Showing papers by "Rafael Radi published in 2023"
TL;DR: In this article , the Ser/Thr phosphatase calcineurin was identified as a new target of nitroalkylation by nitro-oleic acid, which reduced the transcriptional activity of NFAT and modulated pro-inflammatory cytokine production by activated T cells.
Abstract: Significance In addition to maintaining the fluidity of the plasma membrane, some unsaturated fatty acids are involved in signal transduction. Inflammatory environments enhance the reaction of these lipids with nitrogen-derived reactive species to form electrophilic nitro-fatty acids (NO2-FAs) that display increased reactivity toward cellular nucleophiles. By selective nitroalkylation of Cys residues on key signaling regulatory proteins, NO2-FAs exert effective anti-inflammatory actions in some preclinical animal models of autoimmunity and allergy. Here we have identified the Ser/Thr phosphatase calcineurin as a new target of nitroalkylation by nitro-oleic acid. The nitroalkylation of calcineurin on Cys372 reduces the transcriptional activity of NFAT and modulates pro-inflammatory cytokine production by activated T cells. Our results underscore how NO2-FAs may control T cell-mediated immune responses.
1 citations
TL;DR: In this paper , the authors performed an in-depth analysis of human Glutamine Synthetase (GS) in vitro and found that ONOO- exposure led to a dose-dependent loss of HsGS activity, the oxidation of cysteine, methionine, and tyrosine residues and also the nitration of tryptophan.
1 citations
TL;DR: In this article , it was shown that inactivation by hydrogen peroxide is strongly enhanced in the presence of carbon dioxide/bicarbonate, which is most likely responsible for the enhanced inactivation.
Abstract: Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) contains an active site Cys and is one of the most sensitive cellular enzymes to oxidative inactivation and redox regulation. Here, we show that inactivation by hydrogen peroxide is strongly enhanced in the presence of carbon dioxide/bicarbonate. Inactivation of isolated mammalian GAPDH by H2O2 increased with increasing bicarbonate concentration and was sevenfold faster in 25 mM (physiological) bicarbonate compared with bicarbonate-free buffer of the same pH. H2O2 reacts reversibly with CO2 to form a more reactive oxidant, peroxymonocarbonate (HCO4-), which is most likely responsible for the enhanced inactivation. However, to account for the extent of enhancement, we propose that GAPDH must facilitate formation and/or targeting of HCO4- to promote its own inactivation. Inactivation of intracellular GAPDH was also strongly enhanced by bicarbonate: treatment of Jurkat cells with 20 µM H2O2 in 25 mM bicarbonate buffer for 5 min caused almost complete GAPDH inactivation, but no loss of activity when bicarbonate was not present. H2O2-dependent GAPDH inhibition in bicarbonate buffer was observed even in the presence of reduced peroxiredoxin 2 and there was a significant increase in cellular glyceraldehyde-3-phosphate/dihydroxyacetone phosphate. Our results identify an unrecognized role for bicarbonate in enabling H2O2 to influence inactivation of GAPDH and potentially reroute glucose metabolism from glycolysis to the pentose phosphate pathway and NAPDH production. They also demonstrate what could be wider interplay between CO2 and H2O2 in redox biology and the potential for variations in CO2 metabolism to influence oxidative responses and redox signaling.
1 citations
TL;DR: In this paper , it was shown that HsPrx3 is oxidized and hyperoxidized by fFA-OOHs including those derived from arachidonic acid and eicosapentaenoic acid peroxidation at position 15.
Abstract: Human peroxiredoxin 3 (HsPrx3) is a thiol-based peroxidase responsible for the reduction of most hydrogen peroxide and peroxynitrite formed in mitochondria. Mitochondrial disfunction can lead to membrane lipoperoxidation, resulting in the formation of lipid-bound fatty acid hydroperoxides (LFA-OOHs) which can be released to become free fatty acid hydroperoxides (fFA-OOHs). Herein, we report that HsPrx3 is oxidized and hyperoxidized by fFA-OOHs including those derived from arachidonic acid and eicosapentaenoic acid peroxidation at position 15 with remarkably high rate constants of oxidation (>3.5 × 107 M−1s−1) and hyperoxidation (~2 × 107 M−1s−1). The endoperoxide-hydroperoxide PGG2, an intermediate in prostanoid synthesis, oxidized HsPrx3 with a similar rate constant, but was less effective in causing hyperoxidation. Biophysical methodologies suggest that HsPrx3 can bind hydrophobic structures. Indeed, molecular dynamic simulations allowed the identification of a hydrophobic patch near the enzyme active site that can allocate the hydroperoxide group of fFA-OOHs in close proximity to the thiolate in the peroxidatic cysteine. Simulations performed using available and herein reported kinetic data indicate that HsPrx3 should be considered a main target for mitochondrial fFA-OOHs. Finally, kinetic simulation analysis support that mitochondrial fFA-OOHs formation fluxes in the range of nM/s are expected to contribute to HsPrx3 hyperoxidation, a modification that has been detected in vivo under physiological and pathological conditions.
1 citations