td>
+
       <td>65.25 &#181;l </td>
 
     </tr>
 
     </tr>
 
     <tr>
 
     <tr>
 
       <td><strong><p>Vol<sub>H<span>2</span>O</sub></p></strong></td>
 
       <td><strong><p>Vol<sub>H<span>2</span>O</sub></p></strong></td>
       <td>1.125 &#181;L</td>
+
       <td>1.125 &#181;l</td>
       <td>32.65 &#181;L</td>
+
       <td>32.65 &#181;l</td>
 
     </tr>
 
     </tr>
 
     <tr>
 
     <tr>
 
       <td><strong><p>Vol<sub>Buffer Cutsmart (10X)</sub></p></strong></td>
 
       <td><strong><p>Vol<sub>Buffer Cutsmart (10X)</sub></p></strong></td>
       <td>5.63 &#181;L </td>
+
       <td>5.63 &#181;l </td>
       <td>163.12 &#181;L </td>
+
       <td>163.12 &#181;l </td>
 
     </tr>
 
     </tr>
 
     <tr>
 
     <tr>
 
       <td><strong><p>Vol<sub>total</sub></p></strong></td>
 
       <td><strong><p>Vol<sub>total</sub></p></strong></td>
       <td>56 /&#181;L </td>
+
       <td>56 /&#181;l </td>
       <td>326.27 /&#181;L </td>
+
       <td>326.27 /&#181;l </td>
 
   </tbody>
 
   </tbody>
 
</table>
 
</table>
Line 1,016: Line 1,020:
 
     <figcaption>
 
     <figcaption>
  
<p><U> Aim:</U>This step check the digestion efficiency of E1(3 tubes) / E2 (12 tubes) / B2(14 tubes). Moreover, the inserts will be purified during this step because they will be extracted from the gel. </br> </br><U> Protocol:</U> follow in this <a href="https://2016.igem.org/Team:Pasteur_Paris/Science">link</a>
+
<p><U> Aim:</U>This step check the digestion efficiency of E1(3 tubes) / E2 (12 tubes) / B2(14 tubes). Moreover, the inserts will be purified during this step because they will be extracted from the gel. </br> </br>
 +
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/6/60/T--Pasteur_Paris--Gel_electrophoresis_protocol.pdf">link</a>
 
</br></br>
 
</br></br>
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
Line 1,029: Line 1,034:
 
&bull; Agarose </br>
 
&bull; Agarose </br>
 
&bull; UV table </br>
 
&bull; UV table </br>
&bull; BET </br>
+
&bull; BET </br></br>
  
  
Method: Each well can contain 40 &#181;l so we made two big gels with 20x2 lines on each. </br> Each sample will contain 62 &#181;l as we add 7 &#181;l of loading dye. They will be divided into two wells. </br>
+
<U>Method:</U></br> Each well can contain 40 &#181;l so we made two big gels with 20x2 lines on each. </br> Each sample will contain 62 &#181;l as we add 7 &#181;l of loading dye. They will be divided into two wells. </br>
 
Deposit table (/// means EMPTY to make the cut easier) </br>
 
Deposit table (/// means EMPTY to make the cut easier) </br>
  
 
Gel 1 Line 1 : </br>
 
Gel 1 Line 1 : </br>
Ladder /// B2(2) / B2(2) /// B2(3) / B2(3) /// B2(4) / B2(4) /// B2(5) / B2(5) /// B2(1) / B2(1) /// B2(6) / B2(6) </br> </br>
+
Loading dye /// B2(2) / B2(2) /// B2(3) / B2(3) /// B2(4) / B2(4) /// B2(5) / B2(5) /// B2(1) / B2(1) /// B2(6) / B2(6) </br> </br>
  
 
Gel 1 Line 2 : </br>
 
Gel 1 Line 2 : </br>
Ladder /// B2(7) / B2(7) /// B2(8) / B2(8) /// B2(9) / B2(9) /// B2(10) / B2(10) /// B2(11) / B2(11) /// B2(12) / B2(12) </br> </br>
+
Loading dye /// B2(7) / B2(7) /// B2(8) / B2(8) /// B2(9) / B2(9) /// B2(10) / B2(10) /// B2(11) / B2(11) /// B2(12) / B2(12) </br> </br>
  
  
 
Gel 2 Line 1 : </br>
 
Gel 2 Line 1 : </br>
Ladder /// E1(1) / E1(1) /// E1(2) / E1(2) /// E1(3) / E1(3) /// E2(1) / E2(1) /// E2(2) / E2(2) /// E2(3) / E2(3) /// E2(4) / E2(4) /// E2(5) / E2(5) /// E2(6) / E2(6) /// E2(7) / E2(7) </br> </br>
+
Loading dye /// E1(1) / E1(1) /// E1(2) / E1(2) /// E1(3) / E1(3) /// E2(1) / E2(1) /// E2(2) / E2(2) /// E2(3) / E2(3) /// E2(4) / E2(4) /// E2(5) / E2(5) /// E2(6) / E2(6) /// E2(7) / E2(7) </br> </br>
  
 
Gel 2 Line 2 : </br>
 
Gel 2 Line 2 : </br>
Ladder /// E2(8) / E2(8) /// E2(9) / E2(9) /// E2(10) / E2(10) /// E2(11) / E2(11) /// E2(12) / E2(12) /// E2(13) / E2(13) /// B2(13) / B2(13) /// B2(14) / B2(14) /// </br> </br>
+
Loading dye /// E2(8) / E2(8) /// E2(9) / E2(9) /// E2(10) / E2(10) /// E2(11) / E2(11) /// E2(12) / E2(12) /// E2(13) / E2(13) /// B2(13) / B2(13) /// B2(14) / B2(14) /// </br> </br>
 
</p>
 
</p>
 
</figcaption>
 
</figcaption>
Line 1,061: Line 1,066:
 
<p><U> Aim:</U>To start a culture for Miniprep of insert A1, A2, D1 and D2. </br>
 
<p><U> Aim:</U>To start a culture for Miniprep of insert A1, A2, D1 and D2. </br>
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
 
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a><br/><br/>
</br></br>
+
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
 
</br>
 
</br>
Line 1,088: Line 1,092:
 
     <figcaption>
 
     <figcaption>
  
<p><U> Aim:</U>To start a culture for Miniprep of insert A1, A2, D1 and D2. </br>
+
<p><U> Aim:</U></br>To start a culture for Miniprep of insert A1, A2, D1 and D2. </br>
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
 
In order to obtain a large amount of plasmid, we need to grow the bacteria overnight. </br> </br>
 
+
<U> Protocol:</U> follow in this <a href="https://static.igem.org/mediawiki/2016/4/4b/T--Pasteur_Paris--Bacterial_culture_protocol.pdf">link</a><br/><br/>
</br></br>
+
 
<U>What we did in the lab:</U>
 
<U>What we did in the lab:</U>
 
</br>
 
</br>
Line 1,110: Line 1,113:
 
   </figure>
 
   </figure>
 
</div>
 
</div>
</div>
+
 
</div>
+
  
 
</body>
 
</body>
  
 
</html>
 
</html>

Latest revision as of 01:27, 20 October 2016