Nuclear factories for signalling and repairing DNA double strand breaks in living fission yeast

doi:10.1093/nar/gkg719

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Nucleic Acids Research, 2003, Vol. 31, No. 17 5064-5073
© 2003 Oxford University Press

Nuclear factories for signalling and repairing DNA double strand breaks in living fission yeast

Peter Meister, Mickaël Poidevin, Stefania Francesconi, Isabelle Tratner, Patrick Zarzov and Giuseppe Baldacci^*

Institut Curie – CNRS UMR 2027, Bâtiment 110, Centre Universitaire, 91405 Orsay Cedex, France

*To whom correspondence should be addressed. Tel: +33 1 698 67185; Fax: +33 1 698 63058; Email: giuseppe.baldacci{at}curie.u-psud.fr

In mammalian and budding yeast cells treated with genotoxicagents, different proteins implicated in detecting, signallingor repairing DNA lesions form nuclear foci. We studied fociformed by proteins involved in these processes in living fissionyeast cells, which is amenable to genetic and molecular analysis.Using fluorescent tags, we analysed subnuclear localisationsof the DNA damage checkpoint protein Rad9, of the homologousrecombination protein Rad22 and of PCNA, which are implicatedin many aspects of DNA metabolism. After inducing double strandbreaks (DSBs) with ionising radiations, Rad22, Rad9 and PCNAform a low number of nuclear foci. Rad9 recruitment to focidepends on the presence of Rad1, Hus1 and Rad17, but is independentof downstream checkpoint effectors and of homologous recombinationproteins. Likewise, Rad22 and PCNA form foci despite inactivehomologous recombination repair and impaired DNA damage checkpoint.Rad22 and Rad9 foci co-localise completely, whereas PCNA co-localiseswith Rad22 and Rad9 only partially. Foci do not disassemblein cells unable to repair DNA by homologous recombination. Thus,in fission yeast, DSBs are detected by the DNA damage checkpointand are repaired by homologous recombination at a few spatiallyconfined subnuclear compartments where Rad22, Rad9 and PCNAconcentrate independently.

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