The Saccharomyces cerevisiae Hyperrecombination Mutant hpr1Delta  Is Synthetically Lethal with Two Conditional Alleles of the Acetyl Coenzyme A Carboxylase Gene and Causes a Defect in Nuclear Export of Polyadenylated RNA

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Molecular and Cellular Biology, May 1999, p. 3415-3422, Vol. 19, No. 5
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The Saccharomyces cerevisiae Hyperrecombination Mutant hpr1 $Delta$ Is Synthetically Lethal with Two Conditional Alleles of the Acetyl Coenzyme A Carboxylase Gene and Causes a Defect in Nuclear Export of Polyadenylated RNA

Roger Schneiter,¹ Cesar E. Guerra,²^, Manfred Lampl,¹ Gabriela Gogg,¹ Sepp D. Kohlwein,¹ and Hannah L. Klein²^,^*

Institut für Biochemie und Lebensmittelchemie, Technische Universität Graz, A-8010 Graz, Austria,¹ and Department of Biochemistry, New York University Medical Center, New York, New York 10016²

Received 20 August 1998/Returned for modification 26 October 1998/Accepted 12 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In a screen for mutants that display synthetic lethal interaction with hpr1 $Delta$ , a hyperrecombination mutant of Saccharomycescerevisiae, we have isolated a novel cold-sensitive allele ofthe acetyl coenzyme A (CoA) carboxylase gene, acc1^cs, encoding the rate-limiting enzyme of fatty acid synthesis. Thesynthetic lethal phenotype of the acc1^cs hpr1 $Delta$ double mutant was only partially complemented by exogenousfatty acids. hpr1 $Delta$ was also synthetically lethal with a previouslyisolated, temperature-sensitive allele of ACC1, mtr7 (mRNA transport),indicating that the lethality of the acc1^cs hpr1 $Delta$ double mutant was not allele specific. The basis for theinteraction between conditional acc1 alleles and hpr1 $Delta$ was investigatedin more detail. In the hpr1 $Delta$ mutant background, acetyl-CoA carboxylaseenzyme activity was reduced about 15-fold and steady-state levelsof biotinylated Acc1p and ACC1 mRNA were reduced 2-fold. The reducedAcc1p activity in hpr1 $Delta$ cells, however, did not result in an alteredlipid or fatty acid composition of the mutant membranes but renderedcells hypersensitive to soraphen A, an inhibitor of Acc1p. Similarto mtr7, hpr1 $Delta$ and acc1^cs mutant cells displayed a defect in nuclear export of polyadenylatedRNA. Oversized transcripts were detected in hpr1 $Delta$ , and rRNA processingwas disturbed, but pre-mRNA splicing appeared wild type. Surprisingly,the transport defect of hpr1 $Delta$ and acc1^cs mutant cells was accompanied by an altered ring-shaped structureof the nucleolus. These observations suggest that the basis forthe synthetic lethal interaction between hpr1 $Delta$ and acc1 may liein a functional overlap of the two mutations in nuclear poly(A)⁺ RNA production and export that results in an altered structureof thenucleolus.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The hpr1 $Delta$ mutant of Saccharomyces cerevisiae was isolated in a screen for mutations that confer an increased mitotic recombination(1, 2). The hpr1 $Delta$ null mutant is temperature sensitive forgrowth at 37°C and displays a 700-fold-elevated rate of mitoticintrachromatid recombination. Hpr1p has two regions of homologyto topoisomerase I, Top1p (3, 40), and hpr1 $Delta$ mutants displaysynthetic lethality with mutations in all three DNA topoisomerasegenes, TOP1, TOP2, and TOP3 (3). A fourth synthetic lethalinteraction has been found between hpr1 $Delta$ and a mutant carryinga deletion of one copy of the histone H3-H4 genes (10).

In hpr1 $Delta$ null mutants, transcription of many physiologically unrelated genes is affected (44) and the temperature-sensitivegrowth phenotype of hpr1 $Delta$ mutants is suppressed by mutations incomponents of the general transcription machinery (12, 27,41). The Hpr1 protein has been found to be in a distinct RNApolymerase II complex (8) and has been suggested to have afunctional role in transcription elongation (9).

To better understand the in vivo function of Hpr1p, a screen was initiated to isolate additional mutants that exhibit syntheticlethal interaction with hpr1 $Delta$ . This screen yielded a novel cold-sensitiveallele of the acetyl coenzyme A (CoA) carboxylase gene, acc1-200^cs, hereafter referred to as acc1^cs (14).

The acetyl-CoA carboxylase gene, ACC1, encodes a biotin-containing enzyme that synthesizes malonyl-CoA from acetyl-CoA andbicarbonate, with the hydrolysis of ATP (4). Acc1p is the rate-limitingenzyme of the de novo fatty acid biosynthetic pathway. Expressionof the ACC1 gene is under coordinate transcriptional regulationby the phospholipid precursors inositol and choline (15). Atemperature-sensitive allele of ACC1, mtr7, has been isolatedin a screen for mutants that affect nuclear export of polyadenylatedRNA (18; for a review, see reference 39). The nuclear transportdefect of this acc1^ts allele has been proposed to be due to a special lipid requirementof the nuclear membrane-nuclear pore complex (31, 33).

