Your search keyword '"Piatti, S."' showing total 97 results

1. Genetic Control of the DNA Polymerase α-Primase complex in the Yeast Saccharomyces cerevisiae

Author

Plevani, P., Foiani, M., Francesconi, S., Pizzagalli, A., Santocanale, C., Muzi, M. Falconi, Piatti, S., Piseri, A., Derossi, D., Longhese, M. P., Locati, F., Tazzi, R., Lucchini, G., Hughes, Patrick, editor, Fanning, Ellen, editor, and Kohiyama, Masamichi, editor

Published

1992

2. Role of the kinetochore protein Ndc10 in mitotic checkpoint activation in Saccharomyces cerevisiae

Author

Fraschini, R., Beretta, A., Lucchini, G., and Piatti, S.

Published

2001

3. Videoinsight® art for care

Author

Russo, R. L., Giovannelli, G., Giunta, T., Piatti, S., ZAFFAGNINI, STEFANO, ROBERTI DI SARSINA, TOMMASO, Russo, R.L., Zaffagnini, Stefano, Roberti di Sarsina, T., Giovannelli, G., Giunta, T., and Piatti, S.

Subjects

Psychology (all)

Abstract

The corporal and psychic dimensions are deeply combined and reciprocally conditioned in the body unit. The improvement of psychological status influences the somatic one. The role that psychology has to play in understanding and improving the recovery after mental or physical stress is really interesting and needs more attention in order to treat the patient as a global unit and not focusing on a single aspect of mental or physical recovery only, in order to promote patient global wellness. The Videoinsight® is a psychological enhancing method that involves the vision of contemporary art videos, selected according to their content and transformative potential, with the intent to catalyze the “insight” psychological experience and to facilitate the process that allows the individual to stimulate sensations, emotions, learning, psycho-aptitude orientation, actions and changes. Insight in psychoanalysis means the capacity to understand the interior psychic pathway and consequently to allow therapeutic transformation. These artistic videos contain a significant psycho-diagnostic and psychotherapeutic meaning that can help treat the psychological and psychosomatic disabilities that are frequently observed after mental or corporal stress, increasing the resistance capacity and improving the cognitive and behavioral power during the recovery process. The Videoinsight® Method has been verified in the clinical, psychological and medical setting: • for the Diagnosis of the Structure and Operation of Personality: the art video reveals similarities with the Projective Rorschach Test; • for the Analysis of Request for Psychological Support and for the Discovery of the Capacity of Trust, Cooperation, and Motivation in the relationship with the Others; • for the Prevention of Psychological Discomfort related to the Crisis of Development (adolescent, post traumatic stress, psychosomatic stress and the one related to physical illness and the aging process); • for the Orientation and Enabling of Attitudes and Functional Talents in support of the healthy personality. They are critical for containment of the weak and dysfunctional parts, supporting a creative and harmonious mental and physical development of the person; • for the Rehabilitation of Psychological Resources following the impairment caused by a physical illness, a trauma, a stress that turns the vulnerability into crisis or into evolutionary stalemate. In particular, in two prospective randomized studies, the Videoinsight® Method was able to accelerate recovery after Anterior Cruciate Ligament reconstruction and also after Total Knee Arthroplasty with improvement of subjective functional score and psychological scales. These results highlight how images are powerful and have a tremendous impact on the personality. Specific images can be very powerful and are able to produce “insight." In this chapter we will describe the Videoinsight® Method and its applications in the psychotherapeutic setting, in distress prevention and in promoting well-being and early recovery during rehabilitation following surgery.

