Regulation of the Sko1 transcriptional repressor by the Hog1 MAP kinase in response to osmotic stress
2001; Springer Nature; Volume: 20; Issue: 5 Linguagem: Inglês
10.1093/emboj/20.5.1123
ISSN1460-2075
AutoresMarkus Proft, Amparo Pascual‐Ahuir, Eulàlia de Nadal, Joaquı́n Ariño, Ramón Serrano, Francesc Posas,
Tópico(s)Biofuel production and bioconversion
ResumoArticle1 March 2001free access Regulation of the Sko1 transcriptional repressor by the Hog1 MAP kinase in response to osmotic stress Markus Proft Markus Proft Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain Search for more papers by this author Amparo Pascual-Ahuir Amparo Pascual-Ahuir Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain Search for more papers by this author Eulàlia de Nadal Eulàlia de Nadal Cell Signaling Unit, Departament de Ciències Experimentals i de la Salut, Universitat Pompeu Fabra (UPF), E-08003 Barcelona, Spain Search for more papers by this author Joaquin Ariño Joaquin Ariño Departament de Bioquímica i Biologia Molecular, Facultat de Veterinària, Universitat Autònoma de Barcelona, E-08193 Barcelona, Spain Search for more papers by this author Ramón Serrano Ramón Serrano Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain Search for more papers by this author Francesc Posas Corresponding Author Francesc Posas Cell Signaling Unit, Departament de Ciències Experimentals i de la Salut, Universitat Pompeu Fabra (UPF), E-08003 Barcelona, Spain Search for more papers by this author Markus Proft Markus Proft Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain Search for more papers by this author Amparo Pascual-Ahuir Amparo Pascual-Ahuir Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain Search for more papers by this author Eulàlia de Nadal Eulàlia de Nadal Cell Signaling Unit, Departament de Ciències Experimentals i de la Salut, Universitat Pompeu Fabra (UPF), E-08003 Barcelona, Spain Search for more papers by this author Joaquin Ariño Joaquin Ariño Departament de Bioquímica i Biologia Molecular, Facultat de Veterinària, Universitat Autònoma de Barcelona, E-08193 Barcelona, Spain Search for more papers by this author Ramón Serrano Ramón Serrano Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain Search for more papers by this author Francesc Posas Corresponding Author Francesc Posas Cell Signaling Unit, Departament de Ciències Experimentals i de la Salut, Universitat Pompeu Fabra (UPF), E-08003 Barcelona, Spain Search for more papers by this author Author Information Markus Proft1, Amparo Pascual-Ahuir1, Eulàlia de Nadal2, Joaquin Ariño3, Ramón Serrano1 and Francesc Posas 2 1Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-CSIC, 46022 Valencia, Spain 2Cell Signaling Unit, Departament de Ciències Experimentals i de la Salut, Universitat Pompeu Fabra (UPF), E-08003 Barcelona, Spain 3Departament de Bioquímica i Biologia Molecular, Facultat de Veterinària, Universitat Autònoma de Barcelona, E-08193 Barcelona, Spain *Corresponding author. E-mail: [email protected] The EMBO Journal (2001)20:1123-1133https://doi.org/10.1093/emboj/20.5.1123 PDFDownload PDF of article text and main figures. ToolsAdd to favoritesDownload CitationsTrack CitationsPermissions ShareFacebookTwitterLinked InMendeleyWechatReddit Figures & Info Exposure of yeast to increases in extracellular osmolarity activates the Hog1 mitogen-activated protein kinase (MAPK), which is essential for the induction of gene expression required for cell survival upon osmotic stress. Several genes are regulated in response to osmotic stress by Sko1, a transcriptional repressor of the ATF/CREB family. We show by in vivo coprecipitation and phosphorylation studies that Sko1 and Hog1 interact and that Sko1 is phosphorylated upon osmotic stress in a Hog1-dependent manner. Hog1 phosphorylates Sko1 in vitro at multiple sites within the N-terminal region. Phosphorylation of Sko1 disrupts the Sko1–Ssn6–Tup1 repressor complex, and consistently, a mutant allele of Sko1, unphosphorylatable by Hog1, exhibits less derepression than the wild type. Interestingly, Sko1 repressor activity is further enhanced in strains with high protein kinase A (PKA) activity. PKA phosphorylates Sko1 near the bZIP domain and mutation of these