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Defective transfer of parental histone decreases frequency of homologous recombination by increasing free histone pools in budding yeast

Srinivasu Karri, Yi Yang,Jiaqi Zhou,Quinn Dickinson, Jing Jia, Yuxin Huang,Zhiquan Wang, Haiyun Gan,Chuanhe Yu

Nucleic acids research(2024)

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Abstract
Recycling of parental histones is an important step in epigenetic inheritance. During DNA replication, DNA polymerase epsilon subunit DPB3/DPB4 and DNA replication helicase subunit MCM2 are involved in the transfer of parental histones to the leading and lagging strands, respectively. Single Dpb3 deletion (dpb3 Delta) or Mcm2 mutation (mcm2-3A), which each disrupts one parental histone transfer pathway, leads to the other's predominance. However, the biological impact of the two histone transfer pathways on chromatin structure and DNA repair remains elusive. In this study, we used budding yeast Saccharomyces cerevisiae to determine the genetic and epigenetic outcomes from disruption of parental histone H3-H4 tetramer transfer. We found that a dpb3 Delta mcm2-3A double mutant did not exhibit the asymmetric parental histone patterns caused by a single dpb3 Delta or mcm2-3A mutation, suggesting that the processes by which parental histones are transferred to the leading and lagging strands are independent. Surprisingly, the frequency of homologous recombination was significantly lower in dpb3 Delta, mcm2-3A and dpb3 Delta mcm2-3A mutants, likely due to the elevated levels of free histones detected in the mutant cells. Together, these findings indicate that proper transfer of parental histones during DNA replication is essential for maintaining chromatin structure and that lower homologous recombination activity due to parental histone transfer defects is detrimental to cells. Graphical Abstract
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