Team:Lyon-INSA-ENS/Project/Ethics

From 2011.igem.org

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<p style="line-height:1.5em; margin-right : 5%">
<p style="line-height:1.5em; margin-right : 5%">
In <i>E. coli</i> the curli-producing system is organized in two divergeant operons with the genes
In <i>E. coli</i> the curli-producing system is organized in two divergeant operons with the genes
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csgA, csgB and csgC on one side and csgD, csgE, csgF and csgG of the other one. So to
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<i>csgA</i>, <i>csgB</i> and <i>csgC</i> on one side and <i>csgD</i>, <i>csgE</i>, <i>csgF</i> and <i>csgG</i> of the other one. So to
achieve the first approach of the project, it is necessary to begin by the creation of three "sub-
achieve the first approach of the project, it is necessary to begin by the creation of three "sub-
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parts": the first one would be the part with the sole promoter PrcnA, the second would be the
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parts": the first one would be the part with the sole promoter P<i>rcnA</i>, the second would be the
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part with the genes csgA and csgB and final one would be the part with the genes csgE, csgF
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part with the genes <i>csgA</i> and <i>csgB</i> and final one would be the part with the genes <i>csgE</i>, <i>csgF</i>
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and csgG.
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and <i>csgG</i>.
  <br/> <br/>
  <br/> <br/>
</p>
</p>
<p style="line-height:1.5em; margin-right : 5%">
<p style="line-height:1.5em; margin-right : 5%">
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The synthesis of this first DNA part (the cobalt-inducible promoter Prcn-csgBAEFG, which is
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The synthesis of this first DNA part (the cobalt-inducible promoter P<i>rcn-csgBAEFG</i>, which is
designed to induce formation of a biofilm and to promote cell adhesion) was conceived as as a
designed to induce formation of a biofilm and to promote cell adhesion) was conceived as as a
competition between two methods: a completely synthetic approach, and a "manual" method
competition between two methods: a completely synthetic approach, and a "manual" method
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<p style="line-height:1.5em; margin-right : 5%">
Both approches were initiated at the same time, and if the second one allowed us to obtain
Both approches were initiated at the same time, and if the second one allowed us to obtain
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PCR amplifications of the correct size (see figure) and a complete Prcn-csgBAEFG
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PCR amplifications of the correct size (see figure) and a complete P<i>rcn-csgBAEFG</i>
construction, unfortunately sequencing analysis revealed unexpected mutations that were not
construction, unfortunately sequencing analysis revealed unexpected mutations that were not
removed before reception of the whole part made by Genecust. In brief the "click and order"
removed before reception of the whole part made by Genecust. In brief the "click and order"

Revision as of 22:46, 20 September 2011





A race between two different strategies was used to obtain the first part




In E. coli the curli-producing system is organized in two divergeant operons with the genes csgA, csgB and csgC on one side and csgD, csgE, csgF and csgG of the other one. So to achieve the first approach of the project, it is necessary to begin by the creation of three "sub- parts": the first one would be the part with the sole promoter PrcnA, the second would be the part with the genes csgA and csgB and final one would be the part with the genes csgE, csgF and csgG.

The synthesis of this first DNA part (the cobalt-inducible promoter Prcn-csgBAEFG, which is designed to induce formation of a biofilm and to promote cell adhesion) was conceived as as a competition between two methods: a completely synthetic approach, and a "manual" method involving PCR steps followed by ligations.

  • The first approach consist in ordering the whole part at a private company (Genecust).

  • The second approach was to made it directly at the bench, this approach included three steps: first the amplification by PCR of each of the sub parts, second a mutagenesis step to remove all the natural internal EcoRI sites located in the sub parts, and finally the ligation of these parts.

Both approches were initiated at the same time, and if the second one allowed us to obtain PCR amplifications of the correct size (see figure) and a complete Prcn-csgBAEFG construction, unfortunately sequencing analysis revealed unexpected mutations that were not removed before reception of the whole part made by Genecust. In brief the "click and order" strategy wins the race !




ENS assystem Biomérieux INSA INSA