Bop1 Is a Mouse WD40 Repeat Nucleolar Protein Involved in 28S and 5.8S rRNA Processing and 60S Ribosome Biogenesis

doi:10.1128/MCB.20.15.5516-5528.2000

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Strezoska, Z.
	Articles by Lau, L. F.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Strezoska, Z.
	Articles by Lau, L. F.

Molecular and Cellular Biology, August 2000, p. 5516-5528, Vol. 20, No. 15
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Bop1 Is a Mouse WD40 Repeat Nucleolar Protein Involved in 28S and 5.8S rRNA Processing and 60S Ribosome Biogenesis

$Z$ aklina Strezoska, Dimitri G. Pestov, and Lester F. Lau^*

Department of Molecular Genetics, University of Illinois at Chicago College of Medicine, Chicago, Illinois 60607-7170

Received 8 March 2000/Returned for modification 15 April 2000/Accepted 11 May 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We have identified and characterized a novel mouse protein, Bop1, which contains WD40 repeats and is highly conserved throughevolution. bop1 is ubiquitously expressed in all mouse tissuesexamined and is upregulated during mid-G₁ in serum-stimulatedfibroblasts. Immunofluorescence analysis shows that Bop1 is localizedpredominantly to the nucleolus. In sucrose density gradients,Bop1 from nuclear extracts cosediments with the 50S-80S ribonucleoproteinparticles that contain the 32S rRNA precursor. RNase A treatmentdisrupts these particles and releases Bop1 into a low-molecular-weightfraction. A mutant form of Bop1, Bop1 $Delta$ , which lacks 231 aminoacids in the N- terminus, is colocalized with wild-type Bop1 inthe nucleolus and in ribonucleoprotein complexes. Expression ofBop1 $Delta$ leads to cell growth arrest in the G₁ phase and resultsin a specific inhibition of the synthesis of the 28S and 5.8SrRNAs without affecting 18S rRNA formation. Pulse-chase analysesshow that Bop1 $Delta$ expression results in a partial inhibition inthe conversion of the 36S to the 32S pre-rRNA and a complete inhibitionof the processing of the 32S pre-rRNA to form the mature 28S and5.8S rRNAs. Concomitant with these defects in rRNA processing,expression of Bop1 $Delta$ in mouse cells leads to a deficit in the cytosolic60S ribosomal subunits. These studies thus identify Bop1 as anovel, nonribosomal mammalian protein that plays a key role inthe formation of the mature 28S and 5.8S rRNAs and in the biogenesisof the 60S ribosomalsubunit.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Biogenesis of the eukaryotic ribosomes occurs in the nucleolus, a complex nuclear organelle that forms around the nucleolarorganizer regions located in heterochromatic chromosomal sitescontaining multiple rRNA genes (69, 81). The organizationof the nucleolus and the assembly of ribosomes are coupled totranscription of rDNA by RNA polymerase I, which synthesizes alarge primary precursor transcript. This precursor transcriptis then processed into the mature 18S, 5.8S, and 28S/25S rRNAs.These rRNAs are assembled into preribosomes with some 80 ribosomalproteins that are transported into the nucleus, and with the 5SrRNA, transcribed by RNA polymerase III outside of the nucleolus(28). A large number of small nucleolar RNAs (snoRNAs) and nonribosomalproteins are also recruited to the nucleolus to participate inthe modification, processing, and assembly of the rRNAs and proteinsinto ribonucleoprotein (RNP) particles. These preribosomal RNP(pre-rRNP) particles mature into nearly complete ribosomal subunitsprior to their export out of thenucleus.

Upon synthesis, the primary precursor rRNA transcript is modified by ribose methylation and pseudouridine conversion and processedthrough a series of nucleolytic cleavages into the matured rRNAs(21) (see Fig. 6). In vertebrates, the arrangement of the 47Sprimary precursor transcript begins with a 5' external transcribedspacer (5'-ETS), followed by the 18S rRNA, internal transcribedspacer 1 (ITS1), 5.8S rRNA, internal transcribed spacer 2 (ITS2),28S rRNA, and the 3' external transcribed spacer (3'-ETS). Althoughin general, processing events occur in a polar fashion from the5' to the 3' end of the nascent transcript, differences in theorder of processing events and intermediates generated have beenreported for different cell types (8, 31, 56). A similararrangement of the primary transcript is also found in yeasts(79), and it is generally thought that while specific processingsites might differ between yeasts and vertebrates, parallel processingpathways appear to exist for eukaryotic organisms from yeaststo mammals (75).

A large number of snoRNAs and nonribosomal nucleolar proteins play critical roles in ribosome biogenesis (21, 75). Morethan 150 snoRNAs have been found in the nucleolus, and some ofthem play key roles in various pre-rRNA processing events includingnucleotide modification and cleavage reactions (45, 76, 83).Although a large number of snoRNAs have been identified and characterized,less is known about the functions of the nonribosomal proteinsin the RNP particles, especially in mammalian systems. Many ofthe recent advances made in the identification of protein factorsinvolved in rRNA processing have come from genetic and biochemicalanalyses in yeast. Among the yeast proteins known to participatein rRNA processing are endoribonucleases (Rnt1p and RNase MRP)(22, 44), 5' $right-arrow$ 3' exoribonucleases (Xrn1p and Rat1p) (35,39), nearly a dozen 3' $right-arrow$ 5' exoribonucleases that comprise theexosome (1, 48), putative ATP-dependent RNA helicases (Drs1p,Sbp4p, Rrp3p, and Rok1p) (18, 54, 78), and a number of noncatalyticnucleolar proteins (Nop1p, Nop2p, Nopp3p, etc.) (34, 36, 66).The total number of nonribosomal proteins involved in rRNA processingis unknown but is likely to be large, as underscored by the complexityof eukaryotic rRNA modification, processing, and ribosomeassembly.

In mammalian systems, relatively few nonribosomal nucleolar proteins have been characterized; the best-studied examples includefibrillarin, a common component of the snoRNPs (43, 53); nucleolin(C23), a pre-rRNA binding protein with multiple functions in processingand ribosome assembly (29, 55, 77); B23, associated withribosome assembly at later stages of maturation (11); and p120,a nucleolar RNA binding protein that cofractionates with 60S-80Spre-rRNA particles (30, 33). In comparison with yeast, themajority of the molecular players in the mammalian rRNA processingmachinery remain unidentified, and their characterization willbe necessary to understand fully the mechanism of rRNA processingand ribosomalassembly.

In a previous study, a genetic selection for growth-inhibitory sequences in mouse cells identified a cDNA, bop1 $Delta$ , whose inducibleexpression results in a powerful but reversible block in the G₁phase (58). Further analysis revealed that bop1 $Delta$ representsa cDNA fragment that encodes an N-terminally truncated form ofa novel protein, Bop1. Sequence analysis showed that bop1 is anevolutionarily conserved gene that encodes an 83-kDa protein withfour WD40 repeats (Fig. 1) (58). The WD40 repeat is a sequencemotif found in a diverse group of functionally distinct proteinsinvolved in the regulation of myriad cellular processes, includingsignal transduction, gene transcription, and mRNA modification(51). Moreover, WD40 proteins are often found to form multiproteincomplexes, suggesting that the WD40 motifs may be involved inprotein-protein interactions (7, 14, 60).

View larger version (13K):
[in this window]
[in a new window]

FIG. 1. Structural features of the Bop1 protein. Schematic representation of the full-length murine Bop1 protein (732 aa) and the amino-terminally truncated Bop1 $Delta$ (501 aa). The four WD repeats, whose consensus structure is as indicated, are shown as solid boxes. Repeats 1 and 4 are close to the consensus structure, while repeats 2 and 3 are more divergent. PEST sequences, often associated with short-lived regulatory proteins, are shown by hatched boxes.

In this study, we demonstrated that Bop1 is a novel component of the 28S branch of the rRNA processing machinery. Bop1 islocalized to the nucleolus and forms part of the large RNP particlesthat probably represent preribosomes. Expression of its N-terminallytruncated mutant form, Bop1 $Delta$ , specifically inhibits the processingof the 32S precursor to form the mature 5.8S and 28S rRNAs andresults in a deficiency of the 60S ribosomal subunits. These resultsidentify Bop1 as a previously unknown player in the processingof the 32S pre-rRNA and in the biogenesis of the 60S ribosomalsubunits and suggest that Bop1 may interact with and coordinatethe activities of proteins that comprise the pre-RNA processingmachinery.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression plasmids. An IPTG (isopropyl- $beta$ -D-thiogalactopyranoside)-inducible expression vector, pX11, drives inducible expression with low backgroundin LAP3 cells (59). Expression constructs with cDNAs encodingeither Bop1 or Bop1 $Delta$ cloned into pX11 have been described previously(58). To express Bop1 or Bop1 $Delta$ N-terminally tagged with a hemagglutininantigen (HA) sequence, a polynucleotide linker encoding the HAtag (23) was inserted into these vectors. To express Bop1 asa glutathione S-transferase (GST) fusion protein in Escherichiacoli, an EcoRI restriction fragment of Bop1 (GenBank accessionno. U77415) corresponding to nucleotides (nt) 442 to 2461 wascloned into pGEX-4T-1 (Pharmacia). To express Bop1 in insect cellsvia a baculovirus expression vector, the full-length 2.4-kb bop1cDNA fragment was cloned in pBlueBacHis2A (Invitrogen), therebydriving the expression of a full-length Bop1 protein with an N-terminal6-histidinetag.

