Nephrin ectodomain engagement results in Src kinase activation, nephrin phosphorylation, Nck recruitment, and actin polymerization
Rakesh Verma, … , Kevin Patrie, Lawrence B. Holzman
Rakesh Verma, … , Kevin Patrie, Lawrence B. Holzman
Published May 1, 2006
Citation Information: J Clin Invest. 2006;116(5):1346-1359. https://doi.org/10.1172/JCI27414.
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Research Article Nephrology

Nephrin ectodomain engagement results in Src kinase activation, nephrin phosphorylation, Nck recruitment, and actin polymerization

Abstract

A properly established and maintained podocyte intercellular junction, or slit diaphragm, is a necessary component of the selective permeability barrier of the kidney glomerulus. The observation that mutation or deletion of the slit diaphragm transmembrane protein nephrin results in failure of podocyte foot process morphogenesis and concomitant proteinuria first suggested the hypothesis that nephrin serves as a component of a signaling complex that directly integrates podocyte junctional integrity with cytoskeletal dynamics. The observations made herein provide the first direct evidence to our knowledge for a phosphorylation-mediated signaling mechanism by which this integrative function is derived. Our data support the model that during podocyte intercellular junction formation, engagement of the nephrin ectodomain induces transient Fyn catalytic activity that results in nephrin phosphorylation on specific nephrin cytoplasmic domain tyrosine residues. We found that this nephrin phosphorylation event resulted in recruitment of the SH2–SH3 domain–containing adapter protein Nck and assembly of actin filaments in an Nck-dependent fashion. Considered in the context of the role of nephrin family proteins in other organisms and the integral relationship of actin dynamics and junction formation, these observations establish a function for nephrin in regulating actin cytoskeletal dynamics.

Authors

Rakesh Verma, Iulia Kovari, Abdul Soofi, Deepak Nihalani, Kevin Patrie, Lawrence B. Holzman

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Figure 6

Nck associates with nephrin.

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Nck associates with nephrin. GST-nephrinCD or its Y1208 mutant was expre...
GST-nephrinCD or its Y1208 mutant was expressed in BL21 or TKB1 E. coli and was affinity purified on glutathione agarose. (A) Immunoblotting with P-nephrin or nonspecific PY antibody demonstrated that expression in TKB1 (but not BL21) cells resulted in phosphorylation on Y1208 and other nephrin tyrosine residues. (B) Purified recombinant GST alone or GST-nephrinCD obtained from either BL21 or TKB1 cells that was bound to glutathione agarose was incubated with isolated mouse glomerular lysate. Washed beads were eluted with glutathione. Eluate was resolved by SDS-PAGE and immunoblotted with the panel of antibodies shown in Table 2. Representative immunoblot was obtained using a pan-Nck antibody that demonstrated association of Nck with tyrosine-phosphorylated wild-type GST-nephrinCD but not unphosphorylated GST-nephrinCD or GST alone.