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Protein Kinase A Regulates Sexual Development and Gluconeogenesis through Phosphorylation of the Zn Finger Transcriptional Activator Rst2p in Fission Yeast

Department of Biophysics and Biochemistry, Graduate School of Science, University of Tokyo, Hongo, Tokyo 113-0033, Japan

Received 12 June 2001/ Returned for modification 26 July 2001/ Accepted 26 September 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

 
Protein kinase A (PKAi a cyclic AMP-dependent protein kinase) negatively regulates sexual development and gluconeogenesis in fission yeast by suppressing the transcription of ste11 required for the former and the transcription of fbp1 required for the latter. Here we show that Rst2p, a zinc finger protein that can bind to the upstream region of ste11 and fbp1 via the STREP motif, mediates the activity of PKA to transcription of these genes. A simple reporter system confirmed that PKA could cause its negative effect on transcription through the combination of Rst2p and STREP. Rst2p was phosphorylated by PKA in vitro at two consensus sequences on it. Substitution of the target threonine residues by alanine made the protein active even in the presence of high PKA activity. Rst2p underwent hyperphosphorylation in the medium lacking glucose, and PKA inhibited this hyperphosphorylation. Rst2p was mainly cytoplasmic under high PKA activity but was concentrated in the nucleus when this activity was lowered, suggesting that PKA might regulate ste11 and fbp1 negatively by excluding Rst2p from the nucleus. However, the shift of Rst2p localization was not perfect under physiological conditions, leaving the possibility that PKA inhibits Rst2p function in another way as well. Although the PKA-Rst2p-STREP pathway is apparently central to the regulation of ste11 and fbp1 transcription in accordance with nutritional conditions, some additional paths are likely to connect nitrogen to repression of ste11 and glucose to repression of fbp1. These paths may ensure the specificity between the type of nutrients in shortage and the type of genes to be expressed.

	INTRODUCTION

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The level of intracellular cyclic AMP (cAMP) changes in accordance with environmental conditions in various organisms. In eukaryotic cells, the major target of cAMP is cAMP-dependent protein kinase A (PKA), and the activity of PKA plays a pivotal role in the regulation of adaptation to the external conditions and the induction of intrinsic cellular differentiation. In both fission yeast and budding yeast, the level of intracellular cAMP is kept high during mitotic growth. Conditions unfavorable for growth cause downregulation of PKA in these microbes, which triggers adaptation to the adverse conditions and the beginning of sexual reproduction. Gross changes in gene expression accompany these responses, indicating that many transcription factors are likely to be regulated by PKA either directly or indirectly.

The fission yeast ste11 gene encodes an HMG transcription factor, which is responsible for expression of many genes required for the initiation of sexual development (35; reviewed in reference 43). Expression of ste11 is under the regulation of PKA. A decrease in the PKA activity, which naturally results from starvation of environmental nutrients, triggers ste11 expression. Another fission yeast gene well characterized as a target of PKA is fbp1, which encodes fructose-1,6-bis-phosphatase (FBPase), a key enzyme in gluconeogenesis (39). Glucose starvation induces fbp1 expression via a reduction of the PKA activity (3, 14, 28). Glucose is known to repress expression of many genes besides the one encoding FBPase in various cell systems, which include genes involved in alternate sugar metabolism, the tricarboxylic acid cycle, respiration, gluconeogenesis, and mitochondrial functions. The entire mechanism of glucose repression remains to be elucidated in both budding yeast and fission yeast, as well as in other eukaryotes. However, it has been established in budding yeast that transcription of the genes for alcohol dehydrogenase II and invertase partly depends on Adr1p (5) and Msn2p (8), respectively. These transcription factors are both C₂H₂ Zn finger proteins and are negatively regulated by PKA (4, 12, 33, 37). In fission yeast, both the PKA pathway (3, 28) and the stress-responsive mitogen-activated protein kinase (MAPK) pathway (34, 36) have been shown to regulate transcription of fbp1 (27), which is also the case with ste11 (18, 19, 30, 36). PKA is an inhibitory factor for expression of both ste11 and fbp1, whereas Spc1/Sty1 MAPK is a stimulatory factor for it. It has been shown, however, that Ste11p is not involved in the control of transcription of fbp1 (24).

