Team:INSA-Lyon/Molecular

From 2014.igem.org

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The very first result we are going to talk about is that even without an His-tag, <b>the wildtype protein is able to chelate nickel</b>. That is something we didn't expect and were surprised to discover. We put, some nickels next to CsgA (for of around 10 Angstroms), and Sybyl computes the simulations (with AMBER FF002 library, cutoff at 12 Ang, during 10 to 20 000 fs). Nickel can be captured by either a <b>group of ketones</b> that are close to each other, but even more surprising, we observed histidines, aspartic acids and other amino acids already present in wildtype CsgA are "grabbing" the ions and litterally pulling them  between the beta strands <b>into the center of the protein for some of them</b>.</br></br></p>
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The very first result we are going to talk about is that even without an His-tag, <b>the wildtype protein is able to chelate nickel</b>. That is something we didn't expect and were surprised to discover. We put some nickels next to CsgA (in a 10 Angstroms radius), and Sybyl computed the simulations (with AMBER FF002 library, cutoff at 12 Ang, during 10 to 20 000 fs). Nickel can be captured by either a <b>group of ketones</b> that are close to each other, but even more surprising, we observed histidines, aspartic acids and other amino acids already present in wildtype CsgA were "grabbing" the ions and litterally pulling them  between the beta strands <b>into the center of the protein in some cases</b>.</br></br></p>
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For the <b>folded conformation</b> the tag, be it His1-tag or His2-tag, covers already existing chelating sites of CsgA, but is still able to chelate nickel ions. The simulations showed that, though it could also fold a little to catch a nickel with two of it's histidines, a bond between the nickel and both the tag AND CsgA often occured, thus being chelated but also stabilising the folded structure of the tag. However, with its reach decreased and the covering of the initial protein chelating sites, we concluded that such a conformation wouldn't bring much more chelating power to the protein.</br></br></p>
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A far as the <b>folded conformation</b> is concerned, both His1-tag or His2-tag, cover already existing chelating sites of CsgA, but are still able to chelate nickel ions. The simulations showed that, though the tag could also fold a little to catch a nickel with two of its histidines, a bond between the nickel and both the tag AND CsgA often occured, thus stabilising the folded structure of the tag. However, with its reach decreased and the covering of the initial protein chelating sites, we concluded that such a conformation wouldn't bring much more chelating power to the protein.</br></br></p>
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Revision as of 18:35, 17 October 2014

Curly'on - IGEM 2014 INSA-LYON

One of the main goals of our modeling work this year was to understand the structure of the curli subunit protein, CsgA and its behavior when engineered with a tag constituted of either six histidines (that we will call His1-tag from now on) or twice that motif (His2-tag), since this peptide is known for its nickel chelation properties.
We then discussed over our results with the wetlab members to define a way to confirm the accuracy of our model, and so we were able to assess that, in accordance with litterature, the best position for the tag was by the C-terminus of the protein. We also determined that the His-tag was more likely to take a floating conformation instead of folding itself around CsgA.


  • Methods


  • CsgA Engineering


  • Ni-Chelation




Conclusion

Overall sum up

Through our molecular study of a CsgA protein engineered with either His1-tag or His2-tag, we came to the conclusion that since it has a longer reach and its mobility makes it more available for chelation, using a tag positioned by the C-terminus of the protein is more relevant than placing it in the middle of the sequence, although doing so may provide a little more chelation power as long as the tag isn't too long.
We also showed that for the tags there exist two possible conformations : one is folded on the side of CsgA and a priori does not increase the already-existing chelating power of CsgA; the other is a "floating" conformation where the tag is not attracted to the protein and is able to improve its chelating power by up to 25%!

What we couldn't achieve

Unfortunately, having very little time and people, there are a few things we couldn't investigate as extensively as we wanted. Here are a few of those things:

  • more simulations with His2-tag. Since they took an awful lot of time, we only ran a handful of them;
  • modelisation of the docking between two CsgA proteins, and the influence of the His-tags, that our lack of experience prevented us to conduct;
  • find out just how many tags can be added without altering the protein properties of adherence and polymerisation;