The DHHC protein Pfa3 affects vacuole-associated palmitoylation of the fusion factor Vac8
The DHHC protein Pfa3 affects vacuole-associated palmitoylation of the fusion factor Vac8
Vacuole biogenesis depends on specific targeting and retention of peripheral membrane proteins. At least three palmitoylated proteins are found exclusively on yeast vacuoles: the fusion factor Vac8, the kinase Yck3, and a novel adaptor protein implicated in microautophagy, Meh1. Here, we analyze the role that putative acyltransferases of the DHHC family play in their localization and function. We find that Pfa3/Ynl326c is required for efficient localization of Vac8 to vacuoles in vivo , while Yck3 or Meh1 localization is not impaired in any of the seven DHHC deletions. Vacuole-associated Vac8 appears to be palmitoylated in a pfa3 mutant, but this population is refractive to further palmitoylation on isolated vacuoles. Vacuole morphology and inheritance, which both depend on Vac8 palmitoylation, appear normal, although there is a reduction in vacuole fusion. Interestingly, Pfa3 is required for the vacuolar localization of not only an SH4 domain that is targeted by myristate/palmitate (as in Vac8) but also one that is targeted by a myristate/basic stretch (as in Src). Our data indicate that Pfa3 has an important but not exclusive function for Vac8 localization to the vacuole.
- University Physicians United States
- California Institute of Technology United States
- University of Geneva Switzerland
- Heidelberg University Germany
Yck3, 570, Saccharomyces cerevisiae Proteins, Palmitoyl Coenzyme A, Casein Kinase I, Lipoproteins, Green Fluorescent Proteins, Vesicular Transport Proteins, Membrane Proteins, Saccharomyces cerevisiae, SH4 domain, membrane targeting, Microscopy, Fluorescence, Mutation, Vacuoles, acylation, Biotinylation, Acyltransferases
Yck3, 570, Saccharomyces cerevisiae Proteins, Palmitoyl Coenzyme A, Casein Kinase I, Lipoproteins, Green Fluorescent Proteins, Vesicular Transport Proteins, Membrane Proteins, Saccharomyces cerevisiae, SH4 domain, membrane targeting, Microscopy, Fluorescence, Mutation, Vacuoles, acylation, Biotinylation, Acyltransferases
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