We have demonstrated previously that transcription of ste11 is regulated directly by the gene product of rst2, namely, Rst2p (20). We isolated the rst2 gene originally as a high-copy-number suppressor of the sterility of the cgs1 mutant, in which PKA is activated constitutively (6). Genetic analysis has indicated that Rst2p functions downstream of the PKA pathway (20). Rst2p has two C₂H₂ Zn finger motifs, similar to Saccharomyces cerevisiae Adr1p, Msn2p, and Mig1p, which are transcription factors involved in glucose repression. Rst2p binds to a STRE (stress response element)-like sequence in the promoter region of ste11 (CCCCTC), which is required for the full activation of ste11 (20). We hereafter call this 6-bp element STREP (stress-starvation response element of Schizosaccharomyces pombe). Cells missing Rst2p can grow mitotically but cannot initiate sexual development.

The above observations led us to a couple of intriguing questions. Is the activity of Rst2p controlled by phosphorylation by PKA? If so, how? Does Rst2p also regulate transcription of fbp1? We address these questions and present our findings here.

	MATERIALS AND METHODS

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Yeast strains, media, and genetic methods. S. pombe strains used in this study are listed in Table 1. Cells were routinely grown on the complete medium YES (26) or the synthetic medium SD at 30°C (29). Synthetic sporulation medium SSA (7) was used to induce mating and sporulation. Two kinds of liquid minimal medium (MM) (26), modified in the carbon source, were used: MMR, containing 8% glucose, as a medium to induce glucose repression and MMD, containing 3% glycerol and 0.1% glucose, as a medium for derepression (15). General genetic methods for S. pombe were described previously (13). Protoplast fusion was performed according to the method of Sipiczki and Ferenczy (32). Transformation and gene tagging replacement were performed as described previously (2). Specific mutations were introduced into the cloned rst2 gene according to the method developed by Kunkel (21). The rst2-M3 allele was integrated into the chromosome, replacing the rst2::ura4⁺ allele of the host strain, by selecting 5'-fluoroorotic acid-resistant transformants.

ß-Galactosidase assay. Several independent colonies of each S. pombe strain transformed with a reporter plasmid were cultured in MMR to 5 x 10⁶ cells/ml. A portion of each culture was sampled, and the remainder was shifted to MMD and further cultured for 3 h before sampling. Cells were harvested by the filtration method described previously (31). The ß-galactosidase activity was determined as described n Alfa et al. (1), although the scale of the reaction was reduced to 60% in volume. At least three independent measurements were done for each type of host strain because the copy number of the reporter plasmid might vary among transformants.

Northern blotting. Cells were harvested by filtration (31). Total RNA was extracted and RNA blot analysis was performed as described previously (40). Poly(A) RNA was selected by using oligo(dT)-cellulose (Invitrogen). We used a 1.3-kb PvuII-PvuII DNA fragment as a probe to detect ste11⁺ mRNA (35) and a PCR-amplified DNA fragment covering the whole open reading frame to detect fbp1⁺ mRNA (39).

Detection of Rst2p by Western blotting. We essentially used a previously described protocol (31), except for a few substantial modifications. Briefly, harvested cells were boiled and then disrupted with glass beads in modified buffer L, which contained 50 mM HEPES-KOH and 400 mM KCl instead of the 50 mM Tris-Cl and 400 mM NaCl used in the original protocol. Each suspension containing 20 µg of protein was separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (22). We used separating acrylamide gels (7.5 or 8.0%) with a mono/bis ratio of 29.8:0.2 to detect Rst2p and a gel (12%) with a mono/bis ratio of 29.2:0.8 to detect Cdc2p. Purified polyclonal anti-Rst2p antibodies (this study) and commercialized anti-Cdc2 antibodies (Santa Cruz Biotechnology) were used as the primary antibodies, and goat anti-rabbit immunoglobulin G (IgG) Fc fragments conjugated with horseradish peroxidase (Jackson Immunoresearch) were used as the secondary antibodies. Enhanced chemiluminescence (Amersham-Pharmacia) was used for immunodetection on the membrane.

Phosphatase treatment. Rst2p was enriched in the precipitate after centrifugation of the cell suspension described above. A precipitated sample containing 30 µg of protein was washed four times with the alkaline phosphatase buffer recommended by the manufacturer (Takara Biomedicals) and suspended thoroughly in the same buffer. Each substrate suspension received 20 U of calf intestinal alkaline phosphatase (Takara Biomedicals) and was incubated at 37°C for 60 min, either with or without the inhibitor mixture (10 mM EGTA, 0.1 M Na₃VO₄, 50 mM ß-glycerophosphate, 15 mM p-nitrophenyl phosphate). The suspension was then boiled with SDS-PAGE sample buffer and subjected to electrophoresis. Immunodetection of Rst2p was done as described above.

