Postreplication Repair and PCNA Modification in Schizosaccharomyces pombe

Jonathan Frampton^*^,, Anja Irmisch^*, Catherine M. Green^*, Andrea Neiss^,, Michelle Trickey^*^,||, Helle D. Ulrich^,¶, Kanji Furuya^*, Felicity Z. Watts^*, Antony M. Carr^*, and Alan R. Lehmann^*

*Genome Damage and Stability Centre, University of Sussex, Falmer, Brighton BN1 9RQ, United Kingdom; Max Planck Institute for Terrestrial Microbiology, 35043 Marburg, Germany; and ^¶Clare Hall Laboratories, Cancer Research UK, South Mimms, Herts EN6 3LD, United Kingdom

Submitted November 3, 2005; Revised March 24, 2006; Accepted April 13, 2006
Monitoring Editor: Orna Cohen-Fix

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ubiquitination of proliferating cell nuclear antigen (PCNA)plays a crucial role in regulating replication past DNA damagein eukaryotes, but the detailed mechanisms appear to vary indifferent organisms. We have examined the modification of PCNAin Schizosaccharomyces pombe. We find that, in response to UVirradiation, PCNA is mono- and poly-ubiquitinated in a mannersimilar to that in Saccharomyces cerevisiae. However in undamagedSchizosaccharomyces pombe cells, PCNA is ubiquitinated in Sphase, whereas in S. cerevisiae it is sumoylated. Furthermorewe find that, unlike in S. cerevisiae, mutants defective inubiquitination of PCNA are also sensitive to ionizing radiation,and PCNA is ubiquitinated after exposure of cells to ionizingradiation, in a manner similar to the response to UV-irradiation.We show that PCNA modification and cell cycle checkpoints representtwo independent signals in response to DNA damage. Finally,we unexpectedly find that PCNA is ubiquitinated in responseto DNA damage when cells are arrested in G2.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cellular mechanisms have evolved from prokaryotes to eukaryotesto cope with a wide variety of endogenous and exogenous DNA-damagingagents. They include DNA repair processes, cell cycle checkpoints,and DNA damage tolerance pathways that allow S phase progressionin the presence of replication-blocking lesions.

Schizosaccharomyces pombe is able to remove UV photoproductsby either classical nucleotide excision repair (NER), or analternative repair pathway, utilizing the UVDE protein to inciseclose to the damaged sites (UVER). In addition, DNA damage toleranceor postreplication repair (PRR) pathways are proposed to copewith replication-blocking lesions during S phase, but littlework has been done on PRR in S. pombe.

PRR in the distantly related Saccharomyces cerevisiae has beenwell characterized genetically (Xiao et al., 2000; Ulrich, 2005)and has been divided into two subpathways: translesion synthesis(TLS) and damage avoidance by template switching. In TLS, whenthe replicative DNA polymerase is stalled at a DNA lesion, itis replaced with a specialized TLS polymerase (polymerase switching).Depending on which TLS polymerase is recruited, the lesion isreplicated in either a relatively error-free mode, for example,using DNA polymerase ${eta}$ (pol ${eta}$ ) to bypass UV-induced cyclobutanepyrimidine dimers or an error-prone mechanism using pol ${zeta}$ andRev1. Alternatively, a template switch can occur, during whichthe newly synthesized sister strand is used as the templateto bypass the lesion through a recombination-like event. Thisis thought to be an error-free mechanism.

Two crucial proteins identified by genetic analyses of PRR inS. cerevisiae are Rad6 and Rad18, which have, respectively,E2 ubiquitin-conjugating (Jentsch et al., 1987) and E3 ubiquitinligase activity. The target of their ubiquitinating activitywas recently identified as the proliferating cell nuclear antigen(PCNA), a ring-shaped sliding clamp that interacts with manydifferent proteins involved in DNA replication and repair (Magaand Hubscher, 2003). When replication is blocked by DNA damage,the single-stranded DNA binding protein Rad18 (Bailly et al.,1997) is thought to bind to exposed regions of single-strandedDNA and recruit Rad6 to the stalled replication machinery. Togetherthey mono-ubiquitinate PCNA on lysine 164 (Hoege et al., 2002).This modification of PCNA results in the activation of TLS polymerases(Stelter and Ulrich, 2003). A similar process in human cellsresults in the mono-ubiquitination of PCNA, and this modificationincreases its affinity for the TLS DNA polymerase, pol ${eta}$ (Kannoucheet al., 2004; Watanabe et al., 2004; Bienko et al., 2005). Thisprovides an attractive mechanism for switching from replicativeto TLS polymerase at the sites of stalled forks. In S. cerevisiae,after mono-ubiquitination of PCNA, Rad5, a protein-bridgingfactor and putative E3 ubiquitin ligase recruits the heterodimerUbc13/Mms2, an E2 ubiquitin-conjugating enzyme (Hofmann andPickart, 1999), to the site of damage through its interactionswith Rad18 (Ulrich and Jentsch, 2000). Rad5 and Ubc13/Mms2 togetherpoly-ubiquitinate PCNA (Hoege et al., 2002) in a noncanonicallysine-63 ubiquitin chain-linked manner (Hofmann and Pickart,1999). Poly-ubiquitinated PCNA is proposed to control the template-switchingevent in PRR. To date, poly-ubiquitination of PCNA has not beenreported in human fibroblasts (Kannouche et al., 2004; Watanabeet al., 2004).

In S. cerevisiae, small ubiquitin-like modifier (SUMO) can alsobe attached to PCNA at lysines 127 and 164 mediated by Ubc9and Siz1, which are a SUMO conjugating E2 and a SUMO E3 ligase,respectively (Hoege et al., 2002; Stelter and Ulrich, 2003).This modification occurs in untreated proliferating cells duringS phase (Hoege et al., 2002) and has been shown to recruit theSrs2 helicase, which helps prevent inappropriate recombinationduring S phase (Papouli et al., 2005; Pfander et al., 2005).

