Difference between revisions of "Team:Exeter/Interlab"

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<p id="pp">The InterLab measurement kit contained 5 devices; (1) J23101+I13504, (2) J23106+I13504, (3) J23117+I13504, Positive and Negative control. The first attempt to transform 5µL of each device into our competent cells found no liquid in the tubes provided. The provided tubes were re-suspended using elution buffer from a Qiagen mini-prep kit.  A transformation of plasmids used in the lab under a strong promoter and GFP was performed mirroring the Interpab protocol to determine if the cells were competent. Spread plates were made and incubated at 37°C.</p>
 
<p id="pp">The InterLab measurement kit contained 5 devices; (1) J23101+I13504, (2) J23106+I13504, (3) J23117+I13504, Positive and Negative control. The first attempt to transform 5µL of each device into our competent cells found no liquid in the tubes provided. The provided tubes were re-suspended using elution buffer from a Qiagen mini-prep kit.  A transformation of plasmids used in the lab under a strong promoter and GFP was performed mirroring the Interpab protocol to determine if the cells were competent. Spread plates were made and incubated at 37°C.</p>
 
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            <span class="caption">Fig.</span>
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<p id="pp">Competent cells containing the previously used strong promoter and GFP coding sequence showed strong expression of GFP. However the competent cells transformed with the iGEM parts showed no growth. A new interlab kit was ordered from iGEM.</p>
 
<p id="pp">Competent cells containing the previously used strong promoter and GFP coding sequence showed strong expression of GFP. However the competent cells transformed with the iGEM parts showed no growth. A new interlab kit was ordered from iGEM.</p>
  

Revision as of 12:47, 19 October 2016