Yeast Exosome Mutants Accumulate 3'-Extended Polyadenylated Forms of U4 Small Nuclear RNA and Small Nucleolar RNAs

doi:10.1128/MCB.20.2.441-452.2000

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Molecular and Cellular Biology, January 2000, p. 441-452, Vol. 20, No. 2
0270-7306/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Yeast Exosome Mutants Accumulate 3'-Extended Polyadenylated Forms of U4 Small Nuclear RNA and Small Nucleolar RNAs

Ambro van Hoof, Pascal Lennertz, and Roy Parker^*

Department of Molecular and Cellular Biology, Howard Hughes Medical Institute, University of Arizona, Tucson, Arizona 85721

Received 16 August 1999/Returned for modification 30 September 1999/Accepted 8 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The exosome is a protein complex consisting of a variety of 3'-to-5' exonucleases that functions both in 3'-to-5' trimmingof rRNA precursors and in 3'-to-5' degradation of mRNA. To determineadditional exosome functions, we examined the processing of avariety of RNAs, including tRNAs, small nuclear RNAs (snRNAs),small nucleolar RNAs (snoRNAs), RNase P, RNase MRP, and SRP RNAs,and 5S rRNAs in mutants defective in either the core componentsof the exosome or in other proteins required for exosome function.These experiments led to three important conclusions. First, exosomemutants accumulate 3'-extended forms of the U4 snRNA and a widevariety of snoRNAs, including snoRNAs that are independently transcribedor intron derived. This finding suggests that the exosome functionsin the 3' end processing of these species. Second, in exosomemutants, transcripts for U4 snRNA and independently transcribedsnoRNAs accumulate as 3'-extended polyadenylated species, suggestingthat the exosome is required to process these 3'-extended transcripts.Third, processing of 5.8S rRNA, snRNA, and snoRNA by the exosomeis affected by mutations of the nuclear proteins Rrp6p and Mtr4p,whereas mRNA degradation by the exosome required Ski2p and wasnot affected by mutations in RRP6 or MTR4. This finding suggeststhat the cytoplasmic and nuclear forms of the exosome representtwo functionally different complexes involved in distinct 3'-to-5'processing and degradationreactions.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The production of a wide variety of RNA species in eukaryotic cells requires specific 3' trimming reactions. Such reactionsoccur in the processing of a diversity of primary transcripts,including those produced by RNA polymerase I, 5.8S rRNA, 18S rRNA,and 25S rRNA (reviewed in reference 35); those produced by RNApolymerase II, including both small nuclear RNAs (snRNAs) andsmall nucleolar RNAs (snoRNAs); and transcripts produced by RNApolymerase III, including tRNAs (reviewed in reference 10) and5S rRNA (33). This diversity of substrates raises the issueof how each unique RNA is properly processed to generate a specificmature 3' end. In addition, mRNAs are subjected to a variety of3' trimming events, including a specific-length trimming of thepoly(A) tail (3), cytoplasmic deadenylation of the mRNA (reviewedin reference 14), and eventual 3'-to-5' degradation of the bodyof the transcript in the cytoplasm (23, 24). An unresolvedquestion is whether these different 3' trimming reactions arecarried out by a few relatively general 3'-to-5' exonucleases,or if there are a large number of specific nucleases that eachact on limited subsets ofsubstrates.

Recent observations have suggested that at least two distinct 3'-to-5' exonucleolytic processing events are performed by thesame exonuclease complex. This is based on the identificationof a multiprotein complex, termed the exosome, that contains atleast 10 different polypeptides that have been shown to be 3'-to-5'exonucleases or have sequence similarity to known 3'-to-5' exonucleases(1, 22). More important, this complex has been shown to berequired both for the 3' processing of 5.8S rRNA in the nucleolus(22) and for the 3'-to-5' pathway of mRNA degradation in thecytoplasm (13). Interestingly, these two different processingreactions appear to require additional proteins that are specificfor each reaction. For example, although 3'-to-5' degradationof mRNA requires Ski2p, Ski3p, and Ski8p, these Ski proteins arenot required for 5.8S rRNA processing (13). Conversely, theSki2p-related protein Mtr4p is known to be required for 5.8S rRNAprocessing (9). Since both Ski2p and Mtr4p are members of theDEVH box family of putative RNA helicases, an appealing modelis that these proteins function in different exosome-mediatedreactions, although it is not known whether Mtr4p also functionsin cytoplasmic mRNAdecay.

Since the components of the exosome are highly conserved and found in both the cytoplasm and the nucleus (1, 37), itwas likely that this complex would have additional roles in 3'-to-5'RNA processing and/or degradation. To identify such roles, wehave systematically screened a number of Saccharomyces cerevisiaemutants defective in exosome function. Mutants impaired in thefunctioning of the nuclear exosome accumulate 3'-extended polyadenylatedforms of U4 snRNA and independently transcribed snoRNAs and showalterations in snoRNAs produced from introns or polycistronictranscripts. This finding suggests that the exosome is involvedin processing of these 3'-extended species. In addition, mutationsin the nuclear proteins Rrp6p and Mtr4p affected processing of5.8S rRNA (2, 9), snRNA, and snoRNA by the exosome. In contrast,mRNA degradation by the exosome required Ski2p, Ski3p, and Ski8pand was not affected by mutations in RRP6 or MTR4. This findingsuggests that the cytoplasmic and nuclear forms of the exosomerepresent two functionally different complexes involved in 3'-to-5'processing and degradationreactions.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains and plasmids. The genotypes of the S. cerevisiae strains used are given in Table 1. All but three strains are completely isogenic to eachother; the exceptions are yRP1379, yRP1223, and yRP1381, whichare partially isogenic as described below.

