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Original Article |
Correspondence to: Herbert Tschochner, Biochemie-Zentrum Heidelberg, Im Neuenheimer Feld 328, D-69120 Heidelberg, Germany. Tel:49-6221-544155 Fax:49-6221-544366 E-mail:im4{at}ix.urz.uni-heidelberg.de.
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Abstract |
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 Top Abstract IntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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A novel ribonucleoprotein complex enriched in nucleolar proteins was purified from yeast extracts and constituents were identified by mass spectrometry. When isolated from rapidly growing cells, the assembly contained ribonucleic acid (RNA) polymerase (pol) I, and some of its transcription factors like TATA-binding protein (TBP), Rrn3p, Rrn5p, Rrn7p, and Reb1p along with rRNA processing factors, like Nop1p, Cbf5p, Nhp2p, and Rrp5p. The small nucleolar RNAs (snoRNAs) U3, U14, and MRP were also found to be associated with the complex, which supports accurate transcription, termination, and pseudouridylation of rRNA. Formation of the complex did not depend on pol I, and the complex could efficiently recruit exogenous pol I into active ribosomal DNA (rDNA) transcription units. Visualization of the complex by electron microscopy and immunogold labeling revealed a characteristic cluster-forming network of nonuniform size containing nucleolar proteins like Nop1p and Fpr3p and attached pol I. Our results support the idea that a functional nucleolar subdomain formed independently of the state of rDNA transcription may serve as a scaffold for coordinated rRNA synthesis and processing.
Key Words: in vitro transcription, Saccharomyces cerevisiae, ribosome biogenesis, matrix assisted laser desorption ionization (MALDI) mass spectrometry, nucleolus
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Introduction |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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The synthesis and processing of RNA require a complex network of protein–protein and protein–nucleic acids interactions. Immunofluoresence and EM observations suggest that all three eukaryotic nuclear RNA polymerases (pols)1 are involved in large transcription factories in distinct regions of the nucleus (
Interestingly, components involved in processing of rRNA, like the small nucleolar RNAs (snoRNAs) U14, U3, and MRP, or the protein Gar1p, were also shown to localize to the dense fibrillar component (
Large pol I–containing protein machineries that combine several enzymatic entities have been reported in plants, mice, and frogs (
A pol I–containing holoenzyme has yet to be reported in yeast. Initiation of transcription by pol I is dependent on the presence of the transcription initiation factors TATA-binding protein (TBP), core factor (CF), upstream activating factor (UAF), and Rrn3p, which have yet to be identified in a preassembled complex. The TATA-binding protein TBP (
Yeast pol I also requires other transcription factors for elongation and termination. These include Reb1p, which binds to the template and stops movement of pol I along the DNA in vitro (
Ribosomal RNA is processed by methylation, pseudouridylation, and cleavage to generate the mature 18S, 5.8S, and 25–28S rRNAs. Several proteins and many snoRNAs are required for these fundamental steps of rRNA maturation (for review see
The snoRNAs can be divided into three classes (
The goal of this study was to investigate how transcription and processing events are coupled. We have reported previously that all factors required for pol I–dependent transcription initiation copurify through several purification steps (
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Materials and Methods |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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Strains and Templates
Yeast wild-type strain BJ926, strain Gpy2 containing hemagglutinin (HA)-tagged A43 (generous gift of Drs. A. Setenac, C. Carles, M. Riva, and G. Peyroche, CEA/Saclay, Gif sur Yvette, France), strain YJV166 (generous gift of D. Tollervey, Institute of Cell and Molecular Biology [ICMB], Edinburgh, UK) (
135; generous gift of Dr. O. Gadal, Biochemie-Zentrum Heidelberg, Heidelberg, Germany), which contained a disruption in the second largest pol I subunit A135, strain NOY797 and NOY844, which contained HA-tagged Rrn7p and Rrn5p, respectively (generous gift of Dr. M. Nomura, University of California Irvine, Irvine, CA) (
In Vitro Transcription
Promoter-dependent and nonspecific transcription reactions were performed as described elsewhere (
Preparation of Whole Cell Extracts and Fractionation by Gel Filtration
Preparations of whole cell extracts (WCEs) on a small scale were performed as described (
Preparation of the Nucleolar RNP Assembly
Fraction PA600 (protein concentration 2.5–5 mg/ml) was prepared as described previously (
Gel Filtration of Fraction PA600 on Superose-6
50 µl of fraction PA600 was loaded on a Superose-6 column (SMART; Amersham Pharmacia Biotech) and processed in buffer BU300 (buffer BU supplemented with 300 mM potassium acetate) with a flow rate of 12.5 µl/min. Fractions of 0.05 ml were collected. 25 µl of each fraction was TCA-precipitated, separated by SDS-PAGE, and analyzed by Western blotting.
