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Mutations in the YRB1 Gene Encoding Yeast Ran-Binding-Protein-1 That Impair Nucleocytoplasmic Transport and Suppress Yeast Mating Defects
Markus Künzlera,b, Joshua Trueheart1,a, Claudio Settea, Eduard Hurtb, and Jeremy Thorneraa Department of Molecular and Cell Biology, Division of Biochemistry and Molecular Biology, University of California, Berkeley, California 94720-3202
b Ruprecht-Karls-Universität Heidelberg, Biochemie-Zentrum Heidelberg, D-69120 Heidelberg, Germany
Corresponding author: Markus Künzler, Ruprecht-Karls-Universität Heidelberg, Biochemie-Zentrum Heidelberg (BZH), Im Neuenheimer Feld 328, 4. OG, D-69120 Heidelberg, Germany., markus.kuenzler{at}urz.uni-heidelberg.de (E-mail)
Communicating editor: M. JOHNSTON
 | ABSTRACT |
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 TOP ABSTRACT MATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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We identified two temperature-sensitive (ts) mutations in the essential gene, YRB1, which encodes the yeast homolog of Ran-binding-protein-1 (RanBP1), a known coregulator of the Ran GTPase cycle. Both mutations result in single amino acid substitutions of evolutionarily conserved residues (A91D and R127K, respectively) in the Ran-binding domain of Yrb1. The altered proteins have reduced affinity for Ran (Gsp1) in vivo. After shift to restrictive temperature, both mutants display impaired nuclear protein import and one also reduces poly(A)+ RNA export, suggesting a primary defect in nucleocytoplasmic trafficking. Consistent with this conclusion, both yrb1ts mutations display deleterious genetic interactions with mutations in many other genes involved in nucleocytoplasmic transport, including SRP1 (
-importin) and several ß-importin family members. These yrb1ts alleles were isolated by their ability to suppress two different types of mating-defective mutants (respectively, fus1
and ste5ts), indicating that reduction in nucleocytoplasmic transport enhances mating proficiency. Indeed, in both yrb1ts mutants, Ste5 (scaffold protein for the pheromone response MAPK cascade) is mislocalized to the cytosol, even in the absence of pheromone. Also, both yrb1ts mutations suppress the mating defect of a null mutation in MSN5, which encodes the receptor for pheromone-stimulated nuclear export of Ste5. Our results suggest that reimport of Ste5 into the nucleus is important in downregulating mating response.
MATING in the yeast Saccharomyces cerevisiae is the culmination of a complex series of events required for cellular and nuclear fusion of two haploid cells of opposite mating type (
Proteins and protein-RNA complexes cross the nuclear envelope through nuclear pores comprised of 
50 different proteins, termed nucleoporins (
Transport receptors bind specifically to the GTP-bound form of Ran via a conserved domain at their N termini (140 residues (
A link between yeast mating and the Ran GTPase cycle was the identification of the srm1-1 mutation, now known to reside in RanGEF1, which suppressed the mating defect of cells lacking pheromone receptors and increased the basal expression of a pheromone-responsive reporter gene () defective in the cell fusion step of mating. Fus1 is a pheromone-induced, O-glycosylated, integral membrane protein that acts at a late stage in mating ( mutant. These data suggest that preventing efficient reimport of Ste5 after its pheromone-induced release from the nucleus sustains the mating-competent state.
