Redox Metabolism and Vascular Calcification in Chronic Kidney Disease.
Natalia Carrillo-LópezSara PanizoBeatriz Martín-CarroJuan Carlos MayoPablo Román-GarcíaRaúl García-CastroJesús María Fernández-GómezMiguel Ángel Hevia-SuárezJulia Martín-VírgalaSara Fernández-VillabrilleLaura Martínez-AriasSara Barrio VázquezLaura Calleros BasilioManuel Naves-DíazJorge Benito Cannata-AndíaIsabel Quirós-GonzálezCristina Alonso-MontesJosé Luis Fernández-MartínPublished in: Biomolecules (2023)
Vascular calcification (VC) is a common complication in patients with chronic kidney disease which increases their mortality. Although oxidative stress is involved in the onset and progression of this disorder, the specific role of some of the main redox regulators, such as catalase, the main scavenger of H 2 O 2 , remains unclear. In the present study, epigastric arteries of kidney transplant recipients, a rat model of VC, and an in vitro model of VC exhibiting catalase (Cts) overexpression were analysed. Pericalcified areas of human epigastric arteries had increased levels of catalase and cytoplasmic, rather than nuclear runt-related transcription factor 2 (RUNX2). In the rat model, advanced aortic VC concurred with lower levels of the H 2 O 2 -scavenger glutathione peroxidase 3 compared to controls. In an early model of calcification using vascular smooth muscle cells (VSMCs), Cts VSMCs showed the expected increase in total levels of RUNX2. However, Cts VMSCs also exhibited a lower percentage of the nucleus stained for RUNX2 in response to calcifying media. In this early model of VC, we did not observe a dysregulation of the mitochondrial redox state; instead, an increase in the general redox state was observed in the cytoplasm. These results highlight the complex role of antioxidant enzymes as catalase by regulation of RUNX2 subcellular location delaying the onset of VC.
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