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    <meta name="description" content="Application Domains - Protein-RNA Interactions"/>
    <meta name="dc.title" content="Application Domains - Protein-RNA Interactions"/>
    <meta name="dc.creator" content="Isaure Chauvot de Beauchêne"/>
    <meta name="dc.creator" content="Antoine Moniot"/>
    <meta name="dc.creator" content="Bernard Maigret"/>
    <meta name="dc.creator" content="Maria Elisa Ruiz Echartea"/>
    <meta name="dc.creator" content="David Ritchie"/>
    <meta name="dc.creator" content="Agnibha Chandra"/>
    <meta name="dc.creator" content="Rohit Roy"/>
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    <meta name="dc.date" content="(SCHEME=ISO8601) 2018-01"/>
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	    Raweb 
	    2018</a> | <a href="http://www.inria.fr/en/teams/capsid">Presentation of the Project-Team CAPSID</a> | <a href="http://capsid.loria.fr/">CAPSID Web Site
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        <h2>Section: 
      Application Domains</h2>
        <h3 class="titre3">Protein-RNA Interactions</h3>
        <p class="participants"><span class="part">Participants</span> :
	Isaure Chauvot de Beauchêne [contact person] , Antoine Moniot, Bernard Maigret, Maria Elisa Ruiz Echartea, David Ritchie, Agnibha Chandra, Rohit Roy.</p>
        <p>As well as playing an essential role in the translation of DNA into proteins,
RNA molecules carry out many other essential biological functions in cells,
often through their interactions with proteins.
A critical challenge in modelling such interactions computationally is that
the RNA is often highly flexible, especially in single-stranded (ssRNA) regions of its structure.
These flexible regions are often very important because it is through their
flexibility that the RNA can adjust its 3D conformation in order to bind to a protein surface.
However, conventional protein-protein docking algorithms generally assume that the 3D
structures to be docked are rigid, and so are not suitable for modeling protein-RNA interactions.
There is therefore much interest in developing protein-RNA docking algorithms which can
take RNA flexibility into account.</p>
        <p>We are currently developing a novel flexible docking algorithm which first docks
small fragments of ssRNA (typically three nucleotides at a time)
onto a protein surface, and then combinatorially reassembles those fragments in order
to recover a contiguous ssRNA structure on the protein surface
<a href="./bibliography.html#capsid-2018-bid58">[44]</a>, <a href="./bibliography.html#capsid-2018-bid59">[45]</a>.
We have since implemented a prototype “forward-backward”
dynamic programming algorithm with stochastic backtracking that allows us to
model protein RNA interactions for ssRNAs of up to 7 nucleotides without requiring
any prior knowledge of the interaction, while still avoiding a brute-force search.
In the frame of our PEPS collaboration “InterANRIL” with the
IMoPA lab (University of Lorraine), we are currently working with biologists to
apply the approach to modeling
certain
long non-coding RNA (lncRNA) complexes.
In order to extend this approach to partially structured RNA
molecules, we have built an automated pipeline to create
(i) libraries of RNA fragments with arbitrary characteristics such as secondary
structure,
and (ii) testing benchmarks for applying those libraries in docking.
In the frame of our LUE-FEDER CITRAM project we
adapted this approach and this pipeline to DNA docking in order to
model the complex formed by a bacterial relaxase and its target DNA.</p>
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