IL-23 reshapes kidney resident cell metabolism and promotes local kidney inflammation
Hao Li, … , Jarrat Jordan, George C. Tsokos
Hao Li, … , Jarrat Jordan, George C. Tsokos
Published May 6, 2021
Citation Information: J Clin Invest. 2021;131(12):e142428. https://doi.org/10.1172/JCI142428.
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Research Article Autoimmunity

IL-23 reshapes kidney resident cell metabolism and promotes local kidney inflammation

Abstract

Interstitial kidney inflammation is present in various nephritides in which serum interleukin 23 (IL-23) is elevated. Here we showed that murine and human renal tubular epithelial cells (TECs) expressing the IL-23 receptor (IL-23R) responded to IL-23 by inducing intracellular calcium flux, enhancing glycolysis, and upregulating calcium/calmodulin kinase IV (CaMK4), which resulted in suppression of the expression of the arginine-degrading enzyme arginase 1 (ARG1), thus increasing in situ levels of free L-arginine. Limited availability of arginine suppressed the ability of infiltrating T cells to proliferate and produce inflammatory cytokines. TECs from humans and mice with nephritis expressed increased levels of IL-23R and CaMK4 but reduced levels of ARG1. TEC-specific deletion of Il23r or Camk4 suppressed inflammation, whereas deletion of Arg1 exacerbated inflammation in different murine disease models. Finally, TEC-specific delivery of a CaMK4 inhibitor specifically curbed renal inflammation in lupus-prone mice without affecting systemic inflammation. Our data offer the first evidence to our knowledge of the immunosuppressive capacity of TECs through a mechanism that involves competitive uptake of arginine and signify the importance of modulation of an inflammatory cytokine in the function of nonlymphoid cells, which leads to the establishment of an inflammatory microenvironment. New approaches to treat kidney inflammation should consider restoring the immunosuppressive capacity of TECs.

Authors

Hao Li, Maria G. Tsokos, Rhea Bhargava, Iannis E. Adamopoulos, Hanni Menn-Josephy, Isaac E. Stillman, Philip Rosenstiel, Jarrat Jordan, George C. Tsokos

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Figure 5

TEC-targeted delivery of the CaMK4 inhibitor KN93 efficiently suppresses renal inflammation in lupus-prone MRL.lpr mice.

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TEC-targeted delivery of the CaMK4 inhibitor KN93 efficiently suppresses...
(A) Cryosection of kidneys from female Il23r-GFP MRL.lpr mice at the indicated ages stained for CD26 (red). Magnification, ×20; scale bar: 20 μm. (B) Immunohistochemical staining of CaMK4 (left) and CaMK2 (right) in the kidneys of female MRL.lpr mice at the indicated ages; boxed areas were digitally magnified. Magnification, ×40; scale bar: 25 μm. (C) Cryosection of kidneys from in MRL.lpr mice at the indicated ages stained for ARG1 (red) and CD26 (green). Magnification, ×20; scale bar: 20 μm. (D) Ten-week-old MRL.lpr mice were administered anti–cadherin-16–coated nanolipogel–rhodamine and euthanized after the indicated time for analysis. Confocal microscopic images show the targeted delivery by rhodamine+ cells in representative kidney areas. Magnification, ×10; scale bar: 50 μm. (EI) Ten-week-old MRL.lpr mice were administered anti–cadherin-16–coated empty nanolipogels (nlg) or nanolipogel-KN93 every 10 days for a total of4 times. Representative images of kidney sections stained with H&E (E) and Masson’s trichrome and PAS (F) with the indicated magnification. Scale bar: 200 μm (×4 magnification) and 25 μm (×40 magnification). (G) Histopathologic scoring of kidneys. (H) The mean ratio of urine albumin and creatinine. (I) Flow cytometric quantification of infiltrating CD4+ T cells and activated macrophages/neutrophils in kidneys. (JL) Bone marrow (BM) reconstitution was carried out by transferring BM from 2-month-old B6.lpr mice to lethally irradiated indicated recipients for 10 months. All recipients were Cdh16-cre+: Cdh16-Cre (control), Cdh16-Cre × Il23rfl/fl (Il23rΔTEC), Cdh16-Cre × Camk4fl/fl (Camk4ΔTEC), and Cdh16-Cre × Arg1fl/fl (Arg1ΔTEC). (J) Representative H&E images of kidneys from the indicated mice; boxed areas were digitally magnified. Magnification, ×5; scale bar: 200 μm. (K) Flow cytometric quantification of CD4+ T cells and activated macrophages/neutrophils in kidneys. (L) Histopathologic scoring of kidneys. Data represent the mean ± SEM; n = 4–6 mice per group in each experiment for 2 independent experiments. *P < 0.05, **P < 0.01, ***P < 0.005 versus control by Student’s t test (G and H) or 2-way ANOVA (K and L).