Initiation of Nucleolar Assembly Is Independent of RNA Polymerase I Transcription

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Vol. 11, Issue 8, 2705-2717, August 2000

Initiation of Nucleolar Assembly Is Independent of RNA Polymerase I Transcription

Thibaut Dousset,^* Chen Wang,^* Céline Verheggen, Danyang Chen, Danièle Hernandez-Verdun, and Sui Huang^§

Institut Jacques Monod, 75251 Paris, France; and Department of Cell and Molecular Biology, Northwestern University Medical School, Chicago, Illinois 60611

Submitted March 28, 2000; Revised May 12, 2000; Accepted May 16, 2000
Monitoring Editor: Elizabeth H. Blackburn

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

This report examines the distribution of an RNA polymerase I transcription factor (upstream binding factor; UBF), pre-rRNAprocessing factors (nucleolin and fibrillarin), and pre-rRNAsthroughout mitosis and postmitotic nucleologenesis in HeLa cells.The results demonstrate that nucleolin, fibrillarin, and pre-rRNAssynthesized at G2/M phase of the previous cell cycle are directlyrecruited to UBF-associated nucleolar organizer regions (NORs)early in telophase before chromosome decondensation. Unlike thefusion of prenucleolar bodies to the nucleoli, this early recruitmentof processing factors and pre-rRNAs is independent of RNA polymeraseI transcription. In the absence of polymerase I transcription,the initial localization of nucleolin, fibrillarin, and pre-rRNAsto UBF-associated NORs generates segregated mininucleoli thatare similar to the larger ones observed in interphase cells grownunder the same conditions. Pre-rRNAs are juxtaposed to UBF-nucleolin-fibrillarincaps that may represent the segregated nucleoli observed by electronmicroscopy. These findings lead to a revised model of nucleologenesis.We propose that nucleolar formation at the end of mitosis resultsfrom direct recruitment of processing factors and pre-rRNAs toUBF-associated NORs before or at the onset of rDNA transcription.This is followed by fusion of prepackaged prenucleolar bodiesinto the nucleolus. Pre-ribosomal ribonucleoproteins synthesizedin the previous cell cycle may contribute to postmitoticnucleologenesis.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The nucleus is a complex structure within which various functions and components are spatially and temporally organized andinterregulated (reviewed by Lamond and Earnshaw, 1998; Dreyfussand Struhl, 1999). Nucleoli represent the most prominent exampleof this organization. The major function of the nucleolus is ribosomebiogenesis (reviewed by Busch and Smetana, 1970). rRNAs are synthesized,processed, cleaved, and assembled with ribosomal proteins in thenucleolus before export to the cytoplasm. The nucleolus is composedof three structurally distinguishable constituents: fibrillarcenters, dense fibrillar components, and granular components,as observed by electron microscopy (reviewed by Busch and Smetana,1970; Hadjiolov, 1985). Although the spatial and temporal relationshipbetween rRNA synthesis and the three structural constituents remainsto be clarified, it is generally thought that transcription ofrDNA takes place in a transient area between the fibrillar centersand the dense fibrillar components and that rRNA processing andpreribosomal particle assembly progress from the dense fibrillarcomponents to the surrounding granular components (reviewed bySpector et al., 1993; Shaw and Jordan, 1995; Scheer and Hock,1999). More recent evidence (reviewed by Pederson, 1998; Garciaand Pillus, 1999) suggests that nucleoli have additional functionsrelated to the cell cycle (Shou et al., 1999; Visintin et al.,1999), cellular aging (Straight et al., 1999), signal recognitionparticle biosynthesis (Jacobson and Pederson, 1998), small RNAprocessing, mRNA transport (reviewed by Pederson, 1998), and p53metabolism (Zhang and Xiong, 1999).

The essential mechanisms of nucleologenesis during postmitotic nucleolar reformation or de novo nucleolar generation in earlyembryogenesis are not clear. Electron microscopic and immunocytochemicalstudies show that at least part of nucleologenesis involves fusionbetween prepackaged prenucleolar bodies (PNBs) and NORs in postmitoticcells (Ochs et al., 1985; Jimenez-Garcia et al., 1994; Fomproixet al., 1998). Such fusion is prevented by treatment with a lowconcentration of actinomycin D (ActD) that inhibits polymeraseI (Pol I) transcription (Ochs et al., 1985). PNBs, spherical bodiesof 0.3-2 µm in diameter, are composed of densely packed RNP granulesand fibrils (Stevens, 1965). The PNBs generally contain factorsinvolved in pre-rRNA processing, including fibrillarin, nucleolin,B23, argyrophilic proteins, Nop52, PMScl-100 protein, and U3,U8, and U14 snoRNP (Ochs and Busch, 1984; Ochs et al., 1985; Jimenez-Garciaet al., 1994; Fomproix and Hernandez-Verdun, 1999; Savino et al.,1999). Before telophase, these complexes are distributed aroundthe chromosomes and diffusely throughout the mitotic cytoplasm(Gautier et al., 1992; Azum-Gelade et al., 1994). As the othernucleolar components, the Pol I transcription machinery, includingthe polymerase complex, and the Pol I-specific transcription factors,such as upstream binding factor (UBF) and SL1, bind to NORs throughoutmitosis when rDNA transcription is inactivated (Scheer and Rose,1984; Roussel et al. 1993; Gebrane-Younes et al., 1997). Interestingly,during mitosis the transcription machinery associates only withNORs that have been transcribed during the previous interphaseand will be transcriptionally active in the next cell cycle (Rousselet al., 1996). Accordingly, they were named competentNORs.