Published

2016

4. The beta4 integrin interactor p27(BBP/eIF6) is an essential nuclear matrix protein involved in 60S ribosomal subunit assembly

Author

Sanvito, F, Piatti, S, Lucchini, G, Marchisio, PC, Biffo, S., VILLA, ANTONELLO, BOSSI, MARIO, Sanvito, F, Piatti, S, Villa, A, Bossi, M, Lucchini, G, Marchisio, P, and Biffo, S

Subjects

Base Sequence, Sequence Homology, Amino Acid, DNA Primer, Molecular Sequence Data, Antigens, Nuclear, Saccharomyces cerevisiae, Recombinant Protein, Mitosi, Immunohistochemistry, Ribosome, Ribosomal Protein, Intermediate Filament Protein, Microscopy, Electron, Cell Nucleolu, Eukaryotic Initiation Factor, Phosphoprotein, Amino Acid Sequence, Carrier Protein, Fluorescent Antibody Technique, Indirect, Saccharomyces cerevisiae Protein, Human, Nuclear Protein

Abstract

p27(BBP/eIF6) is an evolutionarily conserved protein that was originally identified as p27(BBP), an interactor of the cytoplasmic domain of integrin beta4 and, independently, as the putative translation initiation factor eIF6. To establish the in vivo function of p27(BBP/eIF6), its topographical distribution was investigated in mammalian cells and the effects of disrupting the corresponding gene was studied in the budding yeast, Saccharomyces cerevisiae. In epithelial cells containing beta4 integrin, p27(BBP/eIF6) is present in the cytoplasm and enriched at hemidesmosomes with a pattern similar to that of beta4 integrin. Surprisingly, in the absence and in the presence of the beta4 integrin subunit, p27(BBP/eIF6) is in the nucleolus and associated with the nuclear matrix. Deletion of the IIH S. cerevisiae gene, encoding the yeast p27(BBP/eIF6) homologue, is lethal, and depletion of the corresponding gene product is associated with a dramatic decrease of the level of free ribosomal 60S subunit. Furthermore, human p27(BBP/eIF6) can rescue the lethal effect of the iihDelta yeast mutation. The data obtained in vivo suggest an evolutionarily conserved function of p27(BBP/eIF6) in ribosome biogenesis or assembly rather than in translation. A further function related to the beta4 integrin subunit may have evolved specifically in higher eukaryotic cells.

Published

1999

5. Budding yeast Dma proteins control septin dynamics and the spindle position checkpoint by promoting the recruitment of the Elm1 kinase to the bud neck

Author

Merlini, L, Fraschini, R, Boettcher, B, Barral, Y, Lucchini, G, Piatti, S, MERLINI, LAURA, FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Merlini, L, Fraschini, R, Boettcher, B, Barral, Y, Lucchini, G, Piatti, S, MERLINI, LAURA, FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

The first step towards cytokinesis in budding yeast is the assembly of a septin ring at the future site of bud emergence. Integrity of this ring is crucial for cytokinesis, proper spindle positioning, and the spindle position checkpoint (SPOC). This checkpoint delays mitotic exit and cytokinesis as long as the anaphase spindle does not properly align with the division axis. SPOC signalling requires the Kin4 protein kinase and the Kin4-regulating Elm1 kinase, which also controls septin dynamics. Here, we show that the two redundant ubiquitin-ligases Dma1 and Dma2 control septin dynamics and the SPOC by promoting the efficient recruitment of Elm1 to the bud neck. Indeed, dma1 dma2 mutant cells show reduced levels of Elm1 at the bud neck and Elm1-dependent activation of Kin4. Artificial recruitment of Elm1 to the bud neck of the same cells is sufficient to re-establish a normal septin ring, proper spindle positioning, and a proficient SPOC response in dma1 dma2 cells. Altogether, our data indicate that septin dynamics and SPOC function are intimately linked and support the idea that integrity of the bud neck is crucial for SPOC signalling

Published

2012

6. The RSC chromatin-remodelling complex influences mitotic exit and adaptation to the spindle assembly checkpoint by controlling Cdc14 phosphatase

