RRS1, a Conserved Essential Gene, Encodes a Novel Regulatory Protein Required for Ribosome Biogenesis in Saccharomyces cerevisiae

doi:10.1128/MCB.20.6.2066-2074.2000

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Tsuno, A.
	Articles by Mizuta, K.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Tsuno, A.
	Articles by Mizuta, K.

Previous Article | Next Article

Molecular and Cellular Biology, March 2000, p. 2066-2074, Vol. 20, No. 6
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

RRS1, a Conserved Essential Gene, Encodes a Novel Regulatory Protein Required for Ribosome Biogenesis in Saccharomyces cerevisiae

Akiko Tsuno, Keita Miyoshi, Rota Tsujii, Tokichi Miyakawa, and Keiko Mizuta^*

Department of Molecular Biotechnology, Graduate School of Advanced Sciences of Matter, Hiroshima University, Higashi-Hiroshima 739-8527, Japan

Received 18 October 1999/Returned for modification 30 November 1999/Accepted 28 December 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

A secretory defect causes specific and significant transcriptional repression of both ribosomal protein and rRNA genes (K.Mizuta and J. R. Warner, Mol. Cell. Biol. 14:2493-2502, 1994),suggesting the coupling of plasma membrane and ribosome syntheses.In order to elucidate the molecular mechanism of the signalingpathway, we isolated a cold-sensitive mutant with a mutation ina gene termed RRS1 (regulator of ribosome synthesis), which appearedto be defective in the signaling pathway. The rrs1-1 mutationgreatly reduced transcriptional repression of both rRNA and ribosomalprotein genes that is caused by a secretory defect. RRS1 is anovel, essential gene encoding a nuclear protein of 203 aminoacid residues that is conserved in eukaryotes. A conditional rrs1-nullmutant was constructed by placing RRS1 under the control of theGAL1 promoter. Rrs1p depletion caused defects in processing ofpre-rRNA and assembly of ribosomalsubunits.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Balanced synthesis of cellular components is required for normal cell growth. A temperature-sensitive mutation in SLY1, whosegene product is involved in endoplasmic reticulum-to-Golgi trafficking(26), causes the transcriptional repression of both ribosomalprotein and rRNA genes in Saccharomyces cerevisiae (20). Furtherexamination using various sec mutants showed that a defect anywherein the secretory pathway, from a step prior to insertion of thenascent peptide into the endoplasmic reticulum to a step involvedin the formation of the plasma membrane, prevents the continuedsynthesis of the components of the ribosome. Similar results wereobtained following treatment of wild-type cells with the secretoryinhibitors tunicamycin and brefeldin A (20). Furthermore, manytemperature-sensitive mutants in which transcription of ribosomalprotein genes is temperature sensitive appear to be defectivein the secretory pathway (17). As the membrane is the end productof much of the secretory pathway, these results suggest an importantcoupling of plasma membrane and ribosome biosynthesis. We proposedthe existence of a signal transduction pathway from the plasmamembrane to the nucleus. According to this model, a signal generatedby the defect in de novo synthesis of membrane should be transmittedto the nucleus and cause specific and significant transcriptionalrepression of ribosomal genes. It was recently suggested thatstress in the plasma membrane is monitored by Pkc1, which initiatesa signal transduction pathway that leads to the repression (24).In order to elucidate the molecular mechanism of the signal transductionpathway, we have screened for mutants defective in the responseto a secretorydefect.

Here we describe the isolation and molecular characterization of RRS1, encoding an essential nuclear protein of 203 aminoacids. In the rrs1-1 mutant, a secretory defect fails to causetranscriptional repression of either rRNA or ribosomal proteingenes. The mutant gene, rrs1-1, had a single nucleotide differencewithin codon 114, resulting in a stop codon. The amino acid sequenceof Rrs1p is significantly similar to that of a putative proteinencoded by human cDNA. In order to analyze functions of Rrs1p,we constructed a conditional rrs1-null mutant. Depletion of Rrs1paffects pre-rRNA processing and assembly of ribosomal subunits,indicating that Rrs1p is required for proper ribosomebiogenesis.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Yeast strains, plasmids, and media. The yeast strains used in this study are listed in Table 1. Yeast cells were grown in YPD rich medium, YPG, synthetic completemedium containing 2% glucose (SC) or 2% galactose (SCGal), orSC dropout medium, depending on the plasmid markers (10). Yeasttransformation was performed by a lithium acetate procedure (9).

View this table:
[in this window]
[in a new window]

TABLE 1. Yeast strains used in this study

A library consisting of partial Sau3A fragments of S. cerevisiae genomic DNA inserted into a single-copy yeast vector, YCp50,was generously provided by M. D. Rose (29).

For epitope tagging, an NheI site was introduced by PCR into pRRS1 just after the initiation codon. The DNA cassette encodingthree copies of the nine-amino-acid influenza virus hemagglutinin(HA) epitope was obtained by the digestion of pYT11 (33) withNheI and was inserted in frame into the NheI site of pRRS1. Thedigested DNA fragment including epitope-tagged RRS1 was subclonedinto pRS316 (32).

A plasmid containing GAL1 promoter-controlled RRS1 was constructed as follows. pAT-35 (see below) was digested with XbaI andScaI and the 0.8-kb fragment containing the open reading frame(ORF) of RRS1 was placed under the GAL1-promoter in a multi-copyvector pNV7 (25). The DNA fragment containing the GAL1 promoter,RRS1, and the terminator was cloned into a single-copy vector,pRS313 (32).

Cloning of a mutant allele. A mutant allele of the chromosomal RRS1 gene was isolated by PCR. Total chromosomal DNAs were isolated from wild-type andrrs1-1 mutant cells. DNA fragments including RRS1 or rrs1-1 wereamplified by PCR and cloned into pUC19. PCR was carried out twice,and the DNA sequence was determined by using four independentclones.

Indirect immunofluorescence. Indirect immunofluorescence microscopy was done by modification of the procedure described by Pringle et al. (27). Culturesof early-log-phase cells growing in SC medium were fixed by additionof formaldehyde to the medium to a final concentration of 3.2%,followed by agitation for 30 min at room temperature. Fixed cellswere harvested by centrifugation, washed with KPS buffer (100mM potassium phosphate buffer, pH 7.5, with 1.2 M sorbitol) andresuspended in KPS. To remove the cell wall, the cell suspensionwas incubated with 20 µg of Zymolyase 100T per ml and 0.2% $beta$ -mercaptoethanolat 37°C for about 10 min. Spheroplasts were washed with KPS andharvested by gentle centrifugation. Resuspended spheroplasts inKPS were spotted onto polylysine-coated multiwell slides and blockedfor 5 min with PBS-BSA (0.285% Na₂HPO₄, 0.02% KH₂PO₄, 0.8% NaCl,0.02% KCl [pH 7.5], 1 mg of bovine serum albumin per ml). Thecells were incubated with 10 µl of primary antibody (anti-HA.11;Babco) diluted 1:1,000 with PBS-BSA for 1 h at room temperature.After 10 washes with PBS-BSA, the cells were incubated for 1 hwith secondary antibody (rhodamine-conjugated goat-anti-mouseimmunoglobulin G; Jackson ImmunoResearch Laboratory, Inc.) diluted1:300. After 10 washes with PBS-BSA and one with PBS, the cellswere stained with 1 µg of DAPI (4',6'-diamidino-2-phenylindole)per ml in mountingmedium.

Western blot analysis. Western blotting followed standard techniques, and signals were visualized by enhanced chemiluminescence(Amersham).

Northern blot and [methyl-³H]methionine pulse-chase analysis. Northern blot analysis was carried out using 1.5% agarose gels for mRNAs and 1.2% agarose gels for steady-state level of rRNAsin formaldehyde as described previously (4, 20). The oligonucleotidesused for analyzing mature rRNAs and pre-rRNAs were as follows;probes a, b, and c correspond to oligonucleotides B, C and D,respectively, as described by Zanchin and Goldfarb (41), probesd and e correspond to oligonucleotides a and g, respectively,as described by Bergès et al. (1).

[methyl-³H]methionine pulse-chase analysis was carried out using strains grown in SC lacking methionine (SC $-$ Met). Each culturewas pulsed with [methyl-³H]methionine and was chased with nonradioactive methionine (500µg/ml). Samples were taken by pouring cultures onto crushed sterileice. Total RNA was prepared and analyzed on agarosegels.

