Antagonistic Interactions between Yeast Chaperones Hsp104 and Hsp70 in Prion Curing

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Molecular and Cellular Biology, February 1999, p. 1325-1333, Vol. 19, No. 2
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Antagonistic Interactions between Yeast Chaperones Hsp104 and Hsp70 in Prion Curing

Gary P. Newnam,¹ Renee D. Wegrzyn,¹ Susan L. Lindquist,² and Yury O. Chernoff¹^,^*

School of Biology, Georgia Institute of Technology, Atlanta, Georgia 30332-0230,¹ and Howard Hughes Medical Institute and Department of Molecular Genetics and Cell Biology, University of Chicago, Chicago, Illinois 60637²

Received 19 August 1998/Returned for modification 23 September 1998/Accepted 26 October 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

The maintenance of [PSI], a prion-like form of the yeast release factor Sup35, requires a specific concentration of the chaperoneprotein Hsp104: either deletion or overexpression of Hsp104 willcure cells of [PSI]. A major puzzle of these studies was thatoverexpression of Hsp104 alone, from a heterologous promoter,cures cells of [PSI] very efficiently, yet the natural inductionof Hsp104 with heat shock, stationary-phase growth, or sporulationdoes not. These observations pointed to a mechanism for protectingthe genetic information carried by the [PSI] element from vicissitudesof the environment. Here, we show that simultaneous overexpressionof Ssa1, a protein of the Hsp70 family, protects [PSI] from curingby overexpression of Hsp104. Ssa1 protein belongs to the Ssa subfamily,members of which are normally induced with Hsp104 during heatshock, stationary-phase growth, and sporulation. At the molecularlevel, excess Ssa1 prevents a shift of Sup35 protein from theinsoluble (prion) to the soluble (cellular) state in the presenceof excess Hsp104. Overexpression of Ssa1 also increases nonsensesuppression by [PSI] when Hsp104 is expressed at its normal level.In contrast, hsp104 deletion strains lose [PSI] even in the presenceof overproduced Ssa1. Overproduction of the unrelated chaperoneprotein Hsp82 (Hsp90) neither cured [PSI] nor antagonized the[PSI]-curing effect of overproduced Hsp104. Our results suggestit is the interplay between Hsp104 and Hsp70 that allows the maintenanceof [PSI] under natural growthconditions.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Prions are infectious proteins which are believed to cause transmissible neurodegenerative diseases in mammals, such as sheepscrapie, human kuru, and Creutzfeldt-Jacob disease, and bovinespongiform encephalopathy, or "mad cow" disease (see references38 and 50 for reviews). According to the current model, theprion protein (PrP^Sc) is a conformational derivative of the normal protein (PrP^C), which has acquired an ability to influence the normal protein,encoded by the same gene, to adopt the prion conformation. Inthe PrP^Sc conformation, PrP is characterized by increased proteinase resistance,high $beta$ -sheet content, and a capacity to form insoluble aggregates(38, 39).

Recent data suggest that prion-like phenomena, in which self-perpetuating changes in protein conformation alter the phenotypeof the organism, are widespread in nature. It has been hypothesizedthat autocatalyzed misfolding and/or aggregation cause such acommon human disease as Alzheimer's disease (22, 26, 28).Even more remarkably, it has been noted that yeast non-Mendelianelements [URE3] and [PSI] (53) and Podospora non-Mendelian element[Het-S] (8) behave like prions. The propagation of these elementsis believed to be due to the transmission of proteins with a self-perpetuating,functionally altered conformation, rather than to the transmissionof a nucleic acid replicon. Therefore, the prion model providesan additional mechanism of genetic transmission, which is basedon the information coded in the biopolymer's three-dimensionalstructure rather than in its primary sequence. Existence of suchsystems of structural coding has revolutionary implications forour understanding of genetics andevolution.

[PSI] causes translational readthrough (nonsense suppression) in yeast (9, 10). Both genetic and biochemical data stronglysuggest that [PSI] represents a functionally defective form ofthe evolutionary conserved release factor eRF3 (Sup35), whichpropagates through a self-perpetuating change in protein conformation(see references 29, 49, and 55 for reviews). Sup35 overproductiongreatly increases the frequency of the spontaneous appearanceof [PSI] (4, 14). Yeast Sup35 protein forms insoluble proteinase-resistantaggregates in [PSI⁺] cells (35, 36). The insoluble form of the Sup35 protein(Sup35^PSI) stimulates aggregation of the soluble Sup35 protein in cellextracts, thus mimicking the prion-like propagation of the proteinchange in vitro (18, 37). The purified Sup35 protein has alsobeen shown to undergo self-seeded polymerization in vitro, resultingin the formation of Congo red-staining amyloid-like fibers (18,24), similar to those formed by the mammalian PrP (39).

Conformational switches and aggregation events, postulated by the prion model, make it reasonable to expect that chaperoneproteins are involved in prion propagation. Indeed, we have previouslydescribed that [PSI] propagation requires an intermediate amountof the chaperone protein Hsp104 (5). Inactivation of Hsp104cured cells of [PSI], suggesting that Hsp104 may be required fora partial unfolding of the normal protein that makes it susceptibleto assuming a prion-like conformation. However, selective overproductionof Hsp104 also inhibited and eventually cured [PSI], with an efficiencythat correlated with the level of Hsp104 produced. Since it hasbeen shown that Hsp104 function in thermotolerance is to reverseheat-induced aggregation damage (34), one could suggest thatexcess Hsp104 can shift the balance from prion-like aggregatesto partially unfolded intermediates and soluble forms, resultingin the loss of [PSI]. Biochemical experiments confirmed that bothexcess Hsp104 and hsp104 deletions lead to an increase in theproportion of the soluble Sup35 protein relative to insolubleSup35 protein in [PSI⁺] cells (35, 36). In vitro experiments indicate that Hsp104and Sup35 can physically interact with each other under certaincircumstances (43). Recent in vitro data also suggest that Hsp104influences the conformational transitions of mammalian PrP aswell, promoting the acquisition of the structural characteristicsof the disease form, PrP^Sc, with a high degree of specificity (13). This result indicatesthat folding intermediates formed by unrelated prion proteinspossess similar features. Thus, investigating the nature of chaperone-Sup35interaction not only is important for understanding the remarkableprocess that allows the transmission of genetic information byalternative protein conformations in yeast but also may lead toincreased understanding of the general mechanisms of prion-likeconformationalswitches.

