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Differences among brain tumor stem cell types and fetal neural stem cells in focal regions of histone modifications and DNA methylation, broad regions of modifications, and bivalent promoters

BMC Genomics (2014) 15(1)
DOI: 10.1186/1471-2164-15-724
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Abstract

Background: Aberrational epigenetic marks are believed to play a major role in establishing the abnormal features of cancer cells. Rational use and development of drugs aimed at epigenetic processes requires an understanding of the range, extent, and roles of epigenetic reprogramming in cancer cells. Using ChIP-chip and MeDIP-chip approaches, we localized well-established and prevalent epigenetic marks (H3K27me3, H3K4me3, H3K9me3, DNA methylation) on a genome scale in several lines of putative glioma stem cells (brain tumor stem cells, BTSCs) and, for comparison, normal human fetal neural stem cells (fNSCs).Results: We determined a substantial "core" set of promoters possessing each mark in every surveyed BTSC cell type, which largely overlapped the corresponding fNSC sets. However, there was substantial diversity among cell types in mark localization. We observed large differences among cell types in total number of H3K9me3+ positive promoters and peaks and in broad modifications (defined as >50 kb peak length) for H3K27me3 and, to a lesser extent, H3K9me3. We verified that a change in a broad modification affected gene expression of CACNG7. We detected large numbers of bivalent promoters, but most bivalent promoters did not display direct overlap of contrasting epigenetic marks, but rather occupied nearby regions of the proximal promoter. There were significant differences in the sets of promoters bearing bivalent marks in the different cell types and few consistent differences between fNSCs and BTSCs.Conclusions: Overall, our "core set" data establishes sets of potential therapeutic targets, but the diversity in sets of sites and broad modifications among cell types underscores the need to carefully consider BTSC subtype variation in epigenetic therapy. Our results point toward substantial differences among cell types in the activity of the production/maintenance systems for H3K9me3 and for broad regions of modification (H3K27me3 or H3K9me3). Finally, the unexpected diversity in bivalent promoter sets among these multipotent cells indicates that bivalent promoters may play complex roles in the overall biology of these cells. These results provide key information for forming the basis for future rational drug therapy aimed at epigenetic processes in these cells.

Figures

  • Figure 1 Number of peaks and peak-containing promoters for each c epigenetic mark per cell type. This analysis used generous parameters lead promoters possessing each epigenetic mark. Peaks were mapped to proxim promoter, the promoter was scored as positive (see RESULTS and METHOD H3K9me3+ promoters.
  • Figure 2 Universe of promoters that possess each epigenetic mark. A. Examples of each epigenetic mark for a single promoter from each BTSC type. Note great similarity in waveforms across cell types for a given epigenetic mark. Left axis is log2 enrichment ratio. For genomic location (top axis), only single coordinate is shown; genomic distance between tick marks is (panels from left to right): 1 kb, 6 kb, 4 kb, 8 kb. All displayed transcripts extend beyond edge of figure area. B. Diagram of number of promoters that possess a given epigenetic mark in at least one type of BTSC (“universe” set; number in parentheses) and the number that possess it in every BTSC type (“core” set). Number in core set: H3K4me3: 6742; H3K9me3: 1650; H3K27me3: 3198; meC: 5360. See RESULTS and METHODS for details of computation of sets.
  • Figure 3 Comparison of fNSCs and BTSCs. Human fetal neural stem cells were used as model for the normal precursor cells for BTSCs. A. (left) Example of gain of H3K4me3 mark in a promoter in all four BTSC lines, as compared to fNSCs. (right) Example of loss of H3K27me3 mark in all four BTSC lines, as compared to fNSCs. Left axis is log2 enrichment ratio. All displayed transcripts extend beyond edge of figure area. B. Explication of comparison of fNSC promoter sets to BTSC promoter sets by epigenetic mark. “Universe” and “core” sets as in Figure 2. fNSC is left circle in each case. Critical computations in diagram are indicated in bold, italic, underlined font. C. Results of comparison of fNSC and universe or core BTSC sets for each epigenetic mark.
  • Figure 4 Examples of variation among cell types in the extent of bro Note the large differences between B73 and B12 in particular. Left axis is lo indicates differential region, which encompasses transcription start site for Note particularly large difference between B73 and fNSC. Markings for “Tran the + strand (i.e. TSS (transcription start site) on left side of box), while boxe strand (i.e. TSS is on right of box).
  • Figure 5 Differential presence of a broad region of H3K9me3 affects region of H3K9me3 that is missing in other cell types (large arrow). Small a this CACNG7 region reveals H3K9me3 presence in B73 cells but not B12 cel C. Quantitative PCR of mRNA abundance (cDNA) demonstrates that B12 ce (mean + standard deviation) are expressed as fraction of the GAPDH level; using ACTB as a control (see RESULTS).
  • Figure 6 Bivalent Promoters in fNSCs and BTSCs. A. H3K4me3+/H3K27me3+ promoter in fNSCs and B73 cells. Note that both marks are in the proximal promoter but show little overlap. This was the most common pattern. Left axes are log2 enrichment ratio. B. Two patterns for H3K4me3 +/H3K9me3+ promoters (B12 cells). (left) Non-overlapping marks in proximal promoter. This is the most common pattern. (right) Overlapping marks. Left axes are log2 enrichment ratio. C. (left) H3K4me3+/H3K27me3+ promoter counts in each cell line and the number shared with fNSCs. (right) H3K4me3+/H3K9me3+ promoters in each cell line and number shared with fNSCs. ALL refers to bivalent promoters found in all 5 cell types. LOST refers to promoters that are bivalent in fNSCs and lack both marks in every BTSC line. D. Examples of fNSC H3K4me3+/H3K27me3+ promoters that resolve to either H3K27me3+ (left) or H3K4me3+ (right) promoters in the B73 line. Left axes are log2 enrichment ratio. Markings: For A, B, and D, transcripts are shown with arrows and line drawing. All displayed transcripts extend beyond edges of panel in figure. Markings for top axes (genomic coordinate of first tick mark (increment to next tick mark)): A: chr17:33,063,000 (3 kb); B: left: chr3:114,711,000 (1 kb); right: chr19:62,812,000 (1 kb); D: left: chr9:23,790,000 (6 kb); right: chr9:68,541,000 (3 kb).

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Yoo, S., & Bieda, M. C. (2014). Differences among brain tumor stem cell types and fetal neural stem cells in focal regions of histone modifications and DNA methylation, broad regions of modifications, and bivalent promoters. BMC Genomics, 15(1). https://doi.org/10.1186/1471-2164-15-724

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