Author

Rossio, V, Galati, E, Ferrari, M, Pellicioli, A, Sutani, T, Shirahige, K, Lucchini, G, Piatti, S, ROSSIO, VALENTINA, GALATI, ELENA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Rossio, V, Galati, E, Ferrari, M, Pellicioli, A, Sutani, T, Shirahige, K, Lucchini, G, Piatti, S, ROSSIO, VALENTINA, GALATI, ELENA, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

Upon prolonged activation of the spindle assembly checkpoint (SAC) cells escape from mitosis through a mechanism called adaptation or mitotic slippage, which is thought to underlie the resistance of cancer cells to anti-mitotic drugs. We show that this mechanism in budding yeast this mechanism depends on known essential and non-essential regulators of mitotic exit, such as the FEAR pathway for the release of the Cdc14 phosphatase from the nucleolus in early anaphase. Moreover, the RSC chromatin-remodelling complex bound to its accessory subunit Rsc2 is involved in this process as a novel component of the FEAR pathway. We show that Rsc2 interacts physically with the polo kinase Cdc5, a major regulator of Cdc14, and is required for timely phosphorylation of the Cdc14 inhibitor Net1, which is important to free Cdc14 in the active form. Altogether, our data suggest that fine tuning regulators of mitotic exit play an important rolehave important functions during in mitotic progression ofin cells treated with microtubule poisons, and might be promising targets for cancer treatment.

Published

2010

7. Cdc14 inhibition by the spindle assembly checkpoint prevents unscheduled centrosome separation in budding yeast

Author

Chiroli, E, Rancati, G, Catusi, I, Lucchini, G, Piatti, S, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Chiroli, E, Rancati, G, Catusi, I, Lucchini, G, Piatti, S, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

The spindle assembly checkpoint (SAC) is an evolutionarily conserved surveillance mechanism that delays anaphase onset and mitotic exit in response to the lack of kinetochore attachment. Target of the SAC is the E3 ubiquitin ligase anaphase promoting complex (APC) bound to its Cdc20 activator. The Cdc20/APC complex is in turn required for sister chromatid separation and mitotic exit through ubiquitin-mediated proteolysis of securin, thus relieving inhibition of separase that unties sister chromatids. Separase is also involved in the FEAR (Cdc-fourteen early anaphase release) pathway of nucleolar release and activation of the Cdc14 phosphatase, which regulates several microtubule-linked processes at the metaphase/anaphase transition and also drives mitotic exit. Here we report that the SAC prevents separation of microtubule-organizing centers (spindle pole bodies, SPBs) when spindle assembly is defective. Under these circumstances, failure of SAC activation causes unscheduled SPB separation, which requires Cdc20/APC, the FEAR pathway, cytoplasmic dynein and the actin cytoskeleton. We propose that, besides inhibiting sister chromatid separation, the SAC preserves the accurate transmission of chromosomes also by preventing SPBs to migrate far apart until the conditions to assemble a bipolar spindle are satisfied.

Published

2009

8. The spindle position checkpoint: how to deal with spindle misalignment during asymmetric cell division in budding yeast

Author

Fraschini, R, Venturetti, M, Chiroli, E, Piatti, S, FRASCHINI, ROBERTA, PIATTI, SIMONETTA, Fraschini, R, Venturetti, M, Chiroli, E, Piatti, S, FRASCHINI, ROBERTA, and PIATTI, SIMONETTA

Abstract

During asymmetric cell division, spindle positioning is critical to ensure the unequal segregation of polarity factors and generate daughter cells with different sizes or fates. In budding yeast the boundary between mother and daughter cell resides at the bud neck, where cytokinesis takes place at the end of the cell cycle. Since budding and bud neck formation occur much earlier than bipolar spindle formation, spindle positioning is a finely regulated process. A surveillance device called the SPOC (spindle position checkpoint) oversees this process and delays mitotic exit and cytokinesis until the spindle is properly oriented along the division axis, thus ensuring genome stability.