In this study we have investigated genetic and molecular aspectsof PRR in S. pombe. We show that, as in S. cerevisiae, S. pombePCNA is both mono- and poly-ubiquitinated after exposure ofcells to a variety of DNA damaging agents, and these ubiquitinationreactions use the same gene products in the two organisms. However,unlike in S. cerevisiae, cycles of PCNA ubiquitination and de-ubiquitinationoccur during S phases of undamaged cells. We also report thatPCNA ubiquitination is not dependent on the DNA-damage checkpointand that it is induced by ionizing radiation as well as UV.Contrary to currently accepted paradigms, we also find thatPCNA is ubiquitinated in response to DNA damage not only inS phase, but also in cells in G2.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
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Construction of Plasmids
ubc13 was amplified using PCR from cDNA and cloned into pGEX-4T-3(Amersham) using BamHI and XhoI to produce an N-terminal GST-fusion.mms2 was amplified using PCR from cDNA, cloned into PGEM-T Easy(Promega, Southampton, United Kingdom) and then subcloned usingPstI/SpeI into pTYB12 (New England Biolabs, Hitchin, UnitedKingdom). This produces Mms2 fused at its N-terminus to a chitin-bindingdomain (CBD), linked by the self-cleavable VMA1 intein sequence,which allows single-step purification of Mms2 bearing threeadditional amino acids at its N-terminus.

Preparation of Proteins
Recombinant proteins were produced in Escherichia coli Rosetta-gamiB (RGB) cells (Novagen, Madison, WI). The cells were inducedwith 0.4 mM IPTG (isopropyl- $beta$ -D-thiogalactopyranoside) and harvestedafter 16 h of induction at 20°C. Purifications were achievedin a single step by affinity chromatography on the appropriatecolumns (glutathione sepharose [Amersham, Arlington Heights,IL] or chitin beads [New England Biolabs] for GST-Ubc13 or CBD-intein-Mms2,respectively) according to the manufacturers’ recommendations.Purified proteins were dialyzed against 25 mM Tris-HCl, pH 7.5,50 mM NaCl, 0.5 mM EDTA, 10% (vol/vol) glycerol and stored frozenat –80°C.

Ubiquitin Conjugation Assays
Ubiquitin chain synthesis assays contained 5 µM each ofrecombinant Ubc13 and Mms2 using conditions described previously(Ulrich, 2003). Ubiquitin mutants, no lysine (K0), lysine 63to arginine (K63R), lysine 63 only (K63 only), and lysine 48only (K48 only) were purchased from Boston Biochem (Cambridge,MA). Purified S. cerevisiae Ubc13 and Mms2 have been describedpreviously (Ulrich, 2003) and were used at the same concentrationsas the S. pombe proteins.

Strain Constructions
mms2::kanMX6 and ubc13::natMX6 were transformed into cell strain501 (ura4-D18 leu1-32 ade6-704 h^–) as previously described(Bahler et al., 1998; Hentges et al., 2005). The strains wereverified by PCR and Southern blot analysis. Standard proceduresand media were used for propagation and genetic manipulations(Moreno et al., 1991).

The pcn1-K164R mutation was generated as follows: the K164Rmutation was introduced into the pcn1 coding sequence usingsite-directed mutagenesis. This was then cloned 5' to the ura4gene. The mutant sequence was amplified by PCR using 100-basepair primers corresponding to 80 base pairs of the pcn1 5'UTR+ 20-base pair pcn1 coding sequence (5' primer) and to 80 basepairs of the pcn1 3'UTR + 20-base pair ura4 (3' primer). ThePCR product was then transformed into wild-type cells and integrationat the correct locus was confirmed by colony PCR and Southernblotting.

Other strains used in this study are listed in Table 1.

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Table 1. S. pombe strains used in this study

Survival Analysis
For UV irradiation, cells were grown to midlog phase at 30°Cin yeast extract peptone (YEP), plated on yeast extract (YE)plates, and irradiated using a 254-nm UV-C lamp with a fluencerate of 0.5 Jm^–2 s^–1. For ionizing radiation (IR)survivals, exponentially growing cells were ${gamma}$ -irradiated in YEPfrom a ¹³⁷Cs source (dose rate, 8.5 Gy min^–1) before platingon YE plates. Percentage survival was scored as the number ofcolonies on the YE plates after 4 d of incubation at 30°C,relative to that on unirradiated control plates. Each graphis the average of three or more independent experiments. The10% survival rate (D10) was estimated using a line of regressionagainst the survival curve using Microsoft Excel (Redmond, WA).

