C5aR1 promotes acute pyelonephritis induced by uropathogenic E. coli
Ke Li, Kun-Yi Wu, Weiju Wu, Na Wang, Ting Zhang, Naheed Choudhry, Yun Song, Conrad A. Farrar, Liang Ma, Lin-lin Wei, Zhao-Yang Duan, Xia Dong, En-Qi Liu, Zong-Fang Li, Steven H. Sacks, Wuding Zhou
Ke Li, Kun-Yi Wu, Weiju Wu, Na Wang, Ting Zhang, Naheed Choudhry, Yun Song, Conrad A. Farrar, Liang Ma, Lin-lin Wei, Zhao-Yang Duan, Xia Dong, En-Qi Liu, Zong-Fang Li, Steven H. Sacks, Wuding Zhou
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Research Article Nephrology

C5aR1 promotes acute pyelonephritis induced by uropathogenic E. coli

Abstract

C5a receptor 1 (C5aR1) is a G protein–coupled receptor for C5a and also an N-linked glycosylated protein. In addition to myeloid cells, C5aR1 is expressed on epithelial cells. In this study, we examined the role of C5aR1 in bacterial adhesion/colonization of renal tubular epithelium and addressed the underlying mechanisms of this role. We show that acute kidney infection was significantly reduced in mice with genetic deletion or through pharmacologic inhibition of C5aR1 following bladder inoculation with uropathogenic E. coli (UPEC). This was associated with reduced expression of terminal α-mannosyl residues (Man; a ligand for type 1 fimbriae of E. coli) on the luminal surface of renal tubular epithelium and reduction of early UPEC colonization in these mice. Confocal microscopy demonstrated that UPEC bind to Man on the luminal surface of renal tubular epithelium. In vitro analyses showed that C5a stimulation enhances Man expression in renal tubular epithelial cells and subsequent bacterial adhesion, which, at least in part, is dependent on TNF-α driven by C5aR1-mediated intracellular signaling. Our findings demonstrate a previously unknown pathogenic role for C5aR1 in acute pyelonephritis, proposing a potentially novel mechanism by which C5a/C5aR1 signaling mediates upregulation of carbohydrate ligands on renal tubules to facilitate UPEC adhesion.

Authors

Ke Li, Kun-Yi Wu, Weiju Wu, Na Wang, Ting Zhang, Naheed Choudhry, Yun Song, Conrad A. Farrar, Liang Ma, Lin-lin Wei, Zhao-Yang Duan, Xia Dong, En-Qi Liu, Zong-Fang Li, Steven H. Sacks, Wuding Zhou

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Figure 5

Effects of C5a on intracellular signalling, proinflammatory cytokine production, and mannosyl residue expression in renal tubular epithelial cells (in vitro).

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Effects of C5a on intracellular signalling, proinflammatory cytokine pro...
(A) Renal tubular epithelial cells (RTECs) cultured from WT mice were preincubated with or without forskolin (Fsk, a cAMP elevating agent) (10 μM) for 1 hour and stimulated with C5a (0–20 nM) for 30 minutes. Intracellular cAMP levels were measured in the cell lysates, shown as changes relative to control (untreated cells). n = 3/group, resulting from 3 independent experiments. **P < 0.005. (B) Western blot analysis for ERK1/2 and IκB phosphorylation in RTECs after C5a (20 nM) stimulation for up to 30 minutes. In each set of blots, the top row of bands corresponds to membrane incubated with appropriate anti-phospho antibody and the bottom row of bands corresponds to membrane incubated with appropriate total antibody. Relative amounts of protein phosphorylation are shown in the right panel of each set of blots. n = 3/group, resulting from 3 independent experiments. (C) Relative mRNA levels of TNF-α in the RTECs, determined by RT-qPCR. n = 4/group, resulting from 4 independent experiments. ***P < 0.001. (D) Secretion of TNF-α by the RTECs (supernatants from 24-hour cultures), measured by ELISA. n = 3/group, resulting from 3 independent experiments. ***P < 0.001; P = 0.0014 (LPS versus LPS plus C5a treatment). (E) Representative images of Man (green) in RTECs that had been pretreated with control Ig, C5a/control Ig, or C5a/anti–TNF-α antibody for 24 hours. Scale bars: 25 μm. (F) Quantification of Man expression in RTECs in E. n = 6 coverslips/group, resulting from 3 independent experiments. **P < 0.005, ***P < 0.001. Data were analyzed by 1-way ANOVA with Tukey’s multiple comparisons test (A, C, D, and F) or 1-way ANOVA (B).