AI Article Synopsis

  • The study aims to investigate the unknown causes of endometriosis by analyzing different cell types individually from both endometriomas and normal endometrium.
  • Researchers used high-throughput mRNA sequencing and found over 1300 genes that were dysregulated in the stromal cells from ectopic lesions, highlighting pathways related to cell adhesion and immune responses.
  • Findings suggest significant imbalances in the regulation of the complement system in these cells, stressing the importance of studying each cell type independently to understand the disease better.

Article Abstract

The aetiology of endometriosis is still unclear and to find mechanisms behind the disease development, it is important to study each cell type from endometrium and ectopic lesions independently. The objective of this study was to uncover complete mRNA profiles in uncultured stromal cells from paired samples of endometriomas and eutopic endometrium. High-throughput mRNA sequencing revealed over 1300 dysregulated genes in stromal cells from ectopic lesions, including several novel genes in the context of endometriosis. Functional annotation analysis of differentially expressed genes highlighted pathways related to cell adhesion, extracellular matrix-receptor interaction and complement and coagulation cascade. Most importantly, we found a simultaneous upregulation of complement system components and inhibitors, indicating major imbalances in complement regulation in ectopic stromal cells. We also performed experiments to evaluate the effect of endometriosis patients' peritoneal fluid (PF) on complement system gene expression levels, but no significant impact of PF on , and levels was observed. In conclusion, the use of isolated stromal cells enables to determine gene expression levels without the background interference of other cell types. In the future, a new standard design studying all cell types from endometriotic lesions separately should be applied to reveal novel mechanisms behind endometriosis pathogenesis.

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Source
http://dx.doi.org/10.1530/REP-17-0092DOI Listing

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