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Open AccessJournal ArticleDOI

The two isoenzymes for yeast NAD+-dependent glycerol 3-phosphate dehydrogenase encoded by GPD1 and GPD2 have distinct roles in osmoadaptation and redox regulation

TLDR
It is concluded that expression of GPD2 is controlled by a novel, oxygen‐independent, signalling pathway which is required to regulate metabolism under anoxic conditions.
Abstract
The two homologous genes GPD1 and GPD2 encode the isoenzymes of NAD-dependent glycerol 3-phosphate dehydrogenase in the yeast Saccharomyces cerevisiae. Previous studies showed that GPD1 plays a role in osmoadaptation since its expression is induced by osmotic stress and gpd1 delta mutants are osmosensitive. Here we report that GPD2 has an entirely different physiological role. Expression of GPD2 is not affected by changes in external osmolarity, but is stimulated by anoxic conditions. Mutants lacking GPD2 show poor growth under anaerobic conditions. Mutants deleted for both GPD1 and GPD2 do not produce detectable glycerol, are highly osmosensitive and fail to grow under anoxic conditions. This growth inhibition, which is accompanied by a strong intracellular accumulation of NADH, is relieved by external addition of acetaldehyde, an effective oxidizer of NADH. Thus, glycerol formation is strictly required as a redox sink for excess cytosolic NADH during anaerobic metabolism. The anaerobic induction of GPD2 is independent of the HOG pathway which controls the osmotic induction of GPD1. Expression of GPD2 is also unaffected by ROX1 and ROX3, encoding putative regulators of hypoxic and stress-controlled gene expression. In addition, GPD2 is induced under aerobic conditions by the addition of bisulfite which causes NADH accumulation by inhibiting the final, reductive step in ethanol fermentation and this induction is reversed by addition of acetaldehyde. We conclude that expression of GPD2 is controlled by a novel, oxygen-independent, signalling pathway which is required to regulate metabolism under anoxic conditions.

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Journal ArticleDOI

Osmotic Stress Signaling and Osmoadaptation in Yeasts

TL;DR: An integrated understanding of osmoadaptation requires not only knowledge of the function of many uncharacterized genes but also further insight into the time line of events, their interdependence, their dynamics, and their spatial organization as well as the importance of subtle effects.
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Organic osmolytes as compatible, metabolic and counteracting cytoprotectants in high osmolarity and other stresses

TL;DR: Organic osmolytes are small solutes used by cells of numerous water-stressed organisms and tissues to maintain cell volume and have applications in biotechnology, agriculture and medicine, including in vitro rescue of the misfolded protein of cystic fibrosis.
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MAP Kinase Pathways in the Yeast Saccharomyces cerevisiae

TL;DR: The current knowledge of MAPK pathways in yeast is presented and some directions for future research in this area are presented, including how the upstream proteins actually activate the cascade remains unclear.
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On the Trail of a Cereal Killer: Exploring the Biology of Magnaporthe grisea

TL;DR: Recent progress toward understanding the molecular biology of plant infection by M. grisea is reviewed, which involves development of a specialized cell, the appressorium, which generates enormous turgor pressure and physical force, allowing the fungus to breach the host cuticle and invade plant tissue.
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Progress in Metabolic Engineering of Saccharomyces cerevisiae

TL;DR: The current review discusses the relevance of several engineering strategies, such as rational and inverse metabolic engineering, evolutionary engineering, and global transcription machinery engineering, in yeast strain improvement and summarizes existing tools for fine-tuning and regulating enzyme activities and thus metabolic pathways.
References
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Journal ArticleDOI

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TL;DR: DNA binding of the Fos-Jun heterodimer was modulated by reduction-oxidation of a single conserved cysteine residue in the DNA-binding domains of the two proteins, suggesting that transcriptional activity mediated by AP-1 binding factors may be regulated by a redox mechanism.
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