Phosphorylation assay in vitro. Rst2p fused with maltose-binding protein (MBP), together with variants of this fusion protein carrying mutations in the PKA target sites, was produced in bacteria by using expression vector pMAL-cRI (New England Biolabs). The fusion proteins were extracted in buffer E, which contained 25 mM HEPES-KOH (pH 7.5), 600 mM KCl, 1 mM EDTA, 10% glycerol, 1 mM dithiothreitol, 1 mM phenylmethylsulfonyl fluoride, and 1 protease inhibitor cocktail tablet per 10 ml (Complete Mini; Roche Diagnostics). Affinity purification of the MBP fusion proteins was done according to the protocol provided by the manufacturer, except that buffer E was used as the solvent. S. pombe cells producing hemagglutinin (HA)-tagged PKA catalytic subunit (Pka1p) were disrupted with glass beads in buffer I (50 mM Tris-Cl [pH 7.5], 150 mM KCl, 10 mM MgCl₂, 1 mM EDTA, 1 mM dithiothreitol, 25 mM ß-glycerophosphate, 0.1 mM Na₃VO₄, and 1 mM phenylmethylsulfonyl fluoride, supplemented with the protease inhibitor cocktail). HA-Pka1p was immunoprecipitated with monoclonal anti-HA antibody 16B12 (Berkeley Antibody Co.) and protein G-Sepharose (Amersham-Pharmacia). The Sepharose beads were washed twice with buffer I and then washed twice with buffer K (20 mM HEPES-KOH [pH 7.6], 20 mM MgCl₂, 1 mM dithiothreitol, 25 mM ß-glycerophosphate, 0.1 mM Na₃VO₄). About 1 µg of each substrate (MBP-Rst2p) was added to the tube containing immunoprecipitated HA-Pka1p, and the phosphorylation reaction mix was adjusted to the scale of 20 µl with buffer K, which contained 20 µM cold ATP and 5 µCi of [-³²P]ATP (ICN Biomedicals). The reaction mix was incubated for 20 min at room temperature and then boiled with SDS-PAGE sample buffer. The PKA inhibitor PKI was purchased from Sigma.

Fluorescence microscopy. Methanol fixation and indirect immunostaining of S. pombe cells were done essentially according to the method of Gaits et al. (10). HA-tagged Rst2p was stained with anti-HA epitope monoclonal antibody 16B12 as the primary antibody and Alexa 568-conjugated anti-mouse IgG goat antibodies (Molecular Probes) as the secondary antibodies, whereas green fluorescent protein (GFP) was detected by its own fluorescence expressed in living cells. DNA was counterstained with Hoechst 33342. Fluorescence microscopy was performed by using an Axiophoto microscope (Carl Zeiss) with appropriate filters. To optimize expression of Rst2p-3HA from the nmt1 promoter on a multicopy plasmid, cells were first grown to the exponential phase in SD medium, which contained 1.2 µM thiamine, then washed twice with thiamine-free MMR, and finally resuspended in MMR at the concentration of 5 x 10⁶ cells/ml. The suspension was diluted 32-fold with MMR, and cells were grown for five generations before fixation with methanol. A portion of the cells was further shifted to and incubated in the glycerol medium before fixation.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

 
Rst2p is a common transcription factor for the cAMP-repressible genes ste11 and fbp1. Rst2p is a transcription factor for ste11⁺, which functions downstream of the PKA pathway (20). We suspected that Rst2p might also regulate expression of fbp1⁺, another gene known to be controlled by PKA in fission yeast (3, 14, 28). We thus examined growth of the rst2 strain on nonfermentable carbon sources. Expression of fbp1⁺, encoding FBPase, is required to assimilate nonfermentable carbon sources and is induced sharply under such nutritional conditions (39). Without FBPase, cells cannot generate glucose from nonfermentable carbon sources via gluconeogenesis and hence fail to proliferate. The rst2 strain grew very poorly compared to the wild-type strain on medium containing 3% glycerol and 0.1% glucose (data not shown). A trace amount of glucose was added in this assay because S. pombe cells did not feed on glycerol alone for an unclear reason. A more obvious difference was seen on medium containing 3% gluconate, where the wild-type strain grew robustly but the rst2 strain did not grow at all (data not shown).

