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About the Authors:

Patricia L. Opresko

* E-mail: [email protected]

Affiliation: Department of Environmental and Occupational Health, University of Pittsburgh Graduate School of Public Health, Pittsburgh, Pennsylvania, United States of America

Gregory Sowd

Affiliation: Department of Environmental and Occupational Health, University of Pittsburgh Graduate School of Public Health, Pittsburgh, Pennsylvania, United States of America

Hong Wang

Affiliations Department of Pharmacology and Chemical Biology, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania, United States of America, The University of Pittsburgh Cancer Institute, Hillman Cancer Center, Pittsburgh, Pennsylvania, United States of America

Introduction

Werner syndrome (WS) is an autosomal recessive disorder marked by the premature onset of numerous features associated with aging and a predisposition to mesenchymal cancers [1]. WS is caused by loss of the DNA repair protein WRN which is a member of the RecQ family of DNA helicases [2]. E. coli and S. cerevisiase each have a single family member, whereas five members exist in humans: RECQ1, RECQ4, RECQ5, BLM and WRN [3], [4]. Mutations in the human RecQ helicases BLM and RECQ4 also give rise to the cancer predisposition disorders Bloom syndrome (BS) and Rothmund-Thomson syndrome (RTS), respectively [5]. Despite the common feature of genomic instability, these disorders are clinically distinct from WS. While there are no known human disorders caused by defects in RECQ1 or RECQ5, cellular and transgenic mouse studies indicate that loss of these proteins also leads to genomic instability [5]. Thus, RecQ helicases have been classified as “caretakers” of the genome [3].

RecQ helicases have critical roles in regulating homologous recombination (HR) pathways. HR functions in repair of DNA double strand breaks, restoration of collapsed replication forks, and the alternative lengthening of telomeres (ALT) pathway [6]–[9]. Inappropriate HR can lead to loss of heterozygosity due to DNA strand crossovers, chromosome translocations, telomere loss, and tangled DNA intermediates that are potentially toxic if left unresolved [6]. In HR broken DNA ends are processed to generate single stranded tails that are coated by Rad51, which catalyzes invasion of the ssDNA tail into homologous duplex sequence and promotes base pairing between the ssDNA tail and one strand of the duplex [10]. The result is a joint molecule termed a displacement loop (D-loop). If the invading ssDNA terminates in a 3′OH it primes DNA polymerase extension and copying of the homologous sequence [8], [11]. Dissociation of the D-loop can lead to re-annealing of the displaced strand to the ssDNA tail of the other broken end in the synthesis-dependent strand annealing (SDSA) pathway [12]. Alternatively, the tail of the other broken end may also be captured leading to the formation of a double Holliday junction (HJ), which is processed into strand crossover or non-crossover products [13]. RecQ helicases regulate HR by preventing inappropriate events through displacing Rad51 (BLM, RECQ1, RECQ5) [14]–[16] and by dissociating recombination intermediates including various HJ and D-loop constructs [16]–[20]. Unwinding of duplex DNA is catalyzed by RecQ helicases with 3′ to 5′ polarity and requires nucleotide hydrolysis.

WRN is unique among the human RecQ helicases in that the protein also has 3′ to 5′ exonuclease activity [21], and both helicase and exonuclease activities are implicated in the dissociation of HR intermediates. WS cells exhibit defects in resolving HR intermediates that form in response to stalled replication forks, whether induced by blocking lesions or by depleted dNTP pools [22], [23]. The HR defect can be rescued by inhibiting Rad51 [24], and thus the formation of recombination intermediates, but is not rescued by expressing WRN mutants that lack either helicase or exonuclease activities [25]. WRN deficient cells are also prone to abnormal HR at telomeric ends, and exhibit increased telomere loss, telomeric sister chromatid exchanges and spontaneous extra-chromosomal telomeric circles [26]–[29]. Telomeres contain a 3′ single strand (ssDNA) tail that is ∼50 to 150 nt long in vivo [30] and forms protective intra-telomeric D-loops that stabilize the large t-loop [31]. Aberrant HR involving the natural D-loop/t-loop or inappropriate strand invasion into telomeric sequences in other chromatids or chromosomes can lead to telomere loss and abnormal telomere structures [32], [33]. RecQ helicases are also implicated in the resolution step of the recombination-based ALT pathway to lengthen telomeres [34], [35].

WRN acts on many of the same substrates as other human RecQ helicases, but has the potential to process these substrates differently due to the exonuclease activity. Precisely how both WRN biochemical activities contribute to processing HR intermediates is not clear. We and others observed previously that oligomeric non-mobile D-loops are substrates for both the WRN helicase and exonuclease activities, but these constructs could not test for branch migration activity [36], [37]. WRN helicase activity is poorly processive and is unable to completely unwind a 33-bp oligomeric telomeric D-loop in the absence of accessory proteins POT1 or RPA, or assistance from the WRN exonuclease activity [37], [38]. Exonucleolytic degradation shortens the duplex length to be unwound by digesting the invading strand in a 3′ to 5′ direction [37]. Here we extended our previous studies by constructing more biologically relevant mobile D-loops. They have a much longer invading strand that pairs with one strand in a plasmid to form an 84 bp duplex, and can be branch migrated. Based on evidence that WRN regulates recombination at telomeres [39], we also constructed telomeric D-loops for analysis.

In this study we identified mobile plasmid-based D-loops as novel substrates for both WRN helicase driven branch migration and exonuclease activities, and found that telomeric D-loops were disrupted less efficiently than non-telomeric D-loops. In contrast to oligomeric constructs, we show that WRN helicase alone can completely dissociate the 84 bp duplex to release the invading strand from the plasmid D-loop. However, the WRN exonuclease activity alters processing by degrading the long invading strand both prior to and after release from the plasmid D-loop. WRN disrupts plasmid D-loops with a protruding 3′ or 5′ single stranded tail, but a protruding tail is not required for either branch migration or exonuclease activities. Furthermore, we demonstrate that WRN recognizes both the 5′ and 3′ ends of the D-loop duplex, which led us to propose a novel model for WRN loading and processing of biologically relevant D-loop recombination intermediates.

Results

WRN disrupts mobile plasmid D-loops

To generate more biologically relevant D-loops we used RecA to catalyze the invasion of a 120-mer oligonucleotide into negatively supercoiled plasmids. The resulting D-loop contained a 5′ 36 nt ssDNA tail protruding from an 84 bp duplex in which the oligonucleotide base paired with the complementary strand of the plasmid (Fig. 1A–B). The strand invasion duplex sequence for the 5′Tail Telomeric (Tel) D-loop consisted of (TTAGGG)10 flanked by 12 bp of unique sequence to ensure proper alignment of the repeats. The telomeric repeat sequence was scrambled for the non-telomeric 5′Tail D-loop. Both D-loops were stable since no spontaneously released oligonucleotide was detected after purification (Fig. 1B, lanes 6 and 8). The duplex region of the non-telomeric D-loop was susceptible to cleavage by restriction enzymes indicating the invading strand was fully based paired with the plasmid strand (Fig. 1C). Finally, the 3′ 12 bp flanking sequence in the duplex of both D-loops contained an AvaI restriction site that was cleaved to near completion confirming proper based pairing at the 3′end of the invading strand (Fig. 1C). These data demonstrate that the mobile D-loops are stable and contain an invading strand that is completely base paired with the complementary plasmid strand.

[Figure omitted. See PDF.]

Figure 1. Construction of mobile plasmid D-loops.

A. Schematic of 5′ Tail non-telomeric and telomeric (Tel) plasmid D-loops. The star denotes the 5′ end radiolabel. The invading strand of the 5′Tail Tel D-loop base pairs with the plasmid to form an 84 bp duplex with ten (TTAGGG) repeats flanked by 12 bp of unique sequence. The telomeric repeats are scrambled in the non-telomeric D-loop. Restriction enzyme sites are indicated as A, AvaI; B, BlpI. B. RecA generated plamid D-loops are stable. Plasmids (300 µM nucleotides) were mixed with the 5′end-labeled complementary oligonucleotide (3.6 µM nucleotides) and RecA protein (4 µM) (lanes 2 and 4). D-loops (Dlp) were then purified from unincorporated oligonucleotide (ss) (lanes 6 and 8). Reactions were run on a 4–20% polyacrylamide native gel. C. The D-loop invading strand is fully base paired with the plasmid strand. Reactions (20 µl) contained 50 pM purified 5′Tail non-telomeric (Non-Tel) or telomeric (Tel) D-loops and 10 units of the indicated restriction enzyme. Products were run on a 14% polyacrylamide denaturing gel.

https://doi.org/10.1371/journal.pone.0004825.g001

To examine WRN catalytic activities on the plasmid D-loops, the substrates were incubated with increasing WRN concentrations. The reactions were analyzed on a native gel to display D-loop disruption and on a denaturing gel to better visualize the products of the 3′ to 5′ exonuclease activity. WRN protein released a mixture of full length and shortened strands due to the combined action of strand displacement activity and the exonuclease digesting from the 3′OH of the invading strand (Fig. 2A–B). The telomeric sequence was more refractory to displacement and digestion (Fig. 2A–C). Approximately 10-fold more WRN was required to disrupt 50% of the telomeric 5′Tail Tel D-loop (5 nM WRN) compared to the non-telomeric 5′Tail D-loop (0.5 nM WRN). The exonuclease progressed further through the non-telomeric sequence with a maximum of ∼73 nt digested (47 nt product), compared to the telomeric D-loop with a maximum of ∼55 nt digested (66 nt product) (Fig. 2B). The distinct pattern of digestion products for the telomeric 5′Tail Tel D-loop corresponds to termination at the G run of each repeat (Fig. 2B, lanes 9–15) as observed previously for oligomeric forks and D-loops [37], [40]. To examine the mechanism of WRN D-loop displacement, we constructed a forked duplex of similar size and sequence as the telomeric D-loop. Consistent with previous reports [41], an 83 bp duplex is too long for WRN helicase activity to efficiently unwind (Supplemental Fig. S1). This result, along with the finding that WRN helicase cannot completely unwind a 33-bp non-mobile D-loop [37], supports the conclusion that WRN disrupts the 84-bp mobile D-loops through branch migration rather than simply strand separation. Furthermore, even though WRN can digest at the blunt end of a shorter fork (34-bp) [42], WRN exonuclease fails to digest the 83-bp forked duplex (Fig. 2D). Therefore, the plasmid D-loops are preferred substrates for displacement and exonucleolytic attack by WRN protein. In addition, both non-telomeric and telomeric plasmid D-loops are substrates for WRN branch migration and exonucleolytic attack, although the telomeric sequence is more refractory to processing.