Published

2008

9. The budding yeast PP2A(Cdc55) protein phosphatase prevents the onset of anaphase in response to morphogenetic defects

Author

Chiroli, E, Rossio, V, Lucchini, G, Piatti, S, ROSSIO, VALENTINA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Chiroli, E, Rossio, V, Lucchini, G, Piatti, S, ROSSIO, VALENTINA, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

Faithful chromosome transmission requires establishment of sister chromatid cohesion during S phase, followed by its removal at anaphase onset. Sister chromatids are tethered together by cohesin, which is displaced from chromosomes through cleavage of its Mcd1 subunit by the separase protease. Separase is in turn inhibited, up to this moment, by securin. Budding yeast cells respond to morphogenetic defects by a transient arrest in G2 with high securin levels and unseparated chromatids. We show that neither securin elimination nor forced cohesin cleavage is sufficient for anaphase in these conditions, suggesting that other factors contribute to cohesion maintainance in G2. We found that the protein phosphatase PP2A bound to its regulatory subunit Cdc55 plays a key role in this process, uncovering a new function for PP2A(Cdc55) in controlling a noncanonical pathway of chromatid cohesion removal

Published

2007

10. Comment on 'A centrosome-independent role for gamma-TuRC proteins in the spindle assembly checkpoint'

Author

Taylor, S, Hardwick, K, Sawin, K, Biggins, S, Piatti, S, Khodjakov, A, Rieder, C, Salmon, E, Musacchio, A, Taylor, SS, Hardwick, KG, Sawin, KE, Rieder, CL, Salmon, ED, Musacchio, A., PIATTI, SIMONETTA, Taylor, S, Hardwick, K, Sawin, K, Biggins, S, Piatti, S, Khodjakov, A, Rieder, C, Salmon, E, Musacchio, A, Taylor, SS, Hardwick, KG, Sawin, KE, Rieder, CL, Salmon, ED, Musacchio, A., and PIATTI, SIMONETTA

Abstract

Müller et al. (Reports, 27 October 2006, p. 654) showed that inhibition of the gamma-tubulin ring complex (gamma-TuRC) activates the spindle assembly checkpoint (SAC), which led them to suggest that gamma-TuRC proteins play molecular roles in SAC activation. Because gamma-TuRC inhibition leads to pleiotropic spindle defects, which are well known to activate kinetochore-derived checkpoint signaling, we believe that this conclusion is premature.

Published

2007

11. Disappearance of the budding yeast Bub2-Bfa1 complex from the mother-bound spindle pole contributes to mitotic exit

Author

Fraschini, R, D'Ambrosio, C, Venturetti, M, Lucchini, G, Piatti, S, FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Fraschini, R, D'Ambrosio, C, Venturetti, M, Lucchini, G, Piatti, S, FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

Budding yeast spindle position checkpoint is engaged by misoriented spindles and prevents mitotic exit by inhibiting the G protein Tem1 through the GTPase-activating protein (GAP) Bub2/Bfa1. Bub2 and Bfa1 are found on both duplicated spindle pole bodies until anaphase onset, when they disappear from the mother-bound spindle pole under unperturbed conditions. In contrast, when spindles are misoriented they remain symmetrically localized at both SPBs. Thus, symmetric localization of Bub2/Bfa1 might lead to inhibition of Tem1, which is also present at SPBs. Consistent with this hypothesis, we show that a Bub2 version symmetrically localized on both SPBs throughout the cell cycle prevents mitotic exit in mutant backgrounds that partially impair it. This effect is Bfa1 dependent and can be suppressed by high Tem1 levels. Bub2 removal from the mother-bound SPB requires its GAP activity, which in contrast appears to be dispensable for Tem1 inhibition. Moreover, it correlates with the passage of one spindle pole through the bud neck because it needs septin ring formation and bud neck kinases. © The Rockefeller University Press.

