iCLIP identifies novel roles for SAFB1 in regulating RNA processing and neuronal function

被引:20
作者
Rivers, Caroline [1 ]
Idris, Jalilah [1 ,2 ]
Scott, Helen [1 ]
Rogers, Mark [3 ]
Lee, Youn-Bok [4 ]
Gaunt, Jessica [1 ]
Phylactou, Leonidas [5 ]
Curk, Tomaz [6 ]
Campbell, Colin [2 ]
Ule, Jernej [7 ]
Norman, Michael [1 ]
Uney, James B. [1 ]
机构
[1] Univ Bristol, Regenerat Med Labs, Sch Clin Sci Cellular & Mol Med, Bristol BS8 1TD, Avon, England
[2] Univ Kuala Lumpur, Inst Med Sci & Technol, Kuala Lumpur 43000, Malaysia
[3] Univ Bristol, Dept Engn & Math, Intelligent Syst Lab, Bristol BS8 1UB, Avon, England
[4] Kings Coll London, Inst Psychiat, MRC Ctr Neurodegenerat Res, London WC2R 2LS, England
[5] Univ Ljubljana, Fac Comp & Informat Sci, SI-1001 Ljubljana, Slovenia
[6] Cyprus Inst Neurol & Genet, CY-1683 Nicosia, Cyprus
[7] UCL Inst Neurol, Dept Mol Neurosci, London WC1N 3BG, England
基金
英国生物技术与生命科学研究理事会; 英国惠康基金; 英国工程与自然科学研究理事会;
关键词
hnRNP; iCLIP; Long non-coding RNA; miRNA; NCAM1; Neuronal; RNA; SAFB1; Splicing; BIPOLAR DISORDER; NUCLEAR-PROTEIN; GENE-EXPRESSION; SCHIZOPHRENIA; BINDING; TRANSCRIPTION; ASSOCIATION; ISOFORMS; ACCUMULATION; COMPLEXES;
D O I
10.1186/s12915-015-0220-7
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Background: SAFB1 is a RNA binding protein implicated in the regulation of multiple cellular processes such as the regulation of transcription, stress response, DNA repair and RNA processing. To gain further insight into SAFB1 function we used iCLIP and mapped its interaction with RNA on a genome wide level. Results: iCLIP analysis found SAFB1 binding was enriched, specifically in exons, ncRNAs, 3' and 5' untranslated regions. SAFB1 was found to recognise a purine-rich GAAGA motif with the highest frequency and it is therefore likely to bind core AGA, GAA, or AAG motifs. Confirmatory RT-PCR experiments showed that the expression of coding and non-coding genes with SAFB1 cross-link sites was altered by SAFB1 knockdown. For example, we found that the isoform-specific expression of neural cell adhesion molecule (NCAM1) and ASTN2 was influenced by SAFB1 and that the processing of miR-19a from the miR-17-92 cluster was regulated by SAFB1. These data suggest SAFB1 may influence alternative splicing and, using an NCAM1 minigene, we showed that SAFB1 knockdown altered the expression of two of the three NCAM1 alternative spliced isoforms. However, when the AGA, GAA, and AAG motifs were mutated, SAFB1 knockdown no longer mediated a decrease in the NCAM1 9-10 alternative spliced form. To further investigate the association of SAFB1 with splicing we used exon array analysis and found SAFB1 knockdown mediated the statistically significant up-and downregulation of alternative exons. Further analysis using RNAmotifs to investigate the frequency of association between the motif pairs (AGA followed by AGA, GAA or AAG) and alternative spliced exons found there was a highly significant correlation with downregulated exons. Together, our data suggest SAFB1 will play an important physiological role in the central nervous system regulating synaptic function. We found that SAFB1 regulates dendritic spine density in hippocampal neurons and hence provide empirical evidence supporting this conclusion. Conclusions: iCLIP showed that SAFB1 has previously uncharacterised specific RNA binding properties that help coordinate the isoform-specific expression of coding and non-coding genes. These genes regulate splicing, axonal and synaptic function, and are associated with neuropsychiatric disease, suggesting that SAFB1 is an important regulator of key neuronal processes.
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页数:15
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