Difference between revisions of "Team:Bordeaux/Description"
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<p align="justify" style="text-indent: 3vw;"> Curdlan belongs to the class of biological response modifiers that enhance or restore normal immune defenses including antitumor, anti-infective, anti-inflammatory, and anticoagulant activities. (REF) As a matter of fact, this β1,3 glucan can stimulate the plant's immune system. More precisely, applied to grapevine plants, <b> sulfated Curdlan </b> induces the <b> accumulation of phytoalexins </b> (organic antimicrobial substances) and the <b> expression of a set of Pathogenesis-Related proteins </b>. </p> | <p align="justify" style="text-indent: 3vw;"> Curdlan belongs to the class of biological response modifiers that enhance or restore normal immune defenses including antitumor, anti-infective, anti-inflammatory, and anticoagulant activities. (REF) As a matter of fact, this β1,3 glucan can stimulate the plant's immune system. More precisely, applied to grapevine plants, <b> sulfated Curdlan </b> induces the <b> accumulation of phytoalexins </b> (organic antimicrobial substances) and the <b> expression of a set of Pathogenesis-Related proteins </b>. </p> | ||
− | <p align="justify"> However, non-sulfated Curdlan doesn't trigger the hypersensitive response characterized by the rapid death of cells in the local region surrounding an infection, avoiding a complete contamination of the plant. This response has been studied in Arabidopsis thaliana through a <b> mutant gene: pmr4 </b>. This mutant is resistant to mildew infections but is <b> unable to induce Pathogenesis-Related proteins expression </b>. | + | <p align="justify"style="text-indent: 3vw;"> However, non-sulfated Curdlan doesn't trigger the hypersensitive response characterized by the rapid death of cells in the local region surrounding an infection, avoiding a complete contamination of the plant. This response has been studied in Arabidopsis thaliana through a <b> mutant gene: pmr4 </b>. This mutant is resistant to mildew infections but is <b> unable to induce Pathogenesis-Related proteins expression </b>. Also, activation of a Pathogenesis-Related protein called PR1 in grapevine is regulated by the <b> salicylic acid signaling pathway </b> . |
− | + | <p align="justify" style="text-indent: 3vw;"> The lack of PR1 expression in non-sulfated Curdlan-treated grapevine could be explained by a negative feedback of glucan. This is demonstrated by the study of a double mutant of pmr4 which restore the susceptibility to mildew. It suggests that linear β-1,3 glucan negatively regulates the salicylic acid pathway. So, sulfation of the glucan would counteract the negative feedback effect. </p> | |
− | The lack of PR1 expression in non-sulfated Curdlan-treated grapevine could be explained by a negative feedback of glucan. This is demonstrated by the study of a double mutant of pmr4 which restore the susceptibility to mildew. It suggests that linear β-1,3 glucan negatively regulates the salicylic acid pathway. | + | |
− | So, sulfation of the glucan would counteract the negative feedback effect. </p> | + | |
<p align="justify"> To conclude, activation of the innate immune system before the invasion of pathogens is a way to improve the resistance of plant against infection and to reduce the use of chemicals products. </p> | <p align="justify"> To conclude, activation of the innate immune system before the invasion of pathogens is a way to improve the resistance of plant against infection and to reduce the use of chemicals products. </p> | ||
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− | <p align="justify" style="text-indent: 3vw;"> In <i> Agrobacterium </i>, three genes (crdA, crdS and crdC) are required for Curdlan production. | + | <p align="justify" style="text-indent: 3vw;"> In <i> Agrobacterium </i>, three genes (crdA, crdS and crdC) are required for Curdlan production. The putative operon crdASC contains crdS, encoding β-(1,3)-glucan synthase catalytic subunit, flanked by two additional genes : crdA and crdC. The first assists translocation of the nascent polymer across the cytoplasmic membrane and the second assists the passage of the nascent polymer across the periplasm. However, all Curdlan biosynthesis is dependent of nitrogen starvation and various parameters. We want to simplify all of this. Finally we would like to sulfate our Curdlan molecules chemically in order to enhance it's effects on the activation of the plant's imune system. It has been shown that sulfated curdlan is much more effective. <b>(ref)</b> To sum it up, we would like to produce Curdlan in <i> Escherichia coli </i> or <i> Saccharomyces cerevisiae </i> and then sulfate it to use it as a preventive treatment for the vine against the mildew infection and continue to produce good wine and make everyone happy. </p> |
− | The putative operon crdASC contains crdS, encoding β-(1,3)-glucan synthase catalytic subunit, flanked by two additional genes : crdA and crdC. The first assists translocation of the nascent polymer across the cytoplasmic membrane and the second assists the passage of the nascent polymer across the periplasm. However, all Curdlan biosynthesis is dependent of nitrogen starvation and various parameters. We want to simplify all of this. Finally we would like to sulfate our Curdlan molecules chemically in order to enhance it's effects on the activation of the plant's imune system. It has been shown that sulfated curdlan is much more effective. <b>(ref)</b> To sum it up, we would like to produce Curdlan in <i> Escherichia coli </i> or <i> Saccharomyces cerevisiae </i> and then sulfate it to use it as a preventive treatment for the vine against the mildew infection and continue to produce good wine and make everyone happy. </p> | + | |
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<p align="justify" style="text-indent: 3vw;"> Since <i> E. coli </i> naturally produces UDP Glucose, adding the beta 1,3 glucan synthase would allow curdlan production. We therefore inserted the three genes which code for the glucan synthase in <i> Agrobacterium </i> (crdASC) into <i> E. coli </i> placing the gene under an easier control than N-starvation by using a constitutive promoter. </p> | <p align="justify" style="text-indent: 3vw;"> Since <i> E. coli </i> naturally produces UDP Glucose, adding the beta 1,3 glucan synthase would allow curdlan production. We therefore inserted the three genes which code for the glucan synthase in <i> Agrobacterium </i> (crdASC) into <i> E. coli </i> placing the gene under an easier control than N-starvation by using a constitutive promoter. </p> | ||
− | <img style= "width: | + | <img style= "width:20vw; height:15vw;" src="https://static.igem.org/mediawiki/2015/1/18/Bordeaux_cell_fluo.jpg";> |
<p class="reference" align ="justify"> <b> Figure 6: strains of agrobacterium producing curdlan (green) observed with a microscope using flurescence (???) SOURCE: Goemar</b> </p> | <p class="reference" align ="justify"> <b> Figure 6: strains of agrobacterium producing curdlan (green) observed with a microscope using flurescence (???) SOURCE: Goemar</b> </p> | ||
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<img style= "width:35vw; height:20vw;" src="https://static.igem.org/mediawiki/2015/2/2e/Bordeaux_Tableau_curdlan.png" > | <img style= "width:35vw; height:20vw;" src="https://static.igem.org/mediawiki/2015/2/2e/Bordeaux_Tableau_curdlan.png" > | ||
− | <b> Figure | + | <b> Figure 7: Curdlan properties and applications </b> <a href ="http://link.springer.com/chapter/10.1007%2F978-1-4615-2486-1_14#page-1"> www.link.springer.com</a> |
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Revision as of 14:59, 15 August 2015