Protein trans-Acting Factors Involved in Ribosome Biogenesis in Saccharomyces cerevisiae

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Molecular and Cellular Biology, December 1999, p. 7897-7912, Vol. 19, No. 12
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

MINIREVIEW
Protein trans-Acting Factors Involved in Ribosome Biogenesis in Saccharomyces cerevisiae

Dieter Kressler,¹ Patrick Linder,¹ and Jesús de la Cruz²^,^*

Département de Biochimie Médicale, Centre Médical Universitaire, Université de Genève, 1211 Genève 4, Switzerland,¹ and Instituto de Bioquímica Vegetal y Fotosíntesis, Universidad de Sevilla-CSIC, 41092 Seville, Spain²

	INTRODUCTION

Top Introduction References

The synthesis of ribosomes is one of the major cellular activities, and in eukaryotes, it takes place primarily, althoughnot exclusively, in a specialized subnuclear compartment termedthe nucleolus (125, 155). There, the rRNA genes are transcribedas precursors (pre-rRNAs), which undergo processing and covalentmodification. Maturation of pre-rRNAs is intimately linked totheir assembly with the ribosomal proteins (r-proteins). Theseprocesses depend on various cis-acting elements (6, 188),and they require a large number of nonribosomal protein trans-actingfactors (97, 174, 193). Experimental evidence suggests thatthe basic outline of ribosome synthesis is conserved throughouteukaryotes. However, most of our knowledge comes from the combinationof molecular genetic and biochemical approaches in the yeast Saccharomycescerevisiae. This minireview is aimed at giving an insight intothe functions of the many protein trans-acting factors involvedin ribosome biogenesis in S. cerevisiae.

	PRE-RRNA PROCESSING AND RIBOSOME ASSEMBLY PATHWAYS

In S. cerevisiae, the large 60S ribosomal subunits are composed of 46 r-proteins and three rRNA species (5S, 5.8S, and 25S)while the small 40S ribosomal subunits contain 32 r-proteins andthe 18S rRNA (142, 201). Three of the four rRNAs (18S, 5.8S,and 25S) are transcribed as a single large pre-rRNA by RNA polymeraseI (RNA pol I), whereas the fourth rRNA (5S) is independently transcribedas a pre-rRNA by RNA pol III (201). All four rRNAs are encodedby a 9.1-kb rDNA unit, which is repeated 100 to 200 times on thelong arm of chromosome XII (Fig. 1A). In the 35S pre-rRNA, whichis the longest detectable precursor, the mature rRNA sequencesare separated by two internal transcribed spacer (ITS) sequences,ITS1 and ITS2, and flanked by two external transcribed spacer(ETS) sequences, a 5' ETS and a 3' ETS (Fig. 1). The 35S pre-rRNAdiffers from the primary RNA pol I transcript at its 3' end becausetranscription termination maps to nucleotide position +210 relativeto the 3' end of the mature 25S rRNA, while the 35S pre-rRNA isextended by 7 to 10 nucleotides (78, 187, 189). Maturationof the 35S pre-rRNA, which contains 10 known processing sites,is a multistep pathway that requires many different trans-actingfactors (Fig. 1B and its legend) (97, 174, 193). Processingof the pre-5S rRNA is independent of 35S pre-rRNA maturation andkinetically faster than formation of mature 18S, 5.8S, and 25SrRNAs (146). The 5' end of the mature 5S rRNA corresponds tothat of the primary transcript, whereas the 3' end is processedfrom a pre-5S rRNA that is extended by 7 to 13 nucleotides (141).Many specific nucleotides within the rRNA also undergo, mainlyshortly after transcription, covalent modification. These modificationsinclude isomerization of uridine to pseudouridine ( $Psi$ ) by baserotation (45 modified nucleotides), methylation of the 2'-hydroxylgroup of sugar residues (2'-O-ribose methylation; 55 modifiednucleotides), and base methylation (about 10 modified nucleotides)(9, 21, 84, 120, 135).

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FIG. 1. Pre-rRNA processing in S. cerevisiae. (A) Structure of an rDNA repeat unit. Each unit contains a large operon encoding the 18S, 5.8S, and 25S rRNAs, which is transcribed by RNA pol I (pr, promoter; tr, terminator; eh, enhancer), and an RNA pol III-transcribed 5S rRNA gene. Mature sequences of the RNA pol I transcript are separated by ITS1 and ITS2 and flanked by a 5' ETS and a 3' ETS. The 5S rRNA gene is located between two nontranscribed spacers (NTS1 and NTS2). Black boxes represent mature rRNAs, white thin bars represent the transcribed spacers, and lines represent the nontranscribed spacers. Processing sites are also indicated. (B) Pre-rRNA processing pathways. The primary RNA pol I transcript is processed at its 3' end to yield the 35S pre-rRNA, which is the longest detectable pre-rRNA. The 35S pre-rRNA is first processed at sites A₀, A₁, and A₂, which results in the separation of the pre-rRNAs destined for the small and large ribosomal subunits. The 20S pre-rRNA is matured by endonucleolytic cleavage at site D. The 27SA₂ precursor is processed by two alternative pathways. In the major pathway, about 85% of 27SA₂ pre-rRNA is cleaved at site A₃ and then 5' $right-arrow$ 3' exonucleolytically digested to site B_1S. In the minor pathway, about 15% of the 27SA₂ molecules are processed at site B_1L. While processing at site B₁ is completed, the 3' end of mature 25S rRNA is generated by processing at site B₂. The subsequent ITS2 processing of both 27SB species appears to be the same. Cleavage at sites C₁ and C₂ releases the mature 25S rRNA and the 7S pre-rRNA. The latter undergoes 3' $right-arrow$ 5' exonucleolytic digestion to the 3' end of the mature 5.8S rRNA. The pre-5S rRNA is processed at its 3' end to generate the mature 5S rRNA. Pseudouridylation and 2'-O-ribose methylation take place on the primary transcript. Note that except for Dim1p, the timing of base methylation and the protein trans-acting factors involved therein have not yet been uncovered. Factors involved in pre-rRNA processing and modification are shown. Colors were assigned to each class of protein trans-acting factors as follows: blue, exo- and endonucleases; red, putative ATP-dependent RNA helicases; green, components involved in pre-rRNA modification; black, others. See the text for further details.

Pre-rRNA processing and modification do not take place on "naked" pre-rRNAs. Instead, pre-rRNAs associate with many of ther-proteins in the nucleolus to form preribosomal particles (182).In addition to r-proteins, the nucleolar preribosomes have longbeen known to contain non-r-proteins (182). The identity of theseproteins has not been clearly established, but they presumablycorrespond to trans-acting factors required for pre-rRNA processingand modification or involved in the assembly of the pre-rRNAswith the r-proteins. Although the pre-rRNA processing pathwayand its intermediates have been fairly well characterized, theassembly process of the rRNAs and the approximately 80 r-proteinsinto mature ribosomal subunits is still poorly understood (Fig.2 and its legend) (93, 180-182, 184).

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FIG. 2. Ribosomal subunit assembly pathway in S. cerevisiae. In the nucleolus, the 35S pre-rRNA associates with many early-associating 40S and 60S r-proteins to form a 90S preribosome. The 5S rRNA forms a stable RNP with Rpl5p (L5, red dot). The 5S rRNA is probably already present in 90S preribosomes; therefore, Rpl5p may belong to the group of early-assembling 60S r-proteins. From the 90S particle, 66S and 43S preribosomes containing the 27S and 20S pre-rRNAs, respectively, are formed. The 66S and the 43S preribosomes contain the late-associating r-proteins. Preribosomes are most likely actively exported through nuclear pores. It has been demonstrated that export of 60S ribosomal subunits requires the nuclear or cytoplasmic Ran cycle and distinct nucleoporins (not shown; for details, see reference 70). It is believed that the 66S particle remains in the nucleus until the 7S pre-rRNA is processed to the mature 5.8S rRNA, while the 43S preribosome is rapidly exported to the cytoplasm, where the final maturation step in the synthesis of the 18S rRNA takes place. Assembly of 60S ribosomal subunits is also completed in the cytoplasm by the final incorporation of some r-proteins. At least three of them (also depicted as red dots), including the P2B and Rpl10p/Qsr1p (L10) r-proteins, can exchange on mature 60S ribosomal subunits in vivo. Preribosomes are drawn as balloons, and the nuclear envelope is depicted as pink rods. Protein trans-acting factors with likely involvement in the assembly of ribosomal subunits are colored as follows: red, putative ATP-dependent RNA helicases; black, others. Only those r-proteins for which an indication about the timing of their association with preribosomal particles is known are shown. See the text for further details.

	PROTEIN TRANS-ACTING FACTORS INVOLVED IN RIBOSOME BIOGENESIS

To date, more than 60 protein trans-acting factors have been described to function in yeast ribosome biogenesis and most likelynot all of them have been identified yet. Most of the proteintrans-acting factors can be grouped into classes according totheir experimental or predicted enzymatic functions and/or theirphysical or functional interactions with small nucleolar RNAs(snoRNAs) or other proteins. These classes include componentsof small nucleolar ribonucleoprotein particles (snoRNPs), rRNA-modifyingenzymes, endo- and exonucleases, and putative RNA helicases. However,not all protein trans-acting factors fall into the above classesand many of these contain particular conserved motifs or domainsthat could mediate important functions such as RNA-protein orprotein-protein interactions. A list of trans-acting factors involvedin ribosome biogenesis and links to databases is accessible atreference 115a.

	PROTEIN TRANS-ACTING FACTORS ASSOCIATED WITH SNORNAS

A large number of protein trans-acting factors that are required for ribosome biogenesis are quite stably associated withsnoRNAs in the form of snoRNP complexes (Table 1). In yeast,there are about 100 different snoRNAs (116, 153), which canbe structurally and functionally grouped into three families.Most snoRNAs belong to either the H/ACA-box or the C/D-box family,whereas the RNA component of RNase MRP constitutes one class byitself (see below) (11, 101, 176).