Published

2006

12. Alfalfa Mob1-like proteins are involved in cell proliferation and are localized in the cell division plane during cytokinesis

Author

Citterio, S, Piatti, S, Albertini, E, Aina, R, Varotto, S, Barcaccia, G, CITTERIO, SANDRA, PIATTI, SIMONETTA, Barcaccia, G., Citterio, S, Piatti, S, Albertini, E, Aina, R, Varotto, S, Barcaccia, G, CITTERIO, SANDRA, PIATTI, SIMONETTA, and Barcaccia, G.

Abstract

Mps-one-binder (Mob) proteins play a crucial role in yeast cytokinesis. After cloning two Mob1-like genes, MsMob1-A and MsMob1-B from alfalfa (Medicago sativa L.) we show that, although they are constitutively expressed in roots, stems, leaves, flowers and pods, their transcripts and proteins are mostly produced in actively proliferating tissues. A polyclonal antibody specifically raised against MsMob1 proteins was used for immunolocalization studies in synchronized root tip cells. The subcellular localization ofMsMob1-like proteins is demonstrated to be cell cycle-regulated. Cytoplasmic localization is faint and diffused during G1 and S. It becomes concentrated in punctuate and fibrillar structures in G2 as well as M phase. At the stage of cytokinesis, the protein is found at the emerging cell plate marking the progressive formation of the septum. Mob1 proteins partially co-localize with microtubules structures functionally related to the spindles and important for cytokinesis in eukaryotic cells. The MsMob1 expression cannot rescue the lethality of the yeast mob1 mutant, suggesting that interaction of Mob1 proteins with their effectors may be speciesspecific. Localization of Mob1 proteins in the inner layer of the root cap indicates an additional function for this class of proteins in plants, which is likely related to the onset of programmed cell death.

Published

2006

13. The spindle position checkpoint in budding yeast: the motherly care of MEN.

Author

Piatti, S, Venturetti, M, Chiroli, E, Fraschini, R, PIATTI, SIMONETTA, FRASCHINI, ROBERTA, Piatti, S, Venturetti, M, Chiroli, E, Fraschini, R, PIATTI, SIMONETTA, and FRASCHINI, ROBERTA

Abstract

Mitotic exit and cytokinesis must be tightly coupled to nuclear division both in time and space in order to preserve genome stability and to ensure that daughter cells inherit the right set of chromosomes after cell division. This is achieved in budding yeast through control over a signal transduction cascade, the mitotic exit network (MEN), which is required for mitotic CDK inactivation in telophase and for cytokinesis. Current models of MEN activation emphasize on the bud as the place where most control is exerted. This review focuses on recent data that instead point to the mother cell as being the residence of key regulators of late mitotic events.

Published

2006

14. The Saccharomyces cerevisiae 14-3-3 proteins are required for the G 1/S transition, actin cytoskeleton organization and cell wall integrity

Author

Lottersberger, F, Panza, A, Lucchini, G, Piatti, S, Longhese, M, LUCCHINI, GIOVANNA, LONGHESE, MARIA PIA, Lottersberger, F, Panza, A, Lucchini, G, Piatti, S, Longhese, M, LUCCHINI, GIOVANNA, and LONGHESE, MARIA PIA

Abstract

14-3-3 proteins are highly conserved polypeptides that participate in many biological processes by binding phosphorylated target proteins. The Saccharomyces cerevisiae BMH1 and BMH2 genes, whose concomitant deletion is lethal, encode two functionally redundant 14-3-3 isoforms. To gain insights into the essential function(s) shared by these proteins, we searched for high-dosage suppressors of the growth defects of temperature-sensitive bmh mutants. Both the protein kinase C1 (Pkc1) and its upstream regulators Wsc2 and Mid2 were found to act as high dosage suppressors of bmh mutants' temperature sensitivity, indicating a functional interaction between 14-3-3 and Pkc1. Consistent with a role of 14-3-3 proteins in Pkc1-dependent cellular processes, shift to the restrictive temperature of bmh mutants severely impaired initiation of DNA replication, polarization of the actin cytoskeleton, and budding, as well as cell wall integrity. Because Pkc1 acts in concert with the Swi4-Swi6 (SBF) transcriptional activator to control all these processes, the defective G(1)/S transition of bmh mutants might be linked to impaired SBF activity. Indeed, the levels of the G(1) cyclin CLN2 transcripts, which are positively regulated by SBF, were dramatically reduced in bmh mutants. Remarkably, budding and DNA replication defects of bmh mutants were suppressed by CLN2 expression from an SBF-independent promoter, suggesting that 14-3-3 proteins might contribute to regulating the late G(1) transcriptional program.

