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Role of ultrastructural determinants of glomerular permeability in ultrafiltration function loss
Andrea Remuzzi, Sara Conti, Bogdan Ene-Iordache, Susanna Tomasoni, Paola Rizzo, Ariela Benigni, Giuseppe Remuzzi
Andrea Remuzzi, Sara Conti, Bogdan Ene-Iordache, Susanna Tomasoni, Paola Rizzo, Ariela Benigni, Giuseppe Remuzzi
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Research Article Nephrology

Role of ultrastructural determinants of glomerular permeability in ultrafiltration function loss

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Abstract

The epithelial filtration slit is a crucial component of the glomerular capillary membrane, which is essential for maintaining glomerular filtration function. Though chronic kidney diseases are an immense clinical problem, the mechanisms through which structural alterations reduce glomerular water filtration have not yet been understood completely. To investigate the mechanisms underlying filtration function loss, we studied rats with spontaneously occurring progressive kidney disease, either treated with angiotensin II antagonist or untreated, combining high-resolution electron microscopy of the glomerular capillary wall with theoretical water filtration modeling. Under pathological conditions, epithelial filtration pores and the extension of the subpodocyte space were larger than in normal controls. Numerical analyses indicated that these ultrastructural changes increased hydraulic resistance of the glomerular capillary wall by extending coverage of the filtration barrier by the subpodocyte space, with the changes in hydrodynamic forces acting on podocytes likely being responsible for their detachment. Angiotensin II inhibition normalized the subpodocyte space’s hydraulic resistance, restored mechanical podocyte load, and preserved CD151–α3 integrin complex assembly, improving podocyte adherence and survival. Our results show that ultrastructural changes in podocytes are major determinants of the hydraulic resistance of the glomerular capillary wall and highlight the mechanism of podocyte loss in kidney disease progression, as well as the mechanisms underlying angiotensin II inhibition.

Authors

Andrea Remuzzi, Sara Conti, Bogdan Ene-Iordache, Susanna Tomasoni, Paola Rizzo, Ariela Benigni, Giuseppe Remuzzi

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Figure 2

ACEi reduced SPS in proteinuric MWF animals.

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ACEi reduced SPS in proteinuric MWF animals.
(A) Quantification of SPS a...
(A) Quantification of SPS area. *P < 0.05 vs. Wistar; ANOVA with Tukey’s post hoc test. lis, lisinopril. (B) Representative images from Wistar and MWF rats at 20 weeks and in MWF rats treated with lisinopril between 10 and 20 weeks of age. The SPS is highlighted in yellow. Scale bars: 500 nm. Images are representative of 3 rats per group. In proteinuric MWF animals, podocytes are lost by detaching from the GBM as viable cells. Immunoperoxidase staining for WT-1 (C and E) and toluidine blue–stained sections in MWF rats (D and F) showing detached podocytes with viable-appearing nuclei (arrowheads) in the Bowman’s space (C and D) and in the tubular lumen (E and F). Images are representative of 3 rats per group, and 10–12 glomeruli were analyzed per rat. Scale bars: 20 μm for C, E, and F; 10 μm for D.

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