Cell culture. BALB/c 3T3 cells were grown in MEM-10 (minimal essential medium with 10% fetal bovine serum). The cells were brought to quiescenceby growth to confluence and serum starved in MEM-0.5 for 2 days;serum stimulation was accomplished by changing the medium to MEM-10.LAP3 is a clonal cell line derived from NIH 3T3 cells that constitutivelyexpresses the IPTG-inducible transactivator protein LAP267 (5).To create various clonal cell lines, LAP3 cells were cotransfectedwith a hygromycin marker plasmid pHyg (73) and either the emptypX11 vector (line 1-1), pX11-Bop1 (line 45), pX11-Bop1 $Delta$ (lines6 and 8), pX11-HA-Bop1 (line 10), or pX11-HA-Bop1 $Delta$ (line 13) usingthe calcium phosphate coprecipitation method (12). Clonal celllines were selected following transfection by growth in 130 to150 µg of hygromycin (Boehringer Mannheim) per ml. LAP3-derivedcell lines were maintained in Dulbecco's modified Eagle's mediumcontaining 10% calf serum (HyClone) and penicillin-streptomycin(Gibco-BRL). IPTG (dioxane free; Sigma) was added to 1 mM whereindicated.

RNA blot analysis. Where indicated (except for Fig. 11), RNA was isolated using Trizol reagent (Gibco-BRL) as specified by the manufacturer. Thesamples in the experiment shown in Fig. 11 were withdrawn fromsucrose density gradients, treated with proteinase K, and subjectedto phenol-chloroform extraction and isopropanol precipitation.Northern blot hybridization was performed by standard methods(68). The bop1 cDNA probe was synthesized by random primingin the presence of [³²P]dCTP (Decaprime II kit; Ambion). A 40-mer oligonucleotide (5'-GCGTTCGAAGTGTCGATGATCAATGTGTCCTGCAATTCAC-3')complementary to nt 68 to 108 of the 5.8S rRNA and a 33-mer oligonucleotide(5'-ACTGGTGAGGCAGCGGTCCGGGAGGCGCCGACG-3') complementary to nt1480 to 1512 of the ITS2 region of the pre-rRNA were 5'-end labeledusing [ $gamma$ -³²P]ATP and T4 polynucleotidekinase.

Anti-Bop1 antibodies and affinity purification. To raise polyclonal anti-Bop1 antibodies, a Bop1 polypeptide corresponding to amino acids (aa) 131 to 732 was expressed asa GST fusion protein in E. coli (see above). The fusion proteinformed insoluble inclusion bodies, which were solubilized in 5M urea and subjected to sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) (6% polyacrylamide). The GST-Bop1protein band was excised from the gel, and the protein was usedfor immunization of rabbits at the Immunological Resource Centerat University of Illinois at Urbana. Antisera raised against thisfusion protein were affinity purified by a standard method (32)by passage through a Bop1-Sepharose column. To prepare the affinitycolumn, full-length Bop1 with an N-terminal histidine tag wasexpressed in SF9 cells using a baculovirus expression system (Invitrogen)and purified using Pro-Bond resin (Invitrogen) under denaturingconditions as specified by the manufacturer. The protein was furtherdialyzed against 125 mM sodium phosphate (pH 8)-500 mM NaCl andcoupled to cyanogen bromide-activated Sepharose (5 mg of proteinper ml of Sepharose slurry) as specified by the manufacturer (Pharmacia).The anti-Bop1 antiserum was diluted 1:10 in phosphate-bufferedsaline (PBS), passed through the Bop1-Sepharose column, and washedwith 10 mM Tris (pH 7.5)-500 mM NaCl. Bound antibodies were firsteluted with 100 mM glycine (pH 2.5) and then eluted with 100 mMethanolamine (pH 11.5). Eluates were combined, dialyzed againstPBS, and concentrated with Centricon-30 columns (Amicon) or ona protein A-Sepharose column (68).

Western blot analysis. Cells were lysed in radioimmunoprecipitation assay (RIPA) buffer (68), and equal amounts of protein, determined by the DCprotein assay (Bio-Rad), were resolved by SDS-PAGE. For immunoblotanalysis of the sucrose gradient fractions, the proteins fromeach fraction were precipitated with cold 10% trichloroaceticacid and dissolved in 80 µl of Laemmli buffer, half of which wasresolved by SDS-PAGE. Western blot analysis was done by standardmethods (2) using affinity-purified anti-Bop1antibodies.

To analyze proteins associated with ribosomal particles in the nucleus and the cytoplasm, cells were lysed as described belowfor the preparation of nuclear extracts. The cytoplasmic fractionand nuclear sonicate were cleared at 15,000 × g for 15 min andthen centrifuged through 10% sucrose in 10 mM Tris-HCl (pH 7.2)-60mM KCl-10 mM MgSO₄-1 mM dithiothreitol (DTT) at 160,000 × g for4 h at 5°C. The pellets were dissolved in 1% SDS and used forthe isolation of RNA with Trizol and protein analysis by SDS-PAGE.The volumes loaded on a protein gel were normalized for the RNAcontent of the samples as determined by absorbance at 260 nm andelectrophoresis on a formaldehyde-containing agarose gel followedby staining with SYBR Gold (Molecular Probes, Inc.).

Indirect immunofluorescence. Cells were grown on coverslips, incubated with IPTG for 12 h, fixed with paraformaldehyde, permeabilized with 0.5% TritonX-100, and incubated for 1 h at room temperature with either monoclonalanti-HA antibody (Babco), polyclonal anti-HA antibodies (Babco),affinity-purified anti-Bop1 antibodies, or the anti-fibrillarinmonoclonal antibody (72B9) diluted in PBS containing 0.5% bovineserum albumin. After being washed, the cells were incubated witheither fluorescein isothiocyanate (FITC)-conjugated or Texas Red-conjugatedanti-mouse antibodies (Vector Laboratories) or FITC-conjugatedanti-rabbit antibodies (Zymed) and analyzed using a MicroMAX digitalcamera mounted on a Axioplan II Zeiss microscope with differentialinterference contrast (DIC)optics.

Metabolic labeling and analysis of RNA transcripts. Various cell lines were plated in six-well plates at 10⁵ cells per well. One day after being plated, the cells were eitherleft untreated or treated with IPTG for 16 h to induce expression.To measure RNA synthesis, the cells were incubated in medium with[³H]uridine (2.5 µCi/ml) for 30 min and then in nonradioactive mediumfor 2 h. RNA was isolated using Trizol, and label incorporationwas measured by scintillation counting. RNA was subsequently separatedon a 1% agarose gel and transferred to a nylon membrane, whichwas treated with En³Hance (New England Nuclear) and exposed to film. Pulse-chase experimentswere carried out using L-[methyl-³H]methionine due to the rapid turnover of the cellular methioninepool. Cells were preincubated for 15 min in methionine-free mediumand then incubated for 30 min in medium containing L-[methyl-³H]methionine (50 µCi/ml). The cells were then chased in nonradioactivemedium containing 15 µg of methionine per ml for various times,after which the RNA was isolated using Trizol. RNA from the samenumber of cells was analyzed as described above. Where indicated,cells were treated with 5 µM 5-fluorouridine (FUrd) for 15 minprior to labeling. For analysis of the synthesis of 5.8S RNA,³²P labeling was used to increase the sensitivity of detection.Cells to be labeled with radioactive phosphate were pretreatedin phosphate-free medium for 1 h, labeled in medium with [³²P]orthophosphate (³²P_i) (20 µCi/ml) for 1 h, and chased in nonradioactive medium for1.5 h. RNA from the same number of cells was separated on a 10%polyacrylamide-7 M ureagel.

Sucrose density gradient fractionation. To fractionate cytoplasmic ribosomes, cells were harvested by trypsinization 5 min after the addition of 50 µg of cycloheximideper ml to the medium. Equal numbers of cells (determined witha Coulter counter) from each sample were pelleted by low-speedcentrifugation and lysed in 20 mM Tris-HCl (pH 7.2)-130 mM KCl-10mM MgCl₂-2.5 mM DTT-0.5% NP-40-0.5% sodium deoxycholate-10 µgof cycloheximide per ml-0.2 mg of heparin per ml-200 U of RNasinper ml (Promega) for 15 min at 4°C. The lysates were centrifugedat 8,000 × g for 10 min, and the supernatants were layered on10 to 45% (wt/wt) sucrose density gradients in 10 mM Tris-HCl(pH 7.2)-60 mM KCl-10 mM MgCl-1 mM DTT-0.1 mg of heparin per ml.The gradients were centrifuged at 36,000 rpm for 3 h at 5°C ina Beckman SW41Ti rotor and fractionated by upward displacementthrough a Bio-Rad EM-1 UV monitor for continuous measurement ofthe absorbance at 254 nm. Sedimentation constants were calculatedas described previously (46).

