Erratum: Chromatin-associated degradation is defined by UBXN-3/FAF1 to safeguard DNA replication fork progression

Nature Communications 7: Article number: 10612 (2016); Published: 4 February 2016; Updated: 17 May 2016. This Article contains errors in the labelling of Fig. 5 and Supplementary Fig. 6, the former of which was introduced during the production process. In Fig. 5b, an ‘x’ indicating the presence of UBXN-3(SGG)-HIS in lane 6 was inadvertently omitted.

D uplication of the genomic information is a key task for dividing cells. The intricacy of DNA replication is reflected by the plethora of regulatory factors that promote different steps of DNA synthesis 1 . The assembly of DNA replication factors into specialized subcomplexes is tightly controlled to ensure genome stability. Accordingly, misregulation of DNA replication generates fatal consequences, resulting in inefficient DNA synthesis and chromosomal damage, which ultimately cause tumorigenesis or stem-cell depletion [2][3][4][5][6] .
The licensing factor CDT-1 (chromatin and DNA licensing factor 1) initiates the formation of a pre-replication complex (pre-RC) at replication origins once per cell cycle 7,8 . Assembled pre-RCs represent origins that are approved for DNA replication. However, pre-RCs remain passive until their activation during S phase 9,10 . Upon transition into DNA synthesis, the replication activation factors (cell division cycle protein 45) CDC-45 and the Go-Ichi-Nii-San (GINS) complex associate with pre-RCs 11,12 . GINS binding facilitates the recruitment of further replication factors including the DNA polymerases, which triggers the elongation phase of DNA replication 13,14 . A central factor that coordinates the described licensing and elongation events is CDC-48/p97 (Cdc48p in yeast, CDC-48 in nematodes, p97 or (Valosin containing protein) in mammals), VCP a ubiquitinselective ATPase. Importantly, our recent findings identified that CDC-48 links ubiquitin-dependent degradation of CDT-1 to the release of the CDC-45/GINS complex in Caenorhabditis elegans 15,16 . Depletion of CDC-48 or its heterodimeric cofactor UFD-1/NPL-4 (ubiquitin fusion degradation protein 1, nuclear protein localization 4) results in stabilization of CDT-1 exclusively on mitotic chromatin. In addition, CDC-45 and the GINS subunit SLD-5 (synthetic lethal with dpb11-1 protein 5) persist on chromatin, becoming visible after S phase is completed upon CDC-48 UFD-1/NPL-4 inactivation. Thus, CDC-48 coordinates chromatin association of different protein complexes with replication fork progression. Consequently, inhibition of CDC-48 results in severe S-phase progression defects, due to activation of the DNA replication checkpoint 15,16 . Work in Xenopus laevis and human cells identified a related requirement for CDT-1/Cdt1 mobilization and turnover, emphasizing a crucial function of CDC-48/p97 in eukaryotic DNA replication 16,17 .
CDC-48/p97 is a key component of the ubiquitin/proteasome system, important for mobilization and targeting of ubiquitylated substrates for degradation by the 26S proteasome 18 . Interestingly, it regulates diverse cellular processes such as degradation of proteins associated with the endoplasmic reticulum (ERassociated degradation, ERAD) or mitochondria (mitochondriaassociated degradation, MAD), cell-cycle progression and lysosomal proteolysis 18,19 . Recently, CDC-48/p97 emerges as a central regulator of chromatin-associated degradation (CAD), which is relevant to genome stability and human genetic disorders including cancer and accelerated aging [20][21][22][23] . With the increasing number of CDC-48/p97 substrate proteins, it is becoming evident that additional regulatory mechanisms specifying substrate selection at a given time need to be identified. Especially, the cell-cycle-dependent coordination of distinct events during DNA replication necessitates precise spatial and temporal regulation of CDC-48 function at the chromatin 16,[22][23][24][25] .
To address how CDC-48-dependent DNA replication is adjusted with substrate recruitment and cell-cycle progression, we screened for genetic interactors of cdc-48 in C. elegans. Using an RNA interference (RNAi)-based approach, we identified UBXN-3 (ubiquitin regulatory X (UBX) domain-containing protein in nematodes 3) as a crucial factor that coordinates CDC-48-dependent DNA replication events. Embryos with reduced protein levels of both UBXN-3 and CDC-48 recapitulate phenotypes caused by complete depletion of CDC-48, including the accumulation of CDT-1 and GINS on mitotic chromatin. UBXN-3 binds to CDT-1, thus facilitating CDC-48 recruitment for substrate turnover and disassembly at the chromatin. Consequently, depletion of the human homologue FAS-associated factor 1 (FAF1) results in stabilization of CDT-1 protein, pronounced decrease in replication fork velocity, increased number of stalled forks, and newly fired origins, cumulating in the activation of the DNA damage response. In conclusion, our results demonstrate an evolutionarily conserved role of UBXN-3/ FAF1 in orchestrating CAD of DNA replication factors to safeguard genome integrity, which is relevant to the emerging link between FAF1 deletion and cancer development 26 (and references therein).

