Metabolism of hydrogen sulfide (H(2)S) and Production of Reactive Sulfur Species (RSS) by superoxide dismutase

Reactive sulfur species (RSS) such as H(2)S, HS(•), H(2)S(n), (n = 2–7) and HS(2)(•-) are chemically similar to H(2)O and the reactive oxygen species (ROS) HO(•), H(2)O(2), O(2)(•-) and act on common biological effectors. RSS were present in evolution long before ROS, and because both are metabolize...

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Detalles Bibliográficos
Autores principales: Olson, Kenneth R., Gao, Yan, Arif, Faihaan, Arora, Kanika, Patel, Shivali, DeLeon, Eric. R., Sutton, Thomas R., Feelisch, Martin, Cortese-Krott, Miriam M., Straub, Karl D.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier 2017
Materias:
Research Paper
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5725220/
https://www.ncbi.nlm.nih.gov/pubmed/29220697
http://dx.doi.org/10.1016/j.redox.2017.11.009
Descripción
Sumario:Reactive sulfur species (RSS) such as H(2)S, HS(•), H(2)S(n), (n = 2–7) and HS(2)(•-) are chemically similar to H(2)O and the reactive oxygen species (ROS) HO(•), H(2)O(2), O(2)(•-) and act on common biological effectors. RSS were present in evolution long before ROS, and because both are metabolized by catalase it has been suggested that “antioxidant” enzymes originally evolved to regulate RSS and may continue to do so today. Here we examined RSS metabolism by Cu/Zn superoxide dismutase (SOD) using amperometric electrodes for dissolved H(2)S, a polysulfide-specific fluorescent probe (SSP4), and mass spectrometry to identify specific polysulfides (H(2)S(2)-H(2)S(5)). H(2)S was concentration- and oxygen-dependently oxidized by 1 μM SOD to polysulfides (mainly H(2)S(2), and to a lesser extent H(2)S(3) and H(2)S(5)) with an EC(50) of approximately 380 μM H(2)S. H(2)S concentrations > 750 μM inhibited SOD oxidation (IC(50) = 1.25 mM) with complete inhibition when H(2)S > 1.75 mM. Polysulfides were not metabolized by SOD. SOD oxidation preferred dissolved H(2)S over hydrosulfide anion (HS(-)), whereas HS(-) inhibited polysulfide production. In hypoxia, other possible electron donors such as nitrate, nitrite, sulfite, sulfate, thiosulfate and metabisulfite were ineffective. Manganese SOD also catalyzed H(2)S oxidation to form polysulfides, but did not metabolize polysulfides indicating common attributes of these SODs. These experiments suggest that, unlike the well-known SOD-mediated dismutation of two O(2)(•-) to form H(2)O(2) and O(2)((,)) SOD catalyzes a reaction using H(2)S and O(2) to form persulfide. These can then combine in various ways to form polysulfides and sulfur oxides. It is also possible that H(2)S (or polysulfides) interact/react with SOD cysteines to affect catalytic activity or to directly contribute to sulfide metabolism. Our studies suggest that H(2)S metabolism by SOD may have been an ancient mechanism to detoxify sulfide or to regulate RSS and along with catalase may continue to do so in contemporary organisms.

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