To fractionate nuclear extracts, cells were washed twice in PBS and once in ice-cold hypotonic wash buffer (10 mM Tris [pH7.4], 10 mM KCl, 2 mM MgCl) and then left to swell for 20 minin hypotonic lysis buffer (10 mM Tris [pH 7.4], 10 mM KCl, 2 mMMgCl, 0.05% Triton X-100, 1 mM EGTA, 1 mM DTT, 40 µg of phenylmethylsulfonylfluoride per ml, 10 µl of protease inhibitor cocktail [Sigma]per ml) (40). The cells were forced through a 25-gauge needleand centrifuged for 5 min at 700 × g to obtain a pellet of nuclei,which was resuspended in 25 mM Tris (pH 7.5)-100 mM KCl-1 mM DTT-2mM EDTA-0.05% NP-40-1 mM NaF-40 µg of phenylmethylsulfonyl fluorideper ml-10 µl of protease inhibitor cocktail per ml-0.1 U of RNasin(Promega) per ml and sonicated four times for 15 s each with amicrotip (Heat Systems Ultrasonics, Inc.). The nuclear lysatewas centrifuged at 15,000 × g for 15 min, and the resulting supernatantwas overlaid on 10 to 30% (wt/wt) sucrose gradients in 25 mM Tris(pH 7.5)-100 mM KCl-1 mM DTT-2 mM EDTA and centrifuged at 36,000rpm for 3 h at 5°C in a Beckman SW41Ti rotor. Where indicated,the nuclear extract was treated with RNase A (100 µg/ml) for 10min at 30°C before being loaded on the gradient. The gradientswere analyzed asabove.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression of the bop1 gene. Expression of an N-terminally truncated form of Bop1, Bop1 $Delta$ , results in a strong but reversible G₁ growth arrest (58). Thisobservation raised the possibility that the activity of Bop1 mightaffect cell cycle progression and that expression of the bop1gene might be linked to the proliferative state. To determineif bop1 expression is growth regulated, we analyzed RNA isolatedfrom BALB/c 3T3 cells stimulated to reenter the cell cycle fromquiescence (Fig. 2A). bop1 expression was low in quiescent cellsand was induced after serum stimulation, starting at 5 h, reachingmaximal level at 8 h, and slowly declining thereafter. Thus, bop1expression increases in cells stimulated to proliferate, withmaximal expression in mid-G₁. A survey of RNA isolated from variousmouse tissues showed the presence of the 2.6-kb bop1 mRNA in alltissues tested, with the highest level in the testis (Fig. 2B).

View larger version (63K):
[in this window]
[in a new window]

FIG. 2. Expression of bop1. (A) BALB/c 3T3 cells were brought to quiescence (Q) by serum starvation and restimulated with 10% fetal bovine serum. RNA was isolated at the indicated times (in hours) after serum stimulation and analyzed by Northern blotting with ³²P-labeled bop1 cDNA as probe. The RNA blot was stained with methylene blue (lower panel) to show the relative amounts of rRNAs, indicating equal loading of the samples. (B) RNA was isolated from different adult mouse tissues and analyzed by Northern blotting with labeled bop1 cDNA as probe. The lower panel shows methylene blue staining of the same blot to control for loading of the RNA.

Bop1 and Bop1 $Delta$ are localized in the nucleolus. In an effort to determine the function of Bop1, we ascertained its subcellular localization. First, we prepared IPTG-inducibleexpression constructs that drive the expression of either HA-taggedBop1 or Bop1 $Delta$ in LAP3 cells, an NIH 3T3-derived cell line thatsupports IPTG-regulated gene expression (see Materials and Methods).Stable pools of transfected LAP3 cells were induced with IPTGand subjected to immunofluorescence analysis using monoclonalanti-HA antibody (Fig. 3A and B). Cells that express either HA-taggedBop1 or HA-tagged Bop1 $Delta$ showed strong antibody staining in thenucleoli, although a weak and diffuse nucleoplasmic staining wasalso observed. Examination of the same fields using DIC opticsconfirmed the nucleolar localization. Double staining with polyclonalanti-HA antibodies and a monoclonal antifibrillarin antibody (72B9)(62) also confirmed the nucleolar localization of the HA-taggedBop1 and Bop1 $Delta$ (data not shown).

View larger version (184K):
[in this window]
[in a new window]

FIG. 3. Subcellular localization of Bop1 by indirect immunofluorescence. (A and B) Pools of LAP3 cells stably transfected with vectors that express HA-tagged Bop1 (A) or Bop1 $Delta$ (B) were grown on coverslips, induced with IPTG for 12 h, fixed, permeabilized, and stained with monoclonal anti-HA antibody. Antibody-antigen complexes were detected with FITC-conjugated anti-mouse antibody and visualized by fluorescence microscopy. An image of the same field visualized with DIC optics is shown in the lower panels. (C and D) To localize the endogenous Bop1 protein, LAP3 cells were grown on coverslips, fixed, permeabilized, and stained with affinity-purified, polyclonal anti-Bop1 antibodies (C) or the preimmune serum as a control (D).

To reinforce and substantiate the above findings, we determined the subcellular localization of the endogenous Bop1 proteinby using affinity-purified anti-Bop1 antibodies (see Materialsand Methods). These antibodies reacted specifically with Bop1in cell lysates on a denaturing Western blot, where Bop1 exhibitedan apparent molecular mass of ~100 kDa (larger than the calculatedsize of 83 kDa) (Fig. 4). These antibodies were used to demonstratethat various IPTG-inducible cell lines express the appropriategene products upon induction (Fig. 4). Using these antibodies,endogenous Bop1 was also localized to the nucleolus by immunofluorescenceanalysis whereas preimmune serum from the same rabbit did notshow any staining (Fig. 3C and D). No anti-Bop1 staining was detectedin the cytoplasm, although a low level of diffuse staining wasalso detected in the nucleoplasm. Together, these results showthat both endogenous Bop1 and exogenously expressed Bop1 or Bop1 $Delta$ are localized predominantly in the nucleolus.

View larger version (56K):
[in this window]
[in a new window]

FIG. 4. Characterization of the affinity-purified anti-Bop1 antibodies. Clonal lines of LAP3 cells stably transfected with either the empty vector pX11 (line 1-1), pX11-Bop1 (line 45), pX11-Bop1 $Delta$ (line 6), pX11-HA-Bop1 (line 10), or pX11-HA-Bop1 $Delta$ (line 13) were either treated with 1 mM IPTG (+) for 12 h or left untreated ( $-$ ). Cells were lysed in RIPA buffer, and equal amounts of protein from each sample were resolved by SDS-PAGE (8% polyacrylamide) and transferred to a nitrocellulose filter. The blot was incubated with affinity-purified anti-Bop1 antibodies, and chemiluminescent reagents were used for detection. The affinity-purified antibodies recognized a high-molecular-mass band of ~100 kDa (larger than the expected size of 83 kDa), which was increased significantly in a Bop1-overexpressing cell line (line 45). The predicted 55-kDa Bop1 $Delta$ fragment was detected in line 6, which inducibly expresses Bop1 $Delta$ . Addition of the HA tag caused a minor shift in the mobility of both Bop1 and Bop1 $Delta$ in clonal lines 10 and 13, respectively.

Involvement of Bop1 in rRNA processing. The localization of Bop1 in the nucleolus $---$ the site of rRNA synthesis, modification, processing, and ribosome biogenesis $---$ suggeststhat it may play a role in one or more of these processes. ThatBop1 $Delta$ is colocalized with Bop1 and its expression inhibits cellgrowth suggests that it might interfere with the normal functionof Bop1, most probably acting as a dominant negativemutant.

To investigate the function of Bop1, we first examined whether expression of Bop1 or Bop1 $Delta$ affects rRNA synthesis. For thispurpose, we created a set of cell lines that express Bop1 or Bop1 $Delta$ in an IPTG-inducible manner (see Materials and Methods). Theseinducible cell lines were either untreated or treated with IPTG,metabolically labeled with [³H]uridine for 30 min, and subjected to a 2-h chase. Inducibleoverexpression of Bop1 (line 45) showed no effect on the synthesisof the large rRNA precursors (45S and 32S) or the mature 18S and28S rRNAs, resulting in an rRNA pattern indistinguishable fromthat of the untreated cells or the control cell line (line 1-1;the parental LAP3 cells transfected with the empty cloning vector)(Fig. 5). By contrast, expression of Bop1 $Delta$ (lines 6 and 8) stronglyinhibited production of the 28S rRNA whereas the levels of 18SrRNA and the 45S precursor were unchanged (Fig. 5). Bop1 $Delta$ expressionalso resulted in accumulation of the 36S rRNA, normally presentin small amounts. In control experiments where LAP3 cells weretreated with FUrd, a known inhibitor of rRNA processing (84),a complete blockade of production of both 28S and 18S rRNA wasobserved without affecting the formation of the 45S and 32S precursors(Fig. 5). Together, these results suggested that Bop1 $Delta$ did notsignificantly affect the synthesis and initial processing of theprimary rRNA transcript but specifically compromised later processingsteps that lead to maturation of the 28S rRNA.

View larger version (68K):
[in this window]
[in a new window]

FIG. 5. Expression of Bop1 $Delta$ inhibits the generation of 28S rRNA. Clonal cell lines derived from transfection of LAP3 cells with pX11-Bop1 $Delta$ (lines 6 and 8), pX11-Bop1 (line 45), or the pX11 vector (line 1-1) were either treated with IPTG (+) for 16 h or left untreated ( $-$ ). Thereafter, cells were metabolically labeled with [³H]uridine (2.5 µCi/ml) for 30 min and chased in nonradioactive medium for 2 h. In other samples, LAP3 cells were treated with FUrd for 15 min prior to chase. RNA was then isolated, and equal counts per sample were electrophoresed on 1% agarose gel, transferred to a nylon membrane, and visualized by fluorography.