[Figure omitted. See PDF.]

Figure 2. WRN displaces and digests the invading strand of plasmid D-loops.

A. Reactions contained 50 pM of either the 5′Tail non-telomeric (lane 1–6) or the telomeric (Tel) (lanes 7–12) plasmid D-loops. The substrate was incubated with WRN concentrations increasing in doubling steps from 0.62 to 5 nM (lanes 2–5 or 8–11, respectively) for 15 min under standard reaction conditions and run on a 4–20% native polyacrylamide gel. ▴, heat denatured substrate. B. The 5′ Tail non-telomeric (lanes 1–8) or telomeric (lanes 9–15) were incubated with WRN concentrations increasing in doubling steps from 0.078 to 5 nM (lanes 2–8) and 0.15 to 5 nM (lanes 10–15) and run on a 14% denaturing polyacrylamide gel. Numbers represent oligonucleotide size markers. C. The percent total D-loop displacement from reactions in panel A were calculated as described in Materials and Methods and plotted against WRN concentration. WRN and 5′Tail plasmid D-loop, ▪ and dotted line; WRN and 5′Tail Tel plasmid D-loop, • and solid line. Values represent the mean and standard deviation (SD) from at least three independent experiments. D. WRN exonuclease is inactive on an 83 bp forked duplex. Reactions contained 0.25 nM of the 83-bp forked duplex containing ten telomeric repeats (thick black line) with 15 and 8 bp of flanking sequence. The substrate was incubated with WRN concentrations increasing in doubling steps from 0.19 to 25 nM for 15 min under standard reaction conditions. Reactions were run on a 14% denaturing gel.

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WRN can branch migrate the full 84 bp duplex of the plasmid D-loop

To confirm that WRN helicase branch migration activity alone can disrupt the full 84 bp duplex in the plasmid D-loops, we inactivated the WRN exonuclease activity. For this we incubated the 5′Tail non-telomeric and telomeric D-loops with an exonuclease-dead variant of WRN (E84A). Branch migration through the full 84-bp duplex was observed for both D-loops, and was detected at as low as a 3-fold molar excess of E84A-WRN (0.15 nM) over substrate (0.05 nM) for the non-telomeric 5′Tail D-loop (Fig. 3A, lane 2). However, the total percent of D-loops disrupted for the E84A-WRN mutant was decreased compared to wild type WRN (compare Figs. 2A and 3A). In order to examine branch migration activity of the wild type WRN protein preparation in the absence of digestion, we suppressed the WRN exonuclease activity by decreasing the free Mg2+ concentration. Since the WRN exonuclease acts by a two-metal ion dependent mechanism, free divalent cations are required to bind the exonuclease active site [43]–[45]. While WRN helicase remains active at Mg2+∶ATP ratios near 1 [43](data not shown), we found that WRN exonuclease activity is highly dependent on the free Mg2+ concentration. The incubation of WRN and the 5′Tail D-loops in reactions with a molar excess of ATP over Mg2+ (2∶1) resulted in the loss of shortened products in favor of displaced full length strands (Fig. 3B). Decreasing the Mg2+ concentration inhibited the WRN exonuclease activity and reduced the percent of total disrupted D-loops (compare Figs. 2A and 3B). In summary, WRN protein can branch migration through the full 84-bp duplex of the plasmid D-loops, but the percent of D-loop disruption is decreased in the absence of exonuclease activity.

[Figure omitted. See PDF.]

Figure 3. WRN can branch migrate through the full 84 bp duplex to displace the invading strand.

Reactions contained 50 pM of either the 5′Tail non-telomeric (lanes 1–8) or the telomeric (Tel) (lanes 9–14 (A.) or 9–16 (B.)) plasmid D-loops. Reactions were run on 4–20% native polyacrylamide gels and visualized by phosphorimager analysis. ▴, heat denatured substrate. A. Branch migration after exonuclease inactivation with a WRN mutant. The substrate was incubated with E84A-WRN concentrations increasing in doubling steps from 0.15 to 5 nM (lanes 2–7) or from 0.62 to 5 nM (lanes 11–14) for 15 min under standard conditions. B. Branch migration after exonuclease inhibition with limiting Mg2+. The substrate was incubated with wild type WRN concentrations increasing in doubling steps from 0.15 to 5 nM (lanes 2–7, and lanes 10–15) for 15 min in reactions buffer containing 1 mM MgCl2 and 2 mM ATP. The percent total displacement was plotted against E84A-WRN (A.) or wild type WRN (B.) concentration. E84A-WRN or WRN and 5′Tail D-loop, ▪ and dotted line; E84A-WRN or WRN and 5′Tail Tel D-loop, • and solid line. Values are the mean and standard deviation (SD) from two-three independent experiments.

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WRN exonuclease activity digests the invading strand prior to and after release from the D-loop

Next we asked whether the WRN exonuclease digested the invading strand in the context of the D-loop and/or after displacement. The long length of the invading strand (120 nt) in the plasmid D-loops makes it a potential substrate for WRN exonucleolytic attack after release from the D-loop, in contrast to the previously tested 33-bp oligomeric D-loops [37]. WRN exonuclease is inefficient on short ssDNA strands (<40 nt), but extensively digests long 80-mer oligonucleotides due to increased affinity for long ssDNA molecules [46]. To test whether WRN can digest the invading strand in the context of the D-loop, we inhibited branch migration activity by using the analog ATPγS that is not efficiently hydrolyzed by WRN [47]. Branch migration of mobile D-loops by RecQ helicases RECQ1 and BLM require the energy from ATP hydrolysis [16], [19], [48]. Disruption of the 5′Tail D-loops occurred even in the absence of WRN branch migration activity but was reduced approximately 2.5-fold for both the D-loops within the linear range of the titration curve (Fig. 4A–B). However, we observed a loss of the full length products and the appearance of very short ssDNA products that resulted from extensive digestion of the duplex to thermally unstable lengths (Fig. 4A). Similar results were obtained in the absence of ATP or the analog (data not shown). Visualization of the exonuclease products on a denaturing gel clearly shows the extent D-loop digestion progressed further when ATP hydrolysis is inhibited (ATPγS and no ATP) (Fig. 4C, compare lanes 5 to 6 and 7, Fig. 4D compare lanes 8 to 9) for some molecules. The exonuclease-dead WRN mutant (E84A) yielded no detectable digestion products after incubation with either D-loop (Fig. 4C lanes 1–3, Fig. 4D lanes 10–12).

[Figure omitted. See PDF.]

Figure 4. WRN exonuclease digests the long invading strands both prior to and after release from the plasmid D-loops.

A. Reactions contained 50 pM of either the 5′Tail non-telomeric (lane 1–8) or the telomeric (Tel) (lanes 9–15) plasmid D-loops. The substrate was incubated with WRN concentrations increasing by doubling steps from 0.15 to 5 nM (lanes 2–7) or from 0.31 to 5 nM (lanes 10–14) for 15 min under standard reaction conditions except ATP was replaced with ATPγS. Reactions were run on 4–20% native polyacrylamide gels and visualized by phosphorimager analysis. ▴, heat denatured substrate. B. The percent total displacement was calculated as described in Materials and Methods and plotted against WRN concentration. WRN and 5′Tail D-loop, ▪ and dotted line; WRN and 5′Tail Tel D-loop, • and solid line. Values are the mean and standard deviation (SD) from two independent experiments. C. and D. WRN exonuclease on intact and released invading strands. Reactions contained 50 pM of either the non-telomeric (C.) 5′Tail D-loop (lanes 1–7) or 120-mer oligonucleotide (lanes 11–14) or the telomeric (D.) 5′Tail Tel D-loop (lanes 7–12) or 120-mer oligonucleotide (lanes 1–4). The substrates were incubated with WRN (5 nM) or E84A-WRN mutant (X; 5 and 2.5 nM) under standard conditions for 15 min except that either 2 mM ATP, 2 mM ATPγS (γ) or no ATP (-) was added as indicated. Reactions were run on 14% polyacrylamide denaturing gels. Oligonucleotide size markers were loaded for reference.

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Next we asked if WRN can digest the long invading strands after branch migration released them from the D-loop, by incubating WRN with the 120 nt oligomers used to construct the 5′Tail D-loops (Table 1). WRN digestion of the long oligomers was apparent (Figs. 4C lanes 11–14, and 4D lanes 1–4), dose dependent and eliminated upon mutation of the WRN exonuclease domain (Supplemental Fig. S2). The extent of WRN digestion of the long ssDNA molecules was not increased in the absence of ATP hydrolysis (Fig. 4C, lanes 12–14 and Fig. 4D, lanes 2–4), in contrast to digestion of the 5′Tail D-loops. In summary, WRN exonucleolytic attack of the D-loop invading strand does not require branch migration activity and occurs prior to and after release from the D-loop.