To demonstrate the necessity of Rst2p for transcription of fbp1 more directly, we measured the level of fbp1 mRNA in rst2⁺ and rst2 cells by Northern blotting. As shown in Fig. 1A, fbp1 mRNA accumulated significantly in wild-type cells 1 h after the shift from the repression medium (MMR; see Materials and Methods) to the derepression medium (MMD). In contrast, no fbp1 mRNA was detected in rst2 cells, indicating that Rst2p was essential to express fbp1. Scanning of the promoter region of fbp1 revealed one STREP (CCCCTC), the consensus motif for Rst2p binding, at nucleotides -262 to -257 (Fig. 1B). A recent study has shown that this sequence is positioned in a cis regulatory element of fbp1 designated UAS2 (27). We prepared a double-stranded oligonucleotide harboring this sequence (nucleotides -273 to -249) and showed that Rst2p could bind to it in a gel shift assay (data not shown), as was demonstrated with the ste11 upstream sequence (20). These observations strongly suggest that Rst2p is a transcriptional activator of both fbp1 and ste11 and functions via binding to STREP in both cases.

View larger version (37K): [in this window] [in a new window]   FIG. 1. The rst2 gene function is required for transcription of the fbp1 gene. (A) Induction of fbp1 transcription by a medium shift. Cells, either rst2+ (JY333) or rst2 (JX233), were grown in MMR containing 8% glucose to a concentration of 5 x 106 cells/ml and then shifted to MMD containing 3% glycerol and 0.1% glucose. Cells were then harvested at the indicated times after the shift, and the expression of fbp1 and leu1 as an internal control was examined by Northern blotting. RNA (5 µg) was loaded in each lane after denaturation by formamide. (B) Alignment of STREP sequences, recognized by Rst2p, in the upstream activation regions of ste11 and fbp1. The numbers refer to positions relative to the transcriptional start.

View larger version (41K): [in this window] [in a new window]   FIG. 2. Effects of PKA-related mutations on expression of ste11 and fbp1. (A) To examine ste11 expression, cells of each genotype indicated (wild type [wt], JY333; rst2, JX233; cgs1, JX222; pka1, JX384; pka1 rst2, JX282) were grown in MM supplemented with ammonium chloride (+), and some of them were subjected to starvation of nitrogen for 2 h (-). Total RNA was extracted from each preparation and analyzed by Northern blotting. RNA (5 µg) was loaded in each lane after denaturation by formamide. Expression of ste11 and leu1 was detected by appropriate probes. (B) To examine fbp1 expression, cells of each strain (the same as in panel A) were grown in glucose-based MMR (R), and some of them were shifted to glycerol-based MMD (D) and incubated for 1 h. Expression of fbp1 was detected as described in panel A.

View larger version (21K): [in this window] [in a new window]   FIG. 3. An Rst2p- and STREP-dependent reporter system. The lacZ-reporter plasmids used here are constructed as described in Materials and Methods. Various strains as indicated (as defined in Fig. 2) were transformed with a reporter plasmid carrying either the perfect or a mutated STREP sequence. Lysates were prepared from cells grown in MMR (open bars) or derepressed in MMD for 3 h (shaded bars). An assay of ß-galactosidase activity was done as described in Materials and Methods. An average of at least three independent measurements, performed with stable transformants, is shown for each case.

View larger version (33K): [in this window] [in a new window]   FIG. 4. Rst2p activity is likely to be regulated posttranscriptionally. (A) Detection of rst2 mRNA and the gene product before and after a medium shift. To determine the level of rst2 mRNA, extracts were prepared from cells grown in MMD for the indicated duration, as detailed in Fig. 1. Poly(A) RNA was selected from each sample and subjected to gel electrophoresis after denaturation with formamide. We detected leu1 mRNA as an internal loading control (the time for exposure on X-ray film is much shorter than that for rst2 mRNA). For analysis of protein, boiled cell lysates were subjected to SDS-PAGE, followed by immunoblot analysis as described in Materials and Methods. (B) Phosphatase treatment of Rst2p. Protein precipitates prepared from JY333 cells either growing in MMR or incubated in MMD for 1 h were treated with calf intestinal alkaline phosphatase (CIP), with or without the addition of the inhibitor mix, and subjected to SDS-PAGE and immunoblot analysis. (C) Detection of wild-type and mutated Rst2p in PKA-related mutant cells under repressing or derepressing conditions. The M3 mutant form of Rst2p lacks phosphorylatable residues at the two putative PKA-target sites. Cells of JX233 (rst2), JY333 (WT), JW373 (rst2-M3), JX222 (cgs1), JW374 (cgs1 rst2-M3), JX384 (pka1), and JW377 (pka1 rst2-M3) were grown in MMR. A portion of each culture was shifted to MMD and incubated for 1 h. Cell lysates were prepared from the cultures in MMR and MMD and then subjected to SDS-PAGE and immunoblot analysis.