It has been proposed that the activation of rDNA transcription recruits the processing factors to the sites of transcription,thus facilitating PNB fusion (reviewed by Scheer and Hock, 1999).In this context, several studies have attempted to address therelationship between rDNA transcription and nucleolar assembly.Transcription of rDNA appears to induce nucleolus-like structures.Using a yeast rDNA deletion mutant, Oakes et al. (1998) foundthat transcription of rDNA by Pol I from a plasmid induced multiplesmall dense structures, "mininucleoli," whereas transcriptionof rDNA by Pol II formed an aggregated larger structure. Insertionof an actively transcribing rDNA repeat into Drosophila polytenechromosomes resulted in dense mininucleoli around the transcriptionsites (Karpen et al., 1988). These findings demonstrate that transcriptionof rDNA alone generates dense structures that do not resembletypical nucleoli with well-organized and classically defined structuralfeatures. Verheggen et al. (1998) found that during Xenopus laevisdevelopment maternal pre-rRNAs are present in nucleolin-concentratedstructures with features of transcriptionally competent nucleoli.However, rRNA synthesis was not detected with the use of an insitu run-on method, suggesting that nucleoli form before the activationof Pol I transcription. Another group of studies used ActD (Ochset al., 1985) or DNA topoisomerase I inhibitor (Weisenberger etal., 1993) or anti-Pol I antibody injection (Benavente et al.,1987) to assess the regeneration of nucleoli in mammalian cells.The results of these studies suggested that typical nucleoli werenot assembled when cells progressed into G1 under any of theseconditions. Instead, electron micrographs revealed round structurescontaining dense fibrillar and granular elements, or altered PNBs(Ochs et al., 1985; Benavente et al., 1987). These studies suggestthat rDNA transcription may not be necessary or sufficient forthe assembly of typical nucleoli. Therefore, nucleolar assemblyshould be examined as complex integrated events involving rDNAtranscription and other not yet definedmechanisms.

In this paper, we examined the temporal distribution of Pol I transcription and pre-rRNA processing factors, including UBF,nucleolin, and fibrillarin, as well as pre-rRNAs throughout mitosisand the beginning of interphase. We report for the first timethat nucleologenesis also involves direct recruitment of processingfactors and pre-rRNAs to transcription factor-associated NORsvery early at the end of mitosis. Unlike the fusion of PNBs, thisprocess is independent of Pol I transcription. We also find thatpre-rRNAs synthesized in the previous cell cycle participate inthe assembly of daughter cell nucleoli, suggesting that theseRNAs may play a role in structuringnucleoli.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell Cultures

HeLa cells were maintained in DMEM supplemented with 10% FBS at 37°C and 5% CO₂. Cells were passed twice a week. Mitotic cellswere synchronized by treatment with nocodazole at 0.05 µg/ml for4 h, with colchicine at 0.02 µg/ml for 14 h, or were synchronizedby double thymidine block as described (Sirri et al., 1999). Inthe latter case, 9 h after release from 2'-deoxycytidine, 80%of the cells accumulated in early prophase. ActD was added 1 hbefore the harvest at a final concentration of 0.04 µg/ml. Mitoticcells were collected through centrifugation and allowed to progressinto G1 phase in the presence of the same concentration of ActD.One hour to 4 h after reseeding, cells were fixed in 2% formaldehydeand subjected to immunofluorescence or in situ hybridizationstudies.

In Situ Hybridization

In situ hybridization was performed according to a modified protocol described previously (Huang and Spector, 1991; Verheggenet al., 1998). Fixed cells were washed three times for 15 mineach in PBS and permeabilized in 0.5% Triton X-100 for 5 min at4°C. For double labeling with immunodetection of UBF, nucleolin,or fibrillarin, cells were incubated with primary and secondaryantibodies and subsequently fixed again with 2% formaldehyde for5 min. Cells were then rinsed in PBS two times for 15 min eachand once with 2× SSC followed byhybridization.

The probe corresponding to human rRNA 5' external transcribed spacer (ETS) core sequences (+693 to +2921) was provided byDr. J. Sylvester (Sylvester et al., 1986), or a shorter sequence(+933 to +1445) was provided by Dr. M. Olson (Dundr et al., 1998).The probe corresponding to human 28S rRNA (+12,383 to +12,969)was subcloned from p3'ETS that spans the 3' end of 28S and the5' end of the 3'ETS sequence provided by Dr. M. Olson. Probe sequenceswere excised and gel purified. Probes were labeled by nick translationin the presence of biotin-conjugated dUTP or dCTP (Clontech, PaloAlto, CA). One hundred to 500 ng of labeled probe was dried ina Speed-vac, together with 20 µg of Escherichia coli tRNA and5 µg of sheared salmon sperm DNA. The pellet was resuspended in10 µl of deionized formamide, heat-denatured at 75°C for 10 min,and rapidly cooled in ice-water slurry. The final 20-µl hybridizationmixture (2× SSC, 10 mM Tris-HCl, pH 7.2, 1 mM EDTA, 5% dextransulfate, 50% [vol/vol] formamide, denatured probe, tRNA, and shearedsalmon sperm DNA) was applied to each coverslip, which was theninverted onto a ribonuclease-free glass slide and sealed withrubber cement. Hybridization was carried out at 37°C in a humidifiedchamber overnight. After hybridization, cells were washed threetimes in 2× SSC and once in 1× SSC. Signals were detected by incubationwith FITC or Texas Red-conjugated avidin (Jackson ImmunoResearch,West Grove, PA) at a dilution of 1:200 in 4× SSC for 1 h at roomtemperature or a rabbit anti-biotin antibody (Enzo, Farmingdale,NY) amplified by two-step detection with the use of mouse anti-rabbitand FITC-conjugated goat anti-mouse antibody (Jackson ImmunoResearch).Cells were washed in 4× SSC three times beforemounting.

