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Quantitative mass spectrometry and PAR-CLIP to identify RNA-protein interactions.


ABSTRACT: Systematic analysis of the RNA-protein interactome requires robust and scalable methods. We here show the combination of two completely orthogonal, generic techniques to identify RNA-protein interactions: PAR-CLIP reveals a collection of RNAs bound to a protein whereas SILAC-based RNA pull-downs identify a group of proteins bound to an RNA. We investigated binding sites for five different proteins (IGF2BP1-3, QKI and PUM2) exhibiting different binding patterns. We report near perfect agreement between the two approaches. Nevertheless, they are non-redundant, and ideally complement each other to map the RNA-protein interaction network.

SUBMITTER: Scheibe M 

PROVIDER: S-EPMC3479200 | biostudies-literature | 2012 Oct

REPOSITORIES: biostudies-literature

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Quantitative mass spectrometry and PAR-CLIP to identify RNA-protein interactions.

Scheibe Marion M   Butter Falk F   Hafner Markus M   Tuschl Thomas T   Mann Matthias M  

Nucleic acids research 20120809 19


Systematic analysis of the RNA-protein interactome requires robust and scalable methods. We here show the combination of two completely orthogonal, generic techniques to identify RNA-protein interactions: PAR-CLIP reveals a collection of RNAs bound to a protein whereas SILAC-based RNA pull-downs identify a group of proteins bound to an RNA. We investigated binding sites for five different proteins (IGF2BP1-3, QKI and PUM2) exhibiting different binding patterns. We report near perfect agreement b  ...[more]

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