sites eliminates modulation of Sko1 responses to high PKA activity. Thus, Sko1 transcriptional repression is controlled directly by the Hog1 MAPK in response to stress, and this effect is further modulated by an independent signaling mechanism through the PKA pathway. Introduction Mitogen-activated protein kinase (MAPK) cascades are common signaling modules found in both higher and lower eukaryotic cells. Activation of a MAPK results in modification of a set of target proteins, often transcription factors, that allow the generation of appropriate cellular responses to an external stimulus (reviewed in Robinson and Cobb, 1997). Yeast cells have several different MAPK cascades that transduce distinct extracellular stimuli (e.g. mating pheromone and high osmolarity) (reviewed in Gustin et al., 1998). Budding yeast (Saccharomyces cerevisiae) responds to increases in osmolarity in the extracellular environment by activating the Hog1 MAPK cascade (Boguslawski, 1992; Brewster et al., 1993). The yeast HOG pathway is activated by two independent mechanisms, which lead to the phosphorylation and activation of the Hog1 MAPK (reviewed in Gustin et al., 1998). Once activated, Hog1 induces diverse osmo-adaptive responses such as regulation of gene expression. Recent genome-wide transcriptional analyses carried out using DNA chips and filter hybridization showed that a great number of genes are regulated by osmotic stress in a Hog1-dependent manner (Posas et al., 2000; Rep et al., 2000). Among the genes under the control of Hog1 are genes that encode proteins involved in protection against osmotic stress as well as other types of stimuli. The mechanism of gene regulation through activated Hog1 is largely unknown because transcription factors under the control of this MAPK are not well characterized. Several candidates, however, have been proposed; for example, the general stress response transcription factors Msn2 and Msn4, which are regulated by protein kinase A (PKA) upon stress. Unfortunately, their relationship with Hog1 remains unclear (Martinez-Pastor et al., 1996; Schmitt and McEntee, 1996; Görner et al., 1998). Recently it was reported that Hot1, a putative transcriptional regulator, interacts with Hog1 in the two-hybrid system and appears to act downstream of Hog1 (Rep et al., 1999). However, the direct interaction with Hog1 and its regulation by this MAPK are not yet demonstrated. Stimulated expression of some HOG pathway-dependent genes after osmotic stress appears to be the result of transcriptional derepression (Márquez et al., 1998). The bZIP transcriptional repressor Sko1 binds to the so-called cAMP responsive element (CRE) promoter motif (Nehlin et al., 1992; Vincent and Struhl, 1992). Its implication in the transcriptional regulation of osmotic stress-inducible genes has been shown recently for the stress defense genes ENA1 (Proft and Serrano, 1999), HAL1 (Pascual-Ahuir et al., 2001) and GRE2 (Garcia-Gimeno and Struhl, 2000). Genetic data indicate that Sko1 represses stress gene expression from CRE sites by recruiting the general co-repressor complex Ssn6–Tup1. Accordingly, mutants in either one of the three components are hyperresistant to salt stress (Márquez et al., 1998; Proft and Serrano, 1999; Garcia-Gimeno and Struhl, 2000). Induction of Sko1-dependent genes involves the release of repression, and this process is completely dependent on the HOG pathway (Proft and Serrano, 1999; Garcia-Gimeno and Struhl, 2000). In this work we demonstrate biochemically that the Hog1 MAPK regulates the Sko1 transcriptional repressor by direct phosphorylation. We show that Hog1 and Sko1 interact in vivo, we identify the relevant Hog1 phosphorylation sites and analyze their effect on stress-regulated gene expression in vivo. Our results indicate that one important function of activated Hog1 kinase is the phosphorylation and inactivation of the Sko1 repressor by disruption of its association with Ssn6 and Tup1 proteins. Results Sko1 represses HOG-dependent stress gene expression The Sko1 transcriptional repressor has recently been implicated in the osmotic stress-induced expression of some stress defense genes (Proft and Serrano, 1999; Garcia-Gimeno and Struhl, 