Novel 3D human trophoblast culture to explore T. cruzi infection in the placenta

Sofia Apodaca; Marco Di Salvatore; Arturo Muñoz-Calderón; María de Los Ángeles Curto; Silvia A Longhi; Alejandro G Schijman

doi:10.3389/fcimb.2024.1433424

Novel 3D human trophoblast culture to explore T. cruzi infection in the placenta

Front Cell Infect Microbiol. 2024 Aug 6:14:1433424. doi: 10.3389/fcimb.2024.1433424. eCollection 2024.

Authors

Sofia Apodaca¹, Marco Di Salvatore¹, Arturo Muñoz-Calderón¹, María de Los Ángeles Curto¹, Silvia A Longhi¹, Alejandro G Schijman¹

Affiliation

¹ Laboratorio de Biología Molecular de la Enfermedad de Chagas, Instituto de Investigaciones en Ingeniería Genética y Biología Molecular "Dr. Héctor Torres" (INGEBI), Consejo Nacional de Investigaciones Científicas y Técnicas (CONICET), Buenos Aires, Argentina.

Abstract

Introduction: Human trophoblastic cell lines, such as BeWo, are commonly used in 2D models to study placental Trypanosoma cruzi infections. However, these models do not accurately represent natural infections. Three-dimensional (3D) microtissue cultures offer a more physiologically relevant in vitro model, mimicking tissue microarchitecture and providing an environment closer to natural infections. These 3D cultures exhibit functions such as cell proliferation, differentiation, morphogenesis, and gene expression that resemble in vivo conditions.

Methods: We developed a 3D culture model using the human trophoblastic cell line BeWo and nonadherent agarose molds from the MicroTissues® 3D Petri Dish® system. Both small (12-256) and large (12-81) models were tested with varying initial cell numbers. We measured the diameter of the 3D cultures and evaluated cell viability using Trypan Blue dye. Trophoblast functionality was assessed by measuring β-hCG production via ELISA. Cell fusion was evaluated using confocal microscopy, with Phalloidin or ZO-1 marking cell edges and DAPI staining nuclei. T. cruzi infection was assessed by microscopy and quantitative PCR, targeting the EF1-α gene for T. cruzi and GAPDH for BeWo cells, using three parasite strains: VD (isolated from a congenital Chagas disease infant and classified as Tc VI), and K98 and Pan4 (unrelated to congenital infection and classified as Tc I).

Results: Seeding 1000 BeWo cells per microwell in the large model resulted in comparable cellular viability to 2D cultures, with a theoretical diameter of 408.68 ± 12.65 μm observed at 5 days. Functionality, assessed through β-hCG production, exceeded levels in 2D cultures at both 3 and 5 days. T. cruzi infection was confirmed by qPCR and microscopy, showing parasite presence inside the cells for all three tested strains. The distribution and progression of the infection varied with each strain.

Discussion: This innovative 3D model offers a simple yet effective approach for generating viable and functional cultures susceptible to T. cruzi infection, presenting significant potential for studying the placental microenvironment.

Keywords: Trypanosoma cruzi infection; congenital Chagas disease; human trophoblast; placental tropism; quantitative PCR; syncytiotrophoblast; three-dimensional microtissue model.

MeSH terms

Cell Culture Techniques / methods
Cell Culture Techniques, Three Dimensional / methods
Cell Line
Cell Survival
Chagas Disease* / parasitology
Female
Humans
Placenta* / parasitology
Pregnancy
Trophoblasts* / parasitology
Trypanosoma cruzi* / genetics
Trypanosoma cruzi* / growth & development
Trypanosoma cruzi* / physiology

Grants and funding

The author(s) declares financial support was received for the research, authorship, and/or publication of this article. This study was funded by PICT 2017- 0234 and PICT 2020-0862 from the Ministry of Science Technology and Innovation, Argentina to AS (principal investigator) and SL (research associate). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.