Ribosomal DNA (rDNA) encodes the 18S, 5.8S, and 28S rRNA, accounting for â¼70% of cellular transcription. Despite its essential role and links to cancer and aging, quantifying rDNA instability in mammals remains challenging due to its repetitive organization and inherent heterogeneity. Here, we developed a murine rDNA FISH probe and genomic tools tailored for laboratory mouse strains. The results confirmed rDNA cluster locations, revealed substantial inter- and intra-strain as well as intercellular heterogeneity in rDNA organization within inbred mice and unstressed cells, and identified sources of spontaneous and replication-associated DNA double-strand breaks in the rDNA transcription termination region. Using mouse embryonic stem cells, we showed that BRCA1-mediated homologous recombination promotes rDNA instability, the non-homologous end joining factor XRCC1, but not Ku, suppresses intra-cluster deletions, and ATM kinase preserves rDNA cluster stability. Together, these findings establish a platform and tools for studying rDNA instability in animal models relevant to aging and cancer research.
Visualization and quantification of rDNA instabilities in mammalian cells and mouse models.
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作者:Zhu Xiaolu, Jiang Wenxia, Wu Wei, Lee Brian J, Menolfi Demis, Tubbs Anthony, Cupo Olivia M, Malkovskiy Eli, Nester Mattie, Wang Xiaobin S, Sims Peter A, Lin Chyuan-Sheng V, Symington Lorraine, Nussenzweig Andre, McStay Brian, Zha Shan
| 期刊: | Nucleic Acids Research | 影响因子: | 13.100 |
| 时间: | 2026 | 起止号: | 2026 Jan 14; 54(2):gkaf1523 |
| doi: | 10.1093/nar/gkaf1523 | ||
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