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TABLE 1. Strains used in this study

The rrp6 $Delta$ strain was made by crossing yRP840 and yRP841. One copy of the RRP6 gene of the resulting diploid (yRP1375) wasdeleted and replaced by a URA3 marker by transformation with theSacI-to-ClaI fragment of pRP950, resulting in yRP1376. Successfulgene disruption was confirmed by Southern analysis. Tetrads fromyRP1376 were dissected to yield yRP1377. Spores were scored forrrp6 $Delta$ by their slow-growth phenotype and uracil autotrophy. pRP950is a pBluescript SK+ derivative which contains positions $-$ 915to $-$ 15 relative to the AUG codon of RRP6, the URA3 marker, andpositions +82 to +727 relative to the stop codon of RRP6. Thisplasmid was constructed by amplifying these regions from totalgenomic DNA by using oligonucleotides containing restriction enzymerecognition sequences (XbaI, SacII, XhoI, and XmaI, respectively),and cloning the resulting PCR products into pRP312. pRP312 isa pBluescript SK+ derivative that contains the URA3 gene insertedinto the BamHIsite.

yRP1379 was made by crossing strain T208 (a generous gift from Alan M. Tartakoff) to yRP840. Spores were scored for the mtr3-1mutation by their temperaturesensitivity.

Strain yRP1380 was made by crossing yRP686 and yRP687. One copy of the MTR4 gene in the resulting diploid was knocked outby using plasmid pDM (19). Successful gene disruption was confirmedby Southern analysis. The resulting diploid was transformed withplasmid pRM(ts) (19), which carries the mtr4-1 allele on pRS316(32). The resulting diploid was dissected, and spores were scoredfor mtr4::LEU2 by autotrophy and inability to grow on plates containing5-fluoro-orotic acid, for mtr4-1 by the URA3 marker on the plasmid,by temperature-sensitive growth phenotype, and by 5.8S rRNA processingdefect. The resulting strain (yRP1378) was crossed to yRP841,and spores were scored for mtr4-1 as before and for the CUP1::LEU2PM(11a) insert by Northernblotting.

Strain yRP1381 was made by crossing strain yRP1377 to yRP851. yRP851 was made by backcrossing the pap1-1 mutation (25) intothe yRP840 background multiple times. The diploid was dissected,and the double mutant was scored by its uracil autotrophy andpap1-1 temperature-sensitive growth, which was partially suppressedby rrp6 $Delta$ as previously reported (2).

An rnt1 $Delta$ strain was constructed in the yrp840 strain background by amplifying an rnt1 $Delta$ ::Neo^r cassette from a strain obtained from Research Genetics (recordnumber 20825). The PCR product was used to transform the diploidstrain yRP1376, which is heterozygous for rrp6 $Delta$ ::URA3 (see above),and neomycin-resistant colonies were selected. Successful genedeletion was confirmed by Southern analysis. Tetrads from onesuch rnt1 deletion were dissected, and resulting strains werescored for neomycin resistance, uracil autotrophy, and RNA phenotypes.Two complete tetrads that contained all four possible combinationswere analyzed. One of these tetrads yielded strains yRP1416 toyRP1419 and isshown.

RNA extraction and Northern blotting. All yeast strains were grown in standard yeast extract-peptone (YEP) containing 2% galactose or 2% glucose. Strains carryinga deletion of a nonessential gene were grown at 30°C to an opticaldensity at 600 nm of 0.3 to 0.5, and strains carrying a temperature-sensitivemutation were grown similarly at 24°C (a temperature permissivefor all mutations used), followed by incubation for 1 h at 37°C(a temperature restrictive for all mutationsused).

RNA was extracted, cleaved with RNase H, separated on agarose or polyacrylamide gels, transferred, and probed as describedby Jacobs Anderson and Parker (13). Sequences of oligonucleotidesused as probes are given in Table 2.

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TABLE 2. Oligonucleotides used in this study

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Experimental approach. To identify additional functions for the exosome complex, we created a collection of eight strains carrying mutations in differentcomponents of the exosome, or in the proteins related to exosomefunction (Table 3), and then examined a diversity of 3'-to-5'processing reactions in that collection of strains. Three strainsthat contained conditional temperature-sensitive alleles in corecomponents of the exosome (i.e., rrp4-1, ski6-100, and mtr3-1)were used. These core components are thought to be subunits ofboth the nuclear and the cytoplasmic exosome (1) and are allessential. In addition, a strain carrying a deletion of RRP6 wasexamined. Rrp6p is an exonuclease associated with the exosomein nuclear fractions (1), and rrp6 $Delta$ strains have a defect in5.8S rRNA maturation (2). A temperature-sensitive mtr4-1 strainwas also included. Mtr4p is an essential protein required for5.8S rRNA processing by the exosome (9). Last, strains withdeletions of the nonessential SKI2, SKI3, and SKI8 genes wereexamined. These three genes are known to be required for exosome-mediated3'-to-5' degradation of mRNA (13).

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TABLE 3. Mutants used in this study

Yeast strains containing a deletion of a nonessential gene (SKI2, SKI3, SKI8, or RRP6) were grown at 30°C. Therefore, thepool of stable RNA in these strains represent a steady-state condition.In contrast, yeast strains containing conditional mutations inessential genes (RRP4, SKI6, MTR3, and MTR4) were grown at 24°C(a temperature permissive for growth) and shifted to 37°C (a temperaturerestrictive for growth) for 1 h. A relatively short shift to therestrictive temperature was used to minimize the occurrence ofsecondary effects. As a consequence, the pool of stable RNA presentis a mixture of RNA synthesized during growth at the permissivetemperature and RNA synthesized at the restrictive temperature.A wild-type strain was grown under both conditions. Total RNAfrom wild-type and mutant strains was analyzed by Northern blottingusing oligonucleotide probes for a wide variety of RNA species.These included rRNA, tRNA, mRNA, snRNA, snoRNA, and the RNA subunitsof SRP and RNases P and MRP. This collection of RNAs includesspecies transcribed by all three RNA polymerases and includestranscripts previously suggested to be processed from 3'-extendedprecursors, transcripts whose mature 3' end appears to match thepolymerase termination signal, and species for which little, ifanything, is known about 3' endformation.

Importantly, as detailed below, examination of U4 snRNA and snoRNAs revealed several alterations in these transcripts in theski6-100, rrp4-1, rrp6 $Delta$ , mtr3-1, and mtr4-1 mutant strains butnot in the ski2 $Delta$ , ski3 $Delta$ , or ski8 $Delta$ strains. In contrast, to datewe have not found obvious defects in the processing of many otherRNAs, including 5S rRNA, several tRNAs, and the RNA subunits ofSRP and RNases MRP and P in any of the mutant strains examined(data not shown). This observation is consistent with these particularRNA species having mature 3' ends that are formed by transcriptionaltermination, by processing by other 3'-to-5' exonucleases (A.van Hoof, P. Lennertz, and R. Parker, unpublished data), or byredundancy of the exosome with other exonucleases for these functions.In either case, these results serve as negative controls thatindicate that the defects described below are specific to U4 snRNAandsnoRNAs.

