Your search keyword '"Plevani, P."' showing total 14 results

1. Saccharomyces CDK1 phosphorylates Rad53 kinase in metaphase, influencing cellular morphogenesis.

Author

Diani L, Colombelli C, Nachimuthu BT, Donnianni R, Plevani P, Muzi-Falconi M, and Pellicioli A

Subjects

Alleles, Aspartic Acid chemistry, Cell Separation, Checkpoint Kinase 2, DNA Damage, Models, Biological, Mutagenesis, Mutation, Nocodazole pharmacology, Phosphorylation, Serine chemistry, CDC2 Protein Kinase metabolism, Cell Cycle Proteins metabolism, Protein Serine-Threonine Kinases metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism

Abstract

Rad53 is an essential protein kinase governing DNA damage and replication stress checkpoints in budding yeast. It also appears to be involved in cellular morphogenesis processes. Mass spectrometry analyses revealed that Rad53 is phosphorylated at multiple SQ/TQ and at SP/TP residues, which are typical consensus sites for phosphatidylinositol 3-kinase-related kinases and CDKs, respectively. Here we show that Clb-CDK1 phosphorylates Rad53 at Ser(774) in metaphase. This phosphorylation event does not influence the DNA damage and replication checkpoint roles of Rad53, and it is independent of the spindle assembly checkpoint network. Moreover, the Ser-to-Asp mutation, mimicking a constitutive phosphorylation state at site 774, causes sensitivity to calcofluor, supporting a functional linkage between Rad53 and cellular morphogenesis.

Published

2009

2. The 9-1-1 checkpoint clamp physically interacts with polzeta and is partially required for spontaneous polzeta-dependent mutagenesis in Saccharomyces cerevisiae.

Author

Sabbioneda S, Minesinger BK, Giannattasio M, Plevani P, Muzi-Falconi M, and Jinks-Robertson S

Subjects

Base Sequence, Cell Cycle Proteins chemistry, Chromosomes metabolism, Chromosomes ultrastructure, DNA chemistry, DNA Damage, DNA Repair, DNA Replication, DNA-Binding Proteins chemistry, DNA-Directed DNA Polymerase metabolism, Dimerization, Frameshift Mutation, Genome, Fungal, Glutathione Transferase metabolism, Immunoprecipitation, Intracellular Signaling Peptides and Proteins chemistry, Molecular Sequence Data, Mutation, Nuclear Proteins chemistry, Phosphoproteins chemistry, Plasmids metabolism, Proliferating Cell Nuclear Antigen metabolism, Protein Binding, Protein Structure, Tertiary, S Phase, Two-Hybrid System Techniques, Ultraviolet Rays, Cell Cycle Proteins metabolism, DNA-Binding Proteins metabolism, DNA-Directed DNA Polymerase chemistry, Gene Expression Regulation, Fungal, Mutagenesis, Nuclear Proteins metabolism, Phosphoproteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins chemistry, Saccharomyces cerevisiae Proteins metabolism

Abstract

The use of translesion synthesis (TLS) polymerases to bypass DNA lesions during replication constitutes an important mechanism to restart blocked/stalled DNA replication forks. Because TLS polymerases generally have low fidelity on undamaged DNA, the cell must regulate the interaction of TLS polymerases with damaged versus undamaged DNA to maintain genome integrity. The Saccharomyces cerevisiae checkpoint proteins Ddc1, Rad17, and Mec3 form a clamp-like structure (the 9-1-1 clamp) that has physical similarity to the homotrimeric sliding clamp proliferating cell nuclear antigen, which interacts with and promotes the processivity of the replicative DNA polymerases. In this work, we demonstrate both an in vivo and in vitro physical interaction between the Mec3 and Ddc1 subunits of the 9-1-1 clamp and the Rev7 subunit of the Polzeta TLS polymerase. In addition, we demonstrate that loss of Mec3, Ddc1, or Rad17 results in a decrease in Polzeta-dependent spontaneous mutagenesis. These results suggest that, in addition to its checkpoint signaling role, the 9-1-1 clamp may physically regulate Polzeta-dependent mutagenesis by controlling the access of Polzeta to damaged DNA.

