Difference between revisions of "Team:Queens Canada/Modeling"
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<p>In order to test the self-assembly of the AFPs and scaffold proteins with E/K coils, docking simulations were run. These were used to assess the energetic stability of the coiled coil interaction and determine the orientation of the ice-binding surface of the AFP. This was done using <a href="">PyRosetta</a> by following the standard procedure for initial low resolution docking prior to high resolution docking on favourable protein structures. Sorting of low energy dockings was used with consideration given to the proximity of the E/K coils to choose a final selection of proteins for refinement and scoring. The general procedure used is outlined in Figure 8 and the final docked structure reached shown in Figure 9.</p> | <p>In order to test the self-assembly of the AFPs and scaffold proteins with E/K coils, docking simulations were run. These were used to assess the energetic stability of the coiled coil interaction and determine the orientation of the ice-binding surface of the AFP. This was done using <a href="">PyRosetta</a> by following the standard procedure for initial low resolution docking prior to high resolution docking on favourable protein structures. Sorting of low energy dockings was used with consideration given to the proximity of the E/K coils to choose a final selection of proteins for refinement and scoring. The general procedure used is outlined in Figure 8 and the final docked structure reached shown in Figure 9.</p> | ||
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<figcaption>Figure 8. <strong>Flow chart of general protocol used to determine configuration of docked AFP/scaffold complex.</strong> Flow chart starts with PDB files and structures of the proteins of interest, and involves isolating the most stable conformations for further analysis.<a href="#">T3-10 Scaffold</a> and <a href="#">Type III AFP</a>. </figcaption> | <figcaption>Figure 8. <strong>Flow chart of general protocol used to determine configuration of docked AFP/scaffold complex.</strong> Flow chart starts with PDB files and structures of the proteins of interest, and involves isolating the most stable conformations for further analysis.<a href="#">T3-10 Scaffold</a> and <a href="#">Type III AFP</a>. </figcaption> | ||
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− | <img src=" | + | <img src="https://static.igem.org/mediawiki/2015/8/86/Qqq_QGEM_AFPscaff.jpg" /> |
<figcaption>Figure 9. <strong>Final alignment of AFP and scaffold coiled-coil interaction after docking and refinement.</strong>Scaffold subunits are shown in yellow with a rainbow K-coil to demonstrate directionality. An AFP is shown in grey and the ice binding residues are highlighted in orange. </figcaption> | <figcaption>Figure 9. <strong>Final alignment of AFP and scaffold coiled-coil interaction after docking and refinement.</strong>Scaffold subunits are shown in yellow with a rainbow K-coil to demonstrate directionality. An AFP is shown in grey and the ice binding residues are highlighted in orange. </figcaption> | ||
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Revision as of 14:36, 23 August 2015