Saccharomyces cerevisiae SSD1-V Confers Longevity by a Sir2p-Independent Mechanism

doi:10.1534/genetics.166.4.1661

Saccharomyces cerevisiae SSD1-V Confers Longevity by a Sir2p-Independent Mechanism

Matt Kaeberlein^a, Alex A. Andalis^b, Gregory B. Liszt^c, Gerald R. Fink^b, and Leonard Guarente^c
^a Department of Genome Sciences, University of Washington, Seattle, Washington 98195,
^b Whitehead Institute for Biomedical Research, Massachusetts Institute of Technology, Cambridge, Massachusetts 02142
^c Department of Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139

Corresponding author: Matt Kaeberlein, Health Sciences Bldg., K-222, Seattle, Washington 98195-7730., kaeber{at}u.washington.edu (E-mail)

Communicating editor: B. J. ANDREWS

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The SSD1 gene of Saccharomyces cerevisiae is a polymorphic locusthat affects diverse cellular processes including cell integrity,cell cycle progression, and growth at high temperature. We showhere that the SSD1-V allele is necessary for cells to achieveextremely long life span. Furthermore, addition of SSD1-V tocells can increase longevity independently of SIR2, althoughSIR2 is necessary for SSD1-V cells to attain maximal life span.Past studies of yeast aging have been performed in short-livedssd1-d strain backgrounds. We propose that SSD1-V defines apreviously undescribed pathway affecting cellular longevityand suggest that future studies on longevity-promoting genesshould be carried out in long-lived SSD1-V strains.

AGING in Saccharomyces cerevisiae can be studied by mutationsthat extend the replicative life span of mother cells, definedas the number of daughters produced by a given mother cell priorto senescence. One cause of aging in yeast is the accumulationof extrachromosomal ribosomal DNA circles (ERCs), circular DNAmolecules derived from homologous recombination within the ribosomalDNA (rDNA; SINCLAIR and GUARENTE 1997 ). ERCs are self-replicatingand asymmetrically segregated to the mother-cell nucleus duringS-phase, resulting in an exponential increase in ERC copy numberwith age and, ultimately, in cell death (SINCLAIR and GUARENTE1997 ).

One important determinant of yeast longevity is the Sir2 protein(KAEBERLEIN et al. 1999 ). Sir2p is an NAD-dependent histonedeacetylase (IMAI et al. 2000 ; LANDRY et al. 2000 ; SMITHet al. 2000 ) required for transcriptional silencing at telomeres(GOTTSCHLING et al. 1990 ), silent mating (HM) loci (IVY etal. 1986 ; RINE and HERSKOWITZ 1987 ), and the rDNA (BRYK etal. 1997 ; SMITH and BOEKE 1997 ). Mutation of SIR2 resultsin increased rDNA recombination (GOTTLIEB and ESPOSITO 1989), increased ERC formation (KAEBERLEIN et al. 1999 ), and decreasedlife span (KENNEDY et al. 1995 ), whereas overexpression extendslife span by 30–40% (KAEBERLEIN et al. 1999 ). Sir2p isalso required for life-span extension by calorie restriction(CR), demonstrating the importance of this protein as a centralregulator of longevity (LIN et al. 2000 ). Overexpression ofa Sir2p homolog, Sir-2.1, has been shown to extend life spanin the nematode Caenorhabditis elegans, suggesting that Sir2proteins regulate aging in higher eukaryotes as well (TISSENBAUMand GUARENTE 2001 ).

SSD1 is a polymorphic locus that affects diverse cellular processes.Two allele classes, designated SSD1-V and ssd1-d, have beenidentified for SSD1. SSD1-V alleles confer viability in theabsence of the Sit4 protein phosphatase and code for functionalSsd1 protein. In contrast, strains carrying ssd1-d alleles areinviable in the absence of Sit4p (SUTTON et al. 1991 ), andd-type alleles are likely null for Ssd1p function. Both V- andd-type alleles have been found in natural isolates and in laboratorystrains of S. cerevisiae. A recent report (WHEELER et al. 2003) suggests that the SSD1 allele type affects pathogenicity ofyeasts, indicating that allelic variation at the SSD1 locusmay be important for survival under various environmental conditions.