Results
Embryonic survival depends on UBXN-3 function. The ubiquitin-selective segregase CDC-48/p97 is a key regulator of numerous protein degradation pathways within eukaryotic cells 18,19 . Besides substrate turnover in different cellular compartments, we and others identified a central role of CDC-48/p97 in DNA metabolic pathways that safeguard genome stability [20][21][22][23] . This complexity of degradation pathways demands mechanisms that accurately coordinate CDC-48/p97 activity. To identify factors that provide substrate specificity and spatiotemporal regulation of CDC-48 during DNA replication, we performed an RNAi-based candidate screen targeting potential interactors ( Fig. 1a; Supplementary Table 1). A set of 137 RNAi clones was used for depletion of 95 genes, followed by microscopic evaluation of developmental phenotypes and cellcycle progression defects (Fig. 1a,d; Supplementary Table 1). In addition to wild-type (wt) nematodes, downregulation of candidate genes was also performed in viable cdc-48.1(tm544) deletion mutants, representing a sensitized background with a reduction of 80% in total CDC-48 protein levels in embryos (Fig. 1b,c). The remaining 20% of CDC-48 protein are encoded by the cdc-48.2 gene, which provides its essential function under untreated conditions. In fact, the screen identified several genes required for development and viability when depleted in the wt or the cdc-48.1(tm544) mutant (Supplementary Fig. 1e; Supplementary Table 1).
Functional analysis of the ubxn-3(tm6658) deletion mutant further supports our observation that UBXN-3 is required for embryonic survival, particularly when DNA replication is  (Fig. 2d). In addition, significant HU sensitivity was also observed upon ubxn-3 knockdown by RNAi ( Supplementary Fig. 2c). Strikingly, germline-specific expression of mCherry::UBXN-3 restores the basal 30% embryonic lethality of the ubxn-3(tm6658) allele ( Fig. 2b-d). Furthermore, transgenic expression of UBXN-3 in the ubxn-3(tm6658) deletion background complements sensitivity towards npl-4(RNAi) as well as HU (Fig. 2b,d). To provide additional evidence for DNA replication defects, we assessed the accumulation of RAD-51 recombinase on DNA. Similar to embryos lacking UFD-1/NPL-4, codepletion of UBXN-3 and CDC-48.1 resulted in formation of characteristic RAD-51 foci, indicating the formation of DNA double-strand breaks upon replication fork collapse 31,32 ( Fig. 3a; Supplementary Fig. 3a). Besides embryonic defects, HU treatment of young adult worms depleted for UBXN-3 resulted in reduced lifespan, implicating genome instability and premature aging (Fig. 2e). In conclusion, UBXN-3 is critical for embryonic development and compensation of DNA replication stress. CDC-48 function is required for protein degradation in distinct cellular compartments, such as the unfolded protein response in the ER or mitochondria. The expression levels of HSP-4 or HSP-6 chaperones directly monitor defects in degradation of misfolded proteins accumulating in the ER lumen or at mitochondria 33,34 . Importantly, neither HSP-4 nor HSP-6 expression were induced after ubxn-3(RNAi) ( Supplementary Fig. 2a,b). In conclusion, UBXN-3 provides a highly specific role in DNA metabolism.

CDC-48 UBXN-3 governs chromatin-bound replication factors.
Our recent findings identified that CDC-48 works together with the canonical cofactor UFD-1/NPL-4 in degradation and disassembly of chromatin-associated DNA replication factors 16,17 . Consequently, inactivation of the CDC-48 UFD-1/NPL-4 complex causes increased levels of the DNA licensing factor CDT-1 on mitotic chromosomes as well as persistent chromatin association of CDC-45 and SLD-5, a subunit of the tetrameric GINS complex 16 ( Fig. 3b,c,e; Supplementary Fig. 3b,c). In embryonic cell cycles, the loading of DNA replication licensing factors is initiated when cells  are morphologically engaged in mitosis 35 . Consequently, we use the description mitotic CDT-1 stabilization to clearly discriminate between these early licensing events and apparently distinct CDT-1 regulatory mechanisms at later stages 16 . Given the identification of ubxn-3 as a genetic interactor of cdc-48 and npl-4 important for DNA replication and genome stability, we next addressed whether UBXN-3 is involved in the regulation of these CDC-48 targets. Strikingly, depletion of UBXN-3 in the cdc-48.1(tm544) mutant resulted in elevated levels of CDT-1 on mitotic chromatin as revealed by immunostaining (Fig. 3b). In contrast, ubxn-1 or ubxn-2 (RNAi) did not interfere with CDT-1 regulation in the absence of CDC-48.1 ( Fig. 3b; Supplementary Fig. 3b). During unperturbed cell divisions, localization of the replisome components CDC-45 and GINS is restricted to S-phase nuclei 12 These findings suggest that UBXN-3 cooperates with CDC-48 in DNA replication, including degradation of CDT-1 and disassembly of CDC-45/GINS at the chromatin. Consequently, UBXN-3 depletion provokes DNA replication stress, which is reflected by delayed cell-cycle progression due to activation of the intra-S-phase checkpoint.

