Difference between revisions of "Team:Tianjin/Demonstrate"

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<p>After the ligation of<b><i>GHC</i><a href="http://parts.igem.org/Part:BBa_K2407100"> (BBa_K2407100) </a></b> and <i>PRS416</i> Plasmid (<b><i>GHC-416</i></b>), we transformed the E. coli for the augment of our new plasmid——<b><i>GHC-416</i></b>. We examined the transformation result by PCR method to amplify the <i>HO</i> gene in the E. coli which we randomly selected in the plate.   
 
<p>After the ligation of<b><i>GHC</i><a href="http://parts.igem.org/Part:BBa_K2407100"> (BBa_K2407100) </a></b> and <i>PRS416</i> Plasmid (<b><i>GHC-416</i></b>), we transformed the E. coli for the augment of our new plasmid——<b><i>GHC-416</i></b>. We examined the transformation result by PCR method to amplify the <i>HO</i> gene in the E. coli which we randomly selected in the plate.   
 
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   <p>After we got the strain that introduced the <i>red fluorescent protein</i> gene, we let it mate with another mating type haploid yeast, which had plasmid with <i>vika</i> gene. The result is showed as follows:</p>
 
   <p>After we got the strain that introduced the <i>red fluorescent protein</i> gene, we let it mate with another mating type haploid yeast, which had plasmid with <i>vika</i> gene. The result is showed as follows:</p>
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Revision as of 15:10, 30 October 2017

/* OVERRIDE IGEM SETTINGS */

Demonstrate