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"Faces" of the day:

Katharina Jandl

Nina Höller

Nariae Baik-Schneditz

Ellen Heitzer

Marianne Brodmann

Ewald Kolesnik

Bernhard Schwaberger

Maximilian Seles

Gabor Toth-Gayor

Lukas Peter Mileder

Niels Hammer

Christian Josef Hill

Christian Viertler

Philipp Klaritsch

Daniel Scherr

Harald Köfeler

Gerhard Pichler

Roland Malli

Michael Fuchsjäger

Gernot Plank

Peter Fickert

Richard Zigeuner

Peter Holzer

Selected Publication:

SHR Neuro Cancer Cardio Lipid Metab Microb

Degendorfer, G; Chuang, CY; Hammer, A; Malle, E; Davies, MJ.
Peroxynitrous acid induces structural and functional modifications to basement membranes and its key component, laminin.
Free Radic Biol Med. 2015; 89(48):721-733 Doi: 10.1016/j.freeradbiomed.2015.09.018
Web of Science PubMed FullText FullText_MUG

 

Co-authors Med Uni Graz

Hammer Astrid

Malle Ernst

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Abstract:

Basement membranes (BM) are specialized extracellular matrices underlying endothelial cells in the artery wall. Laminin, the most abundant BM glycoprotein, is a structural and biologically active component. Peroxynitrous acid (ONOOH), a potent oxidizing and nitrating agent, is formed in vivo at sites of inflammation from superoxide and nitric oxide radicals. Considerable data supports ONOOH formation in human atherosclerotic lesions, and an involvement of this oxidant in atherosclerosis development and lesion rupture. These effects may be mediated, at least in part, via extracellular matrix damage. In this study we demonstrate co-localization of 3-nitrotyrosine (a product of tyrosine damage by ONOOH) and laminin in human atherosclerotic lesions. ONOOH-induced damage to BM was characterized for isolated murine BM, and purified murine laminin-111. Exposure of laminin-111 to ONOOH resulted in dose-dependent loss of protein tyrosine and tryptophan residues, and formation of 3-nitrotyrosine, 6-nitrotryptophan and the cross-linked material di-tyrosine, as detected by amino acid analysis and Western blotting. These changes were accompanied by protein aggregation and fragmentation as detected by SDS-PAGE. Endothelial cell adhesion to isolated laminin-111 exposed to 10 μM or higher levels of ONOOH was significantly decreased (~25%) compared to untreated controls. These data indicate that laminin is oxidized by equimolar or greater concentrations of ONOOH, with this resulting in structural and functional changes. These modifications, and resulting compromised cell-matrix interactions, may contribute to endothelial cell dysfunction, a weakening of the structure of atherosclerotic lesions, and an increased propensity to rupture. Copyright © 2015 Elsevier Inc. All rights reserved.

Find related publications in this database (using NLM MeSH Indexing)

Animals -

Atherosclerosis - metabolism

Atherosclerosis - pathology

Basement Membrane - pathology

Blotting, Western -

Cells, Cultured -

Chromatography, High Pressure Liquid -

Electrophoresis, Polyacrylamide Gel -

Endothelium, Vascular - metabolism

Endothelium, Vascular - pathology

Enzyme-Linked Immunosorbent Assay -

Extracellular Matrix -

Humans -

Immunohistochemistry -

Laminin - metabolism

Mice -

Microscopy, Confocal -

Oxidants - metabolism

Oxidants - pharmacology

Oxidation-Reduction -

Peroxynitrous Acid - metabolism

Peroxynitrous Acid - pharmacology

Find related publications in this database (Keywords)

Extracellular matrix

Peroxynitrous acid

Laminin

Protein oxidation

Endothelial cells

3-nitrotyrosine

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