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Endothelial TDP-43 controls sprouting angiogenesis and vascular barrier integrity, and its deletion triggers neuroinflammation
Víctor Arribas, … , Bettina Schmid, Eloi Montanez
Víctor Arribas, … , Bettina Schmid, Eloi Montanez
Published February 1, 2024
Citation Information: JCI Insight. 2024;9(5):e177819. https://doi.org/10.1172/jci.insight.177819.
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Research Article Angiogenesis Vascular biology

Endothelial TDP-43 controls sprouting angiogenesis and vascular barrier integrity, and its deletion triggers neuroinflammation

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Abstract

TAR DNA-binding protein 43 (TDP-43) is a DNA/RNA-binding protein that regulates gene expression, and its malfunction in neurons has been causally associated with multiple neurodegenerative disorders. Although progress has been made in understanding the functions of TDP-43 in neurons, little is known about its roles in endothelial cells (ECs), angiogenesis, and vascular function. Using inducible EC-specific TDP-43–KO mice, we showed that TDP-43 is required for sprouting angiogenesis, vascular barrier integrity, and blood vessel stability. Postnatal EC-specific deletion of TDP-43 led to retinal hypovascularization due to defects in vessel sprouting associated with reduced EC proliferation and migration. In mature blood vessels, loss of TDP-43 disrupted the blood-brain barrier and triggered vascular degeneration. These vascular defects were associated with an inflammatory response in the CNS with activation of microglia and astrocytes. Mechanistically, deletion of TDP-43 disrupted the fibronectin matrix around sprouting vessels and reduced β-catenin signaling in ECs. Together, our results indicate that TDP-43 is essential for the formation of a stable and mature vasculature.

Authors

Víctor Arribas, Yara Onetti, Marina Ramiro-Pareta, Pilar Villacampa, Heike Beck, Mariona Alberola, Anna Esteve-Codina, Angelika Merkel, Markus Sperandio, Ofelia M. Martínez-Estrada, Bettina Schmid, Eloi Montanez

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Figure 8

Loss of endothelial TDP-43 triggers inflammation in the CNS.

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Loss of endothelial TDP-43 triggers inflammation in the CNS.
(A) Confoca...
(A) Confocal high-magnification images of P16 control and TDP-43iΔEC spinal cord and brain sections stained for IB4 (green), the microglial marker Iba1 (red), and Ter119 (blue). White squares indicate the magnified ROIs. Note the enhanced Iba1 staining in TDP-43iΔEC samples and the morphological differences between Iba1+ cells from control and TDP-43iΔEC mice. Scale bars: 40 μm. (B) Quantification of Iba1 fluorescence intensity per field and total Iba1+ cells per field in P16 control and TDP-43iΔEC spinal cord and brain as indicated. Data are shown as mean ± SEM. *P < 0.05, **P < 0.01. Mann-Whitney U test. (C) Confocal high-magnification images of P16 control and TDP-43iΔEC spinal cord and brain sections stained for IB4 (green), the astrocytic marker GFAP (red), and Ter119 (blue). White squares indicate the magnified ROIs. Note the presence of reactive astrocytes in TDP-43iΔEC spinal cord and brain. Scale bars: 50 μm (spinal cord) and 40 μm (brain).

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