Immune cells control skin lymphatic electrolyte homeostasis and blood pressure
Helge Wiig, … , Kari Alitalo, Jens Titze
Helge Wiig, … , Kari Alitalo, Jens Titze
Published June 3, 2013
Citation Information: J Clin Invest. 2013;123(7):2803-2815. https://doi.org/10.1172/JCI60113.
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Research Article Immunology

Immune cells control skin lymphatic electrolyte homeostasis and blood pressure

Abstract

The skin interstitium sequesters excess Na+ and Cl in salt-sensitive hypertension. Mononuclear phagocyte system (MPS) cells are recruited to the skin, sense the hypertonic electrolyte accumulation in skin, and activate the tonicity-responsive enhancer-binding protein (TONEBP, also known as NFAT5) to initiate expression and secretion of VEGFC, which enhances electrolyte clearance via cutaneous lymph vessels and increases eNOS expression in blood vessels. It is unclear whether this local MPS response to osmotic stress is important to systemic blood pressure control. Herein, we show that deletion of TonEBP in mouse MPS cells prevents the VEGFC response to a high-salt diet (HSD) and increases blood pressure. Additionally, an antibody that blocks the lymph-endothelial VEGFC receptor, VEGFR3, selectively inhibited MPS-driven increases in cutaneous lymphatic capillary density, led to skin Cl accumulation, and induced salt-sensitive hypertension. Mice overexpressing soluble VEGFR3 in epidermal keratinocytes exhibited hypoplastic cutaneous lymph capillaries and increased Na+, Cl, and water retention in skin and salt-sensitive hypertension. Further, we found that HSD elevated skin osmolality above plasma levels. These results suggest that the skin contains a hypertonic interstitial fluid compartment in which MPS cells exert homeostatic and blood pressure–regulatory control by local organization of interstitial electrolyte clearance via TONEBP and VEGFC/VEGFR3–mediated modification of cutaneous lymphatic capillary function.

Authors

Helge Wiig, Agnes Schröder, Wolfgang Neuhofer, Jonathan Jantsch, Christoph Kopp, Tine V. Karlsen, Michael Boschmann, Jennifer Goss, Maija Bry, Natalia Rakova, Anke Dahlmann, Sven Brenner, Olav Tenstad, Harri Nurmi, Eero Mervaala, Hubertus Wagner, Franz-Xaver Beck, Dominik N. Müller, Dontscho Kerjaschki, Friedrich C. Luft, David G. Harrison, Kari Alitalo, Jens Titze

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Figure 5

HSD leads to skin Na+ and Cl storage and osmotic stress that is not reflected in plasma.

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HSD leads to skin Na+ and Cl– storage and osmotic stress that is not ref...
(A) Na+, Cl, and osmolality in plasma in rats remained unchanged with HSD, while Na+ and Cl content and concentrations increased in skin tissue. (B) HSD increased TonEBP and Vegfc mRNA expression and MPS cell count as well as MAP and interstitial fluid pressure (IFP) in the same rats. (C) Electron-dispersion x-ray scanning electron microprobe analysis of Na+ and Cl concentrations in skin lymph capillaries in DOCA-HSD rats. The arrow denotes lymphatic capillary site from which the spectra were obtained. Scale bar: 20 mm. Lymphatic capillary Na+ was higher than that in plasma. The Cl values were not significantly different. (D) Na+ concentration and osmolality in skin microdialysate and in plasma in rats. (E) Direct plasma and skin-tissue vapor pressure osmolality measurements in rats after 2 weeks of LSD and HSD. DOCA, deoxycorticosterone acetate. *P (diet) < 0.05; P (fluid composition) < 0.05.