2000; Pascual-Ahuir et al., 2001). Among these, GRE2, which encodes a plant isoflavonoid reductase homolog (Garay-Arroyo and Covarrubias, 1999), shows the most pronounced expression pattern upon hyperosmotic shock. We made use of this Sko1-dependent reporter gene to investigate by northern analysis of GRE2 expression during osmotic stress the epistatic relationship between Sko1 and Hog1. As shown in Figure 1, GRE2 expression is strongly repressed when cells are grown in normal medium, while the loss of SKO1 leads to high GRE2 transcript levels (∼13-fold as compared with wild type). GRE2 transcription is induced ∼45-fold upon brief osmotic shock in wild-type cells. This induction is virtually absent (only <2-fold) in sko1Δ cells, due mainly to higher expression under non-stress conditions. In the absence of HOG1, a dramatically reduced induction of GRE2 is observed that is completely suppressed by additional deletion of SKO1 (Figure 1). It is worth noting that Sko1-mediated gene transcription is completely dependent on the kinase activity of Hog1, since expression of a catalytically impaired Hog1 allele [Hog1(KN)] was unable to restore GRE2 expression in a hog1Δ strain (data not shown). Since sko1Δ and hog1Δ sko1Δ mutants showed nearly identically high GRE2 expression, one possible explanation was that Hog1 MAPK would act exclusively through the Sko1 repressor on the transcriptional control of a subset of stress defense genes. Figure 1.Roles of Sko1 and Hog1 in osmotic stress-induced transcription of GRE2. Transcript levels of GRE2 were monitored by northern analysis before and during osmotic stress caused by 0.4 M NaCl. GRE2 mRNA levels were quantified, normalized for the TBP1 internal loading control and depicted in the lower panel. The different small blots presented as well as the quantification data come from the same original blot for each mutant. The isogenic yeast strains W303-1A (wt), MAP19 (sko1Δ), MAP32 (hog1Δ) and MAP33 (hog1Δ sko1Δ) were used. Download figure Download PowerPoint Sko1 is phosphorylated in vivo upon osmotic stress in a Hog1-dependent manner As a first approach to determine the relationship between Sko1 and Hog1, we investigated whether Sko1 is phosphorylated in vivo during hyperosmotic stress. Therefore, we fused the SKO1 gene at its chromosomal locus with a triple haemagglutinin (HA) epitope at the N-terminus. The fully functional HA–Sko1 fusion protein (HA–SKO1) was detected from wild-type and hog1Δ cells using the specific 12CA5 monoclonal antibody against HA. This immunological detection of HA–SKO1 revealed that upon brief shock with 0.4 M NaCl, Sko1 rapidly changes its mobility in SDS–polyacrylamide gels (Figure 2). To test whether this shift in mobility of Sko1 was due to phosphorylation, protein extracts were treated with alkaline phosphatase before western analysis and as expected the mobility shift was eliminated (Figure 2). This effect was reversed by the simultaneous application of phosphatase inhibitors. Moreover, phosphorylation of Sko1 in response to osmotic stress depended completely on Hog1, since HA–SKO1 expressed from hog1Δ cells did not undergo the mobility shift observed in wild-type cells. Taken together, these results show that Sko1 is rapidly phosphorylated upon hyperosmotic shock in vivo and that this modification depends on the Hog1 MAPK. Figure 2.In vivo phosphorylation of Sko1 upon osmotic stress depends on Hog1. HA–SKO1 was expressed from its chromosomal locus in wild-type (MAP37) and hog1Δ (MAP36) cells. Approximately 50 μg of yeast total protein extracts were separated by SDS–PAGE, and the fusion protein was detected by monoclonal HA-specific antibodies. Cells were subjected or not to brief osmotic shock (0.4 M NaCl, 10 min) and the extracts were treated or not with 10 U of alkaline phosphatase in the absence or presence of phosphatase inhibitors as indicated. Control strain (without HA–SKO1) was wild-type strain W303-1A. Download figure Download PowerPoint Sko1 co-immunoprecipitates with Hog1 To obtain biochemical evidence for the interaction of Sko1 and Hog1 in vivo, we tested HA–Sko1 for immunoprecipitation with glutathione S-transferase (GST)–Hog1 or green fluorescent protein (GFP)–Hog1 (Figure 3). Figure 3.In