Purification of pol I
Homogenous pol I-A was a generous gift of C. Carles and colleagues (CEA/Saclay). pol I-p, a mixture of pol I–Rrn3p complex and of initiation inactive pol I, was purified as described previously (
Immunoprecipitation of HA-tagged pol I
4 ml of WCEs (12.5 mg/ml) derived from yeast strain Gpy2, which contained a HA-tagged (and His6-tagged) A43 subunit or control strains, was diluted sevenfold in buffer BU300, supplemented with 10 mg/ml milk powder, and immunoprecipitated with 0.025 ml anti-HA antibodies. Before the incubation with the yeast extracts, the antibodies were cross-linked to 0.05 ml protein A–Sepharose with 20 mM DMP (dimethyl-pimelidate) for 30 min at room temperature according to a protocol described elsewhere (
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Mass Spectrometry and Protein Identification
0.25 ml of the pol I–containing fraction B2000 (4.5 mg/ml) was loaded on a Sephacryl S-300 column and processed in buffer BU600 at a flow rate at 0.4 ml/min. 0.75-ml fractions were collected and 0.4 ml of the fraction with the highest protein concentration, which also contained the highest amount of pol I, was separated by 10% SDS-PAGE and silver-stained. The single bands were excised, washed, in-gel reduced, S-alkylated, and subjected to tryptic digestion as described (
Pseudouridylation
Analysis of pseudouridylation was performed as described previously (
Northern Blot Analysis
0.5 ml of fraction K350, T0, and P600 was phenol/chloroform extracted, ethanol precipitated, and analyzed on an agarose gel to standardize their content of nucleic acids. Finally 0.25% of fraction P600 and 0.13% of fraction K350 and T0 were loaded on a 1.2% agarose/formaldehyde gel. The RNA from WCEs was obtained from 100-ml cultures that were grown to an OD600 of 0.7. 10-ml aliquots were centrifuged for 5 min at 3,000 rpm, then washed in 10 ml diethylpyrocarbonate-water and centrifuged again. The pellet was resuspended in 500 µl diethylpyrocarbonate-water and mixed with 200 µl baked glass beads, 200 µl sterile filtrated detergent mix (2% Triton X-100, 1% SDS, 100 mM NaCl, 10 mM Tris, pH 8, 1 mM EDTA), and 300 µl phenol/chloroform (1:1). The probe was vortexed nine times for 20 s and cooled on ice between the cycles. After centrifugation for 10 min at 4°C at 14,000 g, the supernatant was phenol/chloroform extracted. 2 µl of the hydrous phase was loaded on the gel. Further analysis of the RNA was according to a protocol described elsewhere (
EM
Fractions PA600, PA600 135, and B2000 were diluted 100, 100, and 40 times, respectively, in buffer A (20 mM Hepes, pH 7.8, 2 mM MgCl2, 90 mM KOAc, 20% glycerol) to form the clusters. To prevent cluster formation, buffer A had to be supplemented with KOAc to reach a final concentration >100 mM. 6-nm colloidal gold particles were coupled to antibodies as described by the manufacturer (Aurion). A slight excess of antibodies was allowed to interact with the gold particles to form a stable gold solution at high ionic strength. The solution was centrifuged three times at 45,000 g and the fluffy pellet was resuspended each time in buffer B (5 mM carbonate buffer, pH 9.7) to remove the excess of unbound antibodies. Finally, the solution was centrifuged under the same conditions but the pellet was resuspended in buffer B supplemented with 0.01% Tween 20.
