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DNA Dynamics and Chromosome Structure

DNA Damage-Dependent Nuclear Dynamics of the Mre11 Complex

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Pages 281-288 | Received 20 Jul 2000, Accepted 10 Oct 2000, Published online: 28 Mar 2023
 

Abstract

The Mre11 complex has been implicated in diverse aspects of the cellular response to DNA damage. We used in situ fractionation of human fibroblasts to carry out cytologic analysis of Mre11 complex proteins in the double-strand break (DSB) response. In situ fractionation removes most nucleoplasmic protein, permitting immunofluorescent localization of proteins that become more avidly bound to nuclear structures after induction of DNA damage. We found that a fraction of the Mre11 complex was bound to promyelocyte leukemia protein bodies in undamaged cells. Within 10 min after gamma irradiation, nuclear retention of the Mre11 complex in small granular foci was observed and persisted until 2 h postirradiation. In light of the previous demonstration that the Mre11 complex associated with ionizing radiation (IR)-induced DSBs, we infer that the protein retained under these conditions was associated with DNA damage. We also observed increased retention of Rad51 following IR treatment, although IR induced Rad51 foci were distinct from Mre11 foci. The ATM kinase, which phosphorylates Nbs1 during activation of the S-phase checkpoint, was not required for the Mre11 complex to associate with DNA damage. These data suggest that the functions of the Mre11 complex in the DSB response are implicitly dependent upon its ability to detect DNA damage.

View correction statement:
DNA Damage-Dependent Nuclear Dynamics of the Mre11 Complex

ACKNOWLEDGMENTS

We are grateful to the members of the lab for insights throughout the course of this study and to Mark Kaplan and Mary Ellen Perry for comments and suggestions on the manuscript.

This work was supported by the Milwaukee Foundation, the National Institutes of Health (GM56888 and GM59413), and the Department of Energy (ER62859).

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