| MATERIALS AND METHODS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Strains and growth conditions:
Yeast strains used in this study are listed in Table 1. Strains JTY2483 and JTY2484 were obtained by backcrossing strain 381G-42E-P1 three times against either YPH499 or YPH500. msn5::TRP1 strain HMK30 was derived from strain LH90 ( mutation deletes 90% of the coding sequence (from the FUS1 promoter to codon 460) and was constructed by a two-step gene disruption method (::HIS3 construct excised from plasmid pMK112n (Table 2). To construct strain HMK21, JTY2501 was transformed with plasmid pMK103, sporulated, and a MATa His+ Ura+ 5-fluoro-orotic acid (5-FOA)-sensitive spore was chosen. Strain JTY2486 was obtained by transformation of CRY1 with an EcoRI-SpeI fragment containing the nup2::HIS3 construct excised from plasmid pJON115 (::LEU2 construct (
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Unless indicated otherwise, yeast cells were propagated at 30°. Rich medium (YP), synthetic complete medium (SC), and synthetic minimal medium (SM) were prepared as described ( (
Quantitative mating assays:
Quantitative mating assays were performed as previously described ( tester strains were pregrown at 26° to midlogarithmic phase in selective and rich medium, respectively. Cells were washed with water and 106 cells of the MATa strains to be tested were mixed with 107 cells of the MAT tester strain. In the case of the experiment shown in Table 3, the mixture was spread directly onto precooled (14°) SMGlc plates, the plates were incubated for 3 days at 14°, and then for 3 days at room temperature. The resultant diploid colonies were counted and normalized to the titer of input MATa cells (determined by plating the same dilutions on plates selective for the MATa strain to be tested and incubating for 3 days at room temperature). In the case of the experiment shown in Table 5, the mating mixture was collected on a 0.45-µm pore filter and incubated for 6 hr at 30° on YPGlc. After the incubation, cells were resuspended in SMGlc medium and plated in appropriate dilutions onto SMGlc plates with appropriate nutrients to select for diploids. As a control for the number of viable MATa cells used in the mating mixture, 106 cells of the MATa cells were collected on a separate filter, incubated as above, resuspended in YPGlc, and plated on YPGlc plates at appropriate dilutions. Mating efficiency was expressed as percentage of the input MATa haploids that formed diploid colonies.
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Isolation of yrb1-51:
JTY2024 (MATa fus1) was mutagenized with ethyl methanesulfonate (108 cells/ml; 3% EMS; 1 hr) to 25% survival, and spread on YPGlc plates. After 3 days at 28°, 72,000 colonies were replica plated onto precooled (14°) SMGlc plates containing uracil (20 mg/liter), on which 2 A600 nm units of JY416 (MAT fus1) cells had been spread. These plates were incubated for 4 days at 14°. Candidate clones that gave a positive mating response (35 colonies total) were restreaked from the master plate, retested for suppression, and examined for their ability to grow at various temperatures. A single isolate (JTY2025) displayed a ts phenotype that cosegregated with the ability to suppress the mating defect of the fus1 cells at 14° (data not shown). The mutation conferring these phenotypes was initially named sfo1-1 (suppressor of fus one). In the course of these crosses, it was shown, first, that sfo1 was tightly linked to trp1 (no recombinants in 31 tetrads; distance 
1.6 cM) and, second, by complementation tests, that the sfo1-1 mutation was allelic to stp52, another suppressor of mating defects that was mapped to the same region (
Recovery and analysis of yrb1ts alleles:
The base sequence alterations corresponding to the yrb1-51 and yrb1-52 mutations were determined by cloning and sequencing of DNA isolated from the mutants. The polymerase chain reaction (PCR) was used to amplify 636-bp products comprising the entire YRB1 open reading frame (ORF) using genomic DNA from JTY2026 (yrb1-51) and 381G-42E-P1 (yrb1-52) as the template and oligonucleotide primers, 5'-GGG GAT CCG AAT GTC TAG CGA AGA TAA G-3' (OSFO1) and 5'-GGT CTA GAC GCA AGT AAC AAG C-3' (OSFO5), which corresponded, respectively, to positions -2 to +18 and +635 to +616 of the 201-codon YRB1 sequence (where +1 is the first base of the initiator codon of the ORF) and included restriction sites at their 5'-ends to facilitate cloning of the PCR products. Reaction products were isolated, digested with BamHI and XbaI, and inserted into E. coli vector pUC19 for sequencing. Nucleotide sequence of multiple inserts was determined on both strands using the M13/pUC universal and M13/pUC reverse sequencing primers (New England Biolabs, Beverly, MA) and, when necessary, sequence-specific primers. The single-base-pair mutations recovered were tested for their ability to confer a ts phenotype by first substituting the mutant YRB1 ORFs (excised as SalI fragments from the pUC19 derivatives) for the corresponding segment in pMK103 and then introducing the entire yrb1-51 and yrb1-52 genes as EcoRI-XbaI fragments (excised from the pMK103 derivatives) into pRS314, yielding the TRP1-marked plasmids pMK277 and pMK278, respectively. Finally, HMK21 (yrb1 [pMK103]) was transformed with either pMK277, pMK278, or a control plasmid (pMK275) carrying the normal YRB1 gene, plated on 5-FOA plates at 23° to select against the resident URA3-marked YRB1-containing plasmid (pMK103), and the resulting isolates were analyzed for their ability to grow at elevated temperature.