In mammalian cells, the 36S precursor is processed to form the 32S pre-rRNA, which is further processed to produce the mature28S rRNA and a 12S precursor from which the 5.8S rRNA is generated(Fig. 6). The concomitant block of the 28S rRNA and accumulationof the 36S pre-rRNA described above suggested that Bop1 $Delta$ may inhibitthe processing steps that convert the 36S pre-rRNA into the mature28S rRNA. To evaluate this interpretation and to identify thespecific rRNA processing blocks due to Bop1 $Delta$ expression, pulse-chaseexperiments were performed by metabolic labeling with ³H-labeled methyl methionine. LAP3-derived cell lines that eitherinducibly express Bop1 (line 45) or Bop1 $Delta$ (line 6) and the controlcell line transfected with empty vector (line 1-1) were eitherleft untreated or treated with IPTG, pulse-labeled for 30 min,and chased with excess nonradioactive methionine for various durations(Fig. 7). In the absence of IPTG, each cell line showed the synthesisof the 45S precursor, which was rapidly converted to the 32S pre-rRNAand the mature 18S rRNA within 30 min after pulse-labeling. The36S pre-rRNA is relatively short-lived and does not accumulatesignificantly under these conditions. Processing of the 32S pre-rRNAto the mature 28S RNA appeared to be complete by 60 min afterpulse-labeling. The addition of IPTG to the control cell line(line 1-1) or to the Bop1-expressing cell line (line 45) did notshow any effect on rRNA synthesis or processing. By contrast,expression of Bop1 $Delta$ (line 6) resulted in accumulation of the 36Spre-rRNA and diminution of the amount of 32S pre-rRNA. Whereasproduction of the 18S rRNA appeared normal, maturation of the28S rRNA was completely blocked. By 60 min after pulse-labeling,both the 36S and 32S pre-rRNAs appeared degraded rather than processed,resulting in the presence of only the 18S rRNA. These resultsshow that expression of Bop1 $Delta$ does not affect production of the18S rRNA but completely inhibits formation of the 28S rRNA. Moreover,Bop1 $Delta$ expression elicits an incomplete block in the conversionof the 36S to the 32S pre-rRNA and a complete block in the processingof the 32S to the 28S rRNA (Fig. 6 and 7).

View larger version (17K):
[in this window]
[in a new window]

FIG. 6. Schematic representation of the mammalian rRNA-processing pathway. Mammalian rRNA is transcribed as a single precursor which is further processed by successive nucleolytic cleavages that lead to elimination of the external transcribed spacers, 5'ETS and 3' ETS, and the internal transcribed spacers, ITS1 and ITS2. The sedimentation coefficients (S) of various intermediates and mature products of the processing pathway are indicated. The mammalian 47S precursor is rapidly cleaved at the 5'ETS and at the 3'ETS to give rise to the 45S pre-rRNA. Further processing at the 5'ETS takes place, giving rise to a 41S rRNA precursor, which is rapidly processed to the 18S rRNA and a 36S precursor RNA that contains the sequences of the 5.8S and 28S rRNAs with an intervening sequence (ITS2). The 36S precursor then undergoes cleavage at the 5' end to give rise to a 32S precursor, which is processed to the 28S rRNA and a 12S RNA; the 12S RNA is then further processed to form the 5.8S rRNA.

View larger version (51K):
[in this window]
[in a new window]

FIG. 7. Bop1 $Delta$ inhibits processing of the 36S and 32S precursors to form the 28S rRNA. Clonal LAP3 cell lines transfected with either the empty pX11 vector (line 1-1), pX11-Bop1 (line 45), or pX11-Bop1 $Delta$ (line 6) were either left untreated ( $-$ ) or treated with 1 mM IPTG for 16 h (+) and pulse-labeled with ³H-labeled methyl methionine for 30 min. After a chase in nonradioactive medium plus excess methionine for the indicated times, RNA was isolated, resolved on a 1% agarose gel, transferred to a membrane, and visualized by fluorography.

Bop1 $Delta$ expression inhibits de novo generation of the 12S and 5.8S rRNAs. The 32S pre-rRNA is normally processed to form the mature 28S rRNA and the 12S precursor, from which the 5.8S rRNA is generated(Fig. 6) (21). The complete inhibition of 28S rRNA generationby Bop1 $Delta$ suggested that formation of the 12S and 5.8S rRNAs mightalso be inhibited. To test this possibility, we examined the levelsof the 12S pre-rRNA and the 5.8S rRNA in Bop1 $Delta$ -expressing cells.Total RNA was isolated from various cell lines grown in the presenceor absence of IPTG and subjected to RNA blot analysis using thecoding region of the 5.8S rRNA as probe (Fig. 8A). This probeshould hybridize to and reveal the steady-state levels of the45S, 41S, 36S, 32S, and 12S precursors, as well as the mature5.8S rRNA (Fig. 6). These experiments showed that expression ofBop1 $Delta$ (lines 6 and 8) resulted in the diminution of the amountof 12S pre-rRNA to an undetectable level, with a concomitant accumulationof the 36S precursor. The steady-state level of the mature 5.8SrRNA appeared unchanged during the course of this experiment,given the high levels of preexisting rRNAs.

View larger version (60K):
[in this window]
[in a new window]

FIG. 8. Bop1 $Delta$ expression inhibits generation of the 12S precursor and the 5.8S rRNA. (A) Clonal LAP3 cell lines transfected with either the empty pX11 vector or pX11-Bop1 $Delta$ (lines 6 and 8) were either left untreated or treated with IPTG for 16 h. RNA isolated from the same number of cells was separated on a 1% agarose gel, transferred to a nylon membrane, and hybridized with an oligonucleotide probe complementary to a region in 5.8S rRNA. (B) The parental LAP3 cells or clonal cell lines transfected with either pX11-Bop1 (line 45) or pX11-Bop1 $Delta$ (line 6) were either left untreated or treated with IPTG for 16 h and metabolically labeled with ³²P_i (20 µCi/ml) for 1 h. Following a chase in nonradioactive medium for 1.5 h, RNA was isolated, and equal amounts of RNA from each sample were resolved on a 10% denaturing polyacrylamide gel, which was stained with ethidium bromide for photography (left panel) and dried for autoradiography (right panel).

Inhibition of 12S pre-rRNA formation predicts an inability to generate mature 5.8S rRNA from the newly synthesized rRNA transcript.To test this possibility, we carried out a pulse-labeling experimentto examine the formation of the 5.8S rRNA. Various cell linesgrown with or without IPTG were pulse-labeled with ³²P_i for 1 h and then chased in nonradioactive medium for 1.5 h,and total RNA isolated from these cells was resolved by denaturingacrylamide gel electrophoresis (Fig. 8B). Whereas overexpressionof Bop1 had no effect (line 45), expression of Bop1 $Delta$ (line 6)resulted in nearly complete inhibition in 5.8S rRNA synthesis(Fig. 8B). These results show that expression of Bop1 $Delta$ leads toa block in the processing of the 32S pre-rRNA into the 28S rRNAas well as into the 12S and 5.8S rRNAs. Interestingly, a smalldecrease in the amount of 5S RNA was also observed, possibly reflectinga coordinate regulation between pre-rRNA processing and 5S RNAtranscription (37). In addition, the recruitment of 5S rRNAto the pre-60S particle was shown to be necessary for efficientprocessing of the 27S rRNA precursor in yeast (16). It is possibleto speculate that the recruited 5S rRNA might be degraded togetherwith the improperly processed 32SrRNA.

Expression of Bop1 $Delta$ causes a deficit of the 60S ribosomal subunit. Since both 28S and 5.8S rRNAs are incorporated into the 60S ribosome, a specific block in their generation may result in adeficit in ribosome biogenesis. To examine this possibility, weused sucrose density gradient centrifugation to fractionate cytoplasmicextracts of a cell line that inducibly expressed Bop1 $Delta$ (line 6)(Fig. 9). Upon Bop1 $Delta$ expression by IPTG treatment, significantlyfewer free 60S ribosomal subunits were observed in the cytoplasmwhereas the 40S ribosomal subunits were accumulated to a higherlevel. Compared to untreated cells, the amount of 80S ribosomeswas also decreased. The simplest interpretation of these resultsis that the 60S ribosomal subunits cannot form due to the blockin 28S and 5.8S rRNAs synthesis and that the 40S ribosomal subunitsaccumulate due to a stoichiometric imbalance with the 60S subunit.Although the peaks that corresponded to polysomes appeared somewhatdiminished by Bop1 $Delta$ expression, no global polysome disassemblywas detected. This is consistent with the observation that theoverall rate of translation was unaffected by Bop1 $Delta$ expressionwithin the duration of these experiments as judged by metaboliclabeling with [³⁵S]methionine (data not shown).

View larger version (20K):
[in this window]
[in a new window]

FIG. 9. Expression of Bop1 $Delta$ causes a deficit in 60S ribosomal subunits. The inducible Bop1 $Delta$ expression cell line, line 6, was grown in the absence (A) or presence (B) of IPTG as indicated for 38 h. Cytoplasmic extracts were isolated and separated on a 10 to 45% sucrose density gradient. Profiles of absorbance at 254 nm (A₂₅₄) profiles revealed the positions and relative amounts of the ribosomal subunits in the gradient.