Rst2p derived from repressed cells was subjected to a similar phosphatase treatment (Fig. 4B, lanes 1 to 3). Analysis by SDS-PAGE by using a soft gel (7.5%), as shown here, revealed that Rst2p under the repressing conditions existed in two forms, giving two close but separable bands in electrophoresis (lanes 1 and 3). Rst2p treated by phosphatase appeared to give only the lower band (lane 2). Because the intracellular PKA activity was supposed to be high in the repression medium, we suspected the possibility that the upper band represented Rst2p phosphorylated by PKA. Two lines of evidence, however, denied this possibility. One was that we could detect these two bands in cgs1 (PKA-active) cells just as in wild-type cells (Fig. 4C, lane 2 versus lane 4). The other was that a mutant form of Rst2p that lacked the PKA target sites (M3; see below) still gave the two bands in both wild-type and cgs1 cells (lanes 3 and 5). Thus, we presume that the upper band represents a phosphorylated form of Rst2p but that PKA is not responsible for this phosphorylation.

PKA phosphorylates Rst2p in vitro. Rst2p carried putative PKA target sequences in the vicinity of the zinc finger motifs and in the central region (Fig. 5A). To determine whether PKA could phosphorylate Rst2p in vitro, we performed an assay with bacterially expressed recombinant Rst2p and the catalytic subunit of fission yeast PKA, namely, Pka1p. Pka1p used here was tagged with HA and purified from fission yeast cells by immunoprecipitation. We constructed MBP-Rst2p fusion proteins, bearing either the wild-type Rst2p sequence or the sequences mutated in the putative phosphorylation sites. One of the mutant forms (M1) carried two T-to-A substitutions and one S-to-A substitution in the target site close to the Zn fingers, and the other (M3) carried a T-to-A substitution in the central target site in addition to those in M1 (see Fig. 5A). As shown in Fig. 5B, the wild-type protein was efficiently phosphorylated by Pka1p in vitro (lane 1). This phosphorylation was inhibited largely by the addition of PKI peptide, a specific inhibitor of PKA (lane 2). Pka1p harboring a mutation in the kinase domain (K230R) was incapable of phosphorylation (lane 3). The M1 protein was phosphorylated to a lesser extent but still detectably (lanes 4), and the M3 protein was barely phosphorylated (lane 5). These results demonstrate that Pka1p can phosphorylate Rst2p and, furthermore, that the two presumed target sites on Rst2p assigned above are indeed the sites for phosphorylation by PKA.

View larger version (31K): [in this window] [in a new window]   FIG. 5. Phosphorylation of Rst2p by PKA in vitro. (A) Schematic diagram of Rst2p showing consensus sequences for PKA phosphorylation and a table of mutations introduced into bacterially expressed Rst2p used for in vitro phosphorylation assay. Zinc finger motifs are shown as ovals. (B) Audoradiogram showing phosphorylation of bacterially expressed Rst2p, fused with MBP. The engineered proteins were incubated with [-32P]ATP and PKA immunoprecipitated from fission yeast cells. A kinase-negative PKA variant (K230R) was used in lane 3. The PKA inhibitor 5-24 (PKI) was added to lane 2.

We then investigated effects of the M3 mutation on hyperphosphorylation of Rst2p. Whereas the wild-type Rst2p was not hyperphosphorylated in the repression medium (Fig. 4A, lane 1, and Fig. 4C, lane 2), the M3 mutant was partially hyperphosphorylated in the same medium (Fig. 4C, lane 3). Notably, the pattern of slow-moving bands exhibited by the M3 mutant here was quite similar to those of the wild-type Rst2p and the M3 mutant in PKA-defective cells under the repressing conditions (lane 3 versus lanes 6 and 7). Furthermore, the M3 mutant was phosphorylated more extensively than the wild-type Rst2p in PKA-active cells under the derepressing conditions (lane 12 versus lane 11). These results suggest strongly that PKA suppresses hyperphosphorylation of Rst2p through phosphorylation of its target sites, which are mutated in M3. The data shown in Fig. 4C also suggest that, besides the absence of this direct phosphorylation by PKA, two conditions are essential for the kinase(s) responsible for hyperphosphorylation of Rst2p to become fully active (or the phosphatase to become fully inactive). One is depletion of glucose from the medium (as typically deduced from lane 7), and the other is reduction of the cellular PKA activity below a certain threshold (as typically deduced from lane 12).

