Your search keyword '"Cell Nucleolus chemistry"' showing total 477 results

101. Small subunits of RNA polymerase: localization, levels and implications for core enzyme composition.

Author

Doherty GP, Fogg MJ, Wilkinson AJ, and Lewis PJ

Subjects

Amino Acid Sequence, Bacillus subtilis chemistry, Bacillus subtilis genetics, Cell Nucleolus chemistry, Cell Nucleolus enzymology, Cell Nucleolus genetics, DNA-Directed RNA Polymerases chemistry, DNA-Directed RNA Polymerases genetics, Gene Expression Regulation, Enzymologic, Molecular Sequence Data, Multiprotein Complexes chemistry, Multiprotein Complexes genetics, Protein Multimerization, Protein Subunits chemistry, Protein Subunits genetics, Protein Transport, Bacillus subtilis enzymology, DNA-Directed RNA Polymerases metabolism, Multiprotein Complexes metabolism, Protein Subunits metabolism

Abstract

Bacterial RNA polymerases (RNAPs) contain several small auxiliary subunits known to co-purify with the core α, β and β' subunits. The ω subunit is conserved between Gram-positive and Gram-negative bacteria, while the δ subunit is conserved within, but restricted to, Gram-positive bacteria. Although various functions have been assigned to these subunits via in vitro assays, very little is known about their in vivo roles. In this work we constructed a pair of vectors to investigate the subcellular localization of the δ and ω subunits in Bacillus subtilis with respect to the core RNAP. We found these subunits to be closely associated with RNAP involved in transcribing both mRNA and rRNA operons. Quantification of these subunits revealed δ to be present at equimolar levels with RNAP and ω to be present at around half the level of core RNAP. For comparison, the localization and quantification of RNAP β' and ω subunits in Escherichia coli was also investigated. Similar to B. subtilis, β' and ω closely associated with the nucleoid and formed subnucleoid regions of high green fluorescent protein intensity, but, unlike ω in B. subtilis, ω levels in E. coli were close to parity with those of β'. These results indicate that δ is likely to be an integral RNAP subunit in Gram-positives, whereas ω levels differ substantially between Gram-positives and -negatives. The ω subunit may be required for RNAP assembly and subsequently be turned over at different rates or it may play roles in Gram-negative bacteria that are performed by other factors in Gram-positives.

Published

2010

102. Nucleolar proteomics and viral infection.

Author

Hiscox JA, Whitehouse A, and Matthews DA

Subjects

Animals, Cell Nucleolus metabolism, DNA Virus Infections metabolism, HeLa Cells, Humans, RNA Virus Infections metabolism, Cell Nucleolus chemistry, Proteomics, Virus Diseases metabolism

Abstract

Recent advances in proteomics have been combined with traditional methods for isolation of nucleoli from mammalian and plant cells. This approach has confirmed the growing body of data showing a wide role for the nucleolus in eukaryotic cell biology beyond ribosome generation into many areas of cell function from regulation of the cell cycle, modulation of the cell stress response to innate immune responses. This has been reflected in the growing body of evidence that viruses specifically target the nucleolus by sequestering cellular nucleolar proteins or by targeting viral proteins to the nucleolus in order to maximise viral replication. This review covers those key areas and looks at the latest approaches using high-throughput quantitative proteomics of the nucleolus in virus infected cells to gain an insight into the role of this fascinating compartment in viral infection., (Copyright © 2010 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2010

103. Characterization and prediction of protein nucleolar localization sequences.

Author

Scott MS, Boisvert FM, McDowall MD, Lamond AI, and Barton GJ

Subjects

Cell Line, Tumor, Computational Biology methods, Humans, Nuclear Localization Signals, Nuclear Proteins analysis, Viral Proteins analysis, Viral Proteins chemistry, Cell Nucleolus chemistry, Neural Networks, Computer, Nuclear Proteins chemistry, Protein Sorting Signals

Abstract

Although the nucleolar localization of proteins is often believed to be mediated primarily by non-specific retention to core nucleolar components, many examples of short nucleolar targeting sequences have been reported in recent years. In this article, 46 human nucleolar localization sequences (NoLSs) were collated from the literature and subjected to statistical analysis. Of the residues in these NoLSs 48% are basic, whereas 99% of the residues are predicted to be solvent-accessible with 42% in α-helix and 57% in coil. The sequence and predicted protein secondary structure of the 46 NoLSs were used to train an artificial neural network to identify NoLSs. At a true positive rate of 54%, the predictor's overall false positive rate (FPR) is estimated to be 1.52%, which can be broken down to FPRs of 0.26% for randomly chosen cytoplasmic sequences, 0.80% for randomly chosen nucleoplasmic sequences and 12% for nuclear localization signals. The predictor was used to predict NoLSs in the complete human proteome and 10 of the highest scoring previously unknown NoLSs were experimentally confirmed. NoLSs are a prevalent type of targeting motif that is distinct from nuclear localization signals and that can be computationally predicted.

Published

2010

104. Requirement of phosphatase of regenerating liver-3 for the nucleolar localization of nucleolin during the progression of colorectal carcinoma.

Author

Semba S, Mizuuchi E, and Yokozaki H

Subjects

Adult, Aged, Cell Line, Tumor, Cell Proliferation, Disease Progression, Female, Humans, Male, Middle Aged, Phosphorylation, Nucleolin, Cell Nucleolus chemistry, Colorectal Neoplasms pathology, Neoplasm Proteins physiology, Phosphoproteins analysis, Protein Tyrosine Phosphatases physiology, RNA-Binding Proteins analysis

Abstract

Phosphatase of regenerating liver-3 (PRL-3) is a protein tyrosine phosphatase (PTP) that is frequently overexpressed in liver metastases of colorectal carcinomas (CRCs). The PTP activity of the PRL-3 protein is indispensable for the promotion of distant metastasis of CRC; however, little is known about the effect of PRL-3 on cell growth. In this study, we investigated a novel protein that can connect to PRL-3 to modulate the proliferation of CRC cells. In CRC-derived SW480 cells, transduction of ectopic wild-type PRL-3, but not the C104S catalytic "dead" mutant, up-regulated cell proliferation and increased the population of cells at the S and G(2) /M phases. Also, inhibition of PTP activity of the PRL-3 protein by treatment with the PRL-3 inhibitor suppressed cell proliferation in a dose-dependent manner as well as PRL-3 knockdown by RNA interference. Using a comparative study of monodimensional gel electrophoresis of immunoprecipitates from PRL-3-transfected SW480 cells and subsequent mass spectrometry analysis, nucleolar-specific protein nucleolin (NCL) was identified as a novel PRL-3-binding protein. We confirmed physiological interaction between PRL-3 and NCL, and found that PRL-3 phosphatase activity was associated with the suppression of the phospho-NCL levels and nucleolar assembly of NCL protein. In CRC cases, nucleolar NCL expression was correlated not only with higher levels of PRL-3 expression but also with frequent incidence of lymph node metastasis and a higher clinicopathologic stage. These findings suggest that NCL is involved in PRL-3-mediated cancer progression/metastasis signaling, which plays an important role in the acceleration of CRC growth., (© 2010 Japanese Cancer Association.)

Published

2010

105. Human cellular protein nucleoporin hNup98 interacts with influenza A virus NS2/nuclear export protein and overexpression of its GLFG repeat domain can inhibit virus propagation.

Author

Chen J, Huang S, and Chen Z

Subjects

Animals, Cell Line, Cell Nucleolus chemistry, Cell Nucleus chemistry, Dogs, Humans, Influenza A Virus, H5N1 Subtype growth & development, Microscopy, Confocal, Two-Hybrid System Techniques, Viral Nonstructural Proteins genetics, Host-Pathogen Interactions, Influenza A Virus, H5N1 Subtype physiology, Nuclear Export Signals, Nuclear Pore Complex Proteins metabolism, Protein Interaction Mapping, Viral Nonstructural Proteins metabolism, Virus Replication

Abstract

The non-structural protein NS2, also called nuclear export protein, of influenza A virus contains a leucine-rich nuclear-export signal that could guide viral ribonucleoproteins to cross the nuclear pore complex (NPC) and complete directional nucleocytoplasmic trafficking. In this study, human nucleoporin 98 (hNup98), an NPC protein, was identified as an NS2-binding protein by using yeast two-hybrid screening of a human cDNA library. Interaction between NS2 and hNup98 was confirmed in yeast and mammalian cells. Mapping tests further demonstrated that aa 22-53 in the N-terminal region of NS2 and the glycine-leucine-phenylalanine-glycine (GLFG) repeat domain (aa 1-511) of hNup98 are crucial for the interaction of these two proteins. Confocal microscopy showed that hNup98 could specifically recruit NS2 to the nucleoli and that this process was inhibited by leptomycin B, a specific inhibitor of human chromosomal region maintenance 1 protein. NS2 recruitment to the nucleoli was through the N-terminal GLFG repeat domain of hNup98, but not through the C-terminal domain. Moreover, influenza virus infection downregulated Nup98 levels significantly in 293T and Madin-Darby canine kidney cells. Overexpression of the GLFG repeat domain of hNup98 apparently inhibited virus propagation. Together, these findings reveal the interaction between hNup98 and NS2. The GLFG repeat domain of hNup98 might competitively inhibit the interaction between NS2 and endogenous hNup98, consequently inhibiting virus propagation.

Published

2010

106. NOF1 encodes an Arabidopsis protein involved in the control of rRNA expression.

Author

Harscoët E, Dubreucq B, Palauqui JC, and Lepiniec L

Subjects

Amino Acid Sequence, Arabidopsis chemistry, Arabidopsis genetics, Arabidopsis Proteins chemistry, Cell Nucleolus chemistry, Cell Nucleolus genetics, Cell Nucleolus metabolism, Molecular Sequence Data, Nuclear Proteins chemistry, Protein Transport, RNA, Plant genetics, RNA, Plant metabolism, RNA, Ribosomal metabolism, Sequence Alignment, Arabidopsis metabolism, Arabidopsis Proteins genetics, Arabidopsis Proteins metabolism, Gene Expression Regulation, Plant, Nuclear Proteins genetics, Nuclear Proteins metabolism, RNA, Ribosomal genetics

Abstract

The control of ribosomal RNA biogenesis is essential for the regulation of protein synthesis in eukaryotic cells. Here, we report the characterization of NOF1 that encodes a putative nucleolar protein involved in the control of rRNA expression in Arabidopsis. The gene has been isolated by T-DNA tagging and its function verified by the characterization of a second allele and genetic complementation of the mutants. The nof1 mutants are affected in female gametogenesis and embryo development. This result is consistent with the detection of NOF1 mRNA in all tissues throughout plant life's cycle, and preferentially in differentiating cells. Interestingly, the closely related proteins from zebra fish and yeast are also necessary for cell division and differentiation. We showed that the nof1-1 mutant displays higher rRNA expression and hypomethylation of rRNA promoter. Taken together, the results presented here demonstrated that NOF1 is an Arabidopsis gene involved in the control of rRNA expression, and suggested that it encodes a putative nucleolar protein, the function of which may be conserved in eukaryotes.

Published

2010

107. Quantitative proteomics using stable isotope labeling with amino acids in cell culture reveals changes in the cytoplasmic, nuclear, and nucleolar proteomes in Vero cells infected with the coronavirus infectious bronchitis virus.

