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>Add 0.5 grams of agarose to 50 mL of 1X TAE buffer.</li>
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<li>Add 0.5 grams of agarose to 50 mL of 1X TAE buffer. (1% agarose gel)</li>
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<li>Microwave agarose/TAE until agarose completely dissolved.</li>
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<li>Microwave agarose/TAE until agarose is completely dissolved. (Caution: Will be hot)</li>
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<li>Cool under water, add SYBR safe dye (2.5-3µL).</li>
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<li>Cool under water or let sit until cool.</li>
 +
<li>Add SYBR safe dye (2.5-3µL).</li>
<li>Pour into mold with appropriate comb.</li>
<li>Pour into mold with appropriate comb.</li>
<li>Wait 15 minutes for gel to solidify.</li>
<li>Wait 15 minutes for gel to solidify.</li>
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<li>Load DNA with dye into wells while submerged in 1X TAE.</li>
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<li>Transfer gel to a gel electrophoresis box.</li>
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<li>Load DNA and appropriate DNA standard or ladder with dye into wells while submerged<br /> in 1X TAE buffer.</li>
<li>Run gel at a constant 120V.</li>
<li>Run gel at a constant 120V.</li>
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<li>Check gel periodically.</li>
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<li>Check gel periodically until the dye has run the desired length of the gel.</li>
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<li>View gel under short wavelength or UV light, with proper protection, to check for bands.</li>
</ol>
</ol>
</td>
</td>

Revision as of 23:50, 18 October 2013

Protocols