A novel pathway for the production of hydrogen sulfide from D-cysteine in mammalian cells

Shibuya, Norihiro; Koike, Sachiko; Tanaka, Masataka; Ishigami‐Yuasa, Mari; Kimura, Yoshinobu; Ogasawara, Yuki; Fukui, Kiyoshi; Nagahara, Noriyuki; Kimura, Hideo

doi:10.1038/ncomms2371

Cited by 485 publications

(405 citation statements)

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“…Intracellular levels of bound sulfur were measured using a previously described method [21]. Briefly, N2A cells treated with Na 2 S 4 were washed with ice-cold phosphate-buffered saline (PBS) and resuspended in lysis buffer [10 mM potassium phosphate buffer (pH 7.4), 0.5% Triton X-100, protease inhibitor cocktail complete (EDTA free, Roche Applied Science, Darmstadt, Germany), 10 mM hydroxylamine, and 10 mM benzoic acid].…”

Section: Determination Of Bound Sulfurmentioning

confidence: 99%

Polysulfide exerts a protective effect against cytotoxicity caused by t‐buthylhydroperoxide through Nrf2 signaling in neuroblastoma cells

et al. 2013

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a b s t r a c tPolysulfide is a bound sulfur species derived from endogenous H 2 S. When mouse neuroblastoma, Neuro2A cells were exposed to tert-butyl hydroperoxide after treatment with polysulfide, a significant decline in cell toxicity was observed. Rapid uptake of polysulfides induced translocation of Nrf2 into the nucleus, resulting in acceleration of GSH synthesis and HO-1 expression. We demonstrated that polysulfide reversibly modified Keap1 to form oxidized dimers and induced the translocation of Nrf2. Moreover, polysulfide treatment accelerated Akt phosphorylation, which is a known pathway of Nrf2 phosphorylation. Thus, polysulfide may mediate the activation of Nrf2 signaling, thereby exerting protective effects against oxidative damage in Neuro2A cells.

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Section: Determination Of Bound Sulfurmentioning

confidence: 99%

Polysulfide exerts a protective effect against cytotoxicity caused by t‐buthylhydroperoxide through Nrf2 signaling in neuroblastoma cells

et al. 2013

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“…Kimura has proposed a D-Cys-dependent H 2 S biogenesis as a possible new pathway for H 2 S production in living mammalian cells 12 . Our newly developed FRET-based ratiometric probes have been tested to visualize this new H 2 S biogenesis in situ in living cells.…”

Section: Discussionmentioning

confidence: 99%

“…Recently, they further reported a novel possible pathway for the production of H 2 S from D-cysteine in mammalian cells 12 . As new biogenesis and biological functions of H 2 S continue to emerge [12][13][14][15] , new biocompatible tools to selectively visualize cellular H 2 S in real-time at its site of release are urgently needed 11 .Fluorescent probes could be used for H 2 S detection in a non-invasive manner in living systems [13][14][15][16][17] . The probebased tools have been successfully used to image endogenous H 2 S production from thiol substrates including LCys and glutathione (GSH) 13 or by vascular endothelial growth factor stimulation 17 .…”

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FRET ratiometric probes reveal the chiral-sensitive cysteine-dependent H2S production and regulation in living cells