Published

2005

3. The DNA damage checkpoint response requires histone H2B ubiquitination by Rad6-Bre1 and H3 methylation by Dot1.

Author

Giannattasio M, Lazzaro F, Plevani P, and Muzi-Falconi M

Subjects

Binding Sites, Blotting, Western, Cell Cycle, Cell Cycle Proteins metabolism, Cell Separation, Checkpoint Kinase 2, Chromatin metabolism, Electrophoresis, Polyacrylamide Gel, Enzyme Activation, Flow Cytometry, Histone-Lysine N-Methyltransferase, Intracellular Signaling Peptides and Proteins, Lysine chemistry, Methylation, Phosphorylation, Plasmids metabolism, Protein Serine-Threonine Kinases metabolism, Saccharomyces cerevisiae metabolism, Serine chemistry, Time Factors, Ultraviolet Rays, DNA Damage, Histones metabolism, Histones physiology, Nuclear Proteins metabolism, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins physiology, Ubiquitin metabolism, Ubiquitin-Conjugating Enzymes physiology

Abstract

The cellular response to DNA lesions entails the recruitment of several checkpoint and repair factors to damaged DNA, and chromatin modifications may play a role in this process. Here we show that in Saccharomyces cerevisiae epigenetic modification of histones is required for checkpoint activity in response to a variety of genotoxic stresses. We demonstrate that ubiquitination of histone H2B on lysine 123 by the Rad6-Bre1 complex, is necessary for activation of Rad53 kinase and cell cycle arrest. We found a similar requirement for Dot1-dependent methylation of histone H3. Loss of H3-Lys(79) methylation does not affect Mec1 activation, whereas it renders cells checkpoint-defective by preventing phosphorylation of Rad9. Such results suggest that histone modifications may have a role in checkpoint function by modulating the interactions of Rad9 with chromatin and active Mec1 kinase.

Published

2005

4. Correlation between checkpoint activation and in vivo assembly of the yeast checkpoint complex Rad17-Mec3-Ddc1.

Author

Giannattasio M, Sabbioneda S, Minuzzo M, Plevani P, and Muzi-Falconi M

Subjects

Cell Cycle drug effects, DNA-Binding Proteins, Kinetics, Macromolecular Substances, Nocodazole pharmacology, Nuclear Proteins, Phenotype, Saccharomyces cerevisiae genetics, Signal Transduction, Time Factors, Cell Cycle physiology, Cell Cycle Proteins metabolism, Phosphoproteins metabolism, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae physiology, Saccharomyces cerevisiae Proteins metabolism

Abstract

Rad17-Mec3-Ddc1 forms a proliferating cell nuclear antigen-like complex that is required for the DNA damage response in Saccharomyces cerevisiae and acts at an early step of the signal transduction cascade activated by DNA lesions. We used the mec3-dn allele, which causes a dominant negative checkpoint defect in G1 but not in G2, to test the stability of the complex in vivo and to correlate its assembly and disassembly with the mechanisms controlling checkpoint activation. Under physiological conditions, the mutant complex is formed both in G1 and G2, although the mutant phenotype is detectable only in G1, suggesting that is not the presence of the mutant complex per se to cause a checkpoint defect. Our data indicate that the Rad17-Mec3-Ddc1 complex is very stable, and it takes several hours to replace Mec3 with Mec3-dn within a wild type complex. On the other hand, the mutant complex is rapidly assembled when starting from a condition where the complex is not pre-assembled, indicating that the critical factor for the substitution is the disassembly step rather than complex formation. Moreover, the kinetics of mutant complex assembly, starting from conditions in which the wild type form is present, parallels the kinetics of checkpoint inactivation, suggesting that the complex acts in a stoichiometric way, rather than catalytically.

Published

2003

5. Phosphorylation of the DNA polymerase alpha-primase B subunit is dependent on its association with the p180 polypeptide.