Polyribosome analysis. Yeast cells were grown in 100 ml of medium to mid-log phase and harvested immediately following the addition of cycloheximide(100 µg/ml). The pellet was washed twice with CH buffer (10 mMTris-HCl [pH 7.4], 100 mM NaCl, 30 mM MgCl₂, 50 µg of cycloheximideper ml, 200 µg of heparin per ml) and suspended in 0.3 ml of CHbuffer. After glass-bead lysis of yeast cells, aliquots of supernatantcorresponding to 10 A₂₆₀ units were overlaid on top of 12 ml ofa 10 to 40% (wt/wt) sucrose gradient made in 50 mM Tris-HCl (pH7.6)-12 mM magnesium acetate-50 mM ammonium acetate-1 mM dithiothreitoland centrifuged for 2 h at 40,000 rpm at 4°C in a Beckman SW40Tirotor.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation of yeast mutants unable to respond to the secretory defect. In order to obtain genes which are involved in the signaling pathway, we screened for mutants in which a secretory defectdid not cause the transcriptional repression of ribosomal proteingenes. The strategy is shown in Fig. 1A. A plasmid was generatedin which the HIS3 gene was driven by the promoter of the ribosomalprotein gene RPL28 (according to new nomenclature in reference18; formerly called CYH2). This plasmid was transformed intoa strain with the genotype his3 sly1^ts. These cells are phenotypically His⁺ at 25°C, but at 31°C, just below the nonpermissive temperaturefor sly1, they grow extremely slowly on SC $-$ His plates containing3-aminotriazole because the HIS3 transcription is repressed. Thecells were treated with ethyl methanesulfonate to a survival frequencyof 25% and grown on SC $-$ His plates containing 3-aminotriazole at31°C. A mutant defective in the signaling pathway was expectedto grow much faster than the parental strain. Of an estimated8 × 10⁴ cells plated, 24 colonies that grew rapidly were picked. Eachmutant was tested for its ability to repress transcription ofribosomal protein genes RPL28 and RPL3 (formerly TCM1) in responseto a secretory defect; five mutant strains were selected. In thisstudy, one of them, termed rrs1-1 (regulator of ribosome synthesis),was chosen for further analysis. In rrs1-1 cells, the transcriptionof ribosomal protein genes is not significantly repressed in responseto a secretory defect which is caused by transfer of cells tothe restrictive temperature in the background of sly1 (Fig. 1B)or by addition of a secretory inhibitor, tunicamycin (Fig. 1C).The rrs1-1 mutation does not suppress the temperature sensitivityof sly1 (data not shown), indicating that rrs1-1 is not a suppressorof the secretory defect of the sly1 mutation. Genetic analysisshowed that the mutation is recessive; when the mutant cells werecrossed to parental sly1 cells of the opposite mating type, RPL28was significantly repressed at the restrictive temperature (datanot shown). On sporulation and dissection of asci, the phenotypefor the defect in the response segregated 2:2, indicating thatthis phenotype is due to a single mutation in a nuclear gene.

View larger version (49K):
[in this window]
[in a new window]

FIG. 1. Isolation of rrs1-1 mutant. (A) The strategy used to isolate yeast mutants defective in the signaling in response to a secretory defect. The reporter gene shown in the diagram consists of the coding sequence of the yeast HIS3 gene fused to the promoter of RPL28. Haploid KM003 (sly1 his3) cells carrying this reporter construct cannot grow at 31°C on SC $-$ His plates containing 5 mM 3-aminotriazole. Mutant cells that do not respond to a secretory defect are expected to grow. (B and C) Northern analysis of the rrs1-1 mutant with the secretory defect. (B) Yeast KM003 (sly1 RRS1) and KM101 (sly1 rrs1-1) cells were grown in YPD medium to log phase (optical density at 600 nm = 0.4 to 0.6) at 25°C. Half of the culture was shifted to 36°C, and after 90 min, the cells were harvested. (C) Yeast strains W303a (SEC⁺ RRS1) and KM123 (SEC⁺ rrs1-1) were grown to log phase (optical density at 600 nm = 0.4) at 25°C. Half of the culture was treated with tunicamycin at a final concentration of 1 µg/ml for 4 h at 25°C, and the cells were harvested. Total RNA was prepared and separated by gel electrophoresis. Northern blot analysis was carried out using ³²P-labeled DNA probes specific for RPL28 and RPL3. SnoRNA U3 was used as a marker to check equal loading. Ten micrograms of total RNA was loaded in each lane.

The rrs1-1 mutation also affects the repression of rDNA transcription in response to a secretory defect. As a secretory defect causes transcriptional repression of DNA encoding rRNA (rDNA) as well as ribosomal protein genes (20),we examined whether the rrs1-1 mutation had any effect on therepression of rDNA. We can monitor the synthesis and processingof rRNA by [methyl-³H]methionine pulse-chase analysis, since newly synthesized precursorrRNA is methylated immediately (30, 37). As shown in Fig.2, a secretory defect by shifting sly1 cells to the restrictivetemperature leads to strong repression of rDNA transcription (lane3), and newly synthesized precursor rRNA is processed very slowly(lane 4), consistent with previous data (20). On the other hand,in rrs1-1 mutant cells, a secretory defect does not cause repressionof rDNA transcription (Fig. 2, lanes 7 and 8), indicating thatthe rrs1-1 mutation also affects the signaling pathway from asecretory defect to the repression of rDNA transcription. Whenthe cells were pulse-labeled with [³H]uracil, its incorporation into the trichloroacetic acid-insolublefraction was also strongly reduced under the conditions in whichthe secretory pathway was blocked, indicating that a secretorydefect causes repression of rDNA transcription rather than inhibitionof pre-rRNA methylation (data not shown).

View larger version (64K):
[in this window]
[in a new window]

FIG. 2. The rrs1-1 mutation also affects the transcriptional repression of rDNA in response to a secretory defect. Strains KM003 (sly1 RRS1) and KM101 (sly1 rrs1-1) were grown to log phase (optical density at 600 nm = 1.0) in SC $-$ Met medium at 25°C. Aliquots from each culture were shifted to 37°C for 90 min. Each culture was pulsed with [methyl-³H]methionine (60 µCi/ml) for 5 min and chased with nonradioactive methionine (500 µg/ml). Samples were taken and chilled by pouring onto crushed sterile ice at the time of addition of cold methionine (t = 0) and after a chase time of 10 min. Total RNA was prepared, and 20 µg of each sample was analyzed by electrophoresis. The gel was divided into two pieces. The upper gel was soaked in En³Hance (NEN), dried, and exposed to a film for 3 days (top panel) or for 10 days (middle panel). The lower gel was blotted and probed for U3 (bottom panel).

RRS1 is required for the repression of ribosomal protein genes in response to a secretory defect but not for the heat shock response. Mild heat shock causes the temporary repression of transcription of ribosomal protein genes (7, 11). To determine whetherthis repression acts in the same way as that due to a failurein the secretory pathway, we examined the effect of the rrs1-1mutation on the repression through heat shock at 36°C. As shownin Fig. 3, a ribosomal protein gene, RPL28, was significantlyrepressed 15 min after the temperature shift-up in both the RRS1and the rrs1-1 strains, indicating that the rrs1-1 mutation hadno effect on the heat shock response. In the background of sly1,the RRS1 strain did not recover its RPL28 mRNA level in responseto a secretory defect, whereas rrs1-1 recovered due to a defectin the secretory response, consistent with the data in Fig. 1B.

View larger version (37K):
[in this window]
[in a new window]

FIG. 3. The rrs1-1 mutation affects the secretory defect response but not the heat shock response. Yeast KM003 (sly1 RRS1) and KM101 (sly1 rrs1-1) cells were grown to log phase (optical density at 600 nm = 0.5 to 0.8) in YPD medium at 25°C, and then the culture was shifted to 36°C. Aliquots were taken at the times indicated, and total RNA was prepared. Northern blot analysis was carried out using ³²P-labeled DNA probe specific for RPL28. U3 was used as a marker to check equal loading. Five micrograms of total RNA was loaded in each lane.