Mutations in the phosphorylation sites activate Rst2p ectopically. We investigated biological consequences of mutations introduced into the phosphorylation sites on Rst2p. Cells moderately expressing the rst2-M3 allele showed markedly slow growth and flocculation in a synthetic medium, which contained a sufficient amount of nitrogen to suppress sexual development of wild-type cells. The rst2-M3 strain grew even more slowly than the pka1 strain, which has been shown to grow poorly (24). Inhibition of cell growth by the rst2-M3 mutation was less severe in the cgs1 background, although the reason for this suppression is unclear.

To see the effects of the M1 and M3 mutations on sexual development, we transformed homothallic rst2 cells, whose genetic background was either cgs1⁺ or cgs1, with a multicopy plasmid carrying each rst2 allele connected to the weak nmt1 promoter. The M2 mutation, which harbored a single T-to-A substitution in the central target site, was also examined. Each transformant was grown on SD medium, which represses the nmt1 promoter, and a portion was restreaked on SSA medium, which induced sexual development due to the scarcity of the nitrogen source and also derepresses the nmt1 promoter due to the lack of thiamine. The results are summarized in Fig. 6. When the host cells were cgs1⁺, the wild-type and the mutant rst2 alleles were equally active in the overall induction of sporulation, as assayed by iodine staining (Fig. 6A). A microscopic measurement of the conjugation efficiency of the same samples confirmed that they were nearly equivalent (Fig. 6B). However, when the host cells were cgs1, differences arose among them. The wild-type allele could recover neither overall sporulation (Fig. 6A) nor conjugation (Fig. 6C) in cgs1 rst2 cells. However, each mutant allele could do so, although not very strongly (Fig. 6A,C). The double-mutant allele, M3, was the most active, and the M1 allele appeared to be more active than M2 (Fig. 6A and C).

View larger version (53K): [in this window] [in a new window]   FIG. 6. Unphosphorylatable mutations in the PKA target sites enhances the activity of Rst2p. (A) Iodine-staining assay of sporulation efficiency in various rst2 transformants. Cells of JX231 (h90 cgs1+ rst2) and JW487 (h90 cgs1 rst2) were transformed with pREP81-based plasmids carrying each allele as indicated on the left. They were incubated in patches on SSA plates for 4 days and stained with iodine vapor, which turns sporulated cells dark brown. JY450 cells transformed with the vector plasmid were used as a control. (B) JX231 transformants, shown in panel A, were examined microscopically for their conjugation efficiency. (C) JW487 transformants, shown in panel A, were examined microscopically for their conjugation efficiency. (D) Restoration of ste11 transcription in cgs1 cells by the rst2-M3 allele. Total RNA was prepared from heterothallic (h-) cgs1+ rst2 (JX233) or cgs1 rst2 (JX261) cells transformed with a pREP81-based plasmid carrying either the rst2+ or the rst2-M3 allele. Cells were either growing exponentially in MM (+) or were subjected to nitrogen starvation for 4 h (-). RNA (5 µg) was loaded in each lane after denaturation by formamide and analyzed by Northern blotting. Expression of cam1 and plasmid-borne rst2 was measured as an internal control and for confirmation, respectively.

Rst2p undergoes nucleocytoplasmic shuttling. We investigated subcellular localization of Rst2p. To visualize Rst2p, we tagged this protein with three copies of the HA epitope, and cells producing HA-tagged Rst2p from the fusion gene on the chromosome were stained with anti-HA. The results indicated that Rst2p was cytoplasmic almost exclusively under the repressing conditions (Fig. 7A, R panels). However, it was mainly nuclear under the derepressing conditions (Fig. 7A, D panels). A more statistical discussion will be given below. Essentially the same results were obtained when Rst2p was visualized by the conjugation of the jellyfish GFP (data not shown). A dynamic nature of Rst2p was investigated by using a strain that carried the rst2-GFP fusion gene on the chromosome (JW352). JW352 cells were adapted in MMD for 1 h so that Rst2p-GFP was accumulated in the nucleus, and we applied glucose to these cells at the final concentration of 4%. This caused rapid disappearance of much of the fluorescence from the nucleus (Fig. 7B). This disappearance was blocked by the simultaneous application of leptomycin B, an inhibitor of nuclear export (reviewed in reference 38) (Fig. 7B). GFP alone was distributed throughout the cytoplasm and the nucleus and did not exhibit such a dynamic change in localization in response to glucose (data not shown). These results indicate that Rst2p can undergo nucleocytoplasmic shuttling and that glucose either promotes its export from the nucleus or inhibits its import to the nucleus.

