C3aR-initiated signaling is a critical mechanism of podocyte injury in membranous nephropathy
Qi Zhang, … , Paolo Cravedi, Stefano Da Sacco
Qi Zhang, … , Paolo Cravedi, Stefano Da Sacco
Published January 16, 2024
Citation Information: JCI Insight. 2024;9(4):e172976. https://doi.org/10.1172/jci.insight.172976.
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Research Article Nephrology

C3aR-initiated signaling is a critical mechanism of podocyte injury in membranous nephropathy

Abstract

The deposition of antipodocyte autoantibodies in the glomerular subepithelial space induces primary membranous nephropathy (MN), the leading cause of nephrotic syndrome worldwide. Taking advantage of the glomerulus-on-a-chip system, we modeled human primary MN induced by anti-PLA2R antibodies. Here we show that exposure of primary human podocytes expressing PLA2R to MN serum results in IgG deposition and complement activation on their surface, leading to loss of the chip permselectivity to albumin. C3a receptor (C3aR) antagonists as well as C3AR gene silencing in podocytes reduced oxidative stress induced by MN serum and prevented albumin leakage. In contrast, inhibition of the formation of the membrane-attack-complex (MAC), previously thought to play a major role in MN pathogenesis, did not affect permselectivity to albumin. In addition, treatment with a C3aR antagonist effectively prevented proteinuria in a mouse model of MN, substantiating the chip findings. In conclusion, using a combination of pathophysiologically relevant in vitro and in vivo models, we established that C3a/C3aR signaling plays a critical role in complement-mediated MN pathogenesis, indicating an alternative therapeutic target for MN.

Authors

Qi Zhang, Sofia Bin, Kelly Budge, Astgik Petrosyan, Valentina Villani, Paola Aguiari, Coralien Vink, Jack Wetzels, Hasmik Soloyan, Gaetano La Manna, Manuel Alfredo Podestà, Paolo Molinari, Sargis Sedrakyan, Kevin V. Lemley, Roger E. De Filippo, Laura Perin, Paolo Cravedi, Stefano Da Sacco

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Figure 1

The GOAC recapitulates podocyte injury in vitro.

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The GOAC recapitulates podocyte injury in vitro. (A) Schematic represent...
(A) Schematic representation of the GOAC. (B) Light microscope image, depicting the formation of the barrier (72 hours). Scale bar: 400 µm. (C) Representative image of albumin test (albumin-FITC, 40 mg/mL, yellow) confirming permselectivity. (D) Podocytes in vitro express PLA2R (red). Scale bar: 25 µm. DAPI, blue. (E) Measurement of FITC-albumin in GOAC exposed to anti-PLA2R MN serum (n ≥ 4/group). Additional results in Supplemental Figure 2. (F) PLA2R1 RNA expression following knockdown on hAKPC cells; control: scramble hAKPC cells. (G) Western Blotting showing reduced PLA2R (150 kDa) expression after KD in hAKPC-derived podocytes. β-Actin: 42 KDa; n = 3/group. (H) Measurement of FITC-albumin in GOAC filtrate with PLA2R–knocked-down hAKPC-derived podocytes (groups: regular media, healthy serum and PLA2R-Ab+ MN serum, n ≥ 4/group.) (I) Antibody neutralization by IdeS in MN serum prevents GOAC leakage (n ≥ 4/group). Additional results in Supplemental Figure 5. (J)Complement neutralization by heat-inactivation successfully prevents GOAC injury by MN patient serum (n ≥ 4/group). Additional results in Supplemental Figure 6. (K) C5b-9 (MAC) formation on GOAC after serum exposure. Healthy serum with or without protein S (no MAC, top 2 panels) vs. MN serum (MAC, third panel) in podocin+ cells (red). Protein S prevents MAC formation (lower panel). Yellow arrows: MAC/podocin overlap. Magnified views of GEC (unstained) and podocin+ cells (red) with or without MAC (green); DAPI, blue. Scale bar: 100 µm. (L) MAC neutralization, while preventing C5b-9 formation, does not prevent leakage (n = 4/group). Additional results in Supplemental Figure 6. (M) GOAC exposure to healthy serum (1%), heat-inactivated anti-PLA2R (0.5%) + healthy serum (0.5%), heat-inactivated anti-PLA2R (0.5%) + C6-deficient healthy serum (0.5%), heat-inactivated- anti-PLA2R (0.5%) + anti-PLA2R (0.5%), or heat-inactivated anti-PLA2R (0.5%) + anti-PLA2R (0.5%) + protein S. (n ≥ 4/group). All statistical values determined by 1-way ANOVA with the exclusion of E and G (2-tailed Student’s t test). *P < 0.05 **P < 0.01; ***P < 0.001; ****P < 0.0001.