vivo binding of Hog1 to Sko1. (A) MAP37 strain (which expresses HA-tagged Sko1 from the wild-type locus) was transformed with a plasmid expressing GST or GST–HOG1 under the PGAL1 promoter. Cells were grown in the presence of galactose and samples were taken before (−) or 5 min after (+) the addition of NaCl to a final concentration of 0.4 M. HA–SKO1 was precipitated using anti-HA monoclonal antibody (12CA5) and protein A–Sepharose beads, and the presence of GST proteins in precipitates was probed by immunoblotting using anti-GST (upper panel). Antibody against HA was used to detect the HA–SKO1 fusion protein (lower panel). (B) Yeast MAP37 cells were transformed with a single copy plasmid containing GFP-tagged Hog1, expressed under its own promoter. Cells were grown in the presence of glucose and treated as in (A). HA–SKO1 and GFP–HOG1 in precipitates were probed with anti-HA and anti-GFP antibodies. Download figure Download PowerPoint Yeast MAP37 cells (which express HA-tagged Sko1 from its own genomic locus) were transformed with a plasmid that expresses GST-tagged Hog1 from the GAL1 promoter. Cells were subjected to a brief osmotic shock and Sko1 was immunoprecipitated using specific monoclonal antibodies against HA. The presence of GST–HOG1 in the precipitates was probed by an anti-GST monoclonal antibody. As shown in Figure 3A, Sko1 was able to coprecipitate Hog1 irrespective of the environmental osmotic conditions. The above experiments were performed using the strong GAL1 promoter. Because the amount of Hog1 in those experiments is higher than the physiological conditions, we repeated the Hog1–Sko1 coprecipitation using Hog1 expressed from a centromeric (low copy number) plasmid under the control of its own native promoter. Hog1 was fused to GFP (GFP–HOG1), and transformed into the MAP37 strain (which contains chromosomal HA-tagged Sko1). Yeast MAP37 cells transformed with GFP–HOG1 were subjected to a brief osmotic shock. GFP–HOG1 was precipitated using anti-GFP antibody, and the presence of HA–SKO1 in precipitates was detected using anti-HA monoclonal antibody. Although the levels of protein expression were lower than in the previous experiments, the Sko1–Hog1 interaction was evident. Again, the level of Sko1–Hog1 binding was not affected by osmotic shock (Figure 3B). Thus, Hog1 MAPK binds to the Sko1 transcriptional repressor. Hog1 phosphorylates multiple sites at the N-terminus of Sko1 Sko1 is phosphorylated upon osmotic stress in a Hog1-dependent manner and interacts physically with the MAPK. We then tested whether Sko1 phosphorylation was carried out directly by the Hog1 MAPK, using purified proteins in an in vitro kinase assay. For this purpose, Hog1 and a constitutively activated version of Pbs2 [PBS2(EE)] (EE denotes Ser514→Glu and Thr518→Glu mutations in the activation loop of the Pbs2 MAPKK) were purified as GST fusion proteins from Escherichia coli. In the first step of the reaction Hog1 was activated by phosphorylation in the presence of PBS2(EE) and ATP. Then Sko1, purified from E.coli as a GST-tagged protein and [γ-32P]ATP were added to the reaction. As shown in Figure 4A, only when Sko1 was incubated with pre-activated Hog1, was phosphorylation of Sko1 observed. Figure 4.In vitro phosphorylation of Sko1 by Hog1. (A) In vitro activated Hog1 phosphorylates Sko1. Recombinant tagged proteins were purified from E.coli as described in Materials and methods. Hog1 and the constitutively activated Pbs2 allele [PBS2(EE)] were incubated in presence of kinase buffer and ATP. Sko1 was then added (when indicated) in the presence of radioactive ATP. Phosphorylated proteins were resolved by SDS–PAGE and detected by autoradiography. The position of tagged Sko1 is indicated on the left. (B) Hog1 phosphoryl ates the region between residues 1 and 202 of Sko1. Various Sko1 fragments were tested for their ability to be phosphorylated by an in vitro activated Hog1 (as described in Materials and methods). After in vitro kinase assay, phosphorylated proteins were resolved by SDS–PAGE and detected by autoradiography. The positions of the Sko1 fragments included in the constructs are indicated in parentheses. (C) Mutation of Sko1 Ser108, Thr113 and Ser126 to Ala