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干燥综合征患者长期培养的小唾液腺上皮细胞中细胞特异性全基因组 DNA 甲基化图谱。

Cell-specific epigenome-wide DNA methylation profile in long-term cultured minor salivary gland epithelial cells from patients with Sjögren's syndrome.

机构信息

INSERM U1227 B lymphocytes and autoimmunity, Labex IGO, Réseau épigénétique et réseau canaux ioniques du cancéropole Grand Ouest, Université de Brest, Brest, France.

Department of Pathophysiology, School of Medicine, National University of Athens, Athens, Greece.

出版信息

Ann Rheum Dis. 2017 Mar;76(3):625-628. doi: 10.1136/annrheumdis-2016-210167. Epub 2017 Jan 16.

DOI:10.1136/annrheumdis-2016-210167
PMID:28093418
Abstract

OBJECTIVES

The aetiology of primary Sjögren's syndrome (pSS), also referred to as autoimmune epithelitis, is incompletely understood but includes an epigenetic contribution. Accordingly, the aim of this study was to investigate DNA methylation in salivary gland epithelial cells (SGEC), and to compare results with those publicly available from pSS B and T cells.

METHODS

Long-term cultured SGEC were selected to conduct an epigenome-wide association study (EWAS) in patients with pSS with comparison to controls using the HumanMethylation 450 K array from Illumina.

RESULTS

The analysis of differentially methylated CpG (DMC) uncovered 4662 positions corresponding to 2560 genes, and 575 genes with two or more DMC sites (DMCs), in SGEC as compared with controls. Further analysis highlighted an important proportion of interferon-regulated genes (61%), the calcium pathway (hypomethylated) and the Wnt pathway (hypermethylated). When comparing SGEC with pSS T and/or B cell results, an important overlap was observed with respect to differentially methylated genes (38.8%) and pSS risk factors (71.4%), although such assertion was not true when comparing DMCs.

CONCLUSIONS

This study conducted in SGEC emphasises the role of DNA methylation in pSS pathogenesis and supports the necessity to conduct pure cell analysis for future EWAS studies when analysing salivary glands from patients with pSS.

摘要

目的

原发性干燥综合征(pSS),也称为自身免疫性上皮炎,其病因不完全清楚,但包括表观遗传因素。因此,本研究旨在研究唾液腺上皮细胞(SGEC)中的 DNA 甲基化,并将结果与 pSS B 和 T 细胞的公开数据进行比较。

方法

选择长期培养的 SGEC 进行全基因组甲基化关联研究(EWAS),使用 Illumina 的 HumanMethylation 450 K 阵列,将 pSS 患者与对照进行比较。

结果

与对照组相比,分析差异甲基化 CpG(DMC)发现了 4662 个位置,对应 2560 个基因,以及 575 个有两个或更多 DMC 位点(DMCs)的基因。进一步的分析强调了干扰素调节基因(61%)、钙途径(低甲基化)和 Wnt 途径(高甲基化)的重要比例。当将 SGEC 与 pSS T 和/或 B 细胞的结果进行比较时,在差异甲基化基因(38.8%)和 pSS 风险因素(71.4%)方面观察到重要的重叠,尽管在比较 DMC 时并非如此。

结论

这项在 SGEC 中进行的研究强调了 DNA 甲基化在 pSS 发病机制中的作用,并支持在分析 pSS 患者的唾液腺时,为未来的 EWAS 研究进行纯细胞分析的必要性。

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