Author

Emmott E, Rodgers MA, Macdonald A, McCrory S, Ajuh P, and Hiscox JA

Subjects

Amino Acid Sequence, Animals, Chlorocebus aethiops, Chromatography, Liquid, Electrophoresis, Polyacrylamide Gel, Microscopy, Confocal, Molecular Sequence Data, Tandem Mass Spectrometry methods, Vero Cells, Cell Nucleolus chemistry, Cell Nucleus chemistry, Cytoplasm chemistry, Infectious bronchitis virus pathogenicity, Isotope Labeling methods, Proteomics, Viral Proteins chemistry

Abstract

Virus-host interactions involve complex interplay between viral and host factors, rendering them an ideal target for proteomic analysis. Here we detail a high throughput quantitative proteomics analysis of Vero cells infected with the coronavirus infectious bronchitis virus (IBV), a positive strand RNA virus that replicates in the cytoplasm. Stable isotope labeling with amino acids in cell culture (SILAC) was used in conjunction with LC-MS/MS to identify and quantify 1830 cellular and two viral proteins from IBV-infected cells. Fractionation of cells into cytoplasmic, nuclear, and nucleolar extracts was used to reduce sample complexity and provide information on the trafficking of proteins between the different compartments. Each fraction showed a proportion of proteins exhibiting >or=2-fold changes in abundance. Ingenuity Pathway Analysis revealed that proteins that changed in response to infection could be grouped into different functional categories. These included proteins regulated by NF-kappaB- and AP-1-dependent pathways and proteins involved in the cytoskeleton and molecular motors. A luciferase-based reporter gene assay was used to validate the up-regulation of AP-1- and NF-kappaB-dependent transcription in IBV-infected cells and confirmed using immunofluorescence. Immunofluorescence was used to validate changes in the subcellular localization of vimentin and myosin VI in IBV-infected cells. The proteomics analysis also confirmed the presence of the viral nucleocapsid protein as localizing in the cytoplasm, nucleus, and nucleolus and the viral membrane protein in the cytoplasmic fraction. This research is the first application of SILAC to study total host cell proteome changes in response to positive sense RNA virus infection and illustrates the versatility of this technique as applied to infectious disease research.

Published

2010

108. Efficient extraction of nucleolar proteins for interactome analyses.

Author

Chamousset D, Mamane S, Boisvert FM, and Trinkle-Mulcahy L

Subjects

Carbon Isotopes, HeLa Cells, Humans, Isotope Labeling, Nuclear Proteins isolation & purification, Nuclear Proteins metabolism, Peptide Fragments metabolism, Phosphoprotein Phosphatases chemistry, Phosphoprotein Phosphatases metabolism, Signal Transduction, Trypsin metabolism, Cell Nucleolus chemistry, Nuclear Proteins chemistry, Peptide Fragments chemistry, Proteomics methods

Abstract

The efficient extraction of proteins from purified cellular organelles is critical for in vitro analyses, including identification of protein complex members by affinity purification-based quantitative proteomic approaches. When applied to purified nucleoli, classic nuclear protein extraction methods inefficiently and selectively release only approximately 50% of proteins. Here, we present a method that can extract up to 90% of nucleolar proteins, and apply it in a quantitative interactomic approach to identify nucleolar interaction partners for a mammalian protein phosphatase.

Published

2010

109. Nucleolar changes and fibrillarin redistribution following apatone treatment of human bladder carcinoma cells.

Author

Jamison JM, Gilloteaux J, Perlaky L, Thiry M, Smetana K, Neal D, McGuire K, and Summers JL

Subjects

Carcinoma chemistry, Cell Line, Tumor, Cell Nucleolus chemistry, Cell Nucleolus drug effects, Humans, Urinary Bladder Neoplasms chemistry, Vitamin K pharmacology, Antineoplastic Combined Chemotherapy Protocols pharmacology, Ascorbic Acid pharmacology, Carcinoma ultrastructure, Cell Nucleolus ultrastructure, Chromosomal Proteins, Non-Histone analysis, Urinary Bladder Neoplasms ultrastructure, Vitamin K 3 pharmacology

Abstract

Ascorbate and menadione (Apatone) in a ratio of 100:1 kills tumor cells by autoschizis. In this study, vitamin-induced changes in nucleolar structure were evaluated as markers of autoschizis. Human bladder carcinoma (T24) cells were overlain with vitamins or with culture medium. Supernatants were removed at 1-hr intervals from 1 to 4 hr, and the cells were washed with PBS and prepared for assay. Apatone produced marked alterations in nucleolar structure including redistribution of nucleolar components, formation of ring-shaped nucleoli, condensation and increase of the proportion of perinucleolar chromatin, and the enlargement of nucleolar fibrillar centers. Immunogold labeling of the nucleolar rRNA revealed a granular localization in treated and sham-treated cells, and immunogold labeling of the rDNA revealed a shift from the fibrillar centers to the condensed perinucleolar chromatin. Fibrillarin staining shifted from the fibrillar centers and adjacent regions to a more homogeneous staining of the entire nucleolus and was consistent with the percentage of autoschizic cells detected by flow cytometry. Because autoschizis entails sequential reactivation of DNase I and DNase II, and because the fibrillarin redistribution following DNase I and Apatone treatment is identical, it appears that the nucleolar and fibrillarin changes are markers of autoschizis.

Published

2010

110. State of oncomarker protein B23/nucleophosmin in HeLa cells.

Author

Vladimirova NM, Lobanova NV, and Potapenko NA

Subjects

Amino Acid Sequence, Cell Nucleolus chemistry, Cell Nucleolus metabolism, HeLa Cells, Humans, Molecular Sequence Data, Molecular Weight, Nuclear Proteins isolation & purification, Nuclear Proteins metabolism, Nucleophosmin, Protein Isoforms chemistry, Protein Isoforms isolation & purification, Protein Isoforms metabolism, Protein Multimerization, Nuclear Proteins chemistry

Abstract

Western blot after SDS-PAGE for protein separation showed two immunoreactive bands corresponding to monomers (38-40 kDa) and oligomers (210-230 kDa) of nucleophosmin in HeLa cell lysates. Decreasing the buffer ionic strength during the incubation of cells and nuclei destabilized these oligomers. We also showed the existence of two B23/nucleophosmin pools in nuclei of HeLa cells with different sensitivity to hypotonic buffer treatment: one extractable from the nucleus and the other non-extractable and tightly bound to the nucleus. A detailed structural analysis of the extractable B23 pool was carried out: two closely related nucleophosmin isoforms (B23.1 and B23.2) were identified as a result of analysis of C-terminal amino acid sequences using carboxypeptidase hydrolysis; the N-termini of both isoforms are blocked by an acetyl group. As a result of sequencing of the deacetylated proteins, it has been established that the N-terminal amino acid sequence of nucleophosmin in these preparations is truncated by nine amino acid residues and the acetylated residue is Ser. The truncated monomer of nucleophosmin (represented only by the extractable part of the protein) on addition of magnesium ions to low ionic strength buffer or increase in buffer ionic strength was shown to form oligomers with molecular weights (210-230 kDa) similar to those revealed in the total cell lysate. It should be noted that the set of oligomers in this case differs from the one in total cell lysate. Our strategy of characterization of B23 forms for HeLa cells can be applied for other tumor cells.

Published

2010

111. Isolation of nucleoli.

Author

Hacot S, Coute Y, Belin S, Albaret MA, Mertani HC, Sanchez JC, Rosa-Calatrava M, and Diaz JJ

Subjects

Animals, Humans, Cell Culture Techniques methods, Cell Fractionation methods, Cell Nucleolus chemistry, Electrophoresis, Polyacrylamide Gel methods

Abstract

Nucleoli are now recognized as multi-functional nuclear domains involved in several fundamental cell processes such as ribosome biogenesis, regulation of the assembly of non-ribosomal ribonucleoprotein complexes, tRNA maturation, sequestration of protein, viral infection, and cellular ageing. Extensive proteomic analyses of these nucleolar domains after their purification have contributed to the description of their multiple biological functions. Because nucleoli are the largest and densest nuclear structures, they are easily amenable to purification from nuclei of cultured animal cells using the protocol described in this unit.

Published

2010

112. A triphenylphosphonium-functionalised cyclometalated platinum(II) complex as a nucleolus-specific two-photon molecular dye.

Author

Koo CK, So LK, Wong KL, Ho YM, Lam YW, Lam MH, Cheah KW, Cheng CC, and Kwok WM

Subjects

Animals, Binding Sites, Cell Line, Tumor chemistry, Cell Line, Tumor metabolism, HeLa Cells metabolism, Humans, Ligands, Luminescence, Mice, Microscopy, Confocal methods, Models, Molecular, Molecular Structure, Nuclear Proteins metabolism, Organelles chemistry, Organelles metabolism, Organoplatinum Compounds toxicity, Photons, Platinum, Solutions chemistry, Temperature, Cell Nucleolus chemistry, Fluorescent Dyes chemistry, HeLa Cells chemistry, Nuclear Proteins chemistry, Organoplatinum Compounds chemical synthesis, Organoplatinum Compounds chemistry

Abstract

An organometallic cyclometalated platinum(II) complex, [Pt(L(3))Cl][PF(6)], has been synthesised from a specially designed cyclometalating ligand, HL(3) (triphenyl{5-[3-(6-phenylpyridin-2-yl)-1H-pyrazol-1-yl]pentyl}phosphonium chloride), that contains a pendant carbon chain carrying a terminal cationic triphenylphosphonium moiety. Aside from its room temperature single-photon luminescent properties in solution, [Pt(L(3))Cl](+) can also produce two-photon-induced luminescence at room temperature upon excitation at 700 nm from a mode-locked Ti:sapphire laser. Its two-photon absorption cross-section in DMF at room temperature was measured to be 28.0x10(-50) cm(4) s photon(-1). [Pt(L(3))Cl](+) is able to selectively stain the cell nucleolus. This has been demonstrated by two-photon confocal imaging of live and methanol-fixed HeLa (human cervical carcinoma) and 3T3 (mouse skin fibroblasts) cells. This organelle specificity is likely to be related to its special affinity for proteins within cell nucleoli. As a result of such protein affinity, [Pt(L(3))Cl](+) is an efficient RNA transcription inhibitor and shows rather profound cytotoxicity. On the other hand, the organelle-specific labelling and two-photon-induced luminescent properties of [Pt(L(3))Cl](+) renders it a useful nuclear dye for the 3-dimensional reconstruction of optical sections of thick tissues, for example, mouse ileum tissues, by multiphoton confocal microscopy.