Northern Blot Analysis

RNA was extracted from cells with the use of an RNA Now kit (Biogentex, Seabrook, TX). The RNA extracts were then treatedas described previously (Verheggen et al., 1998). RNAs were denatured(50% formamide, 1.84 M formaldehyde, and 10 mM sodium phosphatebuffer) for 15 min at 68°C and then run on a 0.8% agarose gel.After transfer onto a nitrocellulose filter, rRNAs were revealedby hybridization with ³²P-labeled 5'ETS probes for 20 h at 42°C. Autoradiography was performedwith a Phosphorimager (Molecular Dynamics, Sunnyvale, CA). RNAsize was determined by comparison with an RNA ladder (GIBCO-BRL,Gaithersburg,MD).

Br-UTP Incorporation Assay

The transcription assay was modified from published studies (Jackson et al., 1993; Wansink et al., 1993). Cells were rinsedonce with PBS and once with a Tris buffer (20 mM Tris-HCl, pH7.4, 5 mM MgCl₂, 25% glycerol, 0.5 mM PMSF, 0.5 mM EGTA). Cellswere then permeabilized in the same buffer containing 5 µg/mldigitonin at room temperature for 3 min. Subsequently, cells wereincubated in transcription cocktail (100 mM KCl, 50 mM Tris-HCl,pH 7.4, 5 mM MgCl₂, 0.5 mM EGTA, 25% glycerol, 1 mM PMSF, 2 mMATP, 0.5 mM CTP, 0.5 mM GTP, 0.2 mM Br-UTP, 1 U/ml RNAsin) for5 min at 37°C. At the end of the transcription reaction, cellswere gently rinsed three times with PBS and then fixed in 2% paraformaldehydein PBS for 15min.

Immunolabeling

For immunolabeling, cells were fixed in 2% freshly prepared formaldehyde in PBS for 15 min. Cells were washed three timesfor 10 min each in PBS, and coverslips were then incubated withprimary antibody. Antibodies used in this study included anti-UBF-specifichuman serum at a dilution of 1:300 (Chan et al., 1991; Rousselet al., 1993), anti-nucleolin mAb at a dilution of 1:3000 (Pinol-Roma,1999), anti-fibrillarin human serum at a dilution of 1:100 (Gautieret al., 1994), anti-SC35 at a dilution of 1:1000 (Fu and Maniatis,1990), anti-hnRNP A1 at a dilution of 1:300 (Pinol-Roma and Dreyfuss,1992), and anti-Br-UTP mAb at a dilution of 1:500 (Sigma Chemical,St. Louis, MO) for 1 h at room temperature. Cells were rinsedin PBS, incubated with Texas Red-conjugated goat anti-human antiserumor with FITC or Texas Red-conjugated goat anti-mouse antiserumat a dilution of 1:200 for 1 h at room temperature and then washedthree times for 10 min each in PBS. The coverslips were mountedonto glass slides with mounting medium containing 90% glycerolin PBS with 1 mg/ml paraphenylenediamine as an antifade agent.The mounting medium was adjusted to pH 8.0 with 0.2 M bicarbonatebuffer. Cells were examined with a TCS 4D Leica (Deerfield, IL)confocal microscope equipped with an argon-krypton laser and witha Zeiss (Thornwood, NY) Axiovert microscope equipped with epifluorescenceand differential interference contrast optics. Images were capturedby a SenSys cooled charge-coupled device camera (Photometrics,Tucson, AZ) with the use of Metamorph Image software (UniversalImaging Corp, West Chester,PA).

Electron Microscopy

Cells were fixed in 4% paraformaldehyde and 2% glutaraldehyde for 20 min and washed in PBS containing 0.3 M glycine and 0.1M cacodylate buffer. Cells were then postfixed in 1% osmium tetroxidefor 1 h, dehydrated by incubation in a series of ascending concentrationsof ethanol, and embedded in epon/araldite at 60°C for 48 h. Eighty-nanometersections were poststained with uranyl acetate-lead citrate andexamined at 75 kV with a JEOL (Tokyo, Japan) JEM-1220 transmissionelectronmicroscope.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Pre-rRNA Processing Factors Are Directly Recruited to Active NORs at Early Telophase Independently of rDNA Transcription

To understand the chronological sequence of nucleologenesis, we examined the distribution of a Pol I transcription factor(UBF), pre-rRNA processing factors (nucleolin and fibrillarin),and the spatial relationship between these two groups of factorsthroughout mitosis into early G1. UBF was detected by a specifichuman autoimmune serum (Chan et al., 1991; Roussel et al., 1993),and nucleolin was detected by a mAb, 7G2 (Pinol-Roma, 1999). UBFis associated with competent NORs throughout mitosis (Figure 1,A and B). Nucleolin, in addition to being distributed diffuselythroughout the mitotic cytoplasm, appears to sheath the condensedchromosomes during mitosis (Figure 1A') and forms PNBs at telophase.These observations are similar to the descriptions in the publishedliterature (Scheer and Rose, 1984; Roussel et al., 1996; reviewedby Ginisty et al., 1999). In addition, we find that at early telophasenucleolin is rapidly relocated into daughter cell nuclei and isconcentrated in dots in which UBF-associated competent NORs arepresent (Figure 1, B-B'') before chromosome decondensation (Figure1B'''). Immunolabeling of fibrillarin also shows a similar distribution(our unpublished results). These findings suggest that the recruitmentof processing factors to the competent NORs may take place beforeor at the onset of rDNA transcription and that the initial recruitmentmay not be in the form of fusion with PNBs. This suggestion issupported by the subsequent observations in cells exiting mitosisin the presence of a low concentration of ActD.