View larger version (75K): [in this window] [in a new window]   FIG. 7. Effects of glucose on subcellular localization of Rst2p. (A) Immunostaining of Rst2-3HAp. Cells (JW367) grown in MMR (R panels) were harvested by filtration, transferred to MMD, and incubated for 1 h (D panels). They were stained with anti-HA antibody and counterstained with Hoechst 33342 to visualize the DNA. (B) Addition of glucose promotes exclusion of Rst2p from the nucleus. JW352 cells expressing Rst2p-GFP were adapted in MMD for an hour (no addition). Glucose was added to a portion of the culture to the final concentration of 4% (+Glucose). To block exportin-dependent nuclear export, leptomycin B (0.1 µg/ml) was added simultaneously to a portion (+Glucose +LMB). DNA was stained with Hoechst 33342. Bar, 10 µm. (C) Subcellular localization of Rst2p-GFP in PKA-related mutants. Cells of JW363 lacking PKA (pka1) and cells of JW359 with constitutively active PKA (cgs1), both of which were grown in MM, were observed for GFP fluorescence. Cells of JW355 lacking adenylyl cyclase were first grown in MM containing 2 mM cAMP and 5 mM caffeine to block phosphodiesterase (cyr1 + cAMP). They were filtered, transferred to cAMP-free MM, and incubated for 10 min (cyr1). DNA was stained with Hoechst 33342. The presence of caffeine somehow weakened staining of DNA by Hoechst 33342. Bars, 10 µm.

To see the effects of the M3 mutation on subcellular localization of Rst2p, we expressed HA-tagged Rst2-M3p from a multicopy plasmid in cgs1⁺ and cgs1 cells. HA-tagged Rst2p was expressed similarly as a control. When HA-tagged Rst2p was produced in cgs1⁺ cells, less than 20% of the cells exhibited nuclear accumulation of the protein under the repressing conditions (in MMR), whereas nearly 70% did so under the derepressing conditions (in MMD) (Fig. 8). In contrast, more than 30% of the cells exhibited nuclear accumulation of HA-tagged Rst2-M3p under the repressing conditions, and ca. 50% did so under the derepressing conditions (Fig. 8). These observations suggest that phosphorylation at the two PKA target sites on Rst2p, which are mutated in M3, may be pertinent with nuclear exclusion of the protein. However, the data also imply that PKA affects localization of Rst2p not only through phosphorylation of these sites but also in an additional way(s). Curiously, Rst2-M3p showed highly efficient nuclear accumulation in cgs1 cells placed under the repressing conditions (Fig. 8). The wild-type Rst2p showed extensive cytoplasmic localization in cgs1 cells under the same conditions (Fig. 8). These observations suggest that PKA regulates subcellular localization of Rst2p in a complex manner, probably involving as-yet-unidentified factors.

View larger version (71K): [in this window] [in a new window]   FIG. 8. Quantitative measurements of subcellular localization of the wild-type Rst2p and the M3 mutant under the repressing and derepressing conditions. Rst2p and Rst2-M3p, both tagged with HA, were expressed from the expression vector pREP81 in cells that were either cgs1+ rst2 (JX 233) or cgs1 rst2 (JX 261). Cells cultured in MMR or shifted to MMD (30 min) were stained with anti-HA antibody, and the percentage of cells showing clear nuclear accumulation of Rst2p was culculated for each sample. Bar, 10 µm.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

If fission yeast cells lose the PKA activity completely, which is an unnatural condition realized only in the pka1 or cyr1 strain, the expression of both ste11 and fbp1 becomes constitutive regardless of the nutritional conditions. On the contrary, their expression is always suppressed in the cgs1 strain sustaining high PKA activity. Our analysis has shown that Rst2p lacking the PKA target sites (M3) can cause effects similar to those of the loss of PKA activity with respect to hyperphosphorylation of the protein and can promote ste11 transcription in cgs1 cells starved for nitrogen. These observations strongly suggest that Rst2p is a substrate of PKA in vivo. However, the mutant form of Rst2p cannot induce ste11 transcription in the presence of ample nitrogen, although the complete loss of PKA activity can do so. In other words, the M3 mutant does not replace the loss of PKA completely in induction of ste11 expression. Furthermore, the results presented in Fig. 2, lanes 3 through 6, indicate that nitrogen can yet affect expression of ste11 to some extent independent of the PKA-Rst2 pathway, as has been inferred in previous studies (18, 20, 30, 36, 41). Taking these results together, we propose the scheme shown in Fig. 9 as the most rational based on current knowledge. In this scheme, phosphorylation of Rst2p by PKA serves as the major switch to turn off ste11 expression, but there are additional negative regulatory pathways that bypass Rst2p, one connecting the nitrogen source to ste11 expression and another connecting PKA to ste11 expression.