The immunogold labelings were performed by mixing 1 µl of fraction B2000, 4 µl of buffer A, and 1 µl of the gold-coupled antibody solution diluted to reach a normalized density of gold particles. The incubations were left for 2 h at room temperature then diluted with 38 µl of buffer A. 5 µl of each solution was deposited on a glow-discharged carbon-coated grid, washed with buffer C (10 mM Tris, pH 7.5, 0.01% Tween 20), and negatively stained with a 2% uranyl acetate solution. Micrographs were recorded on Kodak SO163 films at a magnification of 45,000 with a Phillips CM120 transmission electron microscope operating at 100 kV.
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Results |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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A Macromolecular Complex Containing pol I, pol I–dependent Transcription Factors, and Other Nucleolar Proteins
We have described previously the simple derivation of an efficient promoter-dependent pol I–specific in vitro transcription system starting from yeast WCEs (
Indeed, when the distribution of the two exclusively nucleolar proteins, Nop1p and Fpr3p (
To ensure that the whole array of nucleolar factors was not adventitiously associated as a result of nonspecific aggregation in low ionic strength buffers, we monitored the chromatographic behavior of the pol I transcription factors and nucleolar proteins in cell extracts. WCEs were generated under conditions very similar to the ionic strength of the living cell. Proteins of a 100,000-g supernatant of such yeast WCEs were fractionated by size on a Superose-6 column in the presence of 300 mM potassium acetate, and the migration of pol I and other nucleolar factors was monitored. Yeast fibrillarin Nop1p and pol I eluted with an apparent molecular mass of >10 MD from the column (Fig 1 C). Many other nucleolar proteins, such as Fpr3p and Rrp5p (
Physical interaction between pol I and other nucleolar proteins in WCEs was verified by coimmunoprecipitation assays. When whole yeast cell extracts from strains containing a HA-tagged A43 subunit were immunoprecipitated with antibodies directed against the HA epitope, nucleolar proteins like Nop1p and Fpr3p as well as the transcription factors TBP and Reb1p coprecipitated together with pol I (Fig 1 D, lanes 3 and 5). No significant coprecipitation of the nucleolar factors was observed in control experiments with yeast strains lacking an epitope-tagged pol I subunit (Fig 1 D, lane 4; see also Materials and Methods). To rule out that oligomeric nucleic acids might mediate the observed association between pol I and other nucleolar proteins, the immunoprecipitation experiment was repeated with WCEs from which nucleic acids had been removed by treatment with nucleases; the nucleolar proteins still coprecipitated with pol I (Fig 1 D, lane 5).
Affinity chromatography of His6-tagged pol I on Ni-agarose was used to show that the coelution of pol I, initiation factors, and nucleolar factors (Fig 1 E, upper panel) was sufficient to evoke an initiation active complex (Fig 1 E, lower panel). In contrast, high amounts of highly purified pol I-A were not able to initiate transcription.
The coprecipitation and coelution of pol I and all tested nucleolar factors supported the idea that these factors interact in solution, and consequently, might be able to form a large macromolecular assembly.
