Multi-level monitoring of EME1-MUS81 in CPT induced nucleolar rDNA repair

Author:

Bakshi Karishma,Nagamalleswari Easa,Breucker Jan,Eisenhardt Nathalie,Tiwari Richa,González-Prieto Román,Fatouros Chronis,Chaugule Viduth K,Lee Heekyoung,Ilic Dragana,Trulsson Fredrik,Mittler Gerhard,Vertegaal Alfred C.O.,Pichler Andrea

Abstract

AbstractWe identified EME1, the regulatory subunit of the structure-specific endonuclease complex EME1-MUS81, as substrate for the sumoylated UBC9 and demonstrated synergistic functions in promoting Camptothecin (CPT)-induced nucleolar ribosomal DNA (rDNA) repair (Nagamalleswari et al, co-submitted). Sumoylation of EME1 appears complex involving mono- and poly-sumoylation. Hence, we addressed here whether these modifications differentially regulate EME1 functions by analyzing EME1-variant expressing cell lines including mono-sumo(1)ylation and poly-sumo(2)ylation mimetic fusions. We complemented our analysis with the regulated endogenous EME1 interactome and our observation that Trichostatin A (TSA) induced EME1 and UBC9 sumoylation. Our findings are substantiated by identifying several regulatory proteins and by detecting CPT-induced endogenous di- and poly-sumoylated EME1 in different cell fractions. Together, our data suggest that Histone H4 acetylation, two mono-sumoylation events, poly-sumoylation, ISG15 and ubiquitination sequentially and in mutual dependence tightly control the intracellular localization, recruitment to DNA lesions, enzymatic activity, withdrawal from DNA lesions and the stability of EME1.

Publisher

Cold Spring Harbor Laboratory

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