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Palindromes as Substrates for Multiple Pathways of Recombination in Escherichia coli
Gareth A. Cromiea, Catherine B. Millara, Kristina H. Schmidta, and David R. F. Leachaa Institute of Cell and Molecular Biology, University of Edinburgh, Edinburgh EH9 3JR, United Kingdom
Corresponding author: David R. F. Leach, Institute of Cell and Molecular Biology, University of Edinburgh, Darwin Bldg., Kings Bldgs., Mayfield Rd., Edinburgh, Scotland., d.leach{at}ed.ac.uk (E-mail)
Communicating editor: L. S. SYMINGTON
 | ABSTRACT |
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 TOP ABSTRACT MATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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A 246-bp imperfect palindrome has the potential to form hairpin structures in single-stranded DNA during replication. Genetic evidence suggests that these structures are converted to double-strand breaks by the SbcCD nuclease and that the double-strand breaks are repaired by recombination. We investigated the role of a range of recombination mutations on the viability of cells containing this palindrome. The palindrome was introduced into the Escherichia coli chromosome by phage 
lysogenization. This was done in both wt and sbcC backgrounds. Repair of the SbcCD-induced double-strand breaks requires a large number of proteins, including the components of both the RecB and RecF pathways. Repair does not involve PriA-dependent replication fork restart, which suggests that the double-strand break occurs after the replication fork has passed the palindrome. In the absence of SbcCD, recombination still occurs, probably using a gap substrate. This process is also PriA independent, suggesting that there is no collapse of the replication fork. In the absence of RecA, the RecQ helicase is required for palindrome viability in a sbcC mutant, suggesting that a helicase-dependent pathway exists to allow replicative bypass of secondary structures.
LONG DNA palindromes and inverted repeat sequences separated by little intervening sequence confer inviability in Escherichia coli (see 
Palindrome-mediated inviability can be significantly suppressed by mutations in the sbcC or sbcD genes (
SbcCD also acts as a hairpin endonuclease, cleaving hairpin loops near the 5' junction with the duplex stem of the secondary structure (
Recombination proteins in E. coli have been divided into two major systems: the RecB and RecF pathways. A third system, the RecE pathway, involves proteins encoded by a prophage present in only a subset of E. coli strains and is not discussed here. The RecB and RecF pathways involve different sets of proteins acting at the early, presynaptic, stages of recombination.
In the RecB pathway the RecBCD protein complex acts on blunt or near-blunt DNA ends (
sequence its activity is altered, apparently through interaction with the RecD subunit (
The RecF pathway was identified as an alternative recombination system restoring high levels of recombination in recB strains (
3' single-strand exonuclease and the RecQ helicase convert DNA ends into long 3' overhangs of single-stranded DNA (
The RecF and RecB pathways appear to act on different substrates and involve different presynaptic proteins. However, both feed into the same RecA-mediated pathway of strand exchange. This leads to the formation of Holliday junctions that are branch migrated by the RecG and RuvAB proteins and resolved by the RuvC nuclease (
In this study the relationship between SbcCD and recombination at palindromic DNA sites was investigated further using a 246-bp imperfect palindrome and a range of recombination mutant backgrounds. In the presence of SbcCD the palindromic sequence was found to stimulate recombination using a large number of proteins, including the components of both the RecF and RecB pathways. In the absence of SbcCD the palindrome stimulates RecF-gap recombination at high frequency. In the absence of RecA, propagation of the palindrome requires the RecQ helicase.
| MATERIALS AND METHODS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Bacteriophage strains:
DRL246 was constructed by cloning a Zeocin resistance marker in an EcoRI-BglII fragment from pZeoSV2(+) (Invitrogen Corp., San Diego) into the multicloning site of TXF97 (DRL246 as an EcoRI fragment to form DRL282 (this laboratory). Two internal mismatches were introduced into the palindrome sequence during this process.
DRL154 (pal571, 
spi6, cI857, +) contains a 571-bp palindromic sequence (this laboratory). DRL 152 is an isogenic phage lacking the palindrome sequence.
Lysogenization:
Overnight cultures of bacterial strains to be lysogenized were diluted 10-fold in L broth containing 2% maltose and 5 mM Mg2SO4 and grown to a cell density of 4 x 108 cells ml-1 (A650 = 0.9). Cultures were diluted with an equal volume of 10 mM Tris, 10 mM Mg2SO4 pH 8 buffer (TM buffer) to give a final cell density of 2 x 108 pfu ml-1. Bacteriophage lysates were diluted to 2 x 109 pfu ml-1. An aliquot (0.15 ml) of phage was added to 0.15 ml of bacterial cells and allowed to adsorb for 60 min at 30°. Infected cells were diluted in phosphate buffer and appropriate dilutions plated on low-salt (85 mM NaCl) L AGAR plates supplemented with Zeocin (Invitrogen Corp.) at a concentration of 16 µg ml-1 or on L AGAR plates. To prevent the appearance of dnaC suppressor mutations the priA strains DL1133 and DL1134 (Table 1) were grown on minimal liquid medium (Spitzizen Salts supplemented with 0.2% glucose, 15 µg ml-1 threonine, 15 µg ml-1 histidine, 15 µg ml-1 arginine, 15 µg ml-1 leucine). Log phase cultures were then diluted with TM buffer and lysogenized in the same way as the other strains. The recombination efficiency of the priA strains was measured by P1 transduction frequency to check that suppressor mutations had not occurred.
