3' homologous free ends are required for stable joint molecule formation by the RecA and single-stranded binding proteins of Escherichia coli.

Konforti, Boyana; Davis, Ronald W.

doi:10.1073/pnas.84.3.690

Cited by 76 publications

(56 citation statements)

References 14 publications

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“…32P-labeled homologous dsDNA was prepared by digesting supercoiled pUC8 with HaeII, followed by treatment with mung bean nuclease. After separation on 1% agarose gels, the 1.87-kb segment was isolated as described by Tautz and Renz (1983) This method was modified from that of Konforti and Davis (1987). Supercoiled pUC8 was isolated by CsCl/ethidium bromide isopyknic centrifugation (Sambrook et al, 1989).…”

Section: Methodsmentioning

confidence: 99%

“…coli RecA promotes the exchange of DNA strands between a variety of cDNA substrates. Gel electrophoresis has been used extensively to identify the products of this reaction by their mobility (Konforti and Davis, 1987;Griffith and Harris, 1988;McCarthy et al, 1988). However, in crude cellular extracts, other enzymic activities can lead to artifactual products as discussed in detail by Griffith and Harris (1988).…”

Section: Strand-transfer Activity In Chloroplast Extractsmentioning

confidence: 99%

“…In the assays with linear 32P-ssDNA and closed circular dsDNA from pUC8, we used the conditions described by Konforti and Davis (1987) with 10 min of incubation without adding E. coli ssDNAbinding protein. A11 subsequent manipulations were as described above.…”

Section: Permeabilized Chloroplastsmentioning

confidence: 99%

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DNA Strand-Transfer Activity in Pea (Pisum sativum L.) Chloroplasts

Cerutti

Jagendorf

1993

Plant Physiol.

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The occurrence of DNA recombination in plastids of higher plants is well documented. However, little is known at the enzymic level. To begin dissecting the biochemical mechanism(s) involved we focused on a key step: strand transfer between homologous parenta1 DNAs. We detected a RecA-like strand transfer activity in stromal extracts from pea (Pisum sativum 1.) chloroplasts. Formation of joint molecules requires MgZ+, ATP, and homologous substrates. This activity is inhibited by excess single-stranded DNA (ssDNA), suggesting a necessary stoichiometric relation between enzyme and ssDNA. In a nove1 assay with Triton X-100-permeabilized chloroplasts, we also detected strand invasion of the endogenous chloroplast DNA by 3ZP-labeled ssDNA complementary to the 16s rRNA gene. Joint molecules, analyzed by electron microscopy, contained the expected displacement loops.

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Section: Methodsmentioning

confidence: 99%

Section: Strand-transfer Activity In Chloroplast Extractsmentioning

confidence: 99%

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DNA Strand-Transfer Activity in Pea (Pisum sativum L.) Chloroplasts

Cerutti

Jagendorf

1993

Plant Physiol.

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“…Recombination initiated by the RecBCD enzyme begins from such a blunt dsDNA end present at a dsDNA break, produced as the result of DNA damage, a broken replication fork, or conjugal DNA transfer. After binding to this end, the helicase and nuclease activities of RecBCD enzyme convert the dsDNA to a 3Ј-ssDNA overhang, a product that is the preferred substrate for RecA protein-mediated strand invasion (Konforti and Davis 1987;Anderson and Kowalczykowski 1997a,b;for review, see Kowalczykowski and Eggleston 1994). Because RecQ helicase also acts on blunt dsDNA ends and is needed for recombination in a recBCsbcBC background, it was proposed to act as a functional analog of RecBCD enzyme during this processing step (Clark and Sandler 1994;.…”

mentioning

confidence: 99%

RecQ helicase, in concert with RecA and SSB proteins, initiates and disrupts DNA recombination

Harmon¹,

Kowalczykowski²

1998

Genes & Development

258

224

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RecQ helicase is important to homologous recombination and DNA repair in Escherichia coli. We demonstrate that RecQ helicase, in conjunction with RecA and SSB proteins, can initiate recombination events in vitro. In addition, RecQ protein is capable of unwinding a wide variety of DNA substrates, including joint molecules formed by RecA protein. These data are consistent with RecQ helicase assuming two roles in the cell; it can be (1) an initiator of homologous recombination, or (2) a disrupter of joint molecules formed by aberrant recombination. These findings also shed light on the function of the eukaryotic homologs of RecQ helicase, the Sgs1, Blm, and Wrn helicases.

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“…Once a region suitable for recombination is found, RecA initiates a DNA strand exchange reaction that forms a recombination intermediate or joint molecule (Fig. 5) (83,335,345,346,505,638,639). Formation of the joint molecule results in the development of a mobile DNA heteroduplex known as a Holliday junction (146,264,345).…”

Section: Homologous Recombinationmentioning

confidence: 99%

Change Is Good: Variations in Common Biological Mechanisms in the Epsilonproteobacterial GeneraCampylobacterandHelicobacter

Gilbreath

Cody

Merrell

et al. 2011

Microbiol Mol Biol Rev

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SUMMARY Microbial evolution and subsequent species diversification enable bacterial organisms to perform common biological processes by a variety of means. The epsilonproteobacteria are a diverse class of prokaryotes that thrive in diverse habitats. Many of these environmental niches are labeled as extreme, whereas other niches include various sites within human, animal, and insect hosts. Some epsilonproteobacteria, such as Campylobacter jejuni and Helicobacter pylori , are common pathogens of humans that inhabit specific regions of the gastrointestinal tract. As such, the biological processes of pathogenic Campylobacter and Helicobacter spp. are often modeled after those of common enteric pathogens such as Salmonella spp. and Escherichia coli . While many exquisite biological mechanisms involving biochemical processes, genetic regulatory pathways, and pathogenesis of disease have been elucidated from studies of Salmonella spp. and E. coli , these paradigms often do not apply to the same processes in the epsilonproteobacteria. Instead, these bacteria often display extensive variation in common biological mechanisms relative to those of other prototypical bacteria. In this review, five biological processes of commonly studied model bacterial species are compared to those of the epsilonproteobacteria C. jejuni and H. pylori . Distinct differences in the processes of flagellar biosynthesis, DNA uptake and recombination, iron homeostasis, interaction with epithelial cells, and protein glycosylation are highlighted. Collectively, these studies support a broader view of the vast repertoire of biological mechanisms employed by bacteria and suggest that future studies of the epsilonproteobacteria will continue to provide novel and interesting information regarding prokaryotic cellular biology.

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3' homologous free ends are required for stable joint molecule formation by the RecA and single-stranded binding proteins of Escherichia coli.

Cited by 76 publications

References 14 publications

DNA Strand-Transfer Activity in Pea (Pisum sativum L.) Chloroplasts

DNA Strand-Transfer Activity in Pea (Pisum sativum L.) Chloroplasts

RecQ helicase, in concert with RecA and SSB proteins, initiates and disrupts DNA recombination

Change Is Good: Variations in Common Biological Mechanisms in the Epsilonproteobacterial GeneraCampylobacterandHelicobacter

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