Recombination Mediator Proteins: Misnomers That Are Key to Understanding the Genomic Instabilities in Cancer

Recombination mediator proteins have come into focus as promising targets for cancer therapy, with synthetic lethal approaches now clinically validated by the efficacy of PARP inhibitors in treating BRCA2 cancers and RECQ inhibitors in treating cancers with microsatellite instabilities. Thus, understanding the cellular role of recombination mediators is critically important, both to improve current therapies and develop new ones that target these pathways. Our mechanistic understanding of BRCA2 and RECQ began in Escherichia coli. Here, we review the cellular roles of RecF and RecQ, often considered functional homologs of these proteins in bacteria. Although these proteins were originally isolated as genes that were required during replication in sexual cell cycles that produce recombinant products, we now know that their function is similarly required during replication in asexual or mitotic-like cell cycles, where recombination is detrimental and generally not observed. Cells mutated in these gene products are unable to protect and process replication forks blocked at DNA damage, resulting in high rates of cell lethality and recombination events that compromise genome integrity during replication.

Replication substrates created during encounters with DNA damage 3.
The RecF pathway maintains replication following disruption by DNA damage 4.
RecF, RecO, and RecR are required to maintain the replication fork and restore processive replication 5.
RecJ and RecQ process the replication forks following DNA damage to promote resumption from the site where disruption occurred 6.
Evidence that lesion repair occurs at disrupted replication forks to prevent mutations or rearrangements by translesion synthesis or recombination 7.
Maintaining and restoring processive replication is specific to the RecF pathway 8.
Recombination mediators are functionally conserved between bacteria and mammals

Nonrecombinational Roles of Recombination Mediators during Replication
The RecF pathway gene products are often referred to as recombinational mediators and include RecF, RecO, and RecR, along with the processing enzymes RecJ and RecQ. The manner in which a gene is discovered can have a profound effect upon, and often bias, the way in which we think about its cellular function. Meiotic cell cycles, despite being extremely rare, have received a disproportionate amount of scientific attention relative to their mitotic counterparts. Unlike mitosis, these rare specialized cell cycles scramble the genome rather than maintain it, producing 'hybrid' or recombinant DNA molecules derived from two different parents. Although bacteria were long considered to be asexual, ble the genome rather than maintain it, producing 'hybrid' or recombinant DNA molecules derived from two different parents. Although bacteria were long considered to be asexual, following the discovery of conjugation and natural transformation, it became clear that bacteria also had true sexual reproductive cycles that produced hybrid DNA molecules [1]. Recognizing the parallel between bacterial sex and meiosis, Clark and Margulies undertook a genetic screen with the goal of identifying the 'rec' enzymes that were required to produce the recombination events (rearrangements) generating genetic diversity during sexual cycles using E. coli as a model [2][3][4]. It quickly became apparent that mutations in many of these gene products also rendered cells hypersensitive to DNA damage during normal growth [2,5], indicating that these proteins functioned during asexual cell cycles as well. At the time, the only known property of these proteins was that they were required for recombinational products to form during sex. As such, models were developed that speculated recombination occurred in asexual cells as a mechanism of repair [6,7].
However, this early proposal set up a paradox that is difficult to resolve with what is observed in humans and the development of cancer. Essentially, it implies that since recombination is acting as a repair mechanism, the more recombination events observed after DNA damage, the better off the cells should be. However, unlike the specialized events occurring in sex cells, strand exchanges are not normally observed during asexual replicative cycles. Additionally, when recombination events are observed, they are detrimental to the genomic stability and viability of the cell ( Figure 1A). In the clinic, mitotic strand exchange frequencies are used diagnostically and prognostically as markers for cancer and correlate directly with genomic instability, cell death, and carcinogenic transformation [8][9][10][11][12][13][14][15][16].  In healthy cells, few exchanges are observed. By contrast, in cells lacking BLM, a RecQ homolog, recombination events are observed more frequently, and patients are predisposed to developing cancer. RecQ in E. coli is similarly required to suppress illegitimate recombination from occurring [17]. Photos generously provided by S. Wolff and A. A. Sandberg. (B) Experiment demonstrating that DNA damage-induced recombinational exchanges can be observed during replication in E. coli. By growing cells in different isotopic media, the DNA made before and after UV irradiation can be separated based upon their buoyant density in isopycnic alkali CsCl gradients. To test whether recombination can be induced by UV lesions, uvrA mutants defective in nucleotide excision repair were UV irradiated and allowed to recover for one hour. Unlike unirradiated uvrA mutants or irradiated wild-type cells, the DNA made in irradiated uvrA cultures contained more DNA at an intermediate density, demonstrating exchanges between the parental and daughter DNA strands are occurring in these cells (redrawn from [18] which reproduce results reported in [7]). (C) and (D) Although these exchanges were originally interpreted to represent a repair mechanism, the populations in which they were observed and characterized were rendered inviable by the UV treatment.
The same correlation between cell death, genome instability, and the frequency of recombination also occurs in bacteria. In populations undergoing extensive recombination, high levels of genomic instability and cell death also occur [6,7,. This concept is often lost because in the initial studies that characterized replication following DNA damage, recombination was hypothesized to function as a repair mechanism ( Figure 1B). However, in order to observe strand exchanges after DNA damage, these initial studies found it necessary to carry out their experiments in repair-deficient strains (uvr mutants), using doses that were lethal for the populations in which the exchanges were characterized [6,7,49] (Figure 1C,D). Essentially all subsequent studies followed this example [6,7,, excluding DNA repair as a step in the recovery process, and characterizing the process in uvr mutant populations where few of the cells remained viable. Thus, one cannot separate the presence of recombination events from cell death and genomic instability. Additionally, although it was not considered in these original articles, the lack of viability in cells where the recombination events are characterized makes a strong argument for the idea that DNA damage-induced recombination is not acting as a mechanism of repair, but is an aberrant, sometimes lethal, event that results when the normal pathway of recovery is impaired or cannot occur.

Replication Substrates Created during Encounters with DNA Damage
One interesting feature of the substrates generated by replicational encounters with DNA damage is that their structure varies depending upon which template strand contains the DNA lesion. Since DNA polymerization on both strands occurs in a 5 -3 direction, coordinated replication of both templates requires unique enzymatic dynamics for each strand. While the leading-strand template can be synthesized in a continuous, processive 5 -3 manner, the lagging-strand template must be synthesized in a direction opposite to the fork's progress, and requires a primase activity that constantly "reinitiates" the lagging strand polymerization, resulting in discontinuous synthesis of the template (Okazaki fragments). These alternative mechanisms of synthesis present different problems for the replication machinery when it encounters a DNA lesion. In reconstituted systems and in vivo on plasmid substrates, several labs have shown that a blocking lesion in the leadingstrand template disrupts the replisome machinery, arresting replisome progression [72][73][74][75][76]. In contrast, lesions in the lagging-strand template do not disrupt the progression of the replisome, but result in the production of a gap on opposite the strand containing the lesion ( Figure 2). On the chromosome, the transient disruption of replication by UV is associated with an overall inhibition and the production of some limited gapped fragments, consistent with the products observed in vitro [6,18,21,55,77]. In this review, we focus primarily on those events and observations associated with lesions that disrupt the replisome's progression and the mechanism that restores it.