Exosome mutants accumulate 3'-extended forms of snoRNAs and U4 snRNA. (i) The exosome is involved in the processing of independently transcribed snoRNAs and U4 snRNA. snoRNAs are produced from independent transcripts, excised introns, or polycistronic transcripts (reviewed in references 20and 34). To examine the role of the exosome in the processingof independently transcribed snoRNAs, we examined a member ofeach of the two major classes of snoRNAs (Table 2). snoRNAs canstructurally and functionally be divided into C/D box-containingsnoRNAs, required for methylation of the 2' hydroxyl of RNA, andH/ACA box-containing snoRNAs, required for pseudouridyl formationin rRNA. For each class, we examined one snoRNA transcribed froman independent transcription unit. For the C/D box-containingsnoRNAs, we examined snR40; for the H/ACA box-containing snoRNAs,we examinedsnR33.

Two sets of observations suggest that the exosome is involved in the processing of 3'-extended forms of snR33 and snR40. First,in rrp6 $Delta$ strains, the majority of snR33 and snR40 RNA specieswere longer by a few nucleotides (Fig. 1A and C, lower panels).This observation suggested that the exosome, and perhaps Rrp6pspecifically, is involved in the removal of the last few 3' nucleotides,to give rise to the mature 3' end of these RNAs. The second alterationwas that rrp6 $Delta$ , mtr4-1, ski6-100, mtr3-1, and rrp4-1 mutant strainsall accumulated longer heterogeneous forms of the snR33 and snR40transcripts (Fig. 1A and C, top panels). Hybridization of a Northernblot containing RNA from wild-type and rrp6 $Delta$ strains with a probedesigned to hybridize 3' of the mature snR33 showed that the heterogeneouspopulation seen in Fig. 1A represents 3'-extended forms of snR33(Fig. 1B). These observations suggest that snR33 and snR40 aremade as 3'-extended forms that are then processed in a mannerrequiring the exosome (see below).

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FIG. 1. Exosome mutants have defects in processing of independently transcribed snoRNAs and U4 snRNA. Shown are two different exposures of the same Northern blots containing RNA from the indicated strains. All strains were grown in YEP-2% galactose to early to mid-log phase. The ski2 $Delta$ , ski3 $Delta$ , ski8 $Delta$ , and rrp6 $Delta$ strains were grown at 30°C. The ski6-100, rrp4-1, mtr3-1, and mtr4-1 strains were grown at 24°C and incubated for an additional hour at 37°C. Blots were probed for snR33 (A), 3'-extended snR33 (B), snR40 (C), U4 snRNA (D), or 3'-extended U4 snRNA (E). The species of 240 and 212 nt seen in panel C likely represent 5' processing intermediates as recently proposed (5). wt, wild type. Positions of size markers (lanes M) are given in nucleotides.

Mutations affecting exosome function, especially mtr4-1, mtr3-1, ski6-100, and rrp4-1, led to only modest accumulation ofthe heterogeneous 3'-extended forms of snoRNAs. However, thesedefects are likely to be biologically significant for four reasons.First, snoRNAs are thought to be stable, and thus the pool ofsnoRNAs in a temperature-sensitive mutant after 1 h at the restrictivetemperature reflects mostly RNA produced before the shift to therestrictive conditions. Second, the defects seen here are similarin strength to those seen in rRNA processing and mRNA degradationin the same mutants. For example, mutations in RRP4 or MTR4 ledto only modest increases in 3'-extended 5.8S rRNA, which weredetected only by long exposures or with use of probes designednot to hybridize to the mature RNA (9, 22). Third, the defectsseen here are similar in strength to defects in snoRNA 5' processingin a rat1-1 xrn1 $Delta$ double mutant. This mutant accumulates low levelsof 5'-extended forms of snR190, U14, U24, and U18 snoRNAs aftera 2-h incubation at the restrictive temperature (27), some ofwhich were shown to exist only by using probes specific for 5'-extendedforms. Fourth, reproducible accumulation of heterogeneous 3'-extendedspecies were seen for six different snoRNAs from different classes(seebelow).

Analysis of the independently transcribed U4 snRNA revealed results similar to but distinct from those for snR33 and snR40.Wild-type strains accumulated a mature U4 species of 160 nucleotides(nt) and 3'-extended forms of between 270 and 300 nt. In addition,rrp6 $Delta$ , mtr3-1, mtr4-1, ski6-100, and rrp4-1 strains accumulatedRNA species intermediate in size between the mature species andthe 270- to 300-nt species. A heterogeneous population of transcriptswas also seen in the rrp6 $Delta$ strain extending above the 270- to300-nt precursor (Fig. 1D). The use of a specific oligonucleotideprobe 3' of the mature 3' end of the U4 RNA showed that thesespecies were extended on the 3' side of the RNA (Fig. 1E). Thesedata suggest that the exosome is involved in the processing ofthe 3'-extended forms of U4snRNA.

(ii) The exosome is involved in the processing of intron-derived snoRNAs. To determine if the exosome functions in the processing of intron-derived snoRNAs, we examined a member of each of the twomajor classes of snoRNAs. For the C/D box-containing snoRNAs,we examined U24; for the H/ACA box-containing snoRNAs, we examinedsnR44.

Intron-derived snoRNAs also showed altered patterns of accumulation in the various strains examined. First, for U24 in therrp6 $Delta$ strain, the predominant RNA species was slightly largerthan the normal RNA (Fig. 2A). This observation is similar tothat noted above for the independently transcribed snoRNAs snR33and snR40, and it suggests that the exosome, and perhaps Rrp6pspecifically, is involved in the removal of the last few nucleotidesto give rise to the mature 3' end of these transcripts. Second,we observed a slight but reproducible reduction in the level ofsnR44 in the various mutants. The residual snR44 levels variedfrom 10% of the wild-type level in the rrp6 $Delta$ strain to 75% forthe mtr4-1 strain (Fig. 2B). Less drastic reductions were seenfor the level of U24 in various exosome mutants (Fig. 2A). Onepossible interpretation of these observations is that in the absenceof proper 3'-to-5' trimming, snR44 is degraded.

