Difference between revisions of "Team:Pasteur Paris/Microbiology week6"

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<p><h3><B>July 11, 2016: </B></h3></p>
 
<p><h3><B>July 11, 2016: </B></h3></p>
 
     <p>
 
     <p>
         <a href="#exp1"><h4> 74.Culture of BL21DE3 </h4></a></br>  
+
         <a href="#exp1"><h4> 74. Culture of BL21DE3 </h4></a></br>  
 
         <a href="#exp2"><h4> 75. Dephosphorylation of pET43.1a(+)</h4></a></br>
 
         <a href="#exp2"><h4> 75. Dephosphorylation of pET43.1a(+)</h4></a></br>
 
         <a href="#exp3"><h4> 76. Digestion of the new inserts</h4></a></br>  
 
         <a href="#exp3"><h4> 76. Digestion of the new inserts</h4></a></br>  
 
         <a href="#exp4"><h4> 77. Electrophoresis on agarose gel</h4></a></br>  
 
         <a href="#exp4"><h4> 77. Electrophoresis on agarose gel</h4></a></br>  
 
         <a href="#exp5"><h4> 78. Ligation of the inserts</h4></a></br>  
 
         <a href="#exp5"><h4> 78. Ligation of the inserts</h4></a></br>  
        <a href="#exp6"><h4> 79. Transformation of competent cells</h4></a></br>  
+
        <a href="#exp6"><h4> 79. Transformation of competent cells</h4></a></br>  
 
     </p>
 
     </p>
 
<p><h3><B>July 12, 2016:  </B></h3></p>
 
<p><h3><B>July 12, 2016:  </B></h3></p>
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                 <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>
                 • Erlenmeyer flasks 250 ml capacity, IPTG (Iso-propyl Beta thio galactopyranoside) 0.5 M, LB media, carbenicillin at 50 mg/ml, shaking incubator (Infors HT), spectrophotometer.</br></br>
+
                 • Erlenmeyer flasks 250 ml capacity, IPTG (Iso-propyl &beta; thio galactopyranoside) 0.5 M, LB media, carbenicillin at 50 mg/ml, shaking incubator (Infors HT), spectrophotometer.</br></br>
  
 
               <U>Method:</U></br>
 
               <U>Method:</U></br>

Revision as of 17:19, 17 October 2016