Genes 2022, 13, x FOR PEER REVIEW the leading-strand template disrupts the replisome machinery, arresting replisom gression [72][73][74][75][76]. In contrast, lesions in the lagging-strand template do not disrupt th gression of the replisome, but result in the production of a gap on opposite the containing the lesion (Figure 2). On the chromosome, the transient disruption of re tion by UV is associated with an overall inhibition and the production of some l gapped fragments, consistent with the products observed in vitro [6,18,21,55,77]. review, we focus primarily on those events and observations associated with lesion disrupt the replisome's progression and the mechanism that restores it.

Figure 2.
Substrates generated during replication on UV-damaged templates. Based upon o rent understanding, lesions in the leading-strand template disrupt replisome progression. trast, lesions in the lagging-strand template produce gaps but do not disrupt replication.

The RecF Pathway Maintains Replication Following Disruption by DNA Dam
The current model for how RecF pathway gene products maintain replicatio suppress illegitimate recombination is shown in Figure 3, and the supporting e mental evidence from studies using UV-induced DNA damage as a model lesion a sented in the sections that follow. 254-nm UV light induces cyclobutane pyrimid mers and 6-4 photoproducts that block DNA polymerases and disrupt replisome pr sion when encountered in the leading strand ( Figure 3A) [50,72,73,77,78]. We use th disruption to distinguish it from replisome pausing or inactivation. These latter might imply that the replisome could simply resume once a missing precursor or co is resupplied. In E. coli, the disruption of replication at UV-induced lesions involv uncoupling of leading and lagging strand synthesis, exposure of the nascent la strand DNA to exonucleolytic degradation, and the partial dissociation of the replis components [50,51,53,56,58,73,74]. The DNA polymerase, beta clamp, and tau subu the replisome dissociate from the arrested replication fork ( Figure 3B) [58]. Dissoc of these subunits, even in the absence of DNA damage, is sufficient to induce proc events that mimic those seen after DNA damage is encountered [58]. In contrast helicase and primase remain associated with the branched replication fork [58,74,79]. The integrity of the replication fork DNA structure remains intact throu the recovery process, as no 'collapsed forks', double-strand breaks, or broken linear are observed [53,57,80].
The partial disruption of the replisome exposes the nascent DNA to enzymati radation by RecJ, a 5′-3′ single-strand exonuclease, and RecQ, a complementary 3′icase ( Figure 3C) [51,53,81,82]. Together, these enzymes partially degrade the nasce ging strand of the replication fork, which restores the lesion-containing region to a d stranded form that can be repaired by nucleotide excision repair ( Figure 3D) [ 53,56,83,84]. The leading strand appears to remain protected, as degradation on this Substrates generated during replication on UV-damaged templates. Based upon our current understanding, lesions in the leading-strand template disrupt replisome progression. In contrast, lesions in the lagging-strand template produce gaps but do not disrupt replication.

The RecF Pathway Maintains Replication Following Disruption by DNA Damage
The current model for how RecF pathway gene products maintain replication and suppress illegitimate recombination is shown in Figure 3, and the supporting experimental evidence from studies using UV-induced DNA damage as a model lesion are presented in the sections that follow. 254-nm UV light induces cyclobutane pyrimidine dimers and 6-4 photoproducts that block DNA polymerases and disrupt replisome progression when encountered in the leading strand ( Figure 3A) [50,72,73,77,78]. We use the term disruption to distinguish it from replisome pausing or inactivation. These latter terms might imply that the replisome could simply resume once a missing precursor or cofactor is resupplied. In E. coli, the disruption of replication at UV-induced lesions involves the uncoupling of leading and lagging strand synthesis, exposure of the nascent laggingstrand DNA to exonucleolytic degradation, and the partial dissociation of the replisome's components [50,51,53,56,58,73,74]. The DNA polymerase, beta clamp, and tau subunits of the replisome dissociate from the arrested replication fork ( Figure 3B) [58]. Dissociation of these subunits, even in the absence of DNA damage, is sufficient to induce processing events that mimic those seen after DNA damage is encountered [58]. In contrast, both helicase and primase remain associated with the branched replication fork DNA [58,74,79]. The integrity of the replication fork DNA structure remains intact throughout the recovery process, as no 'collapsed forks', double-strand breaks, or broken linear DNA are observed [53,57,80]. however, it also remains possible that other, as yet unidentified, enzymes may catalyze this reaction. Some have postulated that branch migration enzymes, such as RecG or RuvAB, may catalyze this step [87][88][89][90]. However, these enzymes do not appear to be required for this reaction in vivo since replication fork processing and resumption of DNA synthesis occur normally in mutants lacking these enzymes [80,91]. In the absence of RecJ or RecQ, repair cannot occur and the recovery is delayed for 50 min, a time corresponding to when UmuDC translesion polymerase is activated [56]. In recJ and recQ mutants, both  The partial disruption of the replisome exposes the nascent DNA to enzymatic degradation by RecJ, a 5 -3 single-strand exonuclease, and RecQ, a complementary 3 -5 helicase ( Figure 3C) [51,53,81,82]. Together, these enzymes partially degrade the nascent lagging strand of the replication fork, which restores the lesion-containing region to a double-stranded form that can be repaired by nucleotide excision repair ( Figure 3D) [18,[51][52][53]56,83,84]. The leading strand appears to remain protected, as degradation on this strand is not detected [51,57,79]. Presumably, some partial displacement of the leading strand must also occur. We would speculate that this displacement could occur spontaneously due to positive supercoiling Genes 2022, 13, 437 6 of 29 created in the template ahead of the replication fork [85,86]; however, it also remains possible that other, as yet unidentified, enzymes may catalyze this reaction. Some have postulated that branch migration enzymes, such as RecG or RuvAB, may catalyze this step [87][88][89][90]. However, these enzymes do not appear to be required for this reaction in vivo since replication fork processing and resumption of DNA synthesis occur normally in mutants lacking these enzymes [80,91]. In the absence of RecJ or RecQ, repair cannot occur and the recovery is delayed for 50 min, a time corresponding to when UmuDC translesion polymerase is activated [56]. In recJ and recQ mutants, both Cell survival and the resumption of replication become entirely dependent on translesion DNA synthesis [56]. Additionally, this processing plays a key role in suppressing illegitimate recombination, by creating a large single-stranded region on the lagging-strand template at the replication fork for RecA to bind and pair with its sister chromatid [92][93][94][95][96]. This protects the DNA from degradation and helps to ensure that the 3 -end of the disrupted replication fork resumes on the same template, at the same site, from where disruption occurred [17,51,[62][63][64]97].
