Functional characterization of podocyte-expressed THSD7A in experimental membranous nephropathy
Ming Huang, Moritz Lassé, Silke Dehde, Felicitas E. Hengel, Fatih Demir, Anja M. Billing, Ning Song, Larissa Seifert, Oliver Kretz, Florian Grahammer, Ulf Panzer, Sebastian Brähler, Tobias B. Huber, Gunther Zahner, Markus M. Rinschen, Nicola M. Tomas
Ming Huang, Moritz Lassé, Silke Dehde, Felicitas E. Hengel, Fatih Demir, Anja M. Billing, Ning Song, Larissa Seifert, Oliver Kretz, Florian Grahammer, Ulf Panzer, Sebastian Brähler, Tobias B. Huber, Gunther Zahner, Markus M. Rinschen, Nicola M. Tomas
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Research Article Cell biology Immunology Nephrology

Functional characterization of podocyte-expressed THSD7A in experimental membranous nephropathy

Abstract

Although the pathogenic role of autoantibodies targeting the podocyte protein THSD7A in membranous nephropathy (MN) is well described, the consequences of autoantibody binding for podocyte homeostasis and the function of THSD7A remain unclear. Here, we induced an MN model in control and podocyte-specific Thsd7a-KO (Thsd7a–/–) mice using rabbit anti-THSD7A antibodies, followed by transcriptome and proteome analyses. Anti-THSD7A antibodies in WT mice caused significant loss of key slit diaphragm (SD) proteins, such as nephrin and NEPH1, without transcriptional downregulation. Glomeruli showed substantial transcriptomic and proteomic reconfiguration indicative of extensive podocyte injury, including disruptions in podocyte adhesion, cytoskeletal dynamics, and marked upregulation of ubiquitin-proteasome system components, cathepsins, and ADAM proteases. Notably, experiments in C3-deficient mice revealed that proteolytic activation and SD protein loss are driven by complement-independent pathways. Thsd7a–/– mice only displayed a mild phenotype under basal conditions, and they were completely protected from MN development upon anti-THSD7A antibody transfer. Finally, interactome analysis identified a protein complex, including THSD7A and integrin α3, linking THSD7A complexes to pathogenic regulation of cytoskeleton, adhesion, and membrane signaling in MN. Thus, anti-THSD7A antibodies induce profound molecular reconfiguration, including dysregulated proteolytic systems via a complement-independent pathway, revealing potential therapeutic targets in MN.

Authors

Ming Huang, Moritz Lassé, Silke Dehde, Felicitas E. Hengel, Fatih Demir, Anja M. Billing, Ning Song, Larissa Seifert, Oliver Kretz, Florian Grahammer, Ulf Panzer, Sebastian Brähler, Tobias B. Huber, Gunther Zahner, Markus M. Rinschen, Nicola M. Tomas

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Figure 5

Correlation of transcriptomic and proteomic data reveals protein degradation as a key mechanism in THSD7A-associated MN.

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Correlation of transcriptomic and proteomic data reveals protein degrada...
(A) Correlation between transcriptomic and proteomic gene expression levels in experimental THSD7A-associated MN at day 5. After filtering by adjusted P value less than 0.05, the log2 FC of genes (day 5 MN vs. control) from RNA-Seq is plotted against the log2FC of proteins (control + anti-THSD7A IgG group vs. control + control IgG group). The horizontal and vertical dashed lines indicate the threshold log2FC = ± 0.5. Pearson’s correlation and P value were calculated. Colored dots correspond to the differentially expressed genes/proteins. In the legend, homodirectional means upregulated or downregulated both in transcriptome and proteome levels; opposite change is upregulated at one level while downregulated at the other; proteome means only significantly regulated in protein levels; transcriptome means only significantly regulated in transcript level. (B) Heatmaps declaring the log2FC of slit diaphragm genes and proteins in comparison of MN versus control groups. Nonsignificant genes are shown in gray. (C and D) Heatmaps showing the log2FC of protein degradation–associated proteins in proteomic data (C) or genes in bulk RNA-Seq data (D) in MN versus control comparisons. (E) Left: immunofluorescence stainings for ADAM15 (green) and nephrin (red) 5 days after injection of control IgG or anti-THSD7A IgG. Nuclei were counterstained with Hoechst (blue). Scale bars: 10 μm (zoom-out panels); 2 μm (zoom-in panels). Right: quantification (MFI) of ADAM15. **P < 0.01 (unpaired 2-tailed t test). Data shown as mean ± SEM, n = 4 per group.