Literature DB >> 9422981

A quantitative immunofluorescence study of glomerular cell adhesion proteins in proteinuric states.

R Bains1, P N Furness, D R Critchley.   

Abstract

Whenever there is heavy proteinuria, the glomerular epithelial cells, the podocytes, show dramatic morphological changes which clearly demonstrate changes in cell adhesion. However, there is little information on the types of cell adhesion molecules expressed in the normal human glomerulus. Assessments of changes in cell adhesion molecules in human proteinuria have been confined to semi-quantitative immunostaining for integrins, and the results have not been entirely consistent. This study sought first to define which cell adhesion molecules are present in the normal glomerulus, using indirect immunofluorescence and a panel of antibodies directed against transmembrane adhesion proteins and against several cytoplasmic proteins which are known to be involved in adhesion. A wide variety of integrins were detected, the dominant form being alpha 3 beta 1. The cytoplasmic focal adhesion proteins vinculin, talin, paxillin, p130CAS, and pp125FAK were detected, although vinculin appeared to be confined mainly to the mesangium. The only intercellular adhesion molecule detected in the vicinity of the slit diaphragm was ZO-1; the results imply that the slit diaphragm does not bear a close relationship to any other form of intercellular junction. Changes in these adhesion components were also studied in proteinuria, using 18 cases each of minimal change nephropathy, 'early' membranous nephropathy, and normal controls. Fluorescence intensity was measured by image capture using a low light video camera and subsequent digital image analysis, an approach which demonstrated acceptable reproducibility. The most striking changes were an increase in phosphotyrosine and p130CAS in the nephrotic patients. Contrary to previous reports, little change was found in the expression of the most abundant integrins, nor did overall glomerular staining for ZO-1 alter. These results imply a controlled alteration in glomerular cell adhesion in nephrotic states in man, probable representing increased turnover of cell adhesion structures rather than the decrease which has been reported in short-term animal models. This is the first report of increased glomerular phosphotyrosine in man, which is associated with less stable adhesions and may be related to the loss of foot processes. Using human biopsy material, it was not possible to determine which proteins were phosphorylated, but the probable relationships to changes in cytoskeletal structure and slit diaphragm permeability justify further study.

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Year:  1997        PMID: 9422981     DOI: 10.1002/(SICI)1096-9896(199711)183:3<272::AID-PATH914>3.0.CO;2-U

Source DB:  PubMed          Journal:  J Pathol        ISSN: 0022-3417            Impact factor:   7.996


  11 in total

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2.  Glomerular overexpression and increased tyrosine phosphorylation of focal adhesion kinase p125FAK in lupus-prone MRL/MP-lpr/lpr mice.

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4.  Inhibition of podocyte FAK protects against proteinuria and foot process effacement.

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Review 5.  Pathogenesis of proteinuria in idiopathic minimal change disease: molecular mechanisms.

Authors:  Gabriel Cara-Fuentes; William L Clapp; Richard J Johnson; Eduardo H Garin
Journal:  Pediatr Nephrol       Date:  2016-07-06       Impact factor: 3.714

Review 6.  Cell adhesion molecules in chemically-induced renal injury.

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7.  High-glucose and advanced glycosylation end products increased podocyte permeability via PI3-K/Akt signaling.

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Journal:  J Mol Med (Berl)       Date:  2010-01-08       Impact factor: 4.599

8.  Angiotensin II Modulates p130Cas of Podocytes by the Suppression of AMP-Activated Protein Kinase.

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9.  Puromycin aminonucleoside modulates p130Cas of podocytes.

Authors:  Tae-Sun Ha; Ji-Young Choi; Hye-Young Park
Journal:  Korean J Pediatr       Date:  2012-10-29

10.  Ginseng total saponin modulates podocyte p130Cas in diabetic condition.

Authors:  Tae-Sun Ha; Jin-Seok Lee; Ji-Young Choi; Hye-Young Park
Journal:  J Ginseng Res       Date:  2013-03       Impact factor: 6.060

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