RecF, RecO, and RecR function to maintain the integrity of the replication fork DNA and are required for the replisome to reassemble and resume [50,53,54,58,79]. Together, these proteins limit the degradation by RecJ and RecQ, facilitate RecA loading onto the disrupted replisome substrate, which protects the DNA from degradation, and re-pairs the 3 nascent leading strand with its template ( Figure 3E-G). Resumption likely requires RecA to re-pair these strands to create a substrate that the replisome could then resume from. Collectively, RecF pathway activities may provide the substrate necessary for DNA polymerase, and other replisome subunits to reassociate with the helicase-primase complex and restore synthesis.

RecF, RecO, and RecR Are Required to Maintain the Replication Fork and Restore Processive Replication
If the action of a gene product is required to restore replication forks that are blocked by DNA damage, then one would predict that replication would fail to resume in its corresponding irradiated mutant. This is the phenotype exhibited by recF, recO, or recR mutants. The ability to resume replication can be monitored directly using several different approaches [77,[104][105][106][107]. One assay used to measure the ability to resume replication is shown in Figure 4A and involves growing the culture in 5-bromodeoxyuridine, a thymine analog, to quantify the amount of DNA that continues to accumulate after UV irradiation. Cultures receiving either 25 J/m 2 or no irradiation are incubated in medium containing 5-bromodeoxyuridine for 1 h, so that any DNA synthesized during this period is of a greater density than that of DNA synthesized before irradiation. The denser, replicated DNA in each culture can then be separated from the rest of the DNA in isopycnic alkaline CsCl gradients and quantified. By this measure, wild-type cells have fully recovered replication within 1 h, as the amount of replicated DNA in the irradiated culture is nearly equivalent to that of the unirradiated culture. Consistent with the idea that RecF is required to restore replication forks that encounter DNA damage, no further replication is observed in mutants lacking RecF. Other approaches used to measure the resumption of replication have also confirmed these observations [50,53,91,106]. RecF is required to maintain replication forks disrupted by DNA damage. (A) recF mutants fail to restore replication following disruption by UV-induced damage. The amount of replication occurring within 1 h after UV irradiation with 25 J/m 2 was analyzed by alkaline CsCl density gradients. Cells prelabeled with [ 14 C]thymine were irradiated or mock-irradiated, filtered, and allowed to recover for 1 h in media containing [ 3 H]5-bromodeoxyuridine to density label DNA made during this period. Circles, 14 C prelabeled DNA; squares, 3 H replicated DNA. (B) recF mutants are unable to maintain the replication fork processing observed by two-dimensional gel electrophoresis. The migration pattern in 2D agarose gels for linearized pBR322 plasmid after UV treatment. Nonreplicating plasmids run as a linear 4.4 kb fragment. Normal replicating plasmids form Y-shaped structures and migrate more slowly due to their increased size and nonlinear shape, moving as an arc that extends from the linear fragment. Replication intermediates observed after UV damage form double-Y or Xshaped structures that migrate in the cone region. Whereas processing intermediates transiently accumulate in wild-type cells after UV irradiation, no intermediates are observed in recF mutants. (C) The nascent DNA undergoes excessive degradation in recF mutants. [ 3 H]thymidine is added to [ 14 C]thymine-prelabeled cells for 10 s immediately before the cells were filtered and irradiated with 25 J/m 2 in nonradioactive medium. The fraction of the radioactivity remaining in the DNA is plotted against time. Loss of 14 C genomic DNA (open symbols) can be compared to the loss of the 3 H DNA synthesized at the growing fork just prior to irradiation (filled symbols). Squares, wild type; circles, recF. Compiled and redrawn from data reported in [18,53]. RecF is required to maintain replication forks disrupted by DNA damage. (A) recF mutants fail to restore replication following disruption by UV-induced damage. The amount of replication occurring within 1 h after UV irradiation with 25 J/m 2 was analyzed by alkaline CsCl density gradients. Cells prelabeled with [ 14 C]thymine were irradiated or mock-irradiated, filtered, and allowed to recover for 1 h in media containing [ 3 H]5-bromodeoxyuridine to density label DNA made during this period. Circles, 14 C prelabeled DNA; squares, 3 H replicated DNA. (B) recF mutants are unable to maintain the replication fork processing observed by two-dimensional gel electrophoresis. The migration pattern in 2D agarose gels for linearized pBR322 plasmid after UV treatment. Nonreplicating plasmids run as a linear 4.4 kb fragment. Normal replicating plasmids form Y-shaped structures and migrate more slowly due to their increased size and nonlinear shape, moving as an arc that extends from the linear fragment. Replication intermediates observed after UV damage form double-Y or X-shaped structures that migrate in the cone region. Whereas processing intermediates transiently accumulate in wildtype cells after UV irradiation, no intermediates are observed in recF mutants. (C) The nascent DNA undergoes excessive degradation in recF mutants. medium. The fraction of the radioactivity remaining in the DNA is plotted against time. Loss of 14 C genomic DNA (open symbols) can be compared to the loss of the 3 H DNA synthesized at the growing fork just prior to irradiation (filled symbols). Squares, wild type; circles, recF. Compiled and redrawn from data reported in [18,53].
To examine the structure of the disrupted replication forks, two-dimensional (2D) agarose gel analysis has been employed to visualize the structural intermediates associated with arrested replication forks on plasmids such as pBR322 [53,105,108]. Cells containing the plasmid pBR322 are UV irradiated, and the genomic DNA is purified, digested with a restriction enzyme that linearizes the plasmid at its unidirectional origin of replication, and analyzed by 2D agarose gels at times before and after irradiation. In this technique, nonreplicating plasmids migrate as linear 4.4 kb fragments, whereas replicating fragments form Y-shaped structures and migrate more slowly because of their larger size and nonlinear shape. These replicating fragments form an arc that extends out from the linear fragment ( Figure 4B). Following UV irradiation of wild-type cells, RecF, RecO, and RecR, together with RecA, are able to maintain the replication fork DNA, limiting the degradation that occurs. This produces a transient extrusion of the nascent DNA at the blocked replication fork that can be observed on 2D agarose gels [53]. The extruded nascent DNA converts the three-arm active replication fork structure into a four-arm arrested replication intermediate that further retards its mobility in the gel, migrating in a cone region beyond the normal replication arc. By contrast, in the absence of RecF, this extruded DNA is not maintained, the nascent lagging strand is extensively degraded, and the cone region intermediate is not observed.
The processing and degradation that occur at the disrupted replication fork in the cell can also be characterized by following the fate of the genomic and nascent DNA at the replication fork made just prior to irradiation [50,105]. In this approach, exponentially growing, [ 14 C]thymine-prelabeled cultures are pulse labeled with [ 3 H]thymidine for 10 s to label the nascent DNA at replication forks before the culture is transferred to nonradioactive medium and UV irradiated. The 14 C prelabel allows one to compare the degradation occurring in the overall genome to that in the 3 H-labeled DNA made at replication forks. By this technique, one observes that in UV-irradiated wild-type cells, the genomic DNA remains largely intact, while some limited degradation is detected in the nascent DNA at times prior to when replication recovers ( Figure 4C) [18,50,51,53]). In principle, the precipitable 3 H pulse label should remain constant or decrease over time in this assay. However, an increase in precipitable 3 H label is consistently observed in samples once replication has recovered. This is likely due to remaining intracellular pools of labeled nucleotides. In contrast to the limited degradation in wild-type cells, the degradation in recF mutants is much more extensive, resulting in a loss of approximately half of the nascent DNA at the blocked replication forks.
