Journal article
Authors list: Rossbach, O; Hung, LH; Khrameeva, E; Schreiner, S; König, J; Curk, T; Zupan, B; Ule, J; Gelfand, MS; Bindereif, A
Publication year: 2014
Pages: 146-155
Journal: RNA Biology
Volume number: 11
Issue number: 2
ISSN: 1547-6286
eISSN: 1555-8584
Open access status: Green
DOI Link: https://doi.org/10.4161/rna.27991
Publisher: Taylor and Francis Group
Abstract:
Heterogeneous nuclear ribonucleoprotein L (hnRNP L) is a multifunctional RNA-binding protein that is involved in many different processes, such as regulation of transcription, translation, and RNA stability. We have previously characterized hnRNP L as a global regulator of alternative splicing, binding to CA-repeat, and CA-rich RNA elements. Interestingly, hnRNP L can both activate and repress splicing of alternative exons, but the precise mechanism of hnRNP L-mediated splicing regulation remained unclear. To analyze activities of hnRNP L on a genome-wide level, we performed individual-nucleotide resolution crosslinking-immunoprecipitation in combination with deep-sequencing (iCLIP-Seq). Sequence analysis of the iCLIP crosslink sites showed significant enrichment of C/A motifs, which perfectly agrees with the in vitro binding consensus obtained earlier by a SELEX approach, indicating that in vivo hnRNP L binding targets are mainly determined by the RNA-binding activity of the protein. Genome-wide mapping of hnRNP L binding revealed that the protein preferably binds to introns and 3 ' UTR. Additionally, position-dependent splicing regulation by hnRNP L was demonstrated: The protein represses splicing when bound to intronic regions upstream of alternative exons, and in contrast, activates splicing when bound to the downstream intron. These findings shed light on the longstanding question of differential hnRNP L-mediated splicing regulation. Finally, regarding 3 ' UTR binding, hnRNP L binding preferentially overlaps with predicted microRNA target sites, indicating global competition between hnRNP L and microRNA binding. Translational regulation by hnRNP L was validated for a subset of predicted target 3 ' UTRs.
Citation Styles
Harvard Citation style: Rossbach, O., Hung, L., Khrameeva, E., Schreiner, S., König, J., Curk, T., et al. (2014) Crosslinking-immunoprecipitation (iCLIP) analysis reveals global regulatory roles of hnRNP L, RNA Biology, 11(2), pp. 146-155. https://doi.org/10.4161/rna.27991
APA Citation style: Rossbach, O., Hung, L., Khrameeva, E., Schreiner, S., König, J., Curk, T., Zupan, B., Ule, J., Gelfand, M., & Bindereif, A. (2014). Crosslinking-immunoprecipitation (iCLIP) analysis reveals global regulatory roles of hnRNP L. RNA Biology. 11(2), 146-155. https://doi.org/10.4161/rna.27991
