Abstract
SummaryRepair of DNA double strand breaks by the non-homologous end-joining pathway is initiated by the binding of Ku to DNA ends. Given its high affinity for ends, multiple Ku proteins load onto linear DNAs in vitro. However, in cells, Ku loading is limited to ∼1-2 molecules per DNA end. The mechanisms enforcing this limit are currently unknown. Here we show that the catalytic subunit of the DNA-dependent protein kinase (DNA-PKcs), but not its protein kinase activity, is required to prevent excessive Ku entry into chromatin. Ku accumulation is further restricted by two mechanisms: a neddylation/FBXL12-dependent process which actively removes loaded Ku molecules throughout the cell cycle and a CtIP/ATM-dependent mechanism which operates in S-phase. Finally, we demonstrate that the misregulation of Ku loading leads to impaired transcription in the vicinity of DNA ends. Together our data shed light on the multiple layers of coordinated mechanisms operating to prevent Ku from invading chromatin and interfering with other DNA transactions.HighlightsDNA-PKcs structurally blocks Ku sliding into chromatin in human &XenopusA neddylation/FBXL12-dependent mechanism limits Ku accumulation on chromatinIn S-phase, ATM/CtIP overcomes Ku accumulationIn absence of DNA-PKcs, transcription at the DNA end vicinity is inhibitedeTOC blurbThe DNA end binding protein Ku can slide onto naked DNA but this is limited in cells. Using human cells andXenopusegg extracts, DNA-PKcs is identified as the main structural barrier to Ku entry into chromatin, along with two active mechanisms which limit Ku accumulation in absence of DNA-PKcs.Graphical abstract
Publisher
Cold Spring Harbor Laboratory