Team:UC Davis/Protocols

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     <div class="menu_body">
     <div class="menu_body">
<p>Materials</p>
<p>Materials</p>
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<li>10 µL 5x HF Buffer</li>
<li>10 µL 5x HF Buffer</li>
<li>1  uL dNTPs</li>
<li>1  uL dNTPs</li>
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<li>100 ng Template DNA (2 ng/µL)</li>
<li>100 ng Template DNA (2 ng/µL)</li>
<li>0.5 µL DNA Phusion Polymerase</li>
<li>0.5 µL DNA Phusion Polymerase</li>
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<li>Add appropriate amount of ddH<sub>2</sub>O</li>
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<li>Add appropriate amount of ddH<sub>2</sub>O to reach total volume</li>
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50 µL Total
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50 µL Total  
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<li>Run 1% agarose gel for verification. If the gel is good, perform PCR clean up.</li>
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<p><br />
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or for DNA with high G/C content we found a combination of Taq and Pfu gave us better results.
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</p>
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<li>5 µL 10x Buffer</li>
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<li>10 uL Q solution</li>
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<li>2.5 µL Forward Primer</li>
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<li>2.5 µL Reverse Primer</li>
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<li>1.25 µL DNTPs</li>
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<li>100 ng Template DNA (2 ng/µL)</li>
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<li>0.3 µL Taq DNA Polymerase</li>
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<li>0.1 µL Clone Pfu DNA Polymerase</li>
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<li>Add appropriate amount of ddH<sub>2</sub>O to reach total volume</li>
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50 µL Total
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<p><br />
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PCR program
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<ol>
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<li>98º C 30 sec</li>
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<li>98º C 10 sec</li>
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<li>___º C 30 sec  (Temperature depends on Tm of your primers)</li>
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<li>72º C 1 min / kb Repeat Steps 2-4 29x (30x total)</li>
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<li>72º C 5 min</li>
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<li>4º C Hold</li>
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</ol>
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</p>
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<li>Run PCR products on a 1% agarose gel for verification. If the gel is good, perform PCR clean up with your kit of choice.</li>
</div>
</div>
<p class="menu_head">Golden Gate Assembly</p>
<p class="menu_head">Golden Gate Assembly</p>

Revision as of 00:21, 19 October 2013

Protocols