A potential role for SSD1-V as a regulator of cell life spanwas suggested by the observation that SSD1-V suppresses manyphenotypes associated with mutation of the MPT5/UTH4 gene (KAEBERLEINand GUARENTE 2002 ). MPT5 is a post-transcriptional regulator(TADAUCHI et al. 2001 ) involved in regulating the pheromoneresponse (CHEN and KURJAN 1997 ), cell-wall stability (KAEBERLEINand GUARENTE 2002 ), telomere silencing (COCKELL et al. 1998), and longevity (KENNEDY et al. 1995 ). Like SIR2, MPT5 isa limiting factor for longevity: overexpression of MPT5 extendslife span, whereas the deletion of MPT5 has the opposite effect(KENNEDY et al. 1997 ).

SSD1-V suppresses the temperature-sensitive growth defect causedby mutation of MPT5 as well as the sensitivity to calcofluorwhite (CFW) and sodium dodecyl sulfate (SDS; KAEBERLEIN andGUARENTE 2002 ). In strains lacking SSD1-V, deletion of MPT5is synthetically lethal in combination with loss of functionin either of the SBF or CCR4 transcriptional complexes (KAEBERLEINand GUARENTE 2002), both of which function downstream of proteinkinase C (Pkc1p) to promote cell-wall biosynthesis (IGUAL etal. 1996 ; MADDEN et al. 1997 ; CHANG et al. 1999 ). Theseresults were interpreted to suggest that Mpt5p, Ssd1p, and Pkc1pdefine three parallel pathways that function to ensure cellintegrity (KAEBERLEIN and GUARENTE 2002 ).

In addition to suppressing the cell integrity defects, SSD1-Vsuppresses the shortened life span caused by deletion of MPT5(KAEBERLEIN and GUARENTE 2002 ). These observations raise thepossibility that SSD1-V might also promote longevity in wild-typecells. Here we show that addition of a single copy of SSD1-Vto ssd1-d wild-type cells extends life span in at least twodifferent strain backgrounds. Furthermore, life-span extensionby SSD1-V does not require the Sir2 protein, although the presenceof both SSD1-V and SIR2 is necessary for maximal longevity.

MATERIALS AND METHODS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Strains and genetic techniques:
The strains used in this study are listed in Table 1. All strainswere derived from W303R (described in MILLS et al. 1999 ),PSY316 (described in PARK et al. 1999 ), or BKY5 (describedin KENNEDY et al. 1995 ). Genetic crosses, sporulation, andtetrad analysis were carried out as described (SHERMAN and HICKS1991 ). The genotype of inviable spore clones was inferred,when possible, on the basis of marker segregation in viablespore clones from the same tetrad. Unless otherwise noted, cellswere cultured in YPD or synthetic media prepared using conventionalmethods (GUTHRIE and FINK 1991 ). Yeast transformation was accomplishedby the lithium acetate method (GIETZ et al. 1992 ). All othergene deletions were generated by transforming cells with PCR-amplifieddisruption cassettes as described (KAEBERLEIN et al. 1999 ).In each case, the entire open reading frame was removed. Alldisruptions were verified phenotypically or by PCR. The SSD1-Vintegrating plasmids p406SSD1 and p405SSD1 were previously described(KAEBERLEIN and GUARENTE 2002 ). Unless otherwise indicated,all SSD1-V strains contain SSD1-V integrated at the marker locusand still carry the ssd1-d allele at the SSD1 locus. Deletionof ssd1-d does not affect any of the phenotypes tested, includinglife span, growth at 30°, 37°, or 40°, or sensitivityto calcofluor white.

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Table 1. Yeast strains used in this study

Determination of SSD1 allele:
To determine which SSD1 allele was present in PSY316, one copyof the SIT4 gene was deleted in diploid cells. Sporulation ofthese cells revealed that deletion of SIT4 always resulted inlethality in haploid spore clones (n > 20 sit4 ${Delta}$ spores). Thislethality was suppressed by integration of a single copy ofSSD1-V at the URA3 locus. Therefore, we conclude that in PSY316the SSD1 allele type is ssd1-d.

Life span, recombination, and ERC analysis:
Life spans were performed as described (KAEBERLEIN and GUARENTE2002 ). Statistical significance was determined by a Wilcoxonrank-sum test. Average life span is different for P < 0.05. Fig 1 Fig 2 Fig 3 Fig 4 Fig 5 represent data derived from asingle experiment, unless otherwise stated. ERC levels weredetermined as described (DEFOSSEZ et al. 1999 ; KAEBERLEINet al. 1999 ). ERCs were separated on a 0.6% agarose gel withoutaddition of ethidium bromide at 1 V/cm for 48 hr. rDNA recombinationrate was determined as described (KAEBERLEIN et al. 1999 ).