H/ACA-box snoRNPs. In yeast, most, if not all, of the 45 $Psi$ residues are present within the mature rRNA sequences (135). The site-specific pseudouridylationof rRNA requires H/ACA-box snoRNPs, in which the H/ACA-box snoRNAsfunction as guides that specify the uridines to be isomerizedin the pre-rRNA. Site selection is mediated by short base pairingsbetween the snoRNA and the pre-rRNA, and pseudouridylation occursat a fixed distance of about 14 nucleotides from the conservedsnoRNA sequence elements (box H and/or ACA triplet) (57, 131).One H/ACA-box snoRNA, snR30, seems to be exclusively requiredfor the early pre-rRNA processing reactions at sites A₁ and A₂,while the H/ACA-box snoRNA snR10 participates in both early pre-rRNAprocessing reactions and a pseudouridylation event within 25SrRNA (130, 131, 153, 175).

Based on coimmunoprecipitation and purification experiments, the core protein components common to all H/ACA-box snoRNPs havebeen identified. This core particle probably contains two copiesof each of four proteins (Cbf5p, Gar1p, Nhp2p, and Nop10p) andone H/ACA-box snoRNA (63, 197), and it is arranged in a symmetrictwo-domain structure (117, 197). However, the detailed architectureof H/ACA-box snoRNPs, as well as the order of their assembly,remains to be elucidated. The nucleolar protein Cbf5p might bethe $Psi$ -synthase in each snoRNP, since it is homologous to a familyof putative $Psi$ -synthases (87). Indeed, depletion of Cbf5p blocks $Psi$ formation in pre-rRNAs, which is most likely due to the lossof Cbf5p's putative enzymatic function and the codepletion ofH/ACA-box snoRNAs (99). Probably as a consequence of the concomitantcodepletion of snR10 and snR30, Cbf5p depletion inhibits pre-rRNAprocessing at sites A₁ and A₂ and, to a lesser extent, at siteA₀ (99). Interestingly, depletion of Cbf5p also leads to slightlyreduced levels of 25S rRNA and to accumulation of 27SB and 7Spre-rRNAs and of an aberrant extended 5.8S rRNA species (99).This latter phenotype is unique and not related to the loss offunction of any known snoRNA. Furthermore, the depletion of neitherNhp2p nor Nop10p, which also results in the codepletion of H/ACA-boxsnoRNAs, shows such a particular phenotype (63). Therefore,it can be assumed that Cbf5p has other roles in ribosome biogenesisin addition to its function as an integral component of H/ACA-boxsnoRNPs, perhaps through interactions with other trans-actingfactors during the assembly of preribosomes (25, 99). Indeed,the mammalian homolog of Cbf5p, termed NAP57, is associated instoichiometric amounts with another nucleolar protein called Nopp140(124), which is the homolog of the yeast nucleolar acidic andserine-rich protein Srp40p (123). A genetic interaction betweenSrp40p and H/ACA-box snoRNAs has been recently uncovered, therebyindirectly linking Srp40p and Cbf5p (122). Therefore, the Srp40p-Cbf5pcombination seems to, indeed, mirror the Nopp140-NAP57 connectionin mammalian cells. Although the function of Srp40p in ribosomebiogenesis has not been analyzed so far, it has been suggestedthat Srp40p, in analogy to the proposed function of the Nopp140-NAP57complex, might mediate traffic of diverse nuclear components,among them, snoRNAs and preribosomes (72, 122).

Gar1p is a nucleolar protein that contains two regions that are rich in glycine and arginine (GAR domain) (61). The GARdomain is also present in other nucleolar proteins involved inribosome biogenesis (see below), and it is thought to mediateprotein-RNA interactions (61). Neither one of the two GAR domains(one N terminal and one C terminal) of Gar1p is required for cellviability or for in vitro snoRNA binding (10, 61). Gar1p isrequired for pre-rRNA processing at sites A₁ and A₂ (61). Morerecently, it has been demonstrated that Gar1p is involved in globalpre-rRNA pseudouridylation (20) and that it is specificallyassociated with all H/ACA-box snoRNAs (58). However, Gar1p isthe only core component of H/ACA-box snoRNPs whose depletion doesnot alter the steady-state levels of snoRNAs (20, 61). Nevertheless,in the absence of Gar1p, the H/ACA-box snoRNPs are unable to efficientlyassociate with higher-order nucleolar particles. This suggeststhat Gar1p might work by establishing or maintaining interactionsof snoRNPs with the pre-rRNA (cited in references 20 and 99).The putative RNA helicase Rok1p (see below) may assist Gar1p inthis function, since ROK1 was identified in genetic screens forsynthetic lethality with both a conditional gar1 allele and thesnr10 null ( $Delta$ snR10) mutation (191). Furthermore, Gar1p has beenshown to interact with Cbf5p by the yeast two-hybrid system (citedin reference 63).

Nucleolar Nhp2p and Nop10p also specifically associate with all H/ACA-box snoRNAs (63, 197). Nhp2p shares homology witha 53-amino-acid region within the r-protein Rpl30p (formerly L32)that has been implicated in RNA binding (195). Therefore, itis assumed that Nhp2p directly binds to H/ACA-box snoRNAs (63).This binding (and/or the binding of the other H/ACA-box snoRNPcomponents) probably limits further trimming and degradation ofH/ACA-box snoRNAs by the exonucleases Xrn1p and Rat1p (see below)and other nucleases (18, 63, 140). Nop10p, on the other hand,contains no obvious protein motifs (63). Depletion of Nhp2por Nop10p inhibits pre-rRNA processing at sites A₁ and A₂, andas in the case of Cbf5p depletion, this phenotype can be explainedby the codepletion of snR10 and snR30 (63). In addition, sincethe stability of all H/ACA-box snoRNAs is affected, Nhp2p andNop10p depletion also blocks $Psi$ formation (63). Moreover, asin cells lacking Cbf5p, Gar1p is rapidly degraded in the absenceof either Nhp2p or Nop10p, indicating that the integrity of H/ACA-boxsnoRNPs is perturbed (63). However, Nhp2p or Nop10p depletiondoes not lead to the codepletion of Nop10p or Nhp2p, respectively(63).

Apart from the core components, two further proteins, Sen1p and Sbp1p, have been described to associate with certain H/ACA-boxsnoRNAs. The function of Sen1p, a putative RNA helicase, willbe discussed below. The nonessential Sbp1p contains a centralGAR domain followed by an RNA recognition motif (RRM) and acidicand serine-rich stretches; these motifs probably mediate the specificstrong binding to snR10 and the weak binding to snR11 (34).In addition, the $Delta$ sbp1 strain has growth and pre-rRNA processingphenotypes that are similar to those of the $Delta$ snr10 strain (citedin reference 34). However, whether Sbp1p is required for invivo snR10 stability and/or snR10-associated pseudouridylationis notknown.

As mentioned above, the snR30 H/ACA-box snoRNP seems to be solely required for the early pre-rRNA processing reactions atsites A₁ and A₂. Nevertheless, its core composition and structureare similar to those reported for the snR42 H/ACA-box snoRNP,which is exclusively involved in pseudouridylation (117, 197).In clear contrast to the snR10 and U3 snoRNPs (see below), itis unknown if additional proteins are required for the functionof the snR30snoRNP.

C/D-box snoRNPs. Yeast rRNAs contain about 65 methyl groups; 55 of these are linked to the 2'-hydroxyl residue of ribose, while the rest ofthem are attached to the bases (9). Ribose methylation is,in analogy to pseudouridylation, carried out by specific snoRNPsthat contain snoRNAs of the C/D-box family (82, 176). ThesesnoRNAs have one or two sets of well-conserved short sequenceelements, which are called box C and box D (or box C' and boxD', for the second set), and about 10 to 20 nucleotides with sequencecomplementarity to the rRNA. The position of 2'-O-ribose methylationof rRNA is 5 nucleotides upstream of box D (or D') (9, 83).Most of the 55 2'-O-ribose-methylated sites have been recentlyassigned to different guide C/D-box snoRNAs, all of them dispensablefor cell viability (116, 153). In contrast to these, U3 andU14 are essential C/D-box snoRNAs (176). The U3 snoRNA seemsto be exclusively required for pre-rRNA processing at sites A₀to A₂, while the U14 snoRNA is involved in pre-rRNA processingreactions at sites A₁ and A₂ and in a 2'-O-ribose methylationevent within the 18S rRNA (153, 176).

To date, three proteins (Nop1p, Nop56p, and Nop58p) have been identified that probably form the core of all C/D-box snoRNPs(Table 1) (58, 59, 102, 202). In clear contrast to thepresence of the candidate $Psi$ -synthase Cbf5p in H/ACA-box snoRNPs,the putative methylase(s) has not yet been identified as a corecomponent of C/D-box snoRNPs, although an enzymatic role for Nop1pcannot be excluded (132). Moreover, there are several proteinswith predicted rRNA methyltransferase activity that are thoughtto be good candidates (Nop2p, Ncl1p, and Spb1p; see below) (68,92, 203).

