posted on 2025-05-11, 13:01authored byAndrew KellerAndrew Keller, Yue Xin, Stephanie Boer, Jonathan Reinhardt, Rachel Baker, Lidia K. Arciszewska, Peter J. Lewis, David J. Sherratt, Jan Löwe, Ian GraingeIan Grainge
Bacterial chromosomes are most often circular DNA molecules. This can produce a topological problem; a genetic crossover from homologous recombination results in dimerization of the chromosome. A chromosome dimer is lethal unless resolved. A site-specific recombination system catalyses this dimer-resolution reaction at the chromosomal site dif. In Escherichia coli, two tyrosine-family recombinases, XerC and XerD, bind to dif and carry out two pairs of sequential strand exchange reactions. However, what makes the reaction unique among site-specific recombination reactions is that the first step, XerD-mediated strand exchange, relies on interaction with the very C-terminus of the FtsK DNA translocase. FtsK is a powerful molecular motor that functions in cell division, co-ordinating division with clearing chromosomal DNA from the site of septation and also acts to position the dif sites for recombination. This is a model system for unlinking, separating and segregating large DNA molecules. Here we describe the molecular detail of the interaction between XerD and FtsK that leads to activation of recombination as deduced from a co-crystal structure, biochemical and in vivo experiments. FtsKγ interacts with the C-terminal domain of XerD, above a cleft where XerC is thought to bind. We present a model for activation of recombination based on structural data.
Funding
NHMRC
1005697 and ARC FT120100153
History
Journal title
Scientific Reports
Volume
6
Article number
33357
Publisher
Nature Publishing Group
Language
en, English
College/Research Centre
Faculty of Science
School
School of Environmental and Life Sciences
Rights statement
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