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Figure 1. Nucleolin is recruited directly to UBF-associated NORs early in telophase independent of Pol I transcription. Each row represents the same cells immunolabeled for UBF (first column) and nucleolin (second column), UBF and nucleolin overlay (third column), and differential interference contrast images to identify the cell cycle stages (fourth column). Rows A and B represent cells growing in normal medium (A, metaphase; B, telophase). Rows C-E represent cells at different stages through mitosis to G1 in the presence of 0.04 µg/ml ActD. Nucleolin is recruited before the decondensation of chromosomes (B-B''', arrows). The recruitment is not interrupted in the absence of Pol I transcription (D-D''', arrows). Toward late telophase, UBF and nucleolin colocalize to cap-like structures that juxtapose or surround dense bodies (Row E, arrows). Row F represents interphase cells treated with 0.04 µg/ml ActD. Cap-like structures (arrows) are associated with segregated nucleoli. All images are 0.8-µm optical sections obtained with the use of confocal laser scanning microscopy. Bars, 10 µm.

ActD has been shown to prevent RNA polymerases from functioning by intercalating into DNA, preferentially targeting G/C-richsequences (Sobell, 1979). At a very low concentration of 0.04µg/ml, ActD selectively inhibits RNA Pol I activity as a resultof the higher G/C contents of the rDNA (Perry, 1963). Nuclearrun-on experiments show that rRNA transcription in HeLa cellsis reduced to <1% of its normal level within 1 h of ActD (0.04µg/ml) treatment (Penman et al., 1968; D. Chen and S. Huang, unpublishedresults).

To understand nucleologenesis in the absence of Pol I transcription, we compared the localization of UBF, nucleolin, and fibrillarinthroughout mitosis in cells grown in a low concentration of ActDwith those grown in drug-free medium. The results demonstratethat the rDNA transcription factor UBF remains associated withcompetent NORs throughout mitosis and within the newly formednuclei (Figure 1, C and D) in a similar manner in both treatedand nontreated cells (Figure 1, compare A with C and B with D).However, the increase in UBF signal at the active NORs duringnucleologenesis no longer takes place in drug-treated cells (Figure1E), and UBF forms cap-like structures on the newly developedmininucleoli (Figure 1E, arrow). The dynamics of pre-rRNA processingfactors throughout mitosis into early G1 is also significantlychanged in the presence of ActD. Nucleolin no longer sheathescondensed chromosomes during mitosis (Figure 1C'). Nucleolar assemblyin the form of fusion of the PNBs is interrupted (Figure 1E').However, the initial recruitment of nucleolin (Figure 1D', arrows)and fibrillarin (Figure 2A') to UBF-associated NORs continuesin drug-treated cells. The recruited nucleolin (Figure 1E', arrows)and fibrillarin (Figure 2B') at NORs become colocalized with UBF,forming cap-like structures at early G1 phase. These findingsdemonstrate that intercalation of ActD into rDNA does not affectthe association of rDNA transcription machinery to the NORs duringmitosis. Nor does it prevent the initial recruitment of pre-rRNAprocessing factors to the UBF-associated NORs early in telophase.However, it does disrupt the fusion between PNBs and NORs in amanner similar to the descriptions of Ochs et al. (1985) and Benaventeet al. (1987). The findings that the early recruitment of processingfactors are Pol I transcription independent support the idea thatthis process is a novel mechanism of nucleologenesis that takesplace in addition to the process of fusion between PNBs and NORs.

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Figure 2. The recruitment of fibrillarin directly to UBF-associated NORs (arrows) in early telophase is not disrupted in the presence of 0.04 µg/ml ActD (A-A''). When cells progress to early G1, fibrillarin is colocalized with UBF to cap-like structures (B-B''). Each row represents the same cells immunolabeled for UBF (first column) and fibrillarin (second column), UBF and fibrillarin overlay (third column), and phase contrast to identify the cell cycle stages (fourth column). Bar, 10 µm.