PCNA Modification and Detection
For UV-treatment, a total of 10 A₅₉₅ of midlog phase cells weregrown at 30°C in YEP and transferred onto PVDF membranes(Millipore, Bedford, MA; 0.45 µM) using a vacuum pump.The membranes were irradiated with 50 Jm^–2 UV-C (254 nm),or left as untreated controls. The cells were resuspended inYEP and incubated at 30°C for 30 min. For other treatments,a total of 10 A₅₉₅ of midlog phase cells were grown at 30°Cin YEP, and camptothecin (CPT), methyl-methanesulfonate (MMS),or hydroxyurea (HU) was added to a final concentration of 30µM, 0.9 mM (0.01%), or 50 mM, respectively, and incubationcontinued for 3 h at 30°C. Cells were pelleted and washedin water, and the total protein was extracted in 20% trichloraceticacid (TCA) using a ribolyser, before being resuspended in Laemmlibuffer. The lysates were fractionated by SDS-PAGE, transferredto a PVDF membrane, and immunoblotted using affinity-purifiedanti-PCNA antibodies, generated in-house against full-lengthPCNA. To verify that the modified species of PCNA were ubiquitinated,cells were transfected with the vector pMHRep41 expressing ubiquitinN-terminally tagged with two myc-peptide and six histidine epitopes.Transfected cells in midlogarithmic phase were incubated with50 mM HU for 3 h. Cells, 10⁹, were resuspended in 400 µllysis buffer containing 20 mM Tris-HCl, pH 7.5, 40 mM NaCl,2 mM MgCl_2, 8 U/ml benzonase, protease, and phosphatase inhibitors,and 10% glycerol. Cells were lysed using a ribolyser, NaCl wasadded to 0.5 M and SDS to 2%, and the lysates were incubatedfor 15 min at room temperature. After centrifugation at 13,000rpm for 10 min the extracts were frozen in liquid nitrogen.On thawing, they were diluted 20-fold in phosphate-bufferedsaline containing 300 mM extra NaCl, protease inhibitors, 0.1%NP40 and incubated with 40 µl nickel-agarose beads at4°C for 90 min. The beads were washed three times and thenboiled in Laemmli buffer before analysis by SDS-PAGE and immunoblotting.

Cell Cycle Synchronization by Elutriation
Approximately 2 x 10⁹ G2 phase cells were sorted from a midlogphase culture in YEP containing 4 x 10¹⁰ cells by centrifugalelutriation in a Beckman Model J6 M/E elutriator (Fullerton,CA). The G2 phase cells were then incubated at 30°C, and2 x 10⁸ cells were removed every 20 min for a total of 240 min.Two samples of 1 x 10⁸ cells were filtered onto PVDF membranes(Millipore) using a vacuum pump. One membrane was UVC-irradiatedwith 100 Jm^–2, and the other was left untreated. Bothmembranes were transferred to 100 ml YEP and incubated at 30°Cfor 30 min, the cells were then TCA extracted, and extractswere immunoblotted using anti-PCNA antibodies. For each sample,the septation index was examined using 4,6-diamidino-2-phenylindole(DAPI) and calcofluor staining both before UV-C treatment andafter the subsequent 30-min incubation period.

Cell Cycle Synchronization Using a Temperature-sensitive cdc25 Mutant
The temperature-sensitive mutant cdc25.22 arrests in G2 at therestrictive temperature (36°C). A 250-ml cdc25.22 culturewas grown for 18 h at 25°C until midlog phase and the temperaturewas raised to 36°C for 3 h. Elongation of the cells waschecked microscopically to ensure that they were arrested inG2. Cells, 2 x 10⁸, were either treated with 50 µM 4-nitroquinoline(4NQO) or 50 mM HU for 1 h at 36°C or transferred to a PVDFmembrane (Millipore), UV-irradiated with 100 Jm^–2, andincubated for 30 min in YEP at 36°C. The cells were keptat 36°C throughout the experiment. After treatment cellswere TCA extracted and analyzed by immunoblotting using rabbitanti-PCNA antibodies.

Chk1 Activation
Cultures of exponentially growing wild-type, pcn1-K164R, andrad9-T412A (Furuya et al., 2004) cells, each containing an integratedsingle copy of HA-tagged chk1 (Walworth and Bernards, 1996),were split into two; one-half were exposed to 100 Jm^–2UV radiation, and the other remaining unirradiated. Cells werethen incubated for 30 min in YEP at 30°C. TCA extracts wereanalyzed by immunoblotting with anti-HA antibodies.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ubiquitination Activity of Ubc13/Mms2
In S. cerevisiae, after DNA damaging treatments, PCNA is mono-ubiquitinatedby the combined actions of Rad6 and Rad18 and poly-ubiquitinatedby Mms2-Ubc13 and Rad5. The S. pombe orthologues of Rad6 (Rhp6;Reynolds et al., 1990), Rad18 (Rhp18; Verkade et al., 2001)and Rad5 (Rad8; Doe et al., 1993) have been characterized insome detail in previous work from this and other laboratories.S. pombe homologues of Ubc13 and Mms2 were recently identifiedby Brown et al. (2002). We cloned these genes and expressedthe proteins in E. coli to analyze their activities in vitro.S. cerevisiae Ubc13/Mms2 heterodimer functions in vitro as aubiquitin E2-conjugating enzyme forming noncanonical lysine-63linked ubiquitin chains. We have analyzed recombinant S. pombeUbc13 and Mms2 using a ubiquitin conjugation assay (Figure 1A).When ubiquitin and an E1 enzyme were incubated with recombinantMms2 and Ubc13, ubiquitin chains were formed (Figure 1A, lanes2 and 3). These chains were dependent on Mms2 (lanes 10–12)and Ubc13 (lanes 13–15). We also used mutant ubiquitinin which all the lysines were mutated to arginine (lanes 4–6),only K63 was mutated (lanes 7–9), all the lysines exceptK63 were mutated (lanes 16–18), and all but K48 were mutated(lanes 19–21). Only the protein in which K63 was intact(lanes 16–18) supported the formation of polyubiquitinchains, indicating that the polyubiquitination was mediatedby K63 linkage.

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Figure 1. In vitro ubiquitination reactions. (A) Ubiquitination reactions were carried out with E1, recombinant S. pombe Ubc13 and Mms2 and either wild-type or lysine mutants of ubiquitin, and reactions were incubated for 0, 2, or 4 h, as indicated. Reaction products were analyzed by immunoblotting with anti-ubiquitin antibody (note that the apparently anomalous migration in lanes 4–6 resulted from a bubble during transfer and was not reproduced in other experiments). (B) Cross-species interactions of Ubc13 and Mms2 from S. pombe (S.p.) and S. cerevisiae (S.c.). Reactions carried out as in A. Ub, Ub₂, Ub₃, Ub₄: mono-, di-, tri-, and tetra-ubiquitin.