No human homolog of Hsp104 has been identified to date, which raises the question of whether other chaperone proteins thatare conserved in humans influence prion-like transitions. Indeed,in yeast cells, the relationship between the Hsp104 chaperoneand the [PSI] prion-like element presents a paradox (see reference54) that might be explained by interactions with other chaperones.Hsp104 levels increase during growth at high temperatures andupon heat shock (40, 41). When Hsp104 is selectively inducedto similar levels by using a heterologous promoter, up to 90%of the culture is cured of [PSI] (5, 6, 31). Yet growthat 37 to 39°C causes neither inhibition nor curing of [PSI] (44,48), while heat shock at 42 to 55°C causes only low-efficiencycuring of [PSI] (6, 10, 31, 48). It might be postulatedthat other proteins, denatured by heat shock, compete with theSup35 protein for Hsp104, preventing newly induced Hsp104 fromcuring cells of [PSI] under these circumstances. However, Hsp104normally accumulates during heat shock at levels much higher thanrequired to repair heat-induced damage (30). Even more strikingly,[PSI] is very stable in stationary-phase cells and spores (7,10), when Hsp104 levels are also high (41) but protein denaturationis presumablylow.

On the basis of these data, we (6) hypothesized that other heat- and stationary-phase-induced factors interfere with Hsp104'scapacity to cure cells of [PSI], allowing the stable propagationof [PSI] through diverse environmental conditions. Here, we reportthe effects of Ssa1 protein, a yeast member of the Hsp70 family,on Hsp104 mediated-curing of [PSI]. Ssa proteins are abundantchaperones of the yeast cytosol that are coinduced with Hsp104during heat shock, stationary-phase growth, and sporulation (25,51, 52). Moreover, they interact with Hsp104 in thermotolerancein vivo (42) and in protein disaggregation in vitro (17).Since Ssa proteins constitute a single essential complementationgroup with strongly overlapping functions, we have analyzed onlySsa1. To provide a broader range of circumstances in which totest the interactions between Hsp104, Hsp70, and [PSI], we tookadvantage of the existence of distinct types of [PSI] elements.Strong and weak [PSI] elements have stable, heritable differencesin the efficiency of nonsense suppression as well as differentmitotic transmission rates. Because these elements can be propagatedin isogenic yeast strains, they are believed to result from somewhatdifferent, self-perpetuating conformational states of Sup35 (14).Members of the yeast Hsp70 family modify Hsp104's effect on bothtypes of [PSI] element, providing an explanation for the maintenanceof [PSI] under naturalconditions.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Yeast strains. Genotypes of the Saccharomyces cerevisiae strains are shown in Table 1. [PSI⁺] strains OT55 (also called [PSI⁺]1-1-74-D694) and OT56 (also called [PSI⁺]7-74-D694) are independent derivatives of strain 74-D694, inducedby overproduction of the wild-type Sup35 protein as describedpreviously (14). The [psi] ade1-14 strains are red on YPD medium. Presence of [PSI] leadsto the suppression of the ade1-14_UGA allele, detected as growthon adenine-deficient ( $-$ Ade) medium after 3 to 4 (OT56) or 7 to8 (OT55) days of incubation and as white (OT56) or pink (OT55)color on YPD medium. OT56 exhibits higher mitotic stability of[PSI] in the presence of guanidine-HCl than OT55 (14). L-1607is an hsp104::URA3 disruption obtained in strain OT55 as describedpreviously (5). OT46 is a spontaneous Ura derivative of L-1607 which, according to Southern and Westernanalysis, retains the hsp104 deletion (15). GT1-S31 and GT1-S13were recovered from the meiotic progeny of the genetic cross between35-D693 (15) and JN14. GT56-13B was recovered by A. Galkin (inY. Chernoff's lab) from the meiotic progeny of the cross betweenGT1-S13 and OT56.

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TABLE 1. S. cerevisiae strains used

Plasmids. Shuttle plasmids used in this study are shown in Table 2. Plasmid pLA1, which is a pRS313 (45) derivative containing theGAL1,10 promoter, was constructed by L. Arwood in S. Lindquist'slab. Plasmid pSSA1-LEU2, also called pLH101, is a pRS425 derivativecontaining a wild-type SSA1 gene under its normal promoter andwas constructed by L. Henninger in S. Lindquist's lab. PlasmidpH28, constructed by E. Schirmer in S. Lindquist's lab, is a pLA1derivative which contains the entire promoterless HSP104 geneinserted into BamHI-SacI-cut polylinker immediately after GAL1,10promoter. Plasmid pMC3, which contains a promoterless HSP82 genefused into the BamHI site of the GAL1,10 promoter in centromericURA3 vector pBM150 (46), was constructed by M. Fortin in S.Lindquist's lab. Plasmids pUKC815 and pUKC819, kindly providedby M. F. Tuite, contain PGK-lacZ hybrid constructs from pUKC350and pUKC353 (16), respectively, cloned in the centromeric URA3-containingvector YCp50.

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TABLE 2. Shuttle plasmids used

Antibodies. Sup35 antipeptide antibodies specific to amino acid positions 137 to 151 of the Sup35 protein (35), Hsp104-specific antibody8-1 (33), and Hsp82-specific antibodies (2) have been describedpreviously. Ssa-specific polyclonal antibody SSA1 C1delB was kindlyprovided by E. Craig. Secondary anti-rabbit antibodies were purchasedfrom Amersham. Western blotting, reaction to the primary and secondaryantibodies, and detection were performed by the chemiluminescencemethod as described in the Amersham protocol. Densitometry assayswere performed according to Image Tool (developed by Don Wilcox,Brent Dove, Doss McDavid, and David Greer; downloaded from http://www.uthscsa.edu).

Yeast media and growth conditions. Standard yeast media and cultivation conditions (23) were used. Transformation was performed according to the modified Li⁺ procedure (20). Liquid cultures were grown on the shaker, normallyat 200 to 250 rpm, with a liquid/flask volume ratio of 1:5 ormore. Galactose induction on solid medium was performed by replicaplating the yeast strains onto the corresponding synthetic mediumcontaining galactose instead of glucose. To achieve galactoseinduction in liquid medium, yeast cultures were pregrown in thecorresponding synthetic glucose medium up to 2 × 10⁶ to 1 × 10⁷ cells/ml, collected by centrifugation, washed twice with H₂O,and inoculated into the corresponding synthetic medium, containing2% galactose and 2% raffinose, at the starting concentration 2.5× 10⁵ to 5 × 10⁵ cells/ml.

