Difference between revisions of "Team:Aix-Marseille/Modeling"
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| − | <h2 class="title wow Hinge"><span style="color:#8E3B8C"> | + | <h2 class="title wow Hinge"><span style="color:#8E3B8C"><span style="font-family:Armalite Rifle">Our idea</h2></span></span> |
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| − | <p class="space20"><div align="justify"> | + | <p class="space20"><div align="justify"><span style="font-family:Courier New">We are delighted to present our models and hope that they will seem clear and explicit. |
| + | During our project, we have expressed several enzymes and built several systems. Therefore, we needed enzymatic models and computer simulation to assess their effectiveness, their stability, and improved them. | ||
| + | We initially chose 3 laccases (B.subtilis, E.coli, T.thermophilus) and 3 cytochromes C (Shewanella, Cynechocistis, Paracoccus denitrificans). | ||
| + | The purpose of our simulations was to determine a custom linker for each of our constructions. | ||
| + | The challenge was to increase the chances of contact between the two enzymes to allow electron transfer. So we had to simulate a system in which our enzymes are pre-positioned. It also involved the selection of a structured linker (alpha helix) to maintain proper conformation. | ||
| + | Another advantage of a linker is a practical one. In fact, it is easier to manipulate one molecule than two. Then, there is no need to observe a proportion ratio.</span> | ||
| + | </div></p> | ||
| + | </div> | ||
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| − | <div class="success-work | + | <div class="success-work science"> |
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| − | + | <img src="http://i.imgur.com/WJg8VPU.jpg" class="img-responsive" space200> | |
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| − | + | </div> | |
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| − | <h2 class="title wow Hinge"><span style ="color:#000000"> | + | <h2 class="title wow Hinge"><span style ="color:#000000"><span style="font-family:Armalite Rifle">Method</span></h2></span> |
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| − | + | ||
| − | + | <p><div align="justify"><span style ="color:#000000"><span style="font-family:courier new">To calculate and view our linkers, we used several bioinformatic tools and structural biology methods. | |
| − | < | + | We offer a brief summary of these: |
| − | < | + | <li style="list-style-type:circle;"> |
| − | + | <li><b>Swiss-PdbViewer :</b> | |
| + | Swiss-PdbViewer (aka DeepView) is an application that provides a user friendly interface allowing to analyze several proteins at the same time. The proteins can be superimposed in order to deduce structural alignments and compare their active sites or any other relevant parts. Amino acid mutations, H-bonds, angles and distances between atoms are easy to obtain thanks to the intuitive graphic and menu interface.</li> | ||
| + | <li><b>Gromacs :</b> | ||
| + | GROMACS is a versatile package to perform molecular dynamics, i.e. simulate the Newtonian equations of motion for systems with hundreds to millions of particles. It is primarily designed for biochemical molecules like proteins, lipids and nucleic acids that have a lot of complicated bonded interactions, but since GROMACS is extremely fast at calculating the nonbonded interactions (that usually dominate simulations) many groups are also using it for research on non-biological systems, e.g. polymers.</li> | ||
| + | <li><b>VMD :</b> | ||
| + | VMD is a molecular visualization program for displaying, animating, and analyzing large biomolecular systems using 3-D graphics and built-in scripting. VMD supports computers running MacOS X, Unix, or Windows, is distributed free of charge, and includes source code. | ||
| + | |||
| + | All these tools need a pdb file as input. The first step is to download the file pdb corresponding to each of the proteins on RCSB PDB (http://www.rcsb.org/pdb/home/home.do). | ||
| + | Then, you have to pre-position the two proteins using Swiss-pdb Viewer. The electron exchange surface must be up to 15 Angstrom from each other. | ||
| + | It is continued by a minimization step to eliminate steric strain. This calcul considers electrostatic forces, Van der Wall interactions etc… | ||
| + | A conformation is generated from these constraints. It is sufficient to take the coordinates of the N-term residue (A) and C-term (B) and to calculate the distance (AB) between the two to generate a linker suitable. | ||
| + | |||
| + | AB = √( (xA-xB)^2+ 〖(yA-yB)^2+(zA-zB)〗^2 ) | ||
| + | |||
| + | A trun-helix contains 3.6 residues and measures 5.4 Angstrom (1.5 Angstrom per residue).</li> | ||
| + | </ul> | ||
| + | |||
| + | |||
| + | |||
| + | </p></span> | ||
| + | |||
| + | </div> | ||
| + | |||
</p></span></div> | </p></span></div> | ||
Revision as of 17:43, 14 September 2015
Our idea
We are delighted to present our models and hope that they will seem clear and explicit.
During our project, we have expressed several enzymes and built several systems. Therefore, we needed enzymatic models and computer simulation to assess their effectiveness, their stability, and improved them.
We initially chose 3 laccases (B.subtilis, E.coli, T.thermophilus) and 3 cytochromes C (Shewanella, Cynechocistis, Paracoccus denitrificans).
The purpose of our simulations was to determine a custom linker for each of our constructions.
The challenge was to increase the chances of contact between the two enzymes to allow electron transfer. So we had to simulate a system in which our enzymes are pre-positioned. It also involved the selection of a structured linker (alpha helix) to maintain proper conformation.
Another advantage of a linker is a practical one. In fact, it is easier to manipulate one molecule than two. Then, there is no need to observe a proportion ratio.
Method
To calculate and view our linkers, we used several bioinformatic tools and structural biology methods.
We offer a brief summary of these:
Swiss-PdbViewer :
Swiss-PdbViewer (aka DeepView) is an application that provides a user friendly interface allowing to analyze several proteins at the same time. The proteins can be superimposed in order to deduce structural alignments and compare their active sites or any other relevant parts. Amino acid mutations, H-bonds, angles and distances between atoms are easy to obtain thanks to the intuitive graphic and menu interface.
Gromacs :
GROMACS is a versatile package to perform molecular dynamics, i.e. simulate the Newtonian equations of motion for systems with hundreds to millions of particles. It is primarily designed for biochemical molecules like proteins, lipids and nucleic acids that have a lot of complicated bonded interactions, but since GROMACS is extremely fast at calculating the nonbonded interactions (that usually dominate simulations) many groups are also using it for research on non-biological systems, e.g. polymers.
VMD :
VMD is a molecular visualization program for displaying, animating, and analyzing large biomolecular systems using 3-D graphics and built-in scripting. VMD supports computers running MacOS X, Unix, or Windows, is distributed free of charge, and includes source code.
All these tools need a pdb file as input. The first step is to download the file pdb corresponding to each of the proteins on RCSB PDB (http://www.rcsb.org/pdb/home/home.do).
Then, you have to pre-position the two proteins using Swiss-pdb Viewer. The electron exchange surface must be up to 15 Angstrom from each other.
It is continued by a minimization step to eliminate steric strain. This calcul considers electrostatic forces, Van der Wall interactions etc…
A conformation is generated from these constraints. It is sufficient to take the coordinates of the N-term residue (A) and C-term (B) and to calculate the distance (AB) between the two to generate a linker suitable.
AB = √( (xA-xB)^2+ 〖(yA-yB)^2+(zA-zB)〗^2 )
A trun-helix contains 3.6 residues and measures 5.4 Angstrom (1.5 Angstrom per residue).