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Figure 1. SSD1-V extends life span and improves cell integrity. (A) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 SSD1-V ( ${blacksquare}$ ), PSY316 ssd1 ${Delta}$ ::HIS3 (X), and PSY316 ssd1 ${Delta}$ ::HIS3 SSD1-V ( ${blacktriangleup}$ ). Mean life spans and number of cells analyzed were PSY316 22.2 (n = 40), PSY316 SSD1-V 36.2 (n = 40), PSY316 ssd1 ${Delta}$ ::HIS3 21.9 (n = 40), and PSY316 ssd1 ${Delta}$ ::HIS3 SSD1-V 38.0 (n = 40). (B) Life spans were determined for BKY5 ( ${diamondsuit}$ ) and BKY5 SSD1-V ( ${blacktriangleup}$ ). Mean life spans and number of cells analyzed were BKY5 13.0 (n = 40) and BKY5 SSD1-V 24.3 (n = 40). (C) PSY316 cells are unable to grow at temperatures >39° unless SSD1-V is present. Tenfold serial dilutions of a log-phase culture plated onto YPD and incubated at either 30° or 40° for 48 hr are shown.

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Figure 2. SSD1-V and Sir2p act in different pathways to promote longevity. (A) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 sir2 ( ${blacksquare}$ ), and PSY316 sir2 SSD1-V ( ${blacktriangleup}$ ). Mean life spans and number of cells analyzed were PSY316 21.2 (n = 40), PSY316 sir2 10.8 (n = 39), and PSY316 sir2 SSD1-V 15.7 (n = 40). (B) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 sir2 fob1 ( ${blacksquare}$ ), PSY316 0.5% glucose ( ${blacktriangleup}$ ), and PSY316 sir2 fob1 0.5% glucose (X). Mean life spans and number of cells analyzed were PSY316 22.8 (n = 40), PSY316 sir2 fob1 21.2 (n = 39), PSY316 0.5% glucose 27.0 (n = 40), and PSY316 sir2 fob1 0.5% glucose 21.4 (n = 40). (C) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 sir2 fob1 ( ${blacksquare}$ ), PSY316 SSD1-V ( ${blacktriangleup}$ ), and PSY316 sir2 fob1 SSD1-V (X). Mean life spans and number of cells analyzed were PSY316 22.8 (n = 40), PSY316 sir2 fob1 21.2 (n = 39), PSY316 SSD1-V 37.3 (n = 40), and PSY316 sir2 fob1 SSD1-V 30.0 (n = 40). (D) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 SSD1-V ( ${blacksquare}$ ), PSY316 cyt1 ( ${blacktriangleup}$ ), and PSY316 SSD1-V cyt1 (X). Mean life spans and number of cells analyzed were PSY316 21.7 (n = 40), PSY316 SSD1-V 39.3 (n = 40), PSY316 cyt1 22.2 (n = 40), and PSY316 SSD1-V cyt1 37.9 (n = 40). (E) Life spans were determined for PSY316 YPD ( ${diamondsuit}$ ), PSY316 SSD1-V YPD ( ${blacksquare}$ ), PSY316 YPDS ( ${blacktriangleup}$ ), and PSY316 SSD1-V YPDS (X). Mean life spans and number of cells analyzed were PSY316 YPD 19.1 (n = 40), PSY316 SSD1-V YPD 34.8 (n = 40), PSY316 YPDS 30.4 (n = 40), and PSY316 SSD1-V YPDS 39.1 (n = 40).

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Figure 3. SSD1-V does not extend life span by decreasing ERC levels. (A) SSD1-V has no detectable effect on rDNA recombination. rDNA recombination was measured by the frequency at which an ADE2 marker integrated into the rDNA is lost. A total of 33,000 colonies from three independently derived isolates were examined for each strain. (B) DNA from unsorted cells was isolated and electrophoresed as described (KAEBERLEIN et al. 1999

). The gel was transferred and probed with sequence homologous to the rDNA. ERCs are denoted by arrows. The dark band present in both lanes corresponds to genomic rDNA. In this isolate, the long-lived SSD1-V cells have a greater steady-state amount of ERCs than do ssd1-d cells, as quantitated by the ratio of ERC DNA to genomic rDNA. However, in one other independently derived SSD1-V transformant we were unable to detect a significant difference in ERC levels relative to those in wild-type cells. In no case did we detect fewer ERCs in SSD1-V cells.