UBXN-3 and CDC-48 form a functional complex in the nucleus.
Given its functional relevance in DNA replication, we tested whether UBXN-3 is physically linked to chromatin. Indeed, cellular fractionation of C. elegans embryonic lysates confirmed high abundance of UBXN-3, CDC-48 and CDT-1 in purified nuclei (Fig. 4a). Upon disruption of DNA polymers by sonication chromatin-associated proteins relocalized into the soluble nuclear fraction, implicating that UBXN-3 and CDC-48 are associated with the chromatin similar to CDT-1 (Fig. 4a).
UBXN-3 binds to CDC-48-dependent substrate proteins. UBXN-3 belongs to a subclass of cofactors that share the UBX domain as a characteristic CDC-48-binding motif 38,39 . Besides the UBX domain, UBXN-3 harbours a coiled coil (CC) motif, a ubiquitin-associated domain (UBA) and a UAS domain of unknown function 40 (Fig. 5a). Furthermore, the mammalian ortholog FAF1 contains two ubiquitin-like (UBL) domains. To address the requirement of the different domains, we established an in vitro binding assay using purified full-length or truncated variants of UBXN-3 (Fig. 5a). Moreover, the conserved FPK/R motif in the UBX domain was point mutated to analyse CDC-48 interaction 41 ( Fig. 5a; Supplementary Fig. 5a). His-tagged UBXN-3 proteins were coupled to Ni-NTA agarose and incubated with whole-worm lysate. Associated proteins were subsequently eluted with 8 M urea buffer followed by elution of His-tagged proteins in Laemmli buffer ( Fig. 5a; Supplementary Fig. 5b). Importantly, full-length UBXN-3 co-purified with CDC-48 and CDT-1 (Fig. 5b,c), thus confirming the in vivo results shown in Fig. 4. In contrast, a truncated version lacking the UBX and CC domain did not interact with CDC-48, however, was still able to bind CDT-1 and ubiquitin conjugates (Fig. 5b). Conversely, a fragment only consisting of the UBX and CC domain exclusively interacted with CDC-48, indicating that CDC-48 alone is not sufficient for CDT-1 binding (Fig. 5b). Remarkably, point mutations of the FPK motif in the UBX domain were completely impaired in CDC-48 interaction 41 ; however, fully functional in CDT-1 and ubiquitin-conjugate binding ( Fig. 5b; Supplementary Fig. 5a). The interaction with CDT-1 and CDC-48 was not markedly reduced upon npl-4(RNAi), suggesting that the substrate-binding capacity of UBXN-3 is independent of the UFD-1/NPL-4 cofactor ( Fig. 5c; Supplementary Fig. 5c).
These interaction studies provide evidence that UBXN-3 binds the replication factor CDT-1 and other ubiquitylated substrate proteins. Intriguingly, substrate binding occurs independently of CDC-48, suggesting a direct role for UBXN-3 in substrate recruitment.
FAF1 is the homologue of UBXN-3 essential for DNA replication. UBXN-3 is highly conserved in metazoans and its human ortholog is termed FAF1. Notably, various FAF1 mutations have been linked to cancer development; however, a mechanistic role in maintenance of genome stability has not been demonstrated. Therefore, we addressed whether FAF1 is also required to coordinate DNA replication in human cells. In fact, depletion of FAF1 by siRNA resulted in robust activation of the intra-S-phase checkpoint kinases ATR and CHK-1 (Fig. 6a). Moreover, FAF1 depletion caused induction of the DNA damage response, reflected by phosphorylation of ATM and CHK2 DNA repair kinases, as well as histone H2AX (Supplementary Fig. 6a). These observations implicate a conserved functional role of UBXN-3/FAF1 in DNA replication (Figs 2,3 and 6).