Construction of plasmids:
Standard techniques were used for the manipulation of recombinant DNA (
The YRB1 gene was isolated from a yeast genomic library (
To construct a plasmid (pMK112n) carrying the yrb1::HIS3 deletion construct, an internal BglII fragment was excised from the YRB1-containing insert in pMK101 and replaced by a BamHI fragment containing the HIS3 gene, which was inserted in the same transcriptional orientation as YRB1. Construction of plasmid pNOPPATA-GSP1G21V, which expresses a GTPase-defective mutant form of Gsp1, Gsp1(G21V), fused at its N terminus to a cleavage site (ENLYEQG) for tobacco etch virus (TEV) protease and to two immunoglobulin G (IgG) binding domains of Protein A (ProtA), under control of the NOP1 promoter and the ADH1 terminator, has been described previously (
Fusions of full-length Yrb1 to the Gal4 transcriptional activation domain (TAD) and full-length Gsp1(G21V) to the E. coli LexA DNA-binding domain (DBD) were generated via PCR, using the two-hybrid vectors pGAD424 and pBTM116, respectively. Fragments comprising the entire YRB1 ORF were synthesized using 5'-CCG AAT TCG GTC CAG GTG GTA GCG AAG ATA AGA AAC CTG TCG-3' (OSFO15) and the M13/pUC reverse sequencing primer (New England Biolabs) as the primers and pUC19 carrying the chromosomal YRB1-containing EcoRI-XbaI fragment (pMK102), or pUC19 carrying the corresponding fragments from the yrb1-51 or yrb1-52 ORFs, as templates. The PCR products were digested with EcoRI and PstI and inserted into the corresponding sites in pGAD424, yielding pMK199-wt, pMK199-51, and pMK199-52, respectively. Similarly, a fragment comprising the entire ORF coding for Gsp1(G21V) was produced using 5'-GCG AGG CCT TGC CCC AGC TGC TAA CGG TGA AG-3' (OGSP7) and RSET (5'-AAC TGC AGC CAA CTC AGC TTC C-3') as the primers, and E. coli expression vector pRSETB (Invitrogen, Carlsbad, CA) carrying a PCR-mutated genomic PvuII-HindIII fragment coding for Gsp1(G21V) as the template. The resulting PCR product was cleaved with StuI and PstI and inserted into the SmaI and PstI sites of pBTM116, yielding plasmid pMK195-GV.
Plasmid YEplac195-AU-L25NLS-GFP was derived from YEplac195-ADE2-URA3-L25-GFP (
Preparation of rabbit polyclonal anti-Yrb1 antiserum:
To generate a (His)6-Yrb1 fusion protein containing all but the first 10 residues of Yrb1, the corresponding YRB1 coding sequence was excised as a SalI fragment from pMK102 and ligated into the XhoI site of pRSETA (Invitrogen), yielding pMK104. For expression in E. coli, strain BL21(DE3)/pLysS (
Two-hybrid assay:
To assess interactions between LexA(DBD)-Gsp1(G21V) and Gal4(TAD)-Yrb1 fusion proteins, strain JTY2500 harboring the E. coli lacZ gene under control of eight LexA-binding sites was cotransformed with the appropriate pBTM116- and pGAD424-based plasmids. Transformants were grown in SCGlc medium lacking leucine and tryptophan to midexponential phase (A546 nm = 1) and assayed for ß-galactosidase acitivity as described previously (
Preparation of yeast cell extracts:
Yeast cells were washed once with one culture volume of cold phosphate-buffered saline (PBS), aliquoted into 1.5-ml microcentrifuge tubes (20 A546 nm units per tube), and stored as pellets at -70°. Frozen cell pellets were thawed by adding 0.2 ml cold lysis buffer (50 mM Tris-HCl pH 7.5, 150 mM NaCl, 20 mM MgCl2, 10% glycerol, 2 mM DTT, and 1 mM PMSF) and lysed by vigorous vortexing with 0.2 g of acid-washed glass beads (0.45–0.6 mm diameter) for six 30-sec periods (separated by 1-min periods of cooling on ice). The lysate was clarified by centrifugation for 5 min at 13,000 x g at 4° and the protein concentration was determined by a dye-binding method (
Purification of ProtA-TEV-Gsp1(G21V) from yeast:
Transformants of wild-type strain CRY1, coexpressing ProtA-TEV-Gsp1(G21V) from pNOPPATA-GSP1G21V and either Yrb1-GFP, Yrb1(A91D)-GFP, or Yrb1(R127K)-GFP from plasmids pMK284n, pMK294-51, or pMK294-52, respectively, were grown in selective medium at 26° to a A546 nm = 1.5. Purification of Gsp1(G21V) from these cells was performed essentially as described (