Published

2006

15. Mad3/BubR1 phosphorylation during spindle checkpoint activation depends on both polo and aurora kinases in budding yeast

Author

Rancati, G, Crispo, V, Lucchini, G, Piatti, S, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Rancati, G, Crispo, V, Lucchini, G, Piatti, S, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

During mitosis the spindle assembly checkpoint ( SAC) delays the onset of anaphase and mitotic exit until all chromosomes are bipolarly attached to spindle fibers. Both lack of attachment due to spindle/kinetochore defects and lack of tension across kinetochores generate the "wait anaphase" signal transmitted by the SAC, which involves the evolutionarily conserved Mad1, Mad2, Mad3/BubR1, Bub1, Bub3 and Mps1 proteins, and inhibits the activity of the ubiquitin ligase Cdc20/APC, that promotes both sister chromatid dissociation in anaphase and mitotic exit. In particular, Mad3/BubR1 is directly implicated, together with Mad2, in Cdc20 inactivation in both human and yeast cells, suggesting that its activity is likely finely regulated. We show that budding yeast Mad3, like its human orthologue BubR1, is a phosphoprotein that is hyperphosphorylated during mitosis and when SAC activation is triggered by microtubule depolymerizing agents, kinetochore defects or lack of kinetochore tension. In vivo Mad3 phosphorylation depends on the Polo kinase Cdc5 and, to a minor extent, the Aurora B kinase Ipl1. Accordingly, replacing with alanines five serine residues belonging to Polo kinase-dependent putative phosphorylation sites dramatically reduces Mad3 phosphorylation, suggesting that Mad3 is likely an in vivo target of Cdc5

Published

2005

16. Sen34p depletion blocks tRNA splicing in vivo and delays rRNA processing

Author

Volta, V, Ceci, M, Emery, B, Bachi, A, Petfalski, E, Tollervey, D, Linder, P, Marchisio, P, Piatti, S, Biffo, S, Marchisio, PC, Biffo, S., PIATTI, SIMONETTA, Volta, V, Ceci, M, Emery, B, Bachi, A, Petfalski, E, Tollervey, D, Linder, P, Marchisio, P, Piatti, S, Biffo, S, Marchisio, PC, Biffo, S., and PIATTI, SIMONETTA

Abstract

Tif6p (eIF6) is necessary for 60S biogenesis, rRNA maturation and must be released from 60S to permit 80S assembly and translation. We characterized Tif6p interactors. Tif6p is mostly on 66S-60S pre-ribosomes partly free. Tif6p complex(es) contain nucleo-ribosomal factors and Ase1p. Surprisingly, Tif6p particle contains the low-abundance endonuclease Sen34p. We analyzed Sen34p role on rRNA/tRNA synthesis, in vivo. Sen34p depletion impairs tRNA splicing and causes unexpected 80S accumulation. Accordingly, Sen34p overexpression causes 80S decrease and increased polysomes which suggest increased translational efficiency. With delayed kinetics, Sen34p depletion impairs rRNA processing. We conclude that Sen34p is absolutely required for tRNA splicing and that it is a rate-limiting element for efficient translation. Finally, we confirm that Tif6p accompanies 27S pre-rRNA maturation to 25S rRNA and we suggest that Sen34p endonuclease in Tif6p complex may affect also rRNA maturation. (c) 2005 Elsevier Inc. All rights reserved.