Taken together, the failure to restore replication, the lack of replication processing intermediates, and the degradation of the nascent fork DNA that occurs in recF mutants argue that RecF is functionally required to maintain and process replication forks at UV-induced damage in cells. Both recO and recR mutants have been shown to exhibit phenotypes identical to recF with respect to these assays [50,53,54]. These phenotypes are likely to account for the cell death that occurs in irradiated recF, recO, and recR populations.
Several lines of evidence, both in vivo and in vitro, are consistent with this model and suggest that RecF, RecO, and RecR operate at a common step in loading and stabilizing RecA filaments on the replication fork DNA. Mutants lacking any or all of these gene products are equally sensitive to DNA damage, although the sensitivity is less than that conferred by a mutation in recA [4,50,109,110]. Additionally, recF, recO, or recR mutations also similarly delay induction of LexA-regulated genes following DNA damage [111][112][113]. In E. coli, many of the genes upregulated in response to DNA damage are repressed by LexA, which binds to a 20-bp consensus sequence in the operator region of these genes [114][115][116][117]. Once loaded onto single-stranded DNA, RecA becomes conformationally active, serving as a coprotease that promotes the autocatalytic cleavage of the LexA repressor, upregulating transcription from these genes as the cellular concentration of LexA diminishes [118]. Since RecA is required to cleave and inactivate LexA repressors, this supports the idea that there is less activated RecA present at early times after DNA damage in the absence of RecF, RecO, or RecR.
In vitro, interactions between RecO and RecR, and RecF and RecR can be observed in the presence of DNA. RecF, RecO and RecR enhance the ability of RecA to bind and form filaments on single-stranded DNA that is coated with single-strand binding protein (SSB), while limiting growth of the RecA filament to the single-stranded region [95,[119][120][121][122], consistent with the general view that these proteins can stabilize RecA filaments in their activated and bound form. Fluorescently labeled fusion proteins of RecF and RecR track with the replisome in live cells [123]. However, RecO is reported to localize separately to loci in the membrane [123], the meaning of which remains unclear. It is interesting to note that recO is cotranscribed with an essential G protein, whereas recR is cotranscribed with a protein that facilitates integration of membrane-bound G proteins [124]. Speculatively, one could envision RecO providing an anchoring role for the disrupted fork substrate to the membrane where processing may occur.

RecJ and RecQ Process the Replication Forks Following DNA Damage to Promote Resumption from the Site Where Disruption Occurred
While RecF, RecO, and RecR function with RecA to maintain replication fork integrity, the processing or degradation that occurs at the replication fork following arrest is mediated by RecQ and RecJ and is necessary for faithful and rapid recovery of replication from the site of disruption [17,53,56,57,63]. RecQ is a 3 -5 helicase and RecJ is a 5 -3 singlestranded DNA exonuclease [81,82]. As noted above, replication forks arrested by DNA damage undergo processing and some limited degradation that leads to the 4-way branched intermediates observed in 2D agarose gels. In the absence of RecF, the processing is much more extensive, leading to approximately one half of the nascent DNA being degraded and a loss of the processing intermediate structure seen in irradiated wild-type cells on 2D agarose gels. In the absence of RecJ or RecQ, the nascent DNA processing that normally occurs at disrupted replication forks is not detected [51,53]. Furthermore, inactivation of either RecJ or RecQ prevents the extensive degradation of nascent DNA at the replication fork from occurring in the absence of RecF, RecO, or RecR, and restores the processing intermediates of these mutants as observed by 2D agarose gels ( Figure 5A,B) [51,53]. The observations demonstrate that the replication fork intermediates in the cone region are formed through the extrusion of the nascent DNA, and that this is the substrate acted upon by RecJ and RecQ in vivo.
To examine which strands of the nascent DNA are degraded by RecQ and RecJ, the newly synthesized DNA can be pulse labeled with 5-bromodeoxyuridine followed by isolation and enrichment in alkali CsCl gradients. Using probes specific to the leading or lagging strand, it has been shown that the degradation by RecJ and RecQ occurs on the nascent lagging strand ( Figure 5C) [51].
Degradation specific to the nascent lagging strand is consistent with the known polarities and activities of RecJ and RecQ [81,82]. Following the arrest of replication by a template leading-strand lesion, there is expected to be a 3 -end on the nascent leading strand and a 5 -end on the nascent lagging strand ( Figure 6). Based on the polarity of RecQ, which loads onto single-stranded DNA and moves in a 3 -5 direction to displace the complementary strand [82], RecQ would only be able to displace the lagging strand when loaded at the arrested replication fork. Similarly, RecJ, which is a 5 -3 exonuclease specific for single-stranded DNA [81], would only be able to degrade the lagging strand after it has been displaced by RecQ. Nucleolytic processing of the lagging strand also provides an explanation for why only 50% of the nascent DNA appears to be susceptible to degradation, even when replication is prevented from recovering as is seen in recF, recO, or recR mutants [50,51,53,54].
