USP7 and VCPFAF1 define the SUMO/Ubiquitin landscape at the DNA replication fork

Franz, André; Valledor, Pablo; Ubieto-Capella, Patricia; Pilger, Domenic; Galarreta, Antonio; Lafarga, Vanesa; Fernández-Llorente, Alejandro; Vega-Barranco, Guillermo de la; Brave, Fabian den; Hoppe, Thorsten; Fernández-Capetillo, Óscar; Lecona, Emilio

doi:10.1016/j.celrep.2021.109819

Cited by 17 publications

(19 citation statements)

References 70 publications

(104 reference statements)

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“…The evolution of Ubxn7 to specifically link neddylated cullins with their substrates and the processing factor p97 is an additional level of regulation that ensures efficiency in p97 substrate targeting. The role of UBXN-3 in regulating SUMOylated factors at replication forks seems to have been conserved throughout evolution as it is also the case in human immortalized cells (29). It will be very interesting to decipher the contribution of FAF1 and UBXD7 to replisome disassembly in human cells in the future.…”

Section: Ubxn7 and Faf1 During Replicationmentioning

confidence: 92%

“…Immunodepletion of Ubxn7, but not Faf1, from egg extract leads to a delay in replisome disassembly (Figures 2 and 3). The C. elegans homologue of Faf1, UBXN-3, has been shown to be important for CMG helicase unloading by p97 in S-phase and in mitosis (4,11), but also to regulate other replication factors such as CDT-1 and, recently, to regulate SUMOylated factors at DNA replication forks (17,28,29). It is clear, therefore, that UBXN-3 plays a key role in extraction of proteins from chromatin during DNA replication in C. elegans embryos.…”

Section: Ubxn7 and Faf1 During Replicationmentioning

confidence: 99%

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The p97 segregase cofactor Ubxn7 facilitates replisome disassembly during S-phase

Tarcan

Poovathumkadavil

Skagia

et al. 2022

Journal of Biological Chemistry

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Section: Ubxn7 and Faf1 During Replicationmentioning

confidence: 92%

Section: Ubxn7 and Faf1 During Replicationmentioning

confidence: 99%

The p97 segregase cofactor Ubxn7 facilitates replisome disassembly during S-phase

Tarcan

Poovathumkadavil

Skagia

et al. 2022

Journal of Biological Chemistry

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“…An emerging question is how cells would decide between RNF4 mediated degradation and TRIM25 signaling pathways. One exciting candidate could be USP7, a SUMO-targeted ubiquitin protease that cooperates with VCP to define SUMO/ubiquitin levels at replication forks 50, 54 . In support, USP7 has been found to interact with TRIM25 55 , and has a clear preference for cleavage of K48- over K63-linked chains 56 .…”

Section: Discussionmentioning

confidence: 99%

“…Then, poly-sumoylated EME1 is extracted by the AAA ATPase VCP/p97-NPL4-UFD1 complex, which we observed in our EME1-IP (Extended Data Fig. 7) and which is established to extract poly-sumoylated and/or ubiquitinated proteins form replication forks and nucleolar repair condensates [49][50][51][52] . This step likely requires poly-sumoylation-dependent ubiquitination, as it best understood for the STUbL RNF4 but may also apply to TRIM25.…”

Section: Discussionmentioning

confidence: 99%

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

Karishma

Nagamalleswari

Breuker

et al. 2022

Preprint

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We 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.

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“…Additionally, SPRTN can be recruited along with p97 to SUMO-conjugated TOP1-DPCs via the p97 co-factor TEX264, which associates with replication fork presumably tethering SPRTN to DPCs that block ongoing DNA replication ( Fielden et al, 2020 ) ( Figure 1G ). However, the stimulatory function of SUMO on SPRTN activity has yet to be confirmed in vitro , and could be caused by indirect effects due to the global role of SUMOylation on DNA replication ( Lecona et al, 2016 ; Franz et al, 2021 ). In contrast to SPRTN, which is expressed in different cell types, ACRC (GCNA) is mainly expressed in germ cells ( Carmell et al, 2016 ) where it was recently shown to target TOP2-DPCs during meiosis ( Bhargava et al, 2020 ; Dokshin et al, 2020 ) ( Figure 1G ).…”

Section: Role Of Sumo In Dna-protein Crosslink Removal By Dna-protein...mentioning

confidence: 99%

Targeting DNA-Protein Crosslinks via Post-Translational Modifications

Leng

Duxin

2022

Front. Mol. Biosci.

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Covalent binding of proteins to DNA forms DNA-protein crosslinks (DPCs), which represent cytotoxic DNA lesions that interfere with essential processes such as DNA replication and transcription. Cells possess different enzymatic activities to counteract DPCs. These include enzymes that degrade the adducted proteins, resolve the crosslinks, or incise the DNA to remove the crosslinked proteins. An important question is how DPCs are sensed and targeted for removal via the most suited pathway. Recent advances have shown the inherent role of DNA replication in triggering DPC removal by proteolysis. However, DPCs are also efficiently sensed and removed in the absence of DNA replication. In either scenario, post-translational modifications (PTMs) on DPCs play essential and versatile roles in orchestrating the repair routes. In this review, we summarize the current knowledge of the mechanisms that trigger DPC removal via PTMs, focusing on ubiquitylation, small ubiquitin-related modifier (SUMO) conjugation (SUMOylation), and poly (ADP-ribosyl)ation (PARylation). We also briefly discuss the current knowledge gaps and emerging hypotheses in the field.

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USP7 and VCPFAF1 define the SUMO/Ubiquitin landscape at the DNA replication fork

Cited by 17 publications

References 70 publications

The p97 segregase cofactor Ubxn7 facilitates replisome disassembly during S-phase

The p97 segregase cofactor Ubxn7 facilitates replisome disassembly during S-phase

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

Targeting DNA-Protein Crosslinks via Post-Translational Modifications

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