abolishes Hog1 phosphorylation. Full-length Sko1 and the triple mutant SKO1(E) protein (mutant in the Ser108, Thr113 and Ser126) were tested for Hog1 phosphorylation as in (A). After phosphorylation, proteins were resolved by SDS–PAGE and transferred to a nylon membrane. Phosphorylated proteins were detected by autoradiography (upper panel). GST-tagged Sko1 proteins were detected by immunoblot using the anti-GST monoclonal antibody (lower panel). Download figure Download PowerPoint To map the phosphorylation site(s) for Hog1 in Sko1, we created several truncated SKO1 alleles, and expressed them as GST-tagged proteins in E.coli. Truncated forms of Sko1 were purified and subjected to in vitro phosphorylation by activated Hog1 (as described above). An N-terminal fragment containing the first 214 residues was able to be phosphorylated as efficiently as the full-length protein (Figure 4B, lanes 1 and 2). Furthermore, when N-terminal deletions (fragments containing from amino acids 202, 309 and 420 to 647) were tested, phosphorylation was completely abolished (Figure 4B, lanes 3, 4 and 5), indicating that the N-terminus of Sko1 was the target for Hog1 phosphorylation. Five sequences corresponding to the consensus phosphorylation site for MAPKs (Ser-Pro/Thr-Pro) are present in the region comprised between residues 1 and 202, namely Ser94 (KDSP), Ser108 (IISP), Thr113 (ILTP), Ser126 (LLSP) and Ser171 (SSSP). We created point mutant versions to replace Ser and Thr residues with Ala, and tested them for phosphorylation by Hog1. Single mutations of Ser94 and Ser171 did not alter Sko1 phosphorylation, and only when Ser108, Thr113 or Ser126 were mutated, was phosphorylation of Sko1 slightly reduced (data not shown). We then constructed several combinations of mutant sites and tested them for phosphorylation. Sko1 phosphorylation was only abolished in the SKO1(E) mutant, which contains mutations in all three sites, Ser108, Thr113 and Ser126 (Figure 4C). In vivo phosphorylation assays, carried out as described previously, in wild-type cells transformed with a wild-type HA-tagged Sko1 or the mutant HA–SKO1(E) protein, demonstrated that mutation of the three sites in the SKO1(E) allele eliminated most of the mobility shift due to phosphorylation of Sko1 in response to osmotic stress (Figure 5). Figure 5.In vivo phosphorylation of Sko1 mutant proteins. Wild-type or hog1Δ cells were transformed with HA-tagged wild-type Sko1 (SKO1), the Sko1 mutant in the Hog1 phosphorylation sites [SKO1(E)], the Sko1 mutant in the PKA phosphorylation sites [SKO1(M)] or the Sko1 mutant in both Hog1 and PKA phosphorylation sites [SKO1(EM)]. Cells were grown in the presence of galactose for 4 h and samples were taken before (−) or 5 min after (+) the addition of NaCl to a final concentration of 0.4 M, and the extracts were treated (+) or not (−) with 10 U of alkaline phosphatase (AP). HA–SKO1 was detected by immunoblotting using anti-HA monoclonal antibody (12CA5). Download figure Download PowerPoint Taken together, these results indicate that there is a specific cluster of three phosphorylation sites for Hog1, within 19 amino acids, in the N-terminus of Sko1 (depicted in Figure 6). Figure 6.Schematic overview of the phosphorylation sites in the Sko1 protein. Three Hog1 phosphorylation sites are present in the N-terminus of Sko1, whereas three PKA phosphorylation sites are located near the bZIP structural domain. (E) and (M) triple mutations, which correspond to the Hog1 and PKA phosphorylation sites, are indicated. Download figure Download PowerPoint Sko1 is phosphorylated by PKA near the bZIP structural domain SKO1 has been cloned as a multicopy suppressor of the growth defect caused by high PKA activity (Nehlin et al., 1992), although the connection between Sko1 and PKA remained undefined. Several putative PKA consensus motifs are present in Sko1. Thus, we tested whether Sko1 could be phosphorylated by PKA, using purified proteins in an in vitro kinase assay. Indeed, when wild-type GST-tagged Sko1 purified from E.coli was incubated with PKA in the presence of kinase buffer and [γ-32P]ATP, phosphorylation of Sko1 was observed (Figure 7A, lane 1). Figure 7.Sko1 is phosphorylated by PKA in vitro. (A) PKA