To directly assess the role of FAF1 in DNA replication, we analysed the dynamics of individual replication forks by DNA fibre assays. To this end, human osteosarcoma (U2OS), urinary bladder cancer (T24) or kidney embryonic (HEK293) cells were successively pulse labelled with the nucleoside analogues 5-chloro-2 0 -deoxyuridine (CldU) and 5-iodo-2 0 -deoxyuridine (IdU), respectively, and progression of discrete replisomes was visualized by anti-CldU and anti-IdU immunofluorescence (Fig. 6b). Ongoing replication forks are labelled as tracks that contain CldU (red) followed by IdU (green), and measurement of the length of CldU/IdU tracks allows the analysis of replication fork velocity (Fig. 6b). Notably, the analysis of DNA tract length and fork velocity is exclusively based on measurement of symmetric tracts, displaying no statistical differences in the lengths of respective CldU-and IdU-single tracts 22 . In addition, this method enables visualization of stalled replication forks (CldU incorporation only) and firing of dormant origins (IdU incorporation only) as well as fork termination events (Fig. 6b). Strikingly, FAF1 depletion by different siRNAs causes pronounced DNA replication stress phenotypes in several human cell lines (Fig. 6c-i; Supplementary Fig. 6b-h). Quantification of tract lengths indicates severely defective DNA replication fork progression (Fig. 6e,g; Supplementary Fig. 6d,g), accompanied with high rates of replication fork stalling (Fig. 6h), excessive firing of dormant origins (Fig. 6i) and activation of replication stress checkpoint signalling (Fig. 6a). Notably, defects in replication fork progression upon FAF1 depletion can be completely restored upon expression of siRNA-resistant HA-FAF1 ( Supplementary Fig. 6f-h), precluding any off-target effects. To exclude that the detected replication defects are secondary to inherited chromosomal aberrations or checkpoint activation of a previous cell cycle, these experiments were repeated using G0/G1-arrested T24 cells, which did not proliferate during siRNA treatment. After T24 cells were released into S phase, we monitored DNA replication forks by DNA fibre assays. In fact, several independent FAF1 siRNAs recapitulated fork progression defects similar to U2OS and HEK293 cells, reflecting direct problems in DNA synthesis during early steps of chromosomal replication (Fig. 6c-e). Although an individual depletion of either FAF1 or CDT-1 causes severe replication problems, simultaneous depletion of FAF1 together with CDT-1 clearly suppressed impaired fork dynamics (Fig. 6f-i). This finding implicates that the regulation of CDT-1 protein levels is the primary role of FAF1 during DNA   16 .
To show that CDT-1 is a substrate of FAF1 in human cells, we performed co-IP experiments using HA-FAF1 as bait. Nuclear lysates were prepared from HEK cells expressing the p97-E587Q substrate trap variant 42 . In fact, HA-FAF1 co-purifies together with CDT-1 and p97 (Fig. 6j). To validate that FAF1 indeed determines CDT-1 turnover, we analysed protein levels in cycloheximide (CHX)-chase experiments. Strikingly, CHX treatment demonstrates that depletion of FAF1 attenuates CDT-1 degradation, resulting in stabilized protein levels (Fig. 6k). This suggests that UBXN-3/FAF1 recognizes CDT-1 as a substrate to promote p97-dependent proteasomal targeting (Fig. 7a). In summary, FAF1 plays a conserved role in DNA duplication and ensures genome stability.

Discussion
Research during the past two decades led to the discovery of prominent cellular pathways regulated by the ubiquitin-selective ATPase CDC-48/p97 (refs 18,19). Obviously, the increasing number of substrate proteins demands highly selective recruitment mechanisms. Given the recently discovered role of CDC-48/p97 in DNA replication, we were especially interested how CAD is coordinated to guarantee efficient DNA synthesis. As DNA replication is a fundamental cellular process that ensures the faithful propagation of the genomic information in each cell division cycle, our results are relevant to human genetic disorders including oncogenesis and premature aging syndromes 22 .
Using a genetic screening approach, we succeeded in finding a conserved UBX domain protein that provides a substrate selection module, triggering CDC-48/p97-dependent degradation at the chromatin. UBXN-3/FAF1 binds both the licensing factor CDT-1 and CDC-48/p97, and thus safeguards the timely regulation of target recognition at the replication fork. Replication stress emerging upon UBXN-3/FAF1 depletion provokes replication fork collapse and occurrence of genotoxic DNA breaks, activating the replication checkpoint and formation of DNA repair foci. Thus, our findings suggest that UBXN-3/FAF1 is a specific mediator of CAD, especially in the context of DNA replication since it is not essential for CDC-48/p97-mediated unfolded protein response pathways in the ER or mitochondria.
The detailed analysis of DNA replication factors indeed revealed a crucial role of UBXN-3/FAF1 in the regulation of chromatin-loaded CDT-1, as well as chromatin association of CDC-45 and the GINS complex. Analysis of DNA fibre assays highlights the severe consequences of UBXN-3/FAF1 depletion on the DNA replication programme at single-origin resolution ( Fig. 6; Supplementary Fig. 6). Depletion of UBXN-3/FAF1 markedly perturbs progression of replication forks, accompanied by increased numbers of stalled forks and newly fired dormant origins. Notably, this DNA replication defect can be suppressed by codepletion of CDT-1, which thus appears to be a conserved key substrate of UBXN-3/FAF1. Indeed, CHX-chase experiments show that UBXN-3/FAF1 depletion attenuates CDT-1 turnover resulting in stabilized protein levels. Importantly, our binding studies demonstrate that UBXN-3/FAF1 directly interacts with CDT-1 and other ubiquitylated substrates independent of CDC-48 and the UFD-1/NPL-4 cofactor. In accordance with this idea, UBXN-3/FAF1 is localized within the nucleus and associated with chromatin. Together, these data identify UBXN-3/FAF1 as a CDC-48/p97 adaptor and potent mediator of CAD at eukaryotic replisomes (Fig. 7a).