We also showed that S. pombe Ubc13 and Mms2 could function withthe orthologues of their partner proteins from S. cerevisiae(Figure 1B). Both S. pombe Ubc13 together with S. cerevisiaeMms2 (lanes 7–9) and S. pombe Mms2 together with S. cerevisiaeUbc13 (lanes 10–12) were able to catalyze the formationof ubiquitin chains. These data not only demonstrate conservationbetween S. cerevisiae and S. pombe but also strongly imply thatS. pombe Ubc13/Mms2 has a similar mechanism and activity toits S. cerevisiae counterpart.

Modification of PCNA after Treatment with DNA-damaging Agents
We next investigated the modification of PCNA in S. pombe inresponse to DNA damage. In untreated asynchronous S. pombe cultureswe detected both an unmodified and a modified form of PCNA (Figure 2A).The $~$ 8-kDa shift in mobility of the modified band is that expectedfor monoubiquitinated PCNA. After treatment with a variety ofDNA-damaging agents, UV irradiation, CPT, MMS, or HU, more slowlymigrating species of PCNA were observed. The mobilities of thesebands correspond to those expected of polyubiquitinated PCNAspecies. To confirm that the slow migrating bands did indeedrepresent ubiquitinated species of PCNA, we transfected cellswith a plasmid expressing ubiquitin N-terminally tagged withtwo copies of the myc peptide and six histidine residues. Weused wild-type cells and pcn1-K164R mutants in which lysine164 of PCNA is mutated to arginine. After treatment with orwithout HU, cell extracts in SDS buffer were diluted and incubatedwith nickel-agarose beads. Proteins bound to the beads wereanalyzed by SDS-PAGE and immunoblotted with anti-PCNA antibody(Figure 2B). Species of reduced mobility relative to unmodifiedPCNA were observed in wild-type cells transfected with myc-his-ubiquitin(lane 3), and further bands were detected after HU treatment(lane 4). These bands were dependent on K164 (see lanes 7 and8) and on transfection with the tagged ubiquitin construct (seelanes 1, 2, 5, and 6), confirming that they were indeed PCNAubiquitinated exclusively on K164 (note that the Myc₂His₆ epitopetag on the ubiquitin significantly reduces the mobility of theubiquitinated PCNA species). Therefore in S. pombe, the mono-and poly-ubiquitination of PCNA on K164 in response to DNA damageappears to be similar to that in S. cerevisiae.

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Figure 2. Ubiquitination of PCNA in S. pombe in response to DNA damage. (A) Exponentially growing cultures of S. pombe were exposed to 50 Jm^–2 UV and incubated for 30 min or to 30 µM camptothecin (CPT), 0.9 mM MMS, or 50 mM HU for 3 h. The cells were then lysed and analyzed for PCNA modification using anti-PCNA antibody. Ub, Ub₂, Ub₃: mono-, di-, and triubiquitinated PCNA. (B) Cells were transfected with pMHRep41 either as empty vector or expressing Myc₂His₆-tagged ubiquitin and then incubated with or without HU for 3 h. SDS lysates were incubated with Ni-agarose beads, and the bound proteins were analyzed with anti-PCNA antibody. MHUb₁, MHUb₂: PCNA modified with one or two myc-his–tagged ubiquitins. The asterisk represents a nonspecific cross-reacting band. Note that a small amount of unmodified PCNA (<1% of the total PCNA) bound nonspecifically to the beads in all lanes. (C) The indicated mutants were either untreated (–) or exposed to 50 Jm^–2 UV-irradiation (+) and incubated for 30 min before harvesting and analysis as in A. Mono-, di-, and triubiquitinated PCNA bands are indicated with arrowheads. The fainter bands are nonspecific cross-reacting species.

We examined the role of different genes on PCNA modificationafter UV treatment using various deletion strains of the S.pombe orthologues of genes known to be involved in PCNA ubiquitinationin S. cerevisiae. These were (S. cerevisiae orthologues in superscriptwhen nomenclature differs) rhp18^RAD18, rad8^RAD5, mms2, and ubc13,as well as the point mutant pcn1-K164R (Figure 2C). In the pcn1-K164Rand rhp18^rad18 ${Delta}$ mutants (lanes 2 and 3), modification of PCNAwas totally abolished. In contrast, in rad8^rad5, ubc13, andmms2 deletion strains, there was a strong band of the size equivalentto mono-ubiquitinated PCNA, whereas potential poly-ubiquitinatedspecies were no longer detected (lanes 4–6). Similar resultswere obtained after exposure of the same set of mutant strainsto camptothecin (unpublished data).

We carried out epistasis analysis after UV-irradiation of mutantsin genes involved in PCNA ubiquitination. We found that mms2was epistatic with ubc13, rhp18^RAD18 and rad8^RAD5, which isconsistent with the biochemical data (Figure 3A–C). Doublemutants were no more sensitive than the single mutants. Likewisepcn1-K164R, in which PCNA cannot be ubiquitinated, was epistaticwith rhp18^RAD18, rad8^RAD5, and mms2 (Figure 3, D–F, summarizedin Table 2). This suggests that all these genes operate in thesame pathway. We note that the sensitivities of rad8 ${Delta}$ , mms2 ${Delta}$ ,and ubc13 ${Delta}$ were lower than those of rhp18 ${Delta}$ and pcn1-K164R, consistentwith the former group being deficient only in polyubiquitination,whereas the latter are deficient in both mono and polyubiquitinationof PCNA.

