Difference between revisions of "Team:Bordeaux/Description"
Line 145: | Line 145: | ||
<p align="justify" style="text-indent: 3vw;"> To do this , we will extract the FKS1 gene from yeast DNA by amplifying the genomic DNA it by PCR. We will then insert FKS1 in one hand, into plasmid pYES2 with the Gal1 inductif promoter to then integrate the modified plasmid in <i>Saccharomyces cerevisiae </i> and boost the production of curdlan. This strategy did not work. We then tried to put a inductive promoter ahead of the relevant gene by homologous recombination. We put the Gal1 promoter and a selective gene HIS3 ( to select our successful transformants) in front of FKS1. Gal1 promter and HIS3 was extract by PCR from pFA 6a-HIS3MX6-pGAL-3HA . | <p align="justify" style="text-indent: 3vw;"> To do this , we will extract the FKS1 gene from yeast DNA by amplifying the genomic DNA it by PCR. We will then insert FKS1 in one hand, into plasmid pYES2 with the Gal1 inductif promoter to then integrate the modified plasmid in <i>Saccharomyces cerevisiae </i> and boost the production of curdlan. This strategy did not work. We then tried to put a inductive promoter ahead of the relevant gene by homologous recombination. We put the Gal1 promoter and a selective gene HIS3 ( to select our successful transformants) in front of FKS1. Gal1 promter and HIS3 was extract by PCR from pFA 6a-HIS3MX6-pGAL-3HA . | ||
On the other hand, we will integrate the FKS1 gene into the iGEM plasmid pSB1C3 to get our famous BioBrick that we'll send to Boston. This genetic construction with HIST3 gene and GAL promoter was inserted in pSB1C3 by Gibson assembly. However, site-directed mutagenesis may be necessary when integrating the gene into the plasmid because there are restriction sites (EcoR1) that are unwanted within the HIS3 gene. </p> | On the other hand, we will integrate the FKS1 gene into the iGEM plasmid pSB1C3 to get our famous BioBrick that we'll send to Boston. This genetic construction with HIST3 gene and GAL promoter was inserted in pSB1C3 by Gibson assembly. However, site-directed mutagenesis may be necessary when integrating the gene into the plasmid because there are restriction sites (EcoR1) that are unwanted within the HIS3 gene. </p> | ||
− | |||
− | |||
</div> | </div> |
Revision as of 09:35, 16 September 2015