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TABLE 1. Protein components of snoRNPs

Nop1p, which contains an N-terminal GAR domain (156), is structurally and functionally equivalent to human fibrillarin (75).Although early work suggested that Nop1p efficiently precipitatesboth C/D-box and H/ACA-box snoRNAs (156, 177), it now seemsclear that Nop1p is specifically associated with C/D-box snoRNAs(58). Depletion of Nop1p leads to codepletion of methylationguide snoRNAs (as demonstrated for U14 and snR190) but not ofU3 snoRNA (177). Partial inactivation of the U3 snoRNP function,due to the loss of its Nop1p component, and the reduction in thelevels of U14 might be responsible for the pre-rRNA processingdefects at sites A₀ to A₂ that are detected upon depletion ofNop1p (177). Similarly, loss of methylation guide snoRNAs isconsistent with impaired global methylation upon Nop1p depletion.Interestingly, it has been reported that in the nop1-3 mutant,global methylation is dramatically affected without having majoreffects on pre-rRNA processing or ribosome assembly (178). Thisindicates that 2'-O-ribose methylation, as well as $Psi$ synthesis,and pre-rRNA processing are independent events (20, 178). Othernop1 mutants affect the assembly of 60S ribosomal subunits withoutleading to clear pre-rRNA processing and methylation defects (178).Whether this phenotype is the consequence of the loss of particularsnoRNA-pre-rRNA interactions or the impairment of another independentfunction of Nop1p remains to be elucidated. Indeed, Nop1p, butnot any snoRNA, also binds in substoichiometric amounts to anothertrans-acting factor named Nop4p/Nop77p (15). Nop4p is a nucleolarprotein, which has been identified both in a synthetic lethalscreen with a nop1 allele and as a nucleolar antigen (15, 170).Nop4p is made up of a modular primary structure that consistsof three N-terminal RRMs and a fourth incomplete RRM in the C-terminalpart of the protein. The fourth RRM is followed by a region richin lysine and arginine residues, while the first three RRMs areseparated by two regions rich in acidic amino acids. This structuresuggests that Nop4p is able to directly interact with RNA. Moreover,each RRM is required for optimal Nop4p function in vivo (171).Depletion of Nop4p delays 35S pre-rRNA processing and leads toa drastic reduction in the steady-state levels of the 27SA₃ and27SB pre-rRNAs (15). As a consequence, synthesis of mature 25SrRNA and production of 60S ribosomal subunits are reduced (170).It is, however, controversial if Nop4p is involved in rRNA methylation(15, 170). The above pre-rRNA processing phenotype is clearlydifferent from that observed after depletion of Nop1p or the snoRNAU3 or U14. Most likely, Nop4p, in concert with Nop1p, plays arole in the early assembly of 60S ribosomalsubunits.

Nucleolar Nop56p and Nop58p, which are homologous to each other, were also both identified in a synthetic lethal screen withnop1 alleles (59). Nop58p (also named Nop5p) has been simultaneouslyisolated in a screen for nucleolar antigens (202). The primarysequence of both proteins contains several repeats of the KKE/Dmotif, a feature shared with Cbf5p and the putative RNA helicaseDbp3p (198). In the case of Nop58p, these repeats are not requiredfor cell growth, protein targeting to the nucleolus, or stableassociation with snoRNAs (59, 102). Depletion of Nop56p resultsin the inhibition of pre-rRNA processing at sites A₀ to A₂ andreduced steady-state levels of Nop1p; however, neither global2'-O-ribose methylation nor the stability of C/D-box snoRNAs isaffected (96). In contrast, the temperature-sensitive nop56-2mutation leads to the accumulation of 27SB pre-rRNAs and to delayedconversion of these precursors to mature 25S rRNA, which mostlikely accounts for the observed deficiency in the formation of60S ribosomal subunits (59). This pre-rRNA processing phenotypeis similar to that observed upon Nop2p and Spb1p depletion (68,92). The function of Nop58p has been studied in more detail.Nop58p specifically interacts with all C/D-box snoRNAs, includingU3 and U14 (102, 202). Moreover, depletion of Nop58p resultsin the mislocalization of Nop1p (202) and in the instabilityof all C/D-box snoRNAs (102). Consistent with this, depletionof Nop58p leads to inhibition of the A₀-to-A₂ pre-rRNA processingreactions (102), therefore resulting in a reduction of 40S relativeto 60S ribosomal subunits (202). Surprisingly, global methylationis not affected upon Nop58p depletion (102, 202), perhaps thereduced levels of C/D-box snoRNAs are sufficient to promote 2'-O-ribosemethylation but can no longer support pre-rRNA processing (102).

Unfortunately, no information is available concerning the architecture of C/D-box snoRNPs. Due to the conserved nature ofthe C and D boxes and the adjacent terminal stem (C/D-box motif)(9), and because of the requirement of this C/D-box motif forsnoRNA stability and function (83, 154), it is conceivablethat either Nop1p, Nop56p, Nop58p, or the candidate 2'-O-ribosemethylase(s) binds directly to this motif. However, there is noevidence yet for an interaction between any of the putative methyltransferases(apart from Nop1p [see below]) with C/D-boxsnoRNPs.

The U3 snoRNP is a particular C/D-box snoRNP. In addition to the core proteins, it contains unique proteins that are not presentin other C/D-box snoRNPs (Table 1). Sof1p was the first describedU3 snoRNP protein; it was isolated as an extragenic suppressorof the thermosensitive phenotype of a $Delta$ nop1 strain complementedwith human fibrillarin (74). Sof1p is a nucleolar protein whoseprimary structure contains seven WD repeats, which could mediateprotein-protein interactions, and a C-terminal part that is richin charged amino acids (74). Apart from binding exclusivelyto the U3 snoRNA, Sof1p appears to associate with Nop1p in substoichiometricamounts, which is consistent with the fact that Nop1p is a corecomponent of all C/D-box snoRNAs. Depletion of Sof1p leads toimpaired pre-rRNA processing at sites A₀ to A₂ and inhibitionof 18S rRNA production, but it does not result in instabilityof either U3 or Nop1p (74). Consistent with the specific associationof Sof1p with U3, pre-rRNA methylation is not affected upon Sof1pdepletion. Mpp10p and its interacting partners Imp3p and Imp4p(48, 108, 109), Lcp5p (200), and Rrp9p (190) are also U3snoRNP components, and their depletion leads to inhibition ofthe early pre-rRNA cleavages. As reported for Sof1p, U3 stabilityis not affected upon depletion of Mpp10p, Imp3p, or Imp4p (48,109). So far, there are at least nine proteins that are associateddirectly or indirectly with the U3 snoRNA; however, it remainsto be determined whether all of these coexist in the same U3snoRNP.

	RRNA-MODIFYING ENZYMES

As mentioned above, posttranscriptional modification of mature rRNAs occurs mostly on the pre-rRNA. These modifications include $Psi$ formation, 2'-O-ribose methylation, and base methylation (9,120, 135). In contrast to the putative rRNA $Psi$ -synthase Cbf5p(99, 197), which is a subunit of all H/ACA-box snoRNPs (seeabove), the candidate methylase(s) responsible for 2'-O-ribosemethylation has not yet been identified. Proteins with predictedrRNA methyltransferase activity have been detected by sequencecomparison to the human tumor-specific nucleolar protein p120and to putative bacterial rRNA methyltransferases (86). In particular,Nop2p shows strong overall homology to p120 (39). NucleolarNop2p is required for the conversion of the 27SB pre-rRNA intomature 25S rRNA and, thus, for synthesis of 60S ribosomal subunits(68). However, although it seems that 2'-O-ribose methylationat a specific site in the 27S pre-rRNA is delayed upon Nop2p depletion,global methylation is not affected (68). Thus, Nop2p is unlikelyto be the only candidate rRNA methyltransferase (68). Indeed,a similar pre-rRNA processing phenotype is observed when cellsare depleted of the essential protein Spb1p, which also containsa putative S-adenosylmethionine (SAM)-binding motif (92). Theclosest S. cerevisiae homolog of Nop2p is Ncl1p, which contains,in addition to the SAM-binding motif, the evolutionarily conserved"NOL1/NOP2/fmu family signature" motif (203). The nonessentialNcl1p localizes to the nucleus, including the nucleolus, and isconcentrated at the nuclear periphery. Disruption of NCL1 affectsneither cell growth nor steady-state levels of ribosomal subunits;however, it leads to increased sensitivity to the aminoglycosideantibiotic paromomycin, which suggests that ribosome functionis perturbed (31, 54, 138, 162). Niewmierzycka and Clarkehave recently searched the complete S. cerevisiae genome withsequence motifs that are conserved in SAM-dependent methyltransferases.They identified 7 known methyltransferases, including Dim1p (seebelow), and 26 putative methyltransferases (132). Neither Nop2p,Ncl1p, nor Spb1p is among these putative methyltransferases, butinterestingly, Nop1p (certain mutant forms of which affect globalmethylation [see above]) was found by this analysis. Therefore,it cannot be excluded, until otherwise demonstrated, that Nop1pitself is an rRNA 2'-O-ribosemethyltransferase.

Little is known about base methylation in eukaryotes, and in contrast to 2'-O-ribose methylation and $Psi$ formation, it doesnot appear to involve guide snoRNA cofactors. The only base methylationstudied in yeast is the evolutionarily conserved dimethylationof two adjacent adenosines (m^6,2A₁₇₇₉ m^6,2A₁₇₈₀) at the 3' end of the 18S rRNA. The essential protein Dim1pis responsible for these modifications, and it is also requiredfor pre-rRNA processing at sites A₁ and A₂ (95, 98), whichgenerate the 20S pre-rRNA. Since dimethylation occurs on the 20Spre-rRNA (98), this observation is consistent with early reportsthat formation of m^6,2A m^6,2A is a late event in ribosome synthesis (21); it can be concludedthat processing at sites A₁ and A₂ does not require prior dimethylation.In agreement with this model, the dim1-2 mutation strongly inhibitsdimethylation while pre-rRNA processing is practically not affectedat the permissive temperature. Thus, the enzymatic function ofDim1p can be separated from its involvement in pre-rRNA processing(100). The dim1-2 mutant strain displays wild-type growth atthe permissive temperature, indicating that dimethylation is notessential for cell viability. On the other hand, cell extractsprepared from this strain are incompetent for translation in vitro,which suggests that dimethylation is necessary under suboptimalin vitro conditions but only fine tunes ribosomal function invivo (100). Interestingly, pre-rRNA processing is insensitiveto temperature-sensitive mutations in or depletion of Dim1p whentranscription of the rDNA unit is driven by an RNA pol II PGKpromoter, which suggests that Dim1p is not directly required forpre-rRNA processing. Therefore, it is very likely that an activerepression system (quality control) blocks pre-rRNA processingin the absence of the binding of Dim1p to the pre-rRNA (100,103). Moreover, all dim1 mutants are hypersensitive to the aminoglycosideantibiotics paromomycin and neomycin B, even under conditionsin which neither dimethylation nor pre-rRNA processing is clearlyaffected (100). This suggests that Dim1p plays an additionalrole in ribosomeassembly.