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Figure 4. Effect of NCA3 on cell life span. (A) Life spans were determined for PSY316 ( ${diamondsuit}$ ) and PSY316 pADH_NCA3 ( ${blacksquare}$ ). Mean life spans and number of cells analyzed were PSY316 23.4 (n = 80) and PSY316 pADH_NCA3 27.6 (n = 120). Data were pooled from two different experiments. (B) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 nca3 ( ${blacksquare}$ ), PSY316 SSD1-V ( ${blacktriangleup}$ ), and PSY316 nca3 SSD1-V (X). Mean life spans and number of cells analyzed were PSY316 23.3 (n = 40), PSY316 nca3 22.3 (n = 40), PSY316 SSD1-V 37.5 (n = 40), and PSY316 nca3 SSD1-V 32.8 (n = 40).

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Figure 5. MPT5 and SIR2 determine longevity in a pathway parallel to SSD1-V. (A) Life spans were determined for PSY316 ( ${diamondsuit}$ ), PSY316 SSD1-V ( ${blacksquare}$ ), PSY316 mpt5 ( ${blacktriangleup}$ ), and PSY316 mpt5 SSD1-V (X). Mean life spans and number of cells analyzed were PSY316 24.3 (n = 40), PSY316 SSD1-V 35.5 (n = 40), PSY316 mpt5 15.3 (n = 40), and PSY316 mpt5 SSD1-V 22.9 (n = 40). (B) Life spans were determined for W303R ( ${diamondsuit}$ ), W303R pADH_MPT5 ( ${blacksquare}$ ), W303R sir2 ( ${blacktriangleup}$ ), W303R sir2 pADH_MPT5 (X), W303R SIR2/URA3 (*), and W303R SIR2/URA3 pADH_MPT5 (•). This experiment was performed in the W303R strain background because overexpression of MPT5 from the pADH_MPT5 plasmid causes slow growth and decreased viability in strain PSY316. Mean life spans and number of cells analyzed were W303R 20.9 (n = 41), W303R pADH_MPT5 25.8 (n = 70), W303R sir2 11.2 (n = 41), W303R sir2 pADH_MPT5 10.1 (n = 70), W303R SIR2/URA3 27.4 (n = 40), and W303R SIR2/URA3 pADH_MPT5 25.8 (n = 40).

Microarray analysis:
RNA isolation and microarray analysis were performed essentiallyas described (LIN et al. 2002 ). For the purposes of comparativestatistical analyses, candidate genes with altered transcriptlevels in SSD1-V cells relative to wild type were defined assuch if the average ratio of SSD1-V (Cy5) to ssd1-d (Cy3) was>1.5 or <0.667 (1.5-fold decrease) in three independent experiments.All such genes are listed in supplemental Table 1 at http://www.genetics.org/supplemental/).As a control, two independent microarray analyses were performedon ssd1 ${Delta}$ (Cy5) cells relative to ssd1-d (Cy3) cells. The 124genes defined as regulated by CR represent the subset of genesfound to show significant changes in mRNA expression both incells lacking HXK2 and in cells grown on 0.5% glucose (LIN etal. 2002 ). Statistical significance of the overlap betweenregulated genes in different experiments shown in Table 2 wascalculated using a hypergeometric distribution. P values wereobtained from the online hypergeometric distribution calculatorat http://www.alewand.de/stattab/tabdiske.htm. Gene functionannotation was obtained from the Saccharomyces Genome Database.Supplemental Table 1, normalized ratio (Cy5/Cy3), and spotintensity data sets for all experiments presented in this articleare available at http://web.mit.edu/biology/guarente/arrays/kaeberlein.

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Table 2. Overlap in gene expression profiles with CR

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

SSD1-V extends life span and improves growth at high temperature:
Mpt5p is a limiting factor for longevity and functions in apathway parallel to SSD1-V for cell integrity (KAEBERLEIN andGUARENTE 2002 ). On the basis of this genetic interaction, wehypothesized that SSD1-V might also regulate longevity. We firstdetermined that our wild-type strain PSY316 carries the ssd1-dallele at the SSD1 locus, on the basis of the inviability causedby deletion of SIT4 in this background (see MATERIALS AND METHODS).A single copy of SSD1-V integrated at the URA3 locus resultsin an $~$ 50% increase in mean life span (Fig 1A). Integration ofSSD1-V at the SSD1 locus has a similar effect on life span (notshown). Deletion of the chromosomal ssd1-d allele of PSY316has no effect on life span and does not affect life-span extensionby SSD1-V (Fig 1A). Therefore, ssd1-d is a null allele withrespect to life span. All subsequent experiments were carriedout in the parental ssd1-d background.