phosphorylates the region between residues 309 and 420 of Sko1. Full-length or various Sko1 fragments were tested by their ability to be phosphorylated by PKA. Sko1 recombinant tagged proteins were purified from E.coli as described in Materials and methods, and incubated with PKA in the presence of kinase buffer and radioactive ATP. Phosphorylated proteins were resolved by SDS–PAGE and detected by autoradiography. The positions of the Sko1 fragments included in the constructs are indicated in parentheses. (B) Mutation of Sko1 Ser380, Ser393 and Ser399 to Ala abolishes PKA phosphorylation. Full-length Sko1 and the triple mutant SKO1(M) protein (mutant in Ser380, Thr393 and Ser399) were tested for PKA phosphorylation as in (A). After phosphorylation, proteins were resolved by SDS–PAGE and transferred to a nylon membrane. Phosphorylated proteins were detected by autoradiography (upper panel). GST-tagged Sko1 proteins were detected by immunoblot using the anti-GST monoclonal antibody (lower panel). Download figure Download PowerPoint To map the phosphorylation site(s) for PKA in Sko1, we subjected to in vitro phosphorylation several truncated SKO1 alleles, expressed and purified as GST-tagged proteins from E.coli. Neither an N-terminal fragment (containing 314 amino acids) nor a C-terminal fragment (containing the last 227 residues) was able to be phosphorylated by PKA (Figure 7B, lanes 6 and 5). Moreover, a GST fusion protein containing amino acids 309–647 was phosphorylated as efficiently as the full-length protein, indicating that phosphorylation of Sko1 by PKA occurred in a segment of the protein between amino acids 309 and 420. Three sequences corresponding to the canonical phosphorylation site for PKA (RXXS/T) are present in that region: Ser380 (RRMS), Ser393 (RKNS) and Ser399 (RKNS). We created point mutant versions to replace these Ser residues with Ala, and tested them for phosphorylation by PKA. Single mutation of any residue only slightly diminished Sko1 phosphorylation by PKA (data not shown). We then constructed several combinations of mutant sites and tested for phosphorylation. As shown in Figure 7B, phosphorylation of Sko1 by PKA was completely abolished only in the SKO1(M) mutant version, which contains mutations in all three serines (Ser380, Ser393 and Ser399). This indicates that there is a cluster of three phosphorylation sites for PKA (within 20 amino acids) near the bZIP domain of Sko1 (depicted in Figure 6). In vivo phosphorylation assays, carried out as described previously, in wild-type cells transformed with a wild-type HA-tagged Sko1 or the mutant HA-tagged SKO1(M) allele demonstrated that mutation of the three PKA sites in the SKO1(M) allele decreased the Hog1-dependent phosphorylation of Sko1 in response to osmotic stress (Figure 5), as suggested by the absence of changes in protein migration upon stress. Consistently, a Sko1 protein containing mutations in both PKA and Hog1 phosphorylation sites [SKO1(EM)] was unable to be phosphorylated at all upon osmotic stress (Figure 5). Hog1 phosphorylations regulate Sko1-mediated gene repression in vivo Having found that Hog1 phosphorylates Sko1 after osmotic shock at three specific sites, we aimed at identifying the role of these phosphorylations in Sko1-mediated transcriptional repression in vivo. GST–SKO1 (wild type) and GST–SKO1(E) (unphosphorylatable by Hog1) were, therefore, expressed from yeast expression vector pYEX-4T, and the effect on transcription was measured by northern analysis of the Sko1-dependent GRE2 gene. As shown in Figure 8A, the deregulated GRE2 expression pattern of sko1Δ mutants is completely restored to wild-type levels when GST–SKO1 is expressed. We therefore concluded that the GST–SKO1 protein we used in this study functionally replaced the endogenous Sko1. Expression of GST–SKO1(E), which is no longer phosphorylatable by Hog1, resulted in a stronger repression of GRE2 and HAL1 transcript levels (Figure 8A). This enhanced repression was already observed under non-stress conditions, but was even more evident when the cells were treated with 0.4 M NaCl. This result indicated that the Hog1 phosphorylation sites identified by in vitro kinase assays indeed play a functional