Published

2010

113. Nucleolar localization of influenza A NS1: striking differences between mammalian and avian cells.

Author

Volmer R, Mazel-Sanchez B, Volmer C, Soubies SM, and Guérin JL

Subjects

Animals, Cell Line, Cells, Cultured, Chick Embryo, Chickens, Ducks, Epithelial Cells virology, Fibroblasts virology, Humans, Influenza A Virus, H1N1 Subtype genetics, Influenza A Virus, H1N1 Subtype physiology, Influenza A Virus, H3N2 Subtype genetics, Influenza A Virus, H3N2 Subtype physiology, Influenza A virus genetics, Mice, Mice, Inbred BALB C, Protein Sorting Signals, Protein Transport, Cell Nucleolus chemistry, Influenza A virus physiology, Viral Nonstructural Proteins analysis

Abstract

In mammalian cells, nucleolar localization of influenza A NS1 requires the presence of a C-terminal nucleolar localization signal. This nucleolar localization signal is present only in certain strains of influenza A viruses. Therefore, only certain NS1 accumulate in the nucleolus of mammalian cells. In contrast, we show that all NS1 tested in this study accumulated in the nucleolus of avian cells even in the absence of the above described C-terminal nucleolar localization signal. Thus, nucleolar localization of NS1 in avian cells appears to rely on a different nucleolar localization signal that is more conserved among influenza virus strains.

Published

2010

114. Proteomic analysis of rodent ribosomes revealed heterogeneity including ribosomal proteins L10-like, L22-like 1, and L39-like.

Author

Sugihara Y, Honda H, Iida T, Morinaga T, Hino S, Okajima T, Matsuda T, and Nadano D

Subjects

Amino Acid Sequence, Animals, Cell Line, Cell Nucleolus chemistry, Cell Nucleolus metabolism, Electrophoresis, Gel, Two-Dimensional, Female, Humans, Male, Mammals, Mammary Glands, Human metabolism, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Organ Specificity, Rats, Rats, Sprague-Dawley, Ribosomal Proteins genetics, Ribosomal Proteins metabolism, Sequence Alignment, Testis metabolism, Liver chemistry, Mammary Glands, Human chemistry, Proteomics methods, Ribosomal Proteins analysis, Testis chemistry

Abstract

Heterogeneity of ribosome structure, due to variations in ribosomal protein composition, has been shown to be of physiological significance in plants and yeast. Mammalian genomics have demonstrated numerous genes that are paralogous to genes encoding ribosomal proteins. Although the vast majority are considered to be pseudogenes, mRNA expression of a few paralogues, such as human ribosomal protein L39-like/L39-2, has been reported. In the present study, ribosomes from the liver, mammary gland, and testis of rodents were analyzed using a combination of two-dimensional gel electrophoresis under radical-free and highly reducing conditions, and mass spectrometry. This system allowed identification of 78 ribosomal proteins and Rack1 from a single gel. The degree of heterogeneity was far less than that reported for plant and yeast ribosomes, and was in accord with published biochemical and genetic data for mammalian ribosomes. Nevertheless, an uncharacterized paralogue of ribosomal protein L22, ribosomal protein L22-like 1, was identified as a minor ribosomal component. Ribosomal proteins L10-like and L39-like, paralogues of ribosomal proteins L10 and L39, respectively, were found in ribosomes only from the testis. Reverse transcription-polymerase chain reaction yielded supportive evidence for specific expression of L10-like and L39-like in the testis. Newly synthesized L39-like is likely to be transported to the nucleolus, where ribosome biosynthesis occurs, and then incorporated into translating ribosomes in the cytoplasm. Heterogeneity of mammalian testicular ribosomes is structurally non-negligible, and may offer valuable insights into the function of the customized ribosome.

Published

2010

115. A quantitative proteomics analysis of subcellular proteome localization and changes induced by DNA damage.

Author

Boisvert FM, Lam YW, Lamont D, and Lamond AI

Subjects

Antineoplastic Agents, Phytogenic pharmacology, Cell Extracts analysis, Cell Nucleolus drug effects, Cell Nucleolus metabolism, Cytoplasm drug effects, Cytoplasm metabolism, DNA genetics, Etoposide pharmacology, HCT116 Cells, Humans, Isotope Labeling, Molecular Chaperones metabolism, Proteome genetics, Proteome metabolism, Subcellular Fractions chemistry, Subcellular Fractions metabolism, Cell Nucleolus chemistry, Cytoplasm chemistry, DNA Damage, Proteome analysis, Proteomics methods

Abstract

A major challenge in cell biology is to identify the subcellular distribution of proteins within cells and to characterize how protein localization changes under different cell growth conditions and in response to stress and other external signals. Protein localization is usually determined either by microscopy or by using cell fractionation combined with protein blotting techniques. Both these approaches are intrinsically low throughput and limited to the analysis of known components. Here we use mass spectrometry-based proteomics to provide an unbiased, quantitative, and high throughput approach for measuring the subcellular distribution of the proteome, termed "spatial proteomics." The spatial proteomics method analyzes a whole cell extract created by recombining differentially labeled subcellular fractions derived from cells in which proteins have been mass-labeled with heavy isotopes. This was used here to measure the relative distribution between cytoplasm, nucleus, and nucleolus of over 2,000 proteins in HCT116 cells. The data show that, at steady state, the proteome is predominantly partitioned into specific subcellular locations with only a minor subset of proteins equally distributed between two or more compartments. Spatial proteomics also facilitates a proteome-wide comparison of changes in protein localization in response to a wide range of physiological and experimental perturbations, shown here by characterizing dynamic changes in protein localization elicited during the cellular response to DNA damage following treatment of HCT116 cells with etoposide. DNA damage was found to cause dissociation of the proteasome from inhibitory proteins and assembly chaperones in the cytoplasm and relocation to associate with proteasome activators in the nucleus.

Published

2010

116. Immunogold labelling for scanning electron microscopy.

Author

Goldberg MW and Fiserova J

Subjects

Animals, Cell Nucleolus chemistry, Cell Nucleolus immunology, Cell Nucleolus ultrastructure, Cells, Cultured, Gold Colloid immunology, Oocytes cytology, Oocytes growth & development, Oocytes ultrastructure, Xenopus laevis, Gold Colloid chemistry, Immunohistochemistry methods, Microscopy, Electron, Scanning methods

Abstract

Scanning electron microscopes are useful biological tools that can be used to image the surface of whole organisms, tissues, cells, cellular components and macromolecules. Processes and structures that exist at surfaces can be imaged in pseudo or real 3D at magnifications of anything from about x10 to x1,000,000. Therefore a whole multicellular organism, such as a fly, or a single protein embedded in one of its cell membranes can be visualised. In order to identify that protein at high resolution, or to see and quantify its distribution at lower magnifications, samples can be labelled with antibodies. Any surface that can be exposed can potentially be studied in this way. Presented here is a generic method for immunogold labelling for scanning electron microscopy, using two examples of specimens: isolated nuclear envelopes and the cytoskeleton of mammalian culture cells. Various parameters for sample preparation, fixation, immunogold labelling, drying, metal coating and imaging are discussed so that the best immunogold scanning electron microscopy results can be obtained from different types of specimens.

Published

2010

117. Localization of rDNA at nucleolar structural components by immunoelectron microscopy.

Author

Sato S and Sato Y

Subjects

Microscopy, Immunoelectron, Onions chemistry, Onions cytology, Onions ultrastructure, Plant Roots chemistry, Plant Roots cytology, Plant Roots ultrastructure, Cell Nucleolus chemistry, Cell Nucleolus ultrastructure, DNA, Ribosomal analysis

Abstract

Fluorescence in situ hybridization (FISH) shows that DNA encoding ribosomal RNA cistron (rDNA) is localized to small speckles scattered in the nucleolus and the nucleolus-associated chromatin (NAC). This technique cannot however precisely locate rDNA in the nucleolar ultrastructural components such as the fibrillar center (FC), dense fibrillar component (DFC), and granular component (GC). In situ hybridization at the electron microscopic level is suitable for localization of rDNA at the ultrastructural level. We have tried to determine the precise localization of rDNA in the nucleolus of a higher plant by electron microscopic (EM) in situ hybridization using biotin-labeled 18S rDNA and demonstrated that it is exclusively localized in the fibrillar centers (FCs) and the nucleolus-associated chromatin (NAC). A secondary antibody coupled to the smallest (5 nm) colloidal gold particles was used in this technique to increase the label. Another important factor to increase the label was pretreatment with proteinase. Convincing results are obtained when the samples are pretreated with 1 microg/mL proteinase K for 45 min at 37 degrees C before immunogold labeling.

Published

2010

118. The bovine immunodeficiency virus rev protein: identification of a novel lentiviral bipartite nuclear localization signal harboring an atypical spacer sequence.

Author

Gomez Corredor A and Archambault D

Subjects

Amino Acid Sequence, Animals, Cell Nucleolus chemistry, Cell Nucleus chemistry, Cells, Cultured, Gene Products, rev chemistry, Humans, Molecular Sequence Data, Gene Products, rev analysis, Immunodeficiency Virus, Bovine chemistry, Nuclear Localization Signals

Abstract

The bovine immunodeficiency virus (BIV) Rev protein (186 amino acids [aa] in length) is involved in the nuclear exportation of partially spliced and unspliced viral RNAs. Previous studies have shown that BIV Rev localizes in the nucleus and nucleolus of infected cells. Here we report the characterization of the nuclear/nucleolar localization signals (NLS/NoLS) of this protein. Through transfection of a series of deletion mutants of BIV Rev fused to enhanced green fluorescent protein and fluorescence microscopy analyses, we were able to map the NLS region between aa 71 and 110 of the protein. Remarkably, by conducting alanine substitution of basic residues within the aa 71 to 110 sequence, we demonstrated that the BIV Rev NLS is bipartite, maps to aa 71 to 74 and 95 to 101, and is predominantly composed of arginine residues. This is the first report of a bipartite Rev (or Rev-like) NLS in a lentivirus/retrovirus. Moreover, this NLS is atypical, as the length of the sequence between the motifs composing the bipartite NLS, e.g., the spacer sequence, is 20 aa. Further mutagenesis experiments also identified the NoLS region of BIV Rev. It localizes mainly within the NLS spacer sequence. In addition, the BIV Rev NoLS sequence differs from the consensus sequence reported for other viral and cellular nucleolar proteins. In summary, we conclude that the nucleolar and nuclear localizations of BIV Rev are mediated via novel NLS and NoLS motifs.

Published

2009

119. B23 interacts with PES1 and is involved in nucleolar localization of PES1.

Author

Zhang J, Yang Y, and Wu J

Subjects

Base Sequence, Cell Nucleolus chemistry, Cell Nucleolus genetics, Cell Proliferation, Fluorescent Antibody Technique, HeLa Cells, Humans, Immunoblotting, Immunoprecipitation, Molecular Sequence Data, Nuclear Proteins chemistry, Nuclear Proteins genetics, Nucleophosmin, Plasmids genetics, Plasmids metabolism, Protein Binding, Protein Transport, Proteins chemistry, Proteins genetics, RNA Interference, RNA-Binding Proteins, Cell Nucleolus metabolism, Nuclear Proteins metabolism, Proteins metabolism

Abstract

PES1, the human homolog of zebrafish pescadillo, is a nucleolar protein that is essential for cell proliferation. We report herein that a nucleolar marker protein B23 physically interacts with PES1 and is involved in the nucleolar localization of PES1. In vivo interaction between B23 and PES1 was verified by co-immunoprecipitation of endogenous B23 and PES1 proteins, and they showed cellular co-localizations under both normal and actinomycin D-induced stress conditions. Furthermore, we mapped their interaction domains via in vitro pulldown assays. When B23 was knocked down by RNA interference, there appeared an increased nucleoplasmic distribution of PES1. Our results support a previous hypothesis that B23 might be a nucleolar hub protein for protein targeting to the nucleolus, and shed light on the nucleolar localization mechanism of PES1. The physical interaction between B23 and PES1 implies that they may participate in ribosome biogenesis in a protein complex.