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| RESULTS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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The components of both the RecB and RecF pathways are required for palindrome viability in the presence of SbcCD:
A 246-bp interrupted palindromic sequence consisting of inverted repeats of 111 bp separated by a 24-bp spacer is known to confer inviability on its host replicon in the presence of the SbcCD nuclease when the products of the recA, recB, or recC genes are absent (
Two isogenic phage, one containing a 246-bp interrupted palindrome and the other lacking this sequence, were used to identify these recombinational requirements of the 246-bp palindrome. The palindrome-containing phage lysogenized the wt (wild type) strain at approximately equal frequency to the palindrome-free control phage. However, the lysogenization frequency of the palindrome phage was several orders of magnitude lower than that of the control in recA, recB, or recC strains (
In this study a different strain of phage carrying the 246-bp palindrome was used to carry out similar lysogenization frequency studies (DRL282). An isogenic palindrome-free phage was also used (DRL246). These phage encode resistance to the antibiotic Zeocin, allowing selection of lysogens in a wide variety of strains, including those resistant to the antibiotics tetracycline, ampicillin, kanamycin, and chloramphenicol.
Initially, the previous lysogenization results for the wt, recA, and recB backgrounds were replicated in this study (Figure 1). As previously observed (DRL282) compared to the palindrome-free phage (DRL246). This reflected the requirement for recombination involving the RecA and RecBCD proteins for the viability of the cell with the palindrome. This analysis was then extended to a range of other recombination mutants.
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Given that recombination was known to be occurring, it was expected that there would be a requirement for the late-acting recombination proteins RecG, RuvA, and RuvC and indeed the lysogenization frequency of DRL282 was severely reduced in recG, ruvA, and ruvC mutant backgrounds compared to the wt (Figure 1). DRL282 lysogenization was also impaired in the recN background (Figure 1). This is consistent with the role of RecN in other DNA end-based recombination assays (DRL246 was unaffected by these mutations (Figure 1).
The effect of mutations in genes of the RecF pathway was a more open question. In fact mutations in all of the RecF pathway genes studied (recF, recO, recR, recQ, and recJ) caused palindrome-mediated inviability and a specific reduction in the efficiency of DRL282 lysogenization (Figure 2).
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These results indicate that efficient repair of the SbcCD-generated double-strand break requires a wide range of recombination functions, including the components of both the RecB and RecF pathways.
SbcCD-induced double-strand breaks are not associated with PriA-dependent replication fork repair:
Double-strand breaks, caused by replication encountering a nick or lesion, are believed to lead to replication fork collapse and probable disassembly of the replication protein complex (
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In the absence of double-strand breaks the palindrome stimulates recombination via the RecF pathway:
The lysogenization assay was repeated using the same range of recombination mutants as above, but with each carrying an additional mutation in sbcC. Previous analysis of recA, recB, and recC mutants in an sbcC background had demonstrated lysogenization of the palindrome phage at an equally high frequency to that of the palindrome-free control (
The results of this study generally support these findings. DRL282 could lysogenize most of the recombination mutants carrying the additional sbcC mutation at the same high frequency as DRL246 (Figure 4). However, there were two exceptions: the palindrome conferred inviability in the ruvA sbcC and ruvC sbcC double mutants (Figure 4). The RuvA and RuvC proteins are late components of recombination, comprising a component of the RuvAB branch migration complex and a Holliday junction resolvase enzyme, respectively (
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The recombination substrate involved is unlikely to be a DNA break as this would represent a lethal event in the absence of recombination. This suggests, instead, that a single-stranded gap is the substrate. This would also allow another mechanism to fill the gap in the absence of recombination. If this interpretation is correct, then it should be possible to repress the lethality of the unresolved Holliday junctions by preventing their formation. To test this, a range of triple mutants was constructed carrying mutations in ruvA, sbcC, and in a third recombination gene. As expected, mutations in genes encoding proteins involved in the early stages of gap recombination (recA, recF, recO, and recR) restored the lysogenization ability of the palindrome phage in a ruvA background (Figure 5). A mutation in recG, a gene encoding a late-acting junction resolving protein, did not restore viability (Figure 5). This means that RecG is not acting prior to the Ruv proteins, and the lack of any palindrome-mediated viability problem in the sbcC recG background (Figure 4) suggests it is not itself acting at a late stage when unresolved intermediates would be lethal. This implies that RecG may have little role to play in gap recombination.