Analysis of the Resolubilized Complex and Identification of Components by Mass Spectrometry
After precipitation with low ionic strength, the nucleolar proteins could be resolubilized in buffers with moderate salt concentrations (i.e., 600 mM potassium acetate). Gel filtration experiments confirmed that even under these elevated ionic strength conditions, a proportion of a large pol I–containing complex remains associated. To determine the size of the putative assembly, the resolubilized fraction PA600, which contained the putative nucleolar assembly, was clarified and applied to a Superose-6 column. As published previously, most of the pol I eluted from the column in fractions corresponding to a molecular mass between 600–1,500 kD (
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The putative nucleolar assembly present in fraction PA600 could be divided into two fractions, designated B600 and B2000 (Fig 1 A), by chromatography on a BioRex 70 column (
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To identify more proteins of the putative nucleolar assembly, polypeptides in fraction B2000 were then analyzed by mass spectrometry. After a further purification step by gel filtration on Sephacryl S-300 (
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Functional Properties of the Isolated Nucleolar Assembly
Functional analysis of fraction PA600, which contains the putative nucleolar assembly, supported the proposal that we have precipitated a cooperative macromolecular complex of the nucleolus. When the precipitated proteins were redissolved in buffers containing 600 mM potassium acetate, they demonstrated efficient activity in accurate inititation of transcription (Fig 4 A, lane 3) (
Since the transcription termination factor Reb1p also coprecipitated with pol I, the initiation factors, and the other nucleolar proteins (Fig 1 B), we proceeded to assay the putative protein assembly in fraction PA600 for a coordinated transcription termination activity. Indeed, fraction PA600 was also capable of terminating a correctly initiated transcript. In vitro transcription of a circular plasmid containing the pol I promoter and the native termination site resulted in a transcript of the expected size (Fig 4 A, lane 6), whereas no defined transcripts could be detected when transcription was performed with circular plasmids that lacked the termination sequence (Fig 4 A, lane 1). This result provides further evidence that the isolated nucleolar protein assembly contains different distinct functional properties, such as transcription initiation and termination, and that these functions might be linked in a cooperative fashion.
Cbf5p and Nhp2p, two other proteins detected in the isolated nucleolar assembly, were recently reported to be involved in pseudouridylation of rRNA (
Methylation is another common modification of mature rRNA. Fraction PA600, which contained the putative nucleolar assembly, was also able to methylate RNA since transcription in the presence of 14C-labeled S-adenosyl methionine showed the incorporation of 14CH3 in synthesized transcripts (Tschochner, H., unpublished observation).
Taken together, these results suggest that assembly of the different factors within the isolated nucleolar assembly might result in a cooperative enzymatic network that guides both synthesis and maturation of rRNA.
The Isolated Nucleolar Complex Contains snoRNAs
RNA coprecipitated with the nucleolar proteins within the macromolecular assembly. Since several snoRNA-associated proteins that are involved in rRNA processing, like Nop1p, Rrp5p, Nhp2p, and Cbf5p, could be detected in the isolated nucleolar complex, we wondered whether the isolated RNA contained snoRNAs. Indeed, Northern blot analysis revealed the presence of all the tested snoRNAs in the precipitated nucleolar assembly. Among the snoRNAs analyzed were MRP, the Box C and D snoRNAs U3 and U14 (Fig 5), and the box H and ACA snoRNA snR30 (data not shown). Furthermore, substantial amounts of mature 18S rRNA (Fig 5) were also detected. In contrast, RNAs synthesized by pols II and III, like the mRNAs for actin and the translation factor translation elongation factor eEF1 alpha-A chain, and the tRNAs for glutamic acid and leucine, were absent in the isolated nucleolar complex (Fig 5). The amount of precipitated snoRNAs varied between 8% for MRP and 33% for U14, which corresponded to a 4- and 14-fold enrichment, respectively, if the quantities of snoRNAs were related to the amount of proteins present in the corresponding fractions. In contrast, no tRNAs were specifically enriched; <2% of them were precipitated. Taken together, these results provide additional evidence that the purification procedure described herein is highly specific for components organized in the nucleolus, and suggest that RNAs involved in the biogenesis of ribosomes are also present in the isolated nucleolar RNP assembly.