Published

2005

17. Budding yeast PAK kinases regulate mitotic exit by two different mechanisms

Author

Chiroli, E, Fraschini, R, Beretta, A, Tonelli, M, Lucchini, G, Piatti, S, FRASCHINI, ROBERTA, TONELLI, MARIAGRAZIA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Chiroli, E, Fraschini, R, Beretta, A, Tonelli, M, Lucchini, G, Piatti, S, FRASCHINI, ROBERTA, TONELLI, MARIAGRAZIA, LUCCHINI, GIOVANNA, and PIATTI, SIMONETTA

Abstract

We report the characterization of the dominant-negative CLA4t allele of the budding yeast CLA4 gene, encoding a member of the PAK family of protein kinases, which, together with its homologue STE20, plays an essential role in promoting budding and cytokinesis. Overproduction of the Cla4t protein likely inhibits both endogenous Cla4 and Ste20 and causes a delay in the onset of anaphase that correlates with inactivation of Cdc20/APC-dependent proteolysis of both the cyclinB Clb2 and securin. Although the precise mechanism of APC inhibition by Cla4t remains to be elucidated, our results suggest that Cla4 and Ste20 may regulate the first wave of cyclinB proteolysis mediated by Cdc20/APC, which has been shown to be crucial for activation of the Mitotic Exit Network. We show that the Cdk1-inhibitory kinase Swe1 is required for the Cla4t-dependent delay in cell cycle progression, suggesting that it might be required to prevent full Cdc20/APC and MEN activation. In addition, inhibition of PAK kinases by Cla4t prevents mitotic exit also by a Swe1-independent mechanism impinging directly on the MEN activator Tem1

Published

2003

18. Correct spindle elongation at the metaphase/anaphase transition is an APC-dependent event in budding yeast

Author

Severin, F, Hyman, A, Piatti, S, Hyman, AA, Severin, F, Hyman, A, Piatti, S, and Hyman, AA

Abstract

At the metaphase to anaphase transition, chromosome segregation is initiated by the splitting of sister chromatids. Subsequently, spindles elongate, separating the sister chromosomes into two sets. Here, we investigate the cell cycle requirements for spindle elongation in budding yeast using mutants affecting sister chromatid cohesion or DNA replication. We show that separation of sister chromatids is not sufficient for proper spindle integrity during elongation. Rather, successful spindle elongation and stability require both sister chromatid separation and anaphase-promoting complex activation. Spindle integrity during elongation is dependent on proteolysis of the securin Pds1 but not on the activity of the separase Esp1. Our data suggest that stabilization of the elongating spindle at the metaphase to anaphase transition involves Pds1-dependent targets other than Esp1.

Published

2001

19. Activation of S-phase-promoting CDKs in late G1 defines a "point of no return" after which Cdc6 synthesis cannot promote DNA replication in yeast.

Author

Piatti, S, primary, Böhm, T, additional, Cocker, J H, additional, Diffley, J F, additional, and Nasmyth, K, additional

Published

1996

20. Cdc6 is an unstable protein whose de novo synthesis in G1 is important for the onset of S phase and for preventing a ‘reductional’ anaphase in the budding yeast Saccharomyces cerevisiae.

Author

Piatti, S., primary, Lengauer, C., additional, and Nasmyth, K., additional

Published

1995

21. The yeast DNA polymerase-primase complex: Genes and proteins

Author

Plevani, P., Foiani, M., Muzi Falconi, M, Pizzagalli, A., Santocanale, C., Francesconi, S., Valsasnini, P., Comedini, A., Piatti, S., Lucchini, G., Falconi, M.Muzi, and Università degli Studi di Milano [Milano] (UNIMI)

