Myelodysplastic Syndrome-Associated SRSF2 Mutations Cause Splicing Changes by Altering Binding Motif Sequences.

Kenji Suzuki,Ayana Kon,Yusuke Shiozawa,Asuka Hata,So Masaki,Shun Ikeda,Seishi Ogawa,Fumihiko Hakuno,Naoyuki Kataoka,Shin-Ichiro Takahashi

doi:10.3389/fgene.2019.00338

Abstract

Serine/arginine-rich splicing factor 2 (SRSF2) is a member of the SR protein family that is involved in both constitutive and alternative mRNA splicing. Mutations in SRSF2 gene are frequently reported in myelodysplastic syndromes (MDS) and acute myeloid leukemia (AML). It is imperative to understand how these mutations affect SRSF2-mediated splicing and cause MDS. In this study, we characterized MDS-associated SRSF2 mutants (P95H, P95L, and P95R). We found that those mutants and wild-type SRSF2 proteins showed nuclear localization in HeLa cells. In vitro splicing reaction also revealed that mutant proteins associated with both precursor and spliced mRNAs, suggesting that the mutants directly participate in splicing. We established the human myeloid leukemia K562 cell lines that stably expressed myc-tagged wild-type or mutant SRSF2 proteins, and then performed RNA-sequence to analyze the splicing pattern of each cell line. The results revealed that both wild-type and mutants affected splicing of approximately 3,000 genes. Although splice site sequences adjacent to the affected exons showed no significant difference compared to the total exons, exonic motif analyses with both inclusion- and exclusion-enhanced exons demonstrated that wild-type and mutants have different binding sequences in exons. These results indicate that mutations of SRSF2 in MDS change binding properties of SRSF2 to exonic motifs and this causes aberrant splicing.

Highlights

Serine/Arginine rich (SR) proteins are essential splicing factors that confer regulatory activity of alternative splicing (Manley and Krainer, 2010; Howard and Sanford, 2015; Kataoka, 2017)
In order to gain insights on how mutations in Serine/arginine-rich splicing factor 2 (SRSF2), one of the splicing factors mutated in myelodysplastic syndromes (MDS) patients, affect splicing, we have prepared the SRSF2 mutant cDNAs carrying three kinds of mutations at 95th position of Proline residue (P95H, L and R) found in MDS patients
Both wild-type and mutants of SRSF2 cDNAs were transfected into HeLa cells and those proteins were expressed as fusions with a myc-tag

Summary

Introduction

Serine/Arginine rich (SR) proteins are essential splicing factors that confer regulatory activity of alternative splicing (Manley and Krainer, 2010; Howard and Sanford, 2015; Kataoka, 2017). SRSF2, which was originally called SC35, is a member of the SR protein family (Fu and Maniatis, 1990; Fu and Ares, 2014; Kataoka, 2017). SRSF2 promotes exon recognition by binding to exonic splicing enhancer (ESE) motifs in precursor of mRNA (pre-mRNA) through its RBD. This promotes both the binding of U2AF heterodimer and U1 snRNP to the upstream 3 splice site and to the downstream 5 splice site, respectively (Chen and Manley, 2009; Fu and Ares, 2014; Kataoka, 2017)

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Results

Conclusion