Loss of Dna2 fidelity results in decreased Exo1-mediated resection at DNA double-strand breaks

A DNA double-strand break (DSB) is one of the most dangerous types of DNA damage that is repaired largely by homologous recombination or nonhomologous end-joining (NHEJ). The interplay of repair factors at the break directs which pathway is used, and a subset of these factors also function in more mutagenic alternative (alt) repair pathways. Resection is a key event in repair pathway choice and extensive resection, which is a hallmark of homologous recombination, and it is mediated by two nucleases, Exo1 and Dna2. We observed differences in resection and repair outcomes in cells harboring nuclease-dead dna2-1 compared with dna2Δ pif1-m2 that could be attributed to the level of Exo1 recovered at DSBs. Cells harboring dna2-1 showed reduced Exo1 localization, increased NHEJ, and a greater resection defect compared with cells where DNA2 was deleted. Both the resection defect and the increased rate of NHEJ in dna2-1 mutants were reversed upon deletion of KU70 or ectopic expression of Exo1. By contrast, when DNA2 was deleted, Exo1 and Ku70 recovery levels did not change; however, Nej1 increased as did the frequency of alt-end joining/microhomology-mediated end-joining repair. Our findings demonstrate that decreased Exo1 at DSBs contributed to the resection defect in cells expressing inactive Dna2 and highlight the complexity of understanding how functionally redundant factors are regulated in vivo to promote genome stability.

Homologous recombination (HR) and nonhomologous end joining (NHEJ) are the canonical pathways of DNA doublestrand break (DSB) repair.HR is an error-free pathway requiring extensive 5 0 end resection, and NHEJ is an errorprone pathway whereby the ends are joined after minimal processing.DNA resection is the major deciding step between these two pathways (1).However, if resection initiates and HR is not possible, then a more mutagenic alternative (alt) repair pathway can be used as a last resort.Microhomology-mediated end joining (MMEJ) is an alt-end-joining (alt-EJ) pathway that occurs at a high frequency in the absence of yKu70/80 (Ku) or when broken ends are not compatible for direct ligation.MMEJ requires 5 0 resection; however, in contrast to HR, the extent of resection in MMEJ is believed to be coordinated with the process of scanning for microhomology in adjacent regions flanking the DSB.The mechanism remains ill defined; however, the repair product from MMEJ contains a deletion corresponding in size to the fragment between the annealed microhomology sequences, which were revealed during resection.
The first responders to a DSB are Ku and Mre11-Rad50-Xrs2 (MRX), and they are important for recruiting additional NHEJ and HR factors (2)(3)(4)(5)(6).The Ku heterodimer also protects the ends from nucleolytic degradation and aids in the localization of Lif1-Dnl4 and Nej1 (3).Dnl4 ligase completes EJ by ligating the DNA with the help of Lif1 and Nej1 (4,(7)(8)(9).The central role of the MRX complex is to tether the loose DNA ends mainly through the structural features of Rad50 (10,11) and to initiate resection through the nuclease activity of Mre11 (12).Sae2 interacts with the MRX complex and activates Mre11 nuclease activity, which forces Ku dissociation.Ku disengagement at the DSB coincides with the initiation of 5 0 to 3 0 end resection by two long-range resection nucleases, Dna2 in complex with Sgs1 helicase, and Exo1 (12)(13)(14).Dna2 and Exo1 nucleases show functional redundancy as Exo1 drives long-range resection in the absence of Dna2 and vice versa (14).The interplay between repair factors in the two canonical pathways regulates the initiation of resection in part through antagonistic relationships between Ku and Exo1 and between Nej1 and Dna2, wherein Nej1 inhibits interactions of Dna2 with Sgs1 and with Mre11 and Sae2 (5,6,15,16).
Here, we determined that the dominant negative effects of dna2-1 were caused by decreased localization of Exo1, a nuclease functionally redundant with Dna2 in DSB repair.In dna2-1 mutant cells, Ku-dependent NHEJ increased and Exo1dependent 5 0 resection decreased.By contrast, in dna2Δ pif1-m2 mutants, Ku70 and Exo1 recruitment to the break remained indistinguishable from WT, but EJ repair occurred mainly through MMEJ.These results demonstrate that Exo1 recovery is impacted by the physical presence of Dna2 and that the interplay between these two nucleases regulates key events that drive repair pathway choice, including the ratio of NHEJ and MMEJ.