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FIG. 2. Exosome mutants have defects in processing of intron-derived snoRNAs. Shown are Northern blots containing RNA from the indicated strains. All strains were grown in YEP-2% galactose to early to mid-log phase. The ski2 $Delta$ , ski3 $Delta$ , ski8 $Delta$ , and rrp6 $Delta$ strains were grown at 30°C. The ski6-100, rrp4-1, mtr3-1, and mtr4-1 strains were grown at 24°C and incubated for an additional hour at 37°C. Blots were probed for U24 (A), snR44 (B), U18 (C), or 3'-extended U18 (D). In panel C, two different exposures of the same Northern blot are shown. wt, wild type. Positions of size markers (lanes M) are given in nucleotides.

We also examined the effects of exosome mutations on the processing of the U18 snoRNA. This snoRNA is embedded within theintron of the EFB1 gene, but it has been shown to be processedby two different pathways (36). In one pathway, it is processedfrom an intron released from the EFB1 pre-mRNA; in the other pathway,it is processed from the primary transcript in a manner that doesnot require splicing. Thus, this snoRNA does not fit neatly ineither the intron-derived or the independently transcribed snoRNAclass.

The defects seen for U18 snoRNA were similar to those seen for other snoRNAs. First, the rrp6 $Delta$ strain primarily accumulateda U18 RNA that was slightly larger than normal, as well as a heterogeneouspopulation of larger species. A strain containing the mtr3-1 mutation(and possibly mtr4-1, ski6-100, and rrp4-1 strains) accumulatedlow levels of heterogeneous species of 200 to 300 nt (Fig. 2C).Probing of a Northern blot with RNA from wild-type and rrp6 $Delta$ strainswith an oligonucleotide probe 3' of the mature 3' end of the U18snoRNA showed that the heterogeneous species in rrp6 $Delta$ were extendedon the 3' side of the RNA (Fig. 2D). The observation that essentiallyno mature U18 accumulates in an rrp6 $Delta$ strain suggests that bothpathways of U18 maturation are affected. Based on the defectsseen in rrp6 $Delta$ , combined with the slight defects seen in otherexosome mutants, we conclude that Rrp6p, and presumably also thecore exosome, is involved in both pathways of U18processing.

The exosome is involved in the processing of polycistronic snoRNAs. To examine the role of the exosome in the processing of polycistronic snoRNAs, we examined two polycistronic precursors. Onetranscript examined contains snR190 and U14 C/D box-containingsnoRNAs, with U14 being the 3' snoRNA (6). The second polycistronictranscript examined contains seven C/D box-containing snoRNAs,in the 5'-to-3' order of snR78, snR77, snR76, snR75, snR74, snR73,and snR72 (28). No H/ACA box-containing snoRNAs derived frompolycistronic transcripts have been described todate.

Exosome mutants showed two distinct defects in the processing of snoRNAs from polycistronic precursors. Similar to what wasseen with other snoRNAs, the rrp6 $Delta$ strain accumulated slightlylarger than normal transcripts for U14, snR73, and snR72 (Fig.3B to D, lower panels). No difference was seen for snR190 (Fig.3A), but a difference of one or a few nucleotides might not beresolved, due to the relatively large size of this snoRNA. WhilesnR33 is similar in size to snR190, we were able to detect aneffect of rrp6 $Delta$ on snR33; thus, if rrp6 $Delta$ results in a larger snR190,this size difference must be smaller than the corresponding sizedifference for snR33. In addition to this effect, rrp6 $Delta$ , mtr3,mtr4, ski6, and rrp4 mutant strains accumulated heterogeneouspopulations of RNAs that were 3'-extended forms of U14, snR73,and possibly snR72 but not of snR190 (Fig. 3). These data, combinedwith the defects seen for independently transcribed and intron-derivedsnoRNAs, suggest that the exosome is involved in the processingof 3'-extended snoRNAs, irrespective of whether they are derivedfrom independent transcripts, introns, or polycistronic transcripts.

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FIG. 3. Exosome mutants have defects in processing of polycistronic snoRNAs. Shown are two different exposures of the same Northern blots containing RNA from the indicated strains. All strains were grown in YEP-2% galactose to early to mid-log phase. The ski2 $Delta$ , ski3 $Delta$ , ski8 $Delta$ , and rrp6 $Delta$ strains were grown at 30°C. The ski6-100, rrp4-1, mtr3-1, and mtr4-1 strains were grown at 24°C and incubated for an additional hour at 37°C. Blots were probed for snR190 (A), U14 (B), snR73 (C), snR72 (D), 3'-extended U14 (E), 3'-extended snR73 (F), or 3'-extended snR72 (G). The species of 385 nt seen in panels A and B likely represents a dicistronic precursor, while the species of 184 nt seen in panel B likely represents U14 that contains a 5' extension but carries the mature 3' end. Based on known Rnt1p cleavage sites, the 238-nt species seen in panels C and F likely represents snR73 that has been released from its precursor but carries 5' and 3' extensions. wt, wild type. Positions of size markers (lanes M) are given in nucleotides.

Exosome mutants accumulate polyadenylated forms of U4 snRNA and some snoRNAs. In the rrp6 $Delta$ mutant and in several of the other exosome mutant strains, we observed a larger heterogeneous population of transcriptsderived from U4 snRNA and snR33, snR40, U18, U14, snR73, and snR72snoRNAs. The simplest explanation is that this population representsa pool of polyadenylated RNAs with poly(A) tails varying in length.To examine this possibility, two experiments were performed. First,RNAs from different mutant strains and a wild-type strain weretreated with RNase H in the presence of oligo(dT). RNase H cleavesRNA in a RNA-DNA duplex and is commonly used in combination witholigo(dT) to remove poly(A) tails in vitro. The products of theseRNase H reactions were analyzed by probing a Northern blot forsnR33. An important observation was that following treatment withRNase H and oligo(dT), the heterogeneous population migrated fasterin the gel. Since the largest stretch of A's encoded in the correspondingregion of the genome (three A's) is not long enough to efficientlyhybridize to oligo(dT), this RNase H induced shift is not causedby a stretch of encoded A's and thus must be the result of a poly(A)tail. Removal of the poly(A) tail by RNase H treatment did notresult in one discrete band, presumably because the poly(A) tailin individual molecules was added at different sites. This issimilar to what occurs with mRNAs. For example, Graber et al.(11) recently analyzed 1,352 unique mRNA 3' ends, which theyfound to be derived from 861 genes. Thus, even in this small sample,the average number of 3' ends per gene was 1.6, indicating thatmany genes produce mRNAs with alternative 3' ends. Our resultsindicate that the heterogeneous population seen in untreated samplescorresponded to polyadenylated snoRNAs. These polyadenylated snR33species are present at low levels in the wild type (Fig. 4A),and these levels are elevated in at least four strains carryingexosome mutations (Fig. 4B).