What is the role of these rRNA modifications? $Psi$ residues are functionally more versatile than uridine residues in that bothN1 and N3 are available for hydrogen bonding. In contrast, 2'-O-ribosemethylation has the opposite effect since it prevents the 2' hydroxylgroup of ribose from hydrogen bonding (120). However, 2'-O-methylgroups can stabilize RNA stems by conferring conformational rigidityon the nucleotide (101 and references therein). Strikingly, mostpseudouridylated and methylated residues are clustered in therRNA domains that carry out important functions during translation.This led to the proposition that rRNA modifications may have adirect role in the function of the ribosome as, for instance,in the peptidyl transfer reaction (120). Alternatively, thesemodifications may play roles in fine-tuning ribosome assembly(174). Deletion of single or multiple guide snoRNAs does notaffect cell growth (116, 139, 153). However, rRNA folding and/orassociation with the r-proteins may still be less efficient inthese strains, even though the growth disadvantage is not detectableunder laboratory conditions. In addition, even when global 2'-O-ribosemethylation is completely inhibited, as in the nop1-3 mutant atthe permissive temperature, pre-rRNA processing, ribosome assembly,and export of ribosomal subunits to the cytoplasm continue (178).However, growth of the nop1-3 mutant strain is strongly affectedat the nonpermissive temperature, which implies that ribosomescontaining severely undermethylated rRNA are most likely deficientin some important translational function (120, 178). Intriguingly,in bacteria, partially functional 30S and 50S ribosomal subunitscan be reconstituted with in vitro-transcribed 16S and 23S rRNAs,respectively (35, 62, 80). This suggests that, at leastin prokaryotes, posttranscriptional modification of rRNAs is notessential for the assembly or function of ribosomalsubunits.

	ENDO- AND EXO-RNASES

Several endo- and exonucleases carry out the different processing reactions during maturation of pre-rRNAs. The largest detectablepre-rRNA is the 35S pre-rRNA, and it differs from the primaryRNA pol I transcript at its 3' end (Fig. 1). The 35S pre-rRNAis generated by endonucleolytic cleavage of the primary transcriptbetween nucleotide positions +45 and +15 relative to the 3' endof the mature 25S rRNA. This cleavage is then followed by shorteningof the pre-rRNA up to position +7 (78). These first processingevents are dependent on Rnt1p. The $Delta$ rnt1 strain, which displaysa very strong slow-growth phenotype and temperature sensitivity(30), and the rnt1-1 mutant strain accumulate the primary transcriptin vivo (2, 94). Rnt1p is a double-strand-specific endo-RNasethat is homologous to bacterial RNase III (2, 8). In vivo,the Rnt1p cleavage sites map between nucleotide positions +14and +49, which is in perfect agreement with the reported processingsites within the primary RNA pol I transcript (94). Moreover,recombinant Rnt1p is able to cleave a synthetic 3' ETS substrate21 nucleotides downstream of the 3' end of the 25S rRNA (2),which is within the reported region where in vivo processing takesplace. The so far unidentified product of the RNA82 gene is probablyalso required for 3' ETS processing because the rna82-1 mutationaffects 3'-end processing of transcripts derived from artificialrDNA minigene reporters. In the rna82-1 mutant strain, the majorityof transcripts extend to nucleotide positions between +15 and+10, instead of being matured to the 3' end of the 25S rRNA asobserved for the wild-type strain (78).

The earliest processing event in the 35S pre-rRNA is the endonucleolytic cleavage at site A₀, which is dependent on the U3snoRNP (13, 69). In vitro, Rnt1p cleaves a model 5' ETS substrateat site A₀ in the absence of other factors and the rnt1-1 mutationleads to depletion of the 33S pre-rRNA (2). Therefore, it seemslikely that Rnt1p is required for pre-rRNA processing at siteA₀. Recent data, however, seem to exclude a direct role for Rnt1pin cleavage at site A₀ because, although kinetically delayed,cleavage at this site still occurs in the $Delta$ rnt1 mutant strain(94). Therefore, if Rnt1p is involved in cleavage at site A₀,this function can be partially fulfilled by another endonuclease(s).This would then resemble very much the situation in Escherichiacoli, where RNase III disruption is not lethal and other endonucleasescarry out somewhat redundant functions (8). In addition, pre-rRNAprocessing at sites A₁ and A₂ is also delayed in the $Delta$ rnt1 strain(94). This could be the consequence of codepletion of the matureform of the U14 snoRNA, since Rnt1p is also involved in the correctprocessing of some snRNAs and snoRNAs from precursors, such asthe dicistronic snR190-U14 precursor (1, 29, 30). However,the snR190-U14 precursor probably retains at least some functionality,since U14 is essential for cell viability and depletion of U14does block pre-rRNA processing at sites A₁ and A₂ (113).

RNase MRP is an endo-RNase that cleaves pre-rRNA at site A₃ in vivo and in vitro (32, 118, 158). The RNA component ofRNase MRP, encoded by the NME1/RRP2 gene (115, 159, 160), isa unique snoRNA because it does not contain complementary sequencesthat allow base pairing with the pre-rRNA (see above). MRP RNAis structurally related to RNase P RNA; this suggests that RNaseMRP arose in eukaryotes as a form of RNase P specialized for pre-rRNAprocessing (129). RNase MRP consists, in addition to MRP RNA,of nine integral protein subunits (Table 1) (27, 157), eightof these (Pop1p, Pop3p, Pop4p, Pop5p, Pop6p, Pop7p/Rpp2p, Pop8p,and Rpp1p) being shared between RNase MRP and RNase P (27).The only protein component unique to RNase MRP is Snm1p (157).Mutation in or depletion of the RNA or any of the protein componentsof RNase MRP, except Pop8p (not determined for Snm1p), leads tothe inhibition of cleavage at site A₃. Moreover, depletion ofany protein component of RNase MRP, except Pop3p, leads to codepletionof MRP RNA (27, 33, 45, 119, 158, 168, 169). As a consequence,the synthesis of 5.8S_S is impaired and the ratio of 5.8S_S to 5.8S_L,which is around 7:1 in wild-type cells (45), is strongly decreased.The same phenotype is seen in a mutant carrying a deletion ofthe A₃ cleavage site (64). Intriguingly, cleavage at site A₃is nonessential for cell viability (64) whereas all known componentsof RNase MRP are essential. Therefore, it is likely that RNaseMRP has additional, as yet unidentified, substrates (44, 45,173). Early tRNA maturation reactions, including 5'-terminalprocessing by RNase P, occur in the nucleolus (16), which suggeststhe possibility of direct coordination between tRNA and ribosomebiosynthesis. Interestingly, a mutation in the RNase P RNA subunit(rpr1) leads to the accumulation of an aberrant form of 5.8S rRNAthat is 3' extended for about 30 nucleotides (28). However,the precise role of RNase P in pre-rRNA processing remains obscureand it is possible that the rpr1 mutation affects pre-rRNA processingindirectly. Indeed, depletion of Rpr2p, an exclusive componentof RNase P, decreases the stability of RNase P RNA and impairs5'-end maturation of pre-tRNAs without affecting pre-rRNA processing(27).

It is noteworthy that the endo-RNases responsible for cleavage at processing sites A₁, D, and A₂ have not yet been identified.Moreover, it is only suspected that an endonucleolytic activityis required for processing at site B_1L. In the case of ITS2 processingsites C₁ and C₂, it has to be assumed that at least one (if notboth) of these sites is cleaved endonucleolytically. Unfortunately,no trans-acting factors that are involved in processing at sitesB_1L, C₁, and C₂ have been identified sofar.

In contrast, the enzymes responsible for all exonucleolytic processing reactions have most likely been identified. The essentialRat1p and the nonessential Xrn1p are homologous and functionallyequivalent proteins that have processive 5' $right-arrow$ 3' exo-RNase activityin vitro (7, 76, 105, 165, 167). Xrn1p functions mainlyin the cytoplasm, while Rat1p is a nuclear protein (66, 76).Xrn1p was also purified as a protein having DNA strand exchangeand DNA G4 tetraplex-specific nuclease activity, and its genewas cloned by a number of different genetic selection techniquesthat are not obviously related (see reference 76 and referencestherein). Since the $Delta$ xrn1 strain is severely impaired in 5' $right-arrow$ 3'degradation of mRNA (reviewed in reference 26), the myriad putativeactivities of Xrn1p can be rationalized by a model in which regulationof gene expression is globally deranged due to the inhibitionof 5' $right-arrow$ 3' mRNA decay pathways (76). Moreover, combination ofthe $Delta$ xrn1 mutation with mutations affecting 3' $right-arrow$ 5' degradationof mRNAs leads to synthetic lethality, which confirms that the"essential" function of Xrn1p is its 5' $right-arrow$ 3' exoribonucleolyticactivity and further indicates that efficient mRNA turnover isrequired for cell viability (73). Rat1p has been isolated asrequired for the efficient nucleocytoplasmic trafficking of mRNAs(7), and it was also independently identified in two other,unrelated, genetic screens (47, 79). In analogy to the roleof Xrn1p, it is suspected that the essential function of Rat1pis the 5' $right-arrow$ 3' degradation of nuclear RNAs. The role of Xrn1p andRat1p in pre-rRNA processing is the 5' $right-arrow$ 3' exonucleolytic digestionof the 27SA₃ pre-rRNA up to site B_1S (7, 64). This reactiongenerates the 5' end of the major form of 5.8S rRNA, the 5.8S_SrRNA. Accordingly, 5'-extended forms of 5.8S rRNA accumulate in $Delta$ xrn1 single mutants and more drastically in $Delta$ xrn1 rat1-1 doublemutants (64). In wild-type cells, 5.8S_L rRNA, which is 7 to8 nucleotides longer than 5.8S_S, appears before 5.8S_S rRNA. However,the synthesis of both 5.8S rRNA species is kinetically delayedin a $Delta$ xrn1 rat1-1 double mutant at the nonpermissive temperature(64); the reason for this is not clear, but it could reflectan involvement of Xrn1p and Rat1p in processing at site B_1L. Anotherstill obscure finding is that the putative RNA helicase Rok1p(see below) was isolated as a multicopy suppressor of the benomyl-hypersensitivephenotype of the $Delta$ xrn1 mutant strain (164). Xrn1p and Rat1p arealso required for the degradation of several excised pre-rRNAspacer fragments, namely, the A₀-A₁, D-A₂, and A₂-A₃ fragments(140, 166). The accumulation of these spacer fragments is inagreement with endonucleolytic processing at sites A₀, A₁, D,A₂, and A₃ (2, 32, 42, 64, 158, 192). Moreover, bothXrn1p and Rat1p, in conjunction with Rnt1p, are involved in theposttranscriptional processing of snoRNAs (such as snR190, U14,U18, U24, and several others) from larger precursors (30, 140,144, 196).