PSY316 is a moderately long-lived yeast strain; however, manyyeast aging studies have been carried out in short-lived strainbackgrounds having mean life spans of 10–15 generations.To determine whether the life-span extension by SSD1-V was strainspecific, we integrated SSD1-V into the short-lived strain BKY5.We verified that BKY5 carries an ssd1-d allele (see MATERIALSAND METHODS) as well as a previously identified C-terminal truncatedallele of MPT5 (KENNEDY et al. 1997 ). Addition of SSD1-V toBKY5 results in an 85% increase in mean life span (Fig 1B).Thus, SSD1-V promotes long life span in at least two differentssd1-d strain backgrounds.

We had previously observed that cells from strain PSY316 grownormally at 37°, but are incapable of sustained growth at40°. Cells grown at 40° generally arrest as large-buddedcells with a significant fraction undergoing lysis (data notshown), consistent with a loss of cell-wall integrity at therestrictive temperature. Addition of SSD1-V fully suppressesthese phenotypes and allows growth of PSY316 at 40° (Fig 1C).Addition of SSD1-V to PSY316 also improves growth in thepresence of the cell-wall-perturbing agents CFW and SDS (datanot shown), as previously reported for strain W303R (KAEBERLEINand GUARENTE 2002 ).

SSD1-V extends life span in the absence of SIR2:
The Sir2 protein is a central regulator of yeast longevity,necessary for life-span extension in response to environmentalsignals such as reduced nutrient availability (LIN et al. 2000) and osmotic stress (KAEBERLEIN et al. 2002 ). To place SSD1-Vinto a genetic pathway relative to Sir2p, we integrated theSSD1-V allele into a strain lacking SIR2. Deletion of SIR2 shortenswild-type life span by $~$ 50% (KAEBERLEIN et al. 1999 ). Surprisingly,addition of SSD1-V resulted in a significant life-span extensionin the absence of Sir2p (Fig 2A), although sir2 SSD1-V cellsare shorter lived than SIR2 wild-type cells.

Due to the extremely short life span caused by lack of Sir2p,we also wished to determine the effect of SSD1-V on sir2 fob1double-mutant cells, which have an almost wild-type life span(KAEBERLEIN et al. 1999 ). As predicted by our previously proposedmodel (LIN et al. 2000 , LIN et al. 2002 ), CR by growth onlow glucose fails to extend life span in the absence of SIR2(Fig 2B). In contrast, sir2 fob1 SSD1-V cells grown on 2% glucosehave a life span that is significantly longer than that of sir2fob1 ssd1-d cells (Fig 2C). However, as was the case for sir2SSD1-V cells, sir2 fob1 SSD1-V cells do not live as long asSIR2 FOB1 SSD1-V cells. Therefore, SSD1-V acts in a novel, SIR2-independentpathway for longevity, although Sir2p is required for maximumlongevity in SSD1-V cells.

The Sir2-dependent life-span extension caused by CR is the resultof a metabolic shift from fermentation to respiration (LIN etal. 2002 ). It is possible that a portion of the longevity conferredby SSD1-V is achieved by causing the cell to undergo a similarmetabolic shift. To address this possibility, the effect ofSSD1-V on life span was examined in a respiration-deficientstrain lacking the CYT1 gene encoding cytochrome c1. Mutationof CYT1 prevents life-span extension by CR or by overexpressionof the Hap4p transcription factor (LIN et al. 2002 ). In contrast,SSD1-V extends the life span of cells lacking CYT1 to the sameextent as that of wild-type cells (Fig 2D), suggesting thatthe mechanism of life-span extension by SSD1-V is independentof mitochondrial function and respiration.

High osmolarity extends the life span of ssd1-d but not of SSD1-V cells:
We have previously demonstrated that the osmotic concentrationof media is a determining factor for mother-cell life span.Addition of 1 M sorbitol suppresses the short life span andcell-wall defects of mpt5 ssd1-d cells in the W303 strain background(KAEBERLEIN and GUARENTE 2002 ). Growth on YPD supplementedwith 1 M sorbitol (YPDS), 1 M xylitol, or 1 M glucose also extendsthe life span of MPT5 ssd1-d cells in PSY316 through a SIR2-dependentmechanism (KAEBERLEIN et al. 2002 ). We were therefore interestedin determining whether high osmolarity would affect the lifespan of long-lived SSD1-V cells.

