Please use this identifier to cite or link to this item: http://dr.iiserpune.ac.in:8080/xmlui/handle/123456789/6258
Title: Redox Biochemistry of Hydrogen Sulfide Biogenesis and Oxidation
Other Titles: Hydrogen Sulfide induced reverse electron transfer
Authors: Banerjee, Ruma
GUHA, ARKAJIT
Dept. of Chemistry
20161054
Keywords: Hydrogen Sulfide
Reverse Electron Transfer
Issue Date: Jul-2021
Citation: 42
Abstract: Hydrogen sulfide (H2S) is a gaseous molecule which can act as an inorganic substrate for energy production. On the other hand, high concentrations of H2S can act as a poison by inhibiting cellular respiration, but the mechanism of H2S clearance when respiration is inhibited is unclear. Sulfide quinone oxidoreductase (SQOR) catalyzes the initial step of the mitochondrial sulfide oxidation pathway by oxidizing H2S to a persulfide and transferring the electrons to coenzyme Q (CoQ). In this study, we have investigated how competition between SQOR and other enzymes for use of the CoQ pool modulates the capacity for H2S clearance. Monitoring the oxygen consumption rate by the electron transport chain, we found that cells with compromised complex I or complex II activity exhibit enhanced or decreased ability to clear H2S, respectively, suggesting that both complexes are significant modulators of SQOR activity. When complex IV-dependent respiration was inhibited, complex II was found to work in reverse, oxidizing CoQH2 to CoQ by using fumarate as an alternate electron acceptor and increasing sulfide oxidation capacity. We also demonstrated that the malate aspartate shuttle plays an important role in providing fumarate to sustain SQOR activity under these conditions. Complex II-dependent SQOR activity could be a mechanism by which H2S acts as a protective agent during reperfusion following ischemia, attenuating injury. In related studies, we investigated an altered response to H2S following knock down of persulfide dioxygenase (ETHE1), the second enzyme in the mitochondrial sulfide oxidation pathway. Finally, modulation of cystathionine beta synthase activity by select metabolites was probed
URI: http://dr.iiserpune.ac.in:8080/xmlui/handle/123456789/6258
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