Formation of the 3' end of 5.8S rRNA from its 7S precursor occurs via a 3' $right-arrow$ 5' exonucleolytic processing mechanism (127),which involves a protein complex called the exosome (126). Thiscomplex is composed of at least three 3' $right-arrow$ 5' exonucleases (Rrp4p,Rrp41p/Ski6p, and Rrp44p) and eight putative 3' $right-arrow$ 5' exonucleases(Csl4p, Mtr3p, Rrp40p, Rrp42p, Rrp43p, Rrp45p, Rrp46p, and Rrp6p)(5, 126). The modes of action of the three 3' $right-arrow$ 5' exonucleasesare distinct: Rrp4p acts by a hydrolytic mechanism and has distributiveactivity, whereas Rrp41p and Rrp44p have processive activitiesand act by a phosphorylytic or a hydrolytic mechanism, respectively(126). Mutation in or depletion of most of the exosome componentsimpairs synthesis of 5.8S rRNA, and it leads to the accumulationof 3'-extended forms of the 5.8S rRNA, which may extend up tothe 3' end of the 7S pre-rRNA at site C₂ (extension of around140 nucleotides) (5, 126). Mutations in RRP6 (Rrp6p is homologousto the 3' $right-arrow$ 5' exo-RNase RNase D from E. coli) result in the accumulationof a distinct 5.8S rRNA processing intermediate, termed 5.8S*,that has a normal 5' end but retains about 30 nucleotides of ITS2(22). Interestingly, this intermediate is quite similar to thatdetected upon mutation of the RNase P RNA (see above) (28).The exosome seems to be assisted by the putative RNA helicaseDob1p/Mtr4p (see below), since mutation in DOB1 or depletion ofDob1p and exosome components leads to a similar accumulation ofthe 7S pre-rRNA and depletion of the mature 5.8S rRNAs (42).Moreover, the slow-growth phenotype of the rrp4-1 mutant is syntheticallyenhanced by the dob1-1 mutation, which is in support of a functionalinteraction between the exosome and Dob1p (42). The exosome,together with Ski2p, which is the cytoplasmic homolog of Dob1p,is also required for the 3' $right-arrow$ 5' degradation of cytoplasmic mRNAs(73). Therefore, the exosome may be involved in the degradationof nuclear RNA substrates other than the 7S pre-rRNA and evena role in nuclear poly(A)⁺ RNA turnover can be envisaged. Indeed, depletion of Dob1p orexosome components leads to the accumulation of the 5'-A₀ spacerfragment (42), which is the only spacer fragment degraded ina 3' $right-arrow$ 5' direction. However, the specific contribution of the differentexosome components to the 3' $right-arrow$ 5' exonucleolytic trimming of the7S pre-rRNA, the 5'-A₀ spacer fragment, and other possible RNAsubstrates remains to be determined. It is even likely that notall of the exosome's exonucleases are simultaneously involvedin the degradation of the same RNAsubstrate.

As mentioned in the Introduction, the pre-5S rRNA only needs to be processed at its 3' end. Piper et al. proposed that the3' end of mature 5S rRNA is generated by a single endonucleolyticcleavage, which requires the product of the RNA82 gene (141).In a pulse-chase labeling experiment, rna82-1 mutant cells initiallyaccumulate mainly the pre-5S rRNA, from which the additional nucleotidesare then slowly removed by a 3' $right-arrow$ 5' exonucleolytic mechanism toyield 5S rRNA species that are mostly only up to 3 nucleotideslonger than in wild-type cells (141). A more recent study, however,disagrees with the above findings and rather supports a modelin which 3'-end maturation of pre-5S rRNA relies exclusively ona 3' $right-arrow$ 5' exonucleolytic activity, which simply trims the pre-5SrRNA to the mature form (112). In this model, the exonucleaseactivity is primarily blocked by a secondary structure (helixI) formed between the interacting 5' and 3' ends of the mature5S rRNA. Association of the 5S rRNA with the 5S rRNA-binding proteinRpl5p, which results in the formation of the stable Rpl5p-5S RNPcomplex, appears not to directly influence the maturation processbut rather seems to protect the 5S rRNA from degradation by othernucleases (43, 112).

	PUTATIVE ATP-DEPENDENT RNA HELICASES

The largest class of trans-acting factors involved in ribosome biogenesis contains the RNA helicases of the DEAD-box and relatedfamilies. These protein families are defined by several evolutionarilyconserved motifs, and their members are involved in various RNAmetabolic processes, including pre-mRNA splicing, translationinitiation, RNA degradation, and ribosome biogenesis (40). Manyof these proteins possess an RNA-dependent ATPase activity, whichis sometimes only stimulated by specific RNA substrates (56,134). Since an ATP-dependent RNA helicase activity could onlybe shown for a few of them (discussed in reference 71), theyare collectively referred to as putative ATP-dependent RNA helicases.However, it is generally believed that putative RNA helicasesact as ATP-dependent modulators of RNA structure (40).

Different functions can be envisaged for putative RNA helicases in ribosome biogenesis. (i) An RNA-unwinding activity couldbe required to establish and/or dissociate snoRNA-pre-rRNA basepairings, which are, in most cases, mutually exclusive with respectto the final folding of the rRNA in the mature ribosome. (ii)Putative RNA helicases may functionally assist endo- and exonucleasesby rendering their substrates accessible for the processing reactions.(iii) Finally, they may recruit, rearrange, or dissociate trans-actingfactors and r-proteins within preribosomal particles during theprocessing and assembly reactions by modulating specific intramolecularrRNA, rRNA-protein, or even protein-protein interactions. In theabsence of such a putative RNA helicase, the lack or retardationof the required structural changes may lead to an abortive assembly,which can entail either disassembly of preribosomal particlesand destabilization of pre-rRNA intermediates or accumulationof preribosomal particles and stabilization of pre-rRNAintermediates.

To date, 16 putative RNA helicases have been directly implicated in ribosome biogenesis in S. cerevisiae (40). Seven ofthem, Dbp4p (81), Dbp8p (37), Dhr1p (96), Dhr2p (96),Fal1p (89), Rok1p (191), and Rrp3p (133), are required forthe early pre-rRNA cleavages at sites A₀ to A₂. Depletion of theseputative RNA helicases leads to similar pre-RNA processing defects,even though these proteins carry out nonredundant functions. Therefore,it is likely that not all of them directly assist the cleavagereactions. The observed pre-rRNA processing phenotypes may alsobe the indirect consequence of defective assembly of an earlypreribosomal particle on the pathway to 40S ribosomal subunitformation. Unfortunately, data giving an indication of the functionalenvironment of Dbp8p, Dhr1p, Dhr2p, Fal1p, or Rrp3p are stilllacking. On the other hand, genetic observations suggest a functionalinteraction between Rok1p and both snR10 and Gar1p (191) andbetween Dbp4p and snoRNA U14 (114). However, there is no evidencefor stable physical interactions between these putative RNA helicasesand snoRNAs (81, 191) and they therefore probably associateonly transiently. Recombinant Rrp3p (cited in reference 133)and Rok1p display ATPase activity in vitro (136, 143), and recombinantDbp4p binds nonspecifically to RNA and has an intrinsic ATPaseactivity that is not stimulated by the addition of U14, 18S rRNA,or total RNA (81).