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FIG. 4. Wild-type and exosome mutant strains accumulate polyadenylated snR33. Shown is a Northern blot containing RNA from the indicated strains. All strains were grown in YEP-2% galactose to early to mid-log phase. The rrp6 $Delta$ strain was grown at 30°C. The ski6-100, mtr3-1, and mtr4-1 strains were grown at 24°C and incubated for an additional hour at 37°C. RNA was incubated with RNase H in the presence or absence of oligo(dT) as indicated. (A) Darker exposure of the wild-type (wt) lanes; (B) light exposure of the same gel. Positions of size markers (lane M) are given in nucleotides.

Similar experiments were also done to test whether the heterogeneous populations seen for snR40, U4, U18, U14, snR73, andsnR72 in the rrp6 $Delta$ strain correspond to polyadenylated RNAs. UponRNase H and oligo(dT) treatment, the heterogeneous populationof 3'-extended species for U18, U14, snR73, and snR72 collapsedinto a faster-migrating species (Fig. 5C to F, compare rrp6 lanesto rrp6 +dT lanes). While snR40 and U4 snRNA did not collapseinto a single band upon RNase H and oligo(dT) treatment, the heterogeneousspecies for these two RNA migrate faster after this treatment,indicating that these species were also cleaved. Because the genomicregions just 3' of these RNAs also do not contain long stretchesof A's, this RNase H-induced shift must also be the result ofa poly(A) tail. Thus, the heterogeneous species of all six RNAsare polyadenylated. As a negative control, the same analyses weredone with snR190 and U24, which did not accumulate as heterogeneouspopulations. RNase H and oligo(dT) treatment did not result ina change in the pattern seen for either snR190 or U24 (Fig. 5Gand H), suggesting that these two snoRNAs are not polyadenylated.

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FIG. 5. The rrp6 $Delta$ mutant accumulates polyadenylated forms of snR40, U4, U18, U14, snR73, and snR72 but not U24 or snR190. Shown are Northern blots containing RNA from the indicated strains. All strains were grown in YEP-2% galactose to early to mid-log phase at 24°C. The rrp6 $Delta$ pap1-1 double mutant was incubated for an additional hour at 37°C as indicated. RNA from the rrp6 $Delta$ strain was treated with RNase H and oligo(dT) as indicated. wt, wild type. Positions of size markers (lanes M) are given in nucleotides.

The second experiment to address whether the longer species were polyadenylated was to examine their presence in an rrp6 $Delta$ pap1-1 double-mutant strain. The PAP1 gene encodes the yeast poly(A)polymerase. The pap1-1 allele confers a temperature-sensitivedefect in the addition of poly(A) tails to mRNA (25). Northernblot analysis of RNA from an rrp6 $Delta$ pap1-1 strain grown at 24°Cshowed that this strain accumulated the heterogeneous 3'-extendedtranscripts, but they were shorter than those in the rrp6 $Delta$ controlstrain (Fig. 5A to F, compare rrp6 lanes to rrp6 pap1-1 24C lanes).This indicates a partial defect in polyadenylation, even at thepermissive temperature. More important, the heterogeneous populationdisappeared after a 1-h shift to 37°C (the restrictive temperaturefor pap1-1; Fig. 5A to F, compare rrp6 and rrp6 pap1-1 24C lanesto rrp6 pap1-1 37C lanes), indicating that Pap1p is required forthe accumulation of this heterogeneouspopulation.

We interpret the above data to suggest that at least a portion of the primary transcripts of snoRNAs are produced as polyadenylatedspecies utilizing Pap1p and that the exosome functions to deadenylatethese RNAs (see Discussion). Interestingly, the rrp6 $Delta$ pap1-1 doublemutant did not accumulate abundant 3'-extended nonpolyadenylatedsnoRNAs that would comigrate with the species seen in the rrp6 $Delta$ +dT lanes. This finding indicates that while rrp6 mutants deadenylatethese species slowly, further 3' trimming is not as strongly affected.Finally, the polyadenylated snoRNA species that accumulated inthe rrp6 $Delta$ pap1-1 mutant at 24°C disappeared within 1 h after inactivationof Pap1p. This observation suggests that this strain still containsan activity that can process, or degrade, the polyadenylated snoRNAspecies (see below for furtherdiscussion).

Rnt1p and the exosome act in the same pathway of U4 snRNA processing. Recently it has been shown that Rnt1p, a double-strand-specific endoribonuclease, processes the U4 snRNA at two sites located135 and 169 nt 3' of the mature 3' end, generating precursorsof approximately 300 nt (1a). This is the same size as the 3'-extendedU4 RNA that we detect in our Northern blots and that accumulatesas a polyadenylated species in the rrp6 $Delta$ strain. These observationssuggest two mechanisms for the formation of the polyadenylatedU4 RNAs. In one model, the 3'-extended forms of the U4 snRNA wouldbe made by the assembly of the normal mRNA polyadenylation machineryonto the nascent transcript, which would then lead to cleavageand polyadenylation. This would generate polyadenylated transcriptssimilar in size to the Rnt1p cleavage products but independentlyof Rnt1p. Alternatively, following Rnt1p cleavage, the 3'-extendedU4 snRNA could be a substrate for polyadenylation by Pap1p. Thiswould be striking since it would imply that the poly(A) polymerasecan function on a second class of substrates cleaved by a distinctendonuclease. This latter hypothesis predicts that the formationof the polyadenylated U4 RNAs should be dependent on theRnt1p.