Results
Nuclease-deficient dna2-1 shows abrogated resection at DSB Cells harboring nuclease-dead dna2-1 were more sensitive than dna2Δ pif1-m2 mutants to phleomycin, an agent that causes DNA DSBs, but less sensitive to hydroxyurea, an agent Loss of Dna2 fidelity impacts Exo1-mediated DNA resection inducing replication stress (Fig. 1A, (26,27)).While sensitivities to various genotoxic stressors have been previously reported with dna2 mutants, there has been little work explaining why dna2-1 mutants show greater sensitivity to DSB-causing agents compared with cells harboring the deletion of DNA2 or its binding partner, SGS1 (Figs. 1A and S1).This prompted our side-by-side investigation of dna2Δ pif1-m2 and dna2-1 in DSB repair.Our aims were to evaluate DNA resection, a key early step in HR and then to determine the impact of the dna2 mutations on the functionality of the other DSB repair factors.Dna2 functions in long-range resection and can compensate for Mre11 to initiate resection (14).To this end, resection was determined at two locations, 0.15 and 4.8 kb from the HOinduced DSB using a quantitative PCR (qPCR)-based approach that relies on RsaI as previously described (16,28).Resection produces ssDNA, and if resection goes beyond the RsaI recognition sequence, then the site is not cleaved and can be amplified by PCR (Fig. 1B, loci in blue and purple).Resection at the time points (0-150 min) was similar at both distances from the break in pif1-m2 and WT, indicating that the loss of PIF1 activity did not impact DNA processing at DSB (Fig. 1, C  and D).Furthermore, when we performed chromatin immunoprecipitation (ChIP) at the HO-induced DSB, Dna2 HA levels in pif1-m2 mutants were indistinguishable from WT (Fig. 1E), reinforcing earlier work showing that the disruption of PIF1 did not impact DSB repair (22).Upon deletion of DNA2, resection decreased by approximately twofold, with a slightly greater defect at the distance 4.8 kb from the break (Fig. 1, C and D).A more pronounced defect was observed in dna2-1 mutants as resection was abrogated at both distances (Fig. 1, C and D).Dna2 recovery in dna2-1 mutants was unaltered (Fig. 1E), suggesting that the physical association of this nuclease-dead mutant at the break had a dominant negative impact.
We also observed that dna2-1 mutant cells survived better than dna2Δ pif1-m2 and WT on 2% GAL (Fig. 1A).The genetic background of these cells includes hmlΔ hmrΔ, which prevents HR.Survival on galactose therefore correlates with mutagenic EJ repair, which prevents subsequent HO-cutting as opposed to survival on phleomycin, which creates multiple DSBs throughout the genome that can repair by HR.
To complement the survival assays, we performed an EJ ligation experiment where the DSB was induced with galactose for 2 h before cells were washed and released into glucose to prevent further recutting.At the indicated time points, genomic DNA was prepared, and qPCR was performed with primers spanning the HO recognition site as previously described (Fig. 1B, locus in green; 9).The rate of EJ increased more in dna2-1 compared with dna2Δ pif1-m2 mutants (Fig. 1F).Increased EJ might arise naturally because of decreased HR but could also arise from more NHEJ factors at the DSB in dna2-1 mutants.

