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<li class="nomargin"> <p class="lead">Prepare the PCR mixture for a final volume of 50 µl per reaction and a final primer concentration of 0,8 µM.</p></li> | <li class="nomargin"> <p class="lead">Prepare the PCR mixture for a final volume of 50 µl per reaction and a final primer concentration of 0,8 µM.</p></li> | ||
<li class="nomargin"><p class="lead">Perform the amplification with the following amplification conditions (adjust according to the primers used):</p></li> | <li class="nomargin"><p class="lead">Perform the amplification with the following amplification conditions (adjust according to the primers used):</p></li> | ||
− | <img alt="Image1" src="https://static.igem.org/mediawiki/2018/6/60/T--Madrid-OLM--Experiments--Protocols_--Aptamers--Selex1.jpg | + | <img alt="Image1" src="https://static.igem.org/mediawiki/2018/6/60/T--Madrid-OLM--Experiments--Protocols_--Aptamers--Selex1.jpg" /> |
<li class="nomargin"><p class="lead">Prepare an agarose gel at 3%. Load the samples and perform the electrophoresis at 90V for 50 min.</p></li> | <li class="nomargin"><p class="lead">Prepare an agarose gel at 3%. Load the samples and perform the electrophoresis at 90V for 50 min.</p></li> | ||
<li class="nomargin"><p class="lead">Remove the gel and observe the bands under UV light.</p></li> | <li class="nomargin"><p class="lead">Remove the gel and observe the bands under UV light.</p></li> |
Revision as of 15:15, 10 October 2018
Aptamer's Protocols
Texto de explicacion/ resumen de la pagina.