Standard procedures (23) were used for yeast sporulation, micromanipulation, and tetrad analysis. For isolation of randomspores, sporulating cultures were suspended in H₂O, vortexed withan equal volume of diethyl ether for 5 min, and plated on thesynthetic medium, which was selective for the particular genotype.About 95 to 99% of the colonies are formed by the haploid ascospores,which are more resistant to ether treatment than the vegetative(diploid)cells.

Temperature resistance assays. To measure temperature resistance of the exponential yeast cells, yeast precultures were grown overnight at 25°C with shakingin the corresponding synthetic medium selective for the plasmid(s),diluted to 10⁶ cells/ml, and incubated for another 3 h at 25°C with shaking.After these incubations, 0.5-ml aliquots of each culture wereeither placed directly on ice (control samples) or incubated for5 to 20 min in the 50°C water bath and then placed on ice (heat-shockedsamples). Then, serial dilutions of both heat-shocked and controlsamples were prepared and either pipetted onto the correspondingsynthetic medium, 5 µl per spot (semiquantitative assay), or platedonto the corresponding synthetic medium, 0.1 ml per plate (quantitativeassay). Resulting plates were scored after 3 to 4 days of incubationat 30°C. Temperature resistance of the cultures preinduced at37°C was determined in the same way, except that at 30 min beforeheat shock, 5-ml aliquots of each culture were placed into 37°Cand incubated with shaking for another 30 min, as described previously(40, 41).

To measure temperature resistance of the galactose-induced yeast cells, yeast precultures were grown to 2.4 × 10⁶ cells/ml at 25°C with shaking in 5 ml of the corresponding syntheticglucose medium, selective for the plasmids. Cells were collectedby centrifugation, washed twice with H₂O, resuspended in 50 mlof the same medium containing galactose and raffinose insteadof glucose, and incubated with shaking at 25°C for about two celldivisions, resulting in the final concentration of about 10⁶ cells/ml. Then 0.5-ml aliquots of each culture were taken andheat shocked as describedabove.

Protein isolation and analysis. Hsp104, Hsp70 (Ssa1), and Hsp82 were identified by the reaction to the corresponding antibodies (see above) in the proteinextracts, prepared from yeast cells which had been lysed on avortex mixer with glass beads in 100 mM Tris-HCl (pH 7.5)-0.2M NaCl-1 mM EDTA-0.5 mM dithiothreitol-2 mM phenylmethylsulfonylfluoride-5% glycerol, or in the total-lysate fractions preparedby the centrifugation-fractionation (see below). Extracts werethen separated by the standard sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) procedure. The centrifugation-fractionationperformed as described previously (35), with slight modifications,was used for determination of the Sup35 protein distribution betweenthe soluble and insoluble fractions. Yeast cotransformants weregrown to 5 × 10⁶ cells/ml in either synthetic glucose or synthetic galactose-raffinosemedium, both selective for both plasmids. Cells were lysed ona vortex mixer with glass beads in lysis buffer containing 50mM Tris-HCl (pH 7.5), 10 mM KCl, 5 mM MgCl₂, 0.1 mM EDTA, 0.1mM dithiothreitol, 100 µg of cycloheximide per ml, 2 mM phenylmethylsulfonylfluoride, 1 mM benzamidine, 2 µg of pepstastin A per ml, 10 µgof leupeptin per ml, and 100 µg of RNase A per ml. High concentrationsof proteinase inhibitors were required to keep proteins stablethroughout the fractionation procedure. Cell debris was removedby centrifugation at 3,000 × g to produce a total-lysate fraction.Half of the total lysate was used as a control, while the remainderwas fractionated by centrifugation at 8,300 × g for 15 min. Thesupernatant was placed into a fresh tube, and the pellet was resuspendedin an equal amount of lysis buffer. SDS, glycerol, $beta$ -mercaptoethanol,and Tris-HCl (pH 6.8) were added to every sample up to final concentrationsof 3%, 10%, 3%, and 0.15 M, respectively. Resulting samples wereheated at 95°C for 10 min and run on the standard SDS-polyacrylamidegel. For the protein assays, gels were transferred onto HybondECL nitrocellulose membranes and reacted to the antibodies asdescribedabove.

The $beta$ -galactosidase activity assays. For measuring $beta$ -galactosidase activity, yeast cultures were grown overnight at 30°C with shaking in liquid medium selectivefor the plasmids. Cell extracts were prepared by the standardprocedure (23) and stored at $-$ 70°C. The $beta$ -galactosidase activityin extracts was measured by using a chemiluminescence assay (21),with modifications according to the most recent Tropix, Inc.,protocol, using an Optocomp I luminometer (MGM Instruments, Inc.).The correspondence between relative light units and amounts ofactive $beta$ -galactosidase was determined by using standard solutionsof pure $beta$ -galactosidase, purchased from Sigma. Galacton-Plus andAccelerator were purchased from Tropix; $beta$ -galactosidase activitieswere normalized per 1 mg of total cellular protein, the concentrationof which was determined by the Bradford assay (Bio-Rad).

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

Ssa1 overproduction protects [PSI] from the effects of overproduced Hsp104. As we have shown previously (5), a low-copy-number (centromeric) URA3 plasmid, containing the wild-type HSP104 gene (pYS104),inhibits the ability of [PSI] to suppress a nonsense mutationin the ADE1 gene, ade1-14_UGA. Both a strong (OT56) and a weak(OT55) [PSI⁺] strain, both bearing the ade1-14 allele, became phenotypicallyPsi when they carried this plasmid. That is, they did not grow onthe synthetic medium which contained no adenine and was selectivefor the plasmid. To determine if the Hsp70 family protein Ssa1altered the affect of Hsp104 on [PSI⁺], we cotransformed cells with both pYS104 and a multicopy SSA1plasmid (pSSA1-LEU2). The cells containing both plasmids remainedphenotypically Psi⁺: they grew in the absence of adenine (Fig. 1) and formed pink(OT55) or white (OT56) colonies on YPD, in contrast to more reddishcolonies of the transformants bearing pYS104 alone (not shown).This result suggests that the Ssa protein interferes with Hsp104'sability to inhibit [PSI]-mediated suppression.