UBXN-3/FAF1 is a member of the UBX family of CDC-48/p97 cofactors, which were proposed to provide substrate specificity 38 . However, only few UBX proteins were convincingly shown to target CDC-48/p97 to compartment-specific degradation pathways. In yeast, Ubx2 and Ubx3 mediate ER-associated degradation or non-proteolytic pathways, respectively [43][44][45][46] . Ubx4    and Ubx5 as well as the mammalian ortholog UBXN7 are involved in the cellular response to ultraviolet (UV) light-induced DNA damage 42,47 . In mammalian cells UBX proteins are implicated in cellular functions as diverse as membrane fusion 48 , endolysosomal sorting 49 , lipid metabolism 50 or ciliogenesis 51 . In C. elegans, the functional relevance of UBX proteins is scarcely defined. UBXN-2 is implicated in mitosis, by regulating centrosomal composition 52 . Whereas UBXN-3 joins with UBXN-1 and UBXN-2 in nematode gametogenesis, downregulation of the latter two UBX proteins does not affect DNA replication 30 . Similar to CDC-48 and its cofactor UFD-1/NPL-4, UBXN-3 is localized inside the nucleus during S phase, which is consistent with a role during DNA synthesis. Moreover, cellular fractionation implicates UBXN-3 as well as CDC-48 to be chromatin-associated (Fig. 4a). Deletion of ubxn-3 does not affect the integrity of the CDC-48 UFD-1/NPL-4 complex, excluding indirect effects on DNA synthesis. Conversely, the presence of CDC-48, UFD-1 and NPL-4 appears to be important for the correct nuclear localization of UBXN-3. This study implicates that UBXN-3/FAF1 determines selection of CDC-48/p97 substrates in the nucleus (Fig. 7a). Specifically, UBXN-3/FAF1 facilitates degradation or disassembly of the licensing factor CDT-1 and the GINS complex during DNA synthesis. Interestingly, two recent publications revealed that CDC-48/p97 is required for the release of the MCM helicase together with CDC-45 and GINS (collectively called CMG complex) from chromatin at termination sites of DNA replication 24,25 . Thus, the UBXN-3/FAF1-dependent regulation of CDC-45/GINS might be triggered by MCM-7 ubiquitylation and CMG disassembly. However, the localization of functional GFP fusions of MCM-2, MCM-3 as well as MCM-7 was not affected upon UFD-1 or NPL-4 depletion, in contrast to the CMG components CDC-45 and SLD-5 ( Supplementary Figs 7b and  3c,d) 16,35 . As CMG release requires active DNA synthesis 24,25 , delayed disassembly of CMG complexes might also result from perturbed origin firing patterns. The observation that FAF1 depletion causes inefficient DNA synthesis in several human cell lines, which can be restored upon CDT-1 codepletion strongly argues for defects in DNA replication licensing, which unlikely originate from aberrant fork termination. Attenuated disassembly of CMG complexes at termination sites would be expected to result in increased fork termination events. Conversely, analysis of DNA fibres in FAF1-depleted cells revealed a twofold decrease in fork termination frequency ( Supplementary Fig. 6e), thus unlikely reflecting a primary role of FAF1 in resolving terminated replication forks in metazoans. In support of this, depletion of two topoisomerase-II orthologs top-2 and cin-4 does not result in elevated CDT-1 levels on mitotic chromatin ( Supplementary  Fig. 7a), thus excluding secondary effects of aberrant replication termination 53 . Importantly, fork stalling and firing of dormant origins are consequences of ATR/CHK-1 checkpoint activation 54 , illustrating occurrence of severe DNA replication stress in FAF1-depleted cells. Although control of CDT-1 activity is the primary mechanism of DNA replication regulation by UBXN-3/ FAF1, adjustment of other replication factors might contribute to avoid replication stress. Besides CDT-1, our data show that UBXN-3/FAF1 binds additional ubiquitin conjugates (Fig. 5b,c). Generally, UBXN-3/FAF1 appears to be associated with the chromatin (Fig. 4a). Therefore, UBXN-3/FAF1 presumably acts on several substrates during DNA replication, causing pleiotropic defects on fork progression when absent. This study and our previous work show that codepletion of either CDT-1 or CDC-45/GINS together with UFD-1/NPL-4 is able to suppress checkpoint activation 16 and fork progression defects, supporting the idea that different CDC-48/p97 substrates are targeted throughout the DNA replication programme. Thus, we propose that UBXN-3/FAF1 cooperates with CDC-48/p97 at distinct time points during DNA replication.
