Nuclear translocation of Gln3 in response to nutrient signals requires Golgi-to-endosome trafficking in
            <i>Saccharomyces cerevisiae</i>

Puria, Rekha; Zurita-Martinez, Sara A.; Cárdenas, María E.

doi:10.1073/pnas.0801087105

Cited by 48 publications

(70 citation statements)

References 42 publications

(60 reference statements)

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“…(vii) Gln3-Myc 13 is not uniformly distributed in the cytoplasm of cells grown under repressive conditions but is associated with a cytoplasmic membrane system (49,50). Extending this observation, nuclear Gln3 localization in derepressive conditions was found to require several components that participate in Golgi-to-endosome vesicle transport (51).…”

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confidence: 68%

Distinct Phosphatase Requirements and GATA Factor Responses to Nitrogen Catabolite Repression and Rapamycin Treatment in Saccharomyces cerevisiae

Tate

Georis

Dubois

et al. 2010

Journal of Biological Chemistry

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In yeast, rapamycin (Rap)-inhibited TorC1, and the phosphatases it regulates (Sit4 and PP2A) are components of a conserved pathway regulating the response of eukaryotic cells to nutrient availability. TorC1 and intracellular nitrogen levels regulate the localization of Gln3 and Gat1, the activators of nitrogen catabolite repression (NCR)-sensitive genes whose products are required to utilize poor nitrogen sources. In nitrogen excess, Gln3 and Gat1 are cytoplasmic, and NCR-sensitive transcription is repressed. During nitrogen limitation or Rap treatment, Gln3 and Gat1 are nuclear, and transcription is derepressed. We previously demonstrated that the Sit4 and Pph21/22-Tpd3-Cdc55/Rts1 requirements for nuclear Gln3 localization differ. We now show that Sit4 and Pph21/22-Tpd3-Cdc55/Rts1 requirements for NCR-sensitive and Rap-induced nuclear Gat1 localization markedly differ from those of Gln3. Our data suggest that Gln3 and Gat1 localizations are controlled by two different regulatory pathways. Gln3 localization predominantly responds to intracellular nitrogen levels, as reflected by its stronger NCR-sensitivity, weaker response to Rap treatment, and strong response to methionine sulfoximine (Msx, a glutamine synthetase inhibitor). In contrast, Gat1 localization predominantly responds to TorC1 regulation as reflected by its weaker NCR sensitivity, stronger response to Rap, and immunity to the effects of Msx. Nuclear Gln3 localization in prolinegrown (nitrogen limited) cells exhibits no requirement for Pph21/22-Tpd3/Cdc55, whereas nuclear Gat1 localization under these conditions is absolutely dependent on Pph21/22-Tpd3/Cdc55. Furthermore, the extent to which Pph21/22-Tpd3-Cdc55 is required for the TorC1 pathway (Rap) to induce nuclear Gat1 localization is regulated in parallel with Pph21/22-Tpd3-Cdc55-dependent Gln3 dephosphorylation and NCRsensitive transcription, being highest in limiting nitrogen and lowest when nitrogen is in excess.One consequence of motif, gene, or genome duplication is the subsequent existence of multiple proteins with the same or overlapping functions. In some cases the duplicated genes evolve, acquiring easily distinguishable new functions or regulatory profiles (1-4). In others, the differences are more subtle, and a more careful study is required before they become apparent. This is the case with the Saccharomyces cerevisiae GATA family transcription factors, Gln3 and Gat1/Nil1. Both Gln3 and Gat1 are responsible for nitrogen catabolite repression (NCR) 2 -sensitive expression of genes encoding the transport and enzyme proteins needed to scavenge poor nitrogen sources (e.g. proline) when more readily usable ones are limiting or unavailable (5-8). Gln3 and Gat1 binding sites in NCR-sensitive promoters contain the core sequence GATAA that binds the well characterized zinc finger motif that defines this family of proteins (9 -11).The most apparent differences in the regulation of the GATA factors occur at the level of transcription. GAT1 expression is NCR-sensitive, Gln3-dependent, Gat1-auto-a...