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Figure 3. Epistasis analysis. (A–C) UV survival curves of single and double mutants of mms2 ${Delta}$ with (A) ubc13 ${Delta}$ , (B) rhp18 ${Delta}$ , and (C) rad8 ${Delta}$ . (D–F) UV survival curves of single and double mutants of pcn1-K164R with (D) rhp18 ${Delta}$ , (E) rad8 ${Delta}$ , and (F) mms2 ${Delta}$ . Means ± SEM of three experiments are shown. Double mutants are indicated with a bold line.

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Table 2. Sensitivity to UV-irradiation of different single and double mutants

The results described above demonstrate that PCNA modificationin response to DNA damage in S. pombe is similar to that inS. cerevisiae and has the same genetic requirements.

PCNA Modification and Cell Cycle Checkpoints Respond Independently to DNA Damage
We next addressed the question of whether PCNA ubiquitinationis dependent on an intact DNA-damage checkpoint and vice versa.We examined the ubiquitination of PCNA in a series of strainsdeficient in the DNA-damage checkpoint. The Rad3^Mec1 and Tel1checkpoint kinases control all DNA-damage checkpoints (Carr,2002). However PCNA modification after UV-irradiation in rad3 ${Delta}$ ,tel1 ${Delta}$ , and rad3 ${Delta}$ tel1 ${Delta}$ mutants was similar to that in wild-typecells (Figure 4A). Note that the levels of di- and triubiquitinationvaried between experiments, and we do not consider the apparentincreased levels in the double mutant to be significant. Theimportant conclusion is that PCNA modification is not dependenton an intact DNA-damage checkpoint pathway. To determine ifthe DNA-damage checkpoint is itself dependent on PCNA modification,we have analyzed the phosphorylation of the downstream checkpointtarget, Chk1, in the pcn1-K164R mutant after UV-irradiation.The phosphorylation of Chk1 in pcn1-K164R cells was indistinguishablefrom that of wild-type cells (Figure 4B, lanes 2 and 4). Incontrast, Chk1 phosphorylation was substantially reduced inthe known checkpoint mutant rad9-T412A (Furuya et al., 2004;lane 6). Thus the DNA-damage checkpoint response is not dependenton PCNA ubiquitination. Consistent with these findings, geneticanalysis shows that pcn1-K164R is not epistatic with the DNA-damagecheckpoint gene, rad3 (Figure 4C). Similarly mms2 is not epistaticwith rad3, cds1^RAD53, or chk1 (summarized in Table 2).

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Figure 4. PCNA ubiquitination and cell cycle checkpoints are independent responses. (A) Checkpoint mutants were UV-irradiated (50 Jm^–2) and analyzed for PCNA ubiquitination. Arrowheads indicate ubiquitinated species. (B) Chk1 is activated in pcn1-K164R after exposure to UV. Cultures of exponentially growing wild-type, pcn1-K164R and rad9-T412A cells, both containing an integrated single copy of HA-tagged chk1, were exposed to 100 Jm^–2 UV radiation and then incubated for 30 min. Total cell extracts were analyzed by Western blotting with anti-HA antibodies. Arrowheads indicate activated Chk1. (C) UV survival curves of single and double mutants of pcn1-K164R with rad3 ${Delta}$ .

These results show that ubiquitination of PCNA and activationof the DNA-damage checkpoint are two independent signaling mechanismstriggered by DNA damage.

PRR and Ionizing Radiation
The PRR pathways provide the cell with mechanisms to toleratelesions in DNA during replication. The biologically importantlesions generated in DNA by ionizing radiation are strand breaks,which are thought to inhibit DNA replication by the intra–Sphase checkpoint–dependent arrest of initiation, ratherthan by blocking fork progression. Consistent with this idea,in S. cerevisiae pol30-K164R, mms2 ${Delta}$ , and ubc13 ${Delta}$ are not sensitiveto IR (Xiao et al., 1999; Chen et al., 2005). rad5 ${Delta}$ and rad18 ${Delta}$ mutants are sensitive to IR (Lawrence, 1982; Ahne et al., 1997;Xiao et al., 1999; Chen et al., 2005), but recent data haveshown that this can be attributed to functions of these geneswhich are not involved in ubiquitination of PCNA (Chen et al.,2005).

In striking contrast, we find a novel role in S. pombe for genesinvolved in PCNA ubiquitination after ionizing radiation. Inhuman cells, PCNA is not modified after IR (Kannouche et al.,2004). However, in S. pombe we find that PCNA is modified afterIR (Figure 5A). The pattern of ubiquitination is very similarto that found for UV-irradiated cells (Figure 2), with mono-ubiquitinationdependent on Rhp18 and poly-ubiquitination dependent on Rad8,Ubc13, and Mms2 (Figure 5A). We find that the survival responsesof PRR mutants to IR are strikingly similar to their responsesto UV, which is consistent with this observation. mms2 ${Delta}$ and ubc13 ${Delta}$ are sensitive to IR and are epistatic to each other (Figure 5B)and to rhp18 ${Delta}$ and rad8 ${Delta}$ (Figure 5, C and D). Furthermore, we foundthat pcn1-K164R is also sensitive to IR and is epistatic torhp18, rad8, mms2, and ubc13 (Table 3). We also show that, afterIR treatment, mms2 is not epistatic to genes involved in thecheckpoint pathway, rad3, cds1, and chk1, or in recombinationrepair, rhp54^RAD54 (Table 3).