Published

2009

120. Imprinting regulates mammalian snoRNA-encoding chromatin decondensation and neuronal nucleolar size.

Author

Leung KN, Vallero RO, DuBose AJ, Resnick JL, and LaSalle JM

Subjects

Adult, Animals, Cell Nucleolus genetics, Cell Nucleolus metabolism, Chromatin metabolism, Chromosomes, Mammalian genetics, Chromosomes, Mammalian metabolism, Humans, Male, Mice, Mice, Inbred C57BL, Middle Aged, Neurons chemistry, Prader-Willi Syndrome metabolism, RNA, Small Nucleolar metabolism, Ubiquitin-Protein Ligases genetics, Ubiquitin-Protein Ligases metabolism, snRNP Core Proteins genetics, snRNP Core Proteins metabolism, Cell Nucleolus chemistry, Chromatin Assembly and Disassembly, Genomic Imprinting, Neurons metabolism, Prader-Willi Syndrome genetics, RNA, Small Nucleolar genetics

Abstract

Imprinting, non-coding RNA and chromatin organization are modes of epigenetic regulation that modulate gene expression and are necessary for mammalian neurodevelopment. The only two known mammalian clusters of genes encoding small nucleolar RNAs (snoRNAs), SNRPN through UBE3A(15q11-q13/7qC) and GTL2(14q32.2/12qF1), are neuronally expressed, localized to imprinted loci and involved in at least five neurodevelopmental disorders. Deficiency of the paternal 15q11-q13 snoRNA HBII-85 locus is necessary to cause the neurodevelopmental disorder Prader-Willi syndrome (PWS). Here we show epigenetically regulated chromatin decondensation at snoRNA clusters in human and mouse brain. An 8-fold allele-specific decondensation of snoRNA chromatin was developmentally regulated specifically in maturing neurons, correlating with HBII-85 nucleolar accumulation and increased nucleolar size. Reciprocal mouse models revealed a genetic and epigenetic requirement of the 35 kb imprinting center (IC) at the Snrpn-Ube3a locus for transcriptionally regulated chromatin decondensation. PWS human brain and IC deletion mouse Purkinje neurons showed significantly decreased nucleolar size, demonstrating the essential role of the 15q11-q13 HBII-85 locus in neuronal nucleolar maturation. These results are relevant to understanding the molecular pathogenesis of multiple human neurodevelopmental disorders, including PWS and some causes of autism.

Published

2009

121. Characterization of the nuclear and nucleolar localization signals of bovine herpesvirus-1 infected cell protein 27.

Author

Guo H, Ding Q, Lin F, Pan W, Lin J, and Zheng AC

Subjects

Animals, Artificial Gene Fusion, Bacterial Proteins genetics, Bacterial Proteins metabolism, Cattle, Cell Line, Genes, Reporter, Haplorhini, Luminescent Proteins genetics, Luminescent Proteins metabolism, Mice, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Deletion, Cell Nucleolus chemistry, Herpesvirus 1, Bovine growth & development, Immediate-Early Proteins genetics, Immediate-Early Proteins metabolism, Phosphoproteins genetics, Phosphoproteins metabolism, Protein Sorting Signals, Protein Transport

Abstract

Bovine herpesvirus-1 infected cell protein 27 (BICP27) was detected predominantly in the nucleolus. The open reading frame of BICP27 was fused with the enhanced yellow fluorescent protein (EYFP) gene to investigate its subcellular localization in live cells and BICP27 was able to direct monomeric, dimeric or trimeric EYFP exclusively to the nucleolus. By constructing a series of deletion mutants, the putative nuclear localization signal (NLS) and nucleolar localization signal (NoLS) were mapped to (81)RRAR(84) and (86)RPRRPRRRPRRR(97) respectively. Specific deletion of the putative NLS, NoLS or both abrogated nuclear localization, nucleolar localization or both respectively. Furthermore, NLS was able to direct trimeric EYFP predominantly to the nucleus but excluded from the nucleolus, whereas NoLS targeted trimeric EYFP primarily to the nucleus, and enriched in the nucleolus with faint staining in the cytoplasm. NLS+NoLS directed trimeric EYFP predominantly to the nucleolus with faint staining in the nucleus. Moreover, deletion of NLS+NoLS abolished the transactivating activity of BICP27 on gC promoter, whereas deletion of either NLS or NoLS did not. The study demonstrated that BICP27 is a nucleolar protein, adding BICP27 to the growing list of transactivators which localize to the nucleolus.

Published

2009

122. On the intracellular trafficking of mouse S5 ribosomal protein from cytoplasm to nucleoli.

Author

Matragkou Ch, Papachristou H, Karetsou Z, Papadopoulos G, Papamarcaki T, Vizirianakis IS, Tsiftsoglou AS, and Choli-Papadopoulou T

Subjects

Animals, Blotting, Western, Genes, Reporter, Green Fluorescent Proteins analysis, Green Fluorescent Proteins genetics, HeLa Cells, Humans, Mice, Microscopy, Confocal, Mutagenesis, Phosphorylation, Polymerase Chain Reaction methods, Protein Transport, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins genetics, Cell Nucleolus chemistry, Cell Nucleus chemistry, Cytoplasm chemistry, Ribosomal Proteins analysis, Ribosomal Proteins genetics

Abstract

The non-ribosomal functions of mammalian ribosomal proteins have recently attracted worldwide attention. The mouse ribosomal protein S5 (rpS5) derived from ribosomal material is an assembled non-phosphorylated protein. The free form of rpS5 protein, however, undergoes phosphorylation. In this study, we have (a) investigated the potential role of phosphorylation in rpS5 protein transport into the nucleus and then into nucleoli and (b) determined which of the domains of rpS5 are involved in this intracellular trafficking. In vitro PCR mutagenesis of mouse rpS5 cDNA, complemented by subsequent cloning and expression of rpS5 truncated recombinant forms, produced in fusion with green fluorescent protein, permitted the investigation of rpS5 intracellular trafficking in HeLa cells using confocal microscopy complemented by Western blot analysis. Our results indicate the following: (a) rpS5 protein enters the nucleus via the region 38-50 aa that forms a random coil as revealed by molecular dynamic simulation. (b) Immunoprecipitation of rpS5 with casein kinase II and immobilized metal affinity chromatography analysis complemented by in vitro kinase assay revealed that phosphorylation of rpS5 seems to be indispensable for its transport from nucleus to nucleoli; upon entering the nucleus, Thr-133 phosphorylation triggers Ser-24 phosphorylation by casein kinase II, thus promoting entrance of rpS5 into the nucleoli. Another important role of rpS5 N-terminal region is proposed to be the regulation of protein's cellular level. The repetitively co-appearance of a satellite C-terminal band below the entire rpS5 at the late stationary phase, and not at the early logarithmic phase, of cell growth suggests a specific degradation balancing probably the unassembled ribosomal protein molecules with those that are efficiently assembled to ribosomal subunits. Overall, these data provide new insights on the structural and functional domains within the rpS5 molecule that contribute to its cellular functions.

Published

2009

123. Proteomics analysis of nucleolar SUMO-1 target proteins upon proteasome inhibition.

Author

Matafora V, D'Amato A, Mori S, Blasi F, and Bachi A

Subjects

Animals, Cell Nucleolus chemistry, Cysteine Proteinase Inhibitors metabolism, HeLa Cells, Humans, Isotope Labeling, Leupeptins metabolism, Molecular Sequence Data, SUMO-1 Protein genetics, Cell Nucleolus metabolism, Proteasome Inhibitors, Protein Processing, Post-Translational, Proteomics methods, SUMO-1 Protein metabolism

Abstract

Many cellular processes are regulated by the coordination of several post-translational modifications that allow a very fine modulation of substrates. Recently it has been reported that there is a relationship between sumoylation and ubiquitination. Here we propose that the nucleolus is the key organelle in which SUMO-1 conjugates accumulate in response to proteasome inhibition. We demonstrated that, upon proteasome inhibition, the SUMO-1 nuclear dot localization is redirected to nucleolar structures. To better understand this process we investigated, by quantitative proteomics, the effect of proteasome activity on endogenous nucleolar SUMO-1 targets. 193 potential SUMO-1 substrates were identified, and interestingly in several purified SUMO-1 conjugates ubiquitin chains were found to be present, confirming the coordination of these two modifications. 23 SUMO-1 targets were confirmed by an in vitro sumoylation reaction performed on nuclear substrates. They belong to protein families such as small nuclear ribonucleoproteins, heterogeneous nuclear ribonucleoproteins, ribosomal proteins, histones, RNA-binding proteins, and transcription factor regulators. Among these, histone H1, histone H3, and p160 Myb-binding protein 1A were further characterized as novel SUMO-1 substrates. The analysis of the nature of the SUMO-1 targets identified in this study strongly indicates that sumoylation, acting in coordination with the ubiquitin-proteasome system, regulates the maintenance of nucleolar integrity.

Published

2009

124. A FRET-based assay for characterization of alternative splicing events using peptide nucleic acid fluorescence in situ hybridization.

Author

Blanco AM, Rausell L, Aguado B, Perez-Alonso M, and Artero R

Subjects

Cell Nucleolus chemistry, Cytoplasm chemistry, HeLa Cells, Humans, Microscopy, Confocal, Pepsin A, Protein Isoforms genetics, Protein Isoforms metabolism, RNA, Messenger analysis, Alternative Splicing, Fluorescence Resonance Energy Transfer, In Situ Hybridization, Fluorescence methods, Nucleic Acid Probes chemistry, Peptide Nucleic Acids chemistry

Abstract

We describe a quantitative method for detecting RNA alternative splicing variants that combines in situ hybridization of fluorescently labeled peptide nucleic acid (PNA) probes with confocal microscopy Förster resonance energy transfer (FRET). The use of PNA probes complementary to sequences flanking a given splice junction allows to specifically quantify, within the cell, the RNA isoform generating such splice junction by FRET measure. As a proof of concept we analyzed two alternative splicing events originating from lymphocyte antigen 6 (LY6) complex, locus G5B (LY6G5B) pre-mRNA. These are characterized by the removal of the first intron (Fully Spliced Isoform, FSI) or by retention of such intron (Intron-Retained Isoform, IRI). The use of PNA probe pairs labeled with donor (Cy3) and acceptor (Cy5) fluorophores, suitable to FRET, flanking FSI and IRI specific splice junctions specifically detected both mRNA isoforms in HeLa cells. We have observed that the method works efficiently with probes 5-11 nt apart. The data supports that this FRET-based PNA fluorescence in situ hybridization (FP-FISH) method offers a conceptually new approach for characterizing at the subcellular level not only splice variant isoform structure, location and dynamics but also potentially a wide variety of close range RNA-RNA interactions.

Published

2009

125. Characterization of signals that dictate nuclear/nucleolar and cytoplasmic shuttling of the capsid protein of Tomato leaf curl Java virus associated with DNA beta satellite.