[Figure omitted. See PDF.]

Table 1. Oligonucleotides used in substrate preparations.

https://doi.org/10.1371/journal.pone.0004825.t001

Structural requirements of WRN D-loop branch migration and exonuclease activities

To determine the structural requirements for WRN catalytic activities on the plasmid D-loops, we constructed D-loops with either a protruding 3′ ssDNA tail or no protruding tail (Fig. 5A). WRN disrupted about 50% of the D-loops at ∼0.25 nM and 1 nM protein for the 3′Tail D-loop and No Tail D-loop, respectively, and released a mix of full length and shortened strands (Fig. 5A–C). Importantly, disruption of the 3′Tail D-loop (7.6%) was detected at near equal molar WRN (0.04 nM) and substrate (0.05 nM) concentrations (Fig. 5C). No digestion of the D-loops is detected when the WRN exonuclease domain is mutated (E84A-WRN) (Fig. 5D, lanes 9–12). To ensure that WRN can digest the strands in the context of the D-loop we also examined processing in the absence of branch migration (ATPγS and no ATP). The extent of digestion of the No Tail D-loop invading strand was similar to the 5′Tail D-loop both in the presence of branch migration activity (Fig. 5D lane 5 compare to Fig. 4C lane 5), and in the absence of branch migration activity in which digestion progressed almost to the end of the duplex (Fig. 5D lanes 7–8 compare to Fig. 4C lanes 6–7). However, the 3′Tail D-loops differ in that the exonuclease initiates digestion on ssDNA rather than on duplex DNA. WRN digestion of the 3′Tail D-loop in the absence of branch migration (Fig. 5D, lanes 3–4) confirms that WRN can degrade a 36 nt 3′ssDNA tail protruding from the plasmid D-loop. We did not detect any appreciable digestion into the duplex for the 3′Tail D-loop (Fig. 5D, lanes 3–4), which is expected since WRN needs to degrade the full 36 nt tail prior to encountering the duplex. Consistent with a failure to shorten the duplex region, no disruption of the 3′Tail D-loop was detected upon inhibition of WRN branch migration after 15 min reaction time (data not shown). In summary, a protruding tail is not required for either WRN branch migration or exonuclease activities on a plasmid D-loop, and WRN can digest a 3′ ssDNA tail protruding from the D-loop.

[Figure omitted. See PDF.]

Figure 5. Structural requirements for WRN activity on plasmid D-loops.

A. Schematic of 3′Tail and No Tail D-loops. The star denotes the 5′ end radiolabel. B. Reactions contained 50 pM of either the 3′Tail (lane 1–6) or the No Tail (lanes 7–12) plasmid D-loops. The substrate was incubated with WRN concentrations increasing by doubling steps from 0.62 to 5 nM (lanes 2–5 and 8–11) for 15 min under standard reaction conditions. Reactions were run on 4–20% polyacrylamide native gels and visualized by phosphorimager analysis. ▴, heat denatured substrate. C. The percent total displacement was calculated as described in Materials and Methods and plotted against WRN concentration. WRN and 3′Tail D-loop, ▪ and dotted line; WRN and No Tail D-loop, • and solid line. Values are the mean and standard deviation (SD) from at least three independent experiments. D. Analysis of WRN exonuclease activity. Reactions contained 50 pM of either the 3′Tail (lanes 1–4 and 9–10) or the No Tail (lanes 5–8 and 11–12) D-loops. The substrates were incubated with 5 nM WRN or E84A-WRN mutant (X) under standard conditions for 15 min except that either 2 mM ATP, 2 mM ATPγS (γ) or no ATP (-) was added as indicated. Reactions were run on 14% polyacrylamide denaturing gels. Arrow points to products representing digestion almost to the end of the 84-bp duplex.

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To determine whether the presence of a protruding tail influences the kinetics of WRN D-loop disruption we conducted time course reactions. An increase in total strand displacement occurred as a function of time that began to plateau at about 4 min for the 3′Tail D-loop and 8 min for the 5′ and No Tail D-loops (Fig. 6A–B). The rate of total strand displacement was similar for the 5′ and No Tail D-loops, but was ∼2-fold higher for the 3′ Tail D-loop. Loss of the full length products in favor of extensively degraded products became apparent at the later time points, which most likely reflects additional digestion of the released ssDNA strands (Fig. 6A). To determine the influence of structure on the helicase branch migration activity alone, we examined the kinetics of D-loop disruption by the exonuclease-dead WRN mutant (E84A). The 3′ Tail D-loop was more rapidly disrupted by WRN branch migration activity than the 5′ and No Tail D-loops (Fig. 6C and Supplemental Fig. S3). Furthermore, the kinetics of strand displacement for the E84A-WRN mutant were similar to wild type WRN for the 3′Tail D-loop, but was decreased for the 5′Tail and No Tail D-loops, relative to wild type (Figs. 6B and C). This indicates that the WRN exonuclease activity contributes more to the rate of D-loop disruption for the substrates in which digestion proceeds into the duplex region (5′ and No Tail D-loop), than for the substrate in which duplex was not detectably shortened (3′ D-loop). The identical order of substrate preference was observed when wild type WRN exonuclease activity was inhibited by limiting Mg 2+ concentrations (Supplemental Fig. S3)

[Figure omitted. See PDF.]

Figure 6. Kinetics of WRN activity on plasmid D-loops.

Reactions contained 50 pM of either the 5′Tail, No Tail, or 3′Tail plasmid D-loops as indicated. The 5′ labeled end is indicated with a star. The substrate was incubated with 5 nM WRN (Panel A–B) or 5 nM E84A-WRN mutant (Panel C) for 0.5, 1, 2, 4, 8, 15, 30 min under standard reaction conditions. Reactions were run on 4–20% polyacrylamide native gels and visualized by phosphorimager analysis. ▴, heat denatured substrate. B. and C. The percent total displacement was calculated as described in Materials and Methods and plotted against time for reactions with wild type WRN (B.) or the E84A-WRN mutant (C.). 5′Tail D-loop, ▪ and black line; 3′Tail D-loop, ▴ and blue line; No Tail D-loop, ▾and yellow line. The representative phosphorimage scans for the E84A-WRN reactions are shown in Supplemental Fig. S3A.

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WRN recognizes both junctions of the D-loop

Previous studies showed that WRN can bypass a streptavidin-biotin steric block on the 3′tail of a fork or flap substrate, indicating that WRN can recognize a fork-like junction directly to initiate unwinding. Based on this and other studies with oligomeric forks, D-loop and flap structures [36], [37], [49], we conjectured that WRN would load and initiate branch migration at the 5′ end of the invading strand duplex in the D-loop and translocate 3′ to 5′ along the plasmid strand. If this were true, the action of the WRN exonuclease at the opposite end (3′OH) would require the protein to simultaneously interact with both ends of the 84 bp duplex. Thus, we tested whether WRN D-loop disruption required WRN recognition of the 5′ or 3′end of the invading strand duplex to initiate displacement. We constructed plasmid D-loops containing an invading strand with both a 5′ and 3′ 18 nt ssDNA tail protruding from a 60 bp duplex (Fig. 7). A biotinylated nucleotide was incorporated in the 5′ and/or 3′ tail of the invading strand 2 nt away from the duplex region (junction). To impart a steric block at either the 5′ or 3′ junction or both, the D-loops were pre-incubated with streptavidin to bind the biotin groups. Free streptavidin protein does not inhibit WRN [49]. Importantly, the biotin moiety alone did not inhibit WRN branch migration activity as indicated by rapid disruption of the plasmid D-loops (Fig. 7). However, the WRN exonuclease cannot progress past the biotin (Fig. 7D) which explains the lack of detectable shortened products on the native gels for the D-loops with a biotin near the 3′end (Fig. 7 A and C). Blocking both the 5′ and 3′ junctions resulted in a dramatic reduction in D-loop disruption (Fig. 7A), indicating that the streptavidin-biotin complex effectively blocked WRN recognition of the junctions. In contrast, blocking only the 5′ junction slowed the rate of D-loop disruption by about 4.8-fold but did not prevent branch migration, suggesting that WRN can recognize the 3′ junction (Fig. 7B). Consistent with this, blocking only the 3′ junction also slowed the rate of D-loop disruption, in this case 2.7 fold (Fig. 7C). When either the 3′ or 5′ junction blocked, nearly the same maximal amount of D-loop disruption was eventually achieved as for the corresponding non-blocked D-loop (Fig. 7B–C). Furthermore, a WRN exonuclease-dead mutant can disrupt a D-loop containing a blocked 5′ junction that lacks a 3′ tail, indicating that WRN helicase branch migration from the accessible 3′junction does not require a 3′ tail for loading (Fig. 8). Importantly, the displaced strand exhibited slower mobility in the presence of streptavidin (Fig. 7–8). This confirms that streptavidin remained bound to DNA throughout the reactions, consistent with previous reports that WRN helicase does not dissociate the streptavidin from the DNA [49]. These data indicate that WRN protein can recognize both junction ends of the invading strand duplex, and can effectively disrupt D-loops containing a steric block at one junction but not when both junctions are blocked.

[Figure omitted. See PDF.]

Figure 7. WRN recognized both ends of the invading strand duplex in a plasmid D-loop.