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Figure 5. PCNA ubiquitination in response to ionizing radiation. (A) The indicated mutants were exposed to 500 Gy ionizing radiation and incubated for 1 h. PCNA modification was analyzed in whole cell extracts by immunoblotting. Arrowheads indicate ubiquitinated PCNA bands; note that in this experiment there was a strongly cross-reacting nonspecific band in all samples, indicated with an asterisk (*). (B–D) IR survival curves of single and double mutants of mms2 ${Delta}$ with (B) ubc13 ${Delta}$ , (C) rhp18 ${Delta}$ , and (D) rad8 ${Delta}$ . (E and F) UV and IR survival curves, respectively, of single and double mutants of pcn1-K164R with rhp51 ${Delta}$ . Double mutants indicated with bold lines.

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Table 3. IR sensitivity of various single and double mutants

rhp51 and PRR
It has been proposed in S. cerevisiae that poly-ubiquitinationof PCNA signals for a recombination-dependent template switchmechanism. If this process involves strand invasion mediatedby RAD51, double mutants of genes involved in PRR and recombinationmight be epistatic. In S. pombe, double mutants of rhp51 ${Delta}$ (theortholog of RAD51) with rhp18 ${Delta}$ , rad8 ${Delta}$ , mms2 ${Delta}$ , or ubc13 ${Delta}$ all resultedin slow growth phenotypes. The cells were elongated and hadsevere growth defects and low plating efficiencies (unpublisheddata). rhp51 ${Delta}$ cells are moderately sensitive to UV-irradiation.Strikingly, the double mutants of rhp51 ${Delta}$ with pcn1-K164R (Figure 5E)and rad8 ${Delta}$ or mms2 ${Delta}$ (Table 2) were exquisitely sensitive to UV-irradiation.Synergistic interactions between UBC13 or RAD18 and recombinationrepair genes have also been found recently in S. cerevisiaeafter treatment with 4-NQO (Papouli et al., 2005

) and in theability of S. cerevisiae to replicate a plasmid containing closelyspaced 6–4 photoproducts on each strand (Zhang and Lawrence,2005

). rhp51 ${Delta}$ cells are very sensitive to IR. Nevertheless thedouble mutants are even more sensitive (Figure 5F and Table 3).

PCNA Is Ubiquitinated during S Phase in Undamaged Cells
In early experiments, we noted that a significant proportionof PCNA was modified by monoubiquitination in undamaged cells(e.g., see Figure 2, A and C, lanes 1). To determine if thismodification in undamaged cells was confined to a particularphase of the cell cycle, we synchronized cells in G2 using elutriationand analyzed whether PCNA was modified in S. pombe during thecell cycle. Cell cycle progression was monitored by measuringthe mitotic and septation indices (Figure 6B). Septation occursin early S phase in S. pombe. We observed bands of mono-, di-,and triubiquitinated PCNA specifically during S phase (Figure 6A).To see if this fluctuation in levels of ubiquitinated PCNA speciescould be correlated with corresponding levels of the proteinsinvolved in poly-ubiquitination of PCNA, we measured the levelsof Rhp18, Mms2, and Ubc13 in the same extracts. No significantchanges in the levels of these proteins were detected (unpublisheddata).

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Figure 6. PCNA ubiquitination through the cell cycle. Cells synchronized by elutriation were either mock-irradiated (A) or UV-irradiated (50 Jm^–2; C) at different times after reinoculation and then incubated for 30 min. PCNA modification was analyzed by immunoblotting of whole cell extracts. (B) Cell cycle position was analyzed by microscopic measurement of mitotic index and septation index 30 min after UV-irradiation (UV-treated) or mock treatment (untreated). Note that septation occurs in early S phase in S. pombe.

In S. cerevisiae, PCNA is sumoylated rather than ubiquitinatedduring S phase (Hoege et al., 2002

). Sumoylated PCNA interactsphysically with Srs2, and this recruitment of Srs2 preventsunwanted recombination during S phase. Furthermore, in S. cerevisiae,the DNA-damage sensitivity of mutants in the PRR pathway issuppressed by deletion of the SRS2 gene. In the absence of PRR,recombination-mediated back-up pathways are called into play,but they are inhibited by Srs2. Deletion of SRS2 enables thesepathways to function, resulting in increased resistance to DNAdamage (Papouli et al., 2005

; Pfander et al., 2005

). Howeverwe did not detect any sumoylated PCNA in the experiment of Figure 5A,nor did we find any suppression of the UV sensitivity of S.pombe mms2 ${Delta}$ by deleting srs2 (Table 2). Instead, the genes appearto be epistatic.

PCNA Is Ubiquitinated in Response to DNA Damage in G2
The currently accepted model for ubiquitination of PCNA in responseto DNA damage is that it is triggered by stalling of the replicationmachinery at sites of DNA damage. Mono-ubiquitination is thoughtto mediate the switch from replicative to translesion polymerases,whereas polyubiquitination channels lesions into an error-freedamage avoidance pathway (Hoege et al., 2002; Stelter and Ulrich,2003). It is implicit in this model that ubiquitination of PCNAin response to damage is an S phase–specific process.To test this prediction, we examined PCNA ubiquitination insynchronized cells at different stages of the cell cycle. Atdifferent times after synchronization by elutriation, sampleswere UV-irradiated and incubated for a further 30 min beforeharvesting and analysis for PCNA ubiquitination. Cell cycleprogression as monitored by septation and mitotic index is presentedin Figure 6B. PCNA ubiquitination data are shown in Figure 6,A (unirradiated) and C (irradiated). Modified PCNA species arepresent in highest amounts in S phase cells (Figure 6, A andC, lanes 3–5 and 10–12), but a strong band correspondingto mono-ubiquitinated PCNA is detected in irradiated cells atall time points. Note in particular that samples 1, 7, and 13contained no detectable S phase cells either at the time ofUV-irradiation or at the time of harvesting. These data suggestthat PCNA is, unexpectedly, ubiquitinated in response to DNAdamage even in non-S phase cells.