Bop1 and Bop1 $Delta$ are cosedimented with the 50S-80S pre-rRNP particles. The processing of eukaryotic rRNA occurs coordinately with the assembly of ribosomal particles in the nucleolus (81, 85).Pre-rRNP particles have been identified as several complexes bysucrose density gradients. In the presence of EDTA, these complexes,which contain the 45S, 36S, and 32S pre-rRNAs, sediment in therange of 50S to 80S (42, 47, 82). The apparent involvementof Bop1 in pre-rRNA processing suggested that Bop1 might be associatedwith the pre-rRNP particles. To investigate this possibility,nuclear extracts prepared from the inducible Bop1 $Delta$ -expressingcell line (line 6) were analyzed by sucrose gradient centrifugation(Fig. 10A). Proteins from each gradient fraction were assayed forendogenous Bop1 and ectopically expressed Bop1 $Delta$ by Western blotanalysis. When cells were grown in the absence of IPTG, endogenousBop1 protein sedimented primarily in fractions 5 to 7, which correspondedto the 50S-80S particles (Fig. 10B and C). When expressed, Bop1 $Delta$ was distributed more broadly from fractions 3 through 7 with apeak at fraction 5, where the peak of the endogenous Bop1 wasalso found. Thus, both Bop1 and Bop1 $Delta$ were found in large nuclearparticles with sizes similar to pre-rRNP particles. However, Bop1is not a component of matured ribosomes, since Western blottingof a cytoplasmic ribosomal preparation did not detect any Bop1protein (Fig. 10D).

View larger version (36K):
[in this window]
[in a new window]

FIG. 10. Bop1 and Bop1 $Delta$ cofractionate with the 50S-80S pre-RNP particles in nuclear extracts. (A to C) The inducible Bop1 $Delta$ expression cell line (line 6) was grown in the presence (C) or absence (A and B) of IPTG for 24 h as indicated. Nuclear extracts isolated from these cells were analyzed on 10 to 30% sucrose density gradients, which were fractionated with continuous monitoring of absorbance at 254 nm (A). Individual fractions were electrophoresed on an SDS-10% polyacrylamide gel and subjected to immunoblotting analysis using affinity-purified anti-Bop1 antibodies. Sn, unfractionated soluble nuclear extracts; P, unsoluble pellet. (D) (Left) Immunoblot analysis with anti-Bop1 antibodies detects Bop1 in nuclear RNPs (N) but not cytoplasmic ribosomes (C). (Right) Electrophoretic analysis of RNA in the fractions used for immunoblotting. RNA was extracted from the nucleoprotein complexes and separated by electrophoresis on a formaldehyde-containing agarose gel to demonstrate the presence equivalent amounts of rRNA in both samples.

To substantiate the observation that Bop1 cosediments with the 50S-80S preribosomes, nuclear extracts were fractionated bysucrose density gradients and proteins and RNA from each gradientfractions were analyzed in parallel (Fig. 11). Proteins were resolvedby electrophoresis, blotted, and probed with anti-Bop1 antibodies,while RNA from the same samples was electrophoresed, blotted,stained with methylene blue, and probed with the ³²P-labeled DNA fragment from the ITS2 region, which can recognizethe 47S, 45S, 41S, 36S, and 32S pre-rRNAs. This analysis showedthat the Bop1 protein cosedimented with rRNP particles that containedthe 32S precursor RNA, found in fractions 5 to 8, and that thepeaks for both Bop1 and the 32S rRNA both occurred in fraction6. The 18S rRNA was found mainly in fractions 3 and 4, whereasthe 28S rRNA was found in fractions 4 to 7, with the peak in fraction5. Thus, these results show that Bop1 cosediments with the rRNPparticles containing the 32S pre-rRNA, consistent with a rolefor Bop1 in the processing of the 32S pre-rRNA.

View larger version (33K):
[in this window]
[in a new window]

FIG. 11. Bop1 cofractionates with the 32S precursor and 28S rRNA in the nuclear extract. Nuclear extracts from LAP3 cells were isolated and separated on a 10 to 30% sucrose density gradient. The fractions collected were subjected to parallel analysis of protein and RNA. (A) Proteins from various fractions were electrophoresed on an SDS-10% polyacrylamide gel and immunoblotted with affinity-purified anti-Bop1 antibodies. (B) RNAs from each fraction analyzed in panel A were resolved on a 1% agarose gel and transferred to a nylon filter, which was stained with methylene blue. The staining pattern reveals the fractions containing the 18S and 28S rRNAs. (C) The nylon filter shown in panel B was subjected to hybridization using radioactively labeled sequences from ITS2 as a probe, revealing the 32S precursor RNA. In, unfractionated soluble nuclear extract.

To confirm that Bop1 is a component of rRNP particles, nuclear extracts were either untreated or treated with RNase A beforebeing subjected to fractionation on a sucrose gradient (Fig. 12).As expected, Bop1 cofractionated with rRNP particles in the absenceof RNase A. Treatment with RNase completely destroyed the rRNPparticles, as shown by the absorbance of the gradient at 254 nm.Bop1 protein was completely shifted to the top of the gradienton nuclease digestion, consistent with its release from rRNP particles.In separate experiments, Bop1 $Delta$ was also released from the 50S-80Sfractions to the top of the gradient on RNase A treatment (datanot shown). Together, these results show that as a nucleolar protein,Bop1 is a component of the RNP particles that cosediment withthe pre-rRNP particles containing the 32S pre-rRNA.

View larger version (38K):
[in this window]
[in a new window]

FIG. 12. Bop1 is part of an RNP complex. Nuclear extracts from LAP3 cells were either treated with RNaseA or left untreated as indicated and analyzed on 10 to 30% sucrose density gradients. The gradients were fractionated and monitored for absorbance at 254 nm (top panel). Various fractions were subjected to SDS-PAGE followed by immunoblotting using affinity-purified anti-Bop1 antibodies. In, unfractionated soluble nuclear extract.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study we identified Bop1 as a novel participant in the mammalian nucleolar rRNA processing and ribosome biogenesismachinery. This conclusion is drawn based on data accumulatedthrough two approaches: (i) biochemical studies show that Bop1is a nucleolar protein that forms part of a large, RNA-containingprotein complex that cosediments with pre-rRNP particles containingthe 32S pre-rRNA; and (ii) functional analyses indicate that Bop1plays a role in the maturation of the 28S and 5.8S rRNAs and thebiogenesis of the 60S ribosomalsubunit.

Several lines of evidence provide support for the conclusion that Bop1 is a nonribosomal nucleolar protein that constitutesa component of pre-rRNP particles. Immunofluorescence analysisdemonstrates that both endogenous and ectopically expressed Bop1are localized to the nucleolus (Fig. 3). Sucrose density gradientfractionation of nuclear extracts shows that Bop1 forms part oflarge ribonucleoprotein complexes that sediment at 50S-80S (Fig.10). Treatment of the nuclear preparations with RNase A, whichdestroys pre-rRNP particles, releases Bop1 into low-molecular-weightfractions at the top of the gradient (Fig. 12). Thus, while Bop1is not part of the mature cytosolic ribosomes, these data stronglyindicate that it is a component of the pre-rRNPparticles.

To analyze the function of Bop1, we took advantage of an N-terminally truncated derivative, Bop1 $Delta$ , as a means of interferingwith the activity of the wild-type protein in a dominant manner.Bop1 $Delta$ displays the same nucleolar localization as Bop1 and a similarsedimentation profile in a sucrose density gradient, indicatingthat it resides in the same RNP complexes as the wild-type proteinand thus retains a subset of its functions. Since Bop1 $Delta$ retainsthe WD40 motifs present in the full-length Bop1 (Fig. 1), it isplausible to speculate that Bop1 $Delta$ is able to interact with manyof the same proteins with which Bop1 interacts. However, Bop1 $Delta$ apparently interferes with the normal function of Bop1. Indeed,expression of Bop1 $Delta$ results in a serious defect in the processingof the 28S and 5.8S rRNAs and a deficit of mature 60S ribosomesubunits. This conclusion is supported by a preponderance of evidence.(i) Metabolic labeling shows that expression of Bop1 $Delta$ leads toa specific inhibition of 28S and 5.8S rRNA maturation while havingno effect on the 18S rRNA (Fig. 5 and 8). (ii) Pulse-chase analysisreveals a partial processing block in the conversion of the 36Sto the 32S pre-rRNA and a complete block in the processing ofthe 32S pre-rRNA to the mature 28S rRNA and 12S pre-rRNA and consequentlyto the 5.8S rRNA (Fig. 7 and 8). (iii) Examination of the steady-stateRNA levels shows an accumulation of the 36S rRNA and an inhibitionof 12S pre-rRNA (Fig. 8A), confirming the results of pulse-chaselabeling. (iv) Sedimentation gradients show a marked decreasein the number of cytosolic 60S ribosomal subunits (Fig. 9). Thesefindings strongly implicate Bop1 as an important player in rRNAmaturation, specifically in the conversion of the 32S pre-rRNAinto the 28S rRNA and the 12S precursor. Moreover, both Bop1 andBop1 $Delta$ cosediment with pre-rRNPs that contain the 32S rRNA precursors(Fig. 10 and 11), further corroborating the conclusion that Bop1is involved in the maturation of the 5.8S and 28S rRNAs, a processwith which Bop1 $Delta$ interferes.