Cloning of the RRS1 gene. rrs1-1 mutant cells exhibited a prolonged generation time (about 7 h) at 18°C when cultured in YPD liquid medium. At highertemperatures, the growth rate was not so severely reduced; thegeneration time of rrs1-1 cells was 40% longer than that of wild-typecells at 30°C and 20% longer at 37°C. On a YPD plate, the rrs1-1cells ceased to proliferate at 18°C. The cold sensitivity forgrowth segregated 2:2 in three sets of tetrads from RRS1/rrs1-1diploid cells, and the cold sensitivity was linked to the phenotypefor the defect in the signaling detected in Northern blot analysis(data not shown). Therefore, the wild-type RRS1 gene was clonedby complementation of the cold sensitivity of rrs1-1 cells. rrs1-1cells were transformed with a library of yeast genomic DNA constructedin a URA3⁺ centromere-based vector, YCp50 (29). Of 2 × 10⁴ Ura⁺ transformants, five could grow at 18°C on a YPD plate. Restrictionmaps of the plasmid DNAs recovered from these transformants revealedthat each plasmid has an identical 18-kb insert. We determineda partial DNA sequence of the plasmid. A database search revealedthat the insert carries six complete ORFs and two partial ORFs.To identify the region of the 18-kb DNA insert required for complementation,six subclones were constructed and their complementing activitiesfor the cold-sensitivity of rrs1-1 were checked. The complementingactivity was fully recovered in the plasmid, termed pAT-35, containingthe 1.6-kb EcoRI-SacI fragment. Northern analysis revealed thatthe plasmid complements the defect in the signaling of rrs1-1(data not shown). To confirm that pAT-35 contains the wild-typeversion of the rrs1-1 mutant gene, pAT-35 was subcloned into YIp5and a fragment from the resultant plasmid was integrated intothe rrs1-1 strain. After the transformant was crossed with a wild-typehaploid, dissection of 17 tetrads yielded 17 sets of four spores,all of which could grow at 18°C (data not shown). These resultsindicate that pAT-35 contains RRS1.

Sequences of RRS1. We determined the entire nucleotide sequence of the insert in pAT-35. RRS1 corresponds to ORF YOR294w, identified in the yeastgenome project. RRS1 encodes a novel protein consisting of 203amino acids with a predicted molecular mass of 23 kDa and an isoelectricpoint of 9.9. Although no conserved motifs were detected by usingProsite, a coiled-coil structure was predicted from amino acid34 to 63 by using CoilScan (GCG). A database search revealed thatDNA sequences from Homo sapiens, Caenorhabditis elegans, and Schizosaccharomycespombe can encode proteins with significant similarity to Rrs1p(Fig. 4) with 36.8, 30.9, and 43.6% identities, respectively.The amino acid sequences of the putative human and C. eleganshomologs are longer than that of Rrs1p at C-terminal domain, wheretheir sequence similarity (identity, 26.7%) is lower.

View larger version (63K):
[in this window]
[in a new window]

FIG. 4. Alignment of Rrs1p and related sequences from other species. The amino acid sequence of Rrs1p was predicted by nucleotide sequence that was determined using plasmid pAT-35 by dideoxy chain termination method with a Pharmacia DNA sequencer. The sequence was aligned with the predicted sequences from a database; Schizosaccharomyces pombe SPBC29A3.16 (S.p.) (DDBJ/EMBL/GenBank accession number AL022299), C. elegans cosmid C15H11 (C.e.) (39), and H. sapiens KIAA0112 (H.s.) (23). (A) Schematic alignment of the open reading frames. Amino acid residue numbers are marked. The initial codon of the H. sapiens sequence has not been determined yet and amino acids are numbered from the first methionine of the ORF. Identities to Rrs1p across the highlighted regions are listed on the right. (B) Alignment in single-letter code. Deletions needed for the alignment are indicated by dashes. Identical amino acids are boxed in black. When there are two sets of identical amino acids, one set is boxed in black and the other is shaded in gray.

rrs1-1 produces a truncated protein. In order to determine the mutation point(s), the rrs1-1 gene was amplified by PCR using chromosomal DNA prepared from themutant cells. Sequence analysis showed that rrs1-1 had only onenucleotide difference (a G-to-A transition), within codon 114,resulting in a stop codon. In order to compare the expressionand molecular size between wild-type and mutant Rrs1p, three tandemcopies of a sequence encoding an epitope from the influenza virusHA protein was inserted just after the initial codon of RRS1 orrrs1-1. Each of the fused genes was subcloned into a CEN plasmid.The plasmid containing RRS1-HA could complement both the lethalityof the rrs1-null mutation and the cold sensitivity of the rrs1-1mutation. The plasmid containing rrs1-1-HA could complement thelethality of the rrs1-null mutation and resulted in both coldsensitivity for growth and a defect in the signaling in responseto a secretory defect (data not shown). These results indicatethat the constructions are biologically functional. As shown inFig. 5, the HA-tagged proteins, designated Rrs1-HA and rrs1-1-HA,were detected as 40-kDa and 26-kDa bands on sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) gels, considerably larger thanthe predicted molecular masses of the proteins. The levels ofRrs1-HA and rrs1-1-HA do not change in response to a secretorydefect. It is noteworthy that the truncated protein appears tohave stability similar to that of the wild-type protein.

View larger version (41K):
[in this window]
[in a new window]

FIG. 5. Western blot analysis of Rrs1-HA and rrs1-1-HA. Haploid SEC⁺ cells expressing RRS1-HA (KM111; lanes 1 and 2) and sly1 cells expressing RRS1-HA (KM113; lanes 3 and 4) or rrs1-1-HA (KM114; lanes 5 and 6) were grown in SC medium to log phase at 25°C (lanes 1, 3, and 5). Half of the culture was shifted to 36°C for 90 min (lanes 2, 4, and 6). Crude extracts were denatured in SDS sample buffer and heated at 95°C for 5 min. Equal amounts of protein (44 µg) were subjected to SDS-PAGE and Western blotting using anti-HA. An arrow indicates nonspecific bands. The positions of size markers are shown on the left.

The RRS1 gene product is an essential nuclear protein. An rrs1-null allele was created by replacing the XbaI-BstEII fragment with the LEU2 gene. The DNA fragment containing therrs1::LEU2 disruption was used to transform diploid W303 and KM007(sly1/sly1). Southern blot analysis of genomic DNA isolated fromthe transformants both of W303 and KM007 demonstrated that theresultant diploid cells carried one intact RRS1 gene and one disruptedby insertion of LEU2 (data not shown). Thirteen tetrads from thetransformant of W303 and nine tetrads from the transformant ofKM007 were dissected. All tetrads yielded only two viable spores(data not shown), both of which were Leu. Microscopic inspection of the other spores showed that theystopped dividing after several divisions (data not shown), indicatingthat RRS1 is essential for vegetative growth. Indirect immunofluorescentmicroscopy revealed that Rrs1-HA was localized in the nucleusat 25°C (Fig. 6). The staining region of Rrs1-HA was somewhatlarger than that of DAPI, suggesting that Rrs1-HA was localizedin both the nucleoplasm and the nucleolus.

View larger version (39K):
[in this window]
[in a new window]

FIG. 6. Intracellular localization of Rrs1-HA detected by indirect immunofluorescence. Haploid cells expressing RRS1-HA (KM111) were grown in SC medium at 25°C to early log phase (optical density at 600 nm = 0.1 to 0.15) and stained with anti-HA antibodies (A), DAPI (B), and differential-interference-contrast (DIC) (C). Arrowheads are put at the same positions in panels A and B.

rrs1-1 is defective in rRNA processing and ribosome assembly. Because some Rrs1 protein appears to be localized in the nucleolus, Rrs1p is expected to have a role in ribosome biogenesis.Furthermore, as shown in Fig. 2, maturation of 25S rRNA in rrs1-1mutant cells (lanes 5 and 6) appears to be slower than in wild-typecells (lanes 1 and 2) at a permissive temperature. Thus, we performed[methyl-³H]methionine pulse-chase and polyribosome analyses with wild-typeand rrs1-1 cells at 18°C. rrs1-1 cells cannot proliferate at 18°Con a YPD plate, but they continue to grow at 18°C in liquid cultureat an extremely low rate. As shown in Fig. 7A, in rrs1-1 cells,the rate of processing of pre-rRNA was low and less mature rRNAwas produced than in wild-type cells. The polyribosome profileshowed that in rrs1-1 cells, 80S ribosomes and polyribosomes weredecreased, 40S subunits were accumulated, and half-mer polyribosomesappeared (Fig. 7B), suggesting that 60S subunit production iscompromised more than 40S production.