Pol I and Ongoing RNA Synthesis Is Not Essential for the Nucleolar Assembly; However, pol I Can Be Recruited to the Complex
The various structural components and functional properties of this nucleolar RNP assembly suggested the existence of an active multienzyme complex, in which synthesis and processing of rRNA might take place in a cooperative fashion. To investigate whether the isolated assembly was solely held together by a cooperative transcription-processing event, the structural integrity of the assembly was investigated in conditions in which pol I–dependent transcription has stopped. Thus, cell extracts were prepared from stationary cells in which rRNA synthesis was known to be completely downregulated (135), which is lacking the second largest pol I subunit, and thus, is deficient in pol I–dependent transcription. In this strain, the essential rRNAs were synthesized by pol II transcribing one rDNA unit under the control of a pol II–dependent promoter (135 strain). Similar amounts of proteins and RNA coprecipitated in each of the three preparations to result in fraction PA600g, PA600s, and 135, respectively (data not shown). Western blot analysis confirmed that both pol I–specific transcription factors, such as TBP or Rrn10p (a component of UAF) and termination factor Reb1p, and other nucleolar factors, like Nop1p and Fpr3p, were still associated together. In contrast to wild-type cells, pol I–dependent rRNA synthesis was completely abolished in the complex(es) isolated from stationary cells and the mutant strain (Fig 6 A). In the mutant strain, neither the two largest pol I subunits nor the pol I–associated transcription factor Rrn3p could be detected in the nucleolar complex (Fig 6 A, lane 2). Depletion of the pol I subunit A135 resulted both in a complete disruption of pol I and in the dissociation of most of the pol I subunits from the nucleolar complex, although other transcription initiation factors still assembled within the nucleolar substructure. It is important to note that fraction PA600 135 was neither enriched in pol II nor did it display pol II–dependent transcription activity (data not shown). This result indicates that although the rRNA was synthesized by pol II, in this mutant strain, the rDNA transcribing pol II machinery was not integrated into the nucleolar assembly, and therefore, underlines the specificity of our purification procedure.
In stationary cells, all tested transcription and nucleolar factors, with the exception of Rrn3p, which was demonstrated to be essential for pol I to initiate transcription (
We further investigated whether the pol I–deficient nucleolar assembly was still able to recruit purified pol I and to restore the transcriptional activity. Highly purified pol I preparations like pol I-A and pol I-p, which contained both pol I–Rrn3p complex and free pol I, did not precipitate when dialyzed against buffers with low ionic strength (see Fig 6 C). In contrast, coprecipitation of pol I was observed when dialysis was performed in the presence of the nucleolar complex(es) that had been derived from the mutant 135 strain, which completely lacked pol I (Fig 6B and Fig C). After resolubilization of the coprecipitated pol I and the nucleolar assembly, >85% of the applied nonspecific pol I activity in RNA synthesis was found in the pellet (Fig 6 C). Even more striking, after coprecipitation, the pol I–Rrn3p complex regained its ability to cooperate with the remaining transcription initiation factors to restore an active initiation complex (Fig 6 B, lanes 1–3), whereas in control reactions, neither precipitated mutant PA600 (Fig 6 B, lanes 7–9) nor purified pol I (Fig 6 B, lanes 4–6) showed any transcriptional activity. The purified pol I–Rrn3p complex used for this experiment lacked both the 240-kD TBP-containing complex and the necessary activity in fraction B600, and was therefore incapable of initiating transcription by itself (data not shown; see also
This result indicates that the isolated nucleolar substructure provides a scaffold for the assembly of a variety of nucleolar factors involved in rRNA synthesis and processing, independent of whether pol I–dependent RNA synthesis is turned on or off.
Based on this finding, we developed an in vitro assay to test various fractions for their ability to coprecipitate pol I. Further fractionation of PA600 135, which contained the putative nucleolar assembly on BioRex70, revealed that the pol I–recruiting activity could be separated from the majority of proteins. Fraction B2000 135 of the BioRex column, which contained ~18% of the applied proteins, was able to coprecipitate pol I, whereas the same amount (or a threefold excess [data not shown]) of fraction B600 (135) could not significantly affect the solubility of pol I in low salt buffers (Fig 6 C). We take this as evidence for a feasible enrichment of a structural module that is capable of interacting with pol I and might serve as the structural backbone to associate with other nucleolar proteins, and thus, might be involved in building up the entire isolated nucleolar subcomplex.
Electron Microscopic Analysis of the Nucleolar Assembly
The biochemical evidence of large pol I–containing complexes present in fractions PA600 and B2000 prompted us to investigate the assemblies by EM. When the wild-type PA600 fraction was prepared in the presence of a buffer containing >600 mM KOAc, a homogeneous distribution of particles was observed (data not shown). The dilution of this fraction in the same buffer containing 90 mM KOAc resulted in the formation of loose supramolecular structures 0.1–0.3 µm in size (Fig 7A and Fig B). These assemblies, hereafter identified as clusters, consisted of a barely visible protein network associated with a large number of globular particles 10–15 nm in size located within or at the periphery of these structures.
