Difference between revisions of "Team:EPF Lausanne/Notebook/Protocols"

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             <div class="col-sm-9">
 
             <div class="col-sm-9">
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    <!-- AGAROSE GEL -->
 
               <div id="agarosegel" class="well">     
 
               <div id="agarosegel" class="well">     
 
                 <h1>Agarose Gel</h1>
 
                 <h1>Agarose Gel</h1>
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<p> • Take a picture of the gel at the UV detector</p>
 
<p> • Take a picture of the gel at the UV detector</p>
 
               </div>
 
               </div>
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 +
    <!-- AMINO ACID SOLUTION -->
 
               <div id="aminoacidsolution" class="well">  
 
               <div id="aminoacidsolution" class="well">  
 
                 <h1>Amino acid solution</h1>
 
                 <h1>Amino acid solution</h1>
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<h2>Procedure</h2>
 
<h2>Procedure</h2>
 
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<table style=”width:100%”>
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<thread>
 
<tr>
 
<tr>
 
<th>Stock concentration</th>
 
<th>Stock concentration</th>
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<th>Total quantity for 50 mL</th>
 
<th>Total quantity for 50 mL</th>
 
</tr>
 
</tr>
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<tr>
 
<tr>
 
<th>100 mM Histidine-Hcl (209 g/mol)</th>
 
<th>100 mM Histidine-Hcl (209 g/mol)</th>
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<th> 0.1632 g</th>
 
<th> 0.1632 g</th>
 
</tr>
 
</tr>
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</tbody>
 
</table>
 
</table>
 
<p> • Filter and sterilize solutions</p>
 
<p> • Filter and sterilize solutions</p>
 
<p> •Add 8 mL per liter of selective medium or spread 500  μL on a selective plate</p>
 
<p> •Add 8 mL per liter of selective medium or spread 500  μL on a selective plate</p>
 
               </div>         
 
               </div>         
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    <!-- SECTION 3 -->
 
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               <div id="section3" class="well">         
 
                 <h1>Section 3</h1>
 
                 <h1>Section 3</h1>
 
                 <p>Try to scroll this section and look at the navigation list while scrolling!</p>
 
                 <p>Try to scroll this section and look at the navigation list while scrolling!</p>
 
               </div>
 
               </div>
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    <!-- SECTION 4 -->
 
               <div id="section41" class="well">         
 
               <div id="section41" class="well">         
 
                 <h1>Section 4-1</h1>
 
                 <h1>Section 4-1</h1>

Revision as of 13:21, 21 July 2015

Protocols

Agarose Gel

Materials

• 1X TAE

• Agarose

• Gel Red

• DNA samples

• 6X loading dye

• Nuclease free water

Procedure

Prepare 1.2% agarose gel for small fragments and 3% agarose gel for large fragments

• Mix 50 mL 1X TAE and 0.6 g (1.2%) or 1.5 g (3%) agarose

• Melt in microwave until agarose has melted (about 50 seconds)

• Add 1.3 μL (1.2%) or 1.5 μL (3%) Gel Red

• Pour solution into agarose gel mold with comb

• Let set for 20 minutes or until solid

• Place gel in 1X TAE and remove comb

• Load samples of 200 ng (or 2 μL) DNA mixed with 2 μL 6X loading dye and nuclease free water up to 12 μL

• Run gel at 100-120 Volts for 40-50 minutes (1.2%) or 80 Volts for 2 hours (3%)

• Take a picture of the gel at the UV detector

Amino acid solution

Materials

• Histidine-Hcl

• Uracil

• Leucine

• Tryptophan

Procedure

Stock concentration Final concentration Total quantity for 50 mL
100 mM Histidine-Hcl (209 g/mol) 20.9 g/L 0.418 g
20 mM Uracil (112 g/mol) 2.24 g/L 0.0448 g
100 mM Leucine (131 g/mol) 13.1 g/L 0.262 g
40 mM Tryptophan (204 g/mol) 8.16 g/L 0.1632 g

• Filter and sterilize solutions

•Add 8 mL per liter of selective medium or spread 500 μL on a selective plate

Section 3

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Section 4-1

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Section 4-2

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Still under construction