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Gap recombination at the site of the palindrome is not associated with PriA-dependent replication fork repair:
In an sbcC background both the palindrome and control phage were able to lysogenize a priA mutant at high frequency (Figure 6), indicating either that palindrome-induced replication fork collapse is not occurring in sbcC cells or that it is being repaired in a PriA-independent manner.
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In the absence of recombination the viability of cells carrying the uncleaved palindrome requires the presence of the RecQ helicase:
The 246-bp imperfect palindrome used in this study appears to stimulate the formation of recombinogenic single-stranded gaps during replication in an sbcC mutant background. This indicates that replication has difficulty progressing through the secondary structure formed by this sequence. Presumably recombination using RecFOR fills in this gap. However, this gap can also be filled in the absence of recombination as is demonstrated by the ability of DRL282 to lysogenize sbcC recA cells (Figure 4). One possible method of filling the gap without recombination would be to use a helicase to unwind the secondary structure and so allow replication.
There was an indication that the RecQ helicase might fulfill such a function. It was observed that DRL154 (containing a 571-bp palindrome) could not form plaques on an sbcC recQ background. Normally this phage will form plaques on sbcC, but not wt. The phage produced plaques on all of the sbcC strains used in this study, with the exception of the recQ sbcC double mutant (results not shown). A palindrome-free control, DRL152, was able to form plaques on all backgrounds. It is possible that the difference between the ability of DRL282 to form lysogens in sbcC recQ cells and the inability of DRL154 to form plaques on the same background represents differences in the lengths of the palindromes or between chromosomal and lytic DNA replication. The result of such differences might be to make DRL154 lytic replication more reliant on a recombination-independent replication bypass mechanism than DRL282 when present on the E. coli chromosome. The plating behavior of DRL154 suggested that RecQ could have a role in such a recombination-independent system, especially as the effect was not observed for mutations in the other recF pathway genes (recF, recO, recR, and recJ) or recA in an sbcC background.
The role of RecQ in palindrome viability in an sbcC background in the absence of recombination was then addressed directly by lysogenizing an sbcC recA recQ triple mutant. In this background the palindrome was inviable (Figure 7), indicating that RecQ is required to process palindromes in the absence of recombination in an sbcC mutant.
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| DISCUSSION |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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The resolution of a 246-bp imperfect palindrome in E. coli appears to be a complex affair, where the palindromic substrate can be the target of double-strand break repair, single-strand gap repair, or replicative bypass, depending on the genetic background. In the presence of SbcCD the components of both the RecB and RecF pathways are required for the viability of the palindrome-containing cells. In the absence of SbcCD, recombination still appears to be occurring at a high frequency because ruvA mutations that trap late recombination intermediates are lethal. However, this recombination is not necessary for the viability of the palindrome-containing cells, as demonstrated by the viability of recA mutants. In the absence of both SbcCD and recombination the RecQ helicase is required for cell viability.
In a wild-type E. coli cell the predominant fate of a long palindrome appears to be to stimulate the formation of a double-strand break on the lagging strand. In contrast to what is believed to happen with double-strand breaks derived from fork interactions with a nick or other lesion (
Repair of the double-strand break was expected to involve the products of the RecB pathway that appears to be the dominant end-directed recombination system in wild-type E. coli. It was already known that the RecA and RecB proteins are essential for repair of the palindrome-initiated double-strand break (
More surprising was the discovery that the proteins of the RecF pathway, RecF, RecO, RecR, RecJ, and RecQ, are also essential for viability in the presence of a chromosomal palindrome and SbcCD. In the absence of the RecB pathway, RecF recombination can substitute for its function at DNA ends, but only in sbcB15 and sbcCD mutant strains. In these cases recombinogenic 3' DNA ends are being protected by the mutations affecting the two nucleases, and this is needed for efficient recombination. In wild-type cells the RecF pathway appears to act at DNA ends very infrequently [~1 time in 100 ( 3' nucleases. Another possibility is that both the RecF and RecB pathways are used by the DNA ends at approximately equal frequency (so that mutants in either pathway have a lethal phenotype). The third possibility is that the two ends produced by the SbcCD cleavage event have different recombinational requirements, with one utilizing the RecF pathway and the other the RecB pathway. RecBCD cannot load onto DNA ends that are not blunt or nearly blunt, so that if one of the DNA ends had a long overhang it could not be used as a substrate by RecBCD. This is similar to the suggestion that UV-induced single-strand gaps could be broken to produce DNA ends and that the RecF pathway could act on these if they possessed long single-stranded overhangs (
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In the absence of the SbcCD nuclease, palindromic sequences still stimulate recombination at high frequency. As recombination is unnecessary for viability in this system, and there is no hairpin nuclease, it seems unlikely that the substrate in this situation is a double-strand break. The alternative would be recombination stimulated by a single-strand gap (Figure 9), and the involvement of the RecF pathway proteins RecF, RecO, and RecR suggests that this is in fact the case. Although the RecF pathway proteins can efficiently stimulate recombination at ends in the absence of RecB in an sbcB15 sbcC mutant background, they have an independent role in gap-based recombination in plasmids and recovery from UV radiation ( 3' single-strand exonuclease could produce or extend such regions. The helicase and post-chi nuclease activities of RecBCD (, an activity similar to that of RecFOR (
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It appears that in both the presence and absence of SbcCD the existence of a long palindromic sequence leads to the formation of a single-strand gap containing the palindrome (probably at one side). The lysogenization results with priA strains show that this process of fork progression with a gap left behind does not involve fork collapse. In this sense whether or not the single-strand gap is then converted to a double-strand break by SbcCD is irrelevant; the progression of the fork will not be affected in either event.
