Team:UC Davis/Protocols

From 2013.igem.org

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<p>Procedure</p>
<p>Procedure</p>
<ol>
<ol>
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<li>Prepare agarose gel and use 3 combs to make a bigger well.</li>
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<li>Prepare agarose gel (see gel electrophoresis) and use additional or larger combs to make larger wells.</li>
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<li>Once it has run, use hand held UV lamp (in the dark, wearing goggles) to identify bands. </li>
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<li>Once the gel has run, use preferably a blue light lamp, or UV for a very short time (it will degrade your DNA), (in the dark, wearing goggles and skin protection) to identify bands. </li>
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<li>Cut out desired band with stamp pipette tip and transfer to a clean tube.  The stamp pipette tip can be left in the tube to be cleaned out with a smaller pipette tip. </li>
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<li>Cut out the desired bands with a stamp pipette tip or clean razor and transfer to a clean tube.  The stamp pipette tip can be left in the tube to be cleaned out with a smaller pipette tip. </li>
<table class="gray">
<table class="gray">
<tr>
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Revision as of 23:58, 18 October 2013

Protocols