Difference between revisions of "Team:Toronto/Model"

 
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<li><a href="https://2016.igem.org/Team:Toronto/HP-Gold"><span>gold</span></a></li>
 
<li><a href="https://2016.igem.org/Team:Toronto/HP-Gold"><span>gold</span></a></li>
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<li><a href="https://2016.igem.org/Team:Toronto/HP-Impact"><span>impact</span></a></li>
 
 
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<li><a href="https://2016.igem.org/Team:Toronto/Integrated_Practices"><span>integrated_practices</span></a></li>
 
<li><a href="https://2016.igem.org/Team:Toronto/Integrated_Practices"><span>integrated_practices</span></a></li>
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<div class="content" id="content-main"><div class="row"><div class="col col-lg-8 col-md-12"><div class="content-main"><h3 id="-alert-">★ ALERT!</h3>
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<div class="content" id="content-main"><div class="row"><div class="col col-lg-8 col-md-12"><div class="content-main"><h1 id="modeling-protein-folding-with-rosetta">Modeling Protein Folding with Rosetta</h1>
<p>This page is used by the judges to evaluate your team for the <a href="https://2016.igem.org/Judging/Awards#SpecialPrizes">Best Model award</a>.</p>
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<h3 id="introduction">Introduction</h3>
<p>Delete this box in order to be evaluated for this medal. See more information at <a href="https://2016.igem.org/Judging/Pages_for_Awards/Instructions">Instructions for Pages for awards</a>.</p>
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<p>In order to model and compare the gold(III)-binding ability of a GolS homodimer and two mutant variants, we used the Robetta Full-chain Protein Structure Prediction Server, as well as the Rosetta and pyRosetta modeling software tools. GolS, as a MerR family transcriptional regulator, serves as a kind of natural “gold detector” within S. enterica, but lacks specificity for gold, and is susceptible to cross-reactions with copper(I) and silver(I) (Checa and Soncini, 2011). Further, there is no extant crystal structure for GolS. In conjunction with our Wet Lab’s efforts to improve the gold-selectivity and specificity of GolS, we have modeled the gold(III)-binding potential of a GolS homodimer and two mutated variants (P118A, or alanine-to-phenylananine point mutation at residue 118, and A113T, or alanine-to-threonine point mutation at residue 113). In particular, these mutations were designed to shrink the size of the metal ion binding pocket of GolS. GolS shares a helix-turn-helix metal ion binding domain and almost all major catalytic residues with another MerR transcriptional regulator, CueR, that is sensitive to copper. These catalytic residues include Thr13, Lys15, Arg18, Tyr20, Asn34, Tyr36, Arg37, and Arg54, but have an exception in Ser4 in GolS, which corresponds to the functionally opposed Gly4 in CueR. Given these similarities, our Wet Lab formed the hypothesis that the size and shape of the metal ion binding pocket of MerR family transcriptional regulators may confer binding specificity to a particular metal ion.</p>
<h2 id="modeling">Modeling</h2>
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<h3 id="modeling-the-gols-homodimer-with-rosetta">Modeling the GolS Homodimer with Rosetta</h3>
<p>Mathematical models and computer simulations provide a great way to describe the function and operation of BioBrick Parts and Devices. Synthetic Biology is an engineering discipline, and part of engineering is simulation and modeling to determine the behavior of your design before you build it. Designing and simulating can be iterated many times in a computer before moving to the lab. This award is for teams who build a model of their system and use it to inform system design or simulate expected behavior in conjunction with experiments in the wetlab.</p>
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<p>We modeled GolS as a homodimer for two reasons; firstly, many MerR family transcriptional regulators function as homodimers, and secondly, we predict that monomer-monomer interactions between Cys112 and Cys120 from chain 1 and Ser77 from chain B, (from each side), are necessary for chelation of the metal ion, such that the gold-binding potential of a GolS monomer could not usefully be measured.
<h5 id="inspiration">Inspiration</h5>
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In order to model GolS as a homodimer, we inputted the amino acid sequence of GolS, our desired symmetry constraints, and a CueR template. and used the Robetta 3-D Modeling web service in order to generate a 3D structure for a GolS homodimer. Robetta employs the ‘Ginzu’ method of domain prediction to screen for regions of the query sequence that are homologous to extant experimentally verified models via BLAST, PSI-BLAST, FFASO3, 3D-Jury, and multiple-sequence based alignments. This is followed by alignment of the generated model with the template through the K*Sync method, which utilizes secondary-structure prediction and residue profile-profile comparison (Kim, E.D., Chivian, D., and Baker, D., 2004.) A still image of the generated GolS homodimer is attached below in Appendix I.</p>
<p>Here are a few examples from previous teams:</p>
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<h3 id="modeling-mutant-variants-in-pyrosetta">Modeling Mutant Variants in PyRosetta</h3>
<ul>
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<p>In order to model the mutant variants of GolS, we used PyRosetta’s “pose_from_pdb” function to generate a “pose” structure that could be manipulated within PyRosetta from the Robetta-generated Protein Data Bank (PDB) file of the GolS homodimer. Following “pose” generation, we used the “mutate_residue” function to create two mutant GolS variants: a P118A variant where the Ala118 residue in GolS was converted to Phe118 and a A113T variant where the Ala113 residue in GolS was converted to Thr113, and PyRosetta automatically accounts for resulting changes to rotamers (Chaudhary, Lyskov, and Gray, 2010). </p>
<li><a href="https://2014.igem.org/Team:ETH_Zurich/modeling/overview">ETH Zurich 2014</a></li>
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<h3 id="modeling-gold-binding">Modeling Gold Binding</h3>
<li><a href="https://2014.igem.org/Team:Waterloo/Math_Book">Waterloo 2014</a></li>
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<p>Finally, we created a model for our ligand (gold (III)) within Rosetta, modelled the ability of the GolS homodimer to bind gold(III), and further compared the gold-binding abilities of two mutant versions of GolS, P118A and A113T. First, we downloaded a structural data file (SDF file) containing information of all documented instances of AU3+ functioning as a ligand from RCSB (Berman, Westbrook, Feng, Gililand, Bhat, Weissig, Shindyalov, Bourne, 2000). Following this, we executed Rosetta’s “molfile_to_params” function in order to generate a “params” file for gold(III) containing structural and charge information that allowed for ligand modelling within Rosetta. Due to the fact that gold(III) is a metal ion and is not expected to contain hydrogens, we were able to omit an intermediate cleaning step that is usually required prior to generation of a “params” file.</p>
</ul>
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<h3 id="modeling-the-size-of-the-metal-ion-binding-pocket">Modeling the Size of the Metal Ion Binding Pocket</h3>
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<p>With the known CueR structure in 1Q07, we were able to identify the thiol groups from Cys112 and Cys120 that interact with the gold ion. So we measured the distance between them which was 4.7Å (Appendix 1.B). Our hypothesis was that GolS would have a smaller pocket for the metal binding region and when we measured the distance between the thiol groups in the same residues, we found it to have a distance of 4.5Å. Furthermore, by creating an electron density map around these two residues, we noticed the greater electron density of GolS is a result of the presence of one additional Cysteine atom in GolS (Cys111), compared to CueR, which increases the electron density of the binding pocket such that gold ion docks more easily to GolS than to CueR (Appendix 2).</p>
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<h1 id="appendices">Appendices</h1>
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<h2 id="appendix-1-gols-predicted-structure-and-cuer-and-gols-metal-binding-region-">Appendix 1: GolS predicted structure and CueR and GolS metal binding region.</h2>
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<p><img src="https://static.igem.org/mediawiki/2016/thumb/9/91/Golsxcuer.jpeg/732px-Golsxcuer.jpeg" alt=""></p>
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<h2 id="appendix-2-gols-metal-binding-region-electron-density-cloud">Appendix 2: GolS metal binding region electron density cloud</h2>
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<p><img src="https://static.igem.org/mediawiki/2016/c/cb/Datgols.jpg" alt=""></p>
 