As observed in W303R, growth on YPDS suppressed the temperaturesensitivity and short life span of mpt5 ssd1-d cells in thePSY316 strain background (not shown). Growth on YPDS also dramaticallyincreased life span in wild-type ssd1-d cells by $~$ 60% (Fig 2E).In contrast, growth on YPDS resulted in only a modest 10% increasein the life span of SSD1-V cells.

SSD1-V acts independently of ERC formation or accumulation:
Sir2p and calorie restriction promote longevity by decreasingthe formation and accumulation of ERCs in mother cells (KAEBERLEINet al. 1999 ; LIN et al. 2000 ). To determine whether the longlife span of SSD1-V cells is also due to fewer ERCs, we measuredthe rate of ERC formation and the amount of ERCs present inssd1-d and SSD1-V cells. ERC formation was estimated by determiningthe frequency at which an ADE2 marker integrated into the rDNAis lost, as demonstrated by the presence of half-sectored colonies(KAEBERLEIN et al. 1999 ). No difference was observed betweenSSD1-V and ssd1-d cells by this assay (Fig 3A). Upon directquantitation of ERCs from unsorted cells, we observed that SSD1-Vcells often had higher levels of ERCs than ssd1-d cells (Fig 3B),indicating that the life-span extension caused by SSD1-Vis unlikely to be the result of decreased ERC formation or accumulation.This is consistent with the observation that SSD1-V does notrequire Sir2p to extend life span and may indicate that SSD1-Vincreases the resistance of cells to ERCs (see DISCUSSION).

Transcriptional analysis of SSD1-V:
We previously observed that calorie restriction by growth in0.5% glucose, which promotes long life span, causes characteristicchanges in gene expression that are reproduced in two geneticmodels of CR, namely overexpression of HAP4 and deletion ofHXK2 (LIN et al. 2002 ). More recently, we demonstrated thatgrowth in the presence of high external osmolarity also extendslife span in a SIR2-dependent manner and results in a gene expressionprofile with significant similarity to calorically restrictedcells (KAEBERLEIN et al. 2002 ). Although SSD1 has been implicatedin many different genetic pathways, little is known regardingthe function of the Ssd1 protein. To further understand theeffect of SSD1-V on cell physiology and longevity, we used microarrayanalysis to examine the transcriptional profile of SSD1-V cellsrelative to wild-type ssd1-d cells.

Messenger RNA was harvested from logarithmically growing ssd1 ${Delta}$ ,ssd1-d, or SSD1-V cells. Using RNA derived from three independentexperiments, a total of 97 genes were observed to undergo achange in expression >1.5-fold in SSD1-V cells relative to ssd1-dcells (supplemental Table 1 at http://www.genetics.org/supplemental/).Of these 97 genes, only 6 underwent similar transcriptionalchanges in calorically restricted cells (Table 2). This is onlyslightly greater than the number of genes expected to overlapbetween the SSD1-V and CR data sets by chance and is in contrastto the highly significant overlap in transcriptional changesobserved between CR and HAP4 overexpression (LIN et al. 2002) or between CR and high external osmolarity (KAEBERLEIN etal. 2002 ). Intriguingly, of the 6 genes that show similar transcriptionalchanges in calorically restricted cells and SSD1-V cells, 4are involved in iron-siderochrome transport: FIT1, FIT2, FIT3,and ARN1 (supplemental Table 1 at http://www.genetics.org/supplemental/).

NCA3 mRNA is increased in SSD1-V cells:
One particularly interesting candidate gene that shows alteredmRNA levels in SSD1-V cells is NCA3 (supplemental Table 1 athttp://www.genetics.org/supplemental/). Nca3p is a member ofthe SUN family of proteins (Sim1, Uth1, Nca3, and Sun4) andfunctions to promote maturation of the mitochondrially encodedATP8-ATP6 cotranscript (PELISSIER et al. 1995 ). Upregulation(3.7-fold) of NCA3 by SSD1-V is striking because Nca3p sharesextensive homology (60%) with the aging protein Uth1p. Interestingly,we find that NCA3 mRNA is increased 4-fold in long-lived cellslacking Uth1p (data not shown). Overexpression of NCA3 fromthe ADH1 promoter results in a slight, but reproducible, increasein life span (Fig 4A), suggesting that Nca3p dosage can affectlongevity. However, NCA3 is not required for the majority ofthe life-span extension seen in SSD1-V cells, as demonstratedby the finding that nca3 SSD1-V cells have a life span comparableto that of NCA3 SSD1-V cells (Fig 4B). Therefore, we concludethat increased transcription of NCA3 accounts for, at most,a minor fraction of the longevity-promoting activity of SSD1-V.

