Team:Michigan/Notebook/GelProtocol

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== <font color=dodgerblue size=5> Analytical Gel Standard Protocol </font> ==
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== <font color=royalblue size=5> Analytical Gel Standard Protocol </font> ==
1. Mix 5 &mu;L of DNA with 1 &mu;L of loading dye <br>
1. Mix 5 &mu;L of DNA with 1 &mu;L of loading dye <br>
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== <font color=dodgerblue size=5> Gel Extraction Standard Protocol </font> ==
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== <font color=royalblue size=5> Gel Extraction Standard Protocol </font> ==

Latest revision as of 03:20, 30 October 2008


Michigan iGEM website header.jpg

HOME THE TEAM THE PROJECT REGISTRY PARTS NOTEBOOK


Analytical Gel Standard Protocol

1. Mix 5 μL of DNA with 1 μL of loading dye
2. Pour heated liquid gel (with stoppers and combs in place) according to the number of samples you have to run, and the type of gel electrophoresis apparatus you have
3. Allow gel to cool and solidify
4. Remove all stoppers and combs
5. Fill gel box with TAE until it completely covers the gel
6. Load 3-4 μL of dye/DNA mixture
7. Load ladders for comparison
8. Turn on current to ~45 V
9. Once DNA enters gel, turn up current to ~100 V
10. Allow gel to run until dye is ~3/4 of the way across the gel, depending on the size of your DNA


Gel Extraction Standard Protocol

All of our gel extractions are performed using QIAGEN kits and protocols.


QIAGEN's website can be found [http://www1.qiagen.com/ HERE].


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