Difference between revisions of "Team:UPMC-Paris/Experiments"

 
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We use different cycles programs depending on what we wanted. You can see our <a href="https://2016.igem.org/Team:UPMC-Paris/Notebook">Notebook</a> for more informations.</p>
 
We use different cycles programs depending on what we wanted. You can see our <a href="https://2016.igem.org/Team:UPMC-Paris/Notebook">Notebook</a> for more informations.</p>
  
<p><b><u>Colony PCR:</u></b></p>
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<p><b><u>Dephosphorylation of 5' -ends:</u></b>
 
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<br>
<p><b><u>Ligation:</u></b><br>
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Using Alkaline Phosphatase we use the following protocol:<br>
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<p>1) Make a mix of 1 pmol of DNA (about 1 ug of 3kb plasmid), 2 uL of Phosphatase Buffer, 5 units of Phosphatase and water to reach 20 uL</p>
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<p>2) Incubats 30 minutes, 37°C</p>
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<p>Heat inactivation at 80°C for 20 minutes</p>
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<br>
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<p><b><u>Ligation:</u></b>
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<br>
 
Using T4 DNA Ligase we perform this protocol:<br>
 
Using T4 DNA Ligase we perform this protocol:<br>
 
<u>Reaction setup</u></p>
 
<u>Reaction setup</u></p>
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<li> ➟ Incubate at 25 °C for 30 minutes.</li>
 
<li> ➟ Incubate at 25 °C for 30 minutes.</li>
 
<li> ➟ Immediately purify DNA using PCR clean-up column and elute in ~50 µL.</li>
 
<li> ➟ Immediately purify DNA using PCR clean-up column and elute in ~50 µL.</li>
<li> ➟ OR - Immediately dilute (at least 1:10, but enough such that 0.1-10 ng of ligation product will be transformed) in TE or water </li>
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<li> ➟ OR - Immediately dilute (at least 1:10, but enough such that 0.1-10 ng of ligation product will be transformed in TE or water </li>
 
<li> ➟ Transform 0.1-10 ng of ligation product into chemically or electrocompetent cell line that is compatible with vector</li>
 
<li> ➟ Transform 0.1-10 ng of ligation product into chemically or electrocompetent cell line that is compatible with vector</li>
</ol>
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</ol><br>
 
</div>
 
</div>
 
</div>
 
</div>

Latest revision as of 00:06, 20 October 2016