A schematic is shown of the plasmid D-loops with a invading strand that forms a 60 bp duplex containing 18 nt protruding 5′ and 3′ ssDNA tails. A biotinylated nucleotide (circle) was positioned 2 nt from the duplex on the 3′ and 5′ tails (A), the 5′tail only (B) or the 3′tail only (C). Reactions contained 50 pM of plasmid D-loop that was pre-incubated for 10 min in reaction buffer alone or together with streptavidin as indicated. Then WRN (1.25 nM) was added and reaction aliquots were terminated at 0, 1, 3, 5, 10, 15 and 30 min. Reactions were run on 4–20% native polyacrylamide gels and visualized by phosphorimager analysis. ▴, heat denatured substrate. Dlp, D-loop; sb/ss, streptavidin-bound biotin ssDNA; b/ss biotin ssDNA. The percent total displacement was calculated as described in Materials and Methods and plotted against time. Biotin containing D-loops, ▪ and dotted line; Biotin+Strepavidin containing D-loops, • and solid line. Values represent the mean and standard deviation (SD) from at least three independent experiments. D. WRN exonuclease activity on ssDNA is inhibited by a biotin moiety. Reactions contained 50 pM of the 96-mer 5B Tail (lanes 1–7) or 3B Tail (lanes 8–14) oligonucleotides (Table 1). The substrates were incubated with 1.25 nM WRN and terminated after 0, 1, 3 5, 10, 15 and 30 reaction time under standard conditions. Reactions were run on 14% polyacrylamide denaturing gels.

https://doi.org/10.1371/journal.pone.0004825.g007

[Figure omitted. See PDF.]

Figure 8. WRN disruption of D-loops with a 5′ blocked junction does not require a 3′tail or exonuclease activity.

A schematic is shown of the plasmid D-loop with an invading strand that forms a 60 bp duplex containing a single 18 nt protruding 5′ ssDNA tail. A biotinylated nucleotide (circle) was positioned 2 nt from the duplex on the 5′ tail. Reactions contained 50 pM of plasmid D-loop that was pre-incubated for 10 min in reaction buffer alone or together with streptavidin as indicated. Then WRN (1.25 nM) was added and reaction aliquots were terminated at 0, 1, 3, 5, 10, 15 and 30 min. Reactions were run on 4–20% native polyacrylamide gels and visualized by phosphorimager analysis. ▴, heat denatured substrate. Dlp, D-loop; sb/ss, streptavidin-bound biotin ssDNA; b/ss biotin ssDNA. The percent total displacement was calculated as described in Materials and Methods and plotted against time. Biotin containing D-loops, ▪ and dotted line; Biotin+Strepavidin containing D-loops, • and solid line. Values represent the mean and standard deviation (SD) from two independent experiments.

https://doi.org/10.1371/journal.pone.0004825.g008

Discussion

Increasing evidence supports an important role for WRN protein in mediating the proper dissociation of joint DNA molecules that arise in genomic and telomeric regions during homologous recombination and repair of breaks at collapsed replication forks. WRN was previously shown to displace and degrade the invading strand of static oligomeric-based D-loops with a 5′ tail or no tail, which were designed to mimic an important HR intermediate [36], [37]. However, WRN helicase was unable to efficiently unwind the full 33-bp invaded duplex in a telomeric D-loop without assistance from single strand binding proteins RPA and POT1 or the exonuclease to shorten the duplex [37], [38]. Here, we demonstrate that WRN helicase alone is capable of displacing a much longer telomeric and non-telomeric invading strand (84-bp) from plasmid based D-loop, presumably by promoting branch migration. However, D-loop processing is altered in the presence of WRN exonuclease activity which digests the invading strand both before and after release from the D-loop. We propose that mobile D-loops are particularly suitable HR structures for processing by WRN because they are substrates for both the helicase and exonuclease activities, unlike Holliday junction recombination intermediate. The increased activity of WRN on the more biologically relevant plasmid D-loops, compared to oligomeric D-loops, greatly strengthens the argument that WRN is capable of processing such structures at telomeric ends and during HR in vivo.

WRN processing of static versus mobile D-loops

Our results indicate that WRN helicase and exonuclease process mobile D-loops and static D-loops by different mechanisms. We found that WRN helicase apparent processivity is increased on mobile D-loops, since WRN helicase alone can disrupt mobile D-loops with duplexes that are much longer (84 bp) (Figs. 2–3) than static D-loops that cannot be unwound (33 bp) [37]. We propose that by WRN helicase promoting branch migration through the mobile D-loop, the unpaired plasmid strands anneal and shrink the D-loop (Fig. 9). Thus, if WRN prematurely dissociates before the duplex is completely unwound, the partially unwound invading strand will not reanneal with the plasmid, allowing WRN to rapidly displace the remaining duplex upon rebinding the substrate. The loop cannot shrink in static D-loops since the “bubble” strands are not complementary and the partially unwound invading strand can reanneal if WRN prematurely dissociates. In agreement with our results, RECQ1 helicase also disrupts mobile D-loops by promoting branch migration, but is unable to unwind oligomeric D-loops of similar size [16]. Furthermore, BLM reactions with static D-loops produce intermediates that are not present in the mobile D-loop reactions [48]. Therefore the authors proposed that BLM may disrupt mobile D-loops, but not non-mobile D-loops, in a single step. Thus, WRN may displace mobile D-loops in a single binding step which could account for the increase in apparent processivity on mobile D-loops, compared to non-mobile D-loops which may require multiple binding steps for unwinding. Consistent with the increased apparent processivity of branch migration versus DNA unwinding, WRN was reported to promote migration through ∼2700 bp of duplex DNA in an α-structure recombination intermediate that resembles a Holliday junction [50]. In contrast, WRN unwinding of duplex DNA greater than ∼53 bp was found to require RPA [41](Supplemental Fig. S1).

[Figure omitted. See PDF.]

Figure 9. Bidirectional model for WRN branch migration and exonuclease activity on mobile D-loops.

WRN protein with the helicase (triangle) and exonuclease (crescent) domains are depicted as separate monomers, but could also be linked in a higher oligomeric complex (denoted by a dotted line) such as a tetramer. The D-loops represent an intermediate in recombination, SDSA, and a structure at the telomeric end or ALT pathway. The D-loop depicted contains no pre-existing ssDNA tail although such tails may occur in vivo, such as a 3′ tail in a non-productive D-loop. WRN protein recognizes the 5′ duplex junction and helicase translocation along the plasmid strand in a 3′ to 5′ direction will promote branch migration. WRN also recognizes the 3′ duplex junction and may translocate along the invading strand 3′ to 5′ to promote branch migration, but can also digest the strand 3′ to 5′. In this model helicase driven branch migration proceeds in a bidirectional manner toward the middle causing shrinking of the displacement loop and subsequent release of the invading strand. Branch migration progresses more rapidly than the exonuclease which digests at one end and may cause a “loop out” of ssDNA (last structure). WRN exonuclease activity can also digest the strand after release depending on the length (not depicted here).

https://doi.org/10.1371/journal.pone.0004825.g009

WRN loading on plasmid D-loops

Unlike RECQ1, WRN and BLM do not exhibit polarity of branch migration. RECQ1 branch migrates 3′ to 5′ and requires a 3′ tail [16], [19], however, BLM [48] and WRN (Fig. 5) do not require a tail for branch migration. Therefore, the loading site and the strand upon which WRN translocates are not obvious. WRN exonuclease activation at blunt ends of a fork occurs by protein loading at the forked end [42], [51], and so digestion only occurs on shorter forks (34-bp) and not longer ones (83-bp) (Fig. 1). WRN cannot load on blunt ends [47]. However, the D-loop contains a junction at both duplex ends and we found that accessibility of both junctions is required for optimal D-loop disruption by WRN, suggesting that WRN engages both junctions (Fig. 7). Thus, we propose a bidirectional model for WRN helicase driven branch migration of mobile D-loops (Fig. 9). In this scenario a WRN molecule engages the 5′ junction and translocates 3′ to 5′ along the plasmid strand, and another WRN molecule engages the 3′ junction and translocates 3′ to 5′ along the invading stand while simultaneously digesting the strand. Branch migration would proceed rapidly from both junctions, whereas the exonuclease activity occurs only at the available 3′OH end and progresses more slowly. Consistent with this, the products of branch migration through the 84 bp (full length strands) appeared earlier than the extensively digested products in the time course reactions (Fig. 6). This agrees with previous reports that the helicase progresses faster than the exonuclease activity [42]. In further support, we observed that blocking only one junction slowed the rate of D-loop disruption, but also altered the kinetic curve such that the reaction plateau was delayed (Fig. 7B–C). WRN eventually achieved near maximal D-loop disruption when one junction was blocked, but required more time than was needed for the corresponding unblocked D-loop (Fig. 7B–C). This suggests that WRN can achieve more rapid D-loop disruption when branch migration proceeds from both ends rather than one end. When both junctions were blocked, D-loop strand displacement was barely detectable even after 30 min (Fig. 7A). This suggests that initiation of branch migration was inhibited. However, we cannot distinguish whether separate WRN molecules engage the junction, or if different WRN monomers of a higher oligomeric complex engage the junctions. WRN was recently found to bind model replication forks and Holliday junctions [52] as a tetramer. Structural analysis and single molecule imaging will be key to deciphering these models.

Alternatively, WRN may only recognize and initiate branch migration from one junction in a unidirectional model. For example, the steric block at the 5′ junction might inhibit initiation whereas the steric block downstream at the 3′ junction might inhibit progression. We believe a biotin-streptavidin complex is more likely to inhibit WRN initiation rather than progression for several reasons. The downstream block is outside the duplex region and is also present on the opposite strand that WRN is presumed to track along in a unidirectional model. Bulky DNA adducts in duplex DNA strongly inhibit WRN when present on the translocating strand [53]. Furthermore, once the duplex is shortened to unstable lengths (∼12 bp) it will thermally melt [42], so a downstream block would be ∼14 nt away from WRN when strand displacement occurred. A biotin-streptavidin complex on oligomeric fork and flap substrates did not inhibit WRN unwinding unless the complex was placed at the junction [49]. Thus, we do not favor a unidirectional model.

