Peptide wrwycr Inhibits the Excision of Several Prophages and Traps Holliday Junctions inside Bacteria

Gunderson, Carl W.; Boldt, Jeffrey L.; Authement, R. Nathan; Segall, Anca M.

doi:10.1128/jb.01559-08

Cited by 25 publications

(32 citation statements)

References 33 publications

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“…Another explanation may be the presence of greater concentrations of intracellular iron after wrwycr treatment. Our best current hypothesis is that the effects of wrwycr on DNA repair (Gunderson et al, 2009) and on iron availability are independent, albeit potentially synergistic.…”

Section: Discussionmentioning

confidence: 99%

“…We have identified synthetic hexapeptides that bind Holliday junctions as disulfidebridged dimers and inhibit Holliday junction resolution (Boldt et al, 2004;Kepple et al, 2005). One of these peptides, with the sequence wrwycr (we use the D-amino acid form to limit biological degradation), is a potent, broad-spectrum antimicrobial with the ability to inhibit, in vivo, mechanisms of DNA recombination and damage repair that proceed through a Holliday junction intermediate (Gunderson & Segall, 2006;Gunderson et al, 2009;L. Marcusson and other authors, unpublished data).…”

Section: Introductionmentioning

confidence: 99%

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Escherichia coli enterobactin synthesis and uptake mutants are hypersensitive to an antimicrobial peptide that limits the availability of iron in addition to blocking Holliday junction resolution

2012

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The peptide wrwycr inhibits Holliday junction resolution and is a potent antimicrobial. To study the physiological effects of wrwycr treatment on Escherichia coli cells, we partially screened the Keio collection of knockout mutants for those with increased sensitivity to wrwycr. Strains lacking part of the ferric-enterobactin (iron-bound siderophore) uptake and utilization system, parts of the enterobactin synthesis pathway, TolC (an outer-membrane channel protein) or Fur (an ironresponsive regulator) were hypersensitive to wrwycr. We provide evidence that the DtolC mutant was hypersensitive to wrwycr due to its reduced ability to efflux wrwycr from the cell rather than due to its export of newly synthesized enterobactin. Deleting ryhB, which encodes a small RNA involved in iron regulation, mostly relieved the wrwycr hypersensitivity of the fur and ferricenterobactin uptake mutants, indicating that the altered regulation of a RyhB-controlled gene was at least partly responsible for the hypersensitivity of these strains. Chelatable iron in the cell, measured by electron paramagnetic resonance spectroscopy, increased dramatically following wrwycr treatment, as did expression of Fur-repressed genes and, to some extent, mutation frequency. These incongruous results suggest that while wrwycr treatment caused accumulation of chelatable iron in the cell, iron was not available to bind to Fur. This is corroborated by the observed induction of the suf system, which assembles iron-sulfur clusters in low-iron conditions. Disruption of iron metabolism by wrwycr, in addition to its effects on DNA repair, may make it a particularly effective antimicrobial in the context of the low-iron environment of a mammalian host.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Escherichia coli enterobactin synthesis and uptake mutants are hypersensitive to an antimicrobial peptide that limits the availability of iron in addition to blocking Holliday junction resolution

2012

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“…Peptide wrwycr and its close relatives stabilize HJ intermediates of phage lambda site-specific recombination in E. coli and inhibit the tyrosine recombinase-dependent excision of prophages in both E. coli and Salmonella enterica LT2 (23). Treatment of E. coli with the peptide also resulted in the accumulation of filamentous cells and a 10-fold increase in anucleate cells, suggesting that the loss of bacterial viability was due to the combined effects of DNA breaks and chromosome segregation defects (22).…”

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confidence: 99%

An Antimicrobial Peptide That Targets DNA Repair Intermediates In Vitro Inhibits Salmonella Growth within Murine Macrophages