To determine whether treatment of ActD at 0.04 µg/ml may significantly influence other polymerase activities or nuclear structurein general, we monitored several indicators of Pol II transcriptionand nuclear structure. In situ incorporation of Br-UTP after 5min of pulse labeling was compared between cells treated and nottreated with ActD. Metaphase cells were pretreated with 0.04 µg/mlActD and reseeded in the presence of the drug. Four hours afterreplating, the early G1 cells were briefly permeabilized and incubatedat 37°C in a transcription cocktail containing Br-UTP for 5 min.The results show that Br-UTP incorporation is not detected inmininucleoli of the G1 cells that exit mitosis in the presenceof ActD (Figure 3, A and B, arrows) but is detected in nucleoliof cells grown in drug-free medium (Figure 3, A' and B', arrows).In contrast, the nucleoplasmic incorporation of Br-UTP is notobviously changed in cells treated with ActD (Figure 3, A andA'), demonstrating that ActD treatment at this concentration selectivelyinhibits RNA Pol I transcription with little effect on Pol IIand Pol III transcription. Similar observations were also madein interphase cells treated or not treated with the same concentrationof ActD (our unpublished results). In addition to Br-UTP incorporation,we also examined the localization of an RNA splicing factor whosedistribution is sensitive to RNA Pol II transcription inhibition.Immunolabeling with the use of a mAb specifically recognizingSC35, a member of the SR family (Fu and Maniatis, 1990), doesnot show significant changes in its speckled labeling patternin cells treated with the drug (Figure 3C). Furthermore, the distributionof hnRNP proteins that shuttle between the nucleus and the cytoplasmin a transcription-dependent manner, such as hnRNP A1, was alsoexamined. The hnRNP proteins primarily bind pre-mRNA and are implicatedin the processing and transport of mRNA (recently reviewed byKrecic and Swanson, 1999). HnRNP A1 becomes cytoplasmically distributedduring transcription inhibition with the use of a high concentrationof ActD that inhibits all RNA polymerase activities (Pinol-Romaand Dreyfuss, 1992). Presumably, the nuclear localization is dependenton Pol II transcription. When cells were treated with 0.04 µg/mlActD, the cytoplasmic accumulation of hnRNP A1 was not detected(Figure 3D), suggesting that Pol II transcription is not significantlyaltered. These results demonstrate that 0.04 µg/ml ActD selectivelyinhibits RNA Pol I transcription and does not significantly affectthe nucleoplasmic transcription and the distribution of othernuclear constituents.

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Figure 3. ActD at a concentration of 0.04 µg/ml selectively inhibits Pol I transcription without significantly affecting other polymerases and general nuclear organization. A and A' show the in situ incorporation of Br-UTP, and B and B' show the same cells corresponding to those in A and A' immunolabeled with anti-fibrillarin antibody. Daughter cells grown in the presence of ActD form mininucleoli that are immunolabeled with anti-fibrillarin antibody (B, arrows). They do not incorporate Br-UTP (A, arrows), whereas untreated nucleoli (B', arrows) actively incorporate Br-UTP after pulse labeling (A'). Although Br-UTP incorporation in nucleoli declines in treated cells, the nucleoplasmic Br-UTP incorporation from Pol II and Pol III transcription is not altered (A). The speckled distribution of SC35 (C) and the predominantly nuclear localization of hnRNP A1 (D) are also not changed significantly in treated cells. Bar, 10 µm.

Segregated Mininucleoli That Differ from PNBs Are Developed in the Absence of rDNA Transcription

We reexamined nucleolar development in daughter cells progressing into G1 in the absence of Pol I transcription. Mitotic cellsthat were synchronized with the use of nocodazole were treatedwith ActD (0.04 µg/ml) 1 h before being released into the cellcycle in the presence of the same concentration of ActD. Fourhours after reseeding, the cells were fixed and examined. Comparedwith untreated cells that form typical nucleoli at early G1, treatedcells develop much smaller nucleolus-like structures. These structuresare dense and recognizable by Nomarski or phase contrast microscopy(our unpublished results). To analyze them at higher resolution,G1 cells that had exited mitosis in the presence or absence ofActD were optimally fixed and examined by electron microscopy.In cells treated with ActD, two types of nucleolus-related structureswere observed. The small, round, and electron-dense structuresresemble typical PNBs (Figure 4B, arrows). The PNBs usually arenot detectable in G1 cells because most should have fused to formtypical nucleoli (Figure 4A). Another type of dense structures(Figure 4B, arrowheads), intermediate in size between PNBs andtypical nucleoli, resemble the segregated nucleoli observed ininterphase cells grown at the same concentration of ActD (Figure4C, arrowhead). They contain segregated and densely packed fibrillarand granular components. These structures seem to correspond tothose observed at the light microscopic level, in which the UBF-nucleolin-fibrillarin-containingcaps juxtapose or surround dense structures (Figures 1E and 2,B and B'). We interpret these structures to be segregated mininucleolirather than unfused and altered PNBs. These observations suggestthat mininucleoli, although significantly changed in structure,are able to assemble in the absence of Pol I transcription.

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Figure 4. Electron microscopic observations demonstrate that cells progressing into G1 phase in the presence of 0.04 µg/ml ActD assemble segregated mininucleoli (B, arrowheads). In addition, unfused PNBs could be visualized in the nucleoplasm of treated cells (B, arrows). (A) A normal G1 cell nucleus. (B) A G1 cell exiting mitosis in the presence of 0.04 µg/ml ActD. (C) An interphase cell treated with the same concentration of ActD. Bars, 1 µm.

Pre-rRNAs Synthesized in the Previous Cell Cycle Are Recruited to Newly Formed Daughter Cell Nuclei

To analyze the distribution of rRNAs through mitosis into early G1, we examined rRNA distribution with the use of in situhybridization with probes complementary to either 28S rRNAs or5'ETS core-containing pre-rRNAs. The results demonstrate that28S rRNAs are present in early G1 nuclei in addition to beingdistributed in the cytoplasm (Figure 5, top panels, arrows). Thenuclear 28S rRNAs along with nucleolin are detected in two typesof structures, the growing nucleoli and not-yet-fused PNBs (Figure5, top panels, arrowheads). To determine whether the rRNAs detectedwith the use of the 28S probe represent precursor or mature rRNAs,the 5'ETS probe was used to examine the presence of 45S or 30SrRNAs. Double labeling of 5'ETS containing pre-rRNAs and nucleolin(Figure 5, bottom panels, arrows) reveals a similar observationas that observed with the use of the 28S probe. This finding demonstratesthat at least part of the rRNAs detected with the use of the 28Sprobe in the growing nucleoli and PNBs represent 45S or 30S pre-rRNAs.Although the nucleolus-associated pre-rRNAs could be explainedas newly synthesized rRNAs upon the activation of rDNA transcription,the PNB-associated pre-rRNAs are most likely derived from theprevious cell cycle, because PNBs contain neither rDNA nor PolI transcription factors and therefore could not be the sites ofrDNA synthesis.

