H3K27 acetylation and gene expression analysis reveals differences in placental chromatin activity in fetal growth restriction

N D Paauw; A T Lely; J A Joles; A Franx; P G Nikkels; M Mokry; B B van Rijn

doi:10.1186/s13148-018-0508-x

H3K27 acetylation and gene expression analysis reveals differences in placental chromatin activity in fetal growth restriction

Clin Epigenetics. 2018 Jun 26:10:85. doi: 10.1186/s13148-018-0508-x. eCollection 2018.

Authors

N D Paauw^{1

2}, A T Lely¹, J A Joles³, A Franx¹, P G Nikkels⁴, M Mokry⁵, B B van Rijn^{1

6

2}

Affiliations

¹ 1Department of Obstetrics, Wilhelmina Children's Hospital Birth Center, University Medical Center Utrecht, Utrecht, the Netherlands.
² 6Division Woman and Baby, University Medical Center Utrecht, Postbus 85090, 3508 AB Utrecht, the Netherlands.
³ 2Department of Nephrology and Hypertension, University Medical Center Utrecht, Utrecht, the Netherlands.
⁴ 3Department of Pathology, University Medical Center Utrecht, Utrecht, the Netherlands.
⁵ 4Division of Pediatrics, University Medical Center Utrecht, Utrecht, the Netherlands.
⁶ 5Academic Unit of Human Development and Health, University of Southampton, Southampton, UK.

Abstract

Background: Posttranslational modification of histone tails such as histone 3 lysine 27 acetylation (H3K27ac) is tightly coupled to epigenetic regulation of gene expression. To explore whether this is involved in placenta pathology, we probed genome-wide H3K27ac occupancy by chromatin immunoprecipitation sequencing (ChIP-seq) in healthy placentas and placentas from pathological pregnancies with fetal growth restriction (FGR). Furthermore, we related specific acetylation profiles of FGR placentas to gene expression changes.

Results: Analysis of H3K27ac occupancy in FGR compared to healthy placentas showed 970 differentially acetylated regions distributed throughout the genome. Principal component analysis and hierarchical clustering revealed complete segregation of the FGR and control group. Next, we identified 569 upregulated genes and 521 downregulated genes in FGR placentas by RNA sequencing. Differential gene transcription largely corresponded to expected direction based on H3K27ac status. Pathway analysis on upregulated transcripts originating from hyperacetylated sites revealed genes related to the HIF-1-alpha transcription factor network and several other genes with known involvement in placental pathology (LEP, FLT1, HK2, ENG, FOS). Downregulated transcripts in the vicinity of hypoacetylated sites were related to the immune system and growth hormone receptor signaling. Additionally, we found enrichment of 141 transcription factor binding motifs within differentially acetylated regions. Of the corresponding transcription factors, four were upregulated, SP1, ARNT2, HEY2, and VDR, and two downregulated, FOSL and NR4A1.

Conclusion: We demonstrate a key role for genome-wide alterations in H3K27ac in FGR placentas corresponding with changes in transcription profiles of regions relevant to placental function. Future studies on the role of H3K27ac in FGR and placental-fetal development may help to identify novel targets for therapy of this currently incurable disease.

Keywords: ChIP-seq; Epigenetics; Growth restriction; H3K27ac; Histone acetylation; Placenta; Placental pathology; RNA-seq.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Acetylation
Chromatin Immunoprecipitation / methods
Epigenesis, Genetic
Female
Fetal Development
Fetal Growth Retardation / genetics*
Histones / metabolism*
Humans
Hypoxia-Inducible Factor 1, alpha Subunit / metabolism
Placenta / metabolism*
Pregnancy
Protein Processing, Post-Translational
Receptors, Somatotropin / metabolism
Sequence Analysis, RNA
Transcription Factors

Substances

HIF1A protein, human
Histones
Hypoxia-Inducible Factor 1, alpha Subunit
Receptors, Somatotropin
Transcription Factors