Vitamin D supplementation is associated with slower epigenetic aging

被引:0
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作者
Valentin Max Vetter
Yasmine Sommerer
Christian Humberto Kalies
Dominik Spira
Lars Bertram
Ilja Demuth
机构
[1] Corporate Member of Freie Universität Berlin and Humboldt-Universität zu Berlin,Biology of Aging Working Group, Department of Endocrinology and Metabolic Diseases (Including Division of Lipid Metabolism), Charité – Universitätsmedizin Berlin
[2] Humboldt University Berlin,Department of Psychology
[3] University of Lübeck,Lübeck Interdisciplinary Platform for Genome Analytics (LIGA)
[4] University of Oslo,Center for Lifespan Changes in Brain and Cognition (LCBC), Department of Psychology
[5] Charité - Universitätsmedizin Berlin,BCRT
[6] Charité - Universitätsmedizin Berlin, Berlin Institute of Health Center for Regenerative Therapies
来源
GeroScience | 2022年 / 44卷
关键词
Biological age; DNA methylation age; Epigenetic clock; BASE-II; GendAge; Longitudinal; Vitamin D supplementation;
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学科分类号
摘要
Adverse effects of low vitamin D level on mortality and morbidity are controversially discussed. Especially older people are at risk for vitamin D deficiency and therefore exposed to its potentially harmful consequences. A way of measuring differences in the biological age is through DNA methylation age (DNAm age) and its deviation from chronological age, DNAm age acceleration (DNAmAA). We previously reported on an association between vitamin D deficiency and higher 7-CpG DNAmAA in participants of the Berlin Aging Study II (BASE-II). In this study, we employ a quasi-interventional study design to assess the relationship between DNAmAA of five epigenetic clocks and vitamin D supplementation. Longitudinal data were available for 1,036 participants of BASE-II that were reexamined on average 7.4 years later in the GendAge study (mean age at follow-up: 75.6 years, SD = 3.8 years, age range: 64.9–94.1 years, 51.9% female). DNAmAA was estimated with the 7-CpG clock, Horvath’s clock, Hannum’s clock, PhenoAge, and GrimAge. Methylation data were obtained through methylation-sensitive single nucleotide primer extension (MS-SNuPE) or Illumina’s Infinium “MethylationEPIC” array. Vitamin D–deficient participants who chose to start vitamin D supplementation after baseline examination showed a 2.6-year lower 7-CpG DNAmAA (p = 0.011) and 1.3-year lower Horvath DNAmAA (p = 0.042) compared to untreated and vitamin D–deficient participants. DNAmAA did not statistically differ between participants with successfully treated vitamin D deficiency and healthy controls (p > 0.16). Therefore, we conclude that intake of vitamin D supplement is associated with lower DNAmAA in participants with vitamin D deficiency.
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页码:1847 / 1859
页数:12
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