Author

Ferrari M, Lucchini G, Plevani P, and Foiani M

Subjects

Cell Cycle, DNA Primase, Macromolecular Substances, Molecular Weight, Phosphorylation, Protein Binding, Saccharomyces cerevisiae enzymology, DNA Polymerase II metabolism, DNA Replication, RNA Nucleotidyltransferases metabolism

Abstract

The B subunit of the DNA polymerase (pol) alpha-primase complex executes an essential role at the initial stage of DNA replication in Saccharomyces cerevisiae and is phosphorylated in a cell cycle-dependent manner. In this report, we show that the four subunits of the yeast DNA polymerase alpha-primase complex are assembled throughout the cell cycle, and physical association between newly synthesized pol alpha (p180) and unphosphorylated B subunit (p86) occurs very rapidly. Therefore, B subunit phosphorylation does not appear to modulate p180.p86 interaction. Conversely, by depletion experiments and by using a yeast mutant strain, which produces a low and constitutive level of the p180 polypeptide, we found that formation of the p180.p86 subcomplex is required for B subunit phosphorylation.

Published

1996

6. Purification and characterization of a new DNA polymerase from budding yeast Saccharomyces cerevisiae. A probable homolog of mammalian DNA polymerase beta.

Author

Shimizu K, Santocanale C, Ropp PA, Longhese MP, Plevani P, Lucchini G, and Sugino A

Subjects

Animals, Base Sequence, DNA Polymerase I genetics, DNA Polymerase beta, DNA Primers, DNA-Directed DNA Polymerase genetics, DNA-Directed DNA Polymerase metabolism, Electrophoresis, Polyacrylamide Gel, Escherichia coli genetics, Humans, Kinetics, Magnesium, Molecular Sequence Data, Nucleic Acid Synthesis Inhibitors, Potassium Chloride, Sequence Homology, Nucleic Acid, Substrate Specificity, DNA-Directed DNA Polymerase isolation & purification, Saccharomyces cerevisiae enzymology, Saccharomyces cerevisiae Proteins

Abstract

A new DNA polymerase activity was identified and purified to near homogeneity from extracts of mitotic and meiotic cells of the yeast Saccharomyces cerevisiae. This activity increased at least 5-fold during meiosis, and it was shown to be associated with a 68-kDa polypeptide as determined by SDS-polyacrylamide gel electrophoresis. This new DNA polymerase did not have any detectable 3'-->5' exonuclease activity and preferred small gapped DNA as a template-primer. The activity was inhibited by dideoxyribonucleoside 5'-triphosphates and N-ethylmaleimide but not by concentrations of aphidicolin which completely inhibit either DNA polymerases I (alpha), II (epsilon), or III (delta). Since no polypeptide(s) in the extensively purified DNA polymerase fractions cross-reacted with antibodies raised against yeast DNA polymerases I, II, and III, we called this enzyme DNA polymerase IV. The DNA polymerase IV activity increased at least 10-fold in a yeast strain overexpressing the gene product predicted from the YCR14C open-reading frame (identified on S. cerevisiae chromosome III and provisionally called POLX), while no activity was detected in a strain where POLX was deleted. These results strongly suggest that DNA polymerase IV is encoded by the POLX gene and is a probable homolog of mammalian DNA polymerase beta.

Published

1993

7. The isolated 48,000-dalton subunit of yeast DNA primase is sufficient for RNA primer synthesis.

Author

Santocanale C, Foiani M, Lucchini G, and Plevani P

Subjects

Antibodies, Monoclonal, Chromatography, Affinity, DNA Polymerase II isolation & purification, DNA Polymerase II metabolism, DNA Primase, Electrophoresis, Polyacrylamide Gel, Macromolecular Substances, Molecular Weight, Neutralization Tests, RNA Nucleotidyltransferases metabolism, RNA biosynthesis, RNA Nucleotidyltransferases isolation & purification, Saccharomyces cerevisiae enzymology

