Abstract
Hydrogen peroxide (H2O2) is a key redox signaling molecule that selectively oxidizes cysteines on proteins. It can accomplish this even in the presence of highly efficient and abundant H2O2 scavengers, peroxiredoxins (Prdxs), as it is the Prdxs themselves that transfer oxidative equivalents to specific protein thiols on target proteins via their redox-relay functionality. The first evidence of a mammalian cytosolic Prdx-mediated redox-relay—Prdx1 with the kinase ASK1—was presented a decade ago based on the outcome of a co-immunoprecipitation experiment. A second such redox-relay—Prdx2:STAT3—soon followed, for which further studies provided insights into its specificity, organization, and mechanism. The Prdx1:ASK1 redox-relay, however, has never undergone such a characterization. Here, we combine cellular and in vitro protein–protein interaction methods to investigate the Prdx1:ASK1 interaction more thoroughly. We show that, contrary to the Prdx2:STAT3 redox-relay, Prdx1 interacts with ASK1 at elevated H2O2 concentrations, and that this interaction can happen independently of a scaffolding protein. We also provide evidence of a Prdx2:ASK1 interaction, and demonstrate that it requires a facilitator that, however, is not annexin A2. Our results reveal that cytosolic Prdx redox-relays can be organized in different ways and yet again highlight the differentiated roles of Prdx1 and Prdx2.
Highlights
Hydrogen peroxide (H2 O2 ) is a major reactive oxygen species (ROS) that acts as an intracellular signaling molecule by selective oxidation of cysteines on proteins
The first aim of this study was to confirm the Prdx1:apoptosis signal-regulating kinase 1 (ASK1) interaction reported by Jarvis et al (2012) [14] where the interaction was detected by co-immunoprecipitation on cell lysates
Even though it has been reported that the central regulatory region of ASK1 can serve as a recruitment platform for ASK1 substrates [52], our in vitro results clearly show that the TBD domain alone is sufficient for the Prdx1:ASK1 interaction, ruling out the requirement of another domain of ASK1 acting as a scaffolding protein
Summary
Hydrogen peroxide (H2 O2 ) is a major reactive oxygen species (ROS) that acts as an intracellular signaling molecule by selective oxidation of cysteines on proteins. Prdxs scavenge H2 O2 through the formation of a sulfenic acid (Cys-SOH) on the peroxidatic cysteine (CysP ) with the subsequent formation of a disulfide bond between CysP and the resolving cysteine (CysR ) [8], and are recycled via the thioredoxin pathway (Trx-TrxR-NADPH) [9]. This super-scavenging activity is due to Antioxidants 2021, 10, 1060.
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