Role of integrin-linked kinase in epithelial-mesenchymal transition in crescent formation of experimental glomerulonephritis

doi:10.1093/ndt/gfl243

NDT Advance Access published online on May 25, 2006
Nephrology Dialysis Transplantation, doi:10.1093/ndt/gfl243

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© The Author [2006]. Published by Oxford University Press on behalf of ERA-EDTA. All rights reserved. For Permissions, please email: journals.permissions@oxfordjournals.org
Received September 14, 2005
Accepted April 5, 2006

Original Article

Role of integrin-linked kinase in epithelial-mesenchymal transition in crescent formation of experimental glomerulonephritis

Maki Shimizu ¹, Shuji Kondo ¹, Maki Urushihara ¹, Masanori Takamatsu ¹, Katsuyoshi Kanemoto ², Michio Nagata ², and Shoji Kagami ¹ ^*

¹ Department of Pediatrics, The Institute of Health Bioscience, The University of Tokushima Graduate School, Tokushima, Japan
² Department of Molecular Pathology, Graduate School of Comprehensive Human Sciences, University of Tsukuba, Tsukuba, Japan

^* To whom correspondence should be addressed.
Shoji Kagami, E-mail: kagami{at}clin.med.tokushima-u.ac.jp

Abstract

Background. Glomerular parietal epithelial-mesenchymal transition(EMT) is a key event in crescent formation of glomerulonephritis(GN). Integrin-linked kinase (ILK) is an integrin cytoplasmic-bindingprotein that has been implicated in the regulation of cell adhesion,extracellular matrix organization and EMT. Transforming growthfactor- ${beta}$ (TGF- ${beta}$ ) is involved in the induction and progressionof EMT in several tissues.

Methods. To investigate whether ILKis involved in the crescent formation in GN, we studied theexpression of ILK protein and activity in crescentic GN inducedin Wistar Kyoto (WKY) rats. In addition, we investigated whethertransforming growth factor- ${beta}$ 1 (TGF- ${beta}$ 1) could induce glomerularEMT and ILK by using cultured parietal epithelial cell (PEC).

Results.The expression of ILK was strongly induced in cellular crescentsat day 7 and followed by a decrease in fibrocellular crescentsat day 28. ILK-expressing cells in cellular crescents were double-positivefor protein gene product 9.5 (PEC marker), ${alpha}$ -smooth muscle actin( ${alpha}$ -SMA, myofibroblasts marker) and TGF- ${beta}$ 1, indicating a possiblecontribution of ILK and TGF- ${beta}$ 1 to EMT in crescent formation inGN. Consistent with the finding of histological ILK expressionin crescents, western blot and kinase activity assay showedan increase in both ILK protein and activity, peaking at day7 of GN (3.7- and 3.5-fold of control, respectively). The expressionof ILK increased to 3.1-fold of control when EMT was inducedin cultured PEC by TGF- ${beta}$ 1.

Conclusion. The present results providethe first evidence that expression and activity of ILK are increasedin cellular crescents of experimental GN. Enhanced expressionand activity of ILK, possibly by TGF- ${beta}$ 1, is associated with theinduction of EMT by PEC and thereby, may participate in theformation of cellular crescents in GN.

Keywords: crescent formation; epithelial-mesenchymal transition; integrin-linked kinase.

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