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FIG. 1. Effects of multicopy SSA1 plasmid on Hsp104-induced inhibition and curing of [PSI] in yeast strains OT55 (A) and OT56 (B). Plasmid combinations were as follows: control, YEp13 plus pRS316; Ssa1, pSSA1-LEU2 plus pRS316; Hsp104, YEp13 plus pYS104; Ssa1-Hsp104, pSSA1-LEU2 plus pYS104. (Plasmids YEp13 and pRS316, which contain no HSP genes, were used as matching controls.) To determine Hsp104 levels, proteins were isolated from the cultures growing in liquid $-$ Ura-Leu/glucose medium at 25°C, separated by SDS-PAGE, and reacted to Hsp104-specific antibodies. Experiments were repeated at least two times with the same result and used at least two different transformants of each set. For the loading control, the same protein extracts were reacted to the Sup35 antibodies. In contrast to the previous findings by Paushkin et al. (36), levels of the Sup35 protein in these total lysates, which include both soluble and insoluble fractions (see description of Sup35 aggregation below), always remained constant in the strains used in this study regardless of the presence or absence of [PSI]. Relative protein amounts were also confirmed by Coomassie blue staining (not shown). To determine suppression, transformants grown on $-$ Ura-Leu/glucose medium were replica plated onto $-$ Ura-Leu-Ade/glucose medium and photographed after 6 (A) or 4 (B) days of incubation at 30°C. In each case, at least eight independent transformants for each plasmid combination were tested. No differences in growth between transformants were detected on the control $-$ Ura-Leu/glucose (A and B) plates (not shown). To test for Sup35 aggregation, protein extracts, prepared from the cultures grown in liquid $-$ Ura-His/glucose medium, were fractionated by centrifugation as described previously (35) (see Materials and Methods). For each strain, equal volumes of supernatant (S) and pellet (P) fractions were loaded onto the gel. Distributions of total cellular proteins between S and P fractions were similar for all strains, as verified by Coomassie blue staining (not shown). Experiments were repeated at least two times with at least two different transformants of each set. To examine [PSI] curing, cultures grown in liquid $-$ Ura-Leu/glucose medium were diluted in H₂O, plated onto the same medium (100 to 200 colonies per plate), grown for 3 to 4 days of incubation at 30°C, and replica plated onto 5-fluoroorotic acid medium to get rid of URA3-containing HSP104 plasmid; after 3 days of growth, cultures were replica plated onto $-$ Ade medium and YPD medium, in order to identify [PSI⁺] and [psi] colonies (see Materials and Methods). Ninety-five percent probability levels of variation are shown.

Next we examined whether the Ssa protein had prevented curing of [PSI] by Hsp104. To check whether the pYS104 plasmid hadcured cells of [PSI] or had simply inhibited its phenotypic effect,transformants bearing HSP104 and SSA1 plasmids (or matching controlplasmids) were incubated on $-$ Ura-Leu medium, to select for theplasmids, and grown for 3 days at 30°C. Serial dilutions of eachtransformant were then plated onto $-$ Ura-Leu medium to obtain singlecolonies, and these were then selected for loss of the URA3-containingpYS104 plasmid by replica plating colonies onto 5-fluorooroticacid (23). Finally, colonies were replica plated on $-$ Ade andYPD media to test for the presence of [PSI].

In the strong [PSI⁺] strain, OT56, the vast majority of colonies originating from the pYS104 transformants remained [PSI⁺] after plasmid was cured (Fig. 1B), and the suppressor efficiencyof [PSI] had not been significantly changed, judging from bothgrowth on $-$ Ade and color on YPD. This finding indicates that expressionof Hsp104 from this plasmid had temporarily inhibited the Psi⁺ phenotype, but had not efficiently cured cells of the element,as reported previously (5). In contrast, most pYS104 transformantsof the weak [PSI⁺] strain, OT55, remained [psi] after pYS104 was lost, indicating that Hsp104 had cured themof the [PSI] element. This correlation between the nature of the[PSI] element (strong versus weak) and the efficiency of Hsp104-inducedcuring is in agreement with our previous data (14). Notably,most of the OT55 transformants that had contained both pYS104and pSSA1-LEU2 were [PSI⁺] when pYS104 was lost (Fig. 1A). This result indicates that Ssa1can both negate the ability of Hsp104 to inhibit phenotypic expressionof strong [PSI] elements and interfere with Hsp104-induced curingof weak [PSI]elements.

Strong [PSI⁺] strains such as OT56, which are [PSI⁺] after loss of the low-copy-number HSP104 plasmid, can be cured of [PSI]when HSP104 is expressed at a higher level from a strong induciblepromoter (5). To determine if SSA1 overexpression is able toprotect [PSI] against curing by high levels of Hsp104, we usedthe centromeric plasmids pGAL::SSA1-URA3 and pH28(HIS3), in whichthe GAL promoter was fused to the SSA1 and HSP104 genes, respectively.In strains carrying these constructs, SSA1 and HSP104 overexpressionwas induced by growth on medium containing galactose instead ofglucose. Matching centromeric plasmids, pRS316GAL (URA3) and pLA1(HIS3), without the Hsp104 and Ssa1 coding sequences were usedas controls. All double-plasmid combinations were obtained inthe strong [PSI⁺] strain OT56 and induced on galactose (see Materials and Methods).[PSI]-mediated suppression of ade1-14 on galactose medium andthe proportion of cells that became [PSI⁺] and [psi] after galactose induction were determined. GAL::HSP104-mediatedinhibition of [PSI] suppression was efficient only in the absenceof GAL::SSA1 (Fig. 2), and the curing of [PSI] by induced GAL::HSP104was also reduced significantly in the presence of the inducedGAL::SSA1 (Fig. 2). In the absence of GAL::HSP104, GAL::SSA1 didnot cause [PSI] curing.