Expression of Bop1 $Delta$ under the control of an inducible promoter was previously shown to cause a powerful but reversible G₁growth arrest in mouse fibroblasts (58). The precise mechanismby which Bop1 $Delta$ causes this growth inhibition is unclear. Nevertheless,it is possible to envisage at least two distinct mechanisms bywhich Bop1 $Delta$ may affect cell cycle progression. First, growth arrestdue to Bop1 $Delta$ may be a secondary effect resulting from perturbationsin the translation machinery caused by deficiency of 60S ribosomalsubunits. For example, deficiencies in the translation initiationfactor eIF4E/CDC33 lead to a G₁ growth arrest in yeast (9).Alternatively, Bop1 might play a dual role in both pre-rRNA processingand cell cycle progression, thereby mediating a cross talk betweenthese two distinct cellular pathways. The nucleolus has been implicatedin functions other than rRNA processing and ribosome biogenesis(57), including the regulation of cellular exit from mitosis(4). Exosomes and Xrn1p exonuclease function in mRNA in additionto rRNA processing (10, 17, 50) and may thus affect thesynthesis of cell cycle regulators. The possibility that Bop1might exert an effect on the cell cycle machinery hints at anas yet poorly understood link between the cellular capacity forcoordinating protein synthesis and cell cycle progression. Understandingthe precise role of Bop1 in cell cycle progression will requirefurtherinvestigation.

Consistent with a role for Bop1 in rRNA processing and ribosome maturation, Bop1 appears to be ubiquituously expressed irrespectiveof the tissue type (Fig. 2). Moreover, bop1 mRNA levels beginto rise in mid to late G₁, coincident with the timing of rRNAsynthesis (24, 65, 70). As expected of a protein that playsa role in ribosome maturation, Bop1 appears to be highly conservedthroughout evolution. The mouse Bop1 displays >90% amino acididentity to its human ortholog (KIAA0124) and ~45% identity toa sequence in Saccharomyces cerevisiae (YMR049c). A BLAST searchin the currently available databases also reveals protein codingsequences highly homologous to Bop1 in such diverse organismsas Drosophila melanogaster, Caenorhabditis elegans, and Arabidopsisthaliana.

In this report, we show for the first time the effect of a nucleolar protein on rRNA processing in a mammalian system. Onlya few other mammalian proteins have been implicated in rRNA processingto date, based on the function of their yeast homologs. For example,p120 was originally identified as a tumor proliferation antigen(33) and was later implicated in rRNA processing, since deletionof its yeast homolog, Nop2p, causes a block in the processingof the 27S pre-rRNA to the mature 25S rRNA (36). Consistentwith a role in rRNA processing, p120 was shown to cofractionatewith the 60-80S preribosomal particles in HeLa cell extracts (30).

In yeast, several proteins whose depletion specifically affects processing of the 25S branch of rRNA processing have beenidentified. For example, depletion of the yeast Nop4 protein resultsin the inhibition of the 25S rRNA maturation as well as 60S ribosomal-subunitaccumulation, while production of the 18S rRNA is unaffected (74).Other examples of similar phenotypes result from depletion ofmembers of the DEAD box family of putative ATP-dependent RNA helicasesincluding DRS1 (63), Dbp6p (41), Dbp7p (15), and Spb4p (18),as well as nucleolar proteins Nip7p (87) and Nop8p (86). Theseobservations underscore the notion that processing of the 25S/28Sbranch of rRNA requires complexes of numerous proteins, whosenature is only beginning to be understood. In Xenopus, depletionof the U8 snoRNA (56) also has effects similar to Bop1 $Delta$ expression,namely, an incomplete inhibition of 36S pre-rRNA processing buta complete block of 32S pre-rRNA processing, leading to inhibitionof 28S and 5.8S rRNA production. Immunoprecipitation of Bop1 followedby RNA blotting with an anti-U8 RNA probe failed to detect theU8 RNA (data not shown). In addition, immunoprecipitation of Bop1from cells metabolically labeled with radioactive phosphate followedby PAGE also did not reveal the presence of small RNAs (data notshown). These results suggest that Bop1 is unlikely to be mediatingthe interaction of U8 or other snoRNAs with the rRNAprecursor.

Processing of pre-rRNA and ribosome biogenesis appear to be highly coordinated (19, 49, 64, 80, 81). Consistentwith this notion, there is a dramatic decrease in the amount ofmature 60S ribosomal subunits when maturation of the 28S and 5.8SrRNAs is blocked as a result of Bop1 $Delta$ expression (Fig. 9). Thedeficit in the 60S ribosomal subunit may be a direct result ofthe inability to produce its cognate mature rRNAs. However, wecannot rule out the possibility that Bop1 may also have the distinctfunction of coordinating 60S ribosomal assembly and that thisfunction is compromised by Bop1 $Delta$ .

Analysis of the primary sequence of Bop1 does not suggest an apparent enzymatic activity, although it does show features ofa short-lived, regulatory protein that may participate in criticalprotein-protein interactions. The Bop1 sequence contains clustersof charged amino acid residues, known as PEST sequences, oftenassociated with regulatory and short-lived proteins (13, 61,67). Similar clusters are also observed in a number of nucleolarproteins (71). A putative nuclear localization signal in Bop1is located at aa 360 to 366 (PRQRKMR; underlining indicates positivelycharged residues) (20, 25). Data from the present study withBop1 $Delta$ show that the N-terminal 231 aa are not needed for nucleolarlocation or complex formation with RNP particles but are necessaryfor critical functions illustrated by the consequences of Bop1 $Delta$ expression.

Bop1 contains four WD40 repeats (Fig. 1), a sequence motif found in a large variety of regulatory proteins and known to mediateprotein-protein interactions (26, 27, 51, 52, 72). WD40proteins have been implicated in a number of cellular processes,including various stages of RNA metabolism (3, 6). At present,at least two other nucleolar proteins that contain WD40 repeatshave been identified: the yeast SOF1 (38) and the related (butnot orthologous) human protein hU3-55k (60). Inasmuch as a numberof WD40 repeat proteins are known to form large multiprotein complexes,Bop1 may mediate protein-protein interactions that are importantfor the formation and activities of nucleolar RNPs. Future studiesaimed at the identification and characterization of the proteinswith which Bop1 interacts may yield new insights into the structuralorganization and mechanism of action of the nucleolar pre-rRNA-processingmachinery.

	ACKNOWLEDGMENTS

We thank members of our laboratory for helpful discussions, Michael Pollard for providing the antifibrillarin antibody (72B9),Alisa Katzen and Gary Ramsey for helping with microscopy, andRobert Costa, Nissim Hay, Susan Liebman, and Jeff Greenspan forcritical reading of themanuscript.

This work was supported by a grant from the National Institutes of Health(CA52220).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Genetics, M/C 669, University of Illinois at Chicago, 900 S.Ashland Ave., Chicago, IL 60607. Phone: (312) 996-6978. Fax: (312)996-7034. E-mail: LFLau{at}uic.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. 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].

2. Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1994. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.

3. Ayadi, L., M. Miller, and J. Banroques. 1997. Mutations within the yeast U4/U6 snRNP protein Prp4 affect a late stage of spliceosome assembly. RNA 3:197-209[Abstract].

4. Bachant, J. B., and S. J. Elledge. 1999. Mitotic treasures in the nucleolus. Nature 398:757-758[CrossRef][Medline].

5. Baim, S. B., M. A. Labow, A. J. Levine, and T. Shenk. 1991. A chimeric mammalian transactivator based on the lac repressor that is regulated by temperature and isopropyl $beta$ -D-thiogalactopyranoside. Proc. Natl. Acad. Sci. USA 88:5072-5076[Abstract/Free Full Text].

6. Ben Yehuda, S., I. Dix, C. S. Russell, S. Levy, J. D. Beggs, and M. Kupiec. 1998. Identification and functional analysis of hPRP17, the human homologue of the PRP17/CDC40 yeast gene involved in splicing and cell cycle control. RNA 4:1304-1312[Abstract].

7. Bjorn, S. P., A. Soltyk, J. D. Beggs, and J. D. Friesen. 1989. PRP4 (RNA4) from Saccharomyces cerevisiae: its gene product is associated with the U4/U6 small nuclear ribonucleoprotein particle. Mol. Biol. Cell 9:3698-3709.

8. Bowman, L. H., B. Rabin, and D. Schlessinger. 1981. Multiple ribosomal RNA cleavage pathways in mammalian cells. Nucleic Acids Res. 9:4951-4966[Abstract/Free Full Text].

9. Brenner, C., N. Nakayama, M. Goebl, K. Tanaka, A. Toh-e, and K. Matsumoto. 1988. CDC33 encodes mRNA cap-binding protein eIF-4E of Saccharomyces cerevisiae. Mol. Cell. Biol. 8:3556-3559[Abstract/Free Full Text].

10. Carpousis, A. J., N. F. Vanzo, and L. C. Raynal. 1999. mRNA degradation. A tale of poly(A) and multiprotein machines. Trends Genet. 15:24-28[CrossRef][Medline].

11. Chang, J. H., and M. O. Olson. 1990. Structure of the gene for rat nucleolar protein B23. J. Biol. Chem. 265:18227-18233[Abstract/Free Full Text].

12. Chen, C. A., and H. Okayama. 1988. Calcium phosphate-mediated gene transfer: a highly efficient transfection system for stably transforming cells with plasmid DNA. BioTechniques 6:632-638[Medline].