Nine putative RNA helicases act at different steps during the biogenesis of 60S ribosomal subunits. The nonessential Dbp3pis required for efficient pre-rRNA processing at site A₃ (198).This site is located 5 nucleotides downstream of a proposed stablestem-loop structure (4, 205); thus, Dbp3p could be involvedin the local unwinding of this structure, thereby facilitatingthe assembly of the RNase MRP complex at site A₃ (198). Strainsin which Dob1p/Mtr4p is defective have pre-rRNA processing defectsthat are similar to those of exosome mutants (see above) (42,126), and the specific inhibition of the 3' $right-arrow$ 5' exonucleolyticprocessing of the 7S pre-rRNA to mature 5.8S rRNA is most likelyresponsible for the underaccumulation of 60S ribosomal subunitsin dob1 mutants. Given that Dob1p/Mtr4p does not tightly associatewith the exosome, it may act as a cofactor that prevents stallingof the exosome by unwinding secondary structures (42, 172).The remaining seven putative RNA helicases are likely to be requiredfor early, intermediate, or late structural rearrangement reactionswithin preribosomal particles that are mainly necessary for theformation of 60S ribosomal subunits. The pre-rRNA processing phenotypesobserved upon depletion of Dbp6p and Dbp9p (instability of 35Spre-rRNA-derived processing intermediates and/or decreased formationand steady-state levels of 27SB precursors) suggest that thesetwo proteins are essential for assembly reactions that occur withinearly preribosomal particles (36, 88). Moreover, dbp6 dbp9double mutants are synthetically lethal and the slow-growth phenotypeof some dbp6 mutants is exclusively suppressed by overexpressionof Dbp9p (36). The nonessential Dbp7p (38), whose deletionconfers a strong slow-growth phenotype, and Mak5p (206) mostlikely act downstream of Dbp6p and Dbp9p. Absence of Dbp7p ordepletion of Mak5p results in a weaker decrease in 27SB pre-rRNAlevels and in delayed conversion of the 27SA₂ pre-rRNA to 27SBspecies. In contrast to the above phenotypes, depletion of Spb4pand Dbp10p leads to the accumulation of 27SB pre-rRNAs within66S preribosomal particles (23, 41). The delayed conversionof 27SB species to mature 25S rRNA is more drastic in the absenceof Spb4p; therefore, Spb4p may be responsible for structural rearrangementsthat facilitate cleavage at site C₁ or C₂. The role of Drs1p inthe biogenesis of 60S ribosomal subunits is less clear, and itwas only shown that formation of 25S rRNA is impaired in the cold-sensitivedrs1-1 mutant (148). To characterize the functional environmentof Drs1p, a genetic screen for synthetic lethality with drs1 alleleswas carried out; this screen identified an essential nucleolarprotein that is homologous to pescadillo, which is an essentialgene for embryonic development in zebrafish (3, 149).

In contrast to the 16 putative RNA helicases described above, the involvement of the putative RNA helicase Sen1p in ribosomebiogenesis is most likely indirect. Sen1p seems to be involvedin pre-rRNA processing, since a mutation in SEN1 leads to delayed35S pre-rRNA processing (186); however, the same mutation alsoaffects the levels of intronic pre-tRNAs, snRNAs, and snoRNAsand furthermore leads to the mislocalization of several nucleolarproteins (185, 186). In addition, Sen1p has been reported tointeract with both H/ACA- and C/D-box snoRNAs (186) and to berequired for snoRNA maturation and stability (145).

	FACTORS INVOLVED IN RIBOSOME ASSEMBLY?

The course of the assembly of the different r-proteins into preribosomal particles has been studied mainly by monitoring thekinetics of incorporation of individual r-proteins into cytoplasmicand nuclear ribosomal particles after pulse-labeling of yeastprotoplasts with tritiated amino acids (93). These experimentsindicate that a large number of r-proteins associate with thenucleolar preribosomes at early steps in ribosome maturation,whereas others assemble at later steps or are even only addedin the cytoplasm (Fig. 2 and its legend) (93). It has also beenshown that three large-subunit r-proteins on mature 60S subunitscan exchange in vivo, and the exchangeability of Rpl10p/Qsr1p,in particular, which is required for 60S to 40S subunit joining,suggests the possibility of an additional translational regulatorymechanism (46, 209). Due to the lack of in vitro reconstitutionassays for eukaryotic ribosomes, the above-mentioned studies couldonly be complemented by approaches that examined the abilitiesof the different r-proteins to either bind to pre-rRNA moleculesin vitro (204) or dissociate from purified ribosomal particlesby increasing concentration of ions (52, 106). The affinityof r-proteins for pre-rRNAs and the release of r-proteins by increasingconcentration of ions are in general agreement with the orderof their association with the preribosomal particles during invivo ribosomal subunit assembly. However, the precise order ofthe assembly of the different r-proteins into preribosomal particleshas not yet been unveiled. The roles of the protein trans-actingfactors involved in ribosome assembly are even less clear. Moreover,it is often difficult to exclusively attribute an assembly functionto a protein trans-acting factor, since ribosome assembly andpre-rRNA processing are intimately linked. Indeed, mutation inor depletion of r-proteins generally leads to a pre-rRNA processingphenotype (12, 128, 195). Therefore, we expect that some ofthe above-mentioned protein trans-acting factors also contributein one way or another to ribosome assembly. In this section, wedescribe the protein trans-acting factors that could functionmainly in promoting structural rearrangement reactions duringthe assembly of the preribosomalparticles.

The function of only one protein trans-acting factor, Rrp7p, has so far been linked to the process of 40S ribosomal subunitassembly (Fig. 2). Depletion of Rrp7p leads to general inhibitionof the early pre-rRNA cleavage reactions at A₀ to A₂, with theA₂ site being the most affected. This results in a reduction of18S rRNA synthesis and in a decreased ratio of 40S to 60S ribosomalsubunits (12). Interestingly, the lethality of the $Delta$ rrp7 alleleis suppressed by overexpression of the nearly identical proteinsRps27Ap and Rps27Bp (12), which belong to a small group of 40Ssubunit r-proteins that assemble late into pre-40S ribosomal particles(Fig. 2) (93). This suggests that Rrp7p is required for thecorrect assembly of Rps27A/Bp into pre-40S ribosomal particles(12).

Mutation in or depletion of protein trans-acting factors involved in the assembly of 60S ribosomal subunits often leads toan abortive assembly, which can either entail disassembly of pre-60Sribosomal particles and destabilization of pre-rRNA intermediatesor accumulation of pre-60S ribosomal particles and stabilizationof pre-rRNA intermediates. Disassembly of pre-60S ribosomal particlesis thought to occur when the integrity of early-acting factorsis affected, whereas accumulation of pre-rRNA intermediates canbe attributed to the disfunctionality of late-acting factors (discussedin references 38, 41, and 88). In addition, it is conceivablethat some late assembly events are also critical for the formationof stable pre-60S ribosomal particles or mature 60S ribosomalsubunits. Depletion of Nop4p, Nop8p, and the putative RNA helicasesDbp6p and Dbp9p leads to decreased formation and steady-statelevels of 27S pre-rRNAs (15, 36, 88, 170, 207). Accordingto the above model, these protein trans-acting factors are supposedto act very early in the pathway of 60S ribosomal subunit assembly(Fig. 2). In agreement with a role of Dbp6p in early assemblyevents, two independent rpl3 mutants were identified in a syntheticlethal screen with conditional dbp6 alleles (91). RPL3 encodesthe L3 r-protein of the large ribosomal subunit, which has beenshown to belong to a group of r-proteins that associate earlywith preribosomal particles (Fig. 2) (93). Two further putativeRNA helicases, Dbp7p and Mak5p, are most likely required for earlyassembly reactions downstream of Nop4p, Nop8p, Dbp6p, and Dbp9p(38, 206). In contrast, depletion of the putative RNA helicasesSpb4p and Dbp10p leads to the accumulation of 27S pre-rRNAs within66S preribosomal particles (23, 41). This is in agreementwith their involvement in late assembly events. Delayed conversionof 27SB pre-rRNAs to mature 25S rRNAs and increased steady-statelevels of 27SB pre-rRNAs are also seen upon depletion of Nip7p(208). Nip7p seems to be a multifunctional protein, since itis localized in the nucleus with nucleolar enrichment and in thecytoplasm, where it is associated with free 60S ribosomal subunits(208). Nip7p interacts with both the exclusively nucleolar proteinNop8p and the exosome component Rrp43p, and intriguingly, depletionof either of these proteins leads to pre-rRNA processing phenotypesthat are clearly distinct from that observed upon depletion ofNip7p (126, 207). The ski6-2 mutation in another exosome component,Rrp41p/Ski6p, leads to the accumulation of a 38S particle containing5'-truncated 25S rRNA but no 5.8S rRNA; otherwise, this mutanthas normal amounts of 40S and 60S ribosomal subunits (14). This38S particle corresponds either to an incompletely assembled or,more likely, to a partially degraded 60S ribosomal subunit. Thelatter origin of the 38S particle could be explained by deficientcytoplasmic turnover of "old" 60S ribosomal subunits due to thedecreased 3' $right-arrow$ 5' exonuclease activity of Ski6-2p.

The nonessential gene RSA1 was identified in a genetic screen for synthetic lethality with dbp6 alleles (90). In the $Delta$ rsa1mutant, half-mer polysomes accumulate even though the pool offree 60S ribosomal subunits is only moderately decreased. Thisphenotype is similar to that observed in mutants defective in60S to 40S subunit joining (50, 51). The presence of Rpl10p/Qsr1pin 60S ribosomal subunits is necessary for 60S to 40S subunitjoining to occur (51). Accordingly, Rpl10p/Qsr1p is practicallyabsent from free 60S ribosomal subunits in $Delta$ rsa1 mutant strains(90). Moreover, combination of the $Delta$ rsa1 and qsr1-1 mutationsleads to a strong synthetic growth inhibition (90). Taken together,Rsa1p is likely to be involved in a late step of pre-60S ribosomalsubunit assembly that is required for efficient recruitment ofRpl10p/Qsr1p. Sqt1p is a cytoplasmic protein containing multipleWD repeats that interacts strongly with Rpl10p/Qsr1p in a yeasttwo-hybrid system. Moreover, overexpression of Sqt1p suppressesthe slow-growth phenotype of dominant negative qsr1 truncationmutants (50). Depletion of Sqt1p results in the formation ofhalf-mer polysomes and decreased levels of Rpl10p/Qsr1p on free60S ribosomal subunits (50). A likely explanation is that Sqt1pis involved in the assembly of Rpl10p/Qsr1p into 60S ribosomalsubunits late in the assembly pathway. The function of Nmd3p isalso genetically linked to Rpl10p/Qsr1p because dominant NMD3mutants suppress the growth defect of a temperature-sensitivemutation in RPL10/QSR1 (77). Nmd3p is a cytoplasmic proteinthat sediments at the position of free 60S ribosomal subunitsin sucrose gradients (67). Interestingly, the mature 25S rRNAis rapidly degraded in nmd3 mutant strains, as evidenced by pulse-chaseanalysis, which suggests that Nmd3p is required for the formationof stable 60S ribosomal subunits (67). The stability of 60Sribosomal subunits is also affected in strains depleted of Rpl5p,which assembles as the Rpl5p-5S RNP early into pre-60S ribosomalsubunits (43).

