[No authors listed]
Phosphatidylethanolamine (PE) in the yeast Saccharomyces cerevisiae is synthesized through decarboxylation of phosphatidylserine (PS), catalysed by PS decarboxylase 1 (Psd1p) and 2 (Psd2p) and the cytidine 5'-diphosphate (CDP)-ethanolamine (CDP-Etn) pathway. PSD1 null (psd1Î) and PSD2 null (psd2Î) mutants are viable in a synthetic minimal medium, but a psd1Î psd2Î double mutant exhibits Etn auxotrophy, which is incorporated into PE through the CDP-Etn pathway. We have previously shown that psd1Î is synthetic lethal with deletion of VID22 (vid22Î) [Kuroda et al. (2011) Mol. Microbiol. 80: , 248-265]. In the present study, we found that vid22Î mutant exhibits Etn auxotrophy under PSD1-depressed conditions. Deletion of VID22 in wild-type and PSD1-depressed cells caused partial defects in PE formation through decarboxylation of PS. The enzyme activity of PS decarboxylase in an extract of vid22Î cells was â¼70% of that in wild-type cells and similar to that in psd2Î cells and the PS decarboxylase activity remaining in the PSD1-depressed cells became almost negligible with deletion of VID22. Thus, the vid22Î mutation was suggested to cause a defect in the Psd2p activity. Furthermore, vid22Î cells were shown to be defective in expression of the PSD2 gene tagged with 6ÃHA, the defect being ameliorated by replacement of the native promoter of the PSD2 gene with a CYC1 promoter. In addition, an α-galactosidase reporter assay revealed that the activity of the promoter of the PSD2 gene in vid22Î cells was â¼5% of that in wild-type cells. These results showed that VID22 is required for transcriptional activation of the PSD2 gene.
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