Comparison with other RecQ helicases

Caution should be applied when directly comparing our results with WRN to studies with other human RecQ helicases due to differences in the D-loop constructs examined (size and sequence) and reaction conditions. Nevertheless, WRN is at least as efficient as RECQ1 and BLM in disrupting various plasmid D-loops. In reactions for equivalent times and with similar amounts of 5′ tailed D-loops (∼50 pM), disruption of 50% of the D-loop is achieved with 7.4 nM BLM [48], compared to 0.5 nM WRN (Fig. 2) or ∼1 nM WRN if the exonuclease is inactivated (Fig. 3). RECQ1 preferentially unwinds 3′tailed D-loops, and disruption of approximately 50% of the substrate is achieved by 7.5 nM RECQ1 within ∼2.5 min [16], and by 5 nM WRN within ∼1.5 min even if the exonuclease is inactivated (Fig. 6). Thus, WRN is at least as efficient as BLM and RECQ1 but has the added feature of trimming the invading tails.

Roles for WRN digestion of D-loop recombination intermediates

The activity of WRN exonuclease on plasmid D-loops affords WRN the ability to process these structures differently than other human RecQ helicases. Both the WRN exonuclease and helicase are required for the survival of recombinant progeny after the induction of Rad51-dependent HR intermediates to restore blocked or stalled DNA replication forks [22]–[24]. Our data indicate that both the WRN exonuclease and helicase are active on biologically relevant Rad51-dependent recombination intermediates. In addition to disrupting 3′ end invaded D-loops, we demonstrate for the first time that WRN can also disrupt 5′ end invaded D-loops (3′Tail D-loop) (Fig. 5). Rad51 promotes both 3′ and 5′ end invasion for D-loop production [54], [55], however, the latter is potentially toxic because it is unproductive. A 5′ end invaded D-loop cannot be extended by a polymerase to complete the next steps of HR repair of replication forks, SDSA, or the ALT pathways [6], [11]. While the role for the helicase in branch migration is clear, the role for the exonuclease has several possibilities. First, shortening of the invading strand results in fewer sites for Rad51 re-nucleation after strand release, which would inhibit repeated strand invasion events. Second, if the Rad51 mediated D-loop formation is incomplete such that the 3′ end is not fully paired with the template strand, it cannot be extended by a polymerase in the next steps of HR replication restart, SDSA or ALT pathways. WRN can rescue this unproductive intermediate by degrading the 3′ protruding ssDNA (Fig. 5).

WRN activity on Telomeric D-loops

The decrease in WRN branch migration and exonuclease digestion of the telomeric sequence compared to the non-telomeric sequence have both biochemical and biological implications. Helicase processivity is influenced by base pair stability [56], therefore, differences could be related to duplex stability. However, we detected no obvious differences in thermal melting temperatures for the telomeric sequence compared to the non-telomeric sequence used in this study (Table 1) according to the HyTher web-based program [57]. The ssDNA TTAGGG repeats in the plasmid D-loop have the potential to form G-quadruplex DNA which could impede branch migration and would require resolution by the helicase [58]. The G-quadruplex DNA might also sequester WRN since WRN binds G4 DNA with high affinity [58]. The increased resistance of the telomeric D-loop to branch migration and digestion might also have implications for tighter regulation of processing at the telomeres in vivo. Inappropriate processing of telomeric ends by DNA repair proteins can have dire consequences for the cell and lead to senescence, apoptosis or genomic instability [33]. Untimely release of the telomeric t-loop/D-loop structure at the chromosome ends can activate a DNA damage response [59]. Therefore, resolution of telomeric D-loops might be more dependent on stimulation by telomeric proteins TRF2 and POT1, which regulate recombination at telomeric ends [33]. Consistent with this, POT1 and TRF2 interaction with WRN and were found to regulate WRN activities in vitro [37], [60].

In summary, we report that biologically relevant plasmid based D-loops with relatively long strand invasion duplex regions (84-bp) are substrates for both WRN branch migration and WRN exonuclease activity. WRN activity is not dependent on a protruding ssDNA tail, but the exonuclease is highly dependent on the free Mg2+ concentration. Our results offer a potential explanation for the cellular studies that indicate both WRN activities are required for dissociation of Rad51 dependent recombination intermediates to complete repair and suppress inappropriate recombination at stalled replication forks [25] and telomeric ends [29].

Materials and Methods

Proteins

Recombinant histidine-tagged WRN protein and the exonuclease-dead E84A mutant (X-WRN) were purified using a baculovirus/insect cell expression system and an AKTA Explorer FLPC (GE Healthcare, Piscataway, NJ) as previously described [60] except the HiLoad 16/60 Superdex 200 pg column was replaced with a HiTrap Phenyl HP column. Briefly, fractions containing WRN eluted off the HisTrap FF column were diluted to obtain final concentrations of 2 M NaCl in 20 mM phosphate buffer pH 7.4, 10% glycerol and 0.05% igepal CA-630. The eluent was loaded onto a HiTrap Phenyl HP column equilibrated with HIC buffer (20 mM phosphate buffer pH 7.4, 10% glycerol and 0.05% igepal CA-630) and washed once with HIC buffer containing 1.55 M NaCl prior to elution with 950 mM NaCl in HIC buffer. The eluted fractions containing WRN were loaded onto a HiTrap Desalt 5 ml column to exchange the buffer before loading onto a 1 ml Resource Q column for removal of remaining contaminants as described previously [60]. The concentration of active protein was determined by Bradford Assay (BioRad, Hercules, CA) and standard helicase reactions with a 16-bp forked duplex. Purity was determined by SDS-PAGE and Coomassie staining. All restriction enzymes were from New England Biolabs (Ipswich, MA). RecA protein was from USB Corporation (Cleveland, OH).

DNA Substrates

All oligonucleotides used in this study (Table 1) were from Integrated DNA Technologies (Coralville, IA) and were purified by PAGE or HPLC by the manufacturer. Oligonucleotides were 5′ end-labeled with [γ-32P] ATP (3000 Ci/mmol) (Perkin Elmer, Waltham, MA) using T4 polynucleotide kinase (New England BioLabs, Ipswich, MA), according to the manufacturer's instructions. The plasimds used for making the various 84-bp non-telomeric and telomeric (Tel) D-loops were constructed by cloning the sequence (TTAGGG)10 (Tel10 plasmid) or the scrambled sequence 5′- ATC GGT ATT GGC TTA GCA CTG GCA ATC GGT CTT GCA CTG GCT ATT GGC TTA GGT ATC GCA (Non-tel 10 plasmid) between the bases 111 and 112 of the HSV-tk gene in the previously described pGTK4 plasmid [61]. The plasmids for constructing the 60-bp D-loops used in Figs. 7–8 contained the shorter insert sequence 5′-ATC GGT ATT GGC TTA GCA CTG GCA ATC GGT CTT GCA. The 6 kB plasmids were reduced to 3.6 kB to facilitate gel migration by removing 2363 bp through restriction with AccI followed by re-ligation. The plasmids were purified by two rounds of ethidium-bromide saturated CsCl equilibrium gradient ultracentrifugation (Loftstrand Labs, Gaithersburg, MD). The plasmid based D-loop substrates were constructed as described previously [62]. Briefly RecA (4 µM) was incubated with the invading strand oligonucleotide (3.6 µM nucleotide) for 5 min at 37°C, then the supercoiled plasmid (300 µM nucleotides) was added and incubated for 3 min more. The reactions were terminated by incubation with Proteinase K and SDS for 30 min as described previously [62]. The D-loop constructs were PAGE purified by using 4.5% (37.5∶1) polyacrylamide gels. After the bands were excised the gel slices were placed in dialysis D-tubes (Novagen, Madison, WI) and were subjected to two rounds of electroelution in 1×TBE for 2–4 hrs at 4°C and 120 V. The D-loops were concentrated and exchanged into storage buffer (10 mM Tris-HCl (pH 7.5), 10 mM MgCl2) using micron-30 devices (Amicon). Purification quality and yields were determined by analysis on 4–20% native polyacrylamide gels, followed by visualization and quantitation with a Typhoon phosphorimager and ImageQuant software (GE Healthcare, Piscataway, NJ). Restriction digest analysis of the invading strand in the plasmid D-loops was conducted in reactions (20 µl) containing 50 pM purified D-loops and 10 units of the restriction enzyme indicated in Fig. 1 for 4–5 hr at 37°C, according to the manufacturer's protocol. Products were analyzed on a 14% denaturing polyacrylamide gel.

The 83-bp long forked duplex was constructed by annealing 9 pmol of the 5′end labeled Fork-G oligonucleotide (Table 1) with 12 pmol of the Fork-C complementary strand in 50 µl with 50 mM LiCl at 95°C for 5 min, followed by cooling to room temperature. In order to achieve the final 83-bp length, the fork was restricted with HaeIII and then PAGE purified by running on 8% native polyacrylamide gel and using Qiaex II Gel Extraction Kit (Qiagen, Valencia, CA). Product purity and yield were determined by native PAGE and phosphorimager analysis.

Helicase branch migration and exonuclease reactions

Reactions were performed in standard reaction buffer containing 40 mM Tris-HCl, pH 8.0, 4 mM MgCl2, 5 mM DTT, 100 µg/µl BSA, 14–28 ng/µl yeast tRNA, and 20 mM ATP [42] unless otherwise indicated. DNA substrate and protein concentrations were as indicated in the figure legends. The reactions were initiated by adding WRN protein and were incubated at 37°C for 15 minutes, unless otherwise indicated. For reactions with D-loops containing a biotinylated nucleotide the substrate was pre-incubated at 37°C for 10 minutes in buffer alone or with 1.5 nM streptavidin prior to WRN addition. For analysis of radiolabeled molecules on 4–20% native polyacrylamide gels, the reactions (10 µL) were stopped with 5 µL of 3× stop dye supplemented with 10 µg/mL proteinase K [42] and de-proteinized for 15 min at 37°C. For analysis of the radio-labeled molecules on 14% denaturing gels, the reactions were terminated with an equal volume of formamide stop dye [42]. The helicase reactions with the 83-bp forked duplex were terminated in 3× stop dye with a 10-fold molar excess of cold competitor oligonucleotide to prevent reannealing of the unwound products. After drying the gels, the reactions were visualized using a Typhoon phosphorimager and quantified using ImageQuant software (GE Healthcare, Piscataway, NJ).