To test this prediction, we examined the processing of the U4 snRNA in rnt1 $Delta$ and rnt1 $Delta$ rrp6 $Delta$ double-mutant strains. As expected,the rnt1 $Delta$ strain lacked the approximately 300-nt-long 3'-extendedforms of U4 snRNA that are normally seen in wild-type cells. Moreimportant, in the rnt1 $Delta$ rrp6 $Delta$ double mutant strain the 3'-extendedU4 snRNA species normally seen in rrp6 strains disappeared. Instead,a new heterogeneous species of >500 nt that may itself be polyadenylatedappeared in the double mutant (Fig. 6A). These data strongly suggestthat the polyadenylated U4 RNAs are produced by the addition ofpoly(A) tails to precursors that were cleaved by Rnt1p (see Discussion).For comparison, the processing of U18 snoRNA was analyzed in thernt1 $Delta$ rrp6 $Delta$ strain. Rnt1p has no known role in U18 snoRNA processing,and the rnt1 $Delta$ mutation did not affect U18 processing (Fig. 6B)or prevent the accumulation of polyadenylated U18 species in therrp6 $Delta$ strain, although the abundance of the U18 polyadenylatedspecies was slightly reduced.

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FIG. 6. Rnt1p and Rrp6p act in the same pathway of U4 snRNA processing. Shown are Northern blots containing RNA from the indicated strains. All strains were grown in YEP-2% glucose to early to mid-log phase at 24°C. Blots were probed for U4 snRNA (A) or U18 snoRNA (B) as indicated. wt, wild type. Positions of size markers (lanes M) are given in nucleotides.

Effects of mutations in exosome components on mRNA degradation. Since the exosome is involved in deadenylation of snoRNAs, as well as in 3'-to-5' degradation of mRNA, the exosome might alsofunction in the cytoplasmic deadenylation of mRNA. To examinethis possibility, we measured the deadenylation rate of the MFA2pGand PGK1pG mRNAs (11a) by transcriptional pulse-chase analyses(8). In this analysis, a short pulse of transcription is usedto produce mRNA with long poly(A) tails. The rate of deadenylationcan then be determined in a chase period following transcriptionshutoff. This analysis indicated that ski2 $Delta$ , rrp6 $Delta$ , rrp4-1, ski6-100,and mtr3-1 mutants shortened the poly(A) tail on both PGK1 andMFA2 at rates indistinguishable from those for the wild type (datanot shown). This finding is consistent with prior observationsthat overall mRNA decay rates are not substantially altered inexosome mutants (data not shown and reference 13) and arguesthat the exosome is not required for cytoplasmic deadenylation,although it might be functionally redundant with other 3'-to-5'exonucleases in thecytoplasm.

We also determined the possible role of different exosome subunits in 3'-to-5' mRNA degradation of the body of the transcriptfollowing deadenylation. A simple assay for 3'-to-5' degradationof mRNA is to assess the levels and integrity of a poly(G)-to-3'-endfragment from the MFA2pG transcript (13). This fragment is producedby the 5'-to-3' mRNA decay pathway. Because it is normally degradedby the exosome, it accumulates in mutants defective in 3'-to-5'decay of mRNA (13). As described by Jacobs Anderson and Parker(13), ski2 $Delta$ , ski3 $Delta$ , ski8 $Delta$ , or ski6-100 resulted in the appearanceof a ladder of partially degraded mRNA fragment (Fig. 7). In contrast,the rrp6 $Delta$ and mtr4-1 mutants accumulated MFA2pG mRNA degradationintermediates at levels similar to those for the wild type, indicatingthat Rrp6p and Mtr4p are not required for 3'-to-5' degradationof mRNA.

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FIG. 7. mRNA degradation phenotypes of exosome mutants. Shown is a Northern blot containing RNA from the indicated strains. All strains were grown in YEP-2% galactose to early to mid-log phase. The ski2 $Delta$ , ski3 $Delta$ , ski8 $Delta$ , and rrp6 $Delta$ strains were grown at 30°C. The ski6-100 and mtr4-1 strains were grown at 24°C and incubated for an additional hour at 37°C. The blot was probed with oRP140, which hybridizes to the full-length MFA2pG mRNA and a degradation intermediate as indicated. wt, wild types. Positions of size markers (lane M) are given in nucleotides.

We also genetically tested the involvement of Rrp6p in 3'-to-5' decay of mRNA. This test is based on the observation thatmutations that block 5'-to-3' decay of mRNA (such as deletionof the gene encoding the decapping enzyme, DCP1) are syntheticallylethal with mutations that block the alternative 3'-to-5' pathway(13, 15). A dcp1 $Delta$ strain was crossed with an rrp6 $Delta$ strain,and tetrads from the resulting diploid were dissected. Althoughboth single-mutant strains grow slowly, the double mutant wasrecovered at the expected frequency and did not show an additionalgrowth defect (data not shown). Similarly, an mtr4-1 mutant wascrossed to a dcp1 $Delta$ strain. The double mutants were recovered atthe expected frequency from this cross, and these double mutantsdid not show a more severe growth defect at any temperature tested(23 to 36°C). Thus, both genetic and molecular data indicate thatthe exosome and the Ski2p, Ski3p, and Ski8p are required for 3'-to-5'degradation of mRNA but Rrp6p and Mtr4p are not (seeDiscussion).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The exosome functions in 3'-to-5' processing of some snRNAs and snoRNAs. Our data suggest that the exosome functions in the processing of U4 snRNA and snoRNA species in two manners. One role of theexosome is to deadenylate 3'-extended forms of these transcriptsthat contain poly(A) tails. The key observation is that exosomemutants, and particularly rrp6 $Delta$ strains, accumulate 3'-extendedpolyadenylated U4 snRNA and snoRNA species. Evidence that theseheterogeneous populations are polyadenylated is that they areconverted into shorter species upon treatment with RNase H inthe presence of oligo(dT). In addition, these heterogeneous populationsare shorter in an rrp6 $Delta$ pap1-1 double mutant strain at 24°C thanin the rrp6 $Delta$ mutant and disappear after this double mutant hasbeen shifted to the restrictive temperature of 37°C for 1 h. Sinceboth Rrp6p and Mtr4p are involved in processing of U4 and snoRNAsand both of these proteins have been localized to the nucleus(1, 19), this processing most likely occurs in thenucleus.

