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Genome-scale profiling reveals a subset of genes regulated by DNA methylation that program somatic T-cell phenotypes in humans

机译:基因组规模的分析揭示了受DNA甲基化调节的基因子集,可对人类的体细胞T细胞表型进行编程

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摘要

The aim of this study was to investigate the dynamics and relationship between DNA methylation and gene expression during early T-cell development. Mononuclear cells were collected at birth and at 12 months from 60 infants and were either activated with anti-CD3 for 24 h or cultured in media alone, and the CD4+ T-cell subset purified. DNA and RNA were co-harvested and DNA methylation was measured in 450 000 CpG sites in parallel with expression measurements taken from 25 000 genes. In unstimulated cells, we found that a subset of 1188 differentially methylated loci were associated with a change in expression in 599 genes (adjusted P value<0.01, Β-fold >0.1). These genes were enriched in reprogramming regions of the genome known to control pluripotency. In contrast, over 630 genes were induced following low-level T-cell activation, but this was not associated with any significant change in DNA methylation. We conclude that DNA methylation is dynamic during early T-cell development, and has a role in the consolidation of T-cell-specific gene expression. During the early phase of clonal expansion, DNA methylation is stable and therefore appears to be of limited importance in short-term T-cell responsiveness.
机译:这项研究的目的是调查早期T细胞发育过程中DNA甲基化与基因表达之间的动力学关系。在出生时和第12个月从60名婴儿中收集单核细胞,并用抗CD3激活24小时或单独在培养基中培养,然后纯化CD4 + T细胞亚群。共收获DNA和RNA,并在450 000 CpG位点测量DNA甲基化,同时从25 000个基因进行表达测量。在未刺激的细胞中,我们发现1188个差异甲基化基因座的一个子集与599个基因中的表达变化相关(调整后的P值<0.01,β倍> 0.1)。这些基因富集在已知可控制多能性的基因组重编程区域中。相反,在低水平的T细胞活化后,诱导了630个以上的基因,但这与DNA甲基化的任何显着变化无关。我们得出结论,DNA甲基化在早期T细胞发育过程中是动态的,并在整合T细胞特异性基因表达中发挥作用。在克隆扩增的早期阶段,DNA甲基化是稳定的,因此在短期T细胞反应性中的重要性似乎有限。

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