Difference between revisions of "Team:Arizona State/Experiments"

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<h2> <ins> Amber Mani </ins> </h2>
 
<h2> <ins> Amber Mani </ins> </h2>
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<h2>Plasmid transformation</h2>
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<h3>Introduction</h3>
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<p>How to insert a plasmid into bacteria to transform it.</p3>
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<h3>Materials</h3>
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<ul>
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<li>Get how ever many 50ul tubes of the cells you need to to transform (in our case it was BL21 e. coli)</li>
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<li>Get the plasmid tubes you need, for insertion into the cells. </li>
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<li> Gather PCR tubes to be used for Plasmid DNA dilution, same number of tubes as cells and plasmids.</li>
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<li>Keep everything on ice during preparation. </li>
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<h3>Procedure</h3>
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<p>Calculate the concentrations and transform the cells</p>
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<ol type="1">
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<li> check ng/ul concentrations of each plasmid DNA - want to add about 60ng of DNA to each of the cell tubes. </li>
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<li>Dilute each DNA sample in PCR tube with water and do the math to know how many ul to add of the new dilution to get appx 60ng of DNA for each of the 50ul cell tubes. </li>
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<li>Add the appropriate amount of the plasmid needed into each cell tube. </li>
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<li> Place cell tubes (with plasmids added) on ice for about 2-5 minutes </li>
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<li>Then place tubes on hot plate (42C) for appx 45 seconds </li>
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<li> Finally place cell tubes back on ice for 5 minutes. Suspend and grow newly transformed cells </li>
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<li>Add SOC (300ul) to each cell tube</li>
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<li>Place in shaking incubator (37C) for 30 minutes </li>
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<li> Spin down tubes, max speed for one minute</li>
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<li>Gently tap out liquid and resuspend cells in 100ul SOC </li>
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<li>Plate all 100ul onto petri plate (in our case, AMP plate) and place in regular incubator overnight</li>
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<li>The next day you have access to the freshly transformed, plated and grown cells</li>
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</ol>
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<h2>DNA Gel Extraction from Agarose Gel</h2>
 
<h2>DNA Gel Extraction from Agarose Gel</h2>
 
<h3>Introduction: </h3>
 
<h3>Introduction: </h3>

Revision as of 00:48, 29 September 2017