</div></div><div id="tableofcontents" class="tableofcontents affix sidebar col-lg-4 hidden-xs hidden-sm hidden-md visible-lg-3"><ul class="nav">
 
</div></div><div id="tableofcontents" class="tableofcontents affix sidebar col-lg-4 hidden-xs hidden-sm hidden-md visible-lg-3"><ul class="nav">
<li><a href="#modeling">Modeling</a><ul>
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<li><a href="#introduction">Introduction</a></li>
<li><a href="#inspiration">Inspiration</a></li>
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<li><a href="#modeling-the-gols-homodimer-with-rosetta">Modeling the GolS Homodimer with Rosetta</a></li>
 +
<li><a href="#modeling-mutant-variants-in-pyrosetta">Modeling Mutant Variants in PyRosetta</a></li>
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<li><a href="#modeling-gold-binding">Modeling Gold Binding</a></li>
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<li><a href="#modeling-the-size-of-the-metal-ion-binding-pocket">Modeling the Size of the Metal Ion Binding Pocket</a><ul>
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<li><a href="#appendices">Appendices</a></li>
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<li><a href="#appendix-1--gols-predicted-structure-and-cuer-and-gols-metal-binding-region">Appendix 1: GolS predicted structure and CueR and GolS metal binding region.</a></li>
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<li><a href="#appendix-2--gols-metal-binding-region-electron-density-cloud">Appendix 2: GolS metal binding region electron density cloud</a></li>
 