Abstract

The monoclonal antibody (mAb) 21A6, which specifically inhibits yeast DNA primase activity, has been used to verify whether only one of the two polypeptides of heterodimeric DNA primase (48 and 58 kDa) was responsible for DNA primase function in vitro. Immunoaffinity chromatography of a crude extract from cells of Saccharomyces cerevisiae on a mAb 21A6 protein A-Sepharose 6B column allowed the purification of the p48 primase polypeptide in an isolated form. This polypeptide was not derived through the dissociation of the four-subunit DNA polymerase alpha-primase complex, which can be purified from the same extract by affinity chromatography with a mAb recognizing the DNA polymerase alpha polypeptide. Therefore, free p48 was already present in the yeast extract and, possibly, within the cell. Isolated p48, devoid of any detectable p58 subunit, was sufficient for RNA primer synthesis, although free primase appeared to extend RNA primer-monomers to primer-multimers less efficiently. Primase activity associated with free p48 was highly unstable, indicating that although p48 bears the catalytic site, its association with the other polypeptides of the polymerase-primase complex plays an important role in stabilizing enzyme activity.

Published

1993

8. Polypeptide structure of DNA polymerase I from Saccharomyces cerevisiae.

Author

Badaracco G, Capucci L, Plevani P, and Chang LM

Subjects

Aphidicolin, Centrifugation, Density Gradient, Diterpenes pharmacology, Electrophoresis, Polyacrylamide Gel, Molecular Weight, Protein Denaturation, DNA Polymerase II analysis, DNA-Directed DNA Polymerase analysis, Saccharomyces cerevisiae enzymology

Abstract

DNA polymerase I of the yeast Saccharomyces cerevisiae has been purified to near homogeneity. The enzyme sediments under high salt conditions as a band at 7.4 S and two polypeptides of Mr = 140,000 and 110,000 are resolved by polyacrylamide gel electrophoresis in the presence of sodium dodecyl sulfate. Both polypeptides react with rabbit anti-yeast DNA polymerase I serum and can be shown to be enzymatically active by renaturation in situ after electrophoresis on polyacrylamide gels in the presence of sodium dodecyl sulfate. This high molecular weight form of yeast DNA polymerase I is very sensitive to inhibition by aphidicolin. The biochemical properties of the enzyme and inhibitors that may aid in distinguishing yeast DNA polymerases I and II are also described.

Published

1983

9. Purification and characterization of yeast topoisomerase I.

Author

Badaracco G, Plevani P, Ruyechan WT, and Chang LM

Subjects

DNA Topoisomerases, Type I metabolism, Kinetics, Microscopy, Electron, Molecular Weight, Substrate Specificity, DNA Topoisomerases, Type I isolation & purification, Saccharomyces cerevisiae enzymology

Abstract

Yeast topoisomerase I (Mr = 76,000) has been purified to 80% homogeneity using a combination of ion exchange, gel filtration, and DNA-cellulose chromatography. The enzyme was characterized with respect to its ability to relax supercoiled DNA and to catenate nicked circular DNA. Yeast topoisomerase I will remove both positive and negative turns in DNA supercoils in the absence of ATP and magnesium ion. The products of the catenating activity of the enzyme were examined on agarose gels and in the electron microscope. These analyses indicate that yeast topoisomerase I will generate large catenated DNA networks which appear to rearrange to multimeric linear structures upon long incubation time.

Published

1983

10. Purification and characterization of two forms of DNA-dependent ATPase from yeast.

Author

Plevani P, Badaracco G, and Chang LM

Subjects

Adenosine Triphosphatases isolation & purification, DNA Helicases isolation & purification, DNA Replication, Immunodiffusion, Isoenzymes isolation & purification, Isoenzymes metabolism, Kinetics, Poly T pharmacology, Substrate Specificity, Adenosine Triphosphatases metabolism, DNA Helicases metabolism, Saccharomyces cerevisiae enzymology