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confidence: 68%

Distinct Phosphatase Requirements and GATA Factor Responses to Nitrogen Catabolite Repression and Rapamycin Treatment in Saccharomyces cerevisiae

Tate

Georis

Dubois

et al. 2010

Journal of Biological Chemistry

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“…The Vps-C complex is thought to promote amino acid homeostasis through several mechanisms. First, the Vps-C complex affects amino acid transporter expression and stability (Srivastava et al 2000;Puria et al 2008). Second, Vps-C complexes maintain vacuole integrity, and this organelle plays a key role in storage of amino acids that are acquired from the cytosol or produced directly at the vacuole by protein degradation during the normal recycling of proteins or autophagy (Wiemken and Durr 1974;Kitamoto et al 1988a;Onodera and Ohsumi 2005).…”

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confidence: 99%

Endolysosomal Membrane Trafficking Complexes Drive Nutrient-Dependent TORC1 Signaling to Control Cell Growth in Saccharomyces cerevisiae

et al. 2014

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The rapamycin-sensitive and endomembrane-associated TORC1 pathway controls cell growth in response to nutrients in eukaryotes. Mutations in class C Vps (Vps-C) complexes are synthetically lethal with tor1 mutations and confer rapamycin hypersensitivity in Saccharomyces cerevisiae, suggesting a role for these complexes in TORC1 signaling. Vps-C complexes are required for vesicular trafficking and fusion and comprise four distinct complexes: HOPS and CORVET and their minor intermediaries (i)-CORVET and i-HOPS. We show that at least one Vps-C complex is required to promote TORC1 activity, with the HOPS complex having the greatest input. The vps-c mutants fail to recover from rapamycin-induced growth arrest and show low levels of TORC1 activity. TORC1 promotes cell growth via Sch9, a p70 S6 kinase ortholog. Constitutively active SCH9 or hyperactive TOR1 alleles restored rapamycin recovery and TORC1 activity of vps-c mutants, supporting a role for the Vps-C complexes upstream of TORC1. The EGO GTPase complex Exit from G 0 Complex (EGOC) and its homologous Rag-GTPase complex convey amino acid signals to TORC1 in yeast and mammals, respectively. Expression of the activated EGOC GTPase subunits Gtr1 GTP and Gtr2 GDP partially suppressed vps-c mutant rapamycin recovery defects, and this suppression was enhanced by increased amino acid concentrations. Moreover, vps-c mutations disrupted EGOC-TORC1 interactions. TORC1 defects were more severe for vps-c mutants than those observed in EGOC mutants. Taken together, our results support a model in which distinct endolysosomal trafficking Vps-C complexes promote rapamycin-sensitive TORC1 activity via multiple inputs, one of which involves maintenance of amino acid homeostasis that is sensed and transmitted to TORC1 via interactions with EGOC.T HE Target of rapamycin (TOR) kinases are conserved across eukaryotes and orchestrate myriad cellular processes to control growth in response to nutrients and environmental signals. The Tor kinases form two evolutionarily conserved multi-protein complexes known as TORC1 (Tor complex) and TORC2. TORC1 is sensitive to the immunosuppressive and antiproliferative drug rapamycin, and in Saccharomyces cerevisiae is populated by Tor1 (or, to a lesser extent, Tor2), Kog1, Lst8, and Tco89. TORC1 controls cell growth when nutrients such as amino acids are abundant and serves to maintain robust nutrient transport, ribosome biogenesis, and protein synthesis and concomitantly inhibits autophagy (Heitman et al. 1991;Cardenas et al. 1999;Powers and Walter 1999;Loewith et al. 2002;Reinke et al. 2004;Wullschleger et al. 2006;Loewith and Hall 2011). TORC2 is rapamycin-insensitive and composed of Tor2, Lst8, Bit61/Bit2, Avo1, Avo2, and Avo3; TORC2 controls spatial growth via regulation of actin cytoskeleton polarization (Schmidt et al. 1996;Loewith et al. 2002). Amino acid levels are signaled to yeast TORC1, at least in part, via the leucyl-tRNA synthetase, which binds and influences the guanine nucleotide state of components of the Rag GTPase EGOC (...