The basis for the synthetic lethality between hpr1 $Delta$ and the cold-sensitive acc1^cs allele was investigated in more detail. We find that hpr1 $Delta$ mutantcells have a very strong defect in export of nuclear poly(A)⁺ RNA, a phenotype previously observed in a temperature-sensitiveallele of ACC1 (31), and propose that the lethal interactionbetween hpr1 $Delta$ and acc1^cs is due to a combined effect of the two mutations on nuclear exportof polyadenylatedRNA.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Yeast strains and culture conditions. The S. cerevisiae strains used for these experiments are listed in Table 1. Strains were grown in YEPD medium (1% yeast extract,2% Bacto Peptone, 2% glucose) or synthetic minimal medium (35)supplemented with appropriate amino acids and glucose. Mediumsupplemented with fatty acids contained 1% Tween 40, 0.015% palmiticacid, and 0.015% stearic acid (28). Soraphen A, a kind giftfrom A. Hinnen, was added to medium from a 10-mg/ml stock solutionin methanol. Optical density at 600 nm was monitored every hourfor growth rate determinations. The exponential growth rate inthe presence of soraphen A was established after a 3-h lag periodand was expressed as a percentage of the growth rate in the absenceof the inhibitor.

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TABLE 1. Yeast strain genotypes and construction

Isolation and analysis of RNA. Total yeast RNA was extracted from exponentially growing cultures as described previously (29). Ten milligrams of RNA perwell was fractionated by electrophoresis through a 0.8% agarose-3.7%formaldehyde gel and prepared for Northern blot analysis as describedpreviously (29). For quantification of ACC1 transcription, ³²P-labeled DNA probes were prepared according to the method inreference 13. Blots were serially hybridized to ACC1-specificand ACT1-specific DNA probes, in that order and without an intermediateprobe-stripping step. After autoradiography of the blots, eachlane in the exposed film was scanned in one dimension with theUltroScan XL system (LKB), and the ACC1/ACT1 ratios of peak areaswere calculated relative to the ratio in the MATa wild-typestrain. For detection of CRY1 message, filters were probed withdigoxigenin-labeled probe and signal was detected by enhancedchemiluminescence with CDP-Star substrate (Tropix, Bedford, Mass.).For the analysis of rRNA processing, mutant cells were transformedwith pRS316 (36) to make them uracil prototrophic. Cells wereincubated at nonpermissive temperatures for 1 h and then labeledwith 0.05 mCi of [³H]uridine per ml for 10min.

Immunofluorescence and in situ hybridization. Early-logarithmic-phase cells were prepared for immunofluorescence microscopy as previously described (31). Mouse monoclonalantibody against the yeast fibrillarin homologue, Nop1p, was appliedat a 1:5,000 dilution (6). Secondary fluorescein isothiocyanate-conjugatedantibody (Oncogene Science, Cambridge, Mass.) was used at a 1:200dilution. Detection of accumulated poly(A)⁺ RNA was performed essentially as described elsewhere (31),with the modification that digoxigenin-labeled oligo(dT)_25-30was used for hybridization. Secondary fluorescein isothiocyanate-conjugatedanti-sheep antibody was used at a 1:200 dilution. Laser scanningmicroscopic analysis was performed with a Leica TCS 4d confocalmicroscope equipped with a PL APO 100×/1.40 objective, and photographswere recorded on Ektachrome 100 film (Eastman Kodak Co., Rochester,N.Y.). Corresponding pictures were recorded with identical pinholeopenings and amplification settings and were printed with thesame exposuretime.

Western blot analysis. Whole-cell protein extracts were prepared as described elsewhere (43), and protein concentration was determined accordingto the method of Lowry et al. (22), with bovine serum albuminas a standard. Proteins were separated by one-dimensional sodiumdodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (20),with 4% stacking and 10% separating gels. Proteins were transferredto nitrocellulose sheets (Hybond C; Amersham) and stained withPonceau S to assess transfer efficiency. Membranes were incubatedovernight in blocking solution containing 5% fat-free dry milkpowder in Tris-buffered saline (TBS) (50 mM Tris-HCl, 150 mM NaCl,pH 8.0). After two washes with TTBS (0.1% Tween 20 in TBS), membraneswere incubated with 10 µg of avidin-peroxidase conjugate (ExtrAvidinperoxidase; Sigma, St. Louis, Mo.), rabbit anti-Acc1p (1:700 [17]),or rabbit anti-glyceraldehyde-3-phosphate dehydrogenase (GAPDH)(1:5,000) per ml, diluted in TBS. Peroxidase-conjugated anti-rabbitimmunoglobulin G (Sigma) was used as secondary antibody. Signaldetection was carried out according to the instructions providedby the manufacturer with the ECL system (Amersham) and the SuperSignalCL-HRP substrate system (Pierce, Rockford, Ill.). Densitometricscanning of X-ray films and quantification of signals were carriedout with NIH Image 1.54software.

