PEER-REVIEWED PUBLICATION

2026

3D fractal topography attenuates inflammation and confers resilience to glomerular podocytes

Wang Y, Dikyol C, et al.

Cell Biomaterials

University of Toronto, Toronto General Research Institute, Terrence Donnelly Centre for Cellular & Biomolecular Research

RESEARCH SUMMARY
This study engineered glomerulus-scale 3D fractal hemispheres (≈200 µm diameter, ≈100 µm height) fabricated via Nanoscribe two-photon polymerization in a flexible IP-PDMS resin to model how physiologically inspired surface fractality regulates human podocyte maturation and inflammatory resilience. Across smooth to increasingly complex fractal indices, intermediate fractality promoted podocyte cytoskeletal branching/orientation, increased slit diaphragm marker nephrin, and elevated ECM-associated markers (e.g., collagen IV), consistent with enhanced maturation. Transcriptomic profiling showed that podocytes on intermediate fractal substrates upregulated nephrogenesis-related programs while suppressing inflammatory and kidney disease–associated pathways (including TNF, IL-17, p53, FoxO, and PI3K-Akt signaling), with supportive cytokine profiling in conditioned media. Under inflammatory challenge with TNF-α and IL-6, podocytes cultured on fractal hemispheres—especially intermediate fractality—exhibited reduced cytokine-induced morphological injury and better maintenance of nephrin localization relative to smooth controls. In Transwell co-culture with THP-1 reporter macrophages, podocytes conditioned on fractal substrates attenuated macrophage inflammatory signaling, reducing NF-κB and IRF activation compared with smooth-surface podocyte conditioning. Overall, the work establishes fractal topography as a tunable biophysical cue that improves podocyte phenotypic stability and dampens inflammatory crosstalk, providing a more physiologically relevant in vitro platform for studying inflammatory kidney disease mechanisms.

CELLSCALE INSTRUMENT USED

MicroTester

Elastic modulus testing of Matrigel-coated 3D printed IP-PDMS hemispheres (smooth and highest-fractality conditions) was performed using a CellScale MicroSquisher (now MicroTester) as a micromechanical compression/indentation platform. Samples were submerged in PBS during testing to prevent Matrigel drying and to maintain hydrated conditions. A manufacturer-supplied tungsten beam (30 mm length, 0.2032 mm diameter for hemispheres; 0.4064 mm for flat IP-PDMS) was used to apply controlled indentation at 1 µm/s. The probe was driven 50 µm into the submerged hemispheres, held for 5 s, and retracted 50 µm at 1 µm/s while recording force–displacement data. The beam–sample contact point was identified to generate force–displacement curves and extract an effective measured stiffness (k_meas) over a 10 µm indentation depth; sample stiffness (k_sample) was then computed using beam stiffness correction (k_beam reported as 1.9265 N/m). Elastic modulus was calculated using a Hertz spherical indentation model assuming Poisson’s ratio ν = 0.45 (to account for Matrigel) and a tip radius R = 100 µm, with n=5 independent samples used for statistical analysis. The resulting modulus (~20 kPa) supported that differences in cellular phenotype across groups were driven primarily by topographical fractality rather than bulk stiffness differences.
AUTHORS

Wang Y., Dikyol C., Wagner K.T., Landau S., Liu C., Okhovatian S., Bodenstein D.F., Vosoughi D., Zhao Y., Shen K., Shakeri A., Wu Q., Radisic M..

PUBLICATION DETAILS
JOURNAL

Cell Biomaterials

YEAR

2026

INSTITUTIONS

University of Toronto, Toronto General Research Institute, Terrence Donnelly Centre for Cellular & Biomolecular Research

COUNTRIES

Canada

INSTRUMENT USED

MicroTester

TESTING METHODS

Hydrated and Temperature Controlled TestingIndentation TestingMicro-Mechanical Testing

RESEARCH APPLICATIONS

Fibrosis & Tissue RemodelingMechanotransductionOrganoid and Tissue Mimetic Systems

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