NHEJ factors at DSBs in dna2 mutants
Prior to comparing the impact of the dna2 mutants on factors driving resection, we determined the localization of proteins essential for NHEJ.Ku70 recovery at DSB increased in dna2-1 mutant cells but not in dna2Δ pif1-m2 mutants (Fig. 2A).By contrast, the recovery of Nej1 increased significantly in both mutants, with dna2Δ pif1-m2 showing a greater increase (Fig. 2B).These data highlight the antagonistic relationship between Dna2 and Nej1 at DSBs (5).The recovery of the other canonical NHEJ factors, Lif1 and Dnl4, in cells harboring either of the dna2 mutant, was indistinguishable from WT (Fig. S2, A and B).
We wanted to determine whether preventing NHEJ would reverse the resection defect of the dna2 mutants and potentially the dominant negative effect of dna2-1 in HR repair.In addition to their essential function in NHEJ, both Ku70 and Nej1 inhibit resection (Fig. S2E).In alignment with our earlier work, deletion of KU70, but not the other core NHEJ factors, reversed the resection defect in both dna2 mutants (Figs. 2, C and D and S2, C and D; (9)).These data indicate that alleviation of the resection defects by ku70Δ was independent of PIF1 status, which differs between the two dna2 mutants.Correlating with the rescue in resection, deletion of KU70, but not NEJ1, suppressed the phleomycin sensitivities of both dna2Δ pif1-m2 and dna2-1 mutants (Fig. 2E).Altogether, suppressing the dominant negative effect of dna2-1 was specific to the loss of Ku70 rather than disruption of NHEJ by ku70Δ as HR-mediated repair was restored in dna2-1 ku70Δ mutants but not in dna2-1 nej1Δ mutants.
To determine the type of EJ that can proceed in these mutants, we utilized a reporter system containing a URA3 marker flanked by two inverted HO recognition sites (Fig. S2F) (29).If both sites are cleaved simultaneously, noncompatible ends are generated and alt-EJ-MMEJ is used.However, because cutting at both sites is not perfectly coordinated, each single cut can still be repaired by NHEJ as previously described (29).In WT cells, the relative frequency of NHEJ and alt-EJ-MMEJ as determined by growth on -URA was 37% and 63%, respectively (Fig. 2F).Notably, the relative frequencies of NHEJ and MMEJ differed between the two dna2 mutants.The frequency of NHEJ increased to 55% in dna2-1 mutants (Fig. 2F).By contrast, when DNA2 was deleted, alt-EJ-MMEJ was the preferred EJ pathway, which we found surprising given Ku70 was similarly recovered at the break site in dna2Δ pif1-m2 and WT cells (Fig. 2, A and F).Consistent with previous work, upon KU70 deletion, EJ occurred through alt-EJ-MMEJ, and the increased NHEJ seen in dna2-1 mutants was reversed by ku70Δ (Fig. 2F).

Nuclease-deficient dna2-1 suppresses Exo1 recruitment to DSB
To bring further insight to events underlying the dna2-1 phenotype, we next determined the impact of dna2-1 and DNA2 deletion on the localization of other factors important for resection, namely Exo1 nuclease and the nucleaseassociated factors, Sae2 and Sgs1.The recovery of Sgs1 and Sae2 was not altered in either mutant background (Fig. S3, A  and B).By contrast, Exo1 was significantly reduced in dna2-1 to almost the level of the nontagged control, whereas its recovery in dna2Δ pif1-m2 was like WT (Fig. 3A).These data Loss of Dna2 fidelity impacts Exo1-mediated DNA resection indicate that Exo1 localization was inhibited by the presence of nuclease-deficient Dna2 at the break rather than the intrinsic loss of Dna2 nuclease activity.
We next compared resection and survival when the dna2 mutants were combined with deletion of EXO1.In line with previous observations, short-range resection (0.15 kb) decreased modestly in exo1Δ single mutant cells (Fig. 3B), but there was an approximately twofold decrease in long-range resection (4.8 kb) 80 to 150 min after DSB induction (Fig. 3C) (14,16).We could not determine resection when Loss of Dna2 fidelity impacts Exo1-mediated DNA resection both nucleases were deleted because of synthetic lethality (SL) (14).However, resection at both distances from the break and phleomycin sensitivity in dna2-1 exo1Δ mutants was indistinguishable from dna2-1 (Fig. 3, B-D).One explanation for the marked decrease in resection in dna2-1 was that expression of this mutant directly blocked the association of Exo1 with DSBs.However, Exo1 was similarly recovered in WT cells, which are DNA2+ PIF1+ and dna2Δ pif1-m2 mutant cells, suggesting neither PIF1 status nor the presence of Dna2 per se directly affected Exo1 recovery.A more plausible model, based on previous work showing Exo1 to be negatively regulated by the presence of Ku (15), is that the pronounced resection defect in dna2-1 mutants resulted from decreased Exo1 because of increased Ku, in addition to the loss of Dna2 nuclease activity.Indeed, upon deletion of KU70, Exo1 recovery increased at the DSB in dna2-1 mutants (Fig. 3E).These data were also consistent with suppression of dna2-1 phleomycin sensitivity by KU70 deletion being Exo1 dependent (Figs.2D and 3D).Resection remained low in dna2-1 exo1Δ ku70Δ triple mutants, as did growth on phleomycin and 2% GAL because both main DSB repair pathways, HR and NHEJ, were disrupted (Fig. 3, D and F).However, alt-EJ-MMEJ was still functional, which could provide some insight as to how a small percentage of triple mutants survived on phleomycin (Figs.3D and S3C).Finally, Exo1 recovery also increased when KU70 was deleted in dna2Δ pif1-m2 (Fig. 3E).These data help explain why the resection defect in dna2Δ pif1-m2 mutants was suppressed by ku70Δ but not by nej1Δ (Fig. 2C), as our earlier work showed the inhibitory effect of Nej1 to be unrelated to Exo1 activity (5,6,9).