View larger version (22K):
[in this window]
[in a new window]

FIG. 7. rrs1-1 mutation causes defect in rRNA processing and ribosome assembly. (A) Pulse-chase analysis of rRNA synthesis. W303a (RRS1, wild type [WT]) and KM123 (rrs1-1) were cultured in SC $-$ Met medium at 18°C overnight. Each culture was pulsed with [methyl-³H]methionine (10 µCi/ml) for 3 min and chased with nonradioactive methionine (500 µg/ml). Samples were taken and chilled by pouring onto crushed sterile ice at the time of addition of cold methionine (t = 0) and after the indicated chase times. Total RNA was prepared and 20 µg of each sample was analyzed by electrophoresis and blotted to a Nytran membrane. The membrane was sprayed with En³Hance (NEN) and exposed to a film for 2 days. The lower gel was blotted and probed for U3. (B) Polyribosome profiles from W303a (a) and KM123 (b). The cells were cultured in YPD at 18°C overnight. Free ribosomal subunits and polyribosomes in cell extracts were separated by sucrose density gradient centrifugation. Arrows indicate half-mer polyribosomes.

RRS1 is required for ribosome biogenesis. In order to achieve conditional expression of RRS1, we constructed a strain in which the chromosomal RRS1 gene was disruptedand a plasmid containing a GAL1-promoter driven RRS1 was introduced.This strain, KM129, could grow on a YPG (galactose) plate butnot on a YPD (glucose) plate (data not shown). In a liquid galactosemedium, KM129 cells grew as fast as wild-type cells. After theshift to a glucose medium, the growth of KM129 cells slowed gradually(Fig. 8A). We performed [methyl-³H]methionine pulse-chase analysis to investigate pre-rRNA synthesis,its processing, and the stability of the rRNAs. In Rrs1p-depletedcells, the rate of processing of pre-rRNA was low and less 25SrRNA was produced than in wild-type cells (Fig. 8B). After a 30-minchase, amounts of 25S rRNA appeared to be somewhat decreased comparedto the level at 20-min chase, suggesting that newly formed 25SrRNA is unstable in Rrs1p-depleted cells. This experiment wasdone in duplicate, and similar results were obtained. Accumulationof 18S rRNA in Rrs1p-depleted cells was also slower than thatin wild-type cells, but the defect appeared to be less severethan for 25S rRNA. The polyribosome profile in Rrs1p-depletedcells showed a decrease in the levels of 80S ribosomes and polyribosome,accumulation of 40S subunits, and the appearance of half-mer polyribosomes(Fig. 8C). These results suggest that Rrs1p depletion affects25S rRNA and 60S subunit production much more than 18S rRNA and40S subunit production.

View larger version (46K):
[in this window]
[in a new window]

FIG. 8. Depletion of Rrs1p causes growth arrest and defect in ribosome biogenesis and in rRNA processing. (A) Growth curves of W303a (RRS1, wild type [WT]) and KM129 (GAL-RRS1) cultured at 25°C in YPGal and shifted to YPD. The change in optical density at 600 nm was monitored after the shift. The cell cultures were diluted to keep the optical density lower than 1.0, and the values were calculated as changes from initial values. (B) Pulse-chase analysis of rRNA synthesis. W303a and KM129 (GAL-RRS1) were cultured in SCGal $-$ Met and shifted to SC $-$ Met for 12 h. Each culture was pulsed with [methyl-³H]methionine (10 µCi/ml) for 3 min and chased with nonradioactive methionine (500 µg/ml). Samples were taken and chilled by pouring onto crushed sterile ice at the time of addition of cold methionine lite(t = 0) and after the indicated chase times. Total RNA was prepared and 20 µg of each sample was analyzed by electrophoresis and blotted to a Nytran membrane. The membrane was sprayed with En³Hance (NEN) and exposed to a film for 2 days. The lower gel was blotted and probed for U3. (C) Polyribosome profiles from W303a (a) and KM129 (GAL-RRS1) (b). The cells were cultured in YPGal and shifted to YPD for 12 h. Free ribosomal subunits and polyribosomes in cell extracts were separated by sucrose density gradient centrifugation. Arrows indicate half-mer polyribosomes.

Steady-state levels of pre-rRNAs in GAL-RRS1 cells were analyzed after the shift to glucose medium for up to 48 h. Followingtransfer of the GAL-RRS1 strain to glucose medium, the 35S pre-rRNAaccumulated slightly up to 24 h (Fig. 9A to C), consistent withthe results of pulse-chase labeling. The reduced levels of both27SA2 (Fig. 9B) and 20S (Fig. 9A) suggest that cleavage at A2is retarded in accordance with the depletion of Rrs1p. In Rrs1p-depletedcells, 23S RNA appears via an aberrant pathway in which the 35Spre-rRNA is not processed at sites A0, A1, and A2 and is insteadcleaved at site A3 in the internal transcribed spacer 1 (Fig.9A and B). The steady-state level of the 25S rRNA decreased duringthe time course of the experiments and levels of both the 20Spre-rRNA and the mature 18S rRNA were also reduced (Fig. 9A andD). The level of 25S rRNA declined more rapidly than that of 18SrRNA; after 12 h of growth in glucose medium, the amount of 25SrRNA was reduced to 39% and the amount of 18S rRNA was 57% (Fig.9F). On the other hand, the level of ribosomal protein L28 mRNAwas not significantly decreased up to 24 h (Fig. 9E), indicatingthat Rrs1p is not required for transcription of ribosomal proteingenes.

View larger version (66K):
[in this window]
[in a new window]

FIG. 9. Northern analysis for steady-state level of pre-rRNAs. The structure of the pre-rRNA and locations of oligonucleotide hybridization probes are shown on the top. W303a (RRS1, wild type [WT]) and KM129 (GAL-RRS1), cultured at 25°C in YPGal, were shifted to YPD and cultured for up to 48 h. Total RNA equivalent to cells at an optical density at 600 nm of 0.5 was used for each sample. Northern blot analysis was carried out using ³²P-labeled DNA probes: probe a (A), probe b (B), probe c (C), probe d for 18S and probe e for 25S (D), and probe for RPL28 and probe for U3 (E). (F) RNA levels were quantified using BAS-1000 (Fuji Photo Film Co.), and the ratio of the radioactivity value at each time point to that at time zero is shown.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Because of the huge amount of ribosome biosynthesis in growing cells, its regulation is essential for the economy of the cells.A functional secretory pathway is required for the normal synthesisof ribosomes, suggesting a coupling between plasma membrane andribosome syntheses (20). In order to elucidate this regulatorymechanism, we isolated the rrs1-1 mutant in which a secretorydefect (sly1^ts) failed to repress transcription of ribosomal protein genes.RRS1 is an essential gene whose function has not been previouslydescribed. Comparison of the Rrs1p sequence with database sequencesshowed that the protein is conserved throughout eukaryotes, butno information about its function is available. The amino acidsequence of Rrs1p has no readily recognizable proteinmotifs.

It is unlikely that rrs1-1 suppresses the defect in the secretory pathway of sly1, because rrs1-1 does not suppress temperaturesensitivity for growth (data not shown) and the rrs1-1 mutationresults in derepression of ribosomal protein genes when the secretorypathway is blocked by using tunicamycin as well as by shiftingsly1 cells to the restrictive temperature (Fig. 1). Western blottinganalysis of functional epitope-tagged Rrs1-HA and rrs1-1-HA indicatesthat rrs1-1-HA has stability similar to that of the wild-typeversion and that a secretory defect does not cause a significantchange in their level, suggesting that the effect of rrs1-1 mutationon the response to a secretory defect is not due to a change ofrrs1-1 concentration in thecell.

