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端粒DNA甲基化缺失揭示的端粒生物学新特征

Novel features of telomere biology revealed by the absence of telomeric DNA methylation.

作者信息

Vega-Vaquero Alejandro, Bonora Giancarlo, Morselli Marco, Vaquero-Sedas María I, Rubbi Liudmilla, Pellegrini Matteo, Vega-Palas Miguel A

机构信息

Technical Superior School of Informatics Engineering, University of Seville, 41080 Seville, Spain;

Department of Molecular, Cell and Developmental Biology, University of California, Los Angeles, California 90095, USA;

出版信息

Genome Res. 2016 Aug;26(8):1047-56. doi: 10.1101/gr.202465.115. Epub 2016 Jul 12.

Abstract

Cytosine methylation regulates the length and stability of telomeres, which can affect a wide variety of biological features, including cell differentiation, development, or illness. Although it is well established that subtelomeric regions are methylated, the presence of methylated cytosines at telomeres has remained controversial. Here, we have analyzed multiple bisulfite sequencing studies to address the methylation status of Arabidopsis thaliana telomeres. We found that the levels of estimated telomeric DNA methylation varied among studies. Interestingly, we estimated higher levels of telomeric DNA methylation in studies that produced C-rich telomeric strands with lower efficiency. However, these high methylation estimates arose due to experimental limitations of the bisulfite technique. We found a similar phenomenon for mitochondrial DNA: The levels of mitochondrial DNA methylation detected were higher in experiments with lower mitochondrial read production efficiencies. Based on experiments with high telomeric C-rich strand production efficiencies, we concluded that Arabidopsis telomeres are not methylated, which was confirmed by methylation-dependent restriction enzyme analyses. Thus, our studies indicate that telomeres are refractory to de novo DNA methylation by the RNA-directed DNA methylation machinery. This result, together with previously reported data, reveals that subtelomeric DNA methylation controls the homeostasis of telomere length.

摘要

胞嘧啶甲基化调节端粒的长度和稳定性,而这会影响多种生物学特征,包括细胞分化、发育或疾病。虽然已知亚端粒区域是甲基化的,但端粒处甲基化胞嘧啶的存在一直存在争议。在这里,我们分析了多个亚硫酸氢盐测序研究,以探讨拟南芥端粒的甲基化状态。我们发现,不同研究中端粒DNA甲基化的估计水平有所不同。有趣的是,我们发现在产生富含C的端粒链效率较低的研究中,端粒DNA甲基化的估计水平较高。然而,这些高甲基化估计是由于亚硫酸氢盐技术的实验局限性所致。我们在线粒体DNA中也发现了类似现象:在产生线粒体读数效率较低的实验中,检测到的线粒体DNA甲基化水平较高。基于产生富含C的端粒链效率较高的实验,我们得出结论,拟南芥端粒没有甲基化,这一结论通过甲基化依赖性限制酶分析得到了证实。因此,我们的研究表明,端粒对RNA介导的DNA甲基化机制的从头DNA甲基化具有抗性。这一结果与先前报道的数据一起表明,亚端粒DNA甲基化控制着端粒长度的稳态。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8072/4971770/f795216f2d20/1047f01.jpg

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