Overexpression of Exo1 restores the resection defect in dna2-1 cells
Our data thus far support a model whereby the dominant negative effect of dna2-1 on resection stemmed from increased Ku70 at the DSB, which in turn inhibited Exo1 localization.This was supported by genetic analysis where deletion of KU70 in dna2-1 resulted in increased Exo1 recovery, increased resection, and decreased sensitivity to phleomycin.We next wanted to determine whether increasing the level of Exo1 could rescue the dominant negative effect of dna2-1 mutants.We utilized a 2μ URA3 plasmid encoding Exo1 (pEM-EXO1) that was previously engineered to investigate the inhibition of Exo1 by Ku (15).Of note, expression of Exo1 did not alter Dna2 recovery in WT or dna2-1 mutants (Fig. 4A).Resection at 0.15 kb in dna2-1 + pEM-EXO1 increased to the level seen in dna2Δ pif1-m2 mutants, although resection in both remained lower than WT (Fig. 4B).At the further distance, 4.8 kb from the DSB, Exo1 expression in both dna2 mutants resulted in a greater rescue where resection in dna2-1 + pEM-EXO1 was like WT + empty vector, and resection in both dna2Δ pif1-m2 and WT + pEM-EXO1 was similarly increased (Fig. 4C).Highlighting the link between resection and in vivo DSB repair, phleomycin sensitivity decreased in both dna2 mutants expressing Exo1 most notably in dna2-1 mutants after 3 days of growth (Fig. 4D).Resection and phleomycin sensitivity in pif1-m2 + pEM-EXO1 was indistinguishable from WT (Figs. 4D and S4, A and B).
Finally, we wanted to determine whether ectopic expression of Exo1 in dna2-1 mutants could restore the balance of NHEJ and alt-EJ-MMEJ repair.Again, we utilized the reporter system where NHEJ and alt-EJ-MMEJ were distinguished by growth on -URA media and where cells were transformed with either pRS425-EXO1 for ectopic expression of Exo1 from a 2μ LEU2 plasmid or empty vector (Fig. S2F).Increased NHEJ and the relative frequency of EJ in dna2-1 mutants was reversed upon Exo1 expression (Figs. 2F and 4E).These findings are consistent with short-range resection and decreased Ku promoting EJ by alt-EJ-MMEJ (Fig. 4F).In WT cells, Exo1 expression also decreased the level of Ku recovered at the DSB; however, the frequency of alt-EJ-MMEJ to NHEJ did not change nor did short-range resection (Fig. 4, E and F).