Nuclear protein import and RNA export assays:
Temperature-sensitive mutants, and their otherwise isogenic wild-type strains, containing plasmids that express constitutively nuclear transport substrates fused to GFP(S65T), namely SV40NLS-Gal4(TAD)-GFP (pGADGFP), GFP-Npl3 (pNOPGFPAU-NPL3), and L25NLS-GFP (YEp195-AU-L25NLS-GFP), were cultivated to early exponential phase (A546 nm = 0.5) in selective SCGlc medium at 23°, split into two equal portions, and incubated at either 23° or 37° for various periods of time. Strains carrying plasmids expressing SV40NLS-GFP-ß-galactosidase (pPS817) under control of the GAL1 promoter were pregrown to early exponential phase (A546 nm = 0.5) in selective SCRaf medium at 23° before Gal (2%) was added to the cultures and the cells were incubated at 23° for another hour (to allow mRNA synthesis and export). The induced cultures were split into two equal portions, and one portion was shifted to 37° for 3 hr, while the other portion was maintained at 23° for the same period. Fluorescence microscopy of living yeast cells expressing GFP fusion proteins was done according to
Miscellaneous:
SDS-PAGE and immunoblotting were conducted as described previously (
| RESULTS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Isolation of yrb1ts mutations as suppressors of mating defects:
The mating deficiency of a fus1 mutant is much more pronounced at 14° than at 30°. At 14°, diploid formation in a MATa fus1 x MAT fus1 cross is <0.5% that of a MATa FUS1 x MAT fus1 cross (Table 3). A screen for extragenic suppressors of this mating defect (see MATERIALS AND METHODS) yielded a single mutation, sfo1-1. This suppressor mutation reproducibly enhanced mating competence of a fus1 mutant 30–50-fold (Table 3), but did not fully restore mating proficiency to the level of a FUS1 cell. The suppressor segregated 2:2 through two backcrosses against a fus1 strain and cosegregated with a recessive ts growth defect (in >15 tetrads analyzed per cross). Genetic mapping of the mutation to the right arm of chromosome IV between CEN4 and the TRP1 gene (data not shown), complementation of the ts growth defect by the wild-type YRB1 gene on a plasmid (data not shown), elimination of the suppression phenotype by plasmid-borne YRB1 (Table 3), and nucleotide sequencing of the mutant DNA (see below) all established that sfo1-1 was a recessive allele of YRB1, which encodes the homolog of mammalian RanBP1 (
A recessive ts mutation, stp52 (sterile pseudoreversion), closely linked to TRP1, was isolated as an extragenic suppressor of the mating defect of a MATaste5-3 x MAT ste5-3 cross at restrictive temperature (
Phenotypic characterization of the yrb1-51 and yrb1-52 mutations:
To understand how alterations in YRB1 can suppress mating-defective mutants, we examined, first, the physiology of the yrb1 mutants. At 23°, yrb1-51 mutant cells grew nearly as well as wild-type cells, whereas the yrb1-52 mutant cells displayed impaired growth already under these conditions; both yrb1-51 and yrb1-52 cells ceased growth and lost viability within 3–6 hr after shift to 37° (data not shown). Similar results were observed for the corresponding homozygous diploids (data not shown). As judged by immunoblotting of cell lysates (Fig 1A), after shift to 37° for 3 hr, the product of the yrb1-51 allele was hardly detectable, whereas the yrb1-52 product remained relatively stable even 6 hr after temperature shift. Thus, the yrb1-51 mutation appears to destabilize the gene product at higher temperature, whereas the yrb1-52 product is stable under the same conditions. Upon prolonged incubation at 37°, an apparent degradation product of Yrb1 accumulated in yrb1-52 cells, but was also observed in the wild-type control cells. Yrb1 was expressed at similar levels in MATa, MAT, and MATa/MAT cells (data not shown) and its level in MATa cells was not elevated in response to treatment with -factor mating pheromone (data not shown).