Song

et al. 2014

Sci Rep

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Hydrogen sulfide (H 2 S) is an endogenously produced gaseous signalling molecule with multiple biological functions. In order to visualize and quantify the endogenous in situ production of H 2 S in living cells, here we developed two new sulphide ratiometric probes (SR400 and SR550) based on fluorescence resonance energy transfer (FRET) strategy for live capture of H 2 S. The FRET-based probes show excellent selectivity toward H 2 S in a high thiol background under physiological buffer. The probe can be used to in situ visualize cysteine-dependent H 2 S production in a chiral-sensitive manner in living cells. The ratiometric imaging studies indicated that D-Cys induces more H 2 S production than that of L-Cys in mitochondria of human embryonic kidney 293 cells (HEK293). The cysteine mimics propargylglycine (PPG) has also been found to inhibit the cysteine-dependent endogenous H 2 S production in a chiral-sensitive manner in living cells. D-PPG inhibited D-Cys-dependent H 2 S production more efficiently than L-PPG, while, L-PPG inhibited L-Cys-dependent H 2 S production more efficiently than D-PPG. Our bioimaging studies support Kimura's discovery of H 2 S production from D-cysteine in mammalian cells and further highlight the potential of D-cysteine and its derivatives as an alternative strategy for classical H 2 S-releasing drugs.H ydrogen sulfide (H 2 S) is an important endogenous signalling molecule along with nitric oxide (NO) and carbon monoxide (CO) 1-3 . H 2 S has also been demonstrated to exert protective effects such as preservation of mitochondrial function, protection of neurons from oxidative stress, inhibition of apoptosis, intervention of neuronal transmission, regulation of inflammation, stimulation of angiogenesis, reduce blood pressure, etc 4-7 . The deregulation of endogenous H 2 S is correlated with the symptoms of Alzheimer's disease, Down syndrome, diabetes and liver cirrhosis [8][9][10] . Kimura et al. indicated that H 2 S is enzymatic generated from L-cysteine (L-Cys) and its derivatives in vivo 7,11 . Recently, they further reported a novel possible pathway for the production of H 2 S from D-cysteine in mammalian cells 12 . As new biogenesis and biological functions of H 2 S continue to emerge [12][13][14][15] , new biocompatible tools to selectively visualize cellular H 2 S in real-time at its site of release are urgently needed 11 .Fluorescent probes could be used for H 2 S detection in a non-invasive manner in living systems [13][14][15][16][17] . The probebased tools have been successfully used to image endogenous H 2 S production from thiol substrates including LCys and glutathione (GSH) 13 or by vascular endothelial growth factor stimulation 17 . Inspired by these work 13,17 , we are interested to image endogenous H 2 S production of all possible pathways in living cells semi-quantitatively or quantitatively, based on ratiometric probes rather than intensity-based probes, in view of that ratiometric measurements can cancel out variability caused by uneven loading and distribution of...

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“…3-MST, along with cysteine aminotransferase (CAT) or D-amino acid oxidase (DAO), produces H 2 S from cysteine and α-ketoglutarate in the mitochondria [11,12]. 3-MST/CAT is localized in thoracic aorta ECs and produces H 2 S [13]; however, a vascular effect of 3-MST/CATderived H 2 S is unknown.…”

Section: Introductionmentioning

confidence: 99%

H2S in the Vasculature: Controversy of Mechanisms in Physiology, Pathology and Beyond

Beyer¹

2015

Cardiol Pharmacol

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Hydrogen sulfide (H 2 S) is an endogenously gaseous messenger with a number of physiological effects. Pharmacological and genetic models point toward an important role for this vasodilator gas in the regulation of vascular tone, cardiac response to ischemia/reperfusion injury, and inflammation among others. Understanding the complex interaction of H 2 S with basic cellular signaling and its impact on endothelial and smooth muscle physiology may provide insights into the early stages of developing vascular inflammation and atherosclerosis or related vascular pathologies. The underlying mechanism of action is not completely understood. Recent evidence suggests a key role of H 2 S in protecting mitochondria against oxidative damage, regulation of ion channels and modulation of eNOS activity. This review will focus on the key role of H 2 S in the regulation of vascular function including free radical production and its physiological role in health and disease.

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A novel pathway for the production of hydrogen sulfide from D-cysteine in mammalian cells

Cited by 485 publications

References 40 publications

Polysulfide exerts a protective effect against cytotoxicity caused by t‐buthylhydroperoxide through Nrf2 signaling in neuroblastoma cells

Polysulfide exerts a protective effect against cytotoxicity caused by t‐buthylhydroperoxide through Nrf2 signaling in neuroblastoma cells

FRET ratiometric probes reveal the chiral-sensitive cysteine-dependent H2S production and regulation in living cells

H2S in the Vasculature: Controversy of Mechanisms in Physiology, Pathology and Beyond

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