Advancing understanding of maternal age: correlating epigenetic clocks in blood and myometrium.

Epigenetics communications Pub Date : 2022-01-01 Epub Date: 2022-05-23 DOI:10.1186/s43682-022-00010-0

Elise N Erickson, Anna K Knight, Alicia K Smith, Leslie Myatt

{"title":"Advancing understanding of maternal age: correlating epigenetic clocks in blood and myometrium.","authors":"Elise N Erickson, Anna K Knight, Alicia K Smith, Leslie Myatt","doi":"10.1186/s43682-022-00010-0","DOIUrl":null,"url":null,"abstract":"Background: Advanced maternal age is currently a term defined by chronological age. However, a group of biomarkers known as epigenetic clocks, which can predict morbidity and mortality, has been used to estimate measures of biological aging. Uterine myometrial function during the process of parturition may be influenced by aging, as labor dystocia, unplanned intrapartum cesarean birth, and postpartum hemorrhage are more common in older individuals. The purpose of this study was to evaluate the use of epigenetic clocks in maternal myometrium and blood for predicting age and to evaluate the correlation of epigenetic age between the tissues.Results: We compared epigenetic age in blood and myometrial samples provided by women undergoing planned cesarean birth at term gestation. Chronological age ranged from 20 to 50 with a median (IQR) age of 35.5(8) years. The MethylationEPIC BeadChip was used to obtain DNA methylation data, and then epigenetic age was calculated using the Horvath, Hannum, GrimAge, and PhenoAge clocks. Spearman correlations of epigenetic age with chronological age were calculated. We tested the relationship of epigenetic age in maternal blood to epigenetic age in myometrium. Age acceleration, for each clock, was also correlated between tissues. Twenty-seven participants provided samples, and 21 matched specimens were included in the final analysis after quality control. Spearman correlation between maternal chronological age and epigenetic age were significant in three of the four clocks (pan-tissue Horvath, Hannum, and GrimAge), for both myometrium and blood samples. Correlations between blood epigenetic age and maternal age ranged from 0.72 to 0.87 (all p < 0.001). Correlations between myometrial epigenetic age and maternal age were also significant (0.62-0.70, p = 0.002), though lower than correlations seen in blood. Maternal blood epigenetic age also correlated with epigenetic age in myometrium with each of these three clocks 0.60 (p = 0.004, Horvath), 0.63 (p = 0.003, Hannum), and 0.80 (p < 0.001, GrimAge). GrimAge age acceleration had the highest correlation between tissues among the clocks (0.49, p = 0.02).Conclusions: Given the limited sample, this study provides insight into the potential use of epigenetic age derived from blood as a proxy for myometrial epigenetic age, which may be a useful biomarker in estimating myometrial biological age in relationship to myometrial dysfunction. GrimAge outperformed the other tested clocks in terms of concordance of epigenetic age and age acceleration between tissues; however, the Horvath and Hannum clocks may be useful depending on the outcome of interest in pregnancy.","PeriodicalId":72947,"journal":{"name":"Epigenetics communications","volume":" ","pages":""},"PeriodicalIF":0.0000,"publicationDate":"2022-01-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9432845/pdf/","citationCount":"2","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Epigenetics communications","FirstCategoryId":"1085","ListUrlMain":"https://doi.org/10.1186/s43682-022-00010-0","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"2022/5/23 0:00:00","PubModel":"Epub","JCR":"","JCRName":"","Score":null,"Total":0}

引用次数: 2

Abstract

Background: Advanced maternal age is currently a term defined by chronological age. However, a group of biomarkers known as epigenetic clocks, which can predict morbidity and mortality, has been used to estimate measures of biological aging. Uterine myometrial function during the process of parturition may be influenced by aging, as labor dystocia, unplanned intrapartum cesarean birth, and postpartum hemorrhage are more common in older individuals. The purpose of this study was to evaluate the use of epigenetic clocks in maternal myometrium and blood for predicting age and to evaluate the correlation of epigenetic age between the tissues.