that normally occurs at disrupted replication forks is not detected [51,53]. Furthermore, inactivation of either RecJ or RecQ prevents the extensive degradation of nascent DNA at the replication fork from occurring in the absence of RecF, RecO, or RecR, and restores the processing intermediates of these mutants as observed by 2D agarose gels ( Figure 5A,B) [51,53]. The observations demonstrate that the replication fork intermediates in the cone region are formed through the extrusion of the nascent DNA, and that this is the substrate acted upon by RecJ and RecQ in vivo.  Although the partial degradation of the nascent lagging strand seems intuitively counterproductive, it serves to move the replication fork back and restore the lesion-containing region to a double-stranded form of DNA that would allow repair to occur. Excision repair requires double-stranded DNA for incision and resynthesis using the complementary strand as a template [99,100]. Consistent with this interpretation, the recovery of DNA synthesis is significantly delayed for 50 min in the absence of RecJ-mediated nascent DNA degradation, and the recovery as well as the survival of the cell become dependent on translesion synthesis by Pol V, arguing that repair enzymes can no longer gain access to the arresting lesion (Figure 7) [56]. The 50 min delay in recovery correlates with the time required for upregulation and activation of Pol V [125][126][127][128], which is the translesion polymerase required for synthesis through UV damage and is responsible for most of the mutagenesis that occurs [129,130]. umuC and umuD, encode the catalytic and regulatory subunits of the Pol V complex, respectively [131,132]. Both genes are upregulated after UV damage in a LexA-dependent manner. However, activation of translesion synthesis is delayed until UmuD is posttranslationally processed to its active form, termed UmuD' [133][134][135]. UmuD shares homology with LexA and undergoes a similar autocatalytic cleavage with RecA bound to single-stranded DNA to form UmuD'. The nascent DNA processing would be expected to generate a more extensive three-stranded substrate at the replication fork for RecA to bind and stabilize, thereby ensuring that replication resumes from the same template and same site at which disruption occurred [17,51,63,64,97]. By analogy, RecQ homologs in yeast, Drosophila, and humans have been Although the partial degradation of the nascent lagging strand seems intuitively counterproductive, it serves to move the replication fork back and restore the lesion-containing region to a double-stranded form of DNA that would allow repair to occur. Excision repair requires double-stranded DNA for incision and resynthesis using the complementary strand as a template [99,100]. Consistent with this interpretation, the recovery of DNA synthesis is significantly delayed for 50 min in the absence of RecJ-mediated nascent DNA degradation, and the recovery as well as the survival of the cell become dependent on translesion synthesis by Pol V, arguing that repair enzymes can no longer gain access to the arresting lesion (Figure 7) [56]. The 50 min delay in recovery correlates with the time required for upregulation and activation of Pol V [125][126][127][128], which is the translesion polymerase required for synthesis through UV damage and is responsible for most of the mutagenesis that occurs [129,130]. umuC and umuD, encode the catalytic and regulatory subunits of the Pol V complex, respectively [131,132]. Both genes are upregulated after UV damage in a LexA-dependent manner. However, activation of translesion synthesis is delayed until UmuD is posttranslationally processed to its active form, termed UmuD' [133][134][135]. UmuD shares homology with LexA and undergoes a similar autocatalytic cleavage with RecA bound to single-stranded DNA to form UmuD'. The nascent DNA processing would be expected to generate a more extensive three-stranded substrate at the replication fork for RecA to bind and stabilize, thereby ensuring that replication resumes from the same template and same site at which disruption occurred [17,51,63,64,97]. By analogy, RecQ homologs in yeast, Drosophila, and humans have been shown to play critical roles in maintaining processive replication and suppressing the frequency of DNA strand exchanges during replication [136][137][138][139][140][141][142][143][144][145][146]. shown to play critical roles in maintaining processive replication and suppressing the frequency of DNA strand exchanges during replication [136][137][138][139][140][141][142][143][144][145][146].

Evidence That Lesion Repair Occurs at Disrupted Replication Forks to Prevent Mutations or Rearrangements by Translesion Synthesis or Recombination
The concept that nucleotide excision repair acts at disrupted replication forks can be inferred from the original survival studies carried out in repair and recombination mutants by Howard-Flanders and Theriot [49]. They found that E. coli cultures lacking either recombination (recA) or excision repair (uvrA) reduced the survival of cultures from doses producing greater than 3500 lesions per genome, to ~20 or 60 lesions per genome, respec-

Evidence That Lesion Repair Occurs at Disrupted Replication Forks to Prevent Mutations or Rearrangements by Translesion Synthesis or Recombination
The concept that nucleotide excision repair acts at disrupted replication forks can be inferred from the original survival studies carried out in repair and recombination mutants by Howard-Flanders and Theriot [49]. They found that E. coli cultures lacking either recombination (recA) or excision repair (uvrA) reduced the survival of cultures from doses producing greater than 3500 lesions per genome, to~20 or 60 lesions per genome, respectively. Further, mutants lacking both uvrA and recA were similarly sensitive, surviving only 1 or 2 lesions (Figure 8). Fundamental genetics argues that the ability to survive UV-irradiation requires both uvr and the rec gene products, as survival synergistically increases in the presence of these proteins, and is reduced to nearly zero in their absence. The few lesions survived by these mutants likely represents the number of lesions that nucleotide excision repair can remove before a replisome encounters one in the case of recA cells, or that translesion synthesis can bypass in the case of uvrA mutants. pathway in nonsexual cell cycles, and focused their interpretation exclusively upon the uvrA mutant relative to the uvrA recA double mutant. In this interpretation, since the recA mutation reduced the survival of excision repair mutants from 60 lesions to 2 lesions, they concluded that the difference could represent a function of recA promoting survival through a recombinational mechanism that was independent of excision repair. Additionally, while we have immense respect and recognize all that these authors have contributed to this field, in this case, we do not believe the data support this interpretation. In trying to understand the cellular function of a gene product, the mutant's phenotype should be compared relative to its wild-type counterpart. If the two pathways were operating independently, then survival promoted in the presence of recA and uvrA might be expected to be additive, or in the range of 100 lesions. Instead, the presence of both these genes allows the parental strain to process and survive several thousand lesions. Indeed, if graphed in its entirety, the bar representing the wild-type strain would extend up twelve pages into the previous article. Critically, this is not how the authors of this study interpreted these data. The authors' hypothesis focused on the idea of whether recombination could function as a repair pathway in nonsexual cell cycles, and focused their interpretation exclusively upon the uvrA mutant relative to the uvrA recA double mutant. In this interpretation, since the recA mutation reduced the survival of excision repair mutants from 60 lesions to 2 lesions, they concluded that the difference could represent a function of recA promoting survival through a recombinational mechanism that was independent of excision repair. Additionally, while we have immense respect and recognize all that these authors have contributed to this field, in this case, we do not believe the data support this interpretation. In trying to understand the cellular function of a gene product, the mutant's phenotype should be compared rela-tive to its wild-type counterpart. If the two pathways were operating independently, then survival promoted in the presence of recA and uvrA might be expected to be additive, or in the range of 100 lesions. Instead, the presence of both these genes allows the parental strain to process and survive several thousand lesions. Indeed, if graphed in its entirety, the bar representing the wild-type strain would extend up twelve pages into the previous article.
The authors' initial interpretation proved influential as almost every study in the decades of research that followed (and many studies still carried out today) exclusively used nucleotide excision repair mutants to characterize DNA damage-induced recombination and generally interpreted the observed exchanges as repair events [6,7,. The rationale offered for using nucleotide excision repair mutants often was that repair suppressed or masked recombination events making them difficult to observe. In looking at these studies, one cannot avoid noting that cell survival and genomic stability are always severely compromised in the populations where recombination was observed, and lethal doses are typically used in order to generate and observe these strand-exchange events. By analogy, consider the conclusions that would be reached if all human studies on how cells survived DNA damage were conducted exclusively in xeroderma pigmentosum cell lines. Thus, one cannot separate cell death and genomic instabilities from the activity of rec gene products functioning in the absence of repair.
One early line of investigation, consistent with the idea that excision repair plays an important role in the RecA-promoted recovery process, comes from the characterization of a phenomenon that was termed "long patch excision repair" [147][148][149]. While characterizing the resynthesis length, or 'patch size' of DNA at repair sites following DNA damage, it was observed that the size distribution in UV-irradiated E. coli was bimodal. Short patches of 10-12 nucleotides appeared at early times, correlating with normal nucleotide excision repair events. However, at times correlating with when replication recovered, much longer "patches" of DNA synthesis were observed in a process that depended on both recA and uvr repair genes. Long repair patches localized at DNA replication forks and were made up of fragments that were either >9000 bases or~1500 bases in length [149]. At the time, the authors concluded that these excision repair-dependent long patches were associated with the efficient recovery of replication and it is notable that their size distribution correlates with those of normal leading and lagging strand synthesis during replication. The results were among the earliest evidence that the recovery of replication depended upon the removal of the blocking lesions by excision repair. A functional synergism between nucleotide excision repair and the RecF pathway was noted by several others in the field who also noted the incongruity of the genetic argument that rec and uvr pathways operate independently. In each case, the authors found that nucleotide excision repair was a primary component of the recA-mediated recovery of replication [150][151][152].