Discussion
We set out to understand why dna2-1 nuclease-dead mutants were more sensitive to DSB-causing agents than dna2Δ mutants.Our results showed that Exo1 localization decreased in cells expressing nuclease-dead Dna2 and that overall resection in dna2-1 was reduced more than in cells where DNA2 or EXO1 were individually deleted.The negative effect of dna2-1 at DSB was caused by Ku-dependent inhibition of Exo1 localization (Fig. 5, A and C).The dna2-1 dominantnegative phenotype was largely overcome by either deleting KU70 or expressing Exo1, as both rescued the resection defect and phleomycin sensitivity.By contrast, neither Exo1 recovery nor Ku70 recovery changed in dna2Δ pif1-m2; however, Nej1 levels markedly increased (Fig. 5B).Our work corroborates previous synthetic genetic array screening where dna2-1 in combination with exo1Δ was viable (30) and suggests that the SL resulting from deletion of both DNA2 and EXO1 stems from something other than a combined loss of nuclease activity, unless dna2-1 has activity in vivo below the level of detection.One possibility is that the pif1-m2 mutation, which is not present in dna2-1, might contribute to the genetic SL interaction as Pif1 and Exo1 were previously shown to coordinate checkpoint signaling at uncapped telomeres (22,31).
The loss of Dna2 nuclease activity by a point mutation had a profound impact on the pathway used in DSB repair, and 5 0 resection was central to the whole process.Ku and Nej1 are negative regulators of resection, and previous work by our laboratory and others showed there to be a division of labor for nuclease inhibition by these NHEJ factors (5,6,8,9,15,16).Nej1 interacts with the binding partners of Dna2, including Mre11, Sae2, and Sgs1 to inhibit Dna2 activity.However, Nej1 does not inhibit Exo1 recruitment.By contrast, Ku binding at DSB directly inhibits the accessibility of Exo1 nuclease to DNA ends, and its recovery at the break site, whereas Dna2 can initiate resection in the presence of Ku (24,25).Thus, the antagonistic relationship between Nej1 and Dna2 is distinct, and independent, from the antagonistic relationship between Ku and Exo1 at DSB.The data presented here highlight a layer of complexity not previously reported in earlier work, where Dna2 fidelity impacts the balance of Ku and Exo1 at the break, a relationship paramount for ensuring DSBs are repaired through the least mutagenic pathway available.
The dna2 mutants impacted EJ differently in the reporter cell line where HR was precluded, a scenario relevant for G1 in the cell cycle.While NHEJ is error prone with the formation of small insertions and deletions, a more harmful outcome arises when resection initiates and more mutagenic alt-EJ-MMEJ proceeds.In dna2-1 mutants, the relative frequency of NHEJ increased and alt-EJ-MMEJ decreased, which was consistent with more Ku recovered at the break.The presence of Ku impacted the type of EJ repair in dna2-1 more than the resection defect.Both dna2-1 exo1Δ and dna2-1 exo1Δ ku70Δ mutants showed similar resection defects, but the increased frequency of NHEJ was Ku dependent (Fig. S3C).On the contrary, there was marked increase in alt-EJ-MMEJ in dna2Δ pif1-m2 mutants, which might have something to do with resection proceeding, albeit at reduced rate, in cells where DNA2 was deleted.However, resection also equally decreased when EXO1 was deleted, and repair occurred predominately through NHEJ (Figs. 3B and S3C).In all, these data might provide insight to the underlying cause of SL resulting from deletion of EXO1 and DNA2, as HR and both EJ pathways would be disrupted.
The EJ observations also suggest that the presence of Ku was not the only regulatory factor determining the type of EJ repair.Rather, our data support a model wherein the frequency of NHEJ to alt-EJ-MMEJ was altered by the relative level of Ku in relation to other repair factors, namely Exo1 and Nej1.Exo1 promoted alt-EJ-MMEJ in the presence of Ku in dna2 mutants, and we observed this under two experimental conditions.First, alt-EJ-MMEJ in dna2-1 mutants increased upon Exo1 expression (Fig. 4E), and second, alt-EJ-MMEJ increased in dna2Δ pif1-m2 mutants, where the level of Nej1 increased, but the levels of Exo1 and Ku70 were unaltered (Figs. 2, A and B and S3C).These phenotypic differences between dna2Δ and dna2-1 indicate the possibility of increased Nej1-dependent alt-EJ-MMEJ repair in dna2Δ cells (32,33).Further work is needed to elucidate whether Nej1 has a role in regulating EJ; however, in support of this model, we recently reported that alt-EJ-MMEJ increased in aging cells as Ku declined, and Nej1 persisted DSBs (34).
Taken together, our data point out the dynamic interplay between Dna2 and Exo1 in DSB repair pathway choice and broaden the understanding of nuclease localization versus nuclease activity in DNA processing at break sites.The characterization of the two dna2 mutants demonstrated that loss of Dna2 nuclease activity through different mutations resulted in different repair outcomes.The work has health relevance, and although DNA2 deletion is embryonic lethal, point mutations are observed in diseases like Seckel syndrome and various kinds of cancer, with the corresponding P504→S mutation of dna2-1 in yeast seen in human cancers (35,36).