Acc1p activity determination. The cytosolic fraction used for Acc1p enzyme activity assays was prepared as follows. Cells were harvested at 1,200 × g for10 min, washed with 0.1 M K₂HPO₄-KH₂PO₄ buffer (pH 6.5), mixedwith breaking buffer (50 mM Tris-HCl, 100 mM NaF, 1 mM EDTA, 10mM $beta$ -mercaptoethanol, 0.25 M sucrose, 1 mM phenylmethylsulfonylfluoride, pH 7.5) and glass beads (0.30-mm diameter) in a ratioof 1:1:1 (wt/vol/wt), and disrupted by four 1-min bursts in aBraun-Melsungen homogenizer under CO₂ cooling. Glass beads werecollected by centrifugation at 3,000 × g for 5 min, and the supernatantwas centrifuged at 20,000 × g for 20 min and centrifuged againat 195,000 × g for 80 min. Saturated (NH₄)₂SO₄ was then addedin three portions within 20 min to 50% saturation, and sampleswere stirred for an additional 30 min. The precipitate was collectedby centrifugation at 15,000 × g, dissolved in HEPES buffer (50mM HEPES, 1 mM EDTA, 0.02% Na-azide, 50% glycerol, pH 7.0), andstored frozen at $-$ 20°C. Enzymatic activities of Acc1p were foundto be stable over a period of 3 weeks after freezing of samples.All steps were carried out at 4°C. Activity of acetyl-CoA carboxylasewas determined by a photometric assay in a coupled enzymatic reactionas described elsewhere (23). All enzyme measurements were carriedout at 24°C.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Synthetic lethality between acc1^cs and hpr1 $Delta$ . The acc1^cs acc1-200^cs allele was recovered in a screen for mutants that display a synthetic lethal interaction with a null alleleof HPR1 (14). The synthetic lethality of the acc1^cs hpr1 $Delta$ double mutant is indicated by the failure to recover sporecolonies of this genotype from a cross between an acc1^cs strain and an hpr1 $Delta$ strain. When the tetrads from this crosswere dissected on a YEPD plate supplemented with fatty acids,the acc1^cs hpr1 $Delta$ double mutant was viable but still showed reduced growthcompared to the single mutant strain or the wild-type strain (Fig.1).

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FIG. 1. acc1^cs is synthetically lethal with hpr1 $Delta$ . Growth of spore segregants from an acc1^cs × hpr1 $Delta$ cross. Asci were dissected on YEPD medium alone or YEPD medium supplemented with fatty acids and incubated for 3 days at 30°C. Germinated spores from each tetrad are arranged in vertical columns (1 to 9), and the corresponding genotypes are indicated by circles below as follows: wild-type spores, open circles; acc1^cs spores, vertically striped circles; hpr1 $Delta$ spores, horizontally striped circles; and double mutant spores, crosshatched circles.

Soraphen A sensitivity of acc1^cs and hpr1 $Delta$ mutants. Soraphen A is a potent inhibitor of Acc1p activity in yeast (42). The acc1^cs allele was found to confer hypersensitivity to soraphen A atthe permissive temperature (Fig. 2A). Since the acc1^cs allele is synthetically lethal with the hpr1 $Delta$ mutation, we examinedthe hpr1 $Delta$ mutant for soraphen A sensitivity. The hpr1 $Delta$ null mutantwas found to be as soraphen A sensitive as the acc1^cs mutant on solid medium (Fig. 2A) and in liquid medium (Fig. 2B).

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FIG. 2. Soraphen A sensitivity of the hpr1 $Delta$ mutant. (A) Strains with indicated genotypes were streaked onto YEPD medium (top) and YEPD medium containing 0.25 mg of soraphen A per ml (bottom) and incubated for 2 days at 30°C. wt, wild type. (B) Dose-response curves to soraphen A. The exponential growth rate was established after a 3-h lag period for various concentrations of soraphen A and is expressed as a percentage of the growth rate in the absence of soraphen A. The results for two strains of each genotype were averaged and plotted against the concentration of soraphen A. Curves are the best fit calculated with respect to Hill's equation (Hill coefficients, 3 to 4). Calculated 50% infective doses are 0.09 mg/ml for the wild type and 0.04 mg/ml for both the acc1^cs and the hpr1 $Delta$ strains.

The synthetic lethal interaction between hpr1 $Delta$ and acc1 is not allele specific. A temperature-sensitive allele of ACC1, mtr7, herein referred to as acc1^ts, had previously been isolated in a screen for conditional mRNAtransport mutants (31). To determine whether the synthetic lethalinteraction between acc1^cs and hpr1 $Delta$ is an allele-specific phenomenon, a cross between acc1^ts and hpr1 $Delta$ was performed. Diploids were sporulated, and tetradswere dissected on YEPD and YEPD plates supplemented with 1 M sorbitol.Sorbitol supplementation has been found to rescue the temperature-dependentgrowth phenotype of both conditional acc1 alleles (data not shown).While acc1^ts hpr1 $Delta$ double mutants were viable on sorbitol-supplemented medium,no acc1^ts hpr1 $Delta$ double mutants were recovered from YEPD or fatty acid-supplementedplates, indicating that acc1^ts is synthetically lethal with hpr1 $Delta$ (Fig. 3).