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Examination of the cell morphology revealed that haploid yrb1-51 cells arrested mostly as enlarged cells with a large bud or as large unbudded cells upon shift to 37° (data not shown; -importin is the adaptor necessary for recognition and nuclear import of proteins that contain a classical nuclear localization signal (NLS) by the Kap95/ß-importin receptor (
Yrb1-51 and Yrb1-52 are altered in conserved residues of the Ran-binding domain and defective for Ran-binding in vivo:
To determine the nature of the alterations in the mutant proteins, PCR was used to recover the YRB1 coding sequences from the mutant strains (see MATERIALS AND METHODS). The DNA sequence of each mutant ORF contained a single point mutation, both of which alter a highly conserved residue in the RBD (Fig 2A). The yrb1-51 mutation is a C-to-A transversion on the coding strand at position 272 (where +1 is the first base of the initiator ATG), which substitutes Asp for Ala at codon 91 (A91D). The yrb1-52 allele is a G-to-A transition on the coding strand at position 380, which substitutes Lys for Arg at codon 127 (R127K). On the basis of homology modeling of Yrb1 on the crystal structure of the first RBD (RanBD1) in mammalian Nup358 (RanBP2) complexed with Ran bound to a nonhydrolyzable GTP analog ( background (see MATERIALS AND METHODS).
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Two independent approaches demonstrated that the yrb1-51 and yrb1-52 mutations interfere with Yrb1-Ran (Gsp1) interaction in vivo. The GTPase-deficient form of Gsp1, Gsp1(G21V), binds more strongly to Yrb1 than normal Gsp1 (
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These results were confirmed by a biochemical procedure (Fig 3B). Yrb1-GFP, Yrb1(A91D)-GFP, or Yrb1(R127K)-GFP, produced from the authentic YRB1 promoter on CEN plasmids, were expressed in wild-type cells (strain CRY1) also producing a ProtA-(TEV site)-Gsp1(G21V) from the constitutive NOP1 promoter on a CEN plasmid. After growth at 26°, protein complexes bound to bead-immobilized ProtA-(TEV site)-Gsp1(G21V)were recovered from cell extracts as described in
yrb1-51 and yrb1-52 mutants are defective in nuclear protein and RNA transport:
To determine if yrb1-51 and yrb1-52 cause defects in nuclear protein import and RNA export, as observed before for the yrb1-1 and yrb1-2 alleles (50% of the cells even 1 hr after the shift (data not shown). Poly(A)+ RNA accumulated in the nucleus in a distinctly punctate pattern, a feature seen in mutants that have a strong RNA export defect, such as mex67-5 (
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To monitor the effect of the yrb1-51 and yrb1-52 mutations on nuclear protein import, four different GFP fusions of nuclear proteins were examined. To assess the -importin/Srp1 and ß-importin/Kap95/Rsl1-dependent pathway, two chimeras containing the SV40 NLS were used: a galactose-inducible SV40NLS-GFP-ß-galactosidase, which is so large it cannot diffuse out of the nucleus after it has been delivered there (
Control strains or yrb1-51 and yrb1-52 mutants carrying the reporter plasmids described above were cultivated in selective medium, shifted to restrictive temperature, and examined by fluorescence microscopy. For the inducible reporter, transformants were grown to midexponential phase in Raf-containing medium at permissive temperature and induced for 1 hr by addition of 2% Gal (to allow for mRNA synthesis and export) before shift to 37°. For all four reporter proteins, there was a significant cytoplasmic accumulation in yrb1-51 and yrb1-52 mutants after shift to 37°, compared to wild-type cells, indicating a general defect in nuclear protein import. Results for SV40NLS-Gal4TAD-GFP (Fig 4B) and L25NLS-GFP (Fig 4C) reporters in homozygous diploid strains are shown; but, similar results were obtained in haploids and for the other two reporters (data not shown). In yrb1-52 cells, the defect was noticeable even at permissive temperature. Our results showing a defect in nuclear protein import in yrb1-52 cells are at odds with a previously published report on the same mutant (