Two sets of observations suggest that the exosome also functions in 3'-to-5' trimming of U4 snRNA and snoRNA species in additionto the role in deadenylation. First, in various exosome mutants,longer discrete species accumulate for a variety of transcripts.For example, discrete 3'-extended U4 transcripts are detectedin the mtr4-1, mtr3-1, rrp4-1, rrp6 $Delta$ , and ski6-100 mutants (Fig.1). Second, the RNase H oligo(dT) treatment showed that the poly(A)tail of independently transcribed snoRNA species was added ata site (or sites) 3' of the mature 3' end (Fig. 4 and 5). If thepoly(A) tail had been added to the mature 3' end, the heterogeneouspopulation would have collapsed into the mature RNA band. Thisresult indicates a requirement for further 3' trimming after removalof the poly(A) tail. This further trimming is not carried outcorrectly in an rrp6 $Delta$ strain, resulting in snoRNAs slightly (2-to 5-nt) larger than wild-type snoRNAs (Fig. 1 and 3). Similarly,the rrp6 $Delta$ strain accumulated snoRNA species that were slightly(~3-nt) larger than wild type for the intron-derived U24 snoRNA,which apparently is not deadenylated by the exosome. We have notseen these slightly larger species in any of the conditional exosomealleles tested. It is not clear whether Rrp6p has a special roleor whether the difference in this particular exosome phenotypeseen between rrp6 $Delta$ and other mutant strains is caused by the specificalleles used (see below). The conclusion that the exosome functionsin the 3'-to-5' trimming of snoRNAs is also supported by similarresults from Allmang et al. (1a).

Relationship of polyadenylation to 3' processing of U4 snRNA and snoRNAs. The accumulation of polyadenylated snRNAs and snoRNAs in the various mutant strains raises the related issues of the mechanismby which these poly(A) tails are produced and the relationshipof the polyadenylation to the normal pathway of transcript maturation.Our data suggest that there are two mechanisms for the polyadenylationof these transcripts. In some cases, it appears that the polyadenylationof the transcript follows cleavage by the RNase III homolog, Rnt1p.The critical observation is that the polyadenylated U4 transcriptsseen in an rrp6 $Delta$ strain are not produced in an rnt1 $Delta$ rrp6 $Delta$ doublemutant (Fig. 6). Since the polyadenylation of the U4 transcriptsalso requires the poly(A) polymerase encoded by the PAP1 gene(Fig. 3), this suggests that the same polymerase that normallyis directed to RNA substrates by the cleavage and polyadenylationmachinery can also add poly(A) tails to 3' ends generated by adifferentendonuclease.

A second possible mechanism for the synthesis of 3'-extended polyadenylated U4 snRNAs and snoRNAs would be by 3' end formationand concurrent polyadenylation, similar to the formation of poly(A)tails on mRNA. This would be similar to the proposed role of polyadenylationin the biogenesis of the telomerase RNA subunit in yeast (7),another stable RNA. This possibility is supported by the observationthat the U18 snoRNA receives a poly(A) tail in a manner that islargely Rnt1p independent (Fig. 6B). In addition, RNase H andoligo(dT) treatment roughly maps the polyadenylation site forsnR73 to about position +30 relative to the mature 3' end. Thisdoes not match the known Rnt1p cleavage site (at position +71).This mechanism of polyadenylation would also be consistent withthe detection of polyadenylated snR33 transcripts in wild-typecells (Fig. 4) and with the detection of a longer heterogeneousU4 snRNA transcript in the rnt1 $Delta$ rrp6 $Delta$ double mutant (Fig. 6A).

A related issue is the relationship of the polyadenylation of the transcripts and their normal processing. For some snoRNAs(e.g., snR33), detection of the polyadenylated species at lowlevels in wild-type strains suggests that these are normal intermediatesin the biogenesis of the transcript. For U4 snRNA and other snRNAs,there are two possible relationships between polyadenylation andnormal processing. First, the polyadenylation of these transcriptscould be a normal step in their biogenesis, and the polyadenylatedspecies is normally rapidly processed by the Rrp6p and the exosomeand is therefore not detectable in wild-type strains. Alternatively,these transcripts could become polyadenylated as a result of ablock in their normal processing. For example, the U4 RNA couldnormally be processed by Rrp6p and the exosome following Rnt1pcleavage, but if this 3' trimming is inhibited by the rrp6 $Delta$ orconditional exosome lesions, the Rnt1p cleavage product, or slightlytrimmed versions of it, could be adenylated by Pap1p. This wouldbe similar to what occurs in Escherichia coli, wherein RNAs resistantto degradation can become polyadenylated in order to promote furtherprocessing (18). At present, these two possibilities cannotbe clearly distinguished. However, since unadenylated 3'-extendedprecursor of most snoRNAs do not accumulate in a pap1-1 rrp6 $Delta$ mutant strain, the addition of poly(A) tails is not a requiredstep in the biogenesis of theseRNAs.

In the cases of U18 and snR73, there may be two independent pathways for processing. One would be initiated by cleavage andpolyadenylation of the nascent transcript relatively close tothe mature 3' end (at approximately +25 and +30, respectively),while the other would be initiated by cleavage and polyadenylationfurther downstream (downstream of the second EFB1 exon and snR72,respectively). An interesting implication of the possibility of3' end formation by different mechanisms is that it allows theproduction of different amounts of individual snoRNAs from onepolycistronic gene or of intron-derived snoRNAs and mRNAs. Thiscould simply be controlled by altering the relative frequencyat which different cleavage and polyadenylation sites are used.The generation of snoRNA 3' ends by two different mechanisms maybe a general phenomenon of many snoRNA and snRNAs. For example,the U5 snRNA in yeast exists as a long and a short form (U5L andU5S), which are produced by alternative cleavage and processingpathways (4).