</ul>
 
</ul>
 
</li>
 
</li>

Latest revision as of 03:17, 20 October 2016

Modeling Protein Folding with Rosetta

Introduction

In order to model and compare the gold(III)-binding ability of a GolS homodimer and two mutant variants, we used the Robetta Full-chain Protein Structure Prediction Server, as well as the Rosetta and pyRosetta modeling software tools. GolS, as a MerR family transcriptional regulator, serves as a kind of natural “gold detector” within S. enterica, but lacks specificity for gold, and is susceptible to cross-reactions with copper(I) and silver(I) (Checa and Soncini, 2011). Further, there is no extant crystal structure for GolS. In conjunction with our Wet Lab’s efforts to improve the gold-selectivity and specificity of GolS, we have modeled the gold(III)-binding potential of a GolS homodimer and two mutated variants (P118A, or alanine-to-phenylananine point mutation at residue 118, and A113T, or alanine-to-threonine point mutation at residue 113). In particular, these mutations were designed to shrink the size of the metal ion binding pocket of GolS. GolS shares a helix-turn-helix metal ion binding domain and almost all major catalytic residues with another MerR transcriptional regulator, CueR, that is sensitive to copper. These catalytic residues include Thr13, Lys15, Arg18, Tyr20, Asn34, Tyr36, Arg37, and Arg54, but have an exception in Ser4 in GolS, which corresponds to the functionally opposed Gly4 in CueR. Given these similarities, our Wet Lab formed the hypothesis that the size and shape of the metal ion binding pocket of MerR family transcriptional regulators may confer binding specificity to a particular metal ion.

Modeling the GolS Homodimer with Rosetta

We modeled GolS as a homodimer for two reasons; firstly, many MerR family transcriptional regulators function as homodimers, and secondly, we predict that monomer-monomer interactions between Cys112 and Cys120 from chain 1 and Ser77 from chain B, (from each side), are necessary for chelation of the metal ion, such that the gold-binding potential of a GolS monomer could not usefully be measured. In order to model GolS as a homodimer, we inputted the amino acid sequence of GolS, our desired symmetry constraints, and a CueR template. and used the Robetta 3-D Modeling web service in order to generate a 3D structure for a GolS homodimer. Robetta employs the ‘Ginzu’ method of domain prediction to screen for regions of the query sequence that are homologous to extant experimentally verified models via BLAST, PSI-BLAST, FFASO3, 3D-Jury, and multiple-sequence based alignments. This is followed by alignment of the generated model with the template through the K*Sync method, which utilizes secondary-structure prediction and residue profile-profile comparison (Kim, E.D., Chivian, D., and Baker, D., 2004.) A still image of the generated GolS homodimer is attached below in Appendix I.

Modeling Mutant Variants in PyRosetta

In order to model the mutant variants of GolS, we used PyRosetta’s “pose_from_pdb” function to generate a “pose” structure that could be manipulated within PyRosetta from the Robetta-generated Protein Data Bank (PDB) file of the GolS homodimer. Following “pose” generation, we used the “mutate_residue” function to create two mutant GolS variants: a P118A variant where the Ala118 residue in GolS was converted to Phe118 and a A113T variant where the Ala113 residue in GolS was converted to Thr113, and PyRosetta automatically accounts for resulting changes to rotamers (Chaudhary, Lyskov, and Gray, 2010).

Modeling Gold Binding

Finally, we created a model for our ligand (gold (III)) within Rosetta, modelled the ability of the GolS homodimer to bind gold(III), and further compared the gold-binding abilities of two mutant versions of GolS, P118A and A113T. First, we downloaded a structural data file (SDF file) containing information of all documented instances of AU3+ functioning as a ligand from RCSB (Berman, Westbrook, Feng, Gililand, Bhat, Weissig, Shindyalov, Bourne, 2000). Following this, we executed Rosetta’s “molfile_to_params” function in order to generate a “params” file for gold(III) containing structural and charge information that allowed for ligand modelling within Rosetta. Due to the fact that gold(III) is a metal ion and is not expected to contain hydrogens, we were able to omit an intermediate cleaning step that is usually required prior to generation of a “params” file.

Modeling the Size of the Metal Ion Binding Pocket

With the known CueR structure in 1Q07, we were able to identify the thiol groups from Cys112 and Cys120 that interact with the gold ion. So we measured the distance between them which was 4.7Å (Appendix 1.B). Our hypothesis was that GolS would have a smaller pocket for the metal binding region and when we measured the distance between the thiol groups in the same residues, we found it to have a distance of 4.5Å. Furthermore, by creating an electron density map around these two residues, we noticed the greater electron density of GolS is a result of the presence of one additional Cysteine atom in GolS (Cys111), compared to CueR, which increases the electron density of the binding pocket such that gold ion docks more easily to GolS than to CueR (Appendix 2).

Appendices

Appendix 1: GolS predicted structure and CueR and GolS metal binding region.

Appendix 2: GolS metal binding region electron density cloud