View larger version (14K): [in this window] [in a new window]   FIG. 9. Diagram of the regulatory network involving the PKA-Rst2p pathway for transcriptional activation of ste11 and fbp1. The pathway established in this study is shown in thick lines. Other possible paths are shown in thin lines.

A portion of Rst2p is phosphorylated in wild-type cells grown in MMR, but PKA, which is supposed to be active in these cells, does not appear to be responsible for this phosphorylation, as discussed in Results. We have thus far been unsuccessful in detecting in vivo phosphorylation of Rst2p by PKA as a shift of the mobility of the protein in gel electrophoresis. However, the results of mutational analysis suggest strongly that PKA affects the activity of Rst2p through both direct phosphorylation and indirect modification. Thus, biochemical evidence is awaited to show critically whether Rst2p is phosphorylated by PKA in living cells.

An unexpected observation is that cells expressing rst2-M3 are more impaired in vegetative growth than pka1 cells in synthetic medium, whereas they grow better than pka1 cells in rich medium. Furthermore, cgs1 suppresses the slow growth of rst2-M3 cells in synthetic medium to some extent. These observations suggest that emergence of Rst2p unphosphorylated by PKA, not precisely harmonized with the state of the PKA activity, can cause certain adverse effects on cell growth. Because both ste11 and fbp1 are unlikely to be fully expressed in rst2-M3 cells under growing conditions, these observations indicate that Rst2p is likely to have a target(s) other than these two genes, which is more closely related to growth control.

This study has revealed a clear correlation between the subcellular localization of Rst2p and the activity of PKA in the cell. When the PKA activity is high, Rst2p tends to be located in the cytoplasm. When it is low, Rst2p tends to be nuclear. Nuclear exclusion of Rst2p in the presence of glucose apparently explains why high PKA activity is inhibitory to the transcription-activating activity of Rst2p. It is currently not conclusive whether phosphorylation by PKA accelerates nuclear export or inhibits nuclear import of Rst2p. Because leptomycin B blocks nuclear export of Rst2p, it appears that Rst2p is exported from the nucleus by the exportin-dependent system. However, our attempts to identify possible nuclear localization signal or nuclear export signal on Rst2p have not been successful so far.

Although phosphorylation by PKA apparently affects nucleocytoplasmic localization of Rst2p, the shift between the cytoplasm and nucleus is never all-to-none under our experimental conditions, suggesting that the phosphorylation may also impair other aspects of Rst2p required for its transcription-activating activity. Judging from the proposed ternary structure of Zn finger domain, as reviewed by Wolfe et al. (42), the N-terminal phosphorylation site, 10 residues apart from the DNA-binding domain (Fig. 6A and C and Fig. 8), does not seem to affect the ability of Rst2p to recognize either a base or a phosphate. Rather, phosphorylated Rst2p may be impaired in the ability to activate the transcription machinery, because there lies a glutamine stretch near the phosphorylation site, as is frequently found in the activating domain of transcription factors. Further studies are necessary to clarify these possibilities.

S. cerevisiae Msn2p and Msn4p, Zn finger proteins that recognize the STRE motif, have been shown to undergo hyperphosphorylation in response to a carbon source shift and heat shock, and high PKA activity blocks this hyperphosphorylation (11). It is suspected, though not proven, that some stress-responsive kinases may be involved in this hyperphosphorylation in S. cerevisiae. Garreau et al. hypothesized further that different stresses may cause different states of hyperphosphorylation (11). It is very intriguing that transcription activators that recognize similar motifs (STRE and STREP) undergo analogous modifications in S. cerevisiae and S. pombe, which are only distantly related in phylogeny. Although the identity of the kinase(s) (and possible antagonizing phosphatase) involved in the hyperphosphorylation of Rst2p remains to be clarified, it appears likely that, in S. pombe, Rst2p undergoes hyperphosphorylation differently under depletion of glucose and depletion of nitrogen. The full activation of fbp1 and that of ste11 may require different levels of hyperphosphorylation of Rst2p. These questions remain to be answered.

	ACKNOWLEDGMENTS

 
We thank N. Jones for helpful advice and plasmids.

This work was supported by a Grant-in-Aid for Specially Promoted Research from the Ministry of Education, Culture, Sports, Science, and Technology of Japan.

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Biophysics and Biochemistry, Graduate School of Science, University of Tokyo, Hongo, Tokyo 113-0033, Japan. Phone: 81-3-3814-9620. Fax: 81-3-5802-2042. E-mail address: myamamot{at}ims.u-tokyo.ac.jp.

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