MPT5 and SIR2 affect longevity in a pathway parallel to SSD1-V:
We have previously demonstrated that MPT5 and SSD1-V act inparallel pathways to promote cell integrity and that SSD1-Vsuppresses the short life span caused by deletion of MPT5 inthe W303R strain background (KAEBERLEIN and GUARENTE 2002 ).As expected, addition of SSD1-V similarly suppresses the shortlife span of cells lacking MPT5 in PSY316 (Fig 5A). It is interestingto note, however, that mpt5 SSD1-V cells have a life span intermediatebetween cells lacking both MPT5 and SSD1-V and cells with functionalcopies of both genes. In fact, mpt5 SSD1-V cells have a lifespan not significantly different from that of the wild-typeMPT5 ssd1-d strain, suggesting that MPT5 and SSD1-V have additiveeffects on longevity, as would be expected for genes functioningin parallel pathways.

Like SSD1-V, overexpression of MPT5 increases mother-cell lifespan (KENNEDY et al. 1997 ). Since SSD1-V is capable of extendingthe life span of cells lacking SIR2, we wished to determinewhether overexpression of MPT5 would have a similar effect.In contrast to SSD1-V, MPT5 overexpression fails to extend thelife span of sir2 fob1 cells (Fig 5B), suggesting that MPT5and SIR2 act in the same pathway to promote longevity. Furthermore,overexpression of SIR2 fails to further extend the life spanof cells in which MPT5 is overexpressed (Fig 5B).

It was previously observed that cells with altered dosage ofMPT5 display changes in telomeric and rDNA silencing (KENNEDY1996 ), suggesting a further link between MPT5 and SIR2. Overexpressionof MPT5 increases rDNA silencing and decreases telomeric silencing,while deletion has an opposite effect (Table 3). Integrationof SSD1-V, in contrast, has no detectable effect on silencingat either locus. Consistent with the inability of MPT5 overexpressionto extend life span in the absence of SIR2, the enhanced rDNAsilencing observed in cells overexpressing MPT5 is fully suppressedby deletion of SIR2 (Table 3). On the basis of these results,we propose that overexpression of MPT5 increases life span byrelocalizing Sir2p from telomeres to the rDNA (see DISCUSSION),thus enhancing the ability of Sir2p to inhibit ERC accumulationin aging mother cells.

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Table 3. Effects of MPT5, SIR2, and SSD1-V on silencing

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

One cause of aging in yeast is the accumulation of ERCs (SINCLAIRand GUARENTE 1997 ). A central regulator of ERC formation andlongevity is the Sir2p histone deacetylase (KAEBERLEIN et al.1999 ). Several genes that regulate yeast life span act by alteringSir2p activity or dosage (KAEBERLEIN et al. 1999 , KAEBERLEINet al. 2002 ; LIN et al. 2000 , LIN et al. 2002 ). Here wepresent evidence that SSD1-V defines a novel Sir2p-independentpathway necessary for cells to achieve extreme longevity.

Two pathways promoting longevity:
We initially began studying SSD1-V on the basis of its abilityto suppress the temperature sensitivity caused by mutation ofthe UTH4/MPT5 gene. Like Sir2p, Mpt5p is limiting for life spanin wild-type cells (KENNEDY et al. 1997 ). Overexpression ofMpt5p increases life span and rDNA silencing in a Sir2p-dependentmanner (Fig 5B, Table 3), suggesting that Mpt5p promotes longevityby increasing Sir2p activity at the rDNA.

In contrast to overexpression of MPT5, addition of a singlecopy of SSD1-V extends life span in both SIR2 wild-type cellsand cells lacking Sir2p (Fig 2A and Fig C). However, the sir2fob1 SSD1-V strain has a life span that is shorter than thatof the SIR2 FOB1 SSD1-V strain, demonstrating that Sir2p isrequired for maximum longevity in SSD1-V cells. This is consistentwith the observation that MPT5 SSD1-V cells have a longer lifespan than mpt5 SSD1-V cells (Fig 5A) and suggests a model wherebyMpt5p and Sir2p function in one pathway to increase life spanwhile Ssd1p functions in a parallel pathway (Fig 6).

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Figure 6. Genetic model for Ssd1p as a regulator of longevity. Ssd1p acts parallel to Sir2p to extend life span. This could involve increasing the cell's resistance to ERCs or could represent an ERC-independent longevity-promoting function. One likely possibility is that SSD1-V results in an altered cell-wall structure that allows mother cells to achieve extreme old age.