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FIG. 2. Hsp104 levels and effects on [PSI] in OT56 cells, which contain galactose-inducible SSA1 and HSP82 constructs. Plasmid combinations used were as follows: control, pRS316GAL plus pLA1; Ssa1, pGAL::SSA1-URA3 plus pLA1; Hsp82, pMC3 plus pLA1; Hsp104, pRS316GAL plus pH28; Ssa1 plus Hsp104, pGAL::SSA1-URA3 plus pH28; Hsp82 plus Hsp104, pMC3 plus pH28. (Plasmids pRS316GAL and pLA1, which contain no HSP genes, were used as matching controls.) Hsp104 levels were determined as described in the legend to Fig. 1 except that cultures were grown in the $-$ Ura-His/galactose-raffinose medium at 25°C. All the samples shown contained the same amount of total protein loaded, as verified by Coomassie blue staining and/or by reaction to the Sup35-specific antibodies, as described for Fig. 1. Each experiment was repeated at least four times with at least two independent transformants per each plasmid combination. Background Hsp104 levels are higher than in Fig. 1 due to partial induction of the chromosomal HSP104 allele during growth on galactose, as described previously (41). To determine suppression, transformants grown on $-$ Ura-His/glucose medium were replica plated onto $-$ Ura-His-Ade/galactose medium and photographed after 6 days of incubation at 30°C. In each case, at least eight independent transformants for each plasmid combination were tested. No differences in growth between transformants were detected on the control $-$ Ura-His/galactose plates (not shown). To test for Sup35 aggregation, protein extracts, prepared from the cultures grown in liquid $-$ Ura-His/galactose-raffinose medium at 25°C, were fractionated by centrifugation as described elsewhere (35) (see Materials and Methods). For each strain, equal volumes of supernatant (S) and pellet (P) fractions were loaded onto the gel. Distributions of total cellular proteins between S and P fractions were similar for all strains, as verified by Coomassie blue staining (not shown). Experiments were repeated at least three times with at least two different transformants of each set. To examine [PSI] curing, cultures grown in liquid $-$ Ura-His/galactose-raffinose medium at 25°C were washed twice with H₂O, diluted in H₂O, plated onto $-$ Ura-His/glucose medium (100 to 200 colonies per plate), grown for 3 to 4 days at 30°C, and replica plated onto $-$ Ura-His-Ade/glucose and YPD media in order to identify [PSI⁺] and [psi] colonies. Ninety-five percent probability levels of variation are shown.

Ssa and Hsp104 protein levels in the overproducer strains. The expression of Hsp70 is tightly controlled by autoregulatory mechanisms. Relatively low levels of Ssa induction in overproducerstrains could be expected, due to both the presence of constitutivelyexpressed members of the Ssa subfamily (52), which cross-reactwith the Ssa antibodies, and the ability of Ssa1 protein to downregulate the transcription of its own gene and that of other SSAgenes (47). Densitometry analysis of the Western blots confirmedthat exponentially growing cells, which bear multiple copies ofthe SSA1 gene, contain 1.53 ± 0.214-fold more Ssa protein thanexponentially growing cells of isogenic transformants carryingthe matching control vectors. Similar levels of Ssa overproduction(1.51 ± 0.127-fold) were achieved with the GAL::SSA1 constructon galactose medium. As previously described (42), Hsp104 overproductionhad no effect on Ssa protein levels (not shown). Western blotresults (Fig. 1 and 2), accompanied by densitometry measurements(not shown), also confirmed that the levels of overproduced Hsp104in these strains were not affected by the overproduction of Ssa1.Both the centromeric pYS104 plasmid on glucose medium (Fig. 1)and the GAL::HSP104 plasmid on galactose medium (Fig. 2) causedan increase in Hsp104 protein levels independently of the Ssa1plasmids. This result suggests that the ability of overproducedSsa1 protein to protect [PSI] from excess Hsp104 is not due toa decrease in Hsp104expression.

Excess Ssa1 prevents accumulation of soluble Sup35 protein in [PSI⁺] cells that overexpress Hsp104. The Sup35^PSI prion protein, found in [PSI⁺] cells, forms insoluble aggregates, in contrast to the normal soluble Sup35 proteinin [psi] cells (35, 36). It has been reported that when Hsp104 hascured cells of [PSI] aggregates, Sup35 protein is soluble. Quiteremarkably, even low levels of Hsp104 overexpression (35, 36)led to a detectable shift in the ratio of soluble to insolubleSup35 protein, although [PSI] curing was inefficient under theseconditions.

Our results (Fig. 1 and 2) confirm that Hsp104 overproduction increases the amount of soluble Sup35 protein versus insolubleSup35 protein in all strains and conditions tested. However, transformantswhich overexpress both SSA1 and HSP104 contained less solubleSup35 protein and more insoluble Sup35 protein than transformantswhich overexpress HSP104 alone. Thus, at the molecular level,higher levels of Ssa1 interfere with the disappearance of Sup35^PSI aggregates, observed during growth in the presence of increasedlevels of Hsp104. In cells expressing Hsp104 at wild-type levels,Ssa1 overproduction showed no reproducible effect on the ratiobetween soluble and insoluble Sup35 protein (Fig. 1 and 2).

Increased levels of Hsp82 protein do not interfere with Hsp104's effect on [PSI]. The expression of Hsp82 is also increased under conditions that induce Hsp104 and Hsp70 (Ssa1): heat shock, stationary-phasegrowth, and sporulation (2). To determine whether Hsp82 modifiesthe effect of Hsp104 on [PSI], GAL::HSP82 and GAL::HSP104 constructswere induced individually and simultaneously in the [PSI⁺] strain OT56, as described for Ssa1. Hsp82 overproduction wasverified by Western blotting (not shown). Normal [PSI] maintenanceand [PSI]-mediated suppression were not affected by Hsp82 overproduction,and Hsp104-mediated inhibition and curing of [PSI] were not affectedby excess Hsp82 (Fig. 2). We also examined whether excess Hsp82affected the solubility of Sup35. There was no effect of excessHsp82 on the distribution of Sup35 protein between the solubleand insoluble fractions in cells that expressed Hsp104 at normallevels or in cells that expressed it at high levels (Fig. 2).Similar results were obtained with the strain OT55 (notshown).

