Difference between revisions of "Team:Bordeaux/Results"
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− | <!-- CHOOSING | + | <!-- CHOOSING MATERIAL ------------------------------------------------------------------------------------------- --> |
− | <h5 align="left"> | + | <h5 align="left">crdS, crdA and crdC genes ?</h5> |
<p align=justify>✵ <b>crdS gene</b> codes the Curdlan synthase. | <p align=justify>✵ <b>crdS gene</b> codes the Curdlan synthase. | ||
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<br>N.B : We tried to work on these three genes. However, amplification attempts by PCR were unsuccessful for crdA and crdC genes.So, in a first time, we focused on cloning crdS gene only.</p> | <br>N.B : We tried to work on these three genes. However, amplification attempts by PCR were unsuccessful for crdA and crdC genes.So, in a first time, we focused on cloning crdS gene only.</p> | ||
− | <h5 align="left"> | + | <h5 align="left">OsmY promoter</h5> |
<align="justify">In <i>Agrobacterium sp.ATCC31749</i>, Curdlan production is started after a nitrogen starvation in stationary phase. So we decided to use OsmY promoter (BBa_J45992) characterized by MIT 2006 iGEM team which is active in stationary phase and under high osmotic pressure condition. This promoter imitates Curdlan biosynthesis in E.coli without the nitrogen stress.</align> | <align="justify">In <i>Agrobacterium sp.ATCC31749</i>, Curdlan production is started after a nitrogen starvation in stationary phase. So we decided to use OsmY promoter (BBa_J45992) characterized by MIT 2006 iGEM team which is active in stationary phase and under high osmotic pressure condition. This promoter imitates Curdlan biosynthesis in E.coli without the nitrogen stress.</align> | ||
− | <h5 align="left"> | + | <h5 align="left">M63 and LB medium</h5> |
<align="justify">Curdlan production was carried out in two different media: LB medium and M63 medium. | <align="justify">Curdlan production was carried out in two different media: LB medium and M63 medium. |
Revision as of 14:04, 9 September 2015