O~6-methylguanine-induced Cell Death Involvesexonuclease 1 As Well As Dna Mismatch Recognition In Vivo

摘要

Alkylation-induced O~6-methylguanine (O~6MeG) DNA lesions can be mutagenic or cytotoxic if unrepaired by the O~6MeG-DNA methyl transferase (Mgmt) protein. O~6MeG pairs with T during DNA replication, and if the O~6MeG:T mismatch persists, a G:C to A:T transition mutation is fixed at the next replication cycle. O~6MeG:T mismatch detection by MutSα and MutLα leads to apoptotic cell death, but the mechanism by which this occurs has been elusive. To explore how mismatch repair mediates O~6MeG-dependent apop tosis, we used an Mgmt-null mouse model combined with either the Msh6-null mutant (defective in mismatch recognition) or the Exo1-null mutant (impaired in the excision step of mismatch repair). Mouse embryonic fibroblasts and bone marrow cells derived from Mgmt-null mice were much more alkylation-sensitive than wild type, as expected. However, ablation of either Msh6 or Exo1 function rendered these Mgmt-null cells just as resistant to alkylation-induced cytotoxicity as wild-type cells. Rapidly proliferating tissues in Mgmt-null mice (bone marrow, thymus, and spleen) are extremely sensitive to apoptosis induced by O~6MeG-producing agents. Here, we show that ablation of either Msh6 or Exo1 function in the Mgmt-null mouse renders these rapidly proliferating tissues alkylation-resistant. However, whereas the Msh6 defect confers total alkylation resistance, the Exo1 defect leads to a variable tissue-specific alkylation resistance phenotype. Our results indicate that Exo1 plays an important role in the induction of apoptosis by unrepaired O~6MeGs.