Author

Sharma P and Ikegami M

Subjects

Begomovirus genetics, DNA Mutational Analysis, Genes, Reporter, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Solanum lycopersicum, Sequence Deletion, Begomovirus physiology, Capsid Proteins genetics, Capsid Proteins metabolism, Cell Nucleolus chemistry, Cell Nucleus chemistry, Protein Sorting Signals, Virus Replication

Abstract

Transport of the viral genome into the nucleus is an obligatory step in the replication cycle of geminiviruses. Capsid proteins (CPs) of geminiviruses are multifunctional proteins thought to be involved in this process. The CP of monopartite geminiviruses is absolutely essential for virus movement. To more precisely examine the role of CP, we have constructed a series of single and double deletions into the coding sequence of Tomato leaf curl Java virus (ToLCJAV) CP and examined sub-cellular localization using transient expression of GFP fusion proteins. In this report, the domains of the CP encoded by ToLCJAV localized in the nucleus/nucleolus and cytoplasm in transfected cells were mapped. Deletion analysis revealed that the Arg-rich cluster from amino acids (aa) (16)KVRRR(20) in the N-terminal region of CP functioned as nuclear/nucleolar localization signals (NLSs). The region from aa (52)RKPR(55) contained basic amino acid cluster was capable to redirect the CP to the nucleus. Further, both transient expression and yeast hybrid assays demonstrated that CP was capable of shuttling between the nucleus and cytoplasm of the cell. Deletion mutant analysis revealed that this property was attributed to a nuclear export signal (NES) sequence consisted of aa ((245)LKIRIY(250)) reside at C-terminal part of CP. This hydrophobic region caused transport of GFP to the cytoplasm. However, ToLCJAV CP NLSs and NES show peculiarities in the number and position of basic residues. Taken together, these results demonstrated that ToLCJAV CP shuttles between the nucleus and cytoplasm, such an activity homolog to bipartite geminivirus BV1 ORF.

Published

2009

126. The nucleolus in Entamoeba histolytica and Entamoeba invadens is located at the nuclear periphery.

Author

Jhingan GD, Panigrahi SK, Bhattacharya A, and Bhattacharya S

Subjects

Animals, Cell Nucleolus chemistry, Cell Nucleus chemistry, Chromosomal Proteins, Non-Histone analysis, Entamoeba chemistry, Entamoeba histolytica chemistry, Entamoeba histolytica ultrastructure, Humans, RNA Polymerase I analysis, Cell Nucleolus ultrastructure, Cell Nucleus ultrastructure, Entamoeba ultrastructure

Abstract

The ribosomal RNA genes in the human parasite Entamoeba histolytica and its reptilian counterpart Entamoeba invadens are located on extrachromosomal circles. The expression of rRNA genes generally takes place in a specialized nuclear compartment-the nucleolus. In Entamoeba species the nuclear space that may be called the nucleolus has yet to be defined. Previous studies showed that the rDNA circles are located at the nuclear periphery. Here we have raised antibodies against the E. histolytica homologue of fibrillarin, a highly conserved protein known to be a marker for nucleolus. These antibodies cross-reacted preferentially with the nuclear periphery, forming a peripheral ring. There was complete colocalization of fibrillarin with the signal obtained by antibodies against E. histolytica RNA polymerase I (but not polymerase II and III), strongly suggesting that the nucleolus in E. histolytica is indeed located at the nuclear periphery. The dynamic nature of the nucleolus was evident when cells were subjected to a variety of growth stresses. Although the peripheral nucleolar structure was retained, stress was accompanied by significant cytoplasmic localization of RNA polymerase I, and to some extent fibrillarin. The nucleolus in E. invadens was also located at the nuclear periphery. When these cells were induced to encyst the nucleolar ring structure was lost, giving way to small, fragmented foci. This study gives the first clear insight into nucleolar structure in Entamoeba.

Published

2009

127. Identification of a perinuclear positioning element in human subtelomeres that requires A-type lamins and CTCF.

Author

Ottaviani A, Schluth-Bolard C, Rival-Gervier S, Boussouar A, Rondier D, Foerster AM, Morere J, Bauwens S, Gazzo S, Callet-Bauchu E, Gilson E, and Magdinier F

Subjects

Animals, Base Sequence, Biological Transport, CCCTC-Binding Factor, Carcinoma genetics, Carcinoma metabolism, Cell Line, Tumor, Cell Nucleolus chemistry, Cell Nucleolus metabolism, Down-Regulation, Epithelial Cells cytology, Epithelial Cells metabolism, Female, Humans, Insulator Elements, Locus Control Region, Protein Binding, Repressor Proteins genetics, Uterine Cervical Neoplasms genetics, Uterine Cervical Neoplasms metabolism, Lamin Type A metabolism, Repressor Proteins metabolism, Telomere chemistry, Telomere metabolism

Abstract

The localization of genes within the nuclear space is of paramount importance for proper genome functions. However, very little is known on the cis-acting elements determining subnuclear positioning of chromosome segments. We show here that the D4Z4 human subtelomeric repeat localizes a telomere at the nuclear periphery. This perinuclear activity lies within an 80 bp sequence included within a region known to interact with CTCF and A-type Lamins. We further show that a reduced level of either CTCF or A-type Lamins suppresses the perinuclear activities of D4Z4 and that an array of multimerized D4Z4 sequence, which has lost its ability to bind CTCF and A-type Lamins, is not localized at the periphery. Overall, these findings reveal the existence of an 80 bp D4Z4 sequence that is sufficient to position an adjacent telomere to the nuclear periphery in a CTCF and A-type lamins-dependent manner. Strikingly, this sequence includes a 30 bp GA-rich motif, which binds CTCF and is present at several locations in the human genome.

Published

2009

128. Dynamic changes of nucleolar DNA configuration and distribution during the cell cycle in Allium sativum cells.

Author

Shang G, Wang F, Hao S, and Jiao M

Subjects

Chromatin metabolism, DNA, Plant metabolism, Staining and Labeling methods, Cell Cycle, Cell Nucleolus chemistry, DNA, Plant chemistry, Garlic physiology, Nucleic Acid Conformation

Abstract

To investigate the correlation between subnucleolar structure and function, the precise distribution and configuration of nucleolar DNA during the cell cycle of Allium sativum were determined using the NAMA-Ur DNA-specific staining technique. We showed that nucleolar DNA is present in two forms: compacted chromatin clumps and a decondensed DNA cloud. The form of the DNA within the nucleolus varied greatly as the cell cycle progressed. During telophase, chromosomes extended into the prenucleolar body. In early G1 phase, DNA was only located in the fibrillar centers in the form of the condensed chromatin clump, while in mid-G1, S and G2 phases, the two forms of DNA were distributed in the fibrillar centers (FC) and dense fibrillar component (DFC). In prophase of mitosis, nucleolar DNA, along with FC and DFC, was linked into a network structure and condensed into a large chromatin clump. The area of the DNA cloud in the dense fibrillar component changed during different phases of the cell cycle. Our results demonstrated that the configuration of nucleolar DNA undergoes a series of decondensations and condensations during the cell cycle to fulfill the function of the nucleoli during the different phases.

Published

2009

129. Non-specific interactions are sufficient to explain the position of heterochromatic chromocenters and nucleoli in interphase nuclei.

Author

de Nooijer S, Wellink J, Mulder B, and Bisseling T

Subjects

Arabidopsis genetics, Cell Nucleus genetics, Chromosomes, Plant chemistry, Computer Simulation, Models, Molecular, Cell Nucleolus chemistry, Heterochromatin chemistry, Interphase genetics

Abstract

The organization of the eukaryote nucleus into functional compartments arises by self-organization both through specific protein-protein and protein-DNA interactions and non-specific interactions that lead to entropic effects, such as e.g. depletion attraction. While many specific interactions have so far been demonstrated, the contributions of non-specific interactions are still unclear. We used coarse-grained molecular dynamics simulations of previously published models for Arabidopsis thaliana chromatin organization to show that non-specific interactions can explain the in vivo localization of nucleoli and chromocenters. Also, we quantitatively demonstrate that chromatin looping contributes to the formation of chromosome territories. Our results are consistent with the previously published Rosette model for Arabidopsis chromatin organization and suggest that chromocenter-associated loops play a role in suppressing chromocenter clustering.

Published

2009

130. Redefining the Scl-70 indirect immunofluorescence pattern: autoantibodies to DNA topoisomerase I yield a specific compound immunofluorescence pattern.

Author

Dellavance A, Gallindo C, Soares MG, da Silva NP, Mortara RA, and Andrade LE

Subjects

Cell Line, Cell Nucleolus chemistry, Cell Nucleus chemistry, Chromosomes chemistry, Cytoplasm chemistry, Fluorescent Antibody Technique, Indirect, Humans, Interphase, Mitosis, Nucleolus Organizer Region chemistry, Scleroderma, Systemic immunology, Autoantibodies immunology, Autoantigens blood, DNA Topoisomerases, Type I immunology, Nuclear Proteins blood

Abstract

Objectives: To report on a novel IIF pattern specifically associated with antibodies to DNA topo I., Methods: A novel compound IF pattern, designated Scl-70 pattern, was characterized in routine ANA-HEp-2 IIF screening. Within the last 3 years, all serum samples presenting the Scl-70 pattern at the ANA-HEp2 IIF screening were tested for anti-topo I reactivity. Conversely, 16 serum samples with known anti-topo I reactivity and affinity-purified anti-topo I antibody preparations were tested for the Scl-70 pattern., Results: The Scl-70 pattern comprised the staining of five cellular regions: nucleus, nucleolus and cytoplasm in interphase cells; nucleolar organizing region (NOR) and chromosomes in mitotic cells. All 81 serum samples selected as Scl-70 pattern reacted with topo I. All 16 anti-topo I samples and antibody preparations reproduced the Scl-70 pattern. This compound IF pattern was consistently observed in different commercial HEp-2 cell slides and in home-made slides with HEp-2 cells and human fibroblasts fixed with alternative protocols. Double IIF experiments demonstrated the co-localization of topo I and human upstream binding factor at the NOR., Conclusions: The Scl-70 pattern belongs to the group of compound IF patterns that hold strong association with the respective autoantibody specificities, such as that observed with centromere protein F (CENP-F) and nuclear mitotic apparatus-1 (NuMA-1) protein. The identification of the Scl-70 pattern at routine ANA-HEp-2 IIF screening may lead to implementation of specific tests for the identification of anti-topo I antibodies. In addition, the Scl-70 pattern outlines cellular domains other than those previously reported for topo I, which is of interest for further understanding the roles of this enzyme in cell biology.

