DNA repair‐deficient premature aging models display accelerated epigenetic age

Author:

Perez Kevin12,Parras Alberto12,Picó Sara1,Rechsteiner Cheyenne1,Haghani Amin3,Brooke Robert4,Mrabti Calida1,Schoenfeldt Lucas12,Horvath Steve345ORCID,Ocampo Alejandro12ORCID

Affiliation:

1. Department of Biomedical Sciences, Faculty of Biology and Medicine University of Lausanne Lausanne Switzerland

2. EPITERNA SA Epalinges Switzerland

3. Altos Labs San Diego California USA

4. Epigenetic Clock Development Foundation Torrance California USA

5. Human Genetics, David Geffen School of Medicine University of California Los Angeles California USA

Abstract

AbstractSeveral premature aging mouse models have been developed to study aging and identify interventions that can delay age‐related diseases. Yet, it is still unclear whether these models truly recapitulate natural aging. Here, we analyzed DNA methylation in multiple tissues of four previously reported mouse models of premature aging (Ercc1, LAKI, Polg, and Xpg). We estimated DNA methylation (DNAm) age of these samples using the Horvath clock. The most pronounced increase in DNAm age could be observed in Ercc1 mice, a strain which exhibits a deficit in DNA nucleotide excision repair. Similarly, we detected an increase in epigenetic age in fibroblasts isolated from patients with progeroid syndromes associated with mutations in DNA excision repair genes. These findings highlight that mouse models with deficiencies in DNA repair, unlike other premature aging models, display accelerated epigenetic age, suggesting a strong connection between DNA damage and epigenetic dysregulation during aging.

Funder

Schweizerischer Nationalfonds zur Förderung der Wissenschaftlichen Forschung

Publisher

Wiley

Subject

Cell Biology,Aging

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