Excess Ssa1 increases the efficiency of nonsense suppression in [PSI⁺] strains. We also examined the effect of Ssa1 on nonsense suppression in [PSI⁺] strains that do not carry Hsp104-overproducing plasmids. Ourprevious data (5, 31) suggested that multiple copies of theSSA1 gene increased the growth of some [PSI⁺] strains on media selective for nonsense suppression and inhibitedthe growth of other [PSI⁺] strains. In both OT55 and OT56 strains bearing the [PSI]-suppressibleade1-14_UGA mutation, plasmid pSSA1-LEU2 increased growth on $-$ Ademedium and decreased accumulation of the red pigment (not shown).A problem in interpreting this observation is that Ssa1 proteinis involved in the general stress response, which helps cellssurvive stressful conditions. It requires 5 to 8 days to forman individual colony on $-$ Ade medium through [PSI]-mediated suppressionof the ade1-14 allele, whereas wild-type cells form colonies onthis medium in 2 days. Thus, better growth of some strains on $-$ Ade medium might be due to an effect of Ssa1 overexpression ongrowth under stressful conditions, rather than an effect on [PSI]-mediatedsuppression. On the other hand, Ssa1 overproduction is known tobe harmful to some yeast strains (47), and this could explainthe inhibition of growth in some Ssa1 overproducers on $-$ Ade medium.To directly measure whether Ssa1 affects [PSI]-mediated suppressionin OT55 and OT56, we used a quantitative assay for the readthroughof nonsense codons. Plasmid pUKC815 bears the promoter and N-terminalend of the yeast PGK gene fused in frame to the bacterial $beta$ -galactosidasegene (PGK-lacZ). In the matching vector for monitoring nonsensesuppression, pUKC819, the PGK and lacZ open reading frames areinterrupted by a UGA mutation (16) (see Materials and Methods).The $beta$ -galactosidase levels per 1 mg of total cellular proteinwere determined in OT56 derivatives transformed with either ofthese vectors, together with plasmid pSSA1-LEU2 or the YEp13 controlplasmid. Efficiencies of suppression were calculated as ratiosof $beta$ -galactosidase activities in matched strains carrying thetwo fusion constructs. Cells which contained the multicopy SSA1plasmid exhibited three- to fourfold-higher efficiencies of suppressionthan cells carrying the vector control (Table 3). Therefore,results of all three assays used to measure nonsense suppressionby [PSI] (i.e., growth on $-$ Ade medium, color, and PGK-lacZ readthrough)correlated to each other in OT56 genetic background. This confirmsthat increased growth on $-$ Ade medium and decreased accumulationof the red pigment, caused by excess Ssa1 protein in OT56 andisogenic OT55, result from a stimulating effect of excess Ssa1on [PSI]-mediated nonsense-suppression rather than from the secondaryeffects on growth.

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TABLE 3. Effect of multicopy SSA1 plasmid on [PSI]-mediated nonsense suppression in strain OT56

Excess Ssa does not produce nonsense suppression in cells carrying a deletion of Hsp104. Deletion of HSP104 in a [PSI⁺] strain heritably cures cells of [PSI], eliminating nonsense suppression. Because Ssa1 increasesthe efficiency of nonsense suppression in cells that overexpressHsp104 and in cells with wild-type levels of Hsp104, we next examinedwhether it would promote sufficient nonsense suppression to compensatefor an hsp104 deletion. The hsp104::URA3 disruption strain L-1607,which bears the [PSI]-suppressible ade1-14 mutation, was transformedwith the multicopy pSSA1-LEU2 plasmid and crossed to the [PSI⁺] strains GT1-S31 and GT56-13B. The resulting diploids, whichare homozygous for ade1-14 and ura3 and heterozygous for the hsp104::URA3disruption, were [PSI⁺]. Isogenic diploids bearing the matching vector without SSA1,YEp13, served as controls. The diploids were sporulated and dissected.Haploid progeny that grew on $-$ Ura-Leu medium, and presumably carriedthe hsp104::URA3 deletion and plasmid pSSA1-LEU2 or YEp13, weretested for the ability to grow on $-$ Ade medium. None did. To increasethe number of colonies that could be tested, we used random sporeplatings to select cells that could grow on $-$ Ura-Leu medium. (Raresurviving diploids were identified by their inability to mateand were discarded.) In both control and Ssa1-overproducing strains,most of the selected colonies were [psi] and could not grow on $-$ Ade medium (Table 4). To determine ifthe rare [PSI⁺] Ura⁺ haploids that carried plasmid pSSA1-LEU2 contained the hsp104::URA3deletion, proteins were examined by Western blotting. All sixcolonies tested expressed full-length Hsp104 protein (Fig. 3).Presumably, these originated from meiotic gene conversion of theura3 marker. Thus, a multicopy SSA1 plasmid cannot produce nonsensesuppression in cells carrying an hsp104 deletion.

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TABLE 4. Analysis of the meiotic progeny of HSP104⁺/hsp104::URA3 diploids

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FIG. 3. Western analysis of the exceptional Ura⁺ [PSI⁺] spore clones from the diploids heterozygous by hsp104::URA3 disruption. Proteins were isolated from six exceptional Ura⁺ [PSI⁺] spore clones, obtained in the meiotic progeny of the diploids GT1-S31 × L-1607 and GT56-13B × L-1607, which bear plasmid pSSA1-LEU2 (lanes 1 to 6), and control hsp104 deletion strain L-1607. Extracts were subjected to SDS-PAGE, transferred onto a nitrocellulose filter, and reacted to Hsp104-specific antibodies. All extracts contained similar amounts of the total cellular protein as verified by Coomassie blue staining (not shown).

