UvsX Recombinase and Dda Helicase Rescue Stalled Bacteriophage T4 DNA Replication Forks in Vitro

Kadyrov, Farid A.; Drake, John W.

doi:10.1074/jbc.m403942200

Cited by 29 publications

(34 citation statements)

References 49 publications

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“…More specifically, we wished to investigate whether there was evidence for E. coli possessing a transient template-switching mechanism of the kind first proposed by Higgins, Kato and Strauss in 1976 (6) for mammalian cells and later proposed for E. coli (4,5,16,19,24). In addition, a mechanism of this kind has been reconstructed in vitro, using purified phage T4 proteins (8,9). However, this model has been difficult to explore experimentally in vivo because the recombination event depends on informa-tional, rather than physical, exchange between DNA strands and because it occurs between identical sister strands.…”

Section: Discussionmentioning

confidence: 99%

“…Because such transfer occurs between genetically identical sister duplexes, exchange cannot be detected by means of genetically marked strains. As a consequence, there is little in vivo evidence to support the occurrence of such a mechanism or to indicate its genetic requirements, such as dependence on RecA, though in vitro results with E. coli and phage T4 proteins strongly support such a model (5,7,8,9,16,17,(19)(20)(21). We have investigated the possible occurrence of such an alternative recombination mechanism for the completion of replication in the face of unrepaired DNA damage by transforming various E. coli strains with plasmids in which each strand carried, at specific staggered positions, a single thyminethymine pyrimidine (6-4) pyrimidinone [T-T (6-4)] lesion.…”

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In Vivo Evidence for a recA -Independent Recombination Process in Escherichia coli That Permits Completion of Replication of DNA Containing UV Damage in Both Strands

2005

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We have investigated recombination mechanisms promoting the completion of replication in the face of unrepaired DNA damage by transforming an isogenic set of uvrA6 excision-defective Escherichia coli strains with pUC-based plasmids in which each strand carried, at staggered positions, a single thymine-thymine pyrimidine (6-4) pyrimidinone lesion. The distance between the lesions was 28 or 8 bp in one orientation relative to the unidirectional ColE1 origin of replication or, in the other orientation, 30 or 10 bp. C-C mismatches placed opposite each of the T-T photoproducts permit unambiguous detection of the three events that can lead to the completion of replication: sister-strand recombination, translesion replication (TR) on the leading strand, and TR on the lagging strand. We find that E. coli possesses a largely constitutive, recAindependent sister-strand recombination mechanism that allows 9% or more of these severely compromised plasmids to be fully replicated. In one orientation, such recombination depends partly on recG and priA but not on ruvA, ruvB, ruvC, or mutS and is largely independent of recF. In the other orientation, recombination is dependent on none of the genes. The strains used did not contain the cryptic phage encoding recET, which encodes enzymes that promote interplasmid recombination. The nature of the recA-independent recombination mechanism is not known but could perhaps result from a template-strand-switching, or copy choice, process.In addition to DNA repair processes, which accurately remove damage arising spontaneously or from overt mutagen exposure, Escherichia coli possesses tolerance mechanisms that promote the completion of genome replication in the presence of unrepaired DNA damage that might otherwise block this process (reviewed in reference 14). Apart from blocking replication, unrepaired damage may also result in the collapse of the replication fork and the production of double-strand breaks, a particularly damaging outcome (13). Two general categories of mechanism exist to overcome the potential lethality arising from incomplete replication of the genome, one employing recombination and the other using translesion replication (TR). In the latter case, DNA polymerase V is used to replicate past the lesion, or for some lesions and circumstances, DNA polymerase IV or DNA polymerase II is used (23). Recombination-based mechanisms serve to rectify two different conditions associated with incomplete replication, the occurrence of single-stranded gaps that remain after reinitiation of replication beyond the site of the lesion and the occurrence of double-strand breaks. Although the first of these requires the activities of the recF pathway and the second depends on the recBC pathway, they both depend on the RecA protein, which is also required for TR (reviewed in reference 14).A third recombination-based mechanism, involving transient template strand switching or copy choice, has been proposed (6) but has proved difficult to investigate experimentally in vivo. Unlike the other m...

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Section: Discussionmentioning

confidence: 99%

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confidence: 99%

In Vivo Evidence for a recA -Independent Recombination Process in Escherichia coli That Permits Completion of Replication of DNA Containing UV Damage in Both Strands

2005

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“…Subsequent enzymological analyses using an eight-protein T4 DNA replication system in vitro showed that strand switching could indeed be promoted by DNA damage in the template strand and that the resulting replication repair was severely compromised when the mutant gp32 and gp41 proteins replaced their wild-type counterparts (Kadyrov and Drake 2003). Then, somewhat surprisingly, an alternative T4 system of replication repair was discovered in vitro in which gp32 and gp41 were replaced by the classical T4 recombinase UvsX and a different T4 DNA helicase, Dda (Kadyrov and Drake 2004). To date, these are the only genetically and enzymologically well-defined replication-repair systems.…”