The idea that repair occurs at the disrupted replication fork is also supported by assays which directly characterize the DNA damage-arrested replisome. Similar to recF mutants, mutants defective in nucleotide excision repair also fail to restore replication after disruption ( Figure 9A). The inhibition of replication is dose dependent and mirrors the inhibition seen in the absence of RecF at all doses [18]. However, the phenotype for uvrA mutants characterized using nascent DNA processing assays, is distinct from that seen in recF mutants ( Figure 9B). Whereas, the nascent DNA undergoes extensive degradation in recF, it remains protected in the uvr mutants and is limited in extent and duration to that seen in wild-type cells. The observation argues that unlike recF, the replication fork is maintained and protected in uvrA mutants, and the inability to resume is simply due to the unremoved obstructing lesion. Unlike in recF mutants, the replication fork remains protected in nucleotide excision repair mutants. The nascent DNA degradation occurring after UV irradiation with 25 J/m 2 was measured as described in Figure 4. Loss of 14 C genomic DNA (open symbols) can be compared to the loss of the 3 H DNA synthesized at the growing fork just prior to irradiation (filled symbols). Squares, wild type; circles, recF; triangles, uvrA. (C) In the absence of nucleotide excision repair, the intermediates at disrupted replication forks are not resolved and aberrant, higher order recombination intermediates accumulate. The migration pattern of replicating plasmids in each strain was analyzed by 2D agarose gel analysis as described in Figure 4. Processing intermediates transiently accumulate and then resolve in wild-type cells. No intermediates are observed in recF mutants. In uvrA mutants, these intermediates persist and go on to form higher-order, recombination intermediates. Redrawn from data reported in [18,53].  Figure 4. Circles, 14 C-prelabeled DNA; squares, 3 H-replicated DNA. (B) Unlike in recF mutants, the replication fork remains protected in nucleotide excision repair mutants. The nascent DNA degradation occurring after UV irradiation with 25 J/m 2 was measured as described in Figure 4. Loss of 14 C genomic DNA (open symbols) can be compared to the loss of the 3 H DNA synthesized at the growing fork just prior to irradiation (filled symbols). Squares, wild type; circles, recF; triangles, uvrA. (C) In the absence of nucleotide excision repair, the intermediates at disrupted replication forks are not resolved and aberrant, higher order recombination intermediates accumulate. The migration pattern of replicating plasmids in each strain was analyzed by 2D agarose gel analysis as described in Figure 4. Processing intermediates transiently accumulate and then resolve in wild-type cells. No intermediates are observed in recF mutants. In uvrA mutants, these intermediates persist and go on to form higher-order, recombination intermediates. Redrawn from data reported in [18,53].
When one examines the structures of the disrupted fork by 2D agarose gel analysis, one observes that replication fork processing begins normally in uvrA mutants, but in the absence of lesion removal, these processing intermediates persist and fail to resolve ( Figure 9C). In UV-irradiated wild-type cells, these intermediates resolve at a time that correlates with when the lesions are removed [53]. In contrast, the absence of lesion removal in uvr mutants leads to higher-order strand-exchange intermediates at later times, consistent with illegitimate recombination events occurring in these dying cells.
Some of the most direct evidence that lesions are repaired at the disrupted replication fork comes from two elegant studies carried out by Bichara et al. [83,84]. A single-stranded plasmid containing a G-AAF adduct (N-2-acetylaminofluorene attached to the C8 position of guanine), was transformed into cells harboring a second endogenous plasmid that contained three closely spaced genetic markers within a region of homology to the lesion-containing plasmid, surviving plasmids were then recovered and scored for the markers they picked up from the homologous plasmid ( Figure 10A). Similar to UV-induced cyclobutane pyrimidine dimers, AAF adducts are bulky lesions that similarly depend upon nucleotide excision repair for removal from the genome [153,154]. The genetic markers were designed to differentiate between nucleotide excision repair (those that only picked up the genetic marker opposite to the lesion on the homologous template), recombination (those that contained extensive regions from the homologous template, having two or all three markers), and translesion synthesis (those in which the middle marker contained an insertion when sequenced). Since nucleotide excision repair cannot occur on singlestranded DNA, all recovered plasmids in this experimental design were forced to undergo strand exchange with the homologous plasmid for either recombination or 'repair' to occur. Surprisingly, the majority of events in wild-type cells used nucleotide excision repair rather than recombination to process the plasmid lesion ( Figure 10B). Nucleotide excision repair events predominated even though the template containing the lesion was required to occur intermolecularly, using a template supplied by the homologous plasmid. In the absence of nucleotide excision repair, survival was modestly reduced and recombination events predominated. As expected, RecA-mediated strand pairing was required for all these events. The frequency of translesion synthesis was very low, although the lack of SOS induction and Pol IV expression may have hindered this possibility in these single event experiments.
In a critical follow-up study, the authors repeated this assay using double-stranded plasmids that contained the lesion in either the leading or lagging-strand template (Figure 10C). Again because of the genetic markers, only plasmids that utilized the intermolecular template could be scored. The authors observed that on recovered plasmids, nucleotide excision repair events still predominated, particularly when the lesion was found in the leading-strand template. In the absence of nucleotide excision repair, plasmid recovery and survival were significantly reduced, and recombination predominated. When the lesion was in the lagging-strand template, which would not be expected to disrupt replication, few plasmids were recovered.