Published

2009

131. Dynamic localization of tripartite motif-containing 22 in nuclear and nucleolar bodies.

Author

Sivaramakrishnan G, Sun Y, Tan SK, and Lin VC

Subjects

Blotting, Northern, Cell Line, Tumor, Flow Cytometry, Fluorescent Antibody Technique, HeLa Cells, Humans, Minor Histocompatibility Antigens, Nuclear Proteins metabolism, RNA, Messenger biosynthesis, Repressor Proteins genetics, Repressor Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, Tripartite Motif Proteins, Cell Nucleolus chemistry, Intranuclear Inclusion Bodies chemistry, Repressor Proteins analysis

Abstract

Tripartite motif-containing 22 (TRIM22) exhibits antiviral and growth inhibitory properties, but there has been no study on the localization and dynamics of the endogenous TRIM22 protein. We report here that TRIM22 is dramatically induced by progesterone in MDA-MB-231-derived ABC28 cells and T47D cells. This induction was associated with an increase in TRIM22 nuclear bodies (NB), and an even more prominent increase in nucleolar TRIM22 bodies. Distinct endogenous TRIM22 NB were also demonstrated in several other cell lines including MCF7 and HeLa cells. These TRIM22 NB resemble Cajal bodies, co-localized with these structures and co-immunoprecipitated with p80-coilin. However, IFNgamma-induced TRIM22 in HeLa and MCF7 cells did not form NB, implying the forms and distribution of TRIM22 are regulated by specific cellular signals. This notion is also supported by the observation that TRIM22 NB undergoes dynamic cell-cycle dependent changes in distribution such that TRIM22 NB started to form in early G0/G1 but became dispersed in the S-phase. In light of its potential antiviral and antitumor properties, the findings here provide an interesting gateway to study the relationship between the different forms and functions of TRIM22.

Published

2009

132. Chromatin: linking structure and function in the nucleolus.

Author

McKeown PC and Shaw PJ

Subjects

Animals, Biological Evolution, Cell Nucleolus chemistry, DNA, Ribosomal genetics, DNA, Ribosomal metabolism, Eukaryotic Cells, Humans, Pol1 Transcription Initiation Complex Proteins metabolism, Transcription, Genetic physiology, Cell Nucleolus genetics, Cell Nucleolus metabolism, Chromatin genetics, Chromatin metabolism

Abstract

The nucleolus is an informative model structure for studying how chromatin-regulated transcription relates to nuclear organisation. In this review, we describe how chromatin controls nucleolar structure through both the modulation of rDNA activity by convergently-evolved remodelling complexes and by direct effects upon rDNA packaging. This packaging not only regulates transcription but may also be important for suppressing internal recombination between tandem rDNA repeats. The identification of nucleolar histone chaperones and novel chromatin proteins by mass spectrometry suggests that structure-specific chromatin components remain to be characterised and may regulate the nucleolus in novel ways. However, it also suggests that there is considerable overlap between nucleolar and non-nucleolar-chromatin components. We conclude that a fuller understanding of nucleolar chromatin will be essential for understanding how gene organisation is linked with nuclear architecture.

Published

2009

133. Localization and importance of the adenovirus E4orf4 protein during lytic infection.

Author

Miron MJ, Blanchette P, Groitl P, Dallaire F, Teodoro JG, Li S, Dobner T, and Branton PE

Subjects

Cell Line, Cell Nucleolus chemistry, Cell Nucleus chemistry, Cytoplasm chemistry, Humans, Mutant Proteins genetics, Mutant Proteins metabolism, RNA, Messenger metabolism, RNA, Viral metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Viral Proteins genetics, Adenoviruses, Human physiology, Viral Proteins metabolism, Virus Replication

Abstract

The human adenovirus type 5 (Ad5) E4orf4 product has been studied extensively although in most cases as expressed from vectors in the absence of other viral products. Thus, relatively little is known about its role in the context of an adenovirus infection. Although considerable earlier work had indicated that the E4orf4 protein is not essential for replication, a recent study using dl359, an Ad5 mutant believed to produce a nonfunctional E4orf4 protein, suggested that E4orf4 is essential for virus growth in primary small-airway epithelial cells (C. O'Shea, et al., EMBO J. 24:1211-1221, 2005). Hence, to examine further the role of E4orf4 during virus infection, we generated for the first time a set of E4orf4 virus mutants in a common Ad5 genetic background. Such mutant viruses included those that express E4orf4 proteins containing various individual point mutations, those defective entirely in E4orf4 expression, and a mutant expressing wild-type E4orf4 fused to the green fluorescent protein. E4orf4 protein was found to localize primarily in nuclear structures shown to be viral replication centers, in nucleoli, and in perinuclear bodies. Importantly, E4orf4 was shown not to be essential for virus growth in either human tumor or primary cells, at least in tissue culture. Unlike E4orf4-null virus, mutant dl359 appeared to exhibit a gain-of-function phenotype that impairs virus growth. The dl359 E4orf4 protein, which contains a large in-frame internal deletion, clustered in aggregates enriched in Hsp70 and proteasome components. In addition, the late viral mRNAs produced by dl359 accumulated abnormally in a nuclear punctate pattern. Altogether, our results indicate that E4orf4 protein is not essential for virus growth in culture and that expression of the dl359 E4orf4 product interferes with viral replication, presumably through interactions with structures in the nucleus.

Published

2009

134. NOPdb: Nucleolar Proteome Database--2008 update.

Author

Ahmad Y, Boisvert FM, Gregor P, Cobley A, and Lamond AI

Subjects

Humans, Internet, Mass Spectrometry, Peptides chemistry, Proteome chemistry, Cell Nucleolus chemistry, Databases, Protein, Nuclear Proteins chemistry

Abstract

An experimental data handling system has been created as an update to the previous Nucleolar Proteome Database (NOPdb3.0: http://www.lamondlab.com/NOPdb3.0/). This updated system is able to manage large data sets identified by multiple mass spectrometry and has been used to analyse highly purified preparations of human nucleoli from different cell lines. The newly created application includes a dynamic relational database, which is kept up to date by laboratory staff. The data are further annotated with information from specific external sources on the web, including the IPI and Gene Ontology databases. In addition, an Application Programming Interface provides external users with a portal to link into the nucleolar proteome database and hence, gain access to continually updated results. From the initial approximately 700 human proteins identified in the previous iteration of the NOPdb, we have now identified over 50 000 peptides contained in over 4500 human proteins from purified nucleoli, providing enhanced coverage of the nucleolar proteome.

Published

2009

135. Heterologous expression ofa histone-like protein from Streptococcus intermedius in Escherichia coli alters the nucleoid structure and inhibits the growth of E. coli.

Author

Liu D, Yumoto H, Murakami K, Hirota K, Kayama S, Taniguchi T, Yamamoto A, Ono T, Matsuo T, and Miyake Y

Subjects

Bacterial Proteins genetics, Cell Nucleolus genetics, Cell Nucleolus metabolism, Cloning, Molecular, DNA, Bacterial chemistry, DNA, Bacterial genetics, DNA, Superhelical chemistry, DNA, Superhelical genetics, Escherichia coli chemistry, Escherichia coli genetics, Escherichia coli metabolism, Histones genetics, Bacterial Proteins metabolism, Cell Nucleolus chemistry, Escherichia coli growth & development, Gene Expression, Histones metabolism, Streptococcus intermedius metabolism

Abstract

Escherichia coli failed to survive after transformation with a Streptococcus intermedius histone-like protein gene (Si-hlp) and its promoter-harbored plasmid. The promoter function of Si-hlp in E. coli was determined using enhanced green fluorescence protein (egfp) gene as a reporter. The inhibitory effect of Si-HLP on E. coli viability was verified by a tetracycline-inducible gene expression system. Further study suggested that Si-HLP may alter the bacterial nucleoid structure, leading to the growth inhibition of E. coli.

Published

2008

136. The nucleoprotein and the viral RNA of infectious salmon anemia virus (ISAV) are localized in the nucleolus of infected cells.

Author

Goić B, Bustamante J, Miquel A, Alvarez M, Vera MI, Valenzuela PD, and Burzio LO

Subjects

Amino Acid Sequence, Animals, Cell Line, Fluorescent Antibody Technique, Indirect, Immunoprecipitation, In Situ Hybridization, Microscopy, Confocal, Molecular Sequence Data, Phosphoproteins analysis, RNA-Binding Proteins analysis, Salmon, Sequence Alignment, Virus Assembly, Virus Replication, Nucleolin, Cell Nucleolus chemistry, Isavirus physiology, Nucleoproteins analysis, RNA, Viral analysis

Abstract

The infectious salmon anemia virus (ISAV), which belongs to the new genus Isavirus of the Orthomyxoviridae family, is an important pathogen of the salmon farming industry. Indirect immunofluorescence assays carried out with monoclonal antibodies specific for the nucleoprotein (NP) reveal differential staining of sub-cellular compartments in infected cells. Particularly interesting was the staining of the nucleolus, which showed co-localization with nucleolin in CHSE-214, EPC and SHK-1 cells infected with ISAV. These results were confirmed by co-immunoprecipitation studies showing an interaction between NP and nucleolin. In addition, in situ hybridization carried out with probes specific for each of the 8 RNA segments of ISAV showed that the genomic as well as the anti-genomic strands were also localized in the nucleolus. These results suggest a role of the nucleolus in the replication and/or in the packaging of the ISAV genome.

Published

2008

137. The major tegument structural protein VP22 targets areas of dispersed nucleolin and marginalized chromatin during productive herpes simplex virus 1 infection.

Author

López MR, Schlegel EF, Wintersteller S, and Blaho JA

Subjects

Animals, Artificial Gene Fusion, Cell Nucleolus chemistry, Cell Nucleus chemistry, Chlorocebus aethiops, Fluorescent Antibody Technique, Genes, Reporter, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Microscopy, Confocal, Protein Binding, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Time Factors, Vero Cells, Nucleolin, Chromatin metabolism, Herpesvirus 1, Human physiology, Phosphoproteins metabolism, RNA-Binding Proteins metabolism, Viral Structural Proteins metabolism

Abstract

The herpes simplex virus (HSV) major tegument structural protein VP22 resides in multiple subcellular regions during productive infection. During an analysis of the molecular determinants of these localizations, we observed that a transfected fusion of the C-terminal portion of VP22, containing its pat4 nuclear localization signal, with GFP lacked nucleolar sparing compared to GFP alone. Thus, the initial goal was to determine whether VP22 associates with nucleoli. Using an optimized indirect immunofluorescence system to visualize nucleolin and viral proteins, we observed that VP22 present in VP22-expressing Vero (V49) cells "surrounded" nucleolin. These two initial findings implied that VP22 might associate directly with nucleoli. We next analyzed HSV-infected cells and observed that at late times, anti-nucleolin immune reactivity was dispersed throughout the nuclei while it retained uniform, circular staining in mock-infected cells. Time course infection experiments indicated that nucleolin initiated its transition from uniform to dispersed structures between 2 and 4 hpi. Comparison of Hoechst stained nuclei showed bright anti-nucleolin staining localized to regions of marginalized chromatin. These effects required de novo infected cell protein synthesis. A portion of VP22 detected in nuclei at 4 and 6 hpi localized to these areas of altered nucleolin and marginalized chromatin. VP22 was excluded from viral replication compartments containing the viral regulatory protein ICP22. Finally, altered nucleolin and marginalized chromatin were detected with a VP22-null virus, indicating that VP22 was not responsible for these nuclear architecture alterations. Thus, we conclude that nuclear VP22 targets unique subnuclear structures early (<6hpi) during herpes simplex virus 1 (HSV-1) infection.