	UNCLASSIFIED PROTEIN TRANS-ACTING FACTORS

Rrp5p is perhaps one of the most interesting trans-acting factors belonging to this class. Rrp5p was identified in a screenfor mutations showing synthetic lethality with the $Delta$ snr10 allele.Rrp5p is the only factor that is simultaneously required for pre-rRNAprocessing at sites A₀, A₁, A₂, and A₃ (194) and therefore forthe synthesis of both the mature 18S and 5.8S_S rRNAs (194). Rrp5pis a large nucleolar protein composed of a modular structure oftwo different kinds of repeats. The N-terminal two-thirds of theprotein contains 12 repeats of the so-called S1 RNA-binding motif(S1-RM), while the C-terminal part contains seven tetratricopeptiderepeats (TPRs) (53, 179). S1-RM is most probably involved inthe binding of single-stranded regions in the rRNA (24). TheTPR motif is a degenerate sequence of 34 amino acids which canmediate inter- and intramolecular protein-protein interactions(104). Large portions of the S1-RM repeats and a short C-terminalfragment containing two TPRs can be individually deleted withoutdramatically affecting cell growth (53), suggesting some sortof functional redundancy among the repeats. Deletions in the S1-RMregion specifically inhibit processing at site A₃; therefore,this region of Rrp5p is required for the synthesis of 5.8S_S rRNA(53). Mutations or deletions in the TPRs affect pre-rRNA processingat sites A₀, A₁, and A₂, which leads to inhibition of 18S rRNAsynthesis (53, 179). Most importantly, Rrp5p can be physicallydivided into two fragments that act in trans to functionally replacethe integral protein (53, 179). One fragment contains mostof the S1-RM repeats, and the other covers the rest of the protein.Thus, both mutational analysis and trans-complementation nicelydemonstrate that the two domains of Rrp5p carry out two distinctfunctions. This supports a model in which Rrp5p acts as the "bridgingfactor" between the machineries required for A₀ to A₂ (snoRNPcomplexes) and A₃ processing (RNase MRP complex) (173). So far,genetic analyses have shown a functional interaction between Rrp5pand some snoRNP components (snR10 and Rok1p) (53, 179, 194),but such an interaction with the RNase MRP complex still remainsto beuncovered.

Two factors, Nop3p and Nsr1p, might mediate nucleocytoplasmic traffic of ribosomal components, although direct experimentalevidence for such an involvement is still lacking. Nop3p (alsoNpl3p) is an essential nuclear (and nucleolar) member of the GARdomain protein family (150). In addition to its GAR domain, whichis present in the C-terminal part of the protein, Nop3p containstwo central RRMs (150). A more recent study indicates that Nop3pshuttles between the nucleus and the cytoplasm (107); however,the observed steady-state nuclear localization indicates thatit must be rapidly reimported. In cells depleted of Nop3p, 27SBpre-rRNA processing is impaired and 27SB pre-rRNAs accumulate(150). In addition, nop3 mutants accumulate poly(A)⁺ RNA in the nucleus (107, 163). Therefore, it has been suggestedthat Nop3p acts as a carrier for poly(A)⁺ RNA export from the nucleus (107). Experimental evidence alsosuggests that Nop3p has an indirect role in protein uptake intothe nucleus (19, 163). Taken together, the pre-rRNA processingdefects observed upon Nop3p depletion can be explained in a modelin which Nop3p is involved in nucleocytoplasmic transport of pre-60Sribosomes; however, the possibility cannot be excluded that Nop3pis required for the nuclear import of any r-protein or proteintrans-acting factor. Nsr1p is a nucleolar protein that is structurallyand functionally similar to mammalian nucleolin (110). Nucleolinis a major nucleolar protein that shuttles between the nucleusand the cytoplasm, recognizes nuclear localization signals, andparticipates in many processes involving RNA, including pre-rRNAprocessing (60, 110, 183). Like Nop3p, Nsr1p contains twocentral RRMs and a C-terminal GAR domain. The N-terminal partconsists of a lysine-rich region followed by serine-rich segmentsand stretches enriched in acidic amino acids (85). Nsr1p isnot essential for cell viability, but $Delta$ nsr1 cells are severelyaffected in growth (85, 110). In addition, due to delayed A₀-to-A₂pre-rRNA processing, the $Delta$ nsr1 mutation results in reduced steady-statelevels of 20S pre-rRNA and mature 18S rRNA and therefore in adeficiency of 40S relative to 60S ribosomal subunits (85, 111).As for Nop3p, the precise role of Nsr1p in ribosome biogenesisis unknown; Nsr1p either plays a direct role in pre-rRNA processingand/or ribosome assembly or participates in the import of an r-proteinor another component required in the above-described processes(111).

Miscellaneous protein trans-acting factors such as Rrp1p (55) and Srd1p (65) have been identified genetically, whereasothers were obtained by specific genetic screens that yieldedclasses of mutants which preferentially affect ribosome biogenesis;these classes include the drs, spb, and mak mutants (137, 147,151). The drs (deficiency of ribosomal subunits) group was isolatedby screening of a collection of cold-sensitive mutants for alteredratios of free 40S to 60S ribosomal subunits or qualitative changesin polysome profiles (147). The drs mutants were grouped intoseven complementation groups, two affecting 60S ribosomal subunitproduction and five affecting 40S ribosomal subunit synthesis(147). Two DRS genes have been identified so far: DRS1 encodesa putative RNA helicase (see above) (148), and DRS2 encodes aplasma membrane ATPase whose function in ribosome biogenesis isunknown (147, 161). The spb mutants are extragenic suppressorsof a mutation in PAB1, which encodes poly(A)⁺ binding protein 1 (151). Except for spb8 (17) and pbp1 (121),all described spb mutations interfere with synthesis of 60S ribosomalsubunits (151). Spb2p is Rpl39p (152), Spb1p is a candidaterRNA methyltransferase (see above) (92), and Spb4p is a putativeRNA helicase (see above) (41, 152). About 30 different makcomplementation groups were identified as mutations that leadto loss of the M1 double-stranded RNA virus encoding the killertoxin (199). Like the spb mutants, most mak mutants are affectedin the biogenesis of 60S ribosomal subunits and no mak mutantshave been identified that are deficient in 40S ribosomal subunits(49, 137, 199). Some MAK genes encode r-proteins (i.e., Rpl3p,Rpl8Ap, and Rpl42Ap), while Mak5p, a putative RNA helicase (seeabove), and Mak21p are involved in the biogenesis of 60S ribosomalsubunits (49, 206). Further studies are required to revealhow qualitative and quantitative alterations of 60S ribosomalsubunits can specifically rescue a pab1 mutation or impede thepropagation of M1 double-stranded RNAviruses.

	CONCLUDING REMARKS AND PERSPECTIVES

Yeast molecular genetics has been a valuable tool for the identification and characterization of a large number of proteintrans-acting factors involved in eukaryotic ribosome biogenesis.However, we still do not understand the precise functions of mostof them and it is likely that many more protein trans-acting factorsplay a role in this complex process. Therefore, different biochemicaland genetic methods, including the systematic functional analysisof yeast open reading frames, have to be exploited in order firstto identify all of the protein trans-acting factors that are directlyinvolved in ribosome biogenesis and second to reveal the networkof physical interactions among the protein trans-acting factorsthemselves and their interactions with r-proteins and/or pre-rRNAs.This knowledge is a prerequisite for tackling the challenge ofunderstanding the timing of the action and the substrate specificityof the different protein trans-acting factors during the pre-rRNAprocessing and ribosome assembly reactions. These efforts shouldallow us to eventually draw a more detailed picture of the assemblyof the different r-proteins and the pre-rRNAs into preribosomesand their maturation to export- and translation-competent ribosomalsubunits.

	ACKNOWLEDGMENTS

We thank our many colleagues who have contributed unpublished results to this review, and we apologize to all those whosework could not be cited owing to space limitations. We are gratefulto K. Tanner, D. Tollervey, and J. Venema for stimulating discussionsand R. Boeck and K. Tanner for critical reading of the manuscript.J.D.L.C. thanks A. Vioque forencouragement.

The work in the authors' laboratory was funded by grants from the Swiss National Science Foundation and the University ofGeneva to P.L. We gratefully acknowledge C. Georgopoulos for support.J.D.L.C. thanks the MEC (Spain) for financialsupport.

	FOOTNOTES

^* Corresponding author. Mailing address: Instituto de Bioquímica Vegetal y Fotosíntesis, Centro de Investigaciones CientíficasIsla de la Cartuja, Avda. Américo Vespucio s/n, Isla de la Cartuja,E-41092 Sevilla, Spain. Phone: 34 95 4489519. Fax: 34 95 4460065.E-mail: jdlcd{at}cica.es.

REFERENCES

Top
Introduction
References

1. Abou Elela, S., and M. Ares, Jr. 1998. Depletion of yeast RNase III blocks correct U2 3' end formation and results in polyadenylated but functional U2 snRNA. EMBO J. 17:3738-3746[Medline].

2. Abou Elela, S., H. Igel, and M. Ares, Jr. 1996. RNase III cleaves eukaryotic preribosomal RNA at a U3 snoRNP-dependent site. Cell 85:115-124[Medline].

3. Allende, M. L., A. Amsterdam, T. Becker, K. Kawakami, N. Gaiano, and N. Hopkins. 1996. Insertional mutagenesis in zebrafish identifies two novel genes, pescadillo and dead eye, essential for embryonic development. Genes Dev. 10:3141-3155[Abstract/Free Full Text].

