Difference between revisions of "Team:Tianjin/Demonstrate"

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   <p>Then we first transformed BBa_K2407306 into <i>Saccharomyces cerevisiae</i> with <i>Synthetic chromosome Ⅴ</i>. Through the screening of <i>SC-Ura</i>  solid medium and PCR experiments, we obtained the required strains called PVUVC. Second, we integrated the second composite part into this chromosome through homologous recombination, allowing the <i>RFP</i> gene to replace the <i>Ura3</i> gene. The <i>5-FOA</i> solid medium and PCR experiments were used to screen correct colony PVRVC. The conversion of the last fragment refers to the previous method. This process is graphically displayed on the above figure.</p>
 
   <p>Then we first transformed BBa_K2407306 into <i>Saccharomyces cerevisiae</i> with <i>Synthetic chromosome Ⅴ</i>. Through the screening of <i>SC-Ura</i>  solid medium and PCR experiments, we obtained the required strains called PVUVC. Second, we integrated the second composite part into this chromosome through homologous recombination, allowing the <i>RFP</i> gene to replace the <i>Ura3</i> gene. The <i>5-FOA</i> solid medium and PCR experiments were used to screen correct colony PVRVC. The conversion of the last fragment refers to the previous method. This process is graphically displayed on the above figure.</p>
   <p>To achieve mating, another mating type of wild type haploid yeast <i>BY4742</i> was used for modification.</p>
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   <p>To achieve mating, another mating type of wild type haploid yeast <i>BY4742</i> was used for modification. By digestion and ligation, we construct vika gene on pRS416 plasmid which contains a selective marker Ura3, and pRS413 plasmid which contains a selective marker His. Then we introduced those two different plasmids into <I>BY4742</I> respectively.</p>
 
   <h4>Results of Characterization of Mating Switcher</h4>
 
   <h4>Results of Characterization of Mating Switcher</h4>
 
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Revision as of 11:51, 27 October 2017

/* OVERRIDE IGEM SETTINGS */

Demonstrate