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FIG. 3. acc1^ts is synthetically lethal with hpr1 $Delta$ . An acc1^ts strain (YRXS12) was crossed with an hpr1 $Delta$ strain (U768-4C), diploids were sporulated, and tetrads were dissected. Four spores of a complete tetrad were replica plated on YEPD plates (top), YEPD supplemented with fatty acids (middle), and YEPD plates supplemented with 1 M sorbitol (bottom) and incubated at 30°C for 3 days. The relevant genotype of the spores is indicated on top. wt, wild type.

hpr1 $Delta$ affects Acc1p activity at the level of transcription. The observation that hpr1 $Delta$ is synthetically lethal with two different conditional acc1 alleles and that hpr1 $Delta$ itself is hypersensitiveto soraphen A suggested that Acc1p activity is affected in thehpr1 $Delta$ mutant. Acc1p enzymatic activity was determined in cytosolicfractions from the wild type and the hpr1 $Delta$ mutant strain. Cellswere grown in YEPD medium at 30°C, cytosol was prepared, and Acc1pactivity was determined as described previously (23). Acc1pactivity in the hpr1 $Delta$ mutant was reduced approximately 15-foldcompared to that in the wild type, as shown by the following data(means ± standard deviations of three determinations): enzymeactivity of wild type, 38.3 × 10⁵ ± 3.7 × 10⁵ $Delta$ E/min/µg; enzyme activity of the hpr1 $Delta$ mutant, 2.6 × 10⁵ ± 1.7 × 10⁵ $Delta$ E/min/µg. This greatly reduced Acc1p activity in the hpr1 $Delta$ mutantbackground, however, did not result in an altered lipid or fattyacid composition of hpr1 $Delta$ mutant cells compared to the wild type(data notshown).

To determine at which level the lack of Hpr1p function affects the activity of Acc1p, we analyzed steady-state levels of biotinylatedAcc1p. Protein was isolated from whole cells and blotted withperoxidase-labeled avidin to simultaneously detect biotinylatedAcc1p and the two pyruvate carboxylase isoenzymes Pyc1p and Pyc2p(Fig. 4). To control for internal loading, GAPDH was detectedby an anti-GAPDH antibody. Signal intensities of these blots werequantified, and ratios of biotinylated Acc1p to biotinylated Pycare listed in Table 2. This analysis revealed that the percentageof biotinylated Acc1p relative to biotinylated Pyc in the hpr1 $Delta$ mutant was 50% of that of the wild type.

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FIG. 4. Western blot analysis of biotinylated Acc1p levels in wild-type and hpr1 $Delta$ cells. Equal amounts of protein (10 µg) isolated from a whole-cell lysate were separated by SDS-gel electrophoresis, blotted, and probed with peroxidase-labeled avidin to detect biotinylated Acc1p and pyruvate carboxylase (Pyc) and anti-GAPDH or anti-Acc1p antibodies. Signal intensities were quantified and are listed in Table 2.

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TABLE 2. Biotinylated levels of Acc1 protein in wild-type and hpr1 $Delta$ cells^a

Preliminary results with a plasmid-borne ACC1-lacZ fusion as a reporter gene indicated that ACC1 expression was reduced twofoldin hpr1 $Delta$ strains compared to the wild type (data not shown). Toconfirm that expression of the chromosomal ACC1 gene was affectedin hpr1 $Delta$ strains, Northern blot analysis was carried out withtotal RNA. The relative levels of steady-state ACC1 mRNA weredetermined by normalization to ACT1 mRNA. For each genotype, theresults from two strains of opposite mating type and from twoseparate experiments were combined. The average ACC1 mRNA level± standard deviation (n = 4) is shown as a percentage of the wild-typevalue. The percentages were as follows: wild type, 100.0 ± 24.0;hpr1 $Delta$ mutant, 45.4 ± 3.8; acc1^cs mutant, 90.7 ± 18.5. No significant difference was found in thelevels of ACC1 message between the acc1^cs mutant and the wild type. In contrast, ACC1 expression was reducedtwofold in the hpr1 $Delta$ mutant compared to the wild type. These dataindicate that the reduced Acc1p activity in the hpr1 $Delta$ mutant ispartially due to a diminished level of steady-state ACC1 messagemade in the absence of Hpr1p and accounts for about half of thereduction in Acc1p activity. The fact that the biotinylated levelsof Acc1p in the hpr1 $Delta$ mutant are also only 50% of the wild-typelevel indicates that transport and stability of the ACC1 messageare not further reduced. Most likely, there is some posttranslationalprocess that is altered in the hpr1 $Delta$ mutant that further reducedthat Acc1pactivity.

Cells lacking Hpr1p have recently been shown to be defective in transcriptional elongation, but transcription initiation oractivation appears not to be affected (9). ACC1 is an unusuallylarge yeast gene of approximately 7 kb. We thus reasoned thatthe combination of a defect in transcriptional elongation anda mutation in a large gene might cause the synthetic lethalitybetween hpr1 $Delta$ and acc1. Conditional acc1 alleles were thereforetested for hypersensitivity towards the transcriptional elongationinhibitor 6-azauracil (5), to see if this would mimic the hpr1 $Delta$ acc1 synthetic lethality. Conditional acc1 mutants were foundto be as sensitive towards 6-azauracil as were wild-type cells(data not shown). Thus, the synthetic lethal interaction betweenhpr1 $Delta$ and acc1 was not due to the reduced transcriptional elongationin the hpr1 $Delta$ mutantbackground.

