Aberrant gene activation in synovial sarcoma relies on SSX specificity and increased PRC1.1 stability

Author:

Benabdallah Nezha S.,Dalal Vineet,Scott R. WilderORCID,Marcous Fady,Sotiriou Afroditi,Kommoss Felix K. F.ORCID,Pejkovska Anastasija,Gaspar Ludmila,Wagner Lena,Sánchez-Rivera Francisco J.ORCID,Ta Monica,Thornton Shelby,Nielsen Torsten O.ORCID,Underhill T. MichaelORCID,Banito AnaORCID

Abstract

AbstractThe SS18-SSX fusion drives oncogenic transformation in synovial sarcoma by bridging SS18, a member of the mSWI/SNF (BAF) complex, to Polycomb repressive complex 1 (PRC1) target genes. Here we show that the ability of SS18-SSX to occupy H2AK119ub1-rich regions is an intrinsic property of its SSX C terminus, which can be exploited by fusion to transcriptional regulators beyond SS18. Accordingly, SS18-SSX recruitment occurs in a manner that is independent of the core components and catalytic activity of BAF. Alternative SSX fusions are also recruited to H2AK119ub1-rich chromatin and reproduce the expression signatures of SS18-SSX by engaging with transcriptional activators. Variant Polycomb repressive complex 1.1 (PRC1.1) acts as the main depositor of H2AK119ub1 and is therefore required for SS18-SSX occupancy. Importantly, the SSX C terminus not only depends on H2AK119ub1 for localization, but also further increases it by promoting PRC1.1 complex stability. Consequently, high H2AK119ub1 levels are a feature of murine and human synovial sarcomas. These results uncover a critical role for SSX-C in mediating gene deregulation in synovial sarcoma by providing specificity to chromatin and further enabling oncofusion binding by enhancing PRC1.1 stability and H2AK119ub1 deposition.

Publisher

Springer Science and Business Media LLC

Subject

Molecular Biology,Structural Biology

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