WT1-interacting protein (Wtip) regulates podocyte phenotype by cell-cell and cell-matrix contact reorganization

Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions. Wt1-interacting protein (Wtip), an Ajuba family LIM domain scaffold protein expressed in the podocyte, coordinates cell adhesion changes and transcriptional responses to regulate podocyte...

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Published in:American journal of physiology. Renal physiology 2012-01, Vol.302 (1), p.F103-F115
Main Authors: Kim, Jane H, Mukherjee, Amitava, Madhavan, Sethu M, Konieczkowski, Martha, Sedor, John R
Format: Article
Language:English
Subjects:
Actins - metabolism
Adherens Junctions - metabolism
alpha Catenin - metabolism
Animals
Apoptosis Regulatory Proteins - physiology
beta Catenin - metabolism
Cadherins - metabolism
Cell adhesion & migration
Cell Adhesion - genetics
Cell Adhesion - physiology
Focal Adhesions - metabolism
Gene expression
Genotype & phenotype
Guanine Nucleotide Exchange Factors - metabolism
Humans
Kidneys
Mice
Phenotype
Podocytes - cytology
Podocytes - metabolism
Proteins
Proto-Oncogene Proteins - metabolism
Rho Guanine Nucleotide Exchange Factors
rhoA GTP-Binding Protein - metabolism
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Summary:Podocytes respond to environmental cues by remodeling their slit diaphragms and cell-matrix adhesive junctions. Wt1-interacting protein (Wtip), an Ajuba family LIM domain scaffold protein expressed in the podocyte, coordinates cell adhesion changes and transcriptional responses to regulate podocyte phenotypic plasticity. We evaluated effects of Wtip on podocyte cell-cell and cell-matrix contact organization using gain-of- and loss-of-function methods. Endogenous Wtip targeted to focal adhesions in adherent but isolated podocytes and then shifted to adherens junctions after cells made stable, homotypic contacts. Podocytes with Wtip knockdown (shWtip) adhered but failed to spread normally. Noncontacted shWtip podocytes did not assemble actin stress fibers, and their focal adhesions failed to mature. As shWtip podocytes established cell-cell contacts, stable adherens junctions failed to form and F-actin structures were disordered. In shWtip cells, cadherin and β-catenin clustered in irregularly distributed spots that failed to laterally expand. Cell surface biotinylation showed diminished plasma membrane cadherin, β-catenin, and α-catenin in shWtip podocytes, although protein expression was similar in shWtip and control cells. Since normal actin dynamics are required for organization of adherens junctions and focal adhesions, we determined whether Wtip regulates F-actin assembly. Undifferentiated podocytes did not elaborate F-actin stress fibers, but when induced to overexpress WTIP, formed abundant stress fibers, a process blocked by the RhoA inhibitor C3 toxin and a RhoA kinase inhibitor. WTIP directly interacted with Rho guanine nucleotide exchange factor (GEF) 12 (Arhgef12), a RhoA-specific GEF enriched in the glomerulus. In conclusion, stable assembly of podocyte adherens junctions and cell-matrix contacts requires Wtip, a process that may be mediated by spatiotemporal regulation of RhoA activity through appropriate targeting of Arhgef12.
ISSN:1931-857X
1522-1466
DOI:10.1152/ajprenal.00419.2011