Polo-like kinase-1 controls proteasome-dependent degradation of Claspin during checkpoint recovery

I Mamely, MATM van Vugt, VAJ Smits, JI Semple… - Current Biology, 2006 - cell.com
Current Biology, 2006cell.com
DNA-damage checkpoints maintain genomic integrity by mediating a cell-cycle delay in
response to genotoxic stress or stalled replication forks. In response to damage, the
checkpoint kinase ATR phosphorylates and activates its effector kinase Chk1 in a process
that critically depends on Claspin [1]. However, it is not known how exactly this kinase
cascade is silenced. Here we demonstrate that the abundance of Claspin is regulated
through proteasomal degradation. In response to DNA damage, Claspin is transiently …
Summary
DNA-damage checkpoints maintain genomic integrity by mediating a cell-cycle delay in response to genotoxic stress or stalled replication forks. In response to damage, the checkpoint kinase ATR phosphorylates and activates its effector kinase Chk1 in a process that critically depends on Claspin [1]. However, it is not known how exactly this kinase cascade is silenced. Here we demonstrate that the abundance of Claspin is regulated through proteasomal degradation. In response to DNA damage, Claspin is transiently stabilized, and its expression depends on Chk1 kinase activity. In addition, we show that Claspin is degraded upon mitotic entry, a process that depends on the β-TrCP-SCF ubiquitin ligase and Polo-like kinase-1 (Plk1). We demonstrate that Claspin interacts with both β-TrCP and Plk1 and that inactivation of these components or the β-TrCP recognition motif in Claspin prevents its mitotic degradation. Interestingly, expression of a nondegradable Claspin mutant inhibits recovery from a DNA-damage-induced checkpoint arrest. Thus, we conclude that Claspin levels are tightly regulated, both during unperturbed cell cycles and after DNA damage. Moreover, our data demonstrate that the degradation of Claspin at the onset of mitosis is an essential step for the recovery of a cell from a DNA-damage-induced cell-cycle arrest.
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