Department of Biochemistry, University of Otago, Dunedin, 9016, New Zealand.
Department of Pathology, University of Otago, Dunedin, 9016, New Zealand.
Clin Epigenetics. 2020 Nov 4;12(1):167. doi: 10.1186/s13148-020-00960-z.
Myalgic Encephalomyelitis/Chronic Fatigue Syndrome (ME/CFS) is a lifelong debilitating disease with a complex pathology not yet clearly defined. Susceptibility to ME/CFS involves genetic predisposition and exposure to environmental factors, suggesting an epigenetic association. Epigenetic studies with other ME/CFS cohorts have used array-based technology to identify differentially methylated individual sites. Changes in RNA quantities and protein abundance have been documented in our previous investigations with the same ME/CFS cohort used for this study.
DNA from a well-characterised New Zealand cohort of 10 ME/CFS patients and 10 age-/sex-matched healthy controls was isolated from peripheral blood mononuclear (PBMC) cells, and used to generate reduced genome-scale DNA methylation maps using reduced representation bisulphite sequencing (RRBS). The sequencing data were analysed utilising the DMAP analysis pipeline to identify differentially methylated fragments, and the MethylKit pipeline was used to quantify methylation differences at individual CpG sites. DMAP identified 76 differentially methylated fragments and Methylkit identified 394 differentially methylated cytosines that included both hyper- and hypo-methylation. Four clusters were identified where differentially methylated DNA fragments overlapped with or were within close proximity to multiple differentially methylated individual cytosines. These clusters identified regulatory regions for 17 protein encoding genes related to metabolic and immune activity. Analysis of differentially methylated gene bodies (exons/introns) identified 122 unique genes. Comparison with other studies on PBMCs from ME/CFS patients and controls with array technology showed 59% of the genes identified in this study were also found in one or more of these studies. Functional pathway enrichment analysis identified 30 associated pathways. These included immune, metabolic and neurological-related functions differentially regulated in ME/CFS patients compared to the matched healthy controls.
Major differences were identified in the DNA methylation patterns of ME/CFS patients that clearly distinguished them from the healthy controls. Over half found in gene bodies with RRBS in this study had been identified in other ME/CFS studies using the same cells but with array technology. Within the enriched functional immune, metabolic and neurological pathways, a number of enriched neurotransmitter and neuropeptide reactome pathways highlighted a disturbed neurological pathophysiology within the patient group.
肌痛性脑脊髓炎/慢性疲劳综合征(ME/CFS)是一种终身致残性疾病,其复杂的病理尚未明确界定。ME/CFS 的易感性涉及遗传易感性和环境因素暴露,表明存在表观遗传关联。其他 ME/CFS 队列的表观遗传学研究使用基于阵列的技术来识别差异甲基化的个体位点。在我们之前使用相同 ME/CFS 队列的研究中,已经记录了 RNA 数量和蛋白质丰度的变化。
从新西兰一个经过充分特征描述的 10 名 ME/CFS 患者和 10 名年龄/性别匹配的健康对照者的外周血单核细胞(PBMC)中分离出 DNA,并使用基于减少代表性亚硫酸氢盐测序(RRBS)的方法生成全基因组规模的 DNA 甲基化图谱。使用 DMAP 分析管道分析测序数据以识别差异甲基化片段,并使用 MethylKit 管道在单个 CpG 位点量化甲基化差异。DMAP 鉴定了 76 个差异甲基化片段,Methylkit 鉴定了 394 个差异甲基化胞嘧啶,包括高甲基化和低甲基化。确定了四个簇,其中差异甲基化 DNA 片段与多个差异甲基化单个胞嘧啶重叠或紧密相邻。这些簇确定了与代谢和免疫活性相关的 17 个蛋白质编码基因的调节区域。对差异甲基化基因体(外显子/内含子)的分析确定了 122 个独特的基因。与使用阵列技术的 ME/CFS 患者和对照者的 PBMC 进行的其他研究进行比较,发现本研究中鉴定的 122 个基因中有 59%也存在于一个或多个这些研究中。功能途径富集分析确定了 30 个相关途径。这些途径包括免疫、代谢和神经相关功能,ME/CFS 患者与匹配的健康对照者相比这些功能受到不同程度的调节。
ME/CFS 患者的 DNA 甲基化模式存在明显差异,可将其与健康对照者明确区分开来。RRBS 中发现的超过一半的基因在使用相同细胞但使用阵列技术的其他 ME/CFS 研究中已经被发现。在富集的免疫、代谢和神经功能途径中,一些富集的神经递质和神经肽反应途径突出了患者组中神经病理生理学的紊乱。
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