For quantitation of strand displacement the percent of displaced products (full length and shortened) were calculated as a function of the total radioactivity in the reaction lane [37]. All values were corrected for background in the no enzyme control and heat denatured substrate lanes.

Supporting Information

[Figure omitted. See PDF.]

Figure S1.

WRN helicase cannot completely unwind an 83 bp telomeric forked duplex. Reactions contained 50 pM of the 84-bp forked duplex containing ten telomeric repeats (thick black line) flanked by 15 and 8 bp of unique sequence. The substrate was incubated with WRN concentrations increasing by doubling steps from 0.039 to 5 nM for 15 min under standard reaction conditions. Reactions were run on an 8% native gel.

https://doi.org/10.1371/journal.pone.0004825.s001

(1.17 MB EPS)

Figure S2.

WRN exonuclease digests free 120 nt single strands. Reactions contained 50 pM of the 5′Tail non-telomeric oligonucleotide (panel A, lanes 1–7; panel B, lanes 1–4) or the telomeric (5′Tail Tel) oligonucleotide (panel A, lanes 8–14; panel B, lanes 5–8) (see Table 1). The substrate was incubated with increasing WRN concentrations (0, 0.15, 0.31, 0.62, 1.2, 2.5 or 5 nM) (panel A) or E84A-WRN mutant (0, 1.2, 2.5, or 5 nM) (panel B) for 15 min under standard reaction conditions. Reactions were run on a 14% denaturing polyacrylamide gel.

https://doi.org/10.1371/journal.pone.0004825.s002

(3.57 MB EPS)

Figure S3.

Kinetics of WRN branch migration activity on plasmid D-loops. Reactions contained 50 pM of either the 5′Tail, No Tail, or 3′ Tail plasmid D-loops as indicated. The 5′ labeled end is indicated with a star. The substrate was incubated with 5 nM E84A-WRN under standard reaction conditions (Panel A) or wild type WRN (Panel B) under modified conditions in which Mg2+ was reduced to 1 mM. Aliquots were removed at 0, 0.5, 1, 2, 4, 8, 15, 30 min and terminated. Reactions were run on 4–20% polyacrylamide native gels and visualized by phosphorimager analysis. Δ, heat denatured substrate. The quantification of the reactions in Panel A is shown in Fig. 6C. B. The percent total displacement was calculated as described in Materials and Methods and plotted against time for reactions with wild type WRN and limiting Mg2+. 5′Tail D-loop, square and black line; 3′ Tail D-loop, triangle and blue line; No Tail D-loop, inverted triangle and yellow line.

https://doi.org/10.1371/journal.pone.0004825.s003

(2.53 MB EPS)

Acknowledgments

We thank the Opresko lab and Dr. Bennett Van Houten for critical reading of the manuscript.

Author Contributions

Conceived and designed the experiments: PLO GS HW. Performed the experiments: PLO GS HW. Analyzed the data: PLO GS HW. Contributed reagents/materials/analysis tools: PLO GS HW. Wrote the paper: PLO.

Citation: Opresko PL, Sowd G, Wang H (2009) The Werner Syndrome Helicase/Exonuclease Processes Mobile D-Loops through Branch Migration and Degradation. PLoS ONE4(3): e4825. https://doi.org/10.1371/journal.pone.0004825

References

1. Kudlow BA, Kennedy BK, Monnat RJ Jr (2007) Werner and Hutchinson-Gilford progeria syndromes: mechanistic basis of human progeroid diseases. Nat Rev Mol Cell Biol 8: 394–404.BA KudlowBK KennedyRJ Monnat Jr2007Werner and Hutchinson-Gilford progeria syndromes: mechanistic basis of human progeroid diseases.Nat Rev Mol Cell Biol8394404

2. Yu CE, Oshima J, Fu YH, Wijsman EM, Hisama F, et al. (1996) Positional cloning of the Werner's syndrome gene. Science 272: 258–262.CE YuJ. OshimaYH FuEM WijsmanF. Hisama1996Positional cloning of the Werner's syndrome gene.Science272258262

3. Hickson ID (2003) RecQ helicases: caretakers of the genome. Nat Rev Cancer 3: 169–178.ID Hickson2003RecQ helicases: caretakers of the genome.Nat Rev Cancer3169178

4. Opresko PL, Cheng WH, Bohr VA (2004) Junction of RecQ helicase biochemistry and human disease. J Biol Chem 279: 18099–18102.PL OpreskoWH ChengVA Bohr2004Junction of RecQ helicase biochemistry and human disease.J Biol Chem2791809918102

5. Brosh RM Jr, Bohr VA (2007) Human premature aging, DNA repair and RecQ helicases. Nucleic Acids Res 35: 7527–7544.RM Brosh JrVA Bohr2007Human premature aging, DNA repair and RecQ helicases.Nucleic Acids Res3575277544

6. Sung P, Klein H (2006) Mechanism of homologous recombination: mediators and helicases take on regulatory functions. Nat Rev Mol Cell Biol 7: 739–750.P. SungH. Klein2006Mechanism of homologous recombination: mediators and helicases take on regulatory functions.Nat Rev Mol Cell Biol7739750

7. Wu L, Hickson ID (2006) DNA helicases required for homologous recombination and repair of damaged replication forks. Annu Rev Genet 40: 279–306.L. WuID Hickson2006DNA helicases required for homologous recombination and repair of damaged replication forks.Annu Rev Genet40279306

8. Heller RC, Marians KJ (2006) Replisome assembly and the direct restart of stalled replication forks. Nat Rev Mol Cell Biol 7: 932–943.RC HellerKJ Marians2006Replisome assembly and the direct restart of stalled replication forks.Nat Rev Mol Cell Biol7932943

9. Tarsounas M, West SC (2005) Recombination at mammalian telomeres: an alternative mechanism for telomere protection and elongation. Cell Cycle 4: 672–674.M. TarsounasSC West2005Recombination at mammalian telomeres: an alternative mechanism for telomere protection and elongation.Cell Cycle4672674

10. Sung P (1994) Catalysis of ATP-dependent homologous DNA pairing and strand exchange by yeast RAD51 protein. Science 265: 1241–1243.P. Sung1994Catalysis of ATP-dependent homologous DNA pairing and strand exchange by yeast RAD51 protein.Science26512411243

11. McIlwraith MJ, Vaisman A, Liu Y, Fanning E, Woodgate R, et al. (2005) Human DNA polymerase eta promotes DNA synthesis from strand invasion intermediates of homologous recombination. Mol Cell 20: 783–792.MJ McIlwraithA. VaismanY. LiuE. FanningR. Woodgate2005Human DNA polymerase eta promotes DNA synthesis from strand invasion intermediates of homologous recombination.Mol Cell20783792

12. Adams MD, McVey M, Sekelsky JJ (2003) Drosophila BLM in double-strand break repair by synthesis-dependent strand annealing. Science 299: 265–267.MD AdamsM. McVeyJJ Sekelsky2003Drosophila BLM in double-strand break repair by synthesis-dependent strand annealing.Science299265267

13. Schwacha A, Kleckner N (1995) Identification of double Holliday junctions as intermediates in meiotic recombination. Cell 83: 783–791.A. SchwachaN. Kleckner1995Identification of double Holliday junctions as intermediates in meiotic recombination.Cell83783791

14. Bugreev DV, Yu X, Egelman EH, Mazin AV (2007) Novel pro- and anti-recombination activities of the Bloom's syndrome helicase. Genes Dev 21: 3085–3094.DV BugreevX. YuEH EgelmanAV Mazin2007Novel pro- and anti-recombination activities of the Bloom's syndrome helicase.Genes Dev2130853094

15. Hu Y, Raynard S, Sehorn MG, Lu X, Bussen W, et al. (2007) RECQL5/Recql5 helicase regulates homologous recombination and suppresses tumor formation via disruption of Rad51 presynaptic filaments. Genes Dev 21: 3073–3084.Y. HuS. RaynardMG SehornX. LuW. Bussen2007RECQL5/Recql5 helicase regulates homologous recombination and suppresses tumor formation via disruption of Rad51 presynaptic filaments.Genes Dev2130733084

16. Bugreev DV, Brosh RM Jr, Mazin AV (2008) RECQ1 Possesses DNA Branch Migration Activity. J Biol Chem 283: 20231–20242.DV BugreevRM Brosh JrAV Mazin2008RECQ1 Possesses DNA Branch Migration Activity.J Biol Chem2832023120242

17. Bachrati CZ, Hickson ID (2003) RecQ helicases: suppressors of tumorigenesis and premature aging. Biochem J 374: 577–606.CZ BachratiID Hickson2003RecQ helicases: suppressors of tumorigenesis and premature aging.Biochem J374577606

18. Ozsoy AZ, Ragonese HM, Matson SW (2003) Analysis of helicase activity and substrate specificity of Drosophila RECQ5. Nucleic Acids Res 31: 1554–1564.AZ OzsoyHM RagoneseSW Matson2003Analysis of helicase activity and substrate specificity of Drosophila RECQ5.Nucleic Acids Res3115541564