Recently, mutations in the CDC-48/p97-associated protease SPRTN (also called DVC1 or C1orf124) were shown to be directly linked to accelerated aging and cancer susceptibility 22,23 . Likewise, aberrations in FAF1 gene expression were identified in cancer patients, however, the causative mechanisms remained unclear [55][56][57][58][59] (and references in Menges et al. 26 ). This study identifies an unexpected role of UBXN-3/FAF1 in faithful DNA duplication and genome integrity. Since chronic replication stress is known to generate chromosomal alterations associated with cancer as well as reduced proliferative capacity of stem cells 5,60-62 , FAF1 misregulation might be linked to oncogenesis and accelerated aging through genome instability. Besides DNA replication, its role in apoptosis and NF-kB signalling further emphasizes that FAF1 represents a potent target for chemotherapy and human genetic studies 26 .
The transgenic lines hhIs149 and hhIs177 were generated for this study. Briefly, ubxn-3 cDNA was cloned into the pAZCherry(N) 63 , whereas mcm-7 cDNA was cloned into the pIC26 expression vectors, respectively 64 . The transgenes were delivered and integrated into the C. elegans genome by particle bombardment 65 .
RNAi. RNAi-mediated depletion was achieved using the feeding method 66 . RNAi bacteria were fed either to L1 larvae or starting at the L3/L4 larval stage at 15°C, until adulthood was reached. dsRNA production was induced with 2 mM Isopropyl-b-D-thiogalactopyranoside (IPTG) (unless otherwise stated) added to the growth media. RNAi constructs were either obtained from the Ahringer or  ORFeome WS112 libraries (Geneservice Ltd, available via Source BioScience, UK, catalogue nos. 3318 and 3320); for depletion of pcn-1 the respective cDNAs was subcloned into the pPD129.36 feeding vector. The empty feeding vector was used as control. Depletion of NPL-4 protein levels was achieved by induction of dsRNA corresponding to the npl-4.2a cDNA.
HU sensitivity. HU sensitivity was monitored by growing worms in the presence of different HU concentrations. Worms were transferred to HU-containing medium after reaching the L4 larval stage to avoid developmental effects. Following RNAi and HU treatment until adulthood, five to six adult worms were kept for 5-6 h on nematode growth medium (NGM) plates for egg laying. The following day, hatched progeny and dead embryos were counted to calculate growth defects. Because of a developmental delay, the analysis of ubxn-3(tm6658) mutants was shifted by one day, respectively.
Lifespan analysis. For lifespan assays, worms were synchronized by bleaching in sodium hypochlorite. Eggs were distributed on RNAi plates. For HU treatment, L4 larvae were transferred to HU-containing RNAi plates. In lifespan assays, first day of adulthood was defined as day 1. Worms were grown at 20°C and monitored daily for survival by touch-provoked movement and pharyngeal pumping, until death. Animals that crawled off the plates or died owing to internal hatching of progeny or extruded organs were censored.
Microscopy and image acquisition. For time-lapse microscopy, embryos were extruded from gravid hermaphrodites with the help of injection needles, transferred onto 3% agar pads in M9 buffer before microscopic analysis. An AxioImager.M1/Z1 microscope equipped with an AxioCam MRm camera (Carl Zeiss) was used for image acquisition. Time-lapse recordings in 90-s intervals were acquired using 2 Â 2 mono binning to avoid photo bleaching and toxicity. To allow direct comparison of signal intensities, images were recorded under identical conditions. Analysis of time-lapse recordings was done in the AxioVision 4.7 software. Timing of cell division was estimated as follows: for the estimation of cell division timing distinct cell-cycle stages (nuclear envelope breakdown (NEBD), completion of mitotic furrow ingression (cytokinesis)) where determined morphologically from differential interference contrast (DIC) images. Time intervals in between theses cell-cycle stages were used to calculate the duration of mitosis (time elapsed between NEBD and cytokinesis of one-cell division) and duration of S phase (time elapsed between cytokinesis and NEBD of two subsequent divisions). The P1 delay refers to a combined estimation of the delay in cell-cycle progression of the P1 cell relative to the AB cell. The P1 delay represents the average delay calculated from the time difference between NEBD on one hand and the completion of cytokinesis in the AB and P1 cell on the other hand 27,28 .
Processing of selected pictures was done in Adobe Photoshop CS4. Images of immunostainings were also acquired with AxioImager.M1/Z1 and AxioCam MRm but using full resolution of the camera. Confocal images were acquired using the Yokogawa CSU-X1 spinning disc module mounted to a Nikon Ti-E microscope stand, operated by Volocity software (PerkinElmer). Z-stacks were recorded with 200 nm distances between optical sections and projected into one single image. Microscopy of DNA fibres was done using a Leica DMRB microscope with a DFC360FX camera.