That nucleotide excision repair was stimulated when the lesion was located in the leading strand, but not the lagging strand, implies that nucleotide excision repair is coupled to replication events. Further and critical to the implications for mechanism, although these experiments were only able to score intermolecular events, the intramolecular template on the lagging strand would clearly be the preferred substrate used following disruption ( Figure 10D), which would be further enhanced by the RecJ-mediated degradation of the nascent lagging strand that occurs [51,56]. It would not be unreasonable to expect the intermolecular reaction to occur with an efficiency that is orders of magnitude higher than that of the intermolecular reaction. Plasmids containing a site-specific AAF adduct were transformed into cells containing a second endogenous, homologous plasmid with three closely spaced, genetic markers. The markers are designed to allow one to determine whether nucleotide excision repair (surviving plasmids only contained the marker at the lesion site), recombination (surviving plasmids contained multiple genetic markers), or translesion synthesis (contained a base-pair insertion at the middle marker) occurred on the surviving plasmids that are recovered. (B) Nucleotide excision repair events predominate at disrupted replication forks. When single-stranded plasmids were used in this assay, nucleotide excision repair predominated over recombination events. Few plasmids were recovered in recA mutants. In the absence of nucleotide excision repair, survival was reduced and recombination events predominated. (C) Nucleotide excision repair occurs when the lesion is in the leading strand, which disrupts replication, but not the lagging strand, which does not disrupt replication. The same assay is repeated as in (B), except transforming a double-stranded plasmid containing an AAF adduct in either the leading-or lagging-strand template. In wild-type cells, nucleotide excision repair events predominated on the recovered plasmids when the lesion was in the leading strand. When the lesion was in the lagging strand the frequency of repair and plasmids recovered was severely reduced. In uvrA mutants, the frequency of plasmids recovered was severely reduced irrespective of whether the lesion was in the leading-or lagging-strand template and re- Figure 10. Nucleotide excision repair occurs at disrupted replication forks. (A) Schematic to measure lesion processing on replicating plasmids. Plasmids containing a site-specific AAF adduct were transformed into cells containing a second endogenous, homologous plasmid with three closely spaced, genetic markers. The markers are designed to allow one to determine whether nucleotide excision repair (surviving plasmids only contained the marker at the lesion site), recombination (surviving plasmids contained multiple genetic markers), or translesion synthesis (contained a base-pair insertion at the middle marker) occurred on the surviving plasmids that are recovered. (B) Nucleotide excision repair events predominate at disrupted replication forks. When single-stranded plasmids were used in this assay, nucleotide excision repair predominated over recombination events. Few plasmids were recovered in recA mutants. In the absence of nucleotide excision repair, survival was reduced and recombination events predominated. (C) Nucleotide excision repair occurs when the lesion is in the leading strand, which disrupts replication, but not the lagging strand, which does not disrupt replication. The same assay is repeated as in (B), except transforming a double-stranded plasmid containing an AAF adduct in either the leading-or lagging-strand template. In wild-type cells, nucleotide excision repair events predominated on the recovered plasmids when the lesion was in the leading strand. When the lesion was in the lagging strand the frequency of repair and plasmids recovered was severely reduced.
In uvrA mutants, the frequency of plasmids recovered was severely reduced irrespective of whether the lesion was in the leading-or lagging-strand template and recombination events predominated.
(D) To be scored in this assay, repair events were required to undergo strand exchange and utilize an intermolecular template for repair. In vivo, the template utilized for repair would be intramolecular, as shown, allowing the reaction to occur with far, far greater frequency and efficiency. Composed and drawn from data reported in [83,84].
Several follow-up studies to this work have placed the lesion on the chromosome [43][44][45][46][47][48]. Unfortunately, these studies reverted to utilizing exclusively repair-deficient mutants, which in our opinion has again removed the biological relevance and led to misinterpretations about what occurs in a wild-type cell that functionally recovers from lesion loads hundreds of times higher than uvr mutants. Yet, as supported by their earlier studies, survival in this situation likely occurs through a mechanism that involves both RecF pathway processing at the fork and lesion removal by nucleotide excision repair, so that the replisome can resume.

Maintaining and Restoring Processive Replication Is Specific to the RecF Pathway
The processing and restoration of the disrupted replication fork are remarkably specific to the RecF pathway proteins. Similar to recF mutants, recBCD, recG and ruvAB mutants are all hypersensitive to DNA damage such as that induced by UV irradiation. As shown in Figure 11A, a moderate dose of 254-nm UV radiation (one from which wild-type cells nearly fully survive) kills more than 99% of cells in all these mutant populations. Based on this hypersensitivity, others have sometimes speculated that these mutants also act at or restore replication forks that encounter DNA damage [87,88,[155][156][157][158][159][160][161][162][163]. However, survival assays, by themselves, do not address the cause of death in these mutants. Additionally, none of these studies utilized assays to directly assess whether RecBCD, RecG and RuvAB process the replication fork or affect the ability to restore replication in vivo. In many cases, this led to misconceptions about the cellular role of these other proteins. Figure 11. Restoring replication after disruption is specific to the recF pathway. (A) recF, recBC, ruvAB, and recG mutants all exhibit high levels of cell lethality following UV-induced DNA damage. The survival of UV-irradiated wild-type, recF, recBC, ruvAB, and recG cells at the doses indicated is plotted. (B) Yet only recF mutants fail to restore replication after UV-induced damage. The amount of DNA synthesized during a 1 h period in UV-irradiated (25 J/m 2 ) or mock-irradiated cultures was determined by density labeling the DNA with 5-bromodeoxyuridine and subsequent isolation in isopycnic alkali CsCl gradients. Open circles, DNA synthesized before treatment ( 14 C); filled squares, DNA synthesized following treatment ( 3 H). The range of 3 H and 14 C axes was kept constant for each strain. Redrawn from data presented in [91,164,165].
Whereas the absence of RecF impairs the recovery of replication after disruption, recBC, recG, and ruvAB mutants each fully recover replication with wild-type kinetics (Figure 11B), indicating that the hypersensitivity of these mutants (i.e., the cause of death) is not associated with a defect in restoring replication after UV damage [50,80,91,107,166]. Although RecBC, RuvAB, and RecG are not essential for replication to resume, it remains possible that these proteins may still act upon or process the disrupted replication forks, and are needed for DNA synthesis to resume at the correct site and using the appropriate template.
However, when one examines the replication intermediates in mutants lacking RecBC, RuvAB, or RecG by 2D agarose gels, cone-region intermediates form in each case Figure 11. Restoring replication after disruption is specific to the recF pathway. (A) recF, recBC, ruvAB, and recG mutants all exhibit high levels of cell lethality following UV-induced DNA damage. The survival of UV-irradiated wild-type, recF, recBC, ruvAB, and recG cells at the doses indicated is plotted. (B) Yet only recF mutants fail to restore replication after UV-induced damage. The amount of DNA synthesized during a 1 h period in UV-irradiated (25 J/m 2 ) or mock-irradiated cultures was determined by density labeling the DNA with 5-bromodeoxyuridine and subsequent isolation in isopycnic alkali CsCl gradients. Open circles, DNA synthesized before treatment ( 14 C); filled squares, DNA synthesized following treatment ( 3 H). The range of 3 H and 14 C axes was kept constant for each strain. Redrawn from data presented in [91,164,165].
Whereas the absence of RecF impairs the recovery of replication after disruption, recBC, recG, and ruvAB mutants each fully recover replication with wild-type kinetics ( Figure 11B), indicating that the hypersensitivity of these mutants (i.e., the cause of death) is not associated with a defect in restoring replication after UV damage [50,80,91,107,166]. Although RecBC, RuvAB, and RecG are not essential for replication to resume, it remains possible that these proteins may still act upon or process the disrupted replication forks, and are needed for DNA synthesis to resume at the correct site and using the appropriate template.
However, when one examines the replication intermediates in mutants lacking RecBC, RuvAB, or RecG by 2D agarose gels, cone-region intermediates form in each case (Figure 12A) [53,80], indicating that the branch migration activity of RuvAB or RecG, or the helicase-nuclease of RecBCD, is not required to catalyze the fork regression in vivo. Unlike recF cells, the nascent DNA degradation in hypersensitive recBC, ruvAB, and recG mutants remains limited and appears similar to wild-type cells following UV-induced DNA damage ( Figure 12B) [51,57,91].
