人脂肪形成过程中的DNA甲基化和果糖的影响。

Giulia Tini, Vijayalakshmi Varma, Rosario Lombardo, Greg T Nolen, Gregory Lefebvre, Patrick Descombes, Sylviane Métairon, Corrado Priami, Jim Kaput, Marie-Pier Scott-Boyer
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引用次数: 5

摘要

背景:脂肪生成的增加和脂肪细胞功能的改变有助于肥胖和相关合并症的发展。与葡萄糖相比,果糖改变了脂肪细胞的代谢,但其对肥胖的调节机制和后果尚不清楚。在诱导脂肪形成后的0、24、48、96、192和384小时,研究人员分析了暴露于0、2.5、5和10 mM果糖的SGBS前脂肪细胞的全基因组甲基化和全球转录组学。结果:与基线(0小时)相比,DNA甲基化的时间依赖性变化发生在脂肪细胞最终成熟的192至384小时之间。与在果糖补充培养基中分化的脂肪细胞相比,在含葡萄糖的对照培养基中分化的脂肪细胞中差异甲基化区(DMRs)的百分比更高(192 h时为0.1%,384 h时为3.2%)(10 mM时为0.0006%,5 mM时为0.001%,2.5 mM时为0.005%,384 h)。5237个差异表达基因在含葡萄糖(5 mM)对照培养基中诱导384 h后共鉴定出1437个DMRs。大部分区域与基因表达呈负相关,666个区域与基因表达呈正相关。结论:我们的研究表明,DNA甲基化在全基因组范围内调节或标志着形态分化的脂肪细胞(192小时)向更成熟和代谢更旺盛的脂肪细胞(384小时)的转变。与较高浓度(5和10毫米)相比,较低浓度(2.5毫米)的果糖对甲基化的影响最为显著,这表明果糖可能在较低浓度下发挥信号/调节作用,而在较高浓度下作为底物发挥作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

DNA methylation during human adipogenesis and the impact of fructose.

DNA methylation during human adipogenesis and the impact of fructose.

DNA methylation during human adipogenesis and the impact of fructose.

DNA methylation during human adipogenesis and the impact of fructose.

Background: Increased adipogenesis and altered adipocyte function contribute to the development of obesity and associated comorbidities. Fructose modified adipocyte metabolism compared to glucose, but the regulatory mechanisms and consequences for obesity are unknown. Genome-wide methylation and global transcriptomics in SGBS pre-adipocytes exposed to 0, 2.5, 5, and 10 mM fructose, added to a 5-mM glucose-containing medium, were analyzed at 0, 24, 48, 96, 192, and 384 h following the induction of adipogenesis.

Results: Time-dependent changes in DNA methylation compared to baseline (0 h) occurred during the final maturation of adipocytes, between 192 and 384 h. Larger percentages (0.1% at 192 h, 3.2% at 384 h) of differentially methylated regions (DMRs) were found in adipocytes differentiated in the glucose-containing control media compared to adipocytes differentiated in fructose-supplemented media (0.0006% for 10 mM, 0.001% for 5 mM, and 0.005% for 2.5 mM at 384 h). A total of 1437 DMRs were identified in 5237 differentially expressed genes at 384 h post-induction in glucose-containing (5 mM) control media. The majority of them inversely correlated with the gene expression, but 666 regions were positively correlated to the gene expression.

Conclusions: Our studies demonstrate that DNA methylation regulates or marks the transformation of morphologically differentiating adipocytes (seen at 192 h), to the more mature and metabolically robust adipocytes (as seen at 384 h) in a genome-wide manner. Lower (2.5 mM) concentrations of fructose have the most robust effects on methylation compared to higher concentrations (5 and 10 mM), suggesting that fructose may be playing a signaling/regulatory role at lower concentrations of fructose and as a substrate at higher concentrations.

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