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“…Like vps15D and vps34D, these other five vps mutants are also defective for vesicular protein transport from the Golgi to the vacuole (Bowers and Stevens 2005). Vps10 is an integral membrane protein that functions as the receptor for carboxypeptidase Y to mediate its trafficking from the late Golgi to late endosome (Bowers and Stevens 2005); and it was recently implicated in promoting nuclear entry of Gln3 (Puria et al 2008); however, eliminating the VPS10 gene conferred no sensitivity to 6-AU or MPA ( Figure 1C). Sensitivity to 6-AU and MPA does not necessarily indicate a transcription elongation defect; however, mutations in bona fide elongation factors have been found to reduce transcriptional induction of IMD2, encoding an MPA-resistant form of IMPDH (McPhillips et al 2004), in response to 6-AU or MPA treatment (Riles et al 2004).…”

Section: Resultsmentioning

confidence: 99%

“…The Ga subunit (Gpa1) of a heterotrimeric G protein activates the PI 3-kinase Vps34 (a class D Vps factor) at the endosomal membrane to promote the transcriptional response to mating factors (Slessareva et al 2006). Activation of genes for utilization of alternative nitrogen sources by Gln3 is enhanced by Vps factors, and it appears that Gln3 must traffic in vesicles containing Vps10 between Golgi and endosome for subsequent nuclear entry (Puria et al 2008). Recently, evidence was presented that the phosphoinositide PI(3,5)P 2 , produced at the late endosome promotes assembly of a transcriptional cofactor complex that enhances galactose induction of GAL gene transcription in the nucleus (Han and Emr 2011).…”

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Vps Factors Are Required for Efficient Transcription Elongation in Budding Yeast

et al. 2013

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There is increasing evidence that certain Vacuolar protein sorting (Vps) proteins, factors that mediate vesicular protein trafficking, have additional roles in regulating transcription factors at the endosome. We found that yeast mutants lacking the phosphatidylinositol 3-phosphate [PI(3)P] kinase Vps34 or its associated protein kinase Vps15 display multiple phenotypes indicating impaired transcription elongation. These phenotypes include reduced mRNA production from long or G+C-rich coding sequences (CDS) without affecting the associated GAL1 promoter activity, and a reduced rate of RNA polymerase II (Pol II) progression through lacZ CDS in vivo. Consistent with reported genetic interactions with mutations affecting the histone acetyltransferase complex NuA4, vps15D and vps34D mutations reduce NuA4 occupancy in certain transcribed CDS. vps15D and vps34D mutants also exhibit impaired localization of the induced GAL1 gene to the nuclear periphery. We found unexpectedly that, similar to known transcription elongation factors, these and several other Vps factors can be cross-linked to the CDS of genes induced by Gcn4 or Gal4 in a manner dependent on transcriptional induction and stimulated by Cdk7/Kin28-dependent phosphorylation of the Pol II C-terminal domain (CTD). We also observed colocalization of a fraction of Vps15-GFP and Vps34-GFP with nuclear pores at nucleus-vacuole (NV) junctions in live cells. These findings suggest that Vps factors enhance the efficiency of transcription elongation in a manner involving their physical proximity to nuclear pores and transcribed chromatin. N EWLY synthesized proteins that are transported from the Golgi to the lysosome/vacuole traverse the endosome, as do ubiquitinated proteins that are removed from the plasma membrane by endocytosis en route to the vacuole for degradation. Ubiquitinated cargo proteins progress through early and late endosomes, are concentrated at the outer membranes of multivesicular bodies (MVB), and are then sequestered in intralumenal vesicles (ILVs) It is thought that ESCRT-0 is recruited from the cytoplasm to the endosomal outer membrane by interaction with the phosphoinositide PI(3)P, where it acts to recruit and concentrate ubiquitinated cargo proteins and transfer them to the ESCRT-I complex. ESCRT-I activates the ESCRT-II heterotrimer that, in turn, recruits the ESCRT-III components, which are believed to assemble filaments instrumental in invagination of the MVB membrane. The AAA-ATPase Vps4, recruited by ESCRT-III subunits, functions to pinch off the membrane invaginations to produce ILVs containing cargo proteins and to recycle the ESCRT factors back to the cytoplasm (Raiborg and Stenmark 2009).

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Nuclear translocation of Gln3 in response to nutrient signals requires Golgi-to-endosome trafficking in Saccharomyces cerevisiae

Cited by 48 publications

References 42 publications

Distinct Phosphatase Requirements and GATA Factor Responses to Nitrogen Catabolite Repression and Rapamycin Treatment in Saccharomyces cerevisiae

Distinct Phosphatase Requirements and GATA Factor Responses to Nitrogen Catabolite Repression and Rapamycin Treatment in Saccharomyces cerevisiae

Endolysosomal Membrane Trafficking Complexes Drive Nutrient-Dependent TORC1 Signaling to Control Cell Growth in Saccharomyces cerevisiae

Vps Factors Are Required for Efficient Transcription Elongation in Budding Yeast

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