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Literature DB >> 9230304

The translocating RecBCD enzyme stimulates recombination by directing RecA protein onto ssDNA in a chi-regulated manner.

Abstract

Double-stranded DNA break repair and homologous recombination in E. coli are initiated by the RecBCD enzyme, which unwinds and simultaneously degrades DNA from a double-stranded DNA end. This process is stimulated by cis-acting DNA elements, known as chi sites. Using both in vitro pairing and nuclease protection assays, we demonstrate that the translocating RecBCD enzyme, which has been activated by chi, coordinates the preferential loading of the homologous pairing protein, RecA, onto the resultant single-stranded DNA downstream of chi. This facilitated loading of RecA protein results in a substantial increase in both the efficiency and rate of in vitro recombination reactions and offers an explanation for stimulation of recombination and repair in vivo by chi.

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Year: 1997 PMID： 9230304 DOI： 10.1016/s0092-8674(00)80315-3

Source DB: PubMed Journal: Cell ISSN： 0092-8674 Impact factor: 41.582

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Cited

130 in total

1. Impairment of lagging strand synthesis triggers the formation of a RuvABC substrate at replication forks.

Authors: M J Flores; H Bierne; S D Ehrlich; B Michel
Journal: EMBO J Date: 2001-02-01 Impact factor: 11.598

2. Palindromes as substrates for multiple pathways of recombination in Escherichia coli.

Authors: G A Cromie; C B Millar; K H Schmidt; D R Leach
Journal: Genetics Date: 2000-02 Impact factor: 4.562

3. The RecBC enzyme loads RecA protein onto ssDNA asymmetrically and independently of chi, resulting in constitutive recombination activation.

Authors: J J Churchill; D G Anderson; S C Kowalczykowski
Journal: Genes Dev Date: 1999-04-01 Impact factor: 11.361

4. RecE/RecT and Redalpha/Redbeta initiate double-stranded break repair by specifically interacting with their respective partners.

Authors: J P Muyrers; Y Zhang; F Buchholz; A F Stewart
Journal: Genes Dev Date: 2000-08-01 Impact factor: 11.361

10. RecFOR function is required for DNA repair and recombination in a RecA loading-deficient recB mutant of Escherichia coli.

Authors: Ivana Ivancić-Baće; Petra Peharec; Suncana Moslavac; Nikolina Skrobot; Erika Salaj-Smic; Krunoslav Brcić-Kostić
Journal: Genetics Date: 2003-02 Impact factor: 4.562

The translocating RecBCD enzyme stimulates recombination by directing RecA protein onto ssDNA in a chi-regulated manner.

1. Impairment of lagging strand synthesis triggers the formation of a RuvABC substrate at replication forks.

2. Palindromes as substrates for multiple pathways of recombination in Escherichia coli.

3. The RecBC enzyme loads RecA protein onto ssDNA asymmetrically and independently of chi, resulting in constitutive recombination activation.

4. RecE/RecT and Redalpha/Redbeta initiate double-stranded break repair by specifically interacting with their respective partners.

5. RecA protein promotes the regression of stalled replication forks in vitro.

Review 6. Historical overview: searching for replication help in all of the rec places.

7. Effects of DNA sequence and structure on binding of RecA to single-stranded DNA.

8. Crossing over between regions of limited homology in Escherichia coli. RecA-dependent and RecA-independent pathways.

9. The RecA proteins of Deinococcus radiodurans and Escherichia coli promote DNA strand exchange via inverse pathways.

10. RecFOR function is required for DNA repair and recombination in a RecA loading-deficient recB mutant of Escherichia coli.