Primary Trophoblast Cultures: Characterization of HLA Profiles and Immune Cell Interactions

Michael Eikmans; Carin van der Keur; Jacqueline D H Anholts; Jos J M Drabbels; Els van Beelen; Susana M Chuva de Sousa Lopes; Marie-Louise van der Hoorn

doi:10.3389/fimmu.2022.814019

Primary Trophoblast Cultures: Characterization of HLA Profiles and Immune Cell Interactions

Front Immunol. 2022 May 13:13:814019. doi: 10.3389/fimmu.2022.814019. eCollection 2022.

Authors

Michael Eikmans¹, Carin van der Keur¹, Jacqueline D H Anholts¹, Jos J M Drabbels¹, Els van Beelen¹, Susana M Chuva de Sousa Lopes², Marie-Louise van der Hoorn³

Affiliations

¹ Department of Immunology, Leiden University Medical Center, Leiden, Netherlands.
² Department of Anatomy and Embryology, Leiden University Medical Center, Leiden, Netherlands.
³ Department of Gynecology and Obstetrics, Leiden University Medical Center, Leiden, Netherlands.

Abstract

Introduction: Trophoblasts are essential in fetal-maternal interaction during pregnancy. The goal was to study HLA profiles of primary trophoblasts derived from placentas, and to investigate their usefulness in studying interaction with immune cells.

Methods: After enzymatic digestion of first-trimester placental tissue from seven donors (6-9 weeks gestation) and trophoblast enrichment we cultured cytotrophoblasts (CTB) in stem cell medium. CTB were differentiated into EVT in a Matrigel-containing medium. A subset of CTB/EVT was profiled for microRNA levels. Expression of classical HLA molecules and of HLA-G was studied by flow cytometry, qPCR, and ELISA. Secondary trophoblast cell lines JAR and JEG-3 were studied as controls. Lymphocytes were investigated during co-culturing with EVT.

Results: The trophoblasts could be easily maintained for several passages, upregulated classical trophoblast markers (GATA3, TFAP2C, chromosome-19 microRNAs), and upon differentiation to EVT they were selective in expressing HLA-C. EVT showed increasing expression of total HLA-G, an increasing proportion of HLA-G1 over G2- and G3 isoforms, and elevated excretion of soluble HLA-G. These features were distinct from those of the secondary trophoblast cell lines. TNF-α and IL-8 represented the most abundantly secreted cytokines by CTB, but their levels were minimal in EVT cultures. As proof of principle, we showed that EVT affect lymphocytes in three-day co-cultures (n=4) by decreasing activation marker HLA-DR.

Conclusion: We verified the possibility culturing trophoblasts from first-term placentas, and their capability of differentiating to HLA-G expressing EVT. This culture model better represents the in-vivo situation than previously studied secondary trophoblast cell lines and enables mechanistic studies of fetal-maternal interactions.

Keywords: HLA-G; culturing; differentiation; immune cell; placenta; pregnancy; stem cell; trophoblast.

MeSH terms

Cell Communication
Cell Line, Tumor
Female
HLA-G Antigens / metabolism
Humans
Placenta* / metabolism
Pregnancy
Trophoblasts* / metabolism

Substances

HLA-G Antigens