Media details
All the yeast strains used in this study are listed in Table S1 with new ones obtained by crosses.The strains were grown on various media in experiments as described.For HO induction of a DSB, YPLG medium is used (1% yeast extract, 2% bacto peptone, 2% lactic acid, 3% glycerol, and 0.05% glucose).For the continuous DSB assay, YPA plates are used (1% yeast extract, 2% bacto peptone, and 0.0025% adenine) supplemented with either 2% glucose or 2% galactose.For the mating type assays, YPAD plates are used (1% yeast extract, 2% bacto peptone, 0.0025% adenine, and 2% dextrose).

ChIP
ChIP assays were performed as previously described (5).Cells were cultured overnight in YPLG at 25 C. Cells were then diluted to equal levels (5 × 10 6 cells/ml) and cultured to one doubling (3-4 h) at 30 C. 2% GAL was added to YPLG, and cells were harvested and crosslinked at various time points using 3.7% formaldehyde solution.Cut efficiencies for all strains are shown in Table S2.Following crosslinking, the cells were washed with ice-cold PBS, and the pellet was stored at −80 C. The pellet was resuspended in lysis buffer (50 mM Hepes [pH 7.5], 1 mM EDTA, 80 mM NaCl, 1% Triton, 1 mM PMSF, and protease inhibitor cocktail), and cells were lysed using Zirconia beads and a bead beater.Chromatin fractionation was performed to enhance the chromatin-bound nuclear fraction by spinning the cell lysate at 13,200 rpm for 15 min and discarding the supernatant.The pellet was resuspended in lysis buffer and sonicated to yield DNA fragments (500 bp in length).The sonicated lysate was then incubated with αHA-, αFLAG-, or αMycantibody-conjugated beads or unconjugated beads (control) for 2 h at 4 C.The beads were washed using wash buffer (100 mM Tris [pH 8], 250 mM LiCl, 150 mM [αHA and αFLAG] or 500 mM [αMyc] NaCl, 0.5% NP-40, 1 mM EDTA, 1 mM PMSF, and protease inhibitor cocktail), and protein-DNA complex was eluted by reverse crosslinking using 1% SDS in TE buffer, followed by proteinase K treatment and DNA isolation via phenol-chloroform-isoamyl alcohol extraction.qPCR was performed using the Applied Biosystem QuantStudio 6 Pro machine.PowerUp SYBR Green Master Mix was used to visualize enrichment at MAT1 (0.15 kb from DSB), and PRE1 was used as an internal control (Table S2).HO cutting was measured in strains used to perform ChIP in Table S3.