Published

2008

138. Nop53p interacts with 5.8S rRNA co-transcriptionally, and regulates processing of pre-rRNA by the exosome.

Author

Granato DC, Machado-Santelli GM, and Oliveira CC

Subjects

Binding Sites, Cell Nucleolus chemistry, DNA-Directed DNA Polymerase metabolism, Exoribonucleases metabolism, Exosome Multienzyme Ribonuclease Complex, Genetic Complementation Test, Nuclear Proteins chemistry, Nuclear Proteins genetics, Polyadenylation, RNA Precursors biosynthesis, RNA, Ribosomal, 5.8S biosynthesis, Saccharomyces cerevisiae enzymology, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins chemistry, Saccharomyces cerevisiae Proteins genetics, Sequence Deletion, Transcription, Genetic, Gene Expression Regulation, Fungal, Nuclear Proteins metabolism, RNA Precursors metabolism, RNA Processing, Post-Transcriptional, RNA, Ribosomal, 5.8S metabolism, Saccharomyces cerevisiae Proteins metabolism

Abstract

In eukaryotes, pre-rRNA processing depends on a large number of nonribosomal trans-acting factors that form intriguingly organized complexes. One of the early stages of pre-rRNA processing includes formation of the two intermediate complexes pre-40S and pre-60S, which then form the mature ribosome subunits. Each of these complexes contains specific pre-rRNAs, ribosomal proteins and processing factors. The yeast nucleolar protein Nop53p has previously been identified in the pre-60S complex and shown to affect pre-rRNA processing by directly binding to 5.8S rRNA, and to interact with Nop17p and Nip7p, which are also involved in this process. Here we show that Nop53p binds 5.8S rRNA co-transcriptionally through its N-terminal region, and that this protein portion can also partially complement growth of the conditional mutant strain Deltanop53/GAL::NOP53. Nop53p interacts with Rrp6p and activates the exosome in vitro. These results indicate that Nop53p may recruit the exosome to 7S pre-rRNA for processing. Consistent with this observation and similar to the observed in exosome mutants, depletion of Nop53p leads to accumulation of polyadenylated pre-rRNAs.

Published

2008

139. To the nucleolar density and size in apoptotic human leukemic myeloblasts produced in vitro by Trichostatin A.

Author

Smetana K, Zápotocky M, Starková J, and Trka J

Subjects

Antigens, Nuclear analysis, Antigens, Nuclear ultrastructure, Cell Line, Tumor, Cell Nucleolus chemistry, Cell Nucleolus drug effects, Granulocyte Precursor Cells drug effects, Humans, Hydroxamic Acids pharmacology, RNA analysis, Apoptosis, Cell Nucleolus ultrastructure, Granulocyte Precursor Cells ultrastructure, Leukemia, Myelogenous, Chronic, BCR-ABL Positive pathology

Abstract

The present study was designed to provide more information on nucleoli in apoptotic cells,which were represented in the present study by cultured leukemic myeloblasts (Kasumi-1 cells). The apoptotic process in these cells was produced by trichostatin A (TSA) that is a histone deacetylase inhibitor with strong cytostatic effects. The selected TSA concentration added to cultures facilitated to study apoptotic and not-apoptotic cells in one and the same specimen. The nucleolar diameter and density were determined using computer assisted measurement and densitometry in specimens stained for RNA. In comparison with not-apoptotic cells, in apoptotic cells, nucleolar mean diameter did not change significantly and nucleolar RNA density was also not apparently different. On the other hand, the cytoplasmic RNA density in apoptotic cells was markedly reduced. Thus it seemed to be possible that the transcribed RNA remained "frozen"within the nucleolus but its transport to the cytoplasm decreased or stopped. However, the possibility of the RNA degradation in the cytoplasm of apoptotic cells based on the present study cannot be eliminated. At this occasion it should be added that AgNORs reflecting nucleolar biosynthetic and cell proliferation activity in apoptotic cells decreased in number or disappeared. The presented results also indicated that large nucleoli intensely stained for RNA need not be necessarily related to the high nucleolar biosynthetic or cell proliferation activity and may be also present in apoptotic cells responding to the cytostatic treatment.

Published

2008

140. Chromatin tethering effects of hNopp140 are involved in the spatial organization of nucleolus and the rRNA gene transcription.

Author

Tsai YT, Lin CI, Chen HK, Lee KM, Hsu CY, Yang SJ, and Yeh NH

Subjects

Cell Nucleolus chemistry, DNA, Ribosomal genetics, DNA, Ribosomal metabolism, DNA, Satellite metabolism, Gene Silencing, Humans, RNA, Ribosomal metabolism, Transcription, Genetic, Cell Nucleolus metabolism, Nuclear Proteins metabolism, Phosphoproteins metabolism

Abstract

The short arms of five human acrocentric chromosomes contain ribosomal gene (rDNA) clusters where numerous mini-nucleoli arise at the exit of mitosis. These small nucleoli tend to coalesce into one or a few large nucleoli during interphase by unknown mechanisms. Here, we demonstrate that the N- and C-terminal domains of a nucleolar protein, hNopp140, bound respectively to alpha-satellite arrays and rDNA clusters of acrocentric chromosomes for nucleolar formation. The central acidic-and-basic repeated domain of hNopp140, possessing a weak self-self interacting ability, was indispensable for hNopp140 to build up a nucleolar round-shaped structure. The N- or the C-terminally truncated hNopp140 caused nucleolar segregation and was able to alter locations of the rDNA transcription, as mediated by detaching the rDNA repeats from the acrocentric alpha-satellite arrays. Interestingly, an hNopp140 mutant, made by joining the N- and C-terminal domains but excluding the entire central repeated region, induced nucleolar disruption and global chromatin condensation. Furthermore, RNAi knockdown of hNopp140 resulted in dispersion of the rDNA and acrocentric alpha-satellite sequences away from nucleolus that was accompanied by rDNA transcriptional silence. Our findings indicate that hNopp140, a scaffold protein, is involved in the nucleolar assembly, fusion, and maintenance.

Published

2008

141. p14ARF interacts with DAXX: effects on HDM2 and p53.

Author

Ivanchuk SM, Mondal S, and Rutka JT

Subjects

Adaptor Proteins, Signal Transducing analysis, Adaptor Proteins, Signal Transducing chemistry, Animals, Binding Sites, Cell Line, Cell Nucleolus chemistry, Cell Nucleus Structures chemistry, Co-Repressor Proteins, Humans, Molecular Chaperones, Nuclear Proteins analysis, Nuclear Proteins chemistry, Repressor Proteins metabolism, SUMO-1 Protein metabolism, Tumor Suppressor Protein p14ARF analysis, Tumor Suppressor Protein p14ARF chemistry, Two-Hybrid System Techniques, Ubiquitination, Adaptor Proteins, Signal Transducing metabolism, Nuclear Proteins metabolism, Proto-Oncogene Proteins c-mdm2 metabolism, Tumor Suppressor Protein p14ARF metabolism, Tumor Suppressor Protein p53 metabolism

Abstract

The p14(ARF) (ARF) tumour suppressor plays an important role in the cellular response to oncogene activation. In this report, we demonstrate an interaction between ARF and DAXX, a highly conserved protein with identified roles in the regulation of gene expression. HDM2 was shown to interact with each of ARF and DAXX upon upregulation of expression as well as at lower expression levels following transfection of ARF and DAXX. Through immunofluorescence analysis, we observed that endogenous ARF and DAXX colocalize both to nucleoli and to nuclear bodies in cell lines that co-express both proteins. Similar results were obtained upon co-transfection of ARF and DAXX. Co-expression of ARF and DAXX was further found to inhibit ARF-mediated HDM2 sumoylation and to induce sumoylation and ubiquitination of DAXX itself, implicating DAXX as a substrate of ARF-mediated post-translational events. We also observed induction of p53 sumoylation in the presence of ARF and DAXX, an effect that was inhibited by upregulation of HDM2 expression. In summary, we have identified DAXX as a novel ARF binding partner and substrate of ARF-mediated sumoylation and suggest that DAXX acts as a modifier of both p53-dependent and p53-independent ARF function.

Published

2008

142. Assays for ribosomal RNA processing and ribosome assembly.

Author

Pestov DG, Lapik YR, and Lau LF

Subjects

Animals, Cell Nucleolus chemistry, Cell Nucleolus metabolism, Centrifugation, Density Gradient, DNA Probes, Humans, Mammals metabolism, RNA, Ribosomal analysis, Radioisotopes analysis, Radioisotopes metabolism, Ribonucleoproteins analysis, Ribonucleoproteins metabolism, Ribosomes chemistry, Cytological Techniques, RNA Processing, Post-Transcriptional, RNA, Ribosomal metabolism, Ribosomes metabolism

Abstract

The synthesis of ribosomes is a major metabolic activity critical for cell growth and homeostasis. Understanding the mechanisms of ribosome biogenesis has important implications for studying both protein synthesis and cell cycle control. This unit describes several techniques for the analysis of rRNA maturation and ribosome assembly adapted for mammalian cells. Metabolic labeling of rRNA and hybridization analysis of precursors can be used to assess changes in rRNA processing that occur under experimental conditions of interest. Separation of preribosomal particles by sucrose gradient centrifugation is suitable for the analysis of proteins associated with preribosomes during their assembly and maturation in the cell nucleus., (Copyright 2008 by John Wiley & Sons, Inc.)

Published

2008

143. Identification of genes that function in the biogenesis and localization of small nucleolar RNAs in Saccharomyces cerevisiae.

Author

Qiu H, Eifert J, Wacheul L, Thiry M, Berger AC, Jakovljevic J, Woolford JL Jr, Corbett AH, Lafontaine DL, Terns RM, and Terns MP

Subjects

Alleles, Cell Nucleolus chemistry, Cell Nucleolus metabolism, Hot Temperature, Mutation, Nuclear Proteins analysis, Nuclear Proteins genetics, Nuclear Proteins metabolism, RNA Precursors metabolism, RNA, Fungal analysis, RNA, Small Nucleolar analysis, Ribonucleoproteins, Small Nucleolar analysis, Ribonucleoproteins, Small Nucleolar genetics, Ribonucleoproteins, Small Nucleolar metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins analysis, Saccharomyces cerevisiae Proteins genetics, Genes, Fungal, RNA, Fungal metabolism, RNA, Small Nucleolar metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism

Abstract

Small nucleolar RNAs (snoRNAs) orchestrate the modification and cleavage of pre-rRNA and are essential for ribosome biogenesis. Recent data suggest that after nucleoplasmic synthesis, snoRNAs transiently localize to the Cajal body (in plant and animal cells) or the homologous nucleolar body (in budding yeast) for maturation and assembly into snoRNPs prior to accumulation in their primary functional site, the nucleolus. However, little is known about the trans-acting factors important for the intranuclear trafficking and nucleolar localization of snoRNAs. Here, we describe a large-scale genetic screen to identify proteins important for snoRNA transport in Saccharomyces cerevisiae. We performed fluorescence in situ hybridization analysis to visualize U3 snoRNA localization in a collection of temperature-sensitive yeast mutants. We have identified Nop4, Prp21, Tao3, Sec14, and Htl1 as proteins important for the proper localization of U3 snoRNA. Mutations in genes encoding these proteins lead to specific defects in the targeting or retention of the snoRNA to either the nucleolar body or the nucleolus. Additional characterization of the mutants revealed impairment in specific steps of U3 snoRNA processing, demonstrating that snoRNA maturation and trafficking are linked processes.