hpr1 $Delta$ and acc1^cs affect nuclear export of polyadenylated RNA. The temperature-sensitive allele of acc1, mtr7, has been isolated in a screen for mutants that affect mRNA transport (mtr[18]; for a review, see reference 39). This function of Acc1pin nuclear export of RNA is not yet fully understood, but it hasbeen suggested that acyl chain elongation and hence the synthesisof the C_26:0 very-long-chain fatty acid are required for a functionalnuclear membrane-nuclear pore complex (31, 33). We thus investigatedwhether the synthetic lethal interaction between hpr1 $Delta$ and theconditional acc1 alleles could be due to a defect of hpr1 $Delta$ innuclear export of polyadenylated RNA. In situ hybridization witha digoxigenin-labeled oligo(dT) probe revealed a very strong defectof hpr1 $Delta$ cells in exporting nuclear poly(A)⁺ RNA at the nonpermissive growth temperature of 37°C in approximately30% of all cells. A similar albeit much weaker (comparable tothat of acc1^ts) defect in mRNA export was also observed in acc1^cs cells (Fig. 5).

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FIG. 5. hpr1 $Delta$ and acc1^cs cells are defective in nuclear export of polyadenylated RNA. Nuclear accumulation of polyadenylated RNA in hpr1 $Delta$ and acc1^cs cells at the nonpermissive temperature is shown. Cells were grown to early logarithmic phase at 23°C and shifted to 37 and 17°C, respectively, for 4 h, and fixed and processed for in situ hybridization with a digoxigenin-labeled oligo(dT)_25-30 probe. Strong accumulation of nuclear poly(A)⁺ RNA was visible in hpr1 $Delta$ and acc1^cs cells shifted to nonpermissive temperatures (arrows in panels D and J) but not in cells grown at permissive temperatures (A and G). DAPI (4',6-diamidino-2-phenylindole) staining and differential interference contrast (DIC) pictures of the same visual field are shown to the right. Bar, 10 µm.

To characterize the transport defect in more detail, we analyzed pre-mRNA splicing and mRNA processing (transcription initiationand 3'-end formation) in hpr1 $Delta$ and acc1^cs mutant cells. Equal amounts of total RNA isolated from cellsincubated at permissive and nonpermissive temperatures were subjectedto Northern blot analysis with CRY1, which codes for a ribosomalprotein (21), as a probe (Fig. 6). As has previously been describedfor a number of temperature-sensitive mutants that block nuclearexport of polyadenylated RNA (e.g., mtr1, mtr3, mtr4, and mtr17[18]), the synthesis of oversized CRY1 transcripts was observedfor hpr1 $Delta$ cells. Oversized transcripts were not detected in anyof the other lanes shown in Fig. 6 even on overexposure of theblot (data not shown). Detection of aberrant transcripts confirmsthe previously proposed function of Hpr1p in some steps of transcription.Similar to acc1^ts (mtr7 [18]), acc1^cs did not affect CRY1 processing.

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FIG. 6. Northern analysis of CRY1 mRNA processing in wild-type, hpr1 $Delta$ , and acc1^cs cells. Ten micrograms of total RNA isolated from cells grown at the permissive temperature (23°C) or shifted for 4 h to a nonpermissive temperature (37 or 17°C) was analyzed by Northern hybridization with CRY1 as a probe. The position of mature CRY1 mRNA (540 bases) is shown. The position of CRY1 pre-mRNA (847 bases) is indicated by the arrow. Oversized transcripts detected in hpr1 $Delta$ cells are indicated by the arrowheads pointing to the right. wt, wild type.

To determine whether the observed block in mRNA export also affects processing of rRNA, mutant strains were incubated at eitherpermissive or nonpermissive temperatures and then pulse-labeledwith [³H]uridine for 10 min at the same temperature. The efficiency oflabeling in hpr1 $Delta$ was greatly reduced at 37°C (2.6%) comparedto 23°C, suggesting that in the hpr1 $Delta$ mutant either the synthesisof RNA, [³H]uridine uptake, or [³H]UTP synthesis is decreased at nonpermissive temperatures. Tonormalize this effect, the labeled RNA samples analyzed on agarosegels each were loaded with equal amounts of radioactivity. Asshown in Fig. 7, rRNA processing appeared to be disturbed in thehpr1 $Delta$ , but not the acc1^cs, mutant. The labeling of all rRNA species was greatly reducedin the hpr1 $Delta$ mutant.

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FIG. 7. rRNA processing in wild-type, hpr1 $Delta$ , and acc1^cs strains. Strains were preincubated for 1 h at permissive or nonpermissive temperatures and pulse-labeled for 10 min with [³H]uridine. RNA was isolated, and equal amounts of incorporated radioactivity were loaded on a denaturing agarose gel. The positions of 35, 32, 27, 25, 20, and 18S rRNA are shown by arrowheads. wt, wild type.

hpr1 $Delta$ and acc1^cs cells display an aberrant ring-shaped nucleolus. The yeast nucleolus is a crescent-shaped structure that makes extensive contact with the nuclear envelope. A defect in nuclearexport of polyadenylated RNA is frequently accompanied by an alteredstructure of the nucleolus, i.e., fragmentation and/or enlargement(18, 32). We thus analyzed the structure of the nucleolusin hpr1 $Delta$ and acc1^cs mutant cells by immunofluorescence microscopy with an antibodyagainst an abundant nucleolar protein, Nop1p (6). As shownin Fig. 8, at permissive temperatures the nucleolus in hpr1 $Delta$ andacc1^cs cells displayed a ring-shaped structure rather than the typicalcrescent-shaped structure seen in wild-type cells. This ring-likestructure collapses into a normal-looking, crescent-shaped nucleolusupon shifting of hpr1 $Delta$ and acc1^cs cells to nonpermissive temperatures (data not shown).