Effects of excess Ssa1 protein on Hsp104-mediated thermotolerance. Next, we tested whether Ssa1 would interfere with the other known function of Hsp104. Hsp104 is a stress tolerance factorthat greatly increases survival in yeast cells exposed to hightemperatures (40, 41). This activity of Hsp104 correlateswith its ability to promote the solubilization of aggregated proteinsdamaged by heat (34). In the absence of Hsp104, excess Ssa1protein partially compensates for the temperature tolerance defect(42). Moreover, Ssa1 protein cooperates with Hsp104 in the reactivationof aggregated proteins in vitro (17). Ssa proteins appear tohave at least two roles in stress tolerance: they bind unfoldedproteins, reducing their tendency to aggregate, and they assistin the Hsp104-mediated reactivation of proteins that have alreadyaggregated. We investigated the effects of Ssa1 on the basal andinducible thermotolerance of yeast cells that contained variouslevels of Hsp104. Exponentially growing cells were grown at 25°C,the conditions under which effects on [PSI]-mediated suppressionwere analyzed. The cells were then shifted directly to 50°C tomeasure basal thermotolerance. An hsp104 deletion derivative ofOT46 carrying control vectors was extremely sensitive to a 50°Cheat shock: only 0.01% of the cells were alive after a 10-minexposure (Fig. 4A). Under the same conditions, the viability ofisogenic strains containing either the multicopy SSA1 plasmidor the low-copy-number HSP104 plasmid was higher, roughly 50-or 1,000-fold, respectively. Thus, as previously described (30,40-42), both the HSP104 gene and multiple copies of the SSA1 geneare able to protect yeast cells against temperature-induced killing,and the effect of HSP104 is much stronger than that of SSA1. However,the OT46 transformant, which contained both multiple copies ofSSA1 and a low-copy-number HSP104 plasmid, was about 15-fold lessviable after 10 min at 50°C and about 3-fold less viable after5 min at 50°C than the isogenic transformant containing HSP104alone (Fig. 4A). Thus, multiple copies of SSA1 interfere withthe temperature tolerance provided by Hsp104.

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FIG. 4. Effects of Ssa1 and Hsp104 on temperature tolerance of yeast cells. Temperature tolerance assays were performed as described in Materials and Methods. Plasmid designations are the same as in Fig. 1. Experiments were repeated twice (A) or four times (B) with similar results.

The same experiment was performed with strain OT56, which contains an intact chromosomal copy of the HSP104 gene (qualitativeresults in Fig. 4B; quantitative results not shown). Additionof the single extra copy of HSP104 increased the temperature resistanceof OT56. Interestingly, our results indicate that strain OT56,carrying a single chromosomal copy of HSP104, is less resistantto 50°C treatment than strain OT46, carrying the HSP104 gene onthe centromeric plasmid. This is likely because the plasmid-borneHSP104 gene yields higher constitutive expression than the chromosomalgene (reference 5 and Fig. 1). Temperature protection by multiplecopies of SSA1 was not detected in OT56. However, the OT56 transformantcontaining both multiple copies of SSA1 and a single extra copyof HSP104 was less temperature resistant than one containing HSP104alone, confirming an inhibitory effect of Ssa1 on basal thermotolerancein cells expressingHsp104.

When OT46 and OT56 cultures were preincubated at 37°C to induce thermotolerance, the temperature resistance of all transformantscontaining HSP104 was greatly increased at 50°C, as reported previouslyfor the other yeast strains (40, 41). Under these conditions,multiple copies of SSA1 did not affect temperature resistanceof the strains containing the HSP104 plasmid as strongly as theydid in the absence of the 37°C pretreatment. We detected an Hsp104-antagonizingeffect of SSA1 only twice in four such experiments (data not shown).We also examined the temperature resistance of OT56 transformantsbearing the galactose-inducible GAL::SSA1 and/or GAL::HSP104 plasmids.Again, GAL::HSP104 conferred temperature resistance to cells growingin galactose medium, independently of the GAL::SSA1 plasmid (datanot shown). Apparently, excess Ssa1 protein interferes with Hsp104-mediatedtemperature tolerance only under some culture conditions. Thismay depend on both levels of Hsp104 induction and the effectsof other factors induced by temperature pretreatment or growthongalactose.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

We have shown that at least one of the proteins of the Hsp70 family, Ssa1, is able to protect the prion-like genetic elementknown as [PSI] from Hsp104-induced curing. This helps to resolvea major paradox concerning the inheritance of [PSI]. Transientselective overproduction of Hsp104 is sufficient to eliminatethe [PSI] element (5), providing one of the strongest geneticarguments that [PSI] represents a new type of inheritance basedupon the transmission of proteins with alternative, self-perpetuatingstructures. However, if Hsp104 is the only factor controlling[PSI], the [PSI] element should be lost during growth at hightemperatures or in stationary phase, when Hsp104 levels increase.Since Ssa levels are also increased under these conditions, ourresults provide a likely explanation for ability of genetic informationcarried by [PSI] to be preserved in the face of environmentalfluctuations.

The Ssa Hsp70 subfamily includes, in addition to Ssa1, the Ssa2, Ssa3, and Ssa4 proteins (47, 51, 52). These proteinsexhibit different patterns of expression. For example, while Ssa2is expressed at a high constitutive level in exponential cells,Ssa1 expression is increased at high temperatures, and Ssa3 andSsa4 are normally expressed only at high temperatures. Duringstationary-phase growth, on the other hand, Ssa3 is the most stronglyinduced (51). These proteins are highly homologous and havestrongly overlapping functions in other protein-folding processes.Thus, any or all of them is likely to play a role in the maintenanceof [PSI], depending on the particular environmental conditions.Determining with certainty which (if any) members of the familypreferentially effect [PSI⁺] will not be easy in vivo. We have constructed several [PSI⁺] strains bearing multiple ssa deletions (ssa1,3, ssa1,2,3, andssa1,3,4) in various genetic backgrounds. In some (but not all)of these multiple-deletion strains, frequencies of [PSI] lossduring growth at 37°C were increased markedly (e.g., loss in 5to 20% of cells, compared to less than 0.5% at 25°C) (7). However,Western blots revealed that multiple ssa deletion strains stillcontain near wild-type levels of Ssa protein. This result is apparentlydue to compensatory induction of the remaining member(s) of SSAfamily in the cells bearing multiple ssa deletions, as describedpreviously (1, 56). Simultaneous inactivation of all fourSSA genes is lethal (52). Therefore, it is not yet possibleto tell whether Ssa is the only factor protecting [PSI] from Hsp104during growth at high temperature and whether Ssa is requiredfor [PSI] maintenance in the normal conditions. Moreover, Hsp70proteins regulate not only their own expression but also thatof many other protein-folding agents, including other Hsps (12)and trehalose (19). We have shown that at least one of these,Hsp82 (a yeast homolog of the mammalian Hsp90) does not play animportant role in [PSI] maintenance. However, we do not know whetherSsa1's affects on [PSI] are an indirect consequence of its positionin these regulatory circuits or direct consequence of interactionwith Sup35, the protein determinant of [PSI].