To exclude the possibility that cytoplasmic localization of the reporter proteins in yrb-51 and yrb1-52 cells was due to "leakiness" of the mutant nuclei, accumulation of constitutively expressed SV40NLS-GFP-ß-galactosidase (encoded by pPS815;
Genetic interactions of yrb1 mutations with nucleocytoplasmic transport factors:
As an independent means to confirm that yrb1-51 and yrb1-52 compromise nucleocytoplasmic trafficking even at permissive temperature, genetic interactions of these alleles with mutations in genes encoding a variety of other factors involved in nucleocytoplasmic transport were examined. Strains carrying mutations of interest were crossed with strains carrying the yrb1-51 or yrb1-52 mutation, and the resulting diploids were sporulated. Double mutant segregants from tetratype asci were compared to each single mutant segregant and to the wild-type segregant for their ability to grow at various temperatures (see Fig 5). Mutations tested included alterations in genes encoding components of the Ran GTPase cycle, nuclear import and export receptors, and nucleoporins (see Table 4). The plc1::HIS3 mutation (::HIS3 yrb1-52, the growth defect was even more severe than for the corresponding double mutant with yrb1-51 (Table 4). Equally pronounced growth defects were observed when yrb1-51 was combined with mutations in genes encoding certain nuclear transport receptors (Table 4). In all these cases, the double mutant was not viable at any temperature (synthetic lethality); for the other genetic interactions observed, double mutants were viable at the permissive temperature (23°) but revealed a restrictive temperature that was considerably (>3°; ++) or slightly (3°; +) lower than the one of any of the two single mutants (synthetic growth defect). Thus, the functions of Yrb1(A91D) and Yrb1(R127K) are at least partially defective even under permissive conditions.
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Nucleocytoplasmic trafficking of Ste5 is altered in yrb1-51 and yrb1-52 cells:
Our results indicate that impaired nucleocytoplasmic transport is the primary cause of the phenotypes of yrb1-51 and yrb1-52 mutants, including, presumably, the ability of these mutations to suppress mating defects. Far1 and Ste5 are currently the only components of the mating pheromone response pathway known to shuttle between nucleus and cytoplasm (
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To obtain further evidence that suppression of mating defects by yrb1-51 and yrb1-52 arises from impairment of nuclear import of Ste5, we tested whether these yrb1ts mutations could suppress the mating defect of a msn5 mutant. Msn5 is thought to be the nuclear receptor required for pheromone-stimulated export of Ste5 from the nucleus ( strain and the wild-type single mutant, and double mutant spores from the resulting tetratype asci were tested for their relative mating proficiency using a quantitative mating assay performed at semipermissive temperature (30°) for the yrb1ts alleles. Both the yrb1-51 and yrb1-52 mutations restored the mating efficiency of the msn5 mutant to essentially the wild-type level (Table 5). This suppression is consistent with the idea that a higher cytoplasmic pool of Ste5 (due to its inefficient nuclear import in the yrb1ts mutants) compensates for its inefficient pheromone-stimulated export from the nucleus (due to the msn5 mutation).