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Figure 5. Pre-rRNAs and 28S rRNAs synthesized at the previous cell cycle reenter early G1 daughter cell nuclei. 28S rRNA probe (top) and 5'ETS core probe (bottom) both hybridize to rRNAs that are associated with growing nucleoli (arrows) and nucleolin-containing PNBs (arrowheads). Bar, 10 µm.

To analyze the stability of pre-rRNAs through mitosis into the next cell cycle, we compared the levels of these RNAs in mitosisand interphase with the use of Northern blotting. Mitotic cellswere synchronized with either colchicine or double thymidine blocks.Equal amounts of total RNA from mitotic and interphase cell lysateswere hybridized with the 5'ETS core probe. The results demonstratethat both 45S and 30S pre-rRNAs are detectable in mitotic cellswith the use of either synchronization protocol (Figure 6A), althoughthe level of the pre-rRNAs is significantly less than that ofinterphase cells. This finding demonstrates that some of the 5'ETScontaining pre-rRNAs made during the previous cell cycle are stablethrough mitosis. This observation is unlikely to be due to anyadverse effects of the drugs used in synchronization because twodifferent methods of synchronization give rise to similar results.To analyze when these pre-rRNAs are synthesized, ActD (0.04 µg/ml)was added at different phases of the cell cycle of synchronizedcells. When rDNA transcription is inhibited during G2 throughmitosis, the level of the mitotic 45S rRNAs is significantly reduced(Figure 6B). In contrast, when rDNA transcription is inhibitedat early telophase, the level of 45S rRNAs is not altered (Figure6B). These findings suggest that 45S or 30S pre-rRNAs are synthesizedpredominantly near the G2/M transition and are maintained throughoutmitosis into G1 of the next cell cycle.

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Figure 6. Pre-rRNAs (45S and 30S) containing 5'ETS core are detected through mitosis and synthesized during G2/M. (A) Northern blot hybridized with 5'ETS core probe showing that 45S and 30S pre-rRNAs are maintained in mitotic cells (M) synchronized with the use of either colchicine (C) or double thymidine block (S). The levels of these RNAs are less than those in interphase (I). (B) Northern blot hybridized with 5'ETS core probe to RNAs from early G1 cells that were treated with 0.04 µg/ml ActD at G2/M (G2) or telophase (Telo). ( $-$ ) RNA extracted from control cells that were not treated with ActD. Treatment in G2 significantly reduces the detectable 45S rRNAs, whereas inhibition of Pol I transcription from mitosis to G1 still allows the maintenance of sizable amounts of 45S rRNA.

To clarify the origin of pre-rRNAs detected in the growing nucleoli and PNBs at the beginning of the cell cycle, we examinedthe distribution of these RNAs in cells progressing into G1 inthe absence of Pol I transcription (Figure 7). Pre-rRNAs weredetected by in situ hybridization with the use of either the 5'ETScore or the 28S probes. The localization of these RNAs was comparedwith the localization of UBF, fibrillarin, and nucleolin. In theabsence of Pol I transcription, pre-rRNAs are observed in 10-20foci in the nucleoplasm (Figure 7). Some are colocalized withnucleolin-associated PNBs that are unable to fuse with NORs (Figure7, A and B, arrowheads). Others are associated with the UBF-associatedNORs that fail to enlarge into typical nucleoli (Figure 7C, arrows).UBF-nucleolin-fibrillarin cap-like structures surround the pre-rRNAstaining (Figure 7, arrows). These caps may represent the densefibrillar cap-like structures observed by electron microscopy(Figure 4), and pre-rRNAs may represent the granular region (Figure4). The presence of pre-rRNAs in new daughter nuclei exiting mitosisin the absence of Pol I transcription further supports the notionthat the pre-rRNAs detected in PNBs and at NORs early in telophaseare derived from the previous cell cycle.

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Figure 7. Pre-rRNAs and possibly 28S rRNAs are recruited to newly formed nuclei in the presence of 0.04 µg/ml ActD. They are colocalized with nucleolin (A and B)-associated PNBs (arrowheads) and are adjacent to UBF (C) and fibrillarin (D)-associated NORs (arrows). Bars, 10 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Direct Recruitment of Nucleolar Factors to NORs Is Independent of PNBs and RNA Pol I Transcription