Previous results suggest that Ssa protein does not influence Sup35 secondary structure in vitro (43). However, this doesnot rule out a possibility of direct interaction between Ssa andSup35, which would not have a major effect on the secondary structure.In vivo interaction could also be assisted by other proteins,which are not present in vitro. It is also possible that Ssa couldspecifically recognize a prion isoform of the Sup35. Further experimentsto determine whether there are specific in vivo interactions betweenSsa and Sup35 are underway.

Ssa1 and Hsp104 functions also interface in another realm, providing cells with tolerance to heat stress. In vivo, Ssa1 overproductionpartially compensates for the loss of temperature tolerance inthe absence of Hsp104 (reference 42 and confirmed herein). Moreover,whereas Hsp104 is dispensable for growth at all temperatures ina wild-type background, it is essential for growth at high temperatureswhen Ssa protein levels are reduced (42). Hsp104 functions instress tolerance as a "molecular crowbar," promoting the resolubilizationof heat-damaged proteins (34). In vitro work points to two differentroles for Ssa in stress tolerance. First, it binds unfolded proteinsand prevents them from aggregating, reducing the requirement forHsp104's disaggregating function. Second, together with anotherchaperone, Ydj1, Ssa1 helps previously aggregated proteins, targetsof Hsp104's disaggregating function, return to the folded state(17). Our finding that overexpressing Ssa1 during log-phasegrowth on glucose interferes with Hsp104's thermotolerance functionswhen cells are shifted directly to high temperatures (Fig. 4)was, therefore, unexpected. There are two likelyexplanations.

First, at certain chaperone concentrations and/or with certain substrates, Ssa might interfere with Hsp104's resolubilizingactivity. It might do so either by binding directly to substratesand preventing Hsp104's interaction with them or by titratingthe free cellular concentration of Hsp104 cofactors, such as Ydj1.This same mechanism might account for Ssa1's ability to interferewith Hsp104-mediated curing of [PSI]. That is, Hsp104 might curecells of [PSI] simply by disaggregating previously aggregatedSup35, and Ssa1 might interfere with this disaggregation. Indeed,we find that a greater fraction of Sup35 remains in the pelletafter lysate fractionation in cells that overexpress both Ssa1and Hsp104 than in cells that overexpress Hsp104 alone (Fig. 1and 2). However, we also find that under some conditions (forexample, after a temperature pretreatment), Ssa1 overexpressiondoes not significantly interfere with Hsp104-mediated thermotolerance.If it is Ssa's interference with Hsp104 mediated [PSI] curingthat saves the [PSI] elements during heat shock, some aspect ofSsa's effects on Sup35 aggregates and heat-damaged aggregateswould have to diverge under these conditions. An attractive possibilityis that while Ssa is assisting Hsp104 in solubilizing the amorphousaggregates, it protects highly ordered protein complexes (e.g.,cytoskeletal networks) from the disassembling effect of the stress-inducedHsp104. This would explain why Hsp104 normally has no effect oncytoskeletal structures. Prion polymers, which resemble some patternsof the highly ordered structures, could also be protected by Ssato some extent. Indeed, mammalian Hsp70 proteins were shown toprotect some cytoskeletal components (in particular, the centrosomeand intermediate filaments) during heat shock (27).

A second explanation for Ssa1's interference with Hsp104-mediated thermotolerance in log-phase cells shifted to high temperaturesis that it acts indirectly, down regulating the basal expressionof other thermotolerance or growth factors. Conditioning preheattreatments, by recruiting Ssa proteins away from regulatory factors(11), would derepress these factors and restore full thermotolerance.These other factors might also interact with Sup35 protein andinfluence its folding transitions during heat shock and stationary-phasegrowth, but the specific roles of these factors and the natureof their interaction with Sup35 is unclear. Indeed, the molecularmechanisms of Hsp104's effects on [PSI] and Sup35 themselves remainto be uncovered. The surprising observation that both overexpressionand inactivation of Hsp104 can cure cells of [PSI] has been explainedby role of Hsp104 in forming of partially unfolded conversionintermediate (5), by stochiometric interaction between suchan intermediate and Hsp104 hexamer (35), or by ability of Hsp104to promote [PSI] segregation by breaking down huge aggregatesinto the small aggregation "seeds" (36). However, none of thesemodels have been directly tested due to inherent difficultiesof the analysis of aggregation-prone substrates invitro.

The remarkable hypothesis that a heritable phenotypic change in yeast could be transmitted by a heritable change in proteinstructure, with no underlying change in a nucleic acid, was firstproposed in 1994 (53). Since then a great deal of genetic, cellbiological, and biochemical data has provided compelling support.We are still a long way from understanding the specific physicalmechanisms that promote the underlying changes in protein state.However, we are now beginning to appreciate the complexity withwhich the [PSI] factor interfaces with the biology of yeast cells.We have now linked the expression of a second major yeast chaperone,a member of the evolutionarily conserved Hsp70 chaperone familywhose expression changes in response to the environment, to theforces that control [PSI] inheritance. Therefore, one group ofchaperone proteins plays a major role in both adaptation to thetemperature stress and control of prion maintenance. This findingprovides a framework for discovering how [PSI] is maintained inthe face of environmental fluctuations. Moreover, further understandingof [PSI] propagation will serve as a powerful tool of investigatingthe molecular pathways by which cells respond to environmentalchanges. The question arises: Is [PSI] a beneficial factor thathas prompted the evolution of mechanisms for its maintenance underdiverse conditions? Or has [PSI], like viruses and transposableelements, learned to take advantage of complex regulatory mechanismsin the cell to promote its ownpropagation?

	ACKNOWLEDGMENTS

We are grateful to A. D. Zink for help in performing the temperature resistance assays. We thank E. Craig for the Ssa-specificantibodies and M. Tuite for the gift of plasmids pUKC815 andpUKC819.

This work was supported by the grant 1R21GM55091 from the National Institute of General Medical Sciences to Y.O.C. and byHoward Hughes Medical Institute funds to S.L.L.

	FOOTNOTES

^* Corresponding author. Mailing address: School of Biology, Georgia Institute of Technology, 310 Ferst Dr., Room 303, Atlanta,GA 30332-0230. Phone: (404) 894-1157. Fax: (404) 894-0519. E-mail:yc22{at}prism.gatech.edu.

REFERENCES

Top
Abstract
Introduction
Materials and methods
Results
Discussion
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