Antibody production. cDNAs encoding cdt-1, npl-4.2 and ubxn-3b were cloned into the pET-21a expression vector (Addgene). Recombinant proteins were expressed in Escherichia coli strain BL21cp (Stratagene) and purified using the Ä KTApurifier system (GE Healthcare) or bench-top method using Ni-NTA agarose (Qiagen). His-tagged purified proteins were used for immunization of rabbits and anti-sera were affinity purified using respective Strep-II-tagged recombinant proteins (BioGenes).
Immunotechniques. Immunostaining of early embryos was done essentially according to the 'freeze-crack' protocol. Gravid worms were dissected onto polylysine-coated slides (Thermo Scientific) and frozen in liquid nitrogen, followed by incubation in methanol at À 20°C for 20 min and in acetone at À 20°C for 20 min. After rehydration in PBS and blocking in 5% BSA, embryos were incubated with primary antibody overnight at 4°C (anti-UBXN- (1:10,000) was done at room temperature, before detection of signals using the Li-Cor Odyssey scanner. Quantification of signal intensities was done using the Odyssey V3.0 software (Li-Cor). The uncropped versions of western blots that have been used to assemble the main figures are collected in Supplementary Fig. 8.
Preparation of worm lysates. Synchronized L1 larvae were kept on control or RNAi plates at 15°C until they reached adulthood. Embryos of gravid worms were collected by bleaching and re-suspended in 2 Â Laemmli buffer. Embryos were sonicated twice for 15 s (Bandelin, Microtip MS 1.5), incubated at 95°C for 5 min, and centrifuged at 14,000g for 5 min before SDS-PAGE analysis. Whole-worm lysates used for subsequent co-IP were prepared as follows: synchronized L1 larvae were grown on NGM-agar plates with OP50 bacteria until they reached adulthood. Worms were collected and washed once in lysis buffer (50 mM Tris (pH 7.2), 50 mM NaCl, 1 mM EDTA and protease inhibitors (Roche)) before shock-freezing in liquid nitrogen. Subsequently, thawed samples were subjected to sonication (four times for 30 s, on ice; 50% power; Sonopuls UW 2200, Bandelin). Samples were centrifuged at 14,000g for 5 min and supernatant subsequently incubated with magnetic Dynabeads Protein A (Novex Life Technologies). Protein concentrations were calculated by extinction at 280 nm using the NanoDrop 8000 (Thermo Scientific).
Cellular fractionation of embryos. Purification of nuclei from embryos was achieved according to published protocols with some modifications 67,68 . Briefly, freshly collected embryos were disrupted in a Wheaton stainless steel homogenizer (7 ml capacity) in nuclear preparation buffer (NPB; 20 mM HEPES, 20 mM KCl, 3 mM MgCl 2 , 2 mM EDTA, 0.5 M sucrose, 1 mM dithiothreitol, 1 mM phenylmethyl sulphonyl fluoride and protease inhibitors (Roche)). Efficient lysis was monitored under the microscope. Cellular debris was collected by three subsequent centrifugation steps at 100g for 1 min at 4°C. Nuclei were collected by centrifugation at 4,000g for 5 min at 4°C. The supernatant contains represents the cytosolic fraction. The nuclei in the pellet were washed twice in detergent buffer (DTB; same as NPB plus 0.25% Igepal, 0.1% Triton X-100) and collected as before at 4,000g centrifugation. After resuspension in one-fourth volume nuclear extraction buffer (NEB; 20 mM HEPES, 350 mM NaCl, 5 mM CaCl 2 , 2 mM EDTA, 25% glycerol, 1 mM dithiothreitol, 1 mM phenylmethyl sulphonyl fluoride and protease inhibitors (Roche)) of the cytosolic fraction, the nuclear fraction was split in two halves. One half was kept on ice while the second half was subjected to sonication (twice for 20 s at 90% power, Bandelin Microtip). Nucleoplasm and chromatin fraction were separated by centrifugation at 20,000g for 10 min at 4°C. Supernatant contains soluble proteins, pellet contains chromatin-associated proteins 69 . After resuspension of the chromatin pellets in NEB all samples were diluted in Laemmli buffer and subjected to sonication (twice for 20 s at 90% power, Bandelin Microtip) before SDS-PAGE analysis.