Willner

Segall

2010

Antimicrob Agents Chemother

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The hexapeptide WRWYCR was previously identified on the basis of its ability to inhibit bacteriophage lambda integrase-mediated recombination by trapping and preventing resolution of the Holliday junction intermediate. This peptide inhibits several unrelated DNA repair enzymes that bind to and process Holliday junctions and branched DNA substrates. WRWYCR and its D stereoisomer, wrwycr, are bactericidal against both Gram-positive and Gram-negative bacteria, causing the accumulation of DNA breaks, chromosome segregation defects, and the filamentation of cells. DNA repair is a novel target of antibiotics. In the present study, we examined the ability of the peptides to inhibit the growth of Salmonella in mammalian cells. J774A.1 macrophage-like cells and murine peritoneal macrophages were infected with Salmonella enterica serovar Typhimurium and grown in the presence or absence of peptide. We found that peptide wrwycr reduced the number of Salmonella cells recovered after 24 h growth in J774A.1 cells by 100 to 1,000 times, depending on the multiplicity of infection. The peptide also inhibited Salmonella growth in peritoneal macrophages, and although higher doses were required, these were not toxic to the host cells. The apparent lower level of potency of the peptide paralleled the lower level of replication of Salmonella and the lower level of permeation of the peptide in the peritoneal macrophages than in the J774.1 cells. Treatment with peptide wrwycr elicited the SOS response in a significant fraction of the intracellular bacteria, as would be expected if the mechanism of bacterial killing was the same in pure culture and in host cells. These results represent a proof of principle of the antimicrobial activities of compounds that target DNA repair.The hexapeptide WRWYCR was previously identified on the basis of its ability to inhibit bacteriophage lambda integrase (Int)-mediated site-specific recombination by accumulating the Holliday junction (HJ) intermediates during the reaction (4). Holliday junctions are also central intermediates in homologous recombination-dependent DNA repair, which often but not exclusively involves RecA-dependent strand invasion. The double-strand breaks that are generated by oxidative damage, irradiation, or interstrand cross-links or nicks that have been converted to double-strand breaks during replication require repair of the break by use of the homology on the sister chromosome (14,15,28). During the repair process, chromosome dimers may arise. Such dimeric chromosomes cannot be properly segregated to daughter cells, unless they are converted to monomers by the Int-related bacterial site-specific recombinases XerC and XerD, which also generate Holliday junction intermediates during recombination at dif sites (3). These processes are extremely important, if not essential; for example, up to 50% of recA mutant cells are nonviable, and the remainder are hypersensitive to any DNA damage (14). Although mutations in XerC and/or XerD are not lethal, they are detrimental to cell growth, ...

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“…6, A-D) reveals a narrow range of FRET values for conformational fluctuations, which neighbors IsoII in its mean FRET value, without evidence for discrete states. As a further test of the generality of peptideinduced conformational changes, we incubated the GC junction with the peptide WRWYCR, which also inhibits Holliday junction resolution (29,31,33). The effects of WRWYCR on GC junction behavior were analogous to those of KWWCRW (data not shown).…”

Section: Resultsmentioning

confidence: 99%

“…Indeed, through screens of a combinatorial library, short synthetic hexapeptides with these properties have been identified (23)(24)(25)(26). These peptides have been shown to impede the unwinding of branched DNA substrates by the RecG helicase of Escherichia coli, to interfere with Holliday junction resolution by the RuvABC complex, and to inhibit site-specific recombination by tyrosine recombinases, with accumulation of the Holliday junction intermediate (23,24,(27)(28)(29)(30)(31).…”

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confidence: 99%

Hexapeptides That Inhibit Processing of Branched DNA Structures Induce a Dynamic Ensemble of Holliday Junction Conformations

Cannon¹,

Kachroo²,

Jarmoskaite³

et al. 2015

Journal of Biological Chemistry

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Peptide wrwycr Inhibits the Excision of Several Prophages and Traps Holliday Junctions inside Bacteria

Cited by 25 publications

References 33 publications

Escherichia coli enterobactin synthesis and uptake mutants are hypersensitive to an antimicrobial peptide that limits the availability of iron in addition to blocking Holliday junction resolution

Escherichia coli enterobactin synthesis and uptake mutants are hypersensitive to an antimicrobial peptide that limits the availability of iron in addition to blocking Holliday junction resolution

An Antimicrobial Peptide That Targets DNA Repair Intermediates In Vitro Inhibits Salmonella Growth within Murine Macrophages

Hexapeptides That Inhibit Processing of Branched DNA Structures Induce a Dynamic Ensemble of Holliday Junction Conformations

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