Results: We compared epigenetic age in blood and myometrial samples provided by women undergoing planned cesarean birth at term gestation. Chronological age ranged from 20 to 50 with a median (IQR) age of 35.5(8) years. The MethylationEPIC BeadChip was used to obtain DNA methylation data, and then epigenetic age was calculated using the Horvath, Hannum, GrimAge, and PhenoAge clocks. Spearman correlations of epigenetic age with chronological age were calculated. We tested the relationship of epigenetic age in maternal blood to epigenetic age in myometrium. Age acceleration, for each clock, was also correlated between tissues. Twenty-seven participants provided samples, and 21 matched specimens were included in the final analysis after quality control. Spearman correlation between maternal chronological age and epigenetic age were significant in three of the four clocks (pan-tissue Horvath, Hannum, and GrimAge), for both myometrium and blood samples. Correlations between blood epigenetic age and maternal age ranged from 0.72 to 0.87 (all p < 0.001). Correlations between myometrial epigenetic age and maternal age were also significant (0.62-0.70, p = 0.002), though lower than correlations seen in blood. Maternal blood epigenetic age also correlated with epigenetic age in myometrium with each of these three clocks 0.60 (p = 0.004, Horvath), 0.63 (p = 0.003, Hannum), and 0.80 (p < 0.001, GrimAge). GrimAge age acceleration had the highest correlation between tissues among the clocks (0.49, p = 0.02).

Conclusions: Given the limited sample, this study provides insight into the potential use of epigenetic age derived from blood as a proxy for myometrial epigenetic age, which may be a useful biomarker in estimating myometrial biological age in relationship to myometrial dysfunction. GrimAge outperformed the other tested clocks in terms of concordance of epigenetic age and age acceleration between tissues; however, the Horvath and Hannum clocks may be useful depending on the outcome of interest in pregnancy.

Abstract Image

查看原文本刊更多论文

推进对母亲年龄的理解:与血液和子宫肌层的表观遗传时钟相关。

背景:高龄产妇目前是一个由实足年龄定义的术语。然而，一组被称为表观遗传时钟的生物标志物，可以预测发病率和死亡率，已被用于估计生物衰老的措施。分娩过程中子宫肌功能可能受到年龄的影响，如难产、意外产时剖宫产和产后出血在老年人中更为常见。本研究的目的是评估母体子宫肌层和血液中表观遗传时钟对预测年龄的作用，并评估两种组织之间表观遗传年龄的相关性。结果:我们比较了足月妊娠接受计划剖宫产的妇女提供的血液和子宫肌瘤样本的表观遗传年龄。实足年龄从20岁到50岁，中位(IQR)年龄为35.5(8)岁。使用MethylationEPIC BeadChip获得DNA甲基化数据，然后使用Horvath, Hannum, GrimAge和PhenoAge时钟计算表观遗传年龄。计算表观遗传年龄与实足年龄的Spearman相关性。我们检测了母体血液表观遗传年龄与子宫肌层表观遗传年龄的关系。每个时钟的年龄加速在组织之间也有相关性。27名参与者提供了样品，21份匹配的样品经质控后纳入最终分析。在子宫肌层和血液样本中，四种时钟(泛组织Horvath、Hannum和GrimAge)中的三种时钟中，母体实足年龄和表观遗传年龄之间的Spearman相关性都是显著的。血液表观遗传年龄与母亲年龄的相关性为0.72 ~ 0.87(均p < 0.001)。子宫内膜表观遗传年龄与母亲年龄之间的相关性也很显著(0.62-0.70,p = 0.002)，尽管低于血液中的相关性。母体血液表观遗传年龄也与肌层表观遗传年龄相关，三个时钟分别为0.60 (p = 0.004, Horvath)、0.63 (p = 0.003, Hannum)和0.80 (p < 0.001, GrimAge)。各时钟组织间的年龄加速相关性最高(0.49,p = 0.02)。结论:在样本有限的情况下，本研究为从血液中获得的表观遗传年龄作为子宫肌层表观遗传年龄的替代指标提供了潜在的见解，这可能是估计子宫肌层生物年龄与子宫肌层功能障碍之间关系的有用生物标志物。在表观遗传年龄和组织间年龄加速的一致性方面，GrimAge优于其他测试时钟;然而，霍瓦特和汉纳姆时钟可能有用，这取决于对怀孕的兴趣的结果。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文求助全文

来源期刊

Epigenetics communications

自引率

0.00%

发文量