Continuous DSB assay and identification of mutations in survivors
Cells were grown overnight in YPLG media at 25 C to saturation.Cells were collected by centrifugation at 2500 rpm for 3 min, and pellets were washed 1× in ddH 2 O and resuspended in ddH 2 O. Cells were counted and spread on YPA plates supplemented with either 2% GLU or 2% GAL.About 1 × 10 3 total cells were plated on glucose, and 1 × 10 5 total cells were plated on galactose.The cells were incubated for 3 to 4 days at room temperature, and colonies were then counted on each plate.Survival was determined by normalizing the number of surviving colonies on the GAL plates to the number of colonies on the GLU plates.About 100 survivors from each strain were scored for the mating type assay as previously described ( 16), and at least 100 survivors were used to make a master plate, which was later replica-plated on -URA plates.The number of survivors on -URA plates was counted to determine the ratio of NHEJ and alt-EJ repair frequencies.

qPCR-based ligation assay
As described previously (9), cells from each strain were grown overnight in 15 ml YPLG to reach an exponentially growing culture of 1 × 10 7 cells/ml.Next, 2.5 ml of the cells were pelleted as "no break" sample, and 2% GAL was added to the remaining cells, to induce a DSB.About 2.5 ml of cells were pelleted after a 3 h incubation as time point 0 sample.After that, GAL was washed off, and the cells were released into YPAD, and respective time point samples were collected.Genomic DNA was purified using standard genomic preparation method by isopropanol precipitation and ethanol washing, and DNA was resuspended in 100 μl ddH 2 O. qPCR was performed using the Applied Biosystem QuantStudio 6 Flex machine.PowerUp SYBR Green Master Mix was used to quantify resection at HO6 (at DSB) locus.The PRE1 locus was used as an internal gene control for normalization.Signals from the HO6/PRE1 time points were normalized to "no break" signals, and % Ligation was determined.The primer sequences are listed in Table S2.

qPCR-based resection assay
Cells from each strain were grown overnight in 15 ml YPLG to reach an exponentially growing culture of 1 × 10 7 cells/ml.Next, 2.5 ml of the cells were pelleted as time point 0 sample, and 2% GAL was added to the remaining cells, to induce a DSB.Following that, respective time point samples were collected.Genomic DNA was purified using standard genomic preparation method by isopropanol precipitation and ethanol washing, and DNA was resuspended in 100 ml ddH 2 O. Genomic DNA was treated with 0.005 μg/μl RNase A for 45 min at 37 C.About 2 μl of DNA was added to tubes containing CutSmart buffer with or without inclusion of the RsaI restriction enzyme and incubated at 37 C for 2 h.qPCR was performed using the Applied Biosystem QuantStudio 6 Flex machine.PowerUp SYBR Green Master Mix was used to quantify resection at the RsaI cut site 0.15 Kb DSB (in the MAT1 locus) and 4.8 Kb.PRE1 was used as a negative control, and the primer sequences are listed in Table S2.RsaI cut DNA was normalized to uncut DNA as previously described to quantify the %ssDNA (28).HO cutting was measured in strains for resection (Table S4).

Figure 5 .
Figure 5. Model depicting how dna2 mutants impact DSB repair, where the presence of nuclease-dead Dna2 at the break inhibits Exo1 nuclease through increased Ku.A, the schematic shows the antagonistic relationship between Ku70/80 (Ku) and Exo1 and Nej1 and Dna2.Ku binding to DNA ends at the break, inhibiting the access of Exo1 nuclease to perform 5 0 resection.Nej1 is a competitive inhibitor of Dna2, blocking interactions between Dna2 and its binding partners at DSBs(1,5,6,8,9,15,16).B, upon deletion of DNA2, Nej1 increased, but Ku and Exo1 levels did not change.In dna2D pif1-m2 mutants, resection decreased approximately twofold as Exo1 was the only functional long-range nuclease at the DSB, and the frequency of alt-EJ-MMEJ markedly increased.C, in dna2-1 mutants, nuclease-dead Dna2 was recruited to the break site.Under this condition, there was a minor increase in Nej1.However, Ku increased, which in turn resulted in Exo1 inhibition.Therefore, in this mutant background, the functionality of both nucleases was compromised, resection was abrogated, and the frequency of NHEJ increased.The dna2-1 resection defect and phleomycin sensitivity were largely reversible either by ectopic expression of Exo1 or by deletion of Ku70.However, only Exo1 expression restored the balance of NHEJ and alt-EJ-MMEJ frequencies to levels observed in WT cells.alt-EJ, alt-end-joining; DSB, double-strand break; MMEJ, microhomology-mediated end joining; NHEJ, nonhomologous end-joining.