Intrinsic endothelial hyperresponsiveness to inflammatory mediators drives acute episodes in models of Clarkson disease
Ararat J. Ablooglu, … , Samir M. Parikh, Kirk M. Druey
Ararat J. Ablooglu, … , Samir M. Parikh, Kirk M. Druey
Published March 19, 2024
Citation Information: J Clin Invest. 2024;134(10):e169137. https://doi.org/10.1172/JCI169137.
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Research Article Vascular biology

Intrinsic endothelial hyperresponsiveness to inflammatory mediators drives acute episodes in models of Clarkson disease

Abstract

Clarkson disease, or monoclonal gammopathy–associated idiopathic systemic capillary leak syndrome (ISCLS), is a rare, relapsing-remitting disorder featuring the abrupt extravasation of fluids and proteins into peripheral tissues, which in turn leads to hypotensive shock, severe hemoconcentration, and hypoalbuminemia. The specific leakage factor(s) and pathways in ISCLS are unknown, and there is no effective treatment for acute flares. Here, we characterize an autonomous vascular endothelial defect in ISCLS that was recapitulated in patient-derived endothelial cells (ECs) in culture and in a mouse model of disease. ISCLS-derived ECs were functionally hyperresponsive to permeability-inducing factors like VEGF and histamine, in part due to increased endothelial nitric oxide synthase (eNOS) activity. eNOS blockade by administration of N(γ)-nitro-l-arginine methyl ester (l-NAME) ameliorated vascular leakage in an SJL/J mouse model of ISCLS induced by histamine or VEGF challenge. eNOS mislocalization and decreased protein phosphatase 2A (PP2A) expression may contribute to eNOS hyperactivation in ISCLS-derived ECs. Our findings provide mechanistic insights into microvascular barrier dysfunction in ISCLS and highlight a potential therapeutic approach.

Authors

Ararat J. Ablooglu, Wei-Sheng Chen, Zhihui Xie, Abhishek Desai, Subrata Paul, Justin B. Lack, Linda A. Scott, A. Robin Eisch, Arkadiusz Z. Dudek, Samir M. Parikh, Kirk M. Druey

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Figure 8

Aberrant eNOS localization and PP2A expression in ISCLS-derived BOECs.

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Aberrant eNOS localization and PP2A expression in ISCLS-derived BOECs. (...
(A) BOECs stained with anti–p-eNOS (left, green) or anti-eNOS (middle, red) antibodies and DAPI. Arrows denote eNOS clusters. Scale bar: 20 μm. (B) Numbers of eNOS clusters/cell. Data indicate the mean ± SEM. n = 3 cell lines/group. *P = 0.03 and **P = 0.006, by 2-way ANOVA with Šidák’s multiple comparisons. (C) Representative immunoblot of PP2A subunits in BOEC lysates (n = 5 donors/group). (D) Quantification of relative protein expression. Data indicate the mean ± SEM. n = 7–9 donors/group. *P = 0.03, by 2-way ANOVA with Šidák’s multiple comparisons. (E) Relative PPP2R1B expression in BOECs evaluated by qPCR (normalized to GAPDH). Data indicate the mean ± SEM. n = 6–9 donors/group. NS, by unpaired, 2-tailed Student’s t test. (F) Representative immunoblot of FLAG-PP2A-Aβ in BOECs transfected with the respective lentiviruses. (G and H) Representative TER (G) and maximum decrease in VEGF-induced TER (H) from t = 0 (arrow) in BOECs infected with control or FLAG–PP2A-β–encoding lentivirus. Data indicate the mean ± SEM. n = 2 donors/group analyzed in 4 independent experiments. **P = 0.001, by unpaired, 2-tailed Student’s t test. (I and J). Representative blot (I) and quantification (J) of p-eNOS/eNOS in control versus FLAG–PP2A-β–overexpressing BOECs stimulated with VEGF (100 ng/mL). Data indicate the mean ± SEM. n = 5 independent experiments. **P = 0.004, by 2-way ANOVA with Šidák’s multiple comparisons.