Rrs1-HA appears to be localized throughout the nucleus, including the nucleolus (Fig. 6). The nucleolus is the site of rRNAsynthesis, rRNA processing, and ribosomal subunit assembly (reviewedin reference 38). Ribosomal proteins newly synthesized in thecytoplasm need to be transported into the nucleolus and assembledwith rRNAs. The assembled preribosomal subunits are then transportedinto the cytoplasm. During ribosome assembly, pre-rRNAs are modifiedand cleaved to mature rRNAs. Pre-rRNA processing and assemblyof ribosomal subunits are tightly linked to each other becausemany ribosomal proteins associate with the pre-rRNA at early stepsprior to cleavage. For example, mutants of the 60S subunit proteinL11 (according to a new nomenclature in reference 18; formerlycalled L16) exhibit a shortage of mature 25S rRNA and accumulationof rRNA precursors (22). Many trans-acting factors have beenfound to be involved in pre-rRNA processing and ribosomal subunitassembly steps (reviewed in reference 34). Some of them havean enzymatic activity such as RNA cleavage, methylation, or pseudouridineformation (2, 12, 13, 19, 31). Others may have a rolein maintaining the structure of the complex containing pre-rRNA(s)and many ribosomal proteins. Depletion of such factors may causestructural changes of the complex and prevent further processingof pre-rRNA. In Rrs1p-depleted cells, pre-rRNA processing is retardedat the A0, A1, and A2 sites, and consequently, less 25S and 18Smature rRNA is produced. Instead, aberrant cleavage produces 23SrRNA, as was shown in other mutants (5, 14, 16, 41).In [methyl-³H]methionine-pulse chase analysis of rrs1-1 and GAL-RRS1 (Fig.7A and 8B), the 20S band appears to be a doublet. The upper bandseems to be 21S produced by aberrant cleavage (35). Steady-statelevels of 18S and 25S rRNAs decline along with depletion of Rrs1p.These results suggest that Rrs1p has a role in maintaining thestructure of preribosomal subunit particles rather than a roleas a specific enzyme in a step of pre-rRNAprocessing.

Interestingly, the rrs1-1 mutation strongly diminished transcriptional repression of both ribosomal protein genes and rDNAin response to a secretory defect (Fig. 1 and 2). These resultssuggest that Rrs1p may have an important role in transcriptionalregulation of both rRNA and ribosomal protein genes. However,neither the rrs1-1 mutation nor the depletion of Rrs1p causesa significant defect in transcription of ribosomal protein genesunder the conditions in which the secretory pathway is normal.Rrs1p may have a role in maintenance of balanced transcriptionbetween the components of the ribosome. Depletion of Rrs1p usinga conditional rrs1-null mutation caused defects in pre-rRNA processingand ribosomal subunit assembly; slow processing of pre-rRNA, reducedproduction of 25S rRNA, decrease in levels of 80S ribosomes andpolyribosomes, accumulation of 40S ribosomal subunits, and theappearance of half-mer polyribosomes which contain 43S initiationcomplexes stalled at the AUG start codon. The result indicatesthat Rrs1p depletion strongly affects maturation of 25S rRNA and60S subunit assembly rather than that of 18S rRNA and 40S subunitassembly. [methyl-³H]methionine pulse-chase analysis and the polyribosome patternfrom the rrs1-1 mutant cells cultured at 18°C also suggest itsdefect in 25S rRNA production and 60S subunit assembly (Fig. 7B).These results suggest that rrs1-1 or Rrs1p depletion affects primarily25S rRNA maturation and 60S subunit assembly. The decline of the18S rRNA level in Rrs1p-depleted cells may be a secondary effect.The cold-sensitive phenotype of the rrs1-1 mutant may be explainedby its defect in assembly of ribosomal subunits; many yeast mutantsthat had defects in ribosomal subunit assembly were isolated byscreening from a collection of cold-sensitive strains (28).

Transcription of ribosomal protein genes is temporarily repressed by heat shock (7, 11). The rrs1-1 allele has littleeffect on the temporary repression of transcription brought aboutby mild heat shock, in contrast to its effect on the secretoryresponse (Fig. 3). This suggests that RRS1 is not required forthe temporary repression of ribosomal protein genes after temperatureshift-up. This also indicates that the mechanism of the secretoryresponse is different from that of the heat shock response, consistentwith the results obtained by using a rap1-17 mutant (21).

The great majority of ribosomal protein genes are driven by a Rap1-binding site(s) (15, 40). A few ribosomal protein genes,including RPL3 (encoding ribosomal protein L3), have no site forRap1 but have a single Abf1-binding site instead (3, 6,8). Yet the transcription of all the ribosomal protein genesappears to be coordinated under several experimental conditions.A secretory defect also causes the coordinated repression of ribosomalprotein genes (20). We showed that the repression of both RPL28(Rap1 driven) and RPL3 (Abf1 driven) was diminished by the C-terminallytruncated rap1-17 mutation (21). This suggests that Rap1 isessential for the repression in response to a secretory defectbut Rap1-binding sites are not necessary as cis-acting elementfor the repression. In this paper, we have demonstrated that therrs1-1 mutation affects the repression of both RPL28 and RPL3(Fig. 1 and 2), suggesting that a common mechanism regulates thetranscription of both types ofgenes.

The mechanism of transcriptional repression of both rRNA and ribosomal protein genes in response to a secretory defect remainsto be elucidated. Our data suggest that Rrs1p is involved in thismechanism, although there are several alternative possibilities.One possibility is that the slow growth of rrs1-1 may result ininsensitivity to a secretory defect. However, other mutants whichexhibit slow growth still respond to a defect in the secretorypathway (data not shown). The second possibility is that a feedbackeffect of a defect in ribosome synthesis of rrs1-1 mutation canovercome the effect caused by a secretory defect. We cannot eliminatethis possibility completely, but the rrs1-1 allele has littleeffect on the temporary repression of transcription of ribosomalprotein genes brought about by mild heat shock (Fig. 3). Thissuggests that the rrs1-1 cells still have a potential to leadthe repression of ribosomal protein genes after temperature shift-up.Thus, we prefer an alternative possibility: the signal from asecretory defect might be transduced through the ribosome assemblymachinery, including Rrs1p. A two-hybrid screen using RRS1 asa bait has suggested that Rrs1p may interact with Rpl11 (Y. Matsuiet al., unpublished data). As Rpl11 is a ribosomal protein localizedon the surface of the large subunit (36), Rrs1p might associatewith the ribosome through interaction with Rpl11. The possibleassociation of Rrs1p with the ribosome is now under investigation.It is possible that ribosomal assembly machinery that involvesan interaction of Rrs1p with Rpl11 might be important for theregulation. According to this model, the mechanism of transcriptionalrepression in response to a secretory defect is tightly linkedto the normal regulatory mechanism that maintains ribosome synthesis.The C-terminal region of Rrs1p that is deleted in rrs1-1 mightbe responsible for the signaling. In this case, transcriptionalrepression of ribosomal protein genes may follow the repressionof rRNA genes and the C-terminal region of Rrs1p may be requiredfor thesignaling.

	ACKNOWLEDGMENTS

We thank E. Tsuchiya, D. Hirata, and A. Wada for valuable discussion, M. D. Rose for yeast genomic DNA library, K. Matsumotoand Y. Ohya for a plasmid, H. Yoshida and Y. Maki for help inpolyribosome analysis, and N. Tanaka for help in the databasesearch. We also thank Y. Matsui and A. Toh-e for communicatingunpublished data. We are particularly grateful to J. R. Warnerfor critical reading of themanuscript.

This research was supported by grants from the Ministry of Education, Science and Culture of Japan and Special CoordinationFunds for Promoting Science and Technology of the Science andTechnology Agency of the Japanesegovernment.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Biotechnology, Graduate School of Advanced Sciences of Matter,Hiroshima University, Kagamiyama 1-4-1, Higashi-Hiroshima 739-8527,Japan. Phone: 81 824 24 7765. Fax: 81 824 22 7196. E-mail: kmizuta{at}ipc.hiroshima-u.ac.jp.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bergès, T., E. Petfalski, D. Tollervey, and E. C. Hurt. 1994. Synthetic lethality with fibrillarin identifies NOP77p, a nucleolar protein required for pre-rRNA processing and modification. EMBO J. 13:3136-3148[Medline].

2. Chu, S., R. H. Archer, J. M. Zengel, and L. Lindahl. 1994. The RNA of Rnase MRP is required for normal processing of ribosomal RNA. Proc. Natl. Acad. Sci. USA 91:659-663[Abstract/Free Full Text].

3. Dorsman, J. C., M. M. Doorenbosch, C. T. C. Maurer, J. H. de Winde, W. H. Mager, R. J. Planta, and L. A. Grivell. 1989. An ARS/silencer binding factor also activates two ribosomal protein genes in yeast. Nucleic Acids Res. 17:4917-4923[Abstract/Free Full Text].

4. Eng, F. J., and J. R. Warner. 1991. Structural basis for the regulation of splicing of a yeast messenger RNA. Cell 65:797-804[CrossRef][Medline].