role in regulating Sko1 repressor activity. There is still some regulation of Sko1, independent of these sites, in agreement with the residual phosphorylation of SKO1(E) in response to osmotic stress (Figure 5). Figure 8.Hog1 and PKA phosphorylations modulate Sko1-mediated repression in vivo. Yeast strains were transformed with the empty vector pYEX-4T (control) or the wild-type GST–Sko1 fusion (SKO1), the GST–Sko1 mutant allele in the Hog1 phosphorylation sites [SKO1(E)], the GST–Sko1 mutant allele in the PKA phosphorylation sites [SKO1(M)] or the GST–Sko1 mutant allele in both Hog1 and PKA phosphorylation sites [SKO1(EM)]. Cells were grown selectively to mid-log phase and then subjected (+) or not (−) to brief osmotic shock (0.4 M NaCl, 10 min). Total RNA was assayed by northern blot analysis for transcript levels of GRE2, HAL1 and TBP1. The induction factor represents the degree of induction plus or minus stress. The different small blots presented as well as the quantification data come from the same original blot for each mutant. (A) Hog1 phosphorylation sites are important for release from Sko1-mediated repression. GST–Sko1 fusions were expressed in wild type (W303-1A) and Δsko1 (MAP19). (B) Sko1-mediated derepression is controlled by Hog1. GST–Sko1 fusions were expressed in Δsko1Δhog1 (MAP33) cells. (C) PKA phosphorylation sites modulate Sko1 function in cells with high PKA activity. GST–Sko1 fusions were expressed in Δsko1Δbcy1 (MAP44) cells. The amount of Sko1 protein was similar for the different alleles and was not altered when cells were bcy1Δ (data not shown). Download figure Download PowerPoint To test whether the observed difference in GRE2 expression by SKO1(E), as compared with wild-type Sko1, was dependent on Hog1 we repeated the above experiment expressing both fusions in a sko1Δ hog1Δ background. Accordingly we found that Sko1 (wild type) and Sko1(E) strongly and equally repressed the expression of GRE2 (Figure 8B). Therefore, the residual osmotic regulation of Sko1(E) is dependent on Hog1. As no Hog1 sites are present in Sko1(E), this suggests that, in addition to phosphorylating Sko1 directly, Hog1 also acts indirectly over the transcriptional regulator, perhaps through an intermediate kinase (see next section). As depicted in Figure 8A, lower panel, very similar results were obtained by northern analysis of another osmolarity-responsive gene, HAL1. High PKA activity modulates Sko1 function As a result of our in vitro kinase assays, a cluster of three consensus sites within Sko1 that are phosphorylated by PKA was identified. To test for the effect of these phosphorylations on Sko1-regulated stress gene expression we expressed GST–SKO1(M) (unphosphorylatable by PKA) in sko1Δ cells and compared its effect on GRE2 transcription with that of wild-type GST–SKO1. As shown in Figure 8A, GST–SKO1(M) and GST–SKO1 equally restored the salt-regulated expression pattern of GRE2. Therefore, the elimination of PKA phosphorylation sites, unlike the Hog1 phosphorylation sites, revealed no obvious phenotype concerning Sko1-regulated gene expression under these conditions (Figure 8A). We then tested whether high cellular PKA activity, achieved by disruption of the negative regulator BCY1, had an effect on Sko1-mediated repression. We expressed GST–SKO1 (wild type and all point mutated alleles) in sko1Δbcy1Δ cells and quantified GRE2 transcription. As illustrated in Figure 8C, high PKA activity only mildly affected the stress-regulated expression of GRE2 when SKO1 (wild type) was present. However, when Hog1 phosphorylation sites were removed [SKO1(E) mutant], a complete repression of GRE2 transcription, much more pronounced than in sko1Δ cells, was observed [compare SKO1(E) in Figure 8A and C]. This led to the conclusion that high PKA activity increases Sko1-mediated repression when the Hog1 phosphorylation sites are absent. To confirm that the PKA-mediated modulation of gene expression was triggered by the PKA sites identified in Sko1, we tested the effect of the elimination of the PKA phosphorylation sites in the SKO1(E) allele by expressing the SKO1(EM) allele in yeast. Indeed, by additional delet
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