It is surprising that the gap recombination that appears to occur frequently in the absence of SbcCD is not necessary for palindrome viability. Replication is unable to process the secondary structure and leaves a gap that would lead to a viability problem if left unfilled. Recombination must be able to unwind the secondary structure and allow the gap to be filled by replication using the other sister as a template. The exact mechanism by which this unwinding occurs is unclear, but it could occur during strand exchange or branch migration. The question then arises as to how the single-strand gap is filled in the absence of recombination. It appears that the RecQ helicase is central to this process. The RecQ protein is a 3' 5' DNA helicase that acts on duplex DNA or duplex DNA with single-stranded overhangs (
E. coli does not possess long perfect palindromic sequences, although short or imperfect palindromes do exist. This is particularly true for the regions of the chromosome that encode rRNA and tRNA sequences. These sequences have the capacity to fold into complicated secondary structures. Even random single-stranded DNA sequences are capable of forming secondary structure of low stability, which may mean that infrequent formation of secondary structure is a normal consequence of DNA being single stranded. The SbcCD nuclease could act to prevent mutagenesis at any of these secondary structures by removing them (
| ACKNOWLEDGMENTS |
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We thank John Connelly for his critical comments and suggestions. This research has been supported by a project grant from the Wellcome Trust. G.A.C. is supported by a Biotechnology and Biological Sciences Research Council studentship.
Manuscript received June 21, 1999; Accepted for publication October 4, 1999.
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 M. R. v. Z. K. Fagundes, C. P. Semighini, I. Malavazi, M. Savoldi, J. F. de Lima, M. H. de Souza Goldman, S. D. Harris, and G. H. Goldman Aspergillus nidulans uvsBATR and scaANBS1 Genes Show Genetic Interactions during Recovery from Replication Stress and DNA Damage Eukaryot. Cell, July 1, 2005; 4(7): 1239 - 1252. [Abstract] [Full Text] [PDF]
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I. V. Manukhov, D. V. Mamaeva, S. M. Rastorguev, N. G. Faleev, E. A. Morozova, T. V. Demidkina, and G. B. Zavilgelsky A Gene Encoding L-Methionine {gamma}-Lyase Is Present in Enterobacteriaceae Family Genomes: Identification and Characterization of Citrobacter freundii L-Methionine {gamma}-Lyase J. Bacteriol., June 1, 2005; 187(11): 3889 - 3893. [Abstract] [Full Text] [PDF]
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B. Carrasco, M. C. Cozar, R. Lurz, J. C. Alonso, and S. Ayora Genetic Recombination in Bacillus subtilis 168: Contribution of Holliday Junction Processing Functions in Chromosome Segregation J. Bacteriol., September 1, 2004; 186(17): 5557 - 5566. [Abstract] [Full Text] [PDF]
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 A. Pluciennik, R. R. Iyer, M. Napierala, J. E. Larson, M. Filutowicz, and R. D. Wells Long CTG{middle dot}CAG Repeats from Myotonic Dystrophy Are Preferred Sites for Intermolecular Recombination J. Biol. Chem., September 6, 2002; 277(37): 34074 - 34086. [Abstract] [Full Text] [PDF]
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 M. Bzymek and S. T. Lovett Instability of repetitive DNA sequences: The role of replication in multiple mechanisms PNAS, July 17, 2001; 98(15): 8319 - 8325. [Abstract] [Full Text] [PDF]
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Z.-H. Zhou, E. Akgun, and M. Jasin Repeat expansion by homologous recombination in the mouse germ line at palindromic sequences PNAS, July 17, 2001; 98(15): 8326 - 8333. [Abstract] [Full Text] [PDF]
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