Nucleologenesis involves the assembly of nucleolar components around rDNA-containing chromosomes to establish morphologicallywell-defined structures at the beginning of interphase. Previousstudies have shown that the formation of nucleoli is the consequenceof, at least in part, the fusion between preassembled particlescontaining pre-rRNA processing factors, PNBs, and transcriptionmachinery-associated NORs (Ochs et al., 1985; Jimenez-Garcia etal., 1994; Fomproix et al., 1998). This process is Pol I transcriptiondependent (Ochs et al., 1985; Benavente et al., 1987). In thisreport, we provide evidence of a previously undefined mechanismduring nucleologenesis. In addition to fusion between NORs andPNBs, pre-rRNA processing factors are directly recruited to NORsearly in telophase before chromatin decondensation. These initialrecruitments are not disrupted in the absence of Pol I transcription.Because the cell cycle progresses despite Pol I transcriptioninhibition, our findings suggest that the initial events couldbe regulated by means other than activation of Pol I transcription.Recently, it was demonstrated that the activation of Pol I transcriptionis dependent on the level of cdc2-cyclin B activity when cellsenter G1 (Sirri et al., 2000). We speculate that the initial recruitmentof pre-rRNA processing factors might be regulated by kinases and/orphosphatases involved in the transition from mitosis to interphase.Pre-rRNA processing factors could be recruited to NORs to forma complex with the existing transcription machinery, and the complexcould subsequently carry out transcription and processing of rRNAsimultaneously. This hypothesis is in agreement with earlier electronmicroscopic observations of active transcription units that suggestthat newly synthesized rRNAs are associated with RNA-binding proteinscotranscriptionally (reviewed by Miller, 1981; Osheim and Beyer1998). Furthermore, recent studies in the RNA Pol II transcriptionsystem show that transcription factors are associated premRNAprocessing factors and may be recruited to the sites of transcriptionin the same complex (Gall et al., 1999) and that premRNA processingtakes place cotranscriptionally (recently reviewed by Bentley,1999). We propose that a similar situation may also take placeduring Pol Itranscription.

Structurally Altered Mininucleoli Are Assembled in the Absence of Pol I Transcription

In this report, we reevaluate nucleologenesis in cells treated with a low concentration of ActD. Cells that progress intoG1 in the absence of Pol I transcription exhibit two types ofnucleolus-related structures, PNBs and segregated nucleoli. Themorphological characteristics of these structures are similarto those illustrated by Ochs et al. (1985) and Benavente et al.(1987). They were described as segregated PNBs or round densefibrogranular structures (Ochs et al., 1985; Benavente et al.,1987). Considering our observations at the light microscopic level,we interpret these structures to be segregated mininucleoli forthe following reasons. 1) Morphologically, these structures resemblesegregated nucleoli of interphase cells treated with the sameconcentration of ActD. They are composed of segregated fibrillarand granular components. 2) These structures appear to correspondto those observed at the light microscopic level, in which UBF-nucleolin-fibrillarincap-like structures juxtapose pre-rRNAs. These segregated structuresare composed of both transcription factor-associated NORs andcomponents of pre-rRNA processing factors; thus, they resemblenucleoli more than PNBs, which typically do not contain rDNA andtranscription factors. Based on these findings, we propose thatnucleologenesis is independent of Pol I transcription. The earlyrecruitment of processing factors and pre-rRNAs to NORs takesplace before or at the onset of Pol I transcription. This modelis in agreement with the observation that nucleolus-like structuresassemble before the onset of rDNA transcription during Xenopuslaevis development (Verheggen et al., 1998). However, the developmentof mature nucleoli by means of PNB fusion does require Pol I transcription,because PNBs fail to fuse with NORs in the presence of a low concentrationof ActD, as also described by Ochs et al. (1985), and Benaventeet al. (1987).

Pre-rRNAs Synthesized in the Previous Cell Cycle May Contribute to Nucleologenesis

Detection of 5'ETS core-containing pre-rRNAs and 28S rRNAs in cells exiting mitosis reveals that pre-rRNAs (45S and 30S) derivedfrom the previous cell cycle are stable through mitosis and reenterdaughter cell nuclei. These RNAs are predominantly synthesizednear the G2/M transition of the last cell cycle and are distributedaround interchromosomal spaces as well as in the mitotic cytoplasm.At telophase, they are recruited to UBF-associated NORs and arecolocalized with nucleolin in PNBs. When Pol I transcription isinhibited, the initial recruitment of pre-rRNAs to the NORs continues.However, the PNB-associated pre-rRNAs no longer fuse with NORsand remain in the nucleoplasm through G1 phase. These findingssuggest that the pre-rRNAs may participate in nucleolar assembly.However, it is not clear whether all the rRNAs detected with theuse of the 28S probe represent pre-rRNAs. When probes for both5'ETS-containing and 28S rRNAs of the same length are used, itappears that the hybridization intensity is stronger for 28S rRNAsthan for 5'ETS-containing rRNAs, suggesting that 28S rRNAs mayalso enter daughter cell nuclei. Our findings provide the firstevidence that pre-rRNAs synthesized in the previous cell cycleare included in the nucleologenesis in newly formed daughter cellnuclei. These findings are consistent with the biochemical analysisthat the 5'ETS-containing 45S, 30S, and the 28S rRNAs are maintainedthrough mitosis (Fan and Penman, 1971; Pinol-Roma, 1999) and thatall of them are detected in nucleolin-containing RNPs (Pinol-Roma,1999). Our observations are also in agreement with the findingsdescribed by Dundr et al. (1998) that pre-rRNAs are present innucleolus-derived foci along with multiple pre-rRNA processingfactors through mitosis (Dundr and Olson, 1998). Furthermore,the presence of pre-rRNAs in newly formed mininucleoli in theabsence of Pol I transcription is in agreement with the observationthat maternal pre-rRNAs are associated with newly formed nucleolibefore the onset of rDNA transcription in Xenopus laevis embryos(Verheggen et al., 1998).