Implications of polyadenylated snoRNAs for the role of the nucleolus in mRNA transport. The demonstration that several different snoRNAs accumulate as polyadenylated species in exosome mutants has implicationsfor the interpretation of nuclear polyadenylated RNA accumulationin various mRNA export mutants. For example, mtr3-1 and mtr4-1strains were initially isolated as mutants that accumulated polyadenylatedRNA in the nucleus, based on in situ hybridization with labeledoligo(dT) (16). This was interpreted as a defect in mRNA exportfrom the nucleus. Moreover, since the in situ localization ofthe polyadenylated species coincided with the nucleolus (17,19), these observations have led to the hypothesis that mRNAmay be transported through the nucleolus (26, 31). An alternativehypothesis is that this nucleolar polyadenylated RNA accumulationin the mtr3-1 and mtr4-1 mutants is due to the accumulation ofpolyadenylated snoRNAs we have described above. This hypothesisis supported by the observation that the poly(A) in situ signalin mtr3-1 and mtr4-1 strains colocalizes with Nop1p, a subunitof the C/D box snoRNA particle (17, 19). Moreover, snoRNAsmay be sufficiently abundant to be detected by in situ hybridization.Thirty-eight independently transcribed snoRNAs and five polycistronicsnoRNA genes have been characterized, and it appears likely thata significant number remain to be discovered. The abundance ofeach snoRNA in yeast cells is not well established, but publishedestimates vary between 10 to 500 and 200 to >1,000 molecules persnoRNA species (20, 29, 30). Considering that there are15,000 mRNA molecules per yeast cell (12), snoRNAs may significantlycontribute to the nucleolar poly(A) signal in mtr3 and mtr4 (andperhaps other)mutants.

Distinct phenotypes seen in rrp6 $Delta$ strains and other exosome mutants. The different phenotypes for snoRNA processing seen in rrp6 $Delta$ strains, compared to other exosome mutants, may have implicationsfor structure-function relationships of the exosome. For example,although an rrp6 $Delta$ strain accumulates mainly snoRNAs with short3' extensions, rrp4-1, ski6-100, mtr3-1, and mtr4-1 strains allaccumulate mainly snoRNAs of wild-type size, with the accumulationof smaller amounts of larger species following a shift to therestrictive temperature. Interestingly, similar results have beenobtained for 5.8S rRNA processing (data not shown; reference 1;compare data in reference 2 with those in references 9 and21). In this case, rrp6 strains accumulate half of their 5.8SrRNA as a species that is approximately 30 nt larger than wild-type5.8S rRNA (2), while other exosome mutants do not. In addition,rrp6 mutants accumulate significantly higher levels of polyadenylatedU4 snRNA and snoRNAs than other exosome mutantstrains.

At least four distinct hypotheses can explain the differences between rrp6 $Delta$ and other exosome mutants. First, the differencemay simply be due to the fact that the rrp6 $Delta$ phenotype is a steady-statephenotype, while the other phenotypes are seen when the cellshave been incubated at the restrictive temperature for a relativelyshort time. Second, the different phenotypes could reflect differentcatalytic roles of exosome subunits. In the case of U4, the phenotypescould result from preferred removal of the poly(A) tail by Rrp6p,followed by processing by any subunit of the exosome, snoRNAswould be processed by preferred removal of the poly(A) tail byRrp6p and specific removal of the last few nucleotides by Rrp6p.Third, Rrp6p might act independently as a monomeric exonucleasein addition to being a part of the exosome. In rrp6 $Delta$ strains,the phenotype would then be more severe because these strainsare missing not only a completely functional exosome but alsothe monomeric form of Rrp6p. Fourth, Rrp6p may not have a catalyticrole at all, but in the absence of Rrp6p an altered exosome thatdoes not fully carry out its normal function may assemble. Thesehypotheses could be tested by analyses of conditional allelesand/or catalytic site mutants of Rrp6p, but no such alleles existat thistime.

Two functionally distinct exosome complexes. Several observations now suggest that the exosome is not a homogeneous complex, but that there are at least two functionallydistinct exosome complexes in the cell that can be distinguishedgenetically. The key observation here is that while some mutationsof exosome subunits (i.e., rrp4-1 and ski6-100) result in defectsin mRNA degradation (13), rRNA processing (13, 22), snRNAprocessing, and snoRNA processing, there are two classes of mutationsthat specifically disrupt some but not other exosome functions.The first class includes rrp6 $Delta$ and mtr4-1, which cause accumulationof 3'-extended forms of 5.8S rRNA, U4 snRNA, and snoRNAs but haveno effect on 3'-to-5' mRNA degradation. In contrast, yeast strainscontaining ski2, ski3, or ski8 deletions are completely defectivein exosome-mediated mRNA degradation but are indistinguishablefrom wild-type strains for all known other exosomefunctions.

Three points suggest that these two functionally distinct sets of processing reactions reflect differences between cytoplasmicand nuclear reactions. First, Rrp6p and Mtr4p are localized tothe nucleus (1, 19), whereas Rrp4p is localized to both thenucleus and the cytoplasm (1). Second, the nature of the processingreactions is consistent with this distinction. For example, rRNA,snRNA, and snoRNA processing are thought to be nuclear events,whereas mRNA degradation is thought to be a cytoplasmic event.Third, purification of exosomes demonstrated that the Rrp6p wasfound only in association with a fraction of the exosome complex(1). It is notable that all of the nuclear events are processingreactions with specific endpoints and that the cytoplasmic mRNAdecay is a complete digestion of the molecule. This suggests thatthere will be features, either of the substrate, or of the differentexosome complexes, which dictate its endpoint in the 3'-to-5'digestion. A detailed understanding of both the biochemical activitiesand structure-function relations of the exosome and its associatedproteins is necessary to resolve thesequestions.

	ACKNOWLEDGMENTS

We thank Alan M. Tartakoff for helpful comments on the manuscript, mtr3-1 and mtr4-1 strains, and mtr4 plasmids. We are gratefulto members of the Parker laboratory and Harold E. Smith for helpfulcomments on themanuscript.

This work was supported by the Howard Hughes Medical Institute and NIH grant GM45443 to R.P.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular and Cellular Biology, Howard Hughes Medical Institute, Universityof Arizona, Tucson AZ 85721. Phone: (520) 621-9347. Fax: (520)621-4524. E-mail: rrparker{at}u.arizona.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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