19. Popuri V, Bachrati CZ, Muzzolini L, Mosedale G, Costantini S, et al. (2008) The Human RecQ helicases, BLM and RECQ1, display distinct DNA substrate specificities. J Biol Chem 283: 17766–17776.V. PopuriCZ BachratiL. MuzzoliniG. MosedaleS. Costantini2008The Human RecQ helicases, BLM and RECQ1, display distinct DNA substrate specificities.J Biol Chem2831776617776

20. Wu L, Hickson ID (2003) The Bloom's syndrome helicase suppresses crossing over during homologous recombination. Nature 426: 870–874.L. WuID Hickson2003The Bloom's syndrome helicase suppresses crossing over during homologous recombination.Nature426870874

21. Huang S, Li B, Gray MD, Oshima J, Mian IS, et al. (1998) The premature ageing syndrome protein, WRN, is a 3′–>5′ exonuclease. Nat Genet 20: 114–116.S. HuangB. LiMD GrayJ. OshimaIS Mian1998The premature ageing syndrome protein, WRN, is a 3′–>5′ exonuclease.Nat Genet20114116

22. Saintigny Y, Makienko K, Swanson C, Emond MJ, Monnat JR Jr (2002) Homologous recombination resolution defect in werner syndrome. Mol Cell Biol 22: 6971–6978.Y. SaintignyK. MakienkoC. SwansonMJ EmondJR Monnat Jr2002Homologous recombination resolution defect in werner syndrome.Mol Cell Biol2269716978

23. Dhillon KK, Sidorova J, Saintigny Y, Poot M, Gollahon K, et al. (2007) Functional role of the Werner syndrome RecQ helicase in human fibroblasts. Aging Cell 6: 53–61.KK DhillonJ. SidorovaY. SaintignyM. PootK. Gollahon2007Functional role of the Werner syndrome RecQ helicase in human fibroblasts.Aging Cell65361

24. Prince PR, Emond MJ, Monnat RJ Jr (2001) Loss of Werner syndrome protein function promotes aberrant mitotic recombination. Genes Dev 15: 933–938.PR PrinceMJ EmondRJ Monnat Jr2001Loss of Werner syndrome protein function promotes aberrant mitotic recombination.Genes Dev15933938

25. Swanson C, Saintigny Y, Emond MJ, Monnat RJ Jr (2004) The Werner syndrome protein has separable recombination and survival functions. DNA Repair 3: 475–482.C. SwansonY. SaintignyMJ EmondRJ Monnat Jr2004The Werner syndrome protein has separable recombination and survival functions.DNA Repair3475482

26. Crabbe L, Verdun RE, Haggblom CI, Karlseder J (2004) Defective telomere lagging strand synthesis in cells lacking WRN helicase activity. Science 306: 1951–1953.L. CrabbeRE VerdunCI HaggblomJ. Karlseder2004Defective telomere lagging strand synthesis in cells lacking WRN helicase activity.Science30619511953

27. Bai Y, Murnane JP (2003) Telomere instability in a human tumor cell line expressing a dominant-negative WRN protein. Hum Genet 113: 337–347.Y. BaiJP Murnane2003Telomere instability in a human tumor cell line expressing a dominant-negative WRN protein.Hum Genet113337347

28. Laud PR, Multani AS, Bailey SM, Wu L, Ma J, et al. (2005) Elevated telomere-telomere recombination in WRN-deficient, telomere dysfunctional cells promotes escape from senescence and engagement of the ALT pathway. Genes Dev 19: 2560–2570.PR LaudAS MultaniSM BaileyL. WuJ. Ma2005Elevated telomere-telomere recombination in WRN-deficient, telomere dysfunctional cells promotes escape from senescence and engagement of the ALT pathway.Genes Dev1925602570

29. Li B, Jog SP, Reddy S, Comai L (2008) WRN controls formation of extrachromosomal telomeric circles and is required for TRF2DeltaB-mediated telomere shortening. Mol Cell Biol 28: 1892–1904.B. LiSP JogS. ReddyL. Comai2008WRN controls formation of extrachromosomal telomeric circles and is required for TRF2DeltaB-mediated telomere shortening.Mol Cell Biol2818921904

30. Chai W, Du Q, Shay JW, Wright WE (2006) Human telomeres have different overhang sizes at leading versus lagging strands. Mol Cell 21: 427–435.W. ChaiQ. DuJW ShayWE Wright2006Human telomeres have different overhang sizes at leading versus lagging strands.Mol Cell21427435

31. Griffith JD, Comeau L, Rosenfield S, Stansel RM, Bianchi A, et al. (1999) Mammalian telomeres end in a large duplex loop. Cell 97: 503–514.JD GriffithL. ComeauS. RosenfieldRM StanselA. Bianchi1999Mammalian telomeres end in a large duplex loop.Cell97503514

32. Wang RC, Smogorzewska A, De Lange T (2004) Homologous recombination generates T-loop-sized deletions at human telomeres. Cell 119: 355–368.RC WangA. SmogorzewskaT. De Lange2004Homologous recombination generates T-loop-sized deletions at human telomeres.Cell119355368

33. de LT (2005) Shelterin: the protein complex that shapes and safeguards human telomeres. Genes Dev 19: 2100–2110.LT de2005Shelterin: the protein complex that shapes and safeguards human telomeres.Genes Dev1921002110

34. Johnson FB, Marciniak RA, McVey M, Stewart SA, Hahn WC, et al. (2001) The Saccharomyces cerevisiae WRN homolog Sgs1p participates in telomere maintenance in cells lacking telomerase. EMBO J 20: 905–913.FB JohnsonRA MarciniakM. McVeySA StewartWC Hahn2001The Saccharomyces cerevisiae WRN homolog Sgs1p participates in telomere maintenance in cells lacking telomerase.EMBO J20905913

35. Cohen H, Sinclair DA (2001) Recombination-mediated lengthening of terminal telomeric repeats requires the Sgs1 DNA helicase. Proc Natl Acad Sci 98: 3174–3179.H. CohenDA Sinclair2001Recombination-mediated lengthening of terminal telomeric repeats requires the Sgs1 DNA helicase.Proc Natl Acad Sci9831743179

36. Orren DK, Theodore S, Machwe A (2002) The Werner Syndrome Helicase/Exonuclease (WRN) Disrupts and Degrades D- Loops in Vitro. Biochemistry 41: 13483–13488.DK OrrenS. TheodoreA. Machwe2002The Werner Syndrome Helicase/Exonuclease (WRN) Disrupts and Degrades D- Loops in Vitro.Biochemistry411348313488

37. Opresko PL, Otterlei M, Graakjaer J, Bruheim P, Dawut L, et al. (2004) The Werner Syndrome Helicase and Exonuclease Cooperate to Resolve Telomeric D Loops in a Manner Regulated by TRF1 and TRF2. Mol Cell 14: 763–774.PL OpreskoM. OtterleiJ. GraakjaerP. BruheimL. Dawut2004The Werner Syndrome Helicase and Exonuclease Cooperate to Resolve Telomeric D Loops in a Manner Regulated by TRF1 and TRF2.Mol Cell14763774

38. Opresko PL, Mason PA, Podell ER, Lei M, Hickson ID, et al. (2005) POT1 stimulates RecQ helicases WRN and BLM to unwind telomeric DNA substrates. J Biol Chem 280: 32069–32080.PL OpreskoPA MasonER PodellM. LeiID Hickson2005POT1 stimulates RecQ helicases WRN and BLM to unwind telomeric DNA substrates.J Biol Chem2803206932080

39. Opresko PL (2007) Telomere ResQue and preservation-Roles for the Werner syndrome protein and other RecQ helicases. Mech Ageing Dev 129: 79–90.PL Opresko2007Telomere ResQue and preservation-Roles for the Werner syndrome protein and other RecQ helicases.Mech Ageing Dev1297990

40. Opresko PL, von Kobbe C, Laine JP, Harrigan J, Hickson ID, et al. (2002) Telomere-binding Protein TRF2 Binds to and Stimulates the Werner and Bloom Syndrome Helicases. J Biol Chem 277: 41110–41119.PL OpreskoC. von KobbeJP LaineJ. HarriganID Hickson2002Telomere-binding Protein TRF2 Binds to and Stimulates the Werner and Bloom Syndrome Helicases.J Biol Chem2774111041119

41. Brosh RM Jr, Orren DK, Nehlin JO, Ravn PH, Kenny MK, et al. (1999) Functional and physical interaction between WRN helicase and human replication protein A. J Biol Chem 274: 18341–18350.RM Brosh JrDK OrrenJO NehlinPH RavnMK Kenny1999Functional and physical interaction between WRN helicase and human replication protein A.J Biol Chem2741834118350

42. Opresko PL, Laine JP, Brosh RM Jr, Seidman MM, Bohr VA (2001) Coordinate Action of the Helicase and 3′ to 5′ Exonuclease of Werner Syndrome Protein. J Biol Chem 276: 44677–44687.PL OpreskoJP LaineRM Brosh JrMM SeidmanVA Bohr2001Coordinate Action of the Helicase and 3′ to 5′ Exonuclease of Werner Syndrome Protein.J Biol Chem2764467744687

43. Choudhary S, Sommers JA, Brosh RM Jr (2004) Biochemical and kinetic characterization of the DNA helicase and exonuclease activities of werner syndrome protein. J Biol Chem 279: 34603–34613.S. ChoudharyJA SommersRM Brosh Jr2004Biochemical and kinetic characterization of the DNA helicase and exonuclease activities of werner syndrome protein.J Biol Chem2793460334613

