| Literature DB >> 27816420 |
Vijay Tejwani1, Franz-Josef Schmitt2, Svea Wilkening2, Ingo Zebger2, Marius Horch2, Oliver Lenz2, Thomas Friedrich3.
Abstract
Ralstonia eutropha is a hydrogen-oxidizing ("Knallgas") bacterium that can easily switch between heterotrophic and autotrophic metabolism to thrive in aerobic and anaerobic environments. Its versatile metabolism makes R. eutropha an attractive host for biotechnological applications, including H2-driven production of biodegradable polymers and hydrocarbons. H2 oxidation by R. eutropha takes place in the presence of O2 and is mediated by four hydrogenases, which represent ideal model systems for both biohydrogen production and H2 utilization. The so-called soluble hydrogenase (SH) couples reversibly H2 oxidation with the reduction of NAD+ to NADH and has already been applied successfully in vitro and in vivo for cofactor regeneration. Thus, the interaction of the SH with the cellular NADH/NAD+ pool is of major interest. In this work, we applied the fluorescent biosensor Peredox to measure the [NADH]:[NAD+] ratio in R. eutropha cells under different metabolic conditions. The results suggest that the sensor operates close to saturation level, indicating a rather high [NADH]:[NAD+] ratio in aerobically grown R. eutropha cells. Furthermore, we demonstrate that multicomponent analysis of spectrally-resolved fluorescence lifetime data of the Peredox sensor response to different [NADH]:[NAD+] ratios represents a novel and sensitive tool to determine the redox state of cells. Copyright ÂEntities:
Keywords: Decay-associated spectra; Fluorescence lifetime; Fluorescence sensor protein; Hydrogenase; NADH:NAD(+) ratio; Ralstonia eutropha
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Year: 2016 PMID: 27816420 DOI: 10.1016/j.bbabio.2016.11.001
Source DB: PubMed Journal: Biochim Biophys Acta Bioenerg ISSN: 0005-2728 Impact factor: 3.991