13. Chevaillier, P. 1993. Pest sequences in nuclear proteins. Int. J. Biochem. 25:479-482[CrossRef][Medline].

14. Dalrymple, M. A., S. Petersen-Bjorn, J. D. Friesen, and J. D. Beggs. 1989. The product of the PRP4 gene of S. cerevisiae shows homology to beta subunits of G proteins. Cell 58:811-812[CrossRef][Medline].

15. Daugeron, M. C., and P. Linder. 1998. Dbp7p, a putative ATP-dependent RNA helicase from Saccharomyces cerevisiae, is required for 60S ribosomal subunit assembly. RNA 4:566-581[Abstract].

16. Dechampesme, A. M., O. Koroleva, I. Leger-Silvestre, N. Gas, and S. Camier. 1999. Assembly of 5S ribosomal RNA is required at a specific step of the pre-rRNA processing pathway. J. Cell Biol. 145:1369-1380[Abstract/Free Full Text].

17. Decker, C. J. 1998. The exosome: a versatile RNA processing machine. Curr. Biol. 8:R238-R240[CrossRef][Medline].

18. de la Cruz, J., D. Kressler, M. Rojo, D. Tollervey, and P. Linder. 1998. Spb4p, an essential putative RNA helicase, is required for a late step in the assembly of 60S ribosomal subunits in Saccharomyces cerevisiae. RNA 4:1268-1281[Abstract].

19. Deshmukh, M., J. Stark, L. C. Yeh, J. C. Lee, and J. L. Woolford, Jr. 1995. Multiple regions of yeast ribosomal protein L1 are important for its interaction with 5 S rRNA and assembly into ribosomes. J. Biol. Chem. 270:30148-30156[Abstract/Free Full Text].

20. Dingwall, C., and R. A. Laskey. 1991. Nuclear targeting sequences $---$ a consensus? Trends Biochem. Sci. 16:478-481[CrossRef][Medline].

21. Eichler, D. C., and N. Craig. 1994. Processing of eukaryotic ribosomal RNA. Prog. Nucleic Acid Res. Mol. Biol. 49:197-239[Medline].

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

23. Field, J., J. Nikawa, D. Broek, B. MacDonald, L. Rodgers, I. A. Wilson, R. A. Lerner, and M. Wigler. 1988. Purification of a RAS-responsive adenylyl cyclase complex from Saccharomyces cerevisiae by use of an epitope addition method. Mol. Cell. Biol. 8:2159-2165[Abstract/Free Full Text].

24. Fujikawa-Yamamoto, K. 1982. RNA dependence in the cell cycle of V79 cells. J. Cell Physiol. 112:60-66[CrossRef][Medline].

25. Garcia-Bustos, J., J. Heitman, and M. N. Hall. 1991. Nuclear protein localization. Biochim. Biophys. Acta 1071:83-101[Medline].

26. Garcia-Higuera, I., J. Fenoglio, Y. Li, C. Lewis, M. P. Panchenko, O. Reiner, T. F. Smith, and E. J. Neer. 1996. Folding of proteins with WD-repeats: comparison of six members of the WD-repeat superfamily to the G protein beta subunit. Biochemistry 35:13985-13994[CrossRef][Medline].

27. Garcia-Higuera, I., C. Gaitatzes, T. F. Smith, and E. J. Neer. 1998. Folding a WD repeat propeller. Role of highly conserved aspartic acid residues in the G protein beta subunit and Sec13. J. Biol. Chem. 273:9041-9049[Abstract/Free Full Text].

28. Geiduschek, E. P., and G. P. Tocchini-Valentini. 1988. Transcription by RNA polymerase III. Annu. Rev. Biochem. 57:873-914[CrossRef][Medline].

29. Ginisty, H., H. Sicard, B. Roger, and P. Bouvet. 1999. Structure and functions of nucleolin. J. Cell Sci. 112:761-772[Abstract].

30. Gustafson, W. C., C. W. Taylor, B. C. Valdez, D. Henning, A. Phippard, Y. Ren, H. Busch, and E. Durban. 1998. Nucleolar protein p120 contains an arginine-rich domain that binds to ribosomal RNA. Biochem. J. 331:387-393.

31. Hadjiolova, K. V., M. Nicoloso, S. Mazan, A. A. Hadjiolov, and J. P. Bachellerie. 1993. Alternative pre-rRNA processing pathways in human cells and their alteration by cycloheximide inhibition of protein synthesis. Eur. J. Biochem. 212:211-215[Medline].

32. Harlow, E., and D. Lane. 1988. Antibodies: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

33. Hazlewood, J., A. Fonagy, D. Henning, J. W. Freeman, R. K. Busch, and H. Busch. 1989. mRNA levels for human nucleolar protein P120 in tumor and nontumor cells. Cancer Commun. 1:29-34[Medline].

34. Henriquez, R., G. Blobel, and J. P. Aris. 1990. Isolation and sequencing of NOP1. A yeast gene encoding a nucleolar protein homologous to a human autoimmune antigen. J. Biol. Chem. 265:2209-2215[Abstract/Free Full Text].

35. Henry, Y., H. Wood, J. P. Morrissey, E. Petfalski, S. Kearsey, and D. Tollervey. 1994. The 5' end of yeast 5.8S rRNA is generated by exonucleases from an upstream cleavage site. EMBO J. 13:2452-2463[Medline].

36. Hong, B., J. S. Brockenbrough, P. Wu, and J. P. Aris. 1997. Nop2p is required for pre-rRNA processing and 60S ribosome subunit synthesis in yeast. Mol. Biol. Cell. 17:378-388.

37. Jackson, A. J., M. Ittmann, and B. F. Pugh. 1995. The BN51 protein is a polymerase (Pol)-specific subunit of RNA Pol III which reveals a link between Pol III transcription and pre-rRNA processing. Mol. Cell. Biol. 15:94-101[Abstract].

38. Jansen, R., D. Tollervey, and E. C. Hurt. 1993. A U3 snoRNP protein with homology to splicing factor PRP4 and G beta domains is required for ribosomal RNA processing. EMBO J. 12:2549-2558[Medline].

39. Johnson, A. W. 1997. Rat1p and Xrn1p are functionally interchangeable exoribonucleases that are restricted to and required in the nucleus and cytoplasm, respectively. Mol. Cell. Biol. 17:6122-6130[Abstract].

40. Jordan, P., M. Mannervik, L. Tora, and M. Carmo-Fonseca. 1996. In vivo evidence that TATA-binding protein/SL1 colocalizes with UBF and RNA polymerase I when rRNA synthesis is either active or inactive. J. Cell Biol. 133:225-234[Abstract/Free Full Text].

41. Kressler, D., J. de la Cruz, M. Rojo, and P. Linder. 1998. Dbp6p is an essential putative ATP-dependent RNA helicase required for 60S-ribosomal-subunit assembly in Saccharomyces cerevisiae. Mol. Cell. Biol. 18:1855-1865[Abstract/Free Full Text].

42. Liau, M. C., and R. P. Perry. 1969. Ribosome precursor particles in nucleoli. J. Cell Biol. 42:272-283[Abstract/Free Full Text].

43. Lischwe, M. A., R. L. Ochs, R. Reddy, R. G. Cook, L. C. Yeoman, E. M. Tan, M. Reichlin, and H. Busch. 1985. Purification and partial characterization of a nucleolar scleroderma antigen (Mr = 34,000; pI, 8.5) rich in NG,NG-dimethylarginine. J. Biol. Chem. 260:14304-14310[Abstract/Free Full Text].

44. Lygerou, Z., C. Allmang, D. Tollervey, and B. Seraphin. 1996. Accurate processing of a eukaryotic precursor ribosomal RNA by ribonuclease MRP in vitro. Science 272:268-270[Abstract].

45. Maxwell, E. S., and M. J. Fournier. 1995. The small nucleolar RNAs. Annu. Rev. Biochem. 64:897-934[CrossRef][Medline].