What might be the function of pre-rRNAs and their binding proteins during nucleologenesis? Several possible explanations areconsidered. 1) These rRNAs may form a macromolecular complex withpre-rRNA processing factors, and the complex may contribute tothe architecture of newly formed nucleoli. 2) The complex mayalso represent a way of regulating the availability and the activestatus of pre-rRNA processing factors. 3) Alternatively, theycould be recruited because of their binding to the processingfactors. It is also intriguing that the existing pre-rRNAs aresegregated from nucleolin, fibrillarin, and UBF in cells thatprogress into G1 when Pol I transcription is inhibited. The significanceand mechanism of the pre-rRNA recruitment to newly formed daughternuclei will be investigatedfurther.

Based on the observations from our laboratory and other laboratories, we propose a revised model of nucleologenesis (Figure8). At early telophase, competent NORs that are associated withthe transcriptional machinery, including UBF, SL1, and RNA PolI, rapidly and directly recruit pre-rRNA processing factors alongwith existing pre-rRNAs. This initial recruitment may take placebefore or at the onset of rDNA transcription. Subsequently, moretranscription and processing factors are also recruited in formsof PNBs to small but enlarging nucleoli. The process of PNB fusionrequires rDNA transcription. Pre-rRNAs derived from the previouscell cycle may contribute to nucleologenesis.

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Figure 8. Scheme of the revised model of nucleologenesis.

	ACKNOWLEDGMENTS

The authors are grateful to J. Sylvester for the rDNA human probes and to G. Géraud for help with confocal microscopy. Weacknowledge the Association pour la Recherche sur le Cancer (contract5304) and the Centre National de la Recherche Scientifique forsupport. Our thanks also extend to Drs. E.K.L. Chen, S. Pinol-Roma,M. Dundr, and M.O.J. Olson for providing antibodies and rDNA constructs.We would also like to thank Drs. S. Adam, R. Moir, T. Pederson,T. Spann, and D. Spector for helpful comments. This work was partiallysupported by grants to S.H. from the National Cancer Institute(1 RO1 CA77560-01A1 and 5 K01 CA74988-03).

	FOOTNOTES

^* These authors contributed equally to thiswork.

^§ Corresponding author. E-mail address: s-huang2{at}nwu.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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				J. C. Politz, L. B. Lewandowski, and T. Pederson Signal recognition particle RNA localization within the nucleolus differs from the classical sites of ribosome synthesis J. Cell Biol., November 7, 2002; 159(3): 411 - 418. [Abstract] [Full Text] [PDF]

				P. Bjork, G. Bauren, S. Jin, Y.-G. Tong, T. R. Burglin, U. Hellman, and L. Wieslander A Novel Conserved RNA-binding Domain Protein, RBD-1, Is Essential For Ribosome Biogenesis Mol. Biol. Cell, October 1, 2002; 13(10): 3683 - 3695. [Abstract] [Full Text] [PDF]

				S. Fujiyama, M. Yanagida, T. Hayano, Y. Miura, T. Isobe, and N. Takahashi Isolation and Proteomic Characterization of Human Parvulin-associating Preribosomal Ribonucleoprotein Complexes J. Biol. Chem., June 21, 2002; 277(26): 23773 - 23780. [Abstract] [Full Text] [PDF]

				V. Sirri, D. Hernandez-Verdun, and P. Roussel Cyclin-dependent kinases govern formation and maintenance of the nucleolus J. Cell Biol., March 18, 2002; 156(6): 969 - 981. [Abstract] [Full Text] [PDF]

				D. Viuff, T. Greve, P. Holm, H. Callesen, P. Hyttel, and P. D. Thomsen Activation of the Ribosomal RNA Genes Late in the Third Cell Cycle of Porcine Embryos Biol Reprod, March 1, 2002; 66(3): 629 - 634. [Abstract] [Full Text] [PDF]

				D. Hernandez-Verdun, P. Roussel, and J. Gebrane-Younes Emerging concepts of nucleolar assembly J. Cell Sci., January 6, 2002; 115(11): 2265 - 2270. [Abstract] [Full Text] [PDF]

				S. Kneissel, W. W. Franke, J. G. Gall, H. Heid, S. Reidenbach, M. Schnolzer, H. Spring, H. Zentgraf, and M. S. Schmidt-Zachmann A Novel Karyoskeletal Protein: Characterization of Protein NO145, the Major Component of Nucleolar Cortical Skeleton in Xenopus Oocytes Mol. Biol. Cell, December 1, 2001; 12(12): 3904 - 3918. [Abstract] [Full Text] [PDF]

				H. G.E. Sutherland, G. K. Mumford, K. Newton, L. V. Ford, R. Farrall, G. Dellaire, J. F. Caceres, and W. A. Bickmore Large-scale identification of mammalian proteins localized to nuclear sub-compartments Hum. Mol. Genet., September 1, 2001; 10(18): 1995 - 2011. [Abstract] [Full Text] [PDF]

				T. M. Savino, J. Gebrane-Younes, J. De Mey, J.-B. Sibarita, and D. Hernandez-Verdun Nucleolar Assembly of the rRNA Processing Machinery in Living Cells J. Cell Biol., May 29, 2001; 153(5): 1097 - 1110. [Abstract] [Full Text] [PDF]

				D. Chen and S. Huang Nucleolar Components Involved in Ribosome Biogenesis Cycle between the Nucleolus and Nucleoplasm in Interphase Cells J. Cell Biol., April 2, 2001; 153(1): 169 - 176. [Abstract] [Full Text] [PDF]