No NLRP3 inflammasome activity in kidney epithelial cells, not even when the NLRP3-A350V Muckle-Wells variant is expressed in podocytes of diabetic mice

被引:9
作者
Kunte, Sophie Carina [1 ]
Marschner, Julian A. [1 ]
Klaus, Martin [1 ]
Honda, Tamisa [1 ]
Li, Chenyu [1 ]
Motrapu, Manga [1 ]
Walz, Christoph [2 ]
Angelotti, Maria Lucia [3 ]
Antonelli, Giulia [3 ,4 ]
Melica, Maria Elena [3 ]
De Chiara, Letizia [3 ]
Semeraro, Roberto [5 ]
Nelson, Peter J. [1 ]
Anders, Hans-Joachim [1 ]
机构
[1] Klinikum Univ Munchen, Nephrol Zentrum, Med Klin & Poliklinik 4, LMU Munchen, Munich, Germany
[2] LMU Munchen, Pathol Inst, Med Fak, Munich, Germany
[3] Univ Florence, Dept Expt & Biomed Sci Mario Serio, Florence, Italy
[4] Meyer Childrens Hosp IRCCS, Nephrol & Dialysis Unit, Florence, Italy
[5] Univ Florence, Dept Expt & Clin Med, Florence, Italy
关键词
inflammasome; inflammation; diabetes; chronic kidney disease; IL-1; proteinuria; ACTIVATION; CONTRIBUTES; IL-1-BETA;
D O I
10.3389/fimmu.2023.1230050
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
BackgroundThe NLRP3 inflammasome integrates several danger signals into the activation of innate immunity and inflammation by secreting IL-1 & beta; and IL-18. Most published data relate to the NLRP3 inflammasome in immune cells, but some reports claim similar roles in parenchymal, namely epithelial, cells. For example, podocytes, epithelial cells critical for the maintenance of kidney filtration, have been reported to express NLRP3 and to release IL-& beta; in diabetic kidney disease, contributing to filtration barrier dysfunction and kidney injury. We questioned this and hence performed independent verification experiments.MethodsWe studied the expression of inflammasome components in human and mouse kidneys and human podocytes using single-cell transcriptome analysis. Human podocytes were exposed to NLRP3 inflammasome agonists in vitro and we induced diabetes in mice with a podocyte-specific expression of the Muckle-Wells variant of NLRP3, leading to overactivation of the Nlrp3 inflammasome (Nphs2Cre;Nlrp3A350V) versus wildtype controls. Phenotype analysis included deep learning-based glomerular and podocyte morphometry, tissue clearing, and STED microscopy of the glomerular filtration barrier. The Nlrp3 inflammasome was blocked by feeding ss-hydroxy-butyrate.ResultsSingle-cell transcriptome analysis did not support relevant NLRP3 expression in parenchymal cells of the kidney. The same applied to primary human podocytes in which NLRP3 agonists did not induce IL-1 & beta; or IL-18 secretion. Diabetes induced identical glomerulomegaly in wildtype and Nphs2Cre;Nlrp3A350V mice but hyperfiltration-induced podocyte loss was attenuated and podocytes were larger in Nphs2Cre;Nlrp3A350V mice, an effect reversible with feeding the NLRP3 inflammasome antagonist ss-hydroxy-butyrate. Ultrastructural analysis of the slit diaphragm was genotype-independent hence albuminuria was identical.ConclusionPodocytes express low amounts of the NLRP3 inflammasome, if at all, and do not produce IL-1 & beta; and IL-18, not even upon introduction of the A350V Muckle-Wells NLRP3 variant and upon induction of podocyte stress. NLRP3-mediated glomerular inflammation is limited to immune cells.
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页数:14
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