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FIG. 8. Ring-shaped structure of the nucleolus in hpr1 $Delta$ and acc1^cs cells. Shown is immunofluorescence localization of the nucleolar antigen Nop1p in hpr1 $Delta$ , acc1^cs, and wild-type cells. Strains were cultivated in YEPD to early logarithmic growth phase and fixed and processed for immunofluorescence detection of Nop1p as described in Materials and Methods (A, D, and G). Arrows in panels A and D point to ring-shaped nucleoli. DAPI (4',6-diamidino-2-phenylindole) staining (B, E, and H) and differential interference contrast (DIC) pictures (C, F, and I) of the same visual field are shown to the right. Bar, 10 µm. wt, wild type.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have described a synthetic lethal interaction between a loss-of-function allele of HPR1 and two conditional alleles ofACC1, encoding yeast acetyl-CoA carboxylase. Acc1p is an essentialcytoplasmic enzyme that catalyzes the rate-limiting step of denovo synthesis of fatty acids. In the hpr1 $Delta$ mutant background,Acc1p activity was reduced approximately 15-fold. This reducedactivity did not result in gross alterations of the lipid or fattyacid composition of the hpr1 $Delta$ mutant but rendered the mutant hypersensitiveto soraphen A, an inhibitor of Acc1p activity. Analysis of steady-statelevels of biotinylated Acc1p and ACC1 mRNA revealed that levelsof biotinylated Acc1p and ACC1 transcripts were reduced twofoldin the absence of Hpr1p, indicating that the lack of Hpr1p affectedcellular Acc1p activity already at the level oftranscription.

Several lines of evidence suggested that the synthetic lethal interaction of hpr1 $Delta$ with conditional acc1 alleles was not simplydue to the combination of a twofold reduction of ACC1 transcriptionwith an enzymatically challenged mutant Acc1p allele. First, likeother genes encoding lipid biosynthetic enzymes, ACC1 transcriptionis under the regulatory control of the transcriptional activatorsIno2p and Ino4p. In the absence of Ino2p or Ino4p, ACC1 transcriptionis reduced two- to threefold (15). acc1^cs ino2 or acc1^cs ino4 double mutants, grown in the presence of 11 µM inositolto rescue the inositol auxotrophy, however, did not show any reducedgrowth compared to the acc1^cs mutant alone (data not shown). Moreover, the hpr1 $Delta$ mutation didnot result in an inositol auxotrophic phenotype or a reductionin INO1 mRNA levels (10), indicating that HPR1 does not functionlike Ino2p and Ino4p in coordinate regulation by inositol (26).Second, ACC1 transcription was reduced twofold in a top1 $Delta$ mutantbackground (data not shown). Unlike hpr1 $Delta$ , however, top1 $Delta$ wasnot synthetically lethal with acc1^cs or acc1^ts. As is the case for the ino2 and ino4 mutants, a twofold reductionof acc1^cs levels in a top1 $Delta$ mutant is thus not sufficient to cause syntheticlethality. These data argue that the interaction between hpr1 $Delta$ and conditional acc1 alleles is characteristic for the way thathpr1 $Delta$ affects ACC1 expression and that the synthetic lethalityis not solely due to a twofold reduction of ACC1 transcriptionin the hpr1 $Delta$ mutantbackground.

The phenotypes that have been studied for hpr1 $Delta$ strains are all related to nuclear events: hyperrecombination of direct repeatsin chromosomal DNA (3), synthetic lethality with a mutant alleleof DNA topoisomerase genes (3), or a mutation in one of thehistone genes (10). The temperature-sensitive growth of hpr1 $Delta$ is suppressed by mutations in SOH genes that play a role in transcription(10). Some of the soh mutants suppress the soraphen A sensitivityof hpr1 $Delta$ and the synthetic phenotype of the acc1^cs hpr1 $Delta$ double mutant (11). The presence of a nuclear localizationsequence in Hpr1p suggests that this protein is most likely nuclear,and recent studies using a FLAG-tagged Hpr1p have confirmed thislocalization (11). Whether Hpr1p is confined to the chromatin-richnucleoplasm or to the nucleolus is currently beinginvestigated.

