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W2089894637 abstract "When Saccharomyces cerevisiae are starved of glucose for a prolonged period of time, gluconeogenic enzymes such as fructose-1,6-bisphosphatase (FBPase), malate dehydrogenase, isocitrate lyase, and phosphoenolpyruvate carboxykinase are induced. However, when glucose is added to prolonged-starved cells, these enzymes are degraded in the vacuole via the vacuole import and degradation (Vid) pathway. The Vid pathway merges with the endocytic pathway to remove intracellular and extracellular proteins simultaneously. Ultrastructural and cell extraction studies indicate that substantial amounts of FBPase were in the extracellular fraction (periplasm) during glucose starvation. FBPase levels in the extracellular fraction decreased after glucose re-feeding in wild-type cells. The decline of FBPase in the extracellular fraction was dependent on the SLA1 and ARC18 genes involved in actin polymerization and endocytosis. Moreover, the reduction of extracellular FBPase was also dependent on the VPS34 gene. VPS34 encodes the PI3 kinase and is also required for the Vid pathway. Vps34p co-localized with actin patches in prolonged-starved cells. In the absence of this gene, FBPase and the Vid vesicle protein Vid24p associated with actin patches before and after the addition of glucose. Furthermore, high levels of FBPase remained in the extracellular fraction in the Δvps34 mutant during glucose re-feeding. When the Asn-736 residue of Vps34p was mutated and when the C-terminal 11 amino acids were deleted, mutant proteins failed to co-localize with actin patches, and FBPase in the extracellular fraction did not decrease as rapidly. We suggest that VPS34 plays a critical role in the decline of extracellular FBPase in response to glucose. When Saccharomyces cerevisiae are starved of glucose for a prolonged period of time, gluconeogenic enzymes such as fructose-1,6-bisphosphatase (FBPase), malate dehydrogenase, isocitrate lyase, and phosphoenolpyruvate carboxykinase are induced. However, when glucose is added to prolonged-starved cells, these enzymes are degraded in the vacuole via the vacuole import and degradation (Vid) pathway. The Vid pathway merges with the endocytic pathway to remove intracellular and extracellular proteins simultaneously. Ultrastructural and cell extraction studies indicate that substantial amounts of FBPase were in the extracellular fraction (periplasm) during glucose starvation. FBPase levels in the extracellular fraction decreased after glucose re-feeding in wild-type cells. The decline of FBPase in the extracellular fraction was dependent on the SLA1 and ARC18 genes involved in actin polymerization and endocytosis. Moreover, the reduction of extracellular FBPase was also dependent on the VPS34 gene. VPS34 encodes the PI3 kinase and is also required for the Vid pathway. Vps34p co-localized with actin patches in prolonged-starved cells. In the absence of this gene, FBPase and the Vid vesicle protein Vid24p associated with actin patches before and after the addition of glucose. Furthermore, high levels of FBPase remained in the extracellular fraction in the Δvps34 mutant during glucose re-feeding. When the Asn-736 residue of Vps34p was mutated and when the C-terminal 11 amino acids were deleted, mutant proteins failed to co-localize with actin patches, and FBPase in the extracellular fraction did not decrease as rapidly. We suggest that VPS34 plays a critical role in the decline of extracellular FBPase in response to glucose." @default.
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W2089894637 date "2012-09-01" @default.
W2089894637 modified "2023-09-26" @default.
W2089894637 title "Vps34p Is Required for the Decline of Extracellular Fructose-1,6-bisphosphatase in the Vacuole Import and Degradation Pathway" @default.
W2089894637 cites W1539881139 @default.
W2089894637 cites W1772777894 @default.
W2089894637 cites W1923816168 @default.
W2089894637 cites W1964069410 @default.
W2089894637 cites W1966322334 @default.
W2089894637 cites W1967085696 @default.
W2089894637 cites W1969875733 @default.
W2089894637 cites W1972718290 @default.
W2089894637 cites W1974724055 @default.
W2089894637 cites W1976010532 @default.
W2089894637 cites W1978112795 @default.
W2089894637 cites W1998354357 @default.
W2089894637 cites W1999477136 @default.
W2089894637 cites W2000702106 @default.
W2089894637 cites W2011692074 @default.
W2089894637 cites W2013131355 @default.
W2089894637 cites W2015503148 @default.
W2089894637 cites W2020456066 @default.
W2089894637 cites W2024600213 @default.
W2089894637 cites W2027351170 @default.
W2089894637 cites W2029758696 @default.
W2089894637 cites W2031169909 @default.
W2089894637 cites W2043886213 @default.
W2089894637 cites W2044285636 @default.
W2089894637 cites W2055188333 @default.
W2089894637 cites W2058250395 @default.
W2089894637 cites W2059433184 @default.
W2089894637 cites W2060941673 @default.
W2089894637 cites W2064733220 @default.
W2089894637 cites W2074286043 @default.
W2089894637 cites W2075430039 @default.
W2089894637 cites W2088336227 @default.
W2089894637 cites W2095630758 @default.
W2089894637 cites W2096330480 @default.
W2089894637 cites W2097000049 @default.
W2089894637 cites W2100167673 @default.
W2089894637 cites W2103421087 @default.
W2089894637 cites W2103917882 @default.
W2089894637 cites W2108305274 @default.
W2089894637 cites W2109034822 @default.
W2089894637 cites W2118401405 @default.
W2089894637 cites W2123777737 @default.
W2089894637 cites W2125452667 @default.
W2089894637 cites W2137339435 @default.
W2089894637 cites W2138871985 @default.
W2089894637 cites W2144535282 @default.
W2089894637 cites W2152600551 @default.
W2089894637 cites W2154834069 @default.
W2089894637 cites W2156594219 @default.
W2089894637 cites W2156810094 @default.
W2089894637 cites W2157839115 @default.
W2089894637 cites W2158644807 @default.
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W2089894637 cites W2170298918 @default.
W2089894637 cites W2170633329 @default.
W2089894637 cites W642194586 @default.
W2089894637 doi "https://doi.org/10.1074/jbc.m112.360412" @default.
W2089894637 hasPubMedCentralId "https://www.ncbi.nlm.nih.gov/pmc/articles/3463303" @default.
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