To confirm these observations, we made use of the temperature-sensitivecdc25.22 mutant, which is blocked in G2 at the restrictive temperature(Nurse et al., 1976). Cells were held at the restrictive temperaturefor 3 h, at which time all of the cells were elongated, showingthat they were indeed arrested in G2. These cells were exposedto HU, 4NQO, or UV, incubated for a further 30 min, and comparedwith asynchronous cells subjected to the identical treatments.Results are shown in Figure 7A. In asynchronous cells, all threetreatments resulted in ubiquitination of PCNA (lanes 2–4).In the G2-arrested cells, HU treatment, which does not damageDNA but inhibits DNA replication by depleting the deoxyribonucleotidepool, did not result in PCNA ubiquitination (lane 6). In contrastin cells treated with 4NQO (lane 7) or UV (lane 8), clear bandscorresponding to mono-, di-, and triubiquitinated PCNA weredetected. As expected, no modifications were seen in the rhp18 ${Delta}$ or pcn1-K164R strains and only mono-ubiquitination in rad8 ${Delta}$ andmms2 ${Delta}$ strains (unpublished data). These data demonstrate thatPCNA is modified in response to DNA damage in G2 cells.

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Figure 7. PCNA ubiquitination in G2. (A) cdc25.22 cells were maintained either at 25°C (asynchronous) or 36°C (G2) for 3 h. Cells were then treated with either 50 mM HU or 50 µM 4NQO for 1 h or UV-irradiated (100 Jm^–2) and incubated for 60 min. (B) cdc25.22 rad13 ${Delta}$ uve1 ${Delta}$ or cdc25.22 rad3 ${Delta}$ tel1 ${Delta}$ triple mutants were treated at as in A. In all cases PCNA modification was analyzed by immunoblotting of whole cell extracts.

We next tested whether this G2 response was triggered by intermediatesin NER or the alternative repair pathway mediated by the UVDEdamage–specific endonuclease. We isolated a rad13^rad2 ${Delta}$ uvde ${Delta}$ cdc25.22 triple mutant strain, which is defective in boththe NER and UVER pathways. We have previously shown that nophotoproducts are removed in rad13 ${Delta}$ uvde ${Delta}$ strains (Yonemasu etal., 1997

). When the triple mutant was held at the restrictivetemperature for 3 h, exposed to 4NQO or UV, and incubated fora further 30 min, the ubiquitination of PCNA was similar tothat in the repair-proficient strain (Figure 7B). We also createda rad3 ${Delta}$ tel1 ${Delta}$ cdc25.22 triple mutant strain that is completelydefective in DNA-damage checkpoint signaling. The level of PCNAubiquitination at the restrictive temperature was similar tothat in the cdc25.22 single mutant. We conclude that PCNA ubiquitinationin G2 is not dependent either on generation of a repair intermediateor on checkpoint activation.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In S. cerevisiae, PCNA is sumoylated at K127 and K164 duringS phase in undamaged cells. After treatment with MMS, PCNA becomesboth mono- and poly-ubiquitinated at K164 (Hoege et al., 2002).In transformed human fibroblasts, we have detected mono-ubiquitinationof PCNA at K164 after UV-irradiation and a variety of DNA-damagingagents, but we have not detected either poly-ubiquitinationor sumoylation (Kannouche et al., 2004 and unpublished observations).In Xenopus laevis, PCNA is mono-ubiquitinated and sumoylatedduring S phase and becomes di-ubiquitinated in response to DNAdamage (Leach and Michael, 2005). In S. pombe we have now foundthat we can easily detect both mono- and poly-ubiquitinationat K164, but we do not detect sumoylation under the same conditions.There thus appear to be differences in PCNA modifications betweenorganisms. The genetic requirements for mono- and poly-ubiquitinationof PCNA in S. pombe are similar to those in S. cerevisiae, namelythat mono-ubiquitination requires Rhp18^Rad18, whereas poly-ubiquitinationrequires Rad8^Rad5, Ubc13, and Mms2. Our data obtained with UV-irradiationof asynchronous cells are consistent with current models forPRR in which blockage of the replication fork at a UV-inducedphotoproduct results in ubiquitination of PCNA. Mono-ubiquitinationhas been shown to increase the affinity of (human) PCNA forpol ${eta}$ and provides a mechanism for switching from replicativeto TLS polymerase (Kannouche et al., 2004; Bienko et al., 2005).Genetic analysis in S. cerevisiae suggests that poly-ubiquitinationchannels damage into error-free damage avoidance pathways (Hoegeet al., 2002). The importance of PCNA ubiquitination is demonstratedby the UV sensitivities of pcn1-K164R, rhp18^rad18 ${Delta}$ ^, rad8^rad5 ${Delta}$ ^,ubc13 ${Delta}$ and mms2 ${Delta}$ . pcn1-K164R and rhp18 ${Delta}$ are deficient in both mono-and poly-ubiquitination and more sensitive than rad8^rad5 ${Delta}$ ^, ubc13 ${Delta}$ and mms2 ${Delta}$ , which are deficient only in poly-ubiquitination. Theseresponses are quite similar to those of the orthologous mutantsin S. cerevisiae (Xiao et al., 2000; Ulrich, 2005). Howeverthere are some minor differences, which relate to the relativeimportance of sumoylation of PCNA in the two organisms. Forexample in S. cerevisiae rad18 ${Delta}$ is considerably more sensitivethan rad30-K164R, but this excess sensitivity is suppressedin the double mutant (Hoege et al., 2002; Papouli et al., 2005).This is related to sumoylation of PCNA in S. cerevisiae, whichstimulates Srs2-mediated inhibition of recombination-mediatedrepair. In the K164R mutant, sumoylation is greatly reduced,so that recombination repair can rescue some of the structuresnormally repaired via TLS. As mentioned above, sumoylation ofPCNA is difficult to detect in S. pombe. Furthermore, the C-terminal138 aa of S. cerevisiae Srs2, shown to mediate the interactionwith sumoylated PCNA (Pfander et al., 2005), are not conservedin the S. pombe ortholog. These observations are consistentwith PCNA sumoylation playing only a minor or no role in S.pombe. There are at least two possible explanations for thisdifference between the two organisms. Sumoylation in S. cerevisiaerecruits Srs2, which suppresses recombination (Papouli et al.,2005; Pfander et al., 2005). Either polyubiquitination in S.pombe somehow takes over the function of sumoylation in S. cerevisiaeor the recombination system in S. pombe may be less active duringS phase than in S. cerevisiae, and it may not be necessary tohave a mechanism to suppress it.