44. Perry JJ, Yannone SM, Holden LG, Hitomi C, Asaithamby A, et al. (2006) WRN exonuclease structure and molecular mechanism imply an editing role in DNA end processing. Nat Struct Mol Biol 13: 414–422.JJ PerrySM YannoneLG HoldenC. HitomiA. Asaithamby2006WRN exonuclease structure and molecular mechanism imply an editing role in DNA end processing.Nat Struct Mol Biol13414422

45. Choi JM, Kang SY, Bae WJ, Jin KS, Ree M, et al. (2007) Probing the roles of active site residues in the 3′-5′ exonuclease of the Werner syndrome protein. J Biol Chem 282: 9941–9951.JM ChoiSY KangWJ BaeKS JinM. Ree2007Probing the roles of active site residues in the 3′-5′ exonuclease of the Werner syndrome protein.J Biol Chem28299419951

46. Machwe A, Xiao L, Orren DK (2006) Length-dependent degradation of single-stranded 3′ ends by the Werner syndrome protein (WRN): implications for spatial orientation and coordinated 3′ to 5′ movement of its ATPase/helicase and exonuclease domains. BMC Mol Biol 7: 6.A. MachweL. XiaoDK Orren2006Length-dependent degradation of single-stranded 3′ ends by the Werner syndrome protein (WRN): implications for spatial orientation and coordinated 3′ to 5′ movement of its ATPase/helicase and exonuclease domains.BMC Mol Biol76

47. Kamath-Loeb AS, Shen JC, Loeb LA, Fry M (1998) Werner Syndrome Protein. Ii. characterization of the integral 3′–>5′ dna exonuclease. J Biol Chem 273: 34145–34150.AS Kamath-LoebJC ShenLA LoebM. Fry1998Werner Syndrome Protein. Ii. characterization of the integral 3′–>5′ dna exonuclease.J Biol Chem2733414534150

48. Bachrati CZ, Borts RH, Hickson ID (2006) Mobile D-loops are a preferred substrate for the Bloom's syndrome helicase. Nucleic Acids Res 34: 2269–2279.CZ BachratiRH BortsID Hickson2006Mobile D-loops are a preferred substrate for the Bloom's syndrome helicase.Nucleic Acids Res3422692279

49. Brosh RM Jr, Waheed J, Sommers JA (2002) Biochemical characterization of the DNA substrate specificity of werner syndrome helicase. J Biol Chem 277: 23236–23245.RM Brosh JrJ. WaheedJA Sommers2002Biochemical characterization of the DNA substrate specificity of werner syndrome helicase.J Biol Chem2772323623245

50. Constantinou A, Tarsounas M, Karow JK, Brosh RM, Bohr VA, et al. (2000) Werner's syndrome protein (WRN) migrates Holliday junctions and co- localizes with RPA upon replication arrest. EMBO Rep 1: 80–84.A. ConstantinouM. TarsounasJK KarowRM BroshVA Bohr2000Werner's syndrome protein (WRN) migrates Holliday junctions and co- localizes with RPA upon replication arrest.EMBO Rep18084

51. Machwe A, Xiao L, Theodore S, Orren DK (2002) DNase I footprinting and enhanced exonuclease function of the bipartite Werner syndrome protein (WRN) bound to partially melted duplex DNA. J Biol Chem 277: 4492–4504.A. MachweL. XiaoS. TheodoreDK Orren2002DNase I footprinting and enhanced exonuclease function of the bipartite Werner syndrome protein (WRN) bound to partially melted duplex DNA.J Biol Chem27744924504

52. Compton SA, Tolun G, Kamath-Loeb AS, Loeb LA, Griffith JD (2008) The Werner syndrome protein binds replication fork and holliday junction DNAs as an oligomer. J Biol Chem 283: 24478–24483.SA ComptonG. TolunAS Kamath-LoebLA LoebJD Griffith2008The Werner syndrome protein binds replication fork and holliday junction DNAs as an oligomer.J Biol Chem2832447824483

53. Driscoll HC, Matson SW, Sayer JM, Kroth H, Jerina DM, et al. (2003) Inhibition of Werner syndrome helicase activity by benzo[c]phenanthrene diol epoxide dA adducts in DNA is both strand-and stereoisomer-dependent. J Biol Chem 278: 41126–41135.HC DriscollSW MatsonJM SayerH. KrothDM Jerina2003Inhibition of Werner syndrome helicase activity by benzo[c]phenanthrene diol epoxide dA adducts in DNA is both strand-and stereoisomer-dependent.J Biol Chem2784112641135

54. Baumann P, Benson FE, West SC (1996) Human Rad51 protein promotes ATP-dependent homologous pairing and strand transfer reactions in vitro. Cell 87: 757–766.P. BaumannFE BensonSC West1996Human Rad51 protein promotes ATP-dependent homologous pairing and strand transfer reactions in vitro.Cell87757766

55. McIlwraith MJ, Van DE, Masson JY, Stasiak AZ, Stasiak A, et al. (2000) Reconstitution of the strand invasion step of double-strand break repair using human Rad51 Rad52 and RPA proteins. J Mol Biol 304: 151–164.MJ McIlwraithDE VanJY MassonAZ StasiakA. Stasiak2000Reconstitution of the strand invasion step of double-strand break repair using human Rad51 Rad52 and RPA proteins.J Mol Biol304151164

56. Donmez I, Rajagopal V, Jeong YJ, Patel SS (2007) Nucleic acid unwinding by hepatitis C virus and bacteriophage t7 helicases is sensitive to base pair stability. J Biol Chem 282: 21116–21123.I. DonmezV. RajagopalYJ JeongSS Patel2007Nucleic acid unwinding by hepatitis C virus and bacteriophage t7 helicases is sensitive to base pair stability.J Biol Chem2822111621123

57. SantaLucia J Jr. (1998) A unified view of polymer, dumbbell, and oligonucleotide DNA nearest-neighbor thermodynamics. Proc Natl Acad Sci U S A 95: 1460–1465.J. SantaLucia Jr.1998A unified view of polymer, dumbbell, and oligonucleotide DNA nearest-neighbor thermodynamics.Proc Natl Acad Sci U S A9514601465

58. Mohaghegh P, Karow JK, Brosh JR Jr, Bohr VA, Hickson ID (2001) The Bloom's and Werner's syndrome proteins are DNA structure-specific helicases. Nucleic Acids Res 29: 2843–2849.P. MohagheghJK KarowJR Brosh JrVA BohrID Hickson2001The Bloom's and Werner's syndrome proteins are DNA structure-specific helicases.Nucleic Acids Res2928432849

59. Verdun RE, Crabbe L, Haggblom C, Karlseder J (2005) Functional human telomeres are recognized as DNA damage in g2 of the cell cycle. Mol Cell 20: 551–561.RE VerdunL. CrabbeC. HaggblomJ. Karlseder2005Functional human telomeres are recognized as DNA damage in g2 of the cell cycle.Mol Cell20551561

60. Sowd G, Lei M, Opresko PL (2008) Mechanism and substrate specificity of telomeric protein POT1 stimulation of the Werner syndrome helicase. Nucleic Acids Res 36: 4242–4256.G. SowdM. LeiPL Opresko2008Mechanism and substrate specificity of telomeric protein POT1 stimulation of the Werner syndrome helicase.Nucleic Acids Res3642424256

61. Hile SE, Yan G, Eckert KA (2000) Somatic mutation rates and specificities at TC/AG and GT/CA microsatellite sequences in nontumorigenic human lymphoblastoid cells. Cancer Res 60: 1698–1703.SE HileG. YanKA Eckert2000Somatic mutation rates and specificities at TC/AG and GT/CA microsatellite sequences in nontumorigenic human lymphoblastoid cells.Cancer Res6016981703

62. Bachrati CZ, Hickson ID (2006) Analysis of the DNA unwinding activity of RecQ family helicases. Methods Enzymol 409: 86–100.CZ BachratiID Hickson2006Analysis of the DNA unwinding activity of RecQ family helicases.Methods Enzymol40986100

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© 2009 Opresko et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.

Abstract

RecQ DNA helicases are critical for preserving genome integrity. Of the five RecQ family members identified in humans, only the Werner syndrome protein (WRN) possesses exonuclease activity. Loss of WRN causes the progeroid disorder Werner syndrome which is marked by cancer predisposition. Cellular evidence indicates that WRN disrupts potentially deleterious intermediates in homologous recombination (HR) that arise in genomic and telomeric regions during DNA replication and repair. Precisely how the WRN biochemical activities process these structures is unknown, especially since the DNA unwinding activity is poorly processive. We generated biologically relevant mobile D-loops which mimic the initial DNA strand invasion step in HR to investigate whether WRN biochemical activities can disrupt this joint molecule. We show that WRN helicase alone can promote branch migration through an 84 base pair duplex region to completely displace the invading strand from the D-loop. However, substrate processing is altered in the presence of the WRN exonuclease activity which degrades the invading strand both prior to and after release from the D-loop. Furthermore, telomeric D-loops are more refractory to disruption by WRN, which has implications for tighter regulation of D-loop processing at telomeres. Finally, we show that WRN can recognize and initiate branch migration from both the 5′ and 3′ ends of the invading strand in the D-loops. These findings led us to propose a novel model for WRN D-loop disruption. Our biochemical results offer an explanation for the cellular studies that indicate both WRN activities function in processing HR intermediates.

Details

Title
The Werner Syndrome Helicase/Exonuclease Processes Mobile D-Loops through Branch Migration and Degradation
Author
Opresko, Patricia L; Sowd, Gregory; Wang, Hong
First page
e4825
Section
Research Article
Publication year
2009
Publication date
Mar 2009
Publisher
Public Library of Science
e-ISSN
19326203
Source type
Scholarly Journal
Language of publication
English
DOI
https://doi.org/10.1371/journal.pone.0004825
ProQuest document ID
1290165826
Copyright
© 2009 Opresko et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.