Mechanism of life-span extension by SSD1-V:
How does SSD1-V act to extend life span? The effect of Sir2pon life span is, at least partially, due to its ability to deacetylaterDNA histones and inhibit ERC formation (KAEBERLEIN et al. 1999). There is no evidence to suggest that SSD1-V affects the rateof ERC formation or accumulation. Addition of SSD1-V had nodetectable effect on rDNA recombination (Fig 3A) or on rDNAsilencing (Table 3) in PSY316. Moreover, we failed to detecta decrease in ERC levels in SSD1-V cells relative to those inssd1-d cells (Fig 3B). While it is still possible that SSD1-Vaffects ERC replication or segregation specifically in agedcells, we feel that this is unlikely to be the case. An alternativepossibility is that SSD1-V makes cells more resistant to ERCs,rather than reducing ERC levels. In support of this hypothesis,we often observed that steady-state ERC levels were increasedin unsorted SSD1-V cells relative to those in wild-type ssd1-dcells (Fig 3B), although this was not always the case. The mechanismby which ERCs induce senescence is currently unknown. One hypothesisis that ERCs bind to and titrate key cellular replication ortranscription factors away from their normal targets. Alternatively,the rapid amplification of rDNA sequence could alter rRNA transcriptionand/or processing, resulting in ribosome dysregulation. Ssd1phas been shown to bind RNA and is predicted to have RNase activity(UESONO et al. 1997 ). Perhaps SSD1-V alters rRNA or ribosomebiogenesis in a manner that makes cells more resistant to ERCs.

One attractive hypothesis is that SSD1-V promotes longevityby increasing cell-wall stability and cell integrity. SSD1-Vsuppresses several temperature-sensitive mutations that weakenthe cell wall (Table 4) and has been found to directly affectcell-wall composition (WHEELER et al. 2003 ). SSD1-V also improvesresistance to the cell-wall-perturbing agents CFW and SDS (KAEBERLEINand GUARENTE 2002 ), increases the maximum temperature at whichPSY316 is capable of growth (Fig 1C), and alters the transcriptionof cell-wall biosynthetic and structural genes. Perhaps thecell wall becomes limiting in very old cells and SSD1-V extendslife span by stabilizing it. How might cell-wall stability limitreplicative life span? The terminal phenotype of yeast cellsin the life-span assay is cell cycle arrest often accompaniedby cell lysis (MCVEY et al. 2001 ). Enhanced cell-wall stabilitymay prevent cell lysis late in life and allow additional celldivisions to occur.

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Table 4. Reported genetic interactions with SSD1-V

Genetic diversity and the study of aging:
The data presented here identify a genetic polymorphism thathas a profound effect on mother-cell life span. Genetic polymorphismshave also been proposed to affect the likelihood of achievingextreme longevity in human populations (e.g., PUCA et al. 2001), as well as in other model systems. Since both ssd1-d andSSD1-V allele types have been isolated from natural yeast populations,the SSD1 locus represents a true polymorphic locus affectinglongevity. In the past, researchers studying aging in yeasthave tended to avoid using long-lived wild-type backgrounds.We speculate that the majority (if not all) of these shorter-livedyeast strains carry ssd1-d alleles. A comprehensive reevaluationof previously identified mutations affecting life span in along-lived SSD1-V background would be of value to the field.

SSD1-V confers extreme longevity on yeast mother cells by apathway independent of Sir2p. Sir2 proteins have been foundto extend life span in animals and, like SIR2, SSD1 homologsare present in yeast, worms, flies, and mammals. Might SSD1family members also promote longevity outside of yeast? Themechanism by which SSD1-V cells achieve up to 85% longer lifespan is still unknown. Further work should be devoted to testingcandidate longevity genes regulated by SSD1-V and to definingthe molecular function of Ssd1p in cells.

ACKNOWLEDGMENTS

We thank N. Bishop, B. Kennedy, and T. Kaeberlein for helpfuldiscussion and insight. This work was supported by grants toL.G. from the National Institutes of Health (NIH), The EllisonMedical Foundation, The Seaver Institute, and the Howard andLinda Stern Fund. G.R.F. is supported by grants from the NIHand is an American Cancer Society Professor of Genetics. A.A.A.is supported by an NIH Training Grant in Genomic Sciences, sponsoredby the Biotechnology Process Engineering Center.

Manuscript received August 13, 2003; Accepted for publication December 23, 2003.

LITERATURE CITED

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
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