We now report that hpr1 $Delta$ cells are conditionally defective in nuclear export of polyadenylated RNA, synthesize oversized CRY1transcripts, are impaired in rRNA processing, and display an aberrantstructure of the nucleolus. These are phenotypic changes thatpreviously have been analyzed to characterize a set of conditionalmutants that block mRNA transport (mtr [18]). A defect in nuclearexport of polyadenylated RNA has previously also been observedin a temperature-sensitive acc1^ts (mtr7) mutant (31), and we now report that a second, cold-sensitiveacc1^cs mutant also has an Mtr phenotype. We thus propose that the basisfor the synthetic phenotype between hpr1 $Delta$ and conditional acc1alleles lies in their common defect in mRNA export and that thecombination of mutations that affect nuclear mRNA export is lethal.This would explain the absence of a synthetic phenotype in theacc1^cs top1 $Delta$ and acc1^cs ino2/4 double mutants. The synthetic phenotype would indicateeither that each mutant slightly decreases mRNA export and thatthe additive effect of the two mutations is lethal or that eachmutant blocks transport through a different pathway (for a review,see reference 39). Whether Hpr1p acts directly or indirectlyto affect transport is not known, but it is likely that Hpr1paffects expression of a gene(s) that is involved in transportand that Acc1p affects nuclear membrane synthesis and hence nuclearpore complex function. M. Chang et al. have suggested that theRNA polymerase II complex in which Hpr1p is found is involvedin the expression of cell wall genes (7). The cell wall defectsof mutants encoding components of the RNA polymerase II complexmay be analogous to the nuclear transport phenotype that we seein hpr1 $Delta$ mutants, which may be caused by a reduced expressionof nuclear transportfactors.

Interestingly, hpr1 $Delta$ and acc1^cs mutant cells display an aberrant circle-shaped nucleolus. The nucleolus is the site of ribosomalDNA (rDNA) transcription by RNA polymerase I, processing of rDNAtranscripts, and assembly of ribosomes (for reviews, see references24, 30, and 34). In wild-type yeast cells, the nucleolusis a crescent-shaped region of the nucleus that stands in closecontact with the nuclear envelope (16). A rounded nucleolarstructure that often lacked extensive contact with the nuclearenvelope has recently been observed for strains that express polymeraseII-transcribed 35S rRNA (25). Furthermore, many of the previouslycharacterized mRNA transport mutants display a fragmented or enlargednucleolus (18), an observation that led us to propose an involvementof the nucleolus or nucleolar proteins in the mRNA export pathway(32). More recently, a correlation between structural alterationsof the nucleolus and aging of yeast cells has also been observed(19). In this case, nucleolar changes appear to be due to theaccumulation of extrachromosomal rDNA circles in old cells (37,38). The significance of the observed morphological alterationsof the nucleolus in hpr1 $Delta$ and acc1^cs mutant cells is not clear at present. Hpr1p affects nuclear eventsthat may be connected to rDNA transcription and/or recombination,but the hpr1 $Delta$ mutant has not been found to have any altered rateof rDNA recombination (3). Acc1p, on the other hand, affectsthe lipid composition of all cellular membranes, including thenuclear envelope that contacts the nucleolus. How this contactbetween nucleolar structures and the nuclear envelope is maintainedis not known. The two proteins thus clearly have distinct functions,and there is no obvious overlap between them. Nevertheless, bothmutants affect nuclear export of polyadenylated RNA and displayan altered nucleolar morphology. We propose that the two mutationsaffect two different, but overlapping, functions required forefficient nucleocytoplasmic transport: the lipid composition ofthe nuclear envelope in the case of the acc1^cs mutation and transcription-packaging of nascent transcripts intoa transport-competent state in the case of the hpr1 $Delta$ mutation.Reducing the efficiency of both processes at the same time islethal.

	ACKNOWLEDGMENTS

We thank S. A. Henry and R. Rothstein for strains, A. Hinnen for the gift of soraphen A, J. P. Aris for the anti-Nop1p antibody,and A. Leber for critically reading themanuscript.

This work was supported by the Swiss National Science Foundation (823A-046702 to R.S.), the Fonds zur Förderung der wissenschaftlichenForschung in Österreich (project 11731 to S.D.K.), and the NationalInstitutes of Health (grant GM30439 to H.L.K.).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry, New York University Medical Center, 550 First Ave., NewYork, NY 10016. Phone: (212) 263-5778. Fax: (212) 263-8166. E-mail:kleinh01{at}mcrcr.med.nyu.edu.

