Expression of placental CD146 is dysregulated by prenatal alcohol exposure and contributes in cortical vasculature development and positioning of vessel-associated oligodendrocytes

Camille Sautreuil; Maryline Lecointre; Jessica Dalmasso; Alexis Lebon; Matthieu Leuillier; François Janin; Matthieu Lecuyer; Soumeya Bekri; Stéphane Marret; Annie Laquerrière; Carole Brasse-Lagnel; Sophie Gil; Bruno J Gonzalez

doi:10.3389/fncel.2023.1294746

Expression of placental CD146 is dysregulated by prenatal alcohol exposure and contributes in cortical vasculature development and positioning of vessel-associated oligodendrocytes

Front Cell Neurosci. 2024 Jan 10:17:1294746. doi: 10.3389/fncel.2023.1294746. eCollection 2023.

Authors

Affiliations

¹ Rouen Université, Inserm U1245 - Team "Epigenetics and Pathophysiology of Neurodevelopmental Disorders", Normandie Université, Normandy Centre for Genomic and Personalized Medicine, Rouen, France.
² Université de Paris, INSERM, UMR-S 1139, 3PHM, Paris, France.
³ Rouen Université, US51 HeRacLeS, PRIMACEN Platform, Faculty of Biological Sciences, Normandie Université, Mont-Saint-Aignan, France.
⁴ Rouen Université, Inserm U1096, Rouen, France.
⁵ Rouen Université, CHU Rouen, Department of Metabolic Biochemistry, Normandie University, Rouen, France.
⁶ Rouen Université, CHU Rouen, Department of Neonatal Pediatrics and Intensive Care, Rouen, France.
⁷ Rouen Université, CHU Rouen, Department of Pathology, Rouen Normandy Hospital, Rouen, France.

Abstract

Recent data showed that prenatal alcohol exposure (PAE) impairs the "placenta-brain" axis controlling fetal brain angiogenesis in human and preclinical models. Placental growth factor (PlGF) has been identified as a proangiogenic messenger between these two organs. CD146, a partner of the VEGFR-1/2 signalosome, is involved in placental angiogenesis and exists as a soluble circulating form. The aim of the present study was to investigate whether placental CD146 may contribute to brain vascular defects described in fetal alcohol spectrum disorder. At a physiological level, quantitative reverse transcription polymerase chain reaction experiments performed in human placenta showed that CD146 is expressed in developing villi and that membrane and soluble forms of CD146 are differentially expressed from the first trimester to term. In the mouse placenta, a similar expression pattern of CD146 was found. CD146 immunoreactivity was detected in the labyrinth zone and colocalized with CD31-positive endothelial cells. Significant amounts of soluble CD146 were quantified by ELISA in fetal blood, and the levels decreased after birth. In the fetal brain, the membrane form of CD146 was the majority and colocalized with microvessels. At a pathophysiological level, PAE induced marked dysregulation of CD146 expression. The soluble form of CD146 decreased in both placenta and fetal blood, whereas it increased in the fetal brain. Similarly, the expression of several members of the CD146 signalosome, such as VEGFR2 and PSEN, was differentially impaired between the two organs by PAE. At a functional level, targeted repression of placental CD146 by in utero electroporation (IUE) of CRISPR/Cas9 lentiviral plasmids resulted in (i) a decrease in cortical vessel density, (ii) a loss of radial vascular organization, and (iii) a reduced density of oligodendrocytes. Statistical analysis showed that the more the vasculature was impaired, the more the cortical oligodendrocyte density was reduced. Altogether, these data support that placental CD146 contributes to the proangiogenic "placenta-brain" axis and that placental CD146 dysfunction contributes to the cortical oligo-vascular development. Soluble CD146 would represent a promising placental biomarker candidate representative of alcohol-induced neurovascular defects in neonates, as recently suggested by PlGF (patents WO2016207253 and WO2018100143).

Keywords: angiogenesis; biomarker; diagnosis; fetal alcohol syndrome; neuroplacentology; neurovascular development.

Grants and funding

The author(s) declare financial support was received for the research, authorship, and/or publication of this article. This work was supported by Rouen University, Normandy University, the Institut National de la Santé et de la Recherche Médicale (INSERM; UMR1245), the Institute of Research and Innovation in Biomedicine (IRIB), the LARC-Neuroscience Network, the Fondation de France, the Fondation pour la Recherche en Alcoologie, the Conseil Régional de Normandie, the French National Research Agency (ANR), the Fonds Européen de Développement Régional (FEDER), the Regional Platform for Cell Imaging (PRIMACEN), and the AlcoBrain network. The AlcoBrain network is a consortium of academic researchers and clinicians. Dr. L. Abily Donval, Prof. V. Biran, Dr. C. Brasse-Lagnel, Dr. A.-G. Cordier, Dr. G. De La Villéon, Dr. T. Fournier, Dr. D. Germanaud, Prof. S. Gil, Dr. B.J. Gonzalez, Dr. P. Gressens, Prof. A. Laquerriére, Dr. M. Lecointre, Prof. S. Marret, and Dr. G. Pinto-Cardoso were involved in the AlcoBrain program, which is focused on the characterization of biomarkers for the early diagnosis of fetal alcohol spectrum disorders.