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DNA 甲基化对人肝和心肌组织 FCGRT 表达的贡献。

Contribution of DNA methylation to the expression of FCGRT in human liver and myocardium.

机构信息

Department of Pharmaceutical Sciences, School of Pharmacy and Pharmaceutical Sciences, The State University of New York at Buffalo, Buffalo, NY, 14214, USA.

Genomics and Bioinformatics Core, New York State Center of Excellence in Bioinformatics and Life Sciences, The State University of New York at Buffalo, Buffalo, NY, 14203, USA.

出版信息

Sci Rep. 2019 Jun 17;9(1):8674. doi: 10.1038/s41598-019-45203-1.

Abstract

FcRn mediates recycling and transcytosis of IgG and albumin in various cell types. The MHC-class-I-like protein of the FcRn heterodimer is encoded by FCGRT. Few determinants of variable FCGRT expression in humans have been identified so far. In this study, we investigated the presence of DNA methylation in regulatory regions of FCGRT in samples of human liver and myocardium tissue, and we examined the impact of FCGRT methylation on FcRn expression in model cell lines. Quantitative DNA methylation analysis of the FCGRT locus revealed differentially methylated regions in DNA from liver and myocardium. Methylation status in individual CpG sites correlated with FCGRT mRNA expression. Data from model cell lines suggest that differential methylation in the -1058 to -587 bp regulatory region of FCGRT contributes to FcRn expression. Chromatin immunoprecipitation assays indicate that CpG site methylation impacts the binding of the methylation sensitive transcription factors Zbtb7a and Sp1. This study provides a foundation to further define the contribution of epigenetic factors during the control of FcRn expression and IgG traffic in human tissues.

摘要

FcRn 介导 IgG 和白蛋白在各种细胞类型中的循环和转胞吞作用。FcRn 异二聚体的 MHC 类 I 样蛋白由 FCGRT 编码。迄今为止,已经确定了人类 FCGRT 表达的少数可变决定簇。在这项研究中,我们研究了人肝和心肌组织样本中 FCGRT 调节区的 DNA 甲基化的存在,并检查了 FCGRT 甲基化对模型细胞系中 FcRn 表达的影响。FCGRT 基因座的定量 DNA 甲基化分析显示,肝和心肌中的 DNA 存在差异甲基化区域。单个 CpG 位点的甲基化状态与 FCGRT mRNA 表达相关。来自模型细胞系的数据表明,FCGRT-1058 至-587 bp 调控区的差异甲基化有助于 FcRn 表达。染色质免疫沉淀分析表明,CpG 位点的甲基化影响了甲基化敏感转录因子 Zbtb7a 和 Sp1 的结合。这项研究为进一步确定在人类组织中控制 FcRn 表达和 IgG 转运过程中表观遗传因素的贡献提供了基础。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f847/6572836/6aa8315a30ef/41598_2019_45203_Fig1_HTML.jpg

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