Protein interaction studies. For co-IP analysis, magnetic Dynabeads Protein A (Novex Life Technologies) were used following the manufacturer's protocol. Dynabeads were mixed with the antibody of choice (10 mg), diluted in 200 ml of PBST (0.01% Tween 20), and crosslinked using BS3 (Thermo Scientific). After crosslinking, worm lysate (1 mg total protein) was added and incubated with the Dynabeads for 30 min at room temperature. After three times washing with washing buffer (50 mM Tris (pH 7.2), 1 mM EDTA, 150 mM NaCl, 10% glycerol and protease inhibitors (Roche)), bound proteins were eluted in Laemmli buffer without b-mercaptoethanol and heated for 10 min at 70°C. b-Mercaptoethanol was added to the eluate just before SDS-PAGE analysis. For analysis of UBXN-3 functional domains, His-tagged proteins were expressed and purified from E. coli using Ni-NTA agarose (Qiagen) and PD10 gel-filtration columns (GE Healthcare). Isolated proteins were snap-frozen in liquid nitrogen and stored at À 80°C. Synchronized adult worms were lysed by sonication (Bandelin Sonopuls) in lysis buffer (50 mM Tris (pH 7), 150 mM NaCl, 0.5 mM EDTA, 5 mM MgCl2, 0.1% Igepal, 15 mM imidazole, protease inhibitors (Roche) and 5 mM iodoacetamide). Proteins coupled to Ni-NTA (50 ml slurry per 1 mg protein) or Ni-NTA agarose alone were incubated with worm lysate (20 Â excess total protein over His-tagged peptides) for 30 min at room temperature. After three times washing with washing buffer (same as lysis buffer with 250 mM NaCl), bound proteins were eluted from agarose beads with elution buffer (50 mM Tris (pH 7), 8 M urea, 100 mM NaH 2 PO 4 and 0.1% Igepal). Remaining proteins were eluted at 95°C in Laemmli buffer.
Co-IP analysis in human cells was achieved via anti-HA agarose beads following the manufacture's protocol. Twenty-four hours before collecting HEK293 cells, expression of the p97-E578Q mutant 42 was induced by doxycycline (1 mg ml À 1 final). In addition, cells were transiently transfected with a plasmid driving the expression of HA-tagged FAF1 or HA as control (pIRESpuro2b vector). HA beads were washed twice in IP buffer (50 mM Tris (pH 8.0), 150 mM NaCl and 0.05% NP-40) and incubated with nuclear lysates for 3 h at 4°C. Nuclear lysates were prepared 69 and after five times washing with IP buffer (supplemented with protease inhibitor cocktail (Roche)) bound proteins were eluted in 2 Â Laemmli buffer (with b-mercaptoethanol) and boiled for 10 min at 95°C.
For preparation of lysates, cells were cultured in 60 or 100 mm dishes and collected 72 h after transfection. Cells were trypsinized, washed with PBS and the cell pellets were re-suspended in lysis buffer (50 mM Tris-HCl (pH 7.5), 120 mM NaCl, 20 mM sodium fluoride, 1 mM EDTA, 6 mM EGTA, 1% Nonidet P-40 and 10% glycerol), and supplemented with protease inhibitor (Roche, complete EDTA free), phosphatase inhibitor (Roche, PhosStop) and N-ethylmaleimide (20 mM). The protein content was estimated using Bio-Rad protein assay reagents. Lysates were resolved in polyacrylamide gels using standard protocols. Membranes were blocked with 5% non-fat dry milk for 1 h with agitation at room temperature. The proteins were detected with respective primary and secondary antibodies and visualized on X-ray film.
To analyse protein CDT-1 turnover, HEK293 cells were grown in DMEM media before addition of CHX (50 mg ml À 1 final concentration). At the selected time points, the cells were collected and cell lysates were prepared as described above, followed by western blot analysis.
DNA fibre assay. Asynchronous U2OS, HEK293 or T24 cells were pulse labelled with 30 mM of CldU (Sigma-Aldrich) for 30 min, washed three times with warm PBS and then 250 mM of IdU (Sigma-Aldrich) pulse were given for an additional 30 min. Labelling of replication forks was terminated by treating the cells with ice-cold PBS. Cells were lysed, and DNA fibres were spread onto glass slides, fixed with methanol and acetic acid, denatured with HCl, blocked with 2% BSA and stained with anti-rat and anti-mouse 5-bromo-2 0 -deoxyuridine (BrdU) that specifically recognize either CldU or IdU. Anti-rat Cy3 (dilution 1:300, Jackson Immuno Research) and anti-mouse Alexa 488 (dilution 1:300, Molecular Probes) were used as the respective secondary antibodies. The analysis of DNA tract length is exclusively based on measurement of symmetric tracts, displaying no statistical differences in the lengths of respective CldU-and IdU-single tracts 22,70 .
Statistical analysis. Statistical analysis was performed using Excel (Microsoft), Prism (GraphPad) and ImageJ software. Statistical significance was calculated with two-tailed paired Student's t-test. Statistical significance of C. elegans lifespan was estimated using the log-rank Mantel-Cox test. Asterisks indicate statistical significances according to common conventions.