| DISCUSSION |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Ran GTPase is one of the most highly conserved proteins in nucleated cells (
A decade ago, before the function of the essential Ran regulator, RanGEF1, was fully appreciated, a ts mutation (srm1-1) in its yeast homolog (SRM1/PRP20/MTR1) was isolated as a suppressor of the mating defect of haploid cells lacking pheromone receptors (
In retrospect, it may seem obvious that perturbation of nucleocytoplasmic transport could affect yeast mating since response to pheromone requires: (a) that some signal carrier enter the nucleus to induce the transcription of genes, (b) that RNPs containing newly synthesized mRNAs for mating-specific components exit the nucleus, and (c) that the translation products of some of those transcripts be recruited back into the nucleus in support of late mating events, like karyogamy (
Because both yrb1ts alleles described here are defective in nuclear protein import, but only one seems impaired in poly(A)+ RNA export, yet both act as suppressors of mating defects, it is presumably the import defect that leads to suppression. Also, it should be recalled that yrb1-51 was isolated on the basis of rescue of the mating debility of a fus1 mutant, which has an intact pheromone response pathway and is only partially mating defective. Likewise, yrb1-52 was isolated on the basis of its ability to rescue ste5 missense mutations (and can do so for ste4 and ste7 missense mutations), but is unable to rescue null alleles in these same genes (
In agreement with the above model, both the yrb1-51 and the yrb1-52 mutations increased the cytoplasmic concentration of Ste5 and were able to suppress the mating defect of a msn5 null mutation. The MSN5 gene encodes a nuclear export receptor of the ß-importin family (-factor under conditions (by inducing the pheromone-responsive reporter FUS1-lacZ) and by undergoing G1 arrest (as judged by the standard halo bioassay; data not shown); hence, these mutants are not defective in early signaling events. If, however, proteins required for late events in mating are maintained longer in the cytosol of yrb1 mutants due to defective nuclear protein import, the efficiency of mating would be enhanced, as observed. Finally, such a model would also explain the spectrum of mating defects that are suppressed by yrb1-51, yrb1-52, and srm1-1. All of the mutations suppressed are in gene products that are targeted, directly or indirectly, to the shmoo tip after pheromone treatment and most are involved in the pheromone-induced remodeling of the cortical cytoskeleton (
complex in response to pheromone binding, is responsible for direct recruitment of major regulators of cytoskeletal structure and cell polarity, including Ste20 (. Finally, Fus1 is an integral membrane protein localized to the tip of the mating projection and is involved in the cell fusion step of mating (
A primary defect of the analyzed yrb1ts mutants in nucleocytoplasmic transport would also explain the observed mitotic phenotypes, since similar mitotic disturbances have been reported for mutants deficient in other factors involved in nucleocytoplasmic transport, for example, Srp1 (-importin;
Although our study cannot rigorously rule out the possibility that Ran or RanBP1 may play some role in the mating pathway independent of their functions in nucleocytoplasmic transport, based on the findings presented here, the observed suppression of mating defects and the defects in mitosis caused by the yrb1-51 and yrb1-52 mutations are most likely direct consequences of impaired import of nuclear proteins. Because of its relatively slow onset, the apparent mRNA export defect manifested by the yrb1-51 allele may reflect an indirect consequence of a primary defect in import.
| FOOTNOTES |
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1 Present address: Microbia, Inc., Cambridge, MA 02139. 
| ACKNOWLEDGMENTS |
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We thank Markus Aebi (Federal Institute of Technology, Zürich, Switzerland), Pierre Belhumeur (McGill University, Montreal), Laura Davis (Brandeis University, Waltham, MA), Gerald Fink (Massachussetts Insitute of Technology, Boston), Molly Fitzgerald-Hayes (University of Massachussetts, Amherst, MA), Anita Hopper (Pennsylvania State University, Hershey, PA), Masayasu Nomura (University of California, Irvine, CA), Pamela Silver (Dana Farber Cancer Center, Boston), Françoise Stutz (Centre Hospitalier Universitaire Vaudois, Lausanne, Switzerland), Alan Tartakoff (Case Western Reserve University, Cleveland), Linda S. Huang (University of California, San Francisco), and Karsten Weis (University of California, Berkeley, CA) for the generous gifts of reagents; Stefan Irniger (Georg-August-Universität, Göttingen, Germany) and Jeff Flick (Vanderbilt University, Nashville, TN) for sharing unpublished results; and Stephanie Richards and Ian Macara (University of Virginia, Charlottesville, VA) for advice and material assistance at the early stages of this work. We are grateful to members of our laboratory, especially Jeanette Gowen Cook, Elana Swartzman, Namrita Dhillon, Lee Bardwell, and Carla Inouye, for technical assistance and valuable discussions. This work was supported by a European Molecular Biology Organization Long-Term Fellowship and funds provided by the Swiss National Science Foundation (to M. Künzler), by National Science Foundation Postdoctoral Fellowship DMB-8807575 and National Cancer Institute Postdoctoral Traineeship CA09041 (to J. Trueheart), by a Postdoctoral Fellowship from the Italian-American Cancer Foundation (to C. Sette), by National Institutes of Health Research Grant GM21841 (to J. Thorner), and by facilities provided by the Berkeley campus Cancer Research Laboratory.
Manuscript received July 13, 2000; Accepted for publication November 21, 2000.
| LITERATURE CITED |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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