Present address: Department of Microbiology and Molecular Genetics, UMDNJ-New Jersey Medical School, Newark, NJ07103.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Aguilera, A., and H. L. Klein. 1989. Genetic and molecular analysis of recombination events in Saccharomyces cerevisiae occurring in the presence of the hyper-recombination mutation hpr1. Genetics 122:503-517[Abstract/Free Full Text].
2.	Aguilera, A., and H. L. Klein. 1988. Genetic control of intrachromosomal recombination in Saccharomyces cerevisiae. I. Isolation and genetic characterization of hyper-recombination mutations. Genetics 119:779-790[Abstract/Free Full Text].
3.	Aguilera, A., and H. L. Klein. 1990. HPR1, a novel yeast gene that prevents intrachromosomal excision recombination, shows carboxy-terminal homology to the Saccharomyces cerevisiae TOP1 gene. Mol. Cell. Biol. 10:1439-1451[Abstract/Free Full Text].
4.	Al-Feel, W., S. S. Chirala, and S. J. Wakil. 1992. Cloning of the yeast FAS3 gene and primary structure of yeast acetyl-CoA carboxylase. Proc. Natl. Acad. Sci. USA 89:4534-4538[Abstract/Free Full Text].
5.	Archambault, J., F. Lacroute, A. Ruet, and J. D. Friesen. 1992. Genetic interaction between transcription elongation factor TFIIS and RNA polymerase II. Mol. Cell. Biol. 12:4142-4152[Abstract/Free Full Text].
6.	Aris, J. P., and G. Blobel. 1988. Identification and characterization of a yeast nucleolar protein that is similar to a rat liver nucleolar protein. J. Cell Biol. 107:17-31[Abstract/Free Full Text].
7.	Chang, M., D. French-Cornay, H. Fan, H. Klein, C. L. Denis, and J. A. Jaehning. 1999. A complex containing RNA polymerase II, Paf1p, Cdc73p, Hpr1p, and Ccr4p plays a role in protein kinase C signaling. Mol. Cell. Biol. 19:1056-1067[Abstract/Free Full Text].
8.	Chang, M., and J. A. Jaehning. 1997. A multiplicity of mediators: alternative forms of transcription complexes communicate with transcriptional regulators. Nucleic Acids Res. 25:4861-4865[Abstract/Free Full Text].
9.	Chavez, S., and A. Aguilera. 1997. The yeast HPR1 gene has a functional role in transcriptional elongation that uncovers a novel source of genome instability. Genes Dev. 11:3459-3470[Abstract/Free Full Text].
10.	Fan, H., and H. L. Klein. 1994. Characterization of mutations that suppress the temperature sensitive growth of the hpr1 $Delta$ mutant of Saccharomyces cerevisiae. Genetics 137:945-956[Abstract].
11.	Fan, H.-Y., and H. L. Klein. Unpublished observation.
12.	Fan, H. Y., K. K. Cheng, and H. L. Klein. 1996. Mutations in the RNA polymerase II transcription machinery suppress the hyperrecombination mutant hpr1 delta of Saccharomyces cerevisiae. Genetics 142:749-759[Abstract].
13.	Feinberg, A. P., and B. Vogelstein. 1984. A technique for radiolabeling DNA restriction endonuclease fragments to high specific activity. Anal. Biochem. 137:266-267[Medline].
14.	Guerra, C. E., and H. L. Klein. 1995. Mapping of the ACC1/FAS3 gene to the right arm of chromosome XIV of Saccharomyces cerevisiae. Yeast 11:697-700[Medline].
15.	Hasslacher, M., A. S. Ivessa, F. Paltauf, and S. D. Kohlwein. 1993. Acetyl-CoA carboxylase from yeast is an essential enzyme and is regulated by factors that control phospholipid metabolism. J. Biol. Chem. 268:10946-10952[Abstract/Free Full Text].
16.	Hurt, E. C., A. Mutvei, and M. Carmo-Fonseca. 1992. The nuclear envelope of the yeast Saccharomyces cerevisiae. Int. Rev. Cytol. 136:145-184[Medline].
17.	Ivessa, A. S., R. Schneiter, and S. D. Kohlwein. 1997. Yeast acetyl-CoA carboxylase is associated with the cytoplasmic surface of the endoplasmic reticulum. Eur. J. Cell Biol. 74:399-406[Medline].
18.	Kadowaki, T., S. Chen, M. Hitomi, E. Jacobs, C. Kumagai, S. Liang, R. Schneiter, D. Singleton, J. Wisniewska, and A. M. Tartakoff. 1994. Isolation and characterization of Saccharomyces cerevisiae mRNA transport-defective (mtr) mutants. J. Cell Biol. 126:649-659[Abstract/Free Full Text].
19.	Kennedy, B. K., M. Gotta, D. A. Sinclair, K. Mills, D. S. McNabb, M. Murthy, S. M. Pak, T. Laroche, S. M. Gasser, and L. Guarente. 1997. Redistribution of silencing proteins from telomeres to the nucleolus is associated with extension of life span in S. cerevisiae. Cell 89:381-391[Medline].
20.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[Medline].
21.	Larkin, J. C., J. R. Thompson, and J. L. Woolford, Jr. 1987. Structure and expression of the Saccharomyces cerevisiae CRY1 gene: a highly conserved ribosomal protein gene. Mol. Cell. Biol. 7:1764-1775[Abstract/Free Full Text].
22.	Lowry, O. H., N. J. Rosebrough, A. L. Farr, and R. J. Randall. 1951. Protein measurement with the Folin phenol reagent. J. Biol. Chem. 193:265-275[Free Full Text].
23.	Matsuhashi, M. 1969. Acetyl-CoA carboxylase from yeast. Methods Enzymol. 14:3-8.
24.	Melese, T., and Z. Xue. 1995. The nucleolus: an organelle formed by the act of building a ribosome. Curr. Opin. Cell Biol. 7:319-324[Medline].
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The Saccharomyces cerevisiae Hyperrecombination Mutant hpr1 Is Synthetically Lethal with Two Conditional Alleles of the Acetyl Coenzyme A Carboxylase Gene and Causes a Defect in Nuclear Export of Polyadenylated RNA

The Saccharomyces cerevisiae Hyperrecombination Mutant hpr1 $Delta$ Is Synthetically Lethal with Two Conditional Alleles of the Acetyl Coenzyme A Carboxylase Gene and Causes a Defect in Nuclear Export of Polyadenylated RNA