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The fraction PA600 135, which contained the presumably nucleolar assembly from the pol I–disrupted strain, also formed supramolecular assemblies in low ionic strength buffers. These structures were, however, different from those formed from the wild-type strain, since the size of the particles was significantly smaller (
7.5 nm) and since the particles seemed to be more closely packed (Fig 7C and Fig D). These data suggest that an underlying complex can form in the absence of pol I, and that pol I can be recruited to this complex by specific protein–protein interactions according to our biochemical data.
Due to the lower background of possible contaminations and the less complex protein composition, we decided to further investigate the pol I–containing assemblies in fraction B2000. This fraction has the same coprecipitation properties as the wild-type fraction PA600, is capable of recruiting pol I (see above), and similar clusters were observed upon lowering the ionic strength. In the presence of >600 mM KOAc, a homogeneous distribution of particles was observed. Digital analysis of EM images of these particles identified these structures as pol I molecules similar in size and shape to the previously analyzed highly purified pol I complexes (
When the ionic strength of the buffer was lowered to 90 mM KOAc, the distribution of the pol I molecules was drastically altered and the vast majority of the molecules was recruited into the clusters. A preliminary image analysis of the particles associated with the clusters showed the characteristic size and shape of pol I molecules. Altogether, these observations indicate that the pol I molecules are assembled into large supramolecular assemblies.
To demonstrate that the nucleolar proteins Nop1p and Fpr3p are also included in the clusters, we analyzed the large pol I–containing complexes by immunogold labeling. Gold-coupled antibodies directed against the nucleolar proteins Nop1p and Fpr3p were incubated with fraction B2000 before cluster formation. The amount of labeled structures was determined for each specific probe and compared with a negative control formed by a gold-coupled nonspecific antibody. The density of the probes was carefully normalized by direct counting of gold particles adsorbed on a carbon film in order to have the same amount of gold particles in the incubation solution. In these conditions, the nonspecific antibody labeled ~11% of the clusters, whereas the probes directed against the nucleolar proteins Fpr3p and Nop1p labeled 62 and 57% of the clusters, respectively (Fig 7G and Fig H). This significant difference was obtained in duplicate and indicated that the nucleolar proteins Fpr3p and Nop1p are part of the large assemblies.
These EM observations clearly show that a large macromolecular assembly, containing Fpr3p and Nop1p, is able to recruit several pol I molecules into a modular structure. The number of polymerases included in these structures depends on the size of the assemblies, precluding the possibility of a stoichiometric complex. These pol I–containing structures differ from protein aggregates by the fact that their thickness is globally monomolecular, and that in some cases, an underlying protein network can be distinguished between the pol I molecules and by the sequential assembly of the structure.
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Discussion |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
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From our results, we suggest the existence of a nucleolar RNP scaffold capable of forming an interface for the association of pol I and components involved in rDNA transcription and rRNA processing in vitro. Furthermore, this assembly is independent of rRNA synthesis. The assembly of these nucleolar factors when derived from growing cells results both in active in vitro transcription initiation and termination complexes, and in the ability to modify rRNA.
Specific Purification of the RNP Complex
The simple derivation and striking enrichment of one or several highly organized nucleolar multienzyme complexes, which comprise a whole variety of in vitro activities, underlines the specificity of the purification procedure, although the nature of the coprecipitation of the nucleolar factors remained obscure. Precipitation was not due to aggregation of chromatin in low salt buffers, a well-known practical problem during purification of nuclear scaffolds and matrices under physiological conditions (for review see
Nucleolar structures seem to be very sensitive to changes in the surrounding salt conditions. For example,
Components of the Nucleolar Assembly
Treatment of the complex with ethidium bromide, RNase, or DNase did not dissociate the assembled components, although incubation with RNase resulted in a significant loss of RNA (data not shown). Neither the genetic disruption of an essential pol I subunit (Fig 6) nor incubation of the soluble complex with an excess of antibodies directed against Nop1p or against the pol I core enzyme was able to affect the formation of the nucleolar complex (data not shown). On the other hand, further fractionation of fraction PA600 derived from the pol I–lacking mutant on BioRex70 (Fig 6 C) or on MonoS (data not shown) revealed fractions that preferentially coprecipitated soluble, purified pol I. We take these findings as evidence that neither RNA, DNA, nor pol I are required to keep the nucleolar substructure assembled. The proteinaceous factors holding the substructure together remain to be determined.