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Templated Mutagenesis in Bacteriophage T4 Involving Imperfect Direct or Indirect Sequence Repeats

Schultz

Drake

2008

Genetics

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Some mutations arise in association with a potential sequence donor that consists of an imperfect direct or reverse repeat. Many such mutations are complex; that is, they consist of multiple close sequence changes. Current models posit that the primer terminus of a replicating DNA molecule dissociates, reanneals with an ectopic template, extends briefly, and then returns to the cognate template, bringing with it a locally different sequence; alternatively, a hairpin structure may form the mutational intermediate when processed by mismatch repair. This process resembles replication repair, in which primer extension is blocked by a lesion in the template; in this case, the ectopic template is the other daughter strand, and the result is errorfree bypass of the lesion. We previously showed that mutations that impair replication repair can enhance templated mutagenesis. We show here that the intensity of templated mutation can be exquisitely sensitive to its local sequence, that the donor and recipient arms of an imperfect inverse repeat can exchange roles, and that double mutants carrying two alleles, each affecting both templated mutagenesis and replication repair, can have unexpected phenotypes. We also record an instance in which the mutation rates at two particular sites change concordantly with a distant sequence change, but in a manner that appears unrelated to templated mutagenesis. T EMPLATED mutations are initiated when a DNA primer strand dissociates from its cognate template and anneals with a fragment of complementary sequence in an ectopic template. The relocated primer may be extended, acquiring a short sequence that is not fully complementary to the original template, and then reanneal with its cognate template. If the acquired noncomplementary bases escape correctly oriented proofreading and mismatch repair, mutations will result. Lynn Ripley (1982) described two models for templated mutagenesis based on imperfect palindromic repeats, in one of which the ectopic template was in the other parental strand and in the other of which the ectopic template was in the daughter strand itself. Examination of other mutations added imperfect direct repeats as mutagenic templates (Ripley et al. 1986;Shinedling et al. 1987). Templated mutations are usually invoked when they simultaneously acquire multiple changes for which a plausible donor template can be found. Despite the intrinsic fascination of templated complex mutations and their potential importance for certain evolutionary paths and some human genetic disorders, the enzymology that creates them has not been characterized.Template switching also occurs in a mutation-avoiding mode called replication repair. In the canonical model for replication repair (Fujiwara and Tatsumi 1976;Higgins et al. 1976), a primer strand whose extension has been blocked by DNA damage switches to the other daughter strand as a template, extends briefly, and then switches back to its cognate template, thus accurately bypassing the damaged site.In 1987, a mechanism for su...

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“…The translesion synthesis pathway is error prone due to the participation of low-fidelity DNA polymerases (21). The cleavage pathway is thought to be the dominant mode in bacteria, while replication repair (through template switching and translesion synthesis) is the dominant mode in T4 and eukaryotes (14).…”

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Hjm/Hel308A DNA Helicase fromSulfolobus tokodaiiPromotes Replication Fork Regression and Interacts with Hjc Endonuclease In Vitro

Hou

et al. 2008

J Bacteriol

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Hjm and Hel308a are novel, RecQ-like DNA helicases recently identified in the euryarchaeotes Pyrococcus furiosus and Methanothermobacter thermautotrophicus, respectively. In this study, an Hjm/Hel308 homologue (designated StoHjm) from Sulfolobus tokodaii, a hyperthermophilic archaeon belonging to the Crenarchaeota subdomain of archaea, was cloned, purified, and characterized. Unlike Hjm and Hel308a, which unwind DNA in a 3-to-5 direction, StoHjm unwound DNA in both 3-to-5 and 5-to-3 directions. Remarkably, StoHjm exhibited structure-specific single-stranded-DNA-annealing and fork regression activities in vitro. In addition, gel filtration, affinity pulldown, and yeast two-hybrid analyses revealed that StoHjm physically interacted with StoHjc, the Holliday junction-specific endonuclease from S. tokodaii. This interaction may have functional significance, because the unwinding activity of StoHjm was inhibited by StoHjc in vitro. These results may suggest that the Hjm/Hel308 family helicases, in association with Hjc endonucleases, are involved in processing of stalled replication forks.

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UvsX Recombinase and Dda Helicase Rescue Stalled Bacteriophage T4 DNA Replication Forks in Vitro

Cited by 29 publications

References 49 publications

In Vivo Evidence for a recA -Independent Recombination Process in Escherichia coli That Permits Completion of Replication of DNA Containing UV Damage in Both Strands

In Vivo Evidence for a recA -Independent Recombination Process in Escherichia coli That Permits Completion of Replication of DNA Containing UV Damage in Both Strands

Templated Mutagenesis in Bacteriophage T4 Involving Imperfect Direct or Indirect Sequence Repeats

Hjm/Hel308A DNA Helicase fromSulfolobus tokodaiiPromotes Replication Fork Regression and Interacts with Hjc Endonuclease In Vitro

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