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Team:Evry/Protocols/15
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| - | <p> | + | <p>After <a href='https://2013.igem.org/Team:Evry/Protocols/07' target='_blank'>PCR</a>, electrophoresis is a method using electrical field to separate DNA or RNA sequences by size. Smaller the fragment is, the more it migrates on the gel. <br> |
Using a DNA ladder, we can know the size of DNA sequence and then check if we have the sequence we wanted. | Using a DNA ladder, we can know the size of DNA sequence and then check if we have the sequence we wanted. | ||
</p> | </p> | ||
<h2> Preparation</h2> | <h2> Preparation</h2> | ||
| + | <p><b>Agarose gel 1% preparation:</b><br/> | ||
| + | Add 0,5 g of Agarose in 50 mL of TAE 1X </br> | ||
| + | (See protocole for TAE 1X preparation <a href='https://2013.igem.org/Team:Evry/Protocols/04' target='_blank'>there</a>)</br> | ||
| + | Put the solution into microwave until Agarose is disolved.</br> | ||
| + | When until the cool down and add 3 mL of Ethidium Bromide (EtBr).</br> | ||
| + | Put the solution in the cuve and let it cool down. </br></p> | ||
| + | |||
| + | <p><b>Mix gel</p></b> | ||
| + | Put 5 μL of PCR product and 1 μL of loading dye 6X in each well.<p> | ||
| + | Do not forget your positive and negative controles, and the kB ladder.</br> | ||
| + | Put in the electrophoresis cell at 100 V during 40 minutes. </p> | ||
| + | |||
| + | |||
<h2> Analysis</h2> | <h2> Analysis</h2> | ||
Revision as of 10:27, 6 September 2013
Gel electrophoresis analysis
Principle
After PCR, electrophoresis is a method using electrical field to separate DNA or RNA sequences by size. Smaller the fragment is, the more it migrates on the gel.
Using a DNA ladder, we can know the size of DNA sequence and then check if we have the sequence we wanted.
Preparation
Agarose gel 1% preparation:
Add 0,5 g of Agarose in 50 mL of TAE 1X
(See protocole for TAE 1X preparation there)
Put the solution into microwave until Agarose is disolved.
When until the cool down and add 3 mL of Ethidium Bromide (EtBr).
Put the solution in the cuve and let it cool down.
Mix gel
Put 5 μL of PCR product and 1 μL of loading dye 6X in each well.Do not forget your positive and negative controles, and the kB ladder. Put in the electrophoresis cell at 100 V during 40 minutes.
Analysis
Site developped by Gabriel Guillocheau
