Abstract
Despite an abundance of studies on chromatin states and dynamics, there is an astonishing dearth of information on the expression of genes responsible for regulating histone and DNA modifications. We used here a set of 156 defined epigenetic modifier genes (EMG) and profiled their expression pattern in cells of different lineages. As reference value, expression data from human embryonic stem cells (hESC) were used. Hepatocyte-like cells were generated from hESC, and their EMG expression was compared to primary human liver cells. In parallel, we generated postmitotic human neurons (Lu d6), and compared their relative EMG expression to human cortex (Ctx). Clustering analysis of all cell types showed that neuronal lineage samples grouped together (94 similarly regulated EMG), as did liver cells (61 similarly-regulated), while the two lineages were clearly distinct. The general classification was followed by detailed comparison of the major EMG groups; genes that were higher expressed in differentiated cells than in hESC included the acetyltransferase KAT2B and the methyltransferase SETD7. Neuro-specific EMGs were the histone deacetylases HDAC5 and HDAC7, and the arginine-methyltransferase PRMT8. Comparison of young (Lu d6) and more aged (Ctx) neuronal samples suggested a maturation-dependent switch in the expression of functionally homologous proteins. For instance, the ratio of the histone H3 K27 methyltransfereases, EZH1 to EZH2, was high in Ctx and low in Lu d6. The same was observed for the polycomb repressive complex 1 (PRC1) subunits CBX7 and CBX8. A large proportion of EMGs in differentiated cells was very differently expressed than in hESC, and absolute levels were significantly higher in neuronal samples than in hepatic cells. Thus, there seem to be distinct qualitative and quantitative differences in EMG expression between cell lineages.
Highlights
Epigenetic modifier genes (EMG) encode the proteins that organize and maintain the chromatin structure of cells
Immunofluorescence staining of human hepatocytes (huHep) showed a ubiquitous expression of the two hepatic markers albumin (ALB) and dipeptidyl-peptidase 4 (DPP4) (Fig. 1B)
Because TET1 was already highly expressed in human embryonic stem cells (hESC) (Ct = 23) there was no significant upregulation visible compared to Ctx
Summary
Epigenetic modifier genes (EMG) encode the proteins that organize and maintain the chromatin structure of cells. They play a key role in the regulation of transcription and they ensure lineage fidelity by controlling the accessibility of DNA in the cell. Other cell identifier genes are upregulated during the cellular maturation phase Such waves of transcriptional changes are found in differentiating embryonic stem cells (ESC) [1]. They are guided and controlled by chromatin structure, which regulates the accessibility of the underlying DNA to sequencespecific regulator proteins such as transcription factors (TFs) or the transcriptional initiation complex [2]. The two classical, simplified variants of chromatin are transcriptionally active ‘‘open’’ euchromatin that allows TF binding and silenced ‘‘closed’’ heterochromatin that prevents binding of TFs to the corresponding DNA sequences [3]
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