5. Gautier, T., T. Bergès, D. Tollervey, and E. Hurt. 1997. Nucleolar KKE/D repeat proteins Nop56p and Nop58p interact with Nop1p and are required for ribosome biogenesis. Mol. Cell. Biol. 17:7088-7098[Abstract].

6. Hamil, K. G., H. G. Nam, and H. M. Fried. 1988. Constitutive transcription of yeast ribosomal protein gene RPL3 is promoted by uncommon cis- and trans-acting elements. Mol. Cell. Biol. 8:4328-4341[Abstract/Free Full Text].

7. Herruer, M. H., W. H. Mager, H. A. Raué, P. Vreken, E. Wilms, and R. J. Planta. 1988. Mild temperature shock affects transcription of yeast ribosomal protein genes as well as the stability of their mRNAs. Nucleic Acids Res. 16:7917-7929[Abstract/Free Full Text].

8. Herruer, M. H., W. H. Mager, T. M. Doorenbosch, P. L. M. Wessels, T. M. Wassenaar, and R. J. Planta. 1989. The extended promoter of the gene encoding ribosomal protein S33 in yeast consists of multiple protein binding elements. Nucleic Acids Res. 17:7427-7439[Abstract/Free Full Text].

9. Ito, H., Y. Fukuda, K. Murata, and A. Kimura. 1983. Transformation of intact yeast cells treated with alkali cations. J. Bacteriol. 153:163-168[Abstract/Free Full Text].

10. Kaiser, C., S. Michaelis, and A. Mitchell. 1994. Methods in yeast genetics. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

11. Kim, C. H., and J. R. Warner. 1983. Mild temperature shock alters the transcription of a discrete class of Saccharomyces cerevisiae genes. Mol. Cell. Biol. 3:457-465[Abstract/Free Full Text].

12. Kiss-Laszlo, Z., Y. Henry, J. Bachellerie, M. Caizergues-Ferrer, and T. Kiss. 1996. Site-specific ribose methylation of preribosomal RNA: a novel function for small nucleolar RNAs. Cell 85:1077-1088[CrossRef][Medline].

13. Lafontaine, D. L. J., C. Bousquet-Antonelli, Y. Henry, M. Caizergues-Ferrer, and D. Tollervey. 1998. The box H+ACA snoRNAs carry Cbf5p, the putative rRNA pseudouridine synthase. Genes Dev. 12:527-537[Abstract/Free Full Text].

14. Lafontaine, D. L. J., T. Preiss, and D. Tollervey. 1998. Yeast 18S rRNA dimethylase Dim1p: a quality control mechanism in ribosome synthesis? Mol. Cell. Biol. 18:2360-2370[Abstract/Free Full Text].

15. Lascaris, R. F., W. H. Mager, and R. Planta. 1999. DNA-binding requirements of the yeast protein Rap1p as selected in silico from ribosomal protein gene promoter sequences. Bioinformatics 15:267-277[Abstract/Free Full Text].

16. Lee, S. J., and S. J. Baserga. 1999. Imp3p and Imp4p, two specific components of the U3 small nucleolar ribonucleoprotein that are essential for pre-18S rRNA processing. Mol. Cell. Biol. 19:5441-5452[Abstract/Free Full Text].

17. Li, B., and J. R. Warner. 1996. Mutation of the Rab6 homologue of Saccharomyces cerevisiae, YPT6, inhibits both early Golgi function and ribosome biosynthesis. J. Biol. Chem. 271:16813-16819[Abstract/Free Full Text].

18. Mager, W. H., R. J. Planta, J.-P. G. Ballesta, J. C. Lee, K. Mizuta, K. Suzuki, J. R. Warner, and J. Woolford. 1997. A new nomenclature for the cytoplasmic ribosomal proteins of Saccharomyces cerevisiae. Nucleic Acids Res. 25:4872-4875[Abstract/Free Full Text].

19. Mitchell, P., E. Petfalski, A. Shevchenko, M. Mann, and D. Tollervey. 1997. The exosome: a conserved eukaryotic RNA processing complex containing multiple 3'-5' exoribonucleases. Cell 91:457-466[CrossRef][Medline].

20. Mizuta, K., and J. R. Warner. 1994. Continued functioning of the secretory pathway is essential for ribosome synthesis. Mol. Cell. Biol. 14:2493-2502[Abstract/Free Full Text].

21. Mizuta, K., R. Tsujii, J. R. Warner, and M. Nishiyama. 1998. The C-terminal silencing domain of Rap1p is essential for the repression of ribosomal protein genes in response to a defect in the secretory pathway. Nucleic Acids Res. 26:1063-1069[Abstract/Free Full Text].

22. Moritz, M., B. A. Pulaski, and J. L. Woolford, Jr. 1991. Assembly of 60S ribosomal subunits is perturbed in temperature-sensitive yeast mutants defective in ribosomal protein L16. Mol. Cell. Biol. 11:5681-5692[Abstract/Free Full Text].

23. Nagase, T., N. Miyajima, A. Tanaka, T. Sazuka, N. Seki, S. Sato, S. Tabata, K.-I. Ishikawa, Y. Kawarabayasi, H. Kotani, and N. Nomura. 1995. Prediction of the coding sequences of unidentified human genes. III. The coding sequences of 40 new genes (KIAA0081-KIAA0120) deduced by analysis of cDNA clones from human cell line KG-1. DNA Res. 2:37-43[Abstract].

24. Nierras, C. R., and J. R. Warner. 1999. Protein kinase C enables the regulatory circuit that connects membrane synthesis to ribosome synthesis in Saccharomyces cerevisiae. J. Biol. Chem. 274:13235-13241[Abstract/Free Full Text].

25. Ninomiya-Tsuji, J., S. Nomoto, H. Yasuda, S. I. Reed, and K. Mutsumoto. 1991. Cloning of a human cDNA encoding a CDC2-related kinase by complementation of a budding yeast cdc28 mutation. Proc. Natl. Acad. Sci. USA 88:9006-9010[Abstract/Free Full Text].

26. Ossig, R., C. Dascher, H.-H. Trepte, H. D. Schmitt, and D. Gallwitz. 1991. The yeast SLY gene products, suppressors of defects in the essential GTP-binding Ypt1 protein, may act in endoplasmic reticulum-to-Golgi transport. Mol. Cell. Biol. 11:2980-2993[Abstract/Free Full Text].

27. Pringle, J. R., A. E. M. Adams, D. G. Drubin, and B. K. Haarer. 1991. Immunofluorescence methods for yeast. Methods Enzymol. 194:565-602[Medline].

28. Ripmaster, T. L., G. P. Vaughn, and J. L. Woolford, Jr. 1993. DRS1 to DRS7, novel genes required for ribosome assembly and function in Saccharomyces cerevisiae. Mol. Cell. Biol. 13:7901-7912[Abstract/Free Full Text].

29. Rose, M. D., P. Novick, J. H. Thomas, D. Botstein, and G. R. Fink. 1987. A Saccharomyces cerevisiae genomic plasmid bank based on a centromere-containing shuttle vector. Gene 60:237-243[CrossRef][Medline].

30. Rotenberg, M. O., and J. L. Woolford, Jr. 1986. Tripartite upstream promoter element essential for expression of Saccharomyces cerevisiae ribosomal protein genes. Mol. Cell. Biol. 6:674-687[Abstract/Free Full Text].

31. Schmitt, M. E., and D. A. Clayton. 1993. Nuclear RNase MRP is required for correct processing of pre-5.8S rRNA in Saccharomyces cerevisiae. Mol. Cell. Biol. 13:7935-7941[Abstract/Free Full Text].

32. Sikorski, R., and P. Hieter. 1989. A system of shuttle vectors and yeast host strains designed for efficient manipulation of DNA in Saccharomyces cerevisiae. Genetics 122:19-27[Abstract/Free Full Text].

33. Takita, Y., Y. Ohya, and Y. Anraku. 1995. The CLS2 gene encodes a protein with multiple membrane-spanning domains that is important Ca2+ tolerance in yeast. Mol. Gen. Genet. 246:269-281[CrossRef][Medline].

34. Tollervey, D. 1996. trans-acting factors in ribosome synthesis. Exp. Cell Res. 229:226-232[CrossRef][Medline].

35. Tollervey, D. 1987. A yeast small nuclear RNA is required for normal processing of pre-ribosomal RNA. EMBO J. 6:4169-4175[Medline].