46. McEwen, C. R.

1.	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].
2.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1994. Current protocols in molecular biology. John Wiley & Sons, Inc., New York, N.Y.
3.	Ayadi, L., M. Miller, and J. Banroques. 1997. Mutations within the yeast U4/U6 snRNP protein Prp4 affect a late stage of spliceosome assembly. RNA 3:197-209[Abstract].
4.	Bachant, J. B., and S. J. Elledge. 1999. Mitotic treasures in the nucleolus. Nature 398:757-758[CrossRef][Medline].
5.	Baim, S. B., M. A. Labow, A. J. Levine, and T. Shenk. 1991. A chimeric mammalian transactivator based on the lac repressor that is regulated by temperature and isopropyl $beta$ -D-thiogalactopyranoside. Proc. Natl. Acad. Sci. USA 88:5072-5076[Abstract/Free Full Text].
6.	Ben Yehuda, S., I. Dix, C. S. Russell, S. Levy, J. D. Beggs, and M. Kupiec. 1998. Identification and functional analysis of hPRP17, the human homologue of the PRP17/CDC40 yeast gene involved in splicing and cell cycle control. RNA 4:1304-1312[Abstract].
7.	Bjorn, S. P., A. Soltyk, J. D. Beggs, and J. D. Friesen. 1989. PRP4 (RNA4) from Saccharomyces cerevisiae: its gene product is associated with the U4/U6 small nuclear ribonucleoprotein particle. Mol. Biol. Cell 9:3698-3709.
8.	Bowman, L. H., B. Rabin, and D. Schlessinger. 1981. Multiple ribosomal RNA cleavage pathways in mammalian cells. Nucleic Acids Res. 9:4951-4966[Abstract/Free Full Text].
9.	Brenner, C., N. Nakayama, M. Goebl, K. Tanaka, A. Toh-e, and K. Matsumoto. 1988. CDC33 encodes mRNA cap-binding protein eIF-4E of Saccharomyces cerevisiae. Mol. Cell. Biol. 8:3556-3559[Abstract/Free Full Text].
10.	Carpousis, A. J., N. F. Vanzo, and L. C. Raynal. 1999. mRNA degradation. A tale of poly(A) and multiprotein machines. Trends Genet. 15:24-28[CrossRef][Medline].
11.	Chang, J. H., and M. O. Olson. 1990. Structure of the gene for rat nucleolar protein B23. J. Biol. Chem. 265:18227-18233[Abstract/Free Full Text].
12.	Chen, C. A., and H. Okayama. 1988. Calcium phosphate-mediated gene transfer: a highly efficient transfection system for stably transforming cells with plasmid DNA. BioTechniques 6:632-638[Medline].
13.	Chevaillier, P. 1993. Pest sequences in nuclear proteins. Int. J. Biochem. 25:479-482[CrossRef][Medline].
14.	Dalrymple, M. A., S. Petersen-Bjorn, J. D. Friesen, and J. D. Beggs. 1989. The product of the PRP4 gene of S. cerevisiae shows homology to beta subunits of G proteins. Cell 58:811-812[CrossRef][Medline].
15.	Daugeron, M. C., and P. Linder. 1998. Dbp7p, a putative ATP-dependent RNA helicase from Saccharomyces cerevisiae, is required for 60S ribosomal subunit assembly. RNA 4:566-581[Abstract].
16.	Dechampesme, A. M., O. Koroleva, I. Leger-Silvestre, N. Gas, and S. Camier. 1999. Assembly of 5S ribosomal RNA is required at a specific step of the pre-rRNA processing pathway. J. Cell Biol. 145:1369-1380[Abstract/Free Full Text].
17.	Decker, C. J. 1998. The exosome: a versatile RNA processing machine. Curr. Biol. 8:R238-R240[CrossRef][Medline].
18.	de la Cruz, J., D. Kressler, M. Rojo, D. Tollervey, and P. Linder. 1998. Spb4p, an essential putative RNA helicase, is required for a late step in the assembly of 60S ribosomal subunits in Saccharomyces cerevisiae. RNA 4:1268-1281[Abstract].
19.	Deshmukh, M., J. Stark, L. C. Yeh, J. C. Lee, and J. L. Woolford, Jr. 1995. Multiple regions of yeast ribosomal protein L1 are important for its interaction with 5 S rRNA and assembly into ribosomes. J. Biol. Chem. 270:30148-30156[Abstract/Free Full Text].
20.	Dingwall, C., and R. A. Laskey. 1991. Nuclear targeting sequences $---$ a consensus? Trends Biochem. Sci. 16:478-481[CrossRef][Medline].
21.	Eichler, D. C., and N. Craig. 1994. Processing of eukaryotic ribosomal RNA. Prog. Nucleic Acid Res. Mol. Biol. 49:197-239[Medline].
22.	Elela, S. A., H. Igel, and M. J. Ares. 1996. RNase III cleaves eukaryotic preribosomal RNA at a U3 snoRNP-dependent site. Cell 85:115-124[CrossRef][Medline].
23.	Field, J., J. Nikawa, D. Broek, B. MacDonald, L. Rodgers, I. A. Wilson, R. A. Lerner, and M. Wigler. 1988. Purification of a RAS-responsive adenylyl cyclase complex from Saccharomyces cerevisiae by use of an epitope addition method. Mol. Cell. Biol. 8:2159-2165[Abstract/Free Full Text].
24.	Fujikawa-Yamamoto, K. 1982. RNA dependence in the cell cycle of V79 cells. J. Cell Physiol. 112:60-66[CrossRef][Medline].
25.	Garcia-Bustos, J., J. Heitman, and M. N. Hall. 1991. Nuclear protein localization. Biochim. Biophys. Acta 1071:83-101[Medline].
26.	Garcia-Higuera, I., J. Fenoglio, Y. Li, C. Lewis, M. P. Panchenko, O. Reiner, T. F. Smith, and E. J. Neer. 1996. Folding of proteins with WD-repeats: comparison of six members of the WD-repeat superfamily to the G protein beta subunit. Biochemistry 35:13985-13994[CrossRef][Medline].
27.	Garcia-Higuera, I., C. Gaitatzes, T. F. Smith, and E. J. Neer. 1998. Folding a WD repeat propeller. Role of highly conserved aspartic acid residues in the G protein beta subunit and Sec13. J. Biol. Chem. 273:9041-9049[Abstract/Free Full Text].
28.	Geiduschek, E. P., and G. P. Tocchini-Valentini. 1988. Transcription by RNA polymerase III. Annu. Rev. Biochem. 57:873-914[CrossRef][Medline].
29.	Ginisty, H., H. Sicard, B. Roger, and P. Bouvet. 1999. Structure and functions of nucleolin. J. Cell Sci. 112:761-772[Abstract].
30.	Gustafson, W. C., C. W. Taylor, B. C. Valdez, D. Henning, A. Phippard, Y. Ren, H. Busch, and E. Durban. 1998. Nucleolar protein p120 contains an arginine-rich domain that binds to ribosomal RNA. Biochem. J. 331:387-393.
31.	Hadjiolova, K. V., M. Nicoloso, S. Mazan, A. A. Hadjiolov, and J. P. Bachellerie. 1993. Alternative pre-rRNA processing pathways in human cells and their alteration by cycloheximide inhibition of protein synthesis. Eur. J. Biochem. 212:211-215[Medline].
32.	Harlow, E., and D. Lane. 1988. Antibodies: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
33.	Hazlewood, J., A. Fonagy, D. Henning, J. W. Freeman, R. K. Busch, and H. Busch. 1989. mRNA levels for human nucleolar protein P120 in tumor and nontumor cells. Cancer Commun. 1:29-34[Medline].
34.	Henriquez, R., G. Blobel, and J. P. Aris. 1990. Isolation and sequencing of NOP1. A yeast gene encoding a nucleolar protein homologous to a human autoimmune antigen. J. Biol. Chem. 265:2209-2215[Abstract/Free Full Text].
35.	Henry, Y., H. Wood, J. P. Morrissey, E. Petfalski, S. Kearsey, and D. Tollervey. 1994. The 5' end of yeast 5.8S rRNA is generated by exonucleases from an upstream cleavage site. EMBO J. 13:2452-2463[Medline].
36.	Hong, B., J. S. Brockenbrough, P. Wu, and J. P. Aris. 1997. Nop2p is required for pre-rRNA processing and 60S ribosome subunit synthesis in yeast. Mol. Biol. Cell. 17:378-388.
37.	Jackson, A. J., M. Ittmann, and B. F. Pugh. 1995. The BN51 protein is a polymerase (Pol)-specific subunit of RNA Pol III which reveals a link between Pol III transcription and pre-rRNA processing. Mol. Cell. Biol. 15:94-101[Abstract].
38.	Jansen, R., D. Tollervey, and E. C. Hurt. 1993. A U3 snoRNP protein with homology to splicing factor PRP4 and G beta domains is required for ribosomal RNA processing. EMBO J. 12:2549-2558[Medline].
39.	Johnson, A. W. 1997. Rat1p and Xrn1p are functionally interchangeable exoribonucleases that are restricted to and required in the nucleus and cytoplasm, respectively. Mol. Cell. Biol. 17:6122-6130[Abstract].
40.	Jordan, P., M. Mannervik, L. Tora, and M. Carmo-Fonseca. 1996. In vivo evidence that TATA-binding protein/SL1 colocalizes with UBF and RNA polymerase I when rRNA synthesis is either active or inactive. J. Cell Biol. 133:225-234[Abstract/Free Full Text].
41.	Kressler, D., J. de la Cruz, M. Rojo, and P. Linder. 1998. Dbp6p is an essential putative ATP-dependent RNA helicase required for 60S-ribosomal-subunit assembly in Saccharomyces cerevisiae. Mol. Cell. Biol. 18:1855-1865[Abstract/Free Full Text].
42.	Liau, M. C., and R. P. Perry. 1969. Ribosome precursor particles in nucleoli. J. Cell Biol. 42:272-283[Abstract/Free Full Text].
43.	Lischwe, M. A., R. L. Ochs, R. Reddy, R. G. Cook, L. C. Yeoman, E. M. Tan, M. Reichlin, and H. Busch. 1985. Purification and partial characterization of a nucleolar scleroderma antigen (Mr = 34,000; pI, 8.5) rich in NG,NG-dimethylarginine. J. Biol. Chem. 260:14304-14310[Abstract/Free Full Text].
44.	Lygerou, Z., C. Allmang, D. Tollervey, and B. Seraphin. 1996. Accurate processing of a eukaryotic precursor ribosomal RNA by ribonuclease MRP in vitro. Science 272:268-270[Abstract].
45.	Maxwell, E. S., and M. J. Fournier. 1995. The small nucleolar RNAs. Annu. Rev. Biochem. 64:897-934[CrossRef][Medline].
46.	McEwen, C. R.