In-cell identification and measurement of RNA-protein interactions.

Graindorge, Antoine; Pinheiro, Inês; Nawrocka, Anna; Mallory, Allison C; Tsvetkov, Peter; Gil, Noa; Carolis, Carlo; Buchholz, Frank; Ulitsky, Igor; Heard, Edith; Taipale, Mikko; Shkumatava, Alena

doi:10.1038/s41467-019-13235-w

Datensatz

DATENSATZ AKTIONENEXPORT

Zur Ablage hinzufügen

Lokale TagsFreigabegeschichteDetailsÜbersicht

Freigegeben

Zeitschriftenartikel

In-cell identification and measurement of RNA-protein interactions.

MPG-Autoren

/cone/persons/resource/persons219042

Buchholz, Frank
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

Externe Ressourcen

Es sind keine externen Ressourcen hinterlegt

Volltexte (beschränkter Zugriff)

Für Ihren IP-Bereich sind aktuell keine Volltexte freigegeben.

Volltexte (frei zugänglich)

Es sind keine frei zugänglichen Volltexte in PuRe verfügbar

Ergänzendes Material (frei zugänglich)

Es sind keine frei zugänglichen Ergänzenden Materialien verfügbar

Zitation

Graindorge, A., Pinheiro, I., Nawrocka, A., Mallory, A. C., Tsvetkov, P., Gil, N., et al. (2019). In-cell identification and measurement of RNA-protein interactions. Nature communications, 10(1): 5317. doi:10.1038/s41467-019-13235-w.

Zitierlink: https://hdl.handle.net/21.11116/0000-0006-7DCA-B

Zusammenfassung

Regulatory RNAs exert their cellular functions through RNA-binding proteins (RBPs). Identifying RNA-protein interactions is therefore key for a molecular understanding of regulatory RNAs. To date, RNA-bound proteins have been identified primarily through RNA purification followed by mass spectrometry. Here, we develop incPRINT (in cell protein-RNA interaction), a high-throughput method to identify in-cell RNA-protein interactions revealed by quantifiable luminescence. Applying incPRINT to long noncoding RNAs (lncRNAs), we identify RBPs specifically interacting with the lncRNA Firre and three functionally distinct regions of the lncRNA Xist. incPRINT confirms previously known lncRNA-protein interactions and identifies additional interactions that had evaded detection with other approaches. Importantly, the majority of the incPRINT-defined interactions are specific to individual functional regions of the large Xist transcript. Thus, we present an RNA-centric method that enables reliable identification of RNA-region-specific RBPs and is applicable to any RNA of interest.