Abstract

Two forms of DNA-dependent ATPase activity have been purified from yeast extracts. The two ATPases differ from each other in chromatographic properties and heat stabilities but have similar molecular weight and reaction properties. DNA-dependent ATPase I has been purified to near homogeneity, while DNA-dependent ATPase II is only partially purified. The two ATPases from yeast are related structurally since antiserum raised against ATPase I cross-react against ATPase II. Yeast DNA-dependent ATPase I has a native molecular weight of about 68,000 and consists of a single polypeptide chain. ATPase II also sediments on sucrose gradient as a 68,000-dalton protein. Both yeast DNA-dependent ATPases hydrolyze dNTPs and rNTPs to their corresponding nucleoside diphosphates and orthophosphate, but dATP and ATP are preferred substrates. In addition to nucleoside triphosphates, both enzymes require a divalent cation and a polynucleotide for activity. Single-stranded DNAs and polydeoxynucleotides are the most effective co-substrates for yeast DNA-dependent ATPases. Addition of yeast DNA-dependent ATPases to DNA synthesis system containing yeast DNA polymerases does not significantly stimulate the rate of DNA synthesis.

Published

1980

11. Affinity labeling of the active center and ribonucleoside triphosphate binding site of yeast DNA primase.

Author

Foiani M, Lindner AJ, Hartmann GR, Lucchini G, and Plevani P

Subjects

Binding Sites, DNA Primase, DNA Replication, Models, Molecular, Protein Conformation, Structure-Activity Relationship, Adenosine Triphosphate analogs & derivatives, Adenosine Triphosphate metabolism, Affinity Labels metabolism, RNA Nucleotidyltransferases metabolism, Saccharomyces cerevisiae enzymology

Abstract

A highly selective affinity labeling procedure has been applied to map the active center of DNA primase from the yeast Saccharomyces cerevisiae. Enzyme molecules that have been modified by covalent attachment of benzaldehyde derivatives of adenine nucleotides are autocatalytically labeled by incubation with a radioactive ribonucleoside triphosphate. The affinity labeling of primase requires a template DNA, is not affected by DNase and RNase treatments, but is sensitive to proteinase K. Both the p58 and p48 subunits of yeast DNA primase appear to participate in the formation of the catalytic site of the enzyme, although UV-photocross-linking with [alpha-32P]ATP locates the ribonucleoside triphosphate binding site exclusively on the p48 polypeptide. The fixation of the radioactive product has been carried out also after the enzymatic reaction. Under this condition the RNA primers synthesized by the DNA polymerase-primase complex under uncoupled DNA synthesis conditions are linked to both DNA primase and DNA polymerase. When DNA synthesis is allowed to proceed first, the labeled RNA chains are fixed exclusively to the DNA polymerase polypeptide. These results, in accord with previous data, have been used to propose a model illustrating the interactions and the putative roles of the polypeptides of the DNA polymerase-primase complex.

Published

1989

12. Polypeptide structure of DNA primase from a yeast DNA polymerase-primase complex.

Author

Plevani P, Foiani M, Valsasnini P, Badaracco G, Cheriathundam E, and Chang LM

Subjects

Centrifugation, Density Gradient, Chromatography, Affinity, DNA Primase, Electrophoresis, Polyacrylamide Gel, Poly T metabolism, Protein Conformation, Saccharomyces cerevisiae enzymology, DNA Replication, DNA-Directed DNA Polymerase analysis, RNA Nucleotidyltransferases analysis

Abstract

An immunoaffinity chromatographic procedure was developed to purify DNA polymerase-DNA primase complex from crude soluble extracts of yeast cells. The immunoabsorbent column is made of mouse monoclonal antibody to yeast DNA polymerase I covalently linked to Protein A-Sepharose. Purification of the complex involves binding of the complex to the immunoabsorbent column and elution with concentrated MgCl2 solutions. After rebinding to the monoclonal antibody column free primase activity is selectively eluted with a lower concentration of MgCl2. Polyacrylamide gel electrophoresis in the presence of sodium dodecyl sulfate showed the presence of five major peptides, p180, p140, p74, p58, and p48 in the immunoaffinity-purified DNA polymerase-DNA primase complex. Free primase and free polymerase fractions obtained by fractionation on the immunoabsorbent column were analyzed on activity gels and immunoblots. These analyses showed that p180 and p140 are DNA polymerase peptides. Two polypeptides of 58 and 48 kDa co-fractionated with the free yeast DNA primase. From sucrose gradient analysis we estimate a molecular weight of 110 kDa for the native DNA primase.