Published

2008

144. In situ comparative studies on subnucleolar distribution and configuration of plant rDNA.

Author

Long H, He J, Sun H, Hao S, and Jiao M

Subjects

Cell Nucleolus ultrastructure, Garlic genetics, Garlic ultrastructure, Pisum sativum genetics, Pisum sativum ultrastructure, Triticum genetics, Triticum ultrastructure, Cell Nucleolus chemistry, DNA, Plant analysis, DNA, Ribosomal analysis

Abstract

The distribution and configurations of nucleolar DNA in Pisum sativum L., Allium sativum L., Triticum aestivum L. were analyzed by specific cytochemical staining using NAMA-Ur. It has been observed that in the nucleoli of different plant species, the DNA occupied different positions in different areas, which may imply a different status and strategy of rDNA transcription. Our results showed irregular clumps of rDNA surrounding FCs in semi-circular formations in P. sativum and T. aestivum, indicating a regular pattern of rDNA distribution and supporting the helix model of rDNA configuration. The rDNA was condensed in some regions and uncondensed in others. Nucleolus-associated chromatin extended from outside the nucleolus to the periphery of the FCs via nucleolar channels, which suggests a possible origin for nucleolar DNA.

Published

2008

145. Nucleolin is required for an efficient herpes simplex virus type 1 infection.

Author

Callé A, Ugrinova I, Epstein AL, Bouvet P, Diaz JJ, and Greco A

Subjects

Cell Fractionation, Chromosomal Proteins, Non-Histone metabolism, DNA-Binding Proteins metabolism, Gene Silencing, HeLa Cells, Humans, Immediate-Early Proteins metabolism, Microscopy, Fluorescence, Phosphoproteins antagonists & inhibitors, RNA, Small Interfering metabolism, RNA-Binding Proteins antagonists & inhibitors, Viral Proteins metabolism, Nucleolin, Cell Nucleolus chemistry, Cell Nucleus virology, Herpesvirus 1, Human growth & development, Phosphoproteins metabolism, RNA-Binding Proteins metabolism

Abstract

Productive infection by herpes simplex virus type 1 (HSV-1), which occurs in the host cell nucleus, is accompanied by dramatic modifications of the nuclear architecture, including profound alterations of nucleolar morphology. Here, we show that the three most abundant nucleolar proteins--nucleolin, B23, and fibrillarin--are redistributed out of the nucleoli as a consequence of HSV-1 infection. We show that the amount of nucleolin increases progressively during the course of infection. We demonstrate for the first time that a nucleolar protein, i.e., nucleolin, colocalizes with ICP8 in the viral replication compartments, at the time when viral replication is effective, suggesting an involvement of nucleolin in the HSV-1 DNA replication process. At later times of infection, a granular form of nucleolin localizes to the cytoplasm, in structures that display the characteristic features of aggresomes, indicating that this form of nucleolin is very probably destined for degradation. The delocalization of nucleolin from the nucleoli requires the viral ICP4 protein or a factor(s) whose expression involves ICP4. Using small interfering RNA technology, we show that viral replication requires a high level of nucleolin expression, demonstrating for the first time a direct role for a nucleolar protein in herpes simplex virus biology.

Published

2008

146. Immunocytochemical demonstration of polyamines in nucleoli and nuclei.

Author

Shin M, Nakamuta H, Oda-Ueda N, Larsson LI, and Fujiwara K

Subjects

Cell Line, Tumor, HeLa Cells, Humans, Immunochemistry methods, Jurkat Cells, Ribosomes chemistry, U937 Cells, Cell Nucleolus chemistry, Cell Nucleus chemistry, Polyamines analysis

Abstract

Although biochemical studies have shown that polyamines (PAs) occur in the nucleus, only few studies have examined the intranuclear distribution of these organic cations. By immunocytochemistry, we have previously demonstrated that PAs are located in ribosomes. We now show that PAs also are present in both nucleoli and nuclei of a variety of cell types. Detection of nucleolar and nuclear PAs required novel pretreatment procedures involving protease and/or DNase digestion of specimens prior to immunoreaction. Double fluorescence staining confirmed the localizations. This suggests that PAs may be important to the formation of ribosomes in nucleoli, as well as adds support to biochemical studies suggesting that PAs are involved in many biological events in the nucleus. Further biochemical studies will be needed to substantiate this hypothesis.

Published

2008

147. The conserved N-terminal domain of herpes simplex virus 1 UL24 protein is sufficient to induce the spatial redistribution of nucleolin.

Author

Bertrand L and Pearson A

Subjects

Animals, COS Cells, Cell Nucleolus chemistry, Cell Nucleus chemistry, Chlorocebus aethiops, Chromosomal Proteins, Non-Histone analysis, Golgi Apparatus chemistry, Microscopy, Confocal, Protein Sorting Signals, Protein Structure, Tertiary, Nucleolin, Herpesvirus 1, Human physiology, Phosphoproteins metabolism, RNA-Binding Proteins metabolism, Viral Proteins metabolism

Abstract

UL24 is widely conserved among herpesviruses but its function during infection is poorly understood. Previously, we discovered a genetic link between UL24 and the herpes simplex virus 1-induced dispersal of the nucleolar protein nucleolin. Here, we report that in the absence of viral infection, transiently expressed UL24 accumulated in both the nucleus and the Golgi apparatus. In the majority of transfected cells, nuclear staining for UL24 was diffuse, but a minor staining pattern, whereby UL24 was present in nuclear foci corresponding to nucleoli, was also observed. Expression of UL24 correlated with the dispersal of nucleolin. This dispersal did not appear to be a consequence of a general disaggregation of nucleoli, as foci of fibrillarin staining persisted in cells expressing UL24. The conserved N-terminal region of UL24 was sufficient to cause this change in subcellular distribution of nucleolin. Interestingly, a bipartite nuclear localization signal predicted within the C terminus of UL24 was dispensable for nuclear localization. None of the five individual UL24 homology domains was required for nuclear or Golgi localization, but deletion of these domains resulted in the loss of nucleolin-dispersal activity. We determined that a nucleolar-targeting signal was contained within the first 60 aa of UL24. Our results show that the conserved N-terminal domain of UL24 is sufficient to specifically induce dispersal of nucleolin in the absence of other viral proteins or virus-induced cellular modifications. These results suggest that UL24 directly targets cellular factors that affect the composition of nucleoli.

Published

2008

148. Lysine 263 residue of NPM/B23 is essential for regulating ATP binding and B23 stability.

Author

Choi JW, Lee SB, Kim CK, Lee KH, Cho SW, and Ahn JY

Subjects

Animals, Binding Sites, Cell Nucleolus chemistry, Cell Proliferation, Lysine genetics, Nuclear Proteins genetics, Nucleophosmin, PC12 Cells, Proteasome Endopeptidase Complex metabolism, Rats, Ubiquitin metabolism, Adenosine Triphosphate metabolism, Lysine chemistry, Nuclear Proteins chemistry, Nuclear Proteins metabolism

Abstract

Here, we show that Nucleophsomin/B23 provides lysine 263 as a critical binding site for ATP. Mutagenesis of lysine 263 to asparagine (K263N) disrupts B23 from ATP binding. While B23 WT exclusively localizes to the nucleolus, the B23-K263N is redistributed from the nucleolus to the nucleoplam. Notably, the K263N mutant is unstable, and displayed rapid degradation. Alteration of K263 induced B23 instability through increased ubiquitination and proteaosomal degradation. Moreover, mutation of K263 impedes the mitogenic effect of B23 in PC12 cells. Thus, K263 is a critical site for ATP binding and required for B23 stability, confining B23 in the nucleolus.

Published

2008

149. Histone H1 of Trypanosoma cruzi is concentrated in the nucleolus region and disperses upon phosphorylation during progression to mitosis.

Author

Gutiyama LM, da Cunha JP, and Schenkman S

Subjects

Animals, Antibodies, Protozoan metabolism, Cytokinesis, Histones analysis, Phosphorylation, Protozoan Proteins analysis, Trypanosoma cruzi chemistry, Trypanosoma cruzi cytology, Cell Nucleolus chemistry, Histones metabolism, Mitosis, Protozoan Proteins metabolism, Trypanosoma cruzi metabolism

Abstract

Phosphorylation of histone H1 is intimately related to the cell cycle progression in higher eukaryotes, reaching maximum levels during mitosis. We have previously shown that in the flagellated protozoan Trypanosoma cruzi, which does not condense chromatin during mitosis, histone H1 is phosphorylated at a single cyclin-dependent kinase site. By using an antibody that recognizes specifically the phosphorylated T. cruzi histone H1 site, we have now confirmed that T. cruzi histone H1 is also phosphorylated in a cell cycle-dependent manner. Differently from core histones, the bulk of nonphosphorylated histone H1 in G(1) and S phases of the cell cycle is concentrated in the central regions of the nucleus, which contains the nucleolus and less densely packed chromatin. When cells pass G(2), histone H1 becomes phosphorylated and starts to diffuse. At the onset of mitosis, histone H1 phosphorylation is maximal and found in the entire nuclear space. As permeabilized parasites preferentially lose phosphorylated histone H1, we conclude that this modification promotes its release from less condensed and nucleolar chromatin after G(2).

Published

2008

150. Effect of roscovitine, a selective cyclin B-dependent kinase 1 inhibitor, on assembly of the nucleolus in mitosis.

Author

Zharskaya OO, Barsukova AS, and Zatsepina OV

Subjects

Animals, Cell Line, Cell Nucleolus drug effects, Cell Nucleolus ultrastructure, Cyclin B antagonists & inhibitors, Electrophoresis, Polyacrylamide Gel, Humans, Mice, Nuclear Proteins analysis, Nuclear Proteins metabolism, Nucleophosmin, Phosphoproteins analysis, Phosphoproteins metabolism, RNA-Binding Proteins analysis, RNA-Binding Proteins metabolism, Roscovitine, Nucleolin, Antineoplastic Agents antagonists & inhibitors, CDC2 Protein Kinase antagonists & inhibitors, Cell Nucleolus chemistry, Mitosis drug effects, Protein Kinase Inhibitors pharmacology, Purines pharmacology

Abstract

It is well known that at the beginning of mitosis the nucleolus disassembles but then reassembles at the end of mitosis. However, the mechanisms of these processes are still unclear. In the present work, we show for the first time that selective inhibition of cyclin B-dependent kinase 1 (CDK1) by roscovitine induces premature assembly of the nucleolus in mammalian cells in metaphase. Treatment of metaphase cells with roscovitine induces formation of structures in their cytoplasm that contain major proteins of the mature nucleolus participating in rRNA processing, such as B23/nucleophosmin, C23/nucleolin, fibrillarin, Nop52, as well as partially processed (immature) 46-45S pre-rRNA. This effect is reproducible in cells of various types; this indicates that general mechanisms regulate early stages of the nucleolus reassembly with CDK1 participation in mammalian cells. Based on our and literature data, we suggest that inactivation of the CDK1-cyclin B complex at the end of mitosis results in dephosphorylation of B23/nucleophosmin and C23/nucleolin; this facilitates their interaction with pre-rRNA and leads to formation of insoluble supramolecular complexes--nucleolus-derived foci.

Published

2008