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RUNX2-P1和Sp7基因启动子处的表观遗传特征控制脐带间充质干细胞的成骨谱系定向分化。

Epigenetic Signatures at the RUNX2-P1 and Sp7 Gene Promoters Control Osteogenic Lineage Commitment of Umbilical Cord-Derived Mesenchymal Stem Cells.

作者信息

Sepulveda Hugo, Aguilar Rodrigo, Prieto Catalina P, Bustos Francisco, Aedo Sócrates, Lattus José, van Zundert Brigitte, Palma Veronica, Montecino Martin

机构信息

Center for Biomedical Research, Universidad Andres Bello, Santiago, Chile.

FONDAP Center for Genome Regulation, Santiago, Chile.

出版信息

J Cell Physiol. 2017 Sep;232(9):2519-2527. doi: 10.1002/jcp.25627. Epub 2017 Mar 28.

DOI:10.1002/jcp.25627
PMID:27689934
Abstract

Wharton's Jelly mesenchymal stem cells (WJ-MSCs) are an attractive potential source of multipotent stem cells for bone tissue replacement therapies. However, the molecular mechanisms involved in their osteogenic conversion are poorly understood. Particularly, epigenetic control operating at the promoter regions of the two master regulators of the osteogenic program, RUNX2/P57 and SP7 has not yet been described in WJ-MSCs. Via quantitative PCR profiling and chromatin immunoprecipitation (ChIP) studies, here we analyze the ability of WJ-MSCs to engage osteoblast lineage. In undifferentiated WJ-MSCs, RUNX2/P57 P1, and SP7 promoters are found deprived of significant levels of the histone post-translational marks that are normally associated with transcriptionally active genes (H3ac, H3K27ac, and H3K4me3). Moreover, the RUNX2 P1 promoter lacks two relevant histone repressive marks (H3K9me3 and H3K27me3). Importantly, RUNX2 P1 promoter is found highly enriched in the H3K4me1 mark, which has been shown recently to mediate gene repression of key regulatory genes. Upon induction of WJ-MSCs osteogenic differentiation, we found that RUNX2/P57, but not SP7 gene expression is strongly activated, in a process that is accompanied by enrichment of activating histone marks (H3K4me3, H3ac, and H3K27ac) at the P1 promoter region. Histone mark analysis showed that SP7 gene promoter is robustly enriched in epigenetic repressive marks that may explain its poor transcriptional response to osteoblast differentiating media. Together, these results point to critical regulatory steps during epigenetic control of WJ-MSCs osteogenic lineage commitment that are relevant for future applications in regenerative medicine. J. Cell. Physiol. 232: 2519-2527, 2017. © 2016 Wiley Periodicals, Inc.

摘要

沃顿胶间充质干细胞(WJ-MSCs)是骨组织替代疗法中多能干细胞的一个有吸引力的潜在来源。然而,其成骨转化所涉及的分子机制仍知之甚少。特别是,在WJ-MSCs中,尚未描述在成骨程序的两个主要调节因子RUNX2/P57和SP7的启动子区域进行的表观遗传控制。通过定量PCR分析和染色质免疫沉淀(ChIP)研究,我们在此分析了WJ-MSCs参与成骨细胞谱系的能力。在未分化的WJ-MSCs中,发现RUNX2/P57 P1和SP7启动子缺乏与转录活性基因(H3ac、H3K27ac和H3K4me3)正常相关的显著水平的组蛋白翻译后修饰。此外,RUNX2 P1启动子缺乏两个相关的组蛋白抑制标记(H3K9me3和H3K27me3)。重要的是,发现RUNX2 P1启动子高度富集H3K4me1标记,最近已证明该标记介导关键调节基因的基因抑制。在诱导WJ-MSCs成骨分化后,我们发现RUNX2/P57基因表达被强烈激活,但SP7基因表达未被激活,在这个过程中,P1启动子区域伴随着激活组蛋白标记(H3K4me3、H3ac和H3K27ac)的富集。组蛋白标记分析表明,SP7基因启动子强烈富集表观遗传抑制标记,这可能解释了其对成骨细胞分化培养基的转录反应较差。总之,这些结果指出了WJ-MSCs成骨谱系定向的表观遗传控制过程中的关键调节步骤,这对于再生医学的未来应用具有重要意义。《细胞生理学杂志》232: 2519 - 2527, 2017。© 2016威利期刊公司

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