AI Article Synopsis

  • Inositolphosphorylceramide (IPC) and its derivatives are essential sphingolipids in yeast, and their synthesis is inhibited by aureobasidin A (AbA), leading to cell stress and apoptosis.
  • Gradual depletion of IPC synthase Aur1 results in ceramide accumulation, which is harmful to cell survival, but overexpressing YPC1, an alkaline ceramidase, can rescue cells under this stress.
  • High-throughput screens show that vesicle-mediated transport among organelles and vacuolar acidification are vital for cell survival when Aur1 is repressed, and while AbA triggers cell wall integrity pathways, it doesn't improve cell viability despite inducing stress.

Article Abstract

Inositolphosphorylceramide (IPC) and its mannosylated derivatives are the only complex sphingolipids of yeast. Their synthesis can be reduced by aureobasidin A (AbA), which specifically inhibits the IPC synthase Aur1. AbA reportedly, by diminishing IPC levels, causes endoplasmic reticulum (ER) stress, an increase in cytosolic calcium, reactive oxygen production, and mitochondrial damage leading to apoptosis. We found that when Aur1 is gradually depleted by transcriptional downregulation, the accumulation of ceramides becomes a major hindrance to cell survival. Overexpression of the alkaline ceramidase YPC1 rescues cells under this condition. We established hydroxylated C26 fatty acids as a reliable hallmark of ceramide hydrolysis. Such hydrolysis occurs only when YPC1 is overexpressed. In contrast, overexpression of YPC1 has no beneficial effect when Aur1 is acutely repressed by AbA. A high-throughput genetic screen revealed that vesicle-mediated transport between Golgi apparatus, endosomes, and vacuole becomes crucial for survival when Aur1 is repressed, irrespective of the mode of repression. In addition, vacuolar acidification becomes essential when cells are acutely stressed by AbA, and quinacrine uptake into vacuoles shows that AbA activates vacuolar acidification. The antioxidant N-acetylcysteine does not improve cell growth on AbA, indicating that reactive oxygen radicals induced by AbA play a minor role in its toxicity. AbA strongly induces the cell wall integrity pathway, but osmotic support does not improve the viability of wild-type cells on AbA. Altogether, the data support and refine current models of AbA-mediated cell death and add vacuolar protein transport and acidification as novel critical elements of stress resistance.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4664882PMC
http://dx.doi.org/10.1128/EC.00117-15DOI Listing

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