36. Tsay, Y.-F., G. Shankweiler, J. Lake, and J. L. Woolford, Jr. 1994. Localization of Saccharomyces cerevisiae ribosomal protein L16 on the surface of 60S ribosomal subunits by immunoelectron microscopy. J. Biol. Chem. 269:7579-7586[Abstract/Free Full Text].

37. Udem, S. A., and J. R. Warner. 1972. Ribosomal RNA synthesis in Saccharomyces cerevisiae. J. Mol. Biol. 65:227-242[CrossRef][Medline].

38. Warner, J. R. 1990. The nucleolus and ribosome formation. Curr. Opin. Cell Biol. 2:521-527[CrossRef][Medline].

39. Wilson, R., et al. 1994. 2.2 Mb of contiguous nucleotide sequence from chromosome III of C. elegans. Nature 368:32-38[CrossRef][Medline].

40. Woolford, J. L., Jr., and J. R. Warner. 1991. The ribosome and its synthesis, p. 587-626. In J. R. Broach, J. R. Pringle, and E. W. Jones (ed.), The molecular and cellular biology of the yeast Saccharomyces: genome dynamics, protein synthesis, and energetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

41. Zanchin, N. I. T., and D. S. Goldfarb. 1999. Nip7p interacts with Nop8p, an essential nucleolar protein required for 60S ribosome biogenesis, and the exosome subunit Rrp43p. Mol. Cell. Biol. 19:1518-1525[Abstract/Free Full Text].

This article has been cited by other articles:

Carnemolla, A., Fossale, E., Agostoni, E., Michelazzi, S., Calligaris, R., De Maso, L., Del Sal, G., MacDonald, M. E., Persichetti, F. (2009). Rrs1 Is Involved in Endoplasmic Reticulum Stress Response in Huntington Disease. J. Biol. Chem. 284: 18167-18173 [Abstract] [Full Text]
Yamada, H., Horigome, C., Okada, T., Shirai, C., Mizuta, K. (2007). Yeast Rrp14p is a nucleolar protein involved in both ribosome biogenesis and cell polarity. RNA 13: 1977-1987 [Abstract] [Full Text]
Nariai, M., Tanaka, T., Okada, T., Shirai, C., Horigome, C., Mizuta, K. (2005). Synergistic defect in 60S ribosomal subunit assembly caused by a mutation of Rrs1p, a ribosomal protein L11-binding protein, and 3'-extension of 5S rRNA in Saccharomyces cerevisiae. Nucleic Acids Res 33: 4553-4562 [Abstract] [Full Text]
Shirai, C., Takai, T., Nariai, M., Horigome, C., Mizuta, K. (2004). Ebp2p, the Yeast Homolog of Epstein-Barr Virus Nuclear Antigen 1-binding Protein 2, Interacts with Factors of Both the 60 S and the 40 S Ribosomal Subunit Assembly. J. Biol. Chem. 279: 25353-25358 [Abstract] [Full Text]
Miyoshi, K., Shirai, C., Mizuta, K. (2003). Transcription of genes encoding trans-acting factors required for rRNA maturation/ribosomal subunit assembly is coordinately regulated with ribosomal protein genes and involves Rap1 in Saccharomyces cerevisiae. Nucleic Acids Res 31: 1969-1973 [Abstract] [Full Text]
Fossale, E., Wheeler, V. C., Vrbanac, V., Lebel, L.-A., Teed, A., Mysore, J. S., Gusella, J. F., MacDonald, M. E., Persichetti, F. (2002). Identification of a presymptomatic molecular phenotype in Hdh CAG knock-in mice. Hum Mol Genet 11: 2233-2241 [Abstract] [Full Text]
Morita, D., Miyoshi, K., Matsui, Y., Toh-e, A., Shinkawa, H., Miyakawa, T., Mizuta, K. (2002). Rpf2p, an Evolutionarily Conserved Protein, Interacts with Ribosomal Protein L11 and Is Essential for the Processing of 27 SB Pre-rRNA to 25 S rRNA and the 60 S Ribosomal Subunit Assembly in Saccharomyces cerevisiae. J. Biol. Chem. 277: 28780-28786 [Abstract] [Full Text]
Miyoshi, K., Tsujii, R., Yoshida, H., Maki, Y., Wada, A., Matsui, Y., Toh-e, A., Mizuta, K. (2002). Normal Assembly of 60 S Ribosomal Subunits Is Required for the Signaling in Response to a Secretory Defect in Saccharomyces cerevisiae. J. Biol. Chem. 277: 18334-18339 [Abstract] [Full Text]
Wade, C., Shea, K. A., Jensen, R. V., McAlear, M. A. (2001). EBP2 Is a Member of the Yeast RRB Regulon, a Transcriptionally Coregulated Set of Genes That Are Required for Ribosome and rRNA Biosynthesis. Mol. Cell. Biol. 21: 8638-8650 [Abstract] [Full Text]
Miyoshi, K., Miyakawa, T., Mizuta, K. (2001). Repression of rRNA synthesis due to a secretory defect requires the C-terminal silencing domain of Rap1p in Saccharomyces cerevisiae. Nucleic Acids Res 29: 3297-3303 [Abstract] [Full Text]
Geiss, G. K., An, M. C., Bumgarner, R. E., Hammersmark, E., Cunningham, D., Katze, M. G. (2001). Global Impact of Influenza Virus on Cellular Pathways Is Mediated by both Replication-Dependent and -Independent Events. J. Virol. 75: 4321-4331 [Abstract] [Full Text]
Iouk, T. L., Aitchison, J. D., Maguire, S., Wozniak, R. W. (2001). Rrb1p, a Yeast Nuclear WD-Repeat Protein Involved in the Regulation of Ribosome Biosynthesis. Mol. Cell. Biol. 21: 1260-1271 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Tsuno, A.
	Articles by Mizuta, K.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Tsuno, A.
	Articles by Mizuta, K.