4. Allmang, C., Y. Henry, H. Wood, J. P. Morrissey, E. Petfalski, and D. Tollervey. 1996. Recognition of cleavage site A₂ in the yeast pre-rRNA. RNA 2:51-62[Abstract].

5. Allmang, C., E. Petfalski, A. Podtelejnikov, M. Mann, D. Tollervey, and P. Mitchell. 1999. The yeast exosome and human PM-Scl are related complexes of 3' $right-arrow$ 5' exonucleases. Genes Dev. 13:2148-2158[Abstract/Free Full Text].

6. Allmang, C., and D. Tollervey. 1998. The role of the 3' external transcribed spacer in yeast pre-rRNA processing. J. Mol. Biol. 278:67-78[Medline].

7. Amberg, D. C., A. L. Goldstein, and C. N. Cole. 1992. Isolation and characterization of RAT1: an essential gene of Saccharomyces cerevisiae required for the efficient nucleocytoplasmic trafficking of mRNA. Genes Dev. 6:1173-1189[Abstract/Free Full Text].

8. Apirion, D., and A. Miczak. 1993. RNA processing in prokaryotic cells. Bioessays 15:113-120[Medline].

9. Bachellerie, J.-P., and J. Cavaillé. 1998. Small nucleolar RNAs guide the ribose methylations of eukaryotic rRNAs, p. 255-272. In H. Grosjean, and R. Benne (ed.), Modification and editing of RNA. ASM Press, Washington, D.C.

10. Bagni, C., and B. Lapeyre. 1998. Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element. J. Biol. Chem. 273:10868-10873[Abstract/Free Full Text].

11. Balakin, A. G., L. Smith, and M. J. Fournier. 1996. The RNA world of the nucleolus: two major families of small RNAs defined by different box elements with related functions. Cell 86:823-834[Medline].

12. Baudin-Baillieu, A., D. Tollervey, C. Cullin, and F. Lacroute. 1997. Functional analysis of Rrp7p, an essential yeast protein involved in pre-rRNA processing and ribosome assembly. Mol. Cell. Biol. 17:5023-5032[Abstract].

13. Beltrame, M., Y. Henry, and D. Tollervey. 1994. Mutational analysis of an essential binding site for the U3 snoRNA in the 5' external transcribed spacer of yeast pre-rRNA. Nucleic Acids Res. 22:5139-5147[Abstract/Free Full Text].

14. Benard, L., K. Carroll, R. C. P. Valle, and R. B. Wickner. 1998. Ski6p is a homolog of RNA-processing enzymes that affects translation of non-poly(A) mRNAs and 60S ribosomal subunit biogenesis. Mol. Cell. Biol. 18:2688-2696[Abstract/Free Full Text].

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

16. Bertrand, E., F. Houser-Scott, A. Kendall, R. H. Singer, and D. R. Engelke. 1998. Nucleolar localization of early tRNA processing. Genes Dev. 12:2463-2468[Abstract/Free Full Text].

17. Boeck, R., B. Lapeyre, C. E. Brown, and A. B. Sachs. 1998. Capped mRNA degradation intermediates accumulate in the yeast spb8-2 mutant. Mol. Cell. Biol. 18:5062-5072[Abstract/Free Full Text].

18. Bortolin, M.-L., P. Ganot, and T. Kiss. 1999. Elements essential for accumulation and function of small nucleolar RNAs directing site-specific pseudouridylation of ribosomal RNAs. EMBO J. 18:457-469[Medline].

19. Bossie, M. A., C. DeHoratius, G. Barcelo, and P. Silver. 1992. A mutant nuclear protein with similarity to RNA binding proteins interferes with nuclear import in yeast. Mol. Biol. Cell 3:875-893[Abstract].

20. Bousquet-Antonelli, C., Y. Henry, J.-P. Gélugne, M. Caizergues-Ferrer, and T. Kiss. 1997. A small nucleolar RNP protein is required for pseudouridylation of eukaryotic ribosomal RNAs. EMBO J. 16:4770-4776[Medline].

21. Brand, R. C., J. Klootwijk, T. J. M. van Steenbergen, A. J. de Kok, and R. J. Planta. 1977. Secondary methylation of yeast ribosomal precursor RNA. Eur. J. Biochem. 75:311-318[Medline]

1.	Abou Elela, S., and M. Ares, Jr. 1998. Depletion of yeast RNase III blocks correct U2 3' end formation and results in polyadenylated but functional U2 snRNA. EMBO J. 17:3738-3746[Medline].
2.	Abou Elela, S., H. Igel, and M. Ares, Jr. 1996. RNase III cleaves eukaryotic preribosomal RNA at a U3 snoRNP-dependent site. Cell 85:115-124[Medline].
3.	Allende, M. L., A. Amsterdam, T. Becker, K. Kawakami, N. Gaiano, and N. Hopkins. 1996. Insertional mutagenesis in zebrafish identifies two novel genes, pescadillo and dead eye, essential for embryonic development. Genes Dev. 10:3141-3155[Abstract/Free Full Text].
4.	Allmang, C., Y. Henry, H. Wood, J. P. Morrissey, E. Petfalski, and D. Tollervey. 1996. Recognition of cleavage site A₂ in the yeast pre-rRNA. RNA 2:51-62[Abstract].
5.	Allmang, C., E. Petfalski, A. Podtelejnikov, M. Mann, D. Tollervey, and P. Mitchell. 1999. The yeast exosome and human PM-Scl are related complexes of 3' $right-arrow$ 5' exonucleases. Genes Dev. 13:2148-2158[Abstract/Free Full Text].
6.	Allmang, C., and D. Tollervey. 1998. The role of the 3' external transcribed spacer in yeast pre-rRNA processing. J. Mol. Biol. 278:67-78[Medline].
7.	Amberg, D. C., A. L. Goldstein, and C. N. Cole. 1992. Isolation and characterization of RAT1: an essential gene of Saccharomyces cerevisiae required for the efficient nucleocytoplasmic trafficking of mRNA. Genes Dev. 6:1173-1189[Abstract/Free Full Text].
8.	Apirion, D., and A. Miczak. 1993. RNA processing in prokaryotic cells. Bioessays 15:113-120[Medline].
9.	Bachellerie, J.-P., and J. Cavaillé. 1998. Small nucleolar RNAs guide the ribose methylations of eukaryotic rRNAs, p. 255-272. In H. Grosjean, and R. Benne (ed.), Modification and editing of RNA. ASM Press, Washington, D.C.
10.	Bagni, C., and B. Lapeyre. 1998. Gar1p binds to the small nucleolar RNAs snR10 and snR30 in vitro through a nontypical RNA binding element. J. Biol. Chem. 273:10868-10873[Abstract/Free Full Text].
11.	Balakin, A. G., L. Smith, and M. J. Fournier. 1996. The RNA world of the nucleolus: two major families of small RNAs defined by different box elements with related functions. Cell 86:823-834[Medline].
12.	Baudin-Baillieu, A., D. Tollervey, C. Cullin, and F. Lacroute. 1997. Functional analysis of Rrp7p, an essential yeast protein involved in pre-rRNA processing and ribosome assembly. Mol. Cell. Biol. 17:5023-5032[Abstract].
13.	Beltrame, M., Y. Henry, and D. Tollervey. 1994. Mutational analysis of an essential binding site for the U3 snoRNA in the 5' external transcribed spacer of yeast pre-rRNA. Nucleic Acids Res. 22:5139-5147[Abstract/Free Full Text].
14.	Benard, L., K. Carroll, R. C. P. Valle, and R. B. Wickner. 1998. Ski6p is a homolog of RNA-processing enzymes that affects translation of non-poly(A) mRNAs and 60S ribosomal subunit biogenesis. Mol. Cell. Biol. 18:2688-2696[Abstract/Free Full Text].
15.	Bergès, T., E. Petfalski, D. Tollervey, and E. C. Hurt. 1994. Synthetic lethality with fibrillarin identifies NOP77p, a nucleolar protein required for pre-rRNA processing and modification. EMBO J. 13:3136-3148[Medline].
16.	Bertrand, E., F. Houser-Scott, A. Kendall, R. H. Singer, and D. R. Engelke. 1998. Nucleolar localization of early tRNA processing. Genes Dev. 12:2463-2468[Abstract/Free Full Text].
17.	Boeck, R., B. Lapeyre, C. E. Brown, and A. B. Sachs. 1998. Capped mRNA degradation intermediates accumulate in the yeast spb8-2 mutant. Mol. Cell. Biol. 18:5062-5072[Abstract/Free Full Text].
18.	Bortolin, M.-L., P. Ganot, and T. Kiss. 1999. Elements essential for accumulation and function of small nucleolar RNAs directing site-specific pseudouridylation of ribosomal RNAs. EMBO J. 18:457-469[Medline].
19.	Bossie, M. A., C. DeHoratius, G. Barcelo, and P. Silver. 1992. A mutant nuclear protein with similarity to RNA binding proteins interferes with nuclear import in yeast. Mol. Biol. Cell 3:875-893[Abstract].
20.	Bousquet-Antonelli, C., Y. Henry, J.-P. Gélugne, M. Caizergues-Ferrer, and T. Kiss. 1997. A small nucleolar RNP protein is required for pseudouridylation of eukaryotic ribosomal RNAs. EMBO J. 16:4770-4776[Medline].
21.	Brand, R. C., J. Klootwijk, T. J. M. van Steenbergen, A. J. de Kok, and R. J. Planta. 1977. Secondary methylation of yeast ribosomal precursor RNA. Eur. J. Biochem. 75:311-318[Medline]

MINIREVIEW Protein trans-Acting Factors Involved in Ribosome Biogenesis in Saccharomyces cerevisiae

MINIREVIEW
Protein trans-Acting Factors Involved in Ribosome Biogenesis in Saccharomyces cerevisiae