Transcriptomics of receptive endometrium in women with sonographic features of adenomyosis

Erika Prašnikar; Tanja Kunej; Mario Gorenjak; Uroš Potočnik; Borut Kovačič; Jure Knez

doi:10.1186/s12958-021-00871-5

Reproductive Biology and Endocrinology (Jan 2022)

Transcriptomics of receptive endometrium in women with sonographic features of adenomyosis

Erika Prašnikar,
Tanja Kunej,
Mario Gorenjak,
Uroš Potočnik,
Borut Kovačič,
Jure Knez

Affiliations

Erika Prašnikar: Department of Reproductive Medicine and Gynaecological Endocrinology, University Medical Centre Maribor
Tanja Kunej: Department of Animal Science, Biotechnical Faculty, University of Ljubljana
Mario Gorenjak: Centre for Human Molecular Genetics and Pharmacogenomics, Faculty of Medicine, University of Maribor
Uroš Potočnik: Centre for Human Molecular Genetics and Pharmacogenomics, Faculty of Medicine, University of Maribor
Borut Kovačič: Department of Reproductive Medicine and Gynaecological Endocrinology, University Medical Centre Maribor
Jure Knez: Department of Gynaecology, University Medical Centre Maribor

DOI: https://doi.org/10.1186/s12958-021-00871-5
Journal volume & issue: Vol. 20, no. 1
pp. 1 – 16

Abstract

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Abstract Background Women with uterine adenomyosis seeking assisted reproduction have been associated with compromised endometrial receptivity to embryo implantation. To understand the mechanisms involved in this process, we aimed to compare endometrial transcriptome profiles during the window of implantation (WOI) between women with and without adenomyosis. Methods We obtained endometrial biopsies LH-timed to the WOI from women with sonographic features of adenomyosis (n=10) and controls (n=10). Isolated RNA samples were subjected to RNA sequencing (RNA-seq) by the Illumina NovaSeq 6000 platform and endometrial receptivity classification with a molecular tool for menstrual cycle phase dating (beREADY®, CCHT). The program language R and Bioconductor packages were applied to analyse RNA-seq data in the setting of the result of accurate endometrial dating. To suggest robust candidate pathways, the identified differentially expressed genes (DEGs) associated with the adenomyosis group in the receptive phase were further integrated with 151, 173 and 42 extracted genes from published studies that were related to endometrial receptivity in healthy uterus, endometriosis and adenomyosis, respectively. Enrichment analyses were performed using Cytoscape ClueGO and CluePedia apps. Results Out of 20 endometrial samples, 2 were dated to the early receptive phase, 13 to the receptive phase and 5 to the late receptive phase. Comparison of the transcriptomics data from all 20 samples provided 909 DEGs (p<0.05; nonsignificant after adjusted p value) in the adenomyosis group but only 4 enriched pathways (Bonferroni p value < 0.05). The analysis of 13 samples only dated to the receptive phase provided suggestive 382 DEGs (p<0.05; nonsignificant after adjusted p value) in the adenomyosis group, leading to 33 enriched pathways (Bonferroni p value < 0.05). These included pathways were already associated with endometrial biology, such as “Expression of interferon (IFN)-induced genes” and “Response to IFN-alpha”. Data integration revealed pathways indicating a unique effect of adenomyosis on endometrial molecular organization (e.g., “Expression of IFN-induced genes”) and its interference with endometrial receptivity establishment (e.g., “Extracellular matrix organization” and “Tumour necrosis factor production”). Conclusions Accurate endometrial dating and RNA-seq analysis resulted in the identification of altered response to IFN signalling as the most promising candidate of impaired uterine receptivity in adenomyosis.

Published in Reproductive Biology and Endocrinology

ISSN: 1477-7827 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Gynecology and obstetrics; Science: Biology (General): Reproduction
Website: https://rbej.biomedcentral.com/

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