1.	Bergès, T., E. Petfalski, D. Tollervey, and E. C. Hurt. 1994. Synthetic lethality with fibrillarin identifies NOP77p, a nucleolar protein required for pre-rRNA processing and modification. EMBO J. 13:3136-3148[Medline].
2.	Chu, S., R. H. Archer, J. M. Zengel, and L. Lindahl. 1994. The RNA of Rnase MRP is required for normal processing of ribosomal RNA. Proc. Natl. Acad. Sci. USA 91:659-663[Abstract/Free Full Text].
3.	Dorsman, J. C., M. M. Doorenbosch, C. T. C. Maurer, J. H. de Winde, W. H. Mager, R. J. Planta, and L. A. Grivell. 1989. An ARS/silencer binding factor also activates two ribosomal protein genes in yeast. Nucleic Acids Res. 17:4917-4923[Abstract/Free Full Text].
4.	Eng, F. J., and J. R. Warner. 1991. Structural basis for the regulation of splicing of a yeast messenger RNA. Cell 65:797-804[CrossRef][Medline].
5.	Gautier, T., T. Bergès, D. Tollervey, and E. Hurt. 1997. Nucleolar KKE/D repeat proteins Nop56p and Nop58p interact with Nop1p and are required for ribosome biogenesis. Mol. Cell. Biol. 17:7088-7098[Abstract].
6.	Hamil, K. G., H. G. Nam, and H. M. Fried. 1988. Constitutive transcription of yeast ribosomal protein gene RPL3 is promoted by uncommon cis- and trans-acting elements. Mol. Cell. Biol. 8:4328-4341[Abstract/Free Full Text].
7.	Herruer, M. H., W. H. Mager, H. A. Raué, P. Vreken, E. Wilms, and R. J. Planta. 1988. Mild temperature shock affects transcription of yeast ribosomal protein genes as well as the stability of their mRNAs. Nucleic Acids Res. 16:7917-7929[Abstract/Free Full Text].
8.	Herruer, M. H., W. H. Mager, T. M. Doorenbosch, P. L. M. Wessels, T. M. Wassenaar, and R. J. Planta. 1989. The extended promoter of the gene encoding ribosomal protein S33 in yeast consists of multiple protein binding elements. Nucleic Acids Res. 17:7427-7439[Abstract/Free Full Text].
9.	Ito, H., Y. Fukuda, K. Murata, and A. Kimura. 1983. Transformation of intact yeast cells treated with alkali cations. J. Bacteriol. 153:163-168[Abstract/Free Full Text].
10.	Kaiser, C., S. Michaelis, and A. Mitchell. 1994. Methods in yeast genetics. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
11.	Kim, C. H., and J. R. Warner. 1983. Mild temperature shock alters the transcription of a discrete class of Saccharomyces cerevisiae genes. Mol. Cell. Biol. 3:457-465[Abstract/Free Full Text].
12.	Kiss-Laszlo, Z., Y. Henry, J. Bachellerie, M. Caizergues-Ferrer, and T. Kiss. 1996. Site-specific ribose methylation of preribosomal RNA: a novel function for small nucleolar RNAs. Cell 85:1077-1088[CrossRef][Medline].
13.	Lafontaine, D. L. J., C. Bousquet-Antonelli, Y. Henry, M. Caizergues-Ferrer, and D. Tollervey. 1998. The box H+ACA snoRNAs carry Cbf5p, the putative rRNA pseudouridine synthase. Genes Dev. 12:527-537[Abstract/Free Full Text].
14.	Lafontaine, D. L. J., T. Preiss, and D. Tollervey. 1998. Yeast 18S rRNA dimethylase Dim1p: a quality control mechanism in ribosome synthesis? Mol. Cell. Biol. 18:2360-2370[Abstract/Free Full Text].
15.	Lascaris, R. F., W. H. Mager, and R. Planta. 1999. DNA-binding requirements of the yeast protein Rap1p as selected in silico from ribosomal protein gene promoter sequences. Bioinformatics 15:267-277[Abstract/Free Full Text].
16.	Lee, S. J., and S. J. Baserga. 1999. Imp3p and Imp4p, two specific components of the U3 small nucleolar ribonucleoprotein that are essential for pre-18S rRNA processing. Mol. Cell. Biol. 19:5441-5452[Abstract/Free Full Text].
17.	Li, B., and J. R. Warner. 1996. Mutation of the Rab6 homologue of Saccharomyces cerevisiae, YPT6, inhibits both early Golgi function and ribosome biosynthesis. J. Biol. Chem. 271:16813-16819[Abstract/Free Full Text].
18.	Mager, W. H., R. J. Planta, J.-P. G. Ballesta, J. C. Lee, K. Mizuta, K. Suzuki, J. R. Warner, and J. Woolford. 1997. A new nomenclature for the cytoplasmic ribosomal proteins of Saccharomyces cerevisiae. Nucleic Acids Res. 25:4872-4875[Abstract/Free Full Text].
19.	Mitchell, P., E. Petfalski, A. Shevchenko, M. Mann, and D. Tollervey. 1997. The exosome: a conserved eukaryotic RNA processing complex containing multiple 3'-5' exoribonucleases. Cell 91:457-466[CrossRef][Medline].
20.	Mizuta, K., and J. R. Warner. 1994. Continued functioning of the secretory pathway is essential for ribosome synthesis. Mol. Cell. Biol. 14:2493-2502[Abstract/Free Full Text].
21.	Mizuta, K., R. Tsujii, J. R. Warner, and M. Nishiyama. 1998. The C-terminal silencing domain of Rap1p is essential for the repression of ribosomal protein genes in response to a defect in the secretory pathway. Nucleic Acids Res. 26:1063-1069[Abstract/Free Full Text].
22.	Moritz, M., B. A. Pulaski, and J. L. Woolford, Jr. 1991. Assembly of 60S ribosomal subunits is perturbed in temperature-sensitive yeast mutants defective in ribosomal protein L16. Mol. Cell. Biol. 11:5681-5692[Abstract/Free Full Text].
23.	Nagase, T., N. Miyajima, A. Tanaka, T. Sazuka, N. Seki, S. Sato, S. Tabata, K.-I. Ishikawa, Y. Kawarabayasi, H. Kotani, and N. Nomura. 1995. Prediction of the coding sequences of unidentified human genes. III. The coding sequences of 40 new genes (KIAA0081-KIAA0120) deduced by analysis of cDNA clones from human cell line KG-1. DNA Res. 2:37-43[Abstract].
24.	Nierras, C. R., and J. R. Warner. 1999. Protein kinase C enables the regulatory circuit that connects membrane synthesis to ribosome synthesis in Saccharomyces cerevisiae. J. Biol. Chem. 274:13235-13241[Abstract/Free Full Text].
25.	Ninomiya-Tsuji, J., S. Nomoto, H. Yasuda, S. I. Reed, and K. Mutsumoto. 1991. Cloning of a human cDNA encoding a CDC2-related kinase by complementation of a budding yeast cdc28 mutation. Proc. Natl. Acad. Sci. USA 88:9006-9010[Abstract/Free Full Text].
26.	Ossig, R., C. Dascher, H.-H. Trepte, H. D. Schmitt, and D. Gallwitz. 1991. The yeast SLY gene products, suppressors of defects in the essential GTP-binding Ypt1 protein, may act in endoplasmic reticulum-to-Golgi transport. Mol. Cell. Biol. 11:2980-2993[Abstract/Free Full Text].
27.	Pringle, J. R., A. E. M. Adams, D. G. Drubin, and B. K. Haarer. 1991. Immunofluorescence methods for yeast. Methods Enzymol. 194:565-602[Medline].
28.	Ripmaster, T. L., G. P. Vaughn, and J. L. Woolford, Jr. 1993. DRS1 to DRS7, novel genes required for ribosome assembly and function in Saccharomyces cerevisiae. Mol. Cell. Biol. 13:7901-7912[Abstract/Free Full Text].
29.	Rose, M. D., P. Novick, J. H. Thomas, D. Botstein, and G. R. Fink. 1987. A Saccharomyces cerevisiae genomic plasmid bank based on a centromere-containing shuttle vector. Gene 60:237-243[CrossRef][Medline].
30.	Rotenberg, M. O., and J. L. Woolford, Jr. 1986. Tripartite upstream promoter element essential for expression of Saccharomyces cerevisiae ribosomal protein genes. Mol. Cell. Biol. 6:674-687[Abstract/Free Full Text].
31.	Schmitt, M. E., and D. A. Clayton. 1993. Nuclear RNase MRP is required for correct processing of pre-5.8S rRNA in Saccharomyces cerevisiae. Mol. Cell. Biol. 13:7935-7941[Abstract/Free Full Text].
32.	Sikorski, R., and P. Hieter. 1989. A system of shuttle vectors and yeast host strains designed for efficient manipulation of DNA in Saccharomyces cerevisiae. Genetics 122:19-27[Abstract/Free Full Text].
33.	Takita, Y., Y. Ohya, and Y. Anraku. 1995. The CLS2 gene encodes a protein with multiple membrane-spanning domains that is important Ca2+ tolerance in yeast. Mol. Gen. Genet. 246:269-281[CrossRef][Medline].
34.	Tollervey, D. 1996. trans-acting factors in ribosome synthesis. Exp. Cell Res. 229:226-232[CrossRef][Medline].
35.	Tollervey, D. 1987. A yeast small nuclear RNA is required for normal processing of pre-ribosomal RNA. EMBO J. 6:4169-4175[Medline].
36.	Tsay, Y.-F., G. Shankweiler, J. Lake, and J. L. Woolford, Jr. 1994. Localization of Saccharomyces cerevisiae ribosomal protein L16 on the surface of 60S ribosomal subunits by immunoelectron microscopy. J. Biol. Chem. 269:7579-7586[Abstract/Free Full Text].
37.	Udem, S. A., and J. R. Warner. 1972. Ribosomal RNA synthesis in Saccharomyces cerevisiae. J. Mol. Biol. 65:227-242[CrossRef][Medline].
38.	Warner, J. R. 1990. The nucleolus and ribosome formation. Curr. Opin. Cell Biol. 2:521-527[CrossRef][Medline].
39.	Wilson, R., et al. 1994. 2.2 Mb of contiguous nucleotide sequence from chromosome III of C. elegans. Nature 368:32-38[CrossRef][Medline].
40.	Woolford, J. L., Jr., and J. R. Warner. 1991. The ribosome and its synthesis, p. 587-626. In J. R. Broach, J. R. Pringle, and E. W. Jones (ed.), The molecular and cellular biology of the yeast Saccharomyces: genome dynamics, protein synthesis, and energetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
41.	Zanchin, N. I. T., and D. S. Goldfarb. 1999. Nip7p interacts with Nop8p, an essential nucleolar protein required for 60S ribosome biogenesis, and the exosome subunit Rrp43p. Mol. Cell. Biol. 19:1518-1525[Abstract/Free Full Text].