Genes 2022, 13, x FOR PEER REVIEW 20 of 30 ( Figure 12A) [53,80], indicating that the branch migration activity of RuvAB or RecG, or the helicase-nuclease of RecBCD, is not required to catalyze the fork regression in vivo. Unlike recF cells, the nascent DNA degradation in hypersensitive recBC, ruvAB, and recG mutants remains limited and appears similar to wild-type cells following UV-induced DNA damage ( Figure 12B) [51,57,91]. The absence of processing intermediates seen at disrupted replication fork is specific to recF mutants. DNA from cells containing the plasmid pBR322 were purified, digested with Pvu II, and analyzed by 2D agarose gels immediately before and 15 min after UV irradiation with 50 J/m 2 . Cone region intermediates resembling those in wild-type cells appear in recBC, recG, and ruvAB mutants, but are missing in recF mutants. These assays strongly argue against the frequently postulated idea that forks collapse to form double-strand breaks at lesions that block replication. This model originally arose from a review article that speculated that if forks collapsed after UV-induced damage, they would form a double-strand break that could account for the UV hypersensitivity of recBC mutants [167,168]. Several subsequent studies built upon this hypothesis, reporting that fragmentation could be detected on the chromosome in recBCD mutants and that fragmentation was exacerbated following inactivation of the replicative helicase, DnaB [89,90,[155][156][157][158][169][170][171][172][173][174][175][176][177]. However, neither this review nor any of the chromosome fragmentation studies employed assays to directly examine the replication fork DNA. On the other hand, when the replication fork DNA was examined directly under these conditions, it was shown that recBCD did not act at or contribute to the degradation that occurred at the replication fork in dnaB mutants or after UV [51,53,57,58,79]. Further, the fragmentation of chromosomes in recBCD mutants has since been shown to localize to the region where replication forks converge to complete replication, but not at sites of replication fork disruption [165,178,179].
One might argue that only a subset or fraction of the arrested replication forks collapse into double-strand breaks. However, recBC mutants are as hypersensitive to UV irradiation as recF mutants ( Figure 11A). Thus, if collapsed replication forks were the cause of recBC mutant hypersensitivity, one would predict that there would be a proportionate loss of the arrested Y-shaped structures, and accumulation of linear broken intermediates on 2D agarose gels. Yet no broken linear intermediates are observed at replication forks in UV-irradiated recBC cells as analyzed by 2D agarose gels [53,80]. Collapse at disrupted replication forks would also predict that recBCD mutants should fail to resume replication after disruption and degrade the nascent DNA at the disrupted fork. However, recBC mutants restore replication and process the nascent DNA at the replication fork normally ( Figures 11B and 12) [50,107,166]. Taken together, this indicates that replication forks do not collapse or form double-strand breaks, but are maintained in a branched, arrested form, and that RecBCD does not act at damage-arrested replisomes in vivo.
Finally, one could also argue that perhaps replication forks collapse when they encounter other forms of damage, but not when they encounter UV-induced damage. While this certainly could be true, it would not explain why recBC mutants are hypersensitive to UV-induced damage. Clearly, some event not associated with the arrested fork arises and requires RecBC function in UV-irradiated cells. If replication fork collapse is not causing death in recBC cells after UV, then it is reasonable to consider that it may not necessarily be responsible for causing cell death following other forms of DNA damage.
Based on the biochemical activity of purified proteins and chromosome fragmentation assays, RuvAB and RecG are proposed to promote the regression of replication forks blocked by DNA damage, which is thought to account for the hypersensitivity of ruvAB and recG mutants [87,89,90,156,[159][160][161]172,176,180]. Again however, if true, one would expect that in the absence of either RuvAB or RecG, regressed replication fork intermediates would not accumulate after UV irradiation, and that the recovery of replication would be impaired or delayed. However, as discussed above, the absence of RuvAB or RecG does not prevent the processing that occurs at the replication fork or affect its ability to recover [57,80,91]. The results argue that cell death, in the absence of RecBC, RecG, or RuvAB is caused by a defect that is not directly associated with restoring DNA replication following disruption.
One alternative possibility for the hypersensitivity of these mutants is suggested by recent studies that have shown RecBC and RecG act in the terminus region of the chromosome and play critical roles in completing DNA replication when replication forks converge (for reviews and discussion of the cellular role of these proteins see [165,178,179,[181][182][183][184][185]. These studies highlight how although these enzymes were thought to be specific for repairing DNA damage, they are required to process intermediates arising during normal replication. These are roles and functions that really have not been considered or addressed experimentally in mammalian cells, but may restructure how we functionally think about the role and frequency of double-strand breaks in the normal replication cycle.

Recombination Mediators Are Functionally Conserved between Bacteria and Mammals
In mammalian systems, the role of the BRCA2 pathway and RECQ helicases in maintaining replication forks and suppressing recombination events in mitotic cells is well established [186][187][188][189][190]. Similar to RecF, RecO or RecR mutants, human cells lacking BRCA2 are impaired in their ability to maintain the replication fork and exhibit high levels of genomic instability [186,188]. Loss of BRCA2 leads to more extensive degradation of disrupted replication forks, which recruit Rad51 paralogs that play critical nonrecombinagenic roles in preventing extensive degradation of the nascent DNA at the replication fork and allowing replication to resume [191]. Although homology between RecF, RecO, or RecR is not necessarily apparent at the sequence level, the parallels are strikingly apparent at the phenotypic and functional level [192].
There are five RecQ homologs in humans, RECQ1, BLM, WRN, RECQ4, and RECQ5. Additionally, although each is likely to be temporally or spatially anchored to a unique place in the cell that defines its function, it is notable that all are associated with cancer-prone disease states and genetic instabilities when mutated (reviewed in [193]). Considering that each RecQ homolog is associated with distinct genetic disorders and cancers, it seems likely that they have separate, but likely related, roles in the cell. What defines their unique functions and whether it relates to tissue-specific expression, the nature of the impediment blocking replication, or even differential processing of leading and lagging-strand templates remains unclear at this time. Both RECQ1 and WRN have been reported to protect the nascent DNA at replication forks from degradation under different conditions or in different tissues, similar to their bacterial counterpart [194][195][196]. Similarly, the hallmark of BLM is its ability to suppress exchanges between sister chromatids during replication as shown in Figure 1A [137,197]. Speculatively, this phenotype may suggest a role for this protein in processing and resolving impediments on the lagging-strand template, which are known to allow replication to continue without arresting the progression of the fork [72][73][74][75][76].
Deciphering the mechanisms by which BRCA2 and RECQ operate in mammalian cells, where genome complexity is amplified and the proportion of replicating cells is reduced, can be more challenging. Yet revealing the cellular function of these gene products is key to developing more effective therapies for cancer and enhancing lethality in cells harboring these mutations. The assays available and developed in E. coli make a strong argument that we should continue to take advantage of this model organism, especially when clear homologs of bacterial proteins can be identified in mammals.

Conflicts of Interest:
The authors declare no conflict of interest.