The splicing factor XAB2 interacts with ERCC1-XPF and XPG for R-loop processing

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作者
Evi Goulielmaki
Maria Tsekrekou
Nikos Batsiotos
Mariana Ascensão-Ferreira
Eleftheria Ledaki
Kalliopi Stratigi
Georgia Chatzinikolaou
Pantelis Topalis
Theodore Kosteas
Janine Altmüller
Jeroen A. Demmers
Nuno L. Barbosa-Morais
George A. Garinis
机构
[1] Foundation for Research and Technology-Hellas,Institute of Molecular Biology and Biotechnology
[2] University of Crete,Department of Biology
[3] Faculdade de Medicina da Universidade de Lisboa,Instituto de Medicina Molecular João Lobo Antunes
[4] Avenida Professor Egas Moniz,Cologne Center for Genomics (CCG), Institute for Genetics
[5] University of Cologne,Proteomics Center, Netherlands Proteomics Center, and Department of Biochemistry
[6] Erasmus University Medical Center,undefined
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RNA splicing, transcription and the DNA damage response are intriguingly linked in mammals but the underlying mechanisms remain poorly understood. Using an in vivo biotinylation tagging approach in mice, we show that the splicing factor XAB2 interacts with the core spliceosome and that it binds to spliceosomal U4 and U6 snRNAs and pre-mRNAs in developing livers. XAB2 depletion leads to aberrant intron retention, R-loop formation and DNA damage in cells. Studies in illudin S-treated cells and Csbm/m developing livers reveal that transcription-blocking DNA lesions trigger the release of XAB2 from all RNA targets tested. Immunoprecipitation studies reveal that XAB2 interacts with ERCC1-XPF and XPG endonucleases outside nucleotide excision repair and that the trimeric protein complex binds RNA:DNA hybrids under conditions that favor the formation of R-loops. Thus, XAB2 functionally links the spliceosomal response to DNA damage with R-loop processing with important ramifications for transcription-coupled DNA repair disorders.
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