The identification of a variety of other proteins, in addition to pol I, in the isolated proteinaceous fraction confirms the existence of a macromolecular assembly of nucleolar components. All of the proteins identified so far could be localized to the nucleolus. Furthermore, some of the determined proteins, like Nop1p, Rrp5p, Nhp2p, and Cbf5p, have already been described to be components of higher organized complexes involved in rRNA processing (see Introduction) or in the assembly of mature ribosomes. For example, Rrp5p was shown to be required for formation of both 18S and 5.8S rRNA and the downregulation of yeast immunophilin Fpr3p, which is exclusively distributed to the nucleolus (
In contrast to the well-characterized pol II holoenzyme, the components identified in the described macromolecular network do not form a stoichiometric complex. It seems more likely that a variable amount of different functional and structural subcomplexes can be gathered in this subnucleolar structure. For instance, several populations of pol I (initiation-competent as well as elongation-active pol I, pol I monomers, and dimers) could be identified in the assembly (
The nonstoichiometric distribution of the components as well as the structural data of the isolated complex based on EM favors the idea that proper nucleolar function might depend on the coalescence of supramolecular assemblies through structural interactions.
Interaction of rDNA-transcription and rRNA-processing Components
Our results provide the first biochemical evidence for a direct linkage between transcription and processing machineries and support previous suggestions (
Another important observation suggesting that processing might occur as the rRNA is synthesized was reported recently.
Finally, a genetic link between a member of the transcription apparatus and one of the processing machinery has also been reported. Overexpression of transcription initiation factor Rrn3p was shown to suppress a mutation in CBF5, a gene required for pseudouridylation of rRNA (
Formation of the Nucleolus
Despite the increasing evidence describing the presence of functional domains in the nucleolus, relatively little is known about the forces that keep these supramolecular assemblies together. It is possible that the RNP assembly described herein represents a structural and operative subunit of the nucleolus. Many of these subunits might join through functional or structural interactions, such as active rRNA synthesis, attachment to the nuclear scaffold (
On the one hand, it has been suggested that nucleolar formation is driven by the procedure of building a ribosome, which implies that a coherent network of the particular synthesis, assembly, and processing reactions finally result in the appearance of a whole organelle. A regularly shaped nucleolus seems to be the consequence of active pol I–dependent gene transcription. For instance, inhibition of pol I–dependent transcription by actinomycin D blocked the formation of the nucleolus (
In contrast, formation of a regular nucleolar structure was observed in pol I–inactive cells during early Xenopus development, which indicated that the organization of a defined nucleolar structure can be independent of the transcription process, but dependent on the presence of unprocessed rRNA (
It is conceivable that different functional domains of the nucleolus are arranged in a supramolecular assembly that provides the structural module of the nucleolus no matter whether transcription is off or on. For instance, pol I could be immobilized in the nucleolus through interaction with the constitutive proteins of the nucleolus. Such an organization might result in the appearance of a regularly shaped nucleolus and suggest that the transcription apparatus might pull through the DNA template rather than moving along the rDNA. Congruent with this idea is the observation that the pol I–dependent transcription machinery is associated to the nuclear scaffold independent of the presence of rDNA (
Consistent with the idea of a superior organization made of single functional and structural subunits is the observation that inhibition of pol I–dependent rRNA synthesis by treatment with actinomycin D causes a redistribution of rDNA genes into clusters at the periphery of the regular nucleolus, whereas the major components of the rRNA transcription machinery including pol I and TBP still colocalize within these transcriptional inactive clusters (