After treatment of cells with DNA-damaging agents, cell cyclecheckpoints are triggered via the activation of Rad3^Mec1 and/orTel1 protein kinases (Carr, 2002). Deletion of either or bothof these genes had no effect on PCNA ubiquitination, and converselycheckpoint activation remained intact in the pcn1-K164R mutant.These data demonstrate that PCNA ubiquitination and checkpointactivation are independent signaling responses, both of whichcan be triggered by stalling of replication forks.

We have found both mono- and poly-ubiquitination of PCNA inS phase S. pombe cells. It is formally possible that this modificationmay arise because of spontaneously stalled replication forks.The intensity of the bands in S phase compared with those seenin stressed asynchronous cells would argue that such pausingmust be relatively prevalent. Irrespective of the nature ofthe trigger for ubiquitination during S phase, PCNA modificationunder such circumstances seems to have limited biological significancebecause there are no major biological effects of abolishingPCNA modifications in growing cells. The proliferation ratesof pcn1-K164R mutant cells, as well as those of rhp18 ${Delta}$ , mms2 ${Delta}$ and ubc13 ${Delta}$ , are similar to that of wild-type cells.

Our working hypothesis to account for these data is that inresponse to single-stranded DNA and/or some other distortionat a stalled replication fork, PCNA is ubiquitinated. If theubiquitination results from DNA damage blocking the replicationmachinery, the increased affinity of mono-ubiquitinated PCNAfor pol ${eta}$ and possibly also for other TLS polymerases will bringabout a polymerase switch and facilitate bypass of the lesion(Kannouche and Lehmann, 2004; Kannouche et al., 2004). In thecase of blocking of the replication fork by HU or stalling atnatural pause sites during unhindered replication, PCNA ubiquitinationwill be activated. However, TLS polymerases are not able toovercome the block caused by HU-induced deoxyribonucleotidedepletion, and there is no reason to suppose that they mightbe able to overcome natural pause sites. Consequently, cellsdeleted in the PCNA ubiquitination genes as well as the pcn1-K164Rmutant proliferate normally, and the pcn1-K164R mutant has normalsensitivity to HU (unpublished data).

A further difference between S. pombe and S. cerevisiae is inthe ubiquitination of PCNA after IR treatment. In S. pombe PCNAis ubiquitinated after IR treatment, and this ubiquitinationmakes an important contribution to cell survival, whereas inS. cerevisiae PCNA modification does not appear to play a significantrole in the response to IR (Xiao et al., 1999; Chen et al.,2005). IR produces single- and double-strand breaks in DNA aswell as different types of base lesions. The major effect ofstrand breaks on DNA replication is to inhibit initiations viathe intra-S checkpoint, rather than to block progression offorks. Indeed double-strand breaks induced by EcoRI in the genomeof S. cerevisiae did not result in ubiquitination of PCNA (Chenet al., 2005). It is possible, therefore, that base lesions,the helical distortion they cause, and/or intermediates in theirrepair result in modification of PCNA.

We have found a large synergistic interaction between rhp51and PRR genes after UV treatment. We interpret these data tosuggest that, after UV-induced DNA damage, S. pombe requiresPCNA polyubiquitination to stabilize a stalled replication fork.If this is inhibited, the replication machinery may collapseand can only be restored by Rhp51-mediated recombination. Inthe absence of both mechanisms, a UV photoproduct in the DNAis likely to be fatal during S phase.

Our most unexpected finding is that PCNA is ubiquitinated afterDNA damage in cells held in G2. This did not appear to be triggeredby repair intermediates because it was also seen in cells completelydeficient in repair of photoproducts. This suggests that itis either the DNA structure generated by the lesions themselvesthat triggers ubiquitination of PCNA or some other effect ofthe damage that is not dependent on DNA replication. One possiblecandidate might be transcription complexes stalled at sitesof damage, though there is no evidence for any involvement ofPCNA in transcription. Our finding of ubiquitination of PCNAin G2 after UV and 4NQO treatments may provide an alternativeexplanation for our observations that PCNA is also ubiquitinatedfollowing treatment with IR.

In conclusion, our studies on S. pombe have revealed that therole of PCNA ubiquitination in the response to DNA damage mightbe more complex than has been envisaged previously. Our resultshave opened up new avenues of research for understanding thefunctions of PCNA modification.

ACKNOWLEDGMENTS

This work was supported in part by Medical Research CouncilProgramme Grants to A.M.C. and A.R.L.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E05-11-1008)on April 26, 2006.

Present addresses: AbCam, Cambridge Science Park, Milton Road,Cambridge, United Kingdom;

^|| Marie Curie Institute, The Chart, Oxted, Surrey RH8 0TL,United Kingdom;

Heidelberg University Biochemistry Centre, 69120 Heidelberg,Germany.

Address correspondence to: Alan R. Lehmann ( a.r.lehmann{at}sussex.ac.uk)

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