Published

1985

13. DNA polymerase I and DNA primase complex in yeast.

Author

Plevani P, Badaracco G, Augl C, and Chang LM

Subjects

Animals, Centrifugation, Density Gradient, DNA Primase, DNA Replication, Mice, Osmolar Concentration, Poly T biosynthesis, Rabbits, DNA Polymerase I metabolism, Multienzyme Complexes metabolism, RNA Nucleotidyltransferases metabolism, Saccharomyces cerevisiae enzymology

Abstract

Chromatographic analysis of poly(dT) replication activity in fresh yeast extracts showed that the activities required co-fractionate with the yeast DNA polymerase I. Since poly(dT) replication requires both a primase and a DNA polymerase, the results of the fractionation studies suggest that these two enzymes might exist as a complex in the yeast extract. Sucrose gradient analysis of concentrated purified yeast DNA polymerase I preparations demonstrates that the yeast DNA polymerase I does sediment as a complex with DNA primase activity. Two DNA polymerase I peptides estimated at 78,000 and 140,000 Da were found in the complex that were absent from the primase-free DNA polymerase fraction. Rabbit anti-yeast DNA polymerase I antibody inhibits DNA polymerase I but not DNA primase although rabbit antibodies are shown to remove DNA primase activity from solution by binding to the complex. Mouse monoclonal antibody to yeast DNA polymerase I binds to free yeast DNA polymerase I as well as the complex, but not to the free DNA primase activity. These results suggest that these two activities exist as a complex and reside on the different polypeptides. Replication of poly(dT) and single-stranded circular phage DNA by yeast DNA polymerase I and primase requires ATP and dNTPs. The size of the primer produced is 8 to 9 nucleotides in the presence of dNTPs and somewhat larger in the absence of dNTPs. Aphidicolin, an inhibitor of yeast DNA polymerase I, is not inhibitory to the yeast DNA primase activity. The primase activity is inhibited by adenosine 5'-(3-thio)tri-phosphate but not by alpha-amanitin. The association of yeast DNA polymerase I and yeast DNA primase can be demonstrated directly by isolation of the complex on a column containing yeast DNA polymerase I mouse monoclonal antibody covalently linked to Protein A-Sepharose. Both DNA polymerase I and DNA primase activities are retained by the column and can be eluted with 3.5 M MgCl2. Part of the primase activity can be dissociated from DNA polymerase on the column with 1 M MgCl2 and this free primase activity can be detected as poly(dT) replication activity in the presence of Escherichia coli polymerase I.

Published

1984

14. Proteolytic degradation of calf thymus terminal deoxynucleotidyl transferase.

Author

Chang LM, Plevani P, and Bollum FJ

Subjects

Animals, Cattle, DNA Nucleotidylexotransferase metabolism, Electrophoresis, Polyacrylamide Gel, Enzyme Activation, Molecular Weight, Protein Denaturation, DNA Nucleotidylexotransferase isolation & purification, DNA Nucleotidyltransferases isolation & purification, Thymus Gland enzymology, Trypsin pharmacology

Abstract

A high molecular weight preparation of terminal transferase containing 58,000- and 44,000-dalton peptides has been purified from calf thymus glands. The relationship of these terminal transferase peptides to the low molecular weight form was established with an immunoblot procedure using rabbit antibody directed against the homogeneous calf thymus low molecular weight terminal transferase (32,000 daltons). The 58,000- and 44,000-dalton enzyme species are each shown to be enzymatically active by renaturation in situ after electrophoresis on polyacrylamide gel in the presence of sodium dodecyl sulfate. These results suggest that the homogeneous terminal transferase previously described is derived from the higher molecular weight species by proteolysis during fractionation. Controlled degradation of the high molecular weight calf thymus terminal transferase with trypsin produces fully active enzyme containing alpha- and beta-peptides similar to those found in the 32,000-dalton species. Isoelectric focusing experiments show a decrease of isoelectric pH of the enzyme with proteolysis.

Published

1982