Subjects

DNA polymerase, [SDV]Life Sciences [q-bio], MESH: RNA Nucleotidyltransferases, MESH: DNA Replication, MESH: Amino Acid Sequence, DNA-Directed DNA Polymerase, Biochemistry, DNA polymerase delta, MESH: Structure-Activity Relationship, Structural Biology, MESH: DNA-Directed DNA Polymerase, Polymerase, Immunoassay, Genetics, 0303 health sciences, DNA clamp, biology, 030302 biochemistry & molecular biology, RNA Nucleotidyltransferases, MESH: Saccharomyces cerevisiae, MESH: DNA Primase, Electrophoresis, Polyacrylamide Gel, Primase, MESH: Immunoassay, DNA Replication, MESH: Mutation, DNA polymerase II, Biophysics, DNA Primase, Saccharomyces cerevisiae, MESH: Sequence Homology, Nucleic Acid, Structure-Activity Relationship, 03 medical and health sciences, Sequence Homology, Nucleic Acid, MESH: DNA Polymerase II, Humans, Amino Acid Sequence, MESH: DNA Polymerase I, 030304 developmental biology, MESH: Humans, Binding Sites, DNA replication, DNA Polymerase II, DNA Polymerase I, MESH: Binding Sites, Mutation, biology.protein, DNA polymerase I, MESH: Electrophoresis, Polyacrylamide Gel

Abstract

International audience; The yeast DNA polymerase-primase complex is composed of four polypeptides designated p180, p74, p58 and p48. All the genes coding for these polypeptides have now been cloned. By protein sequence comparison we found that yeast DNA polymerase I (alpha) shares three major regions of homology with several DNA polymerases. A fourth region, called region P, is conserved in yeast and human DNA polymerase alpha. The site of a temperature-sensitive mutation in the POL1 gene which causes decreased stability of the polymerase-primase complex has been sequenced and falls in this region. We hypothesize that region P is important for protein-protein interactions. Highly selective biochemical methods might be similarly important to distinguish functional domains in the polymerase-primase complex. An autocatalytic affinity labeling procedure has been applied to map the active center of yeast DNA primase. From this approach we conclude that both primase subunits (p48 and p58) participate in the formation of the catalytic site of the enzyme.

Published

1988

22. Cdc14 Inhibition by the Spindle Assembly Checkpoint Prevents Unscheduled Centrosome Separation in Budding Yeast

Author

Elena Chiroli, Ilaria Catusi, Giovanna Lucchini, Giulia Rancati, Simonetta Piatti, Chiroli, E, Rancati, G, Catusi, I, Lucchini, G, and Piatti, S

Subjects

Saccharomyces cerevisiae Proteins, Cell Cycle Proteins, BIO/18 - GENETICA, Spindle Apparatus, CDC20, Protein Serine-Threonine Kinases, Biology, Microtubules, Anaphase-Promoting Complex-Cyclosome, Endopeptidases, Molecular Biology, Alleles, Separase, Anaphase, Centrosome, Kinetochore, Dyneins, Ubiquitin-Protein Ligase Complexes, Articles, Cell Biology, Actins, Spindle apparatus, Cell biology, spindle assembly checkpoint, Cdc14, spindle pole body, sister chromatid separation, genome integrity, Spindle checkpoint, Mitotic exit, Mutation, Saccharomycetales, Protein Tyrosine Phosphatases, Anaphase-promoting complex

Abstract

The spindle assembly checkpoint (SAC) is an evolutionarily conserved surveillance mechanism that delays anaphase onset and mitotic exit in response to the lack of kinetochore attachment. The target of the SAC is the E3 ubiquitin ligase anaphase-promoting complex (APC) bound to its Cdc20 activator. The Cdc20/APC complex is in turn required for sister chromatid separation and mitotic exit through ubiquitin-mediated proteolysis of securin, thus relieving inhibition of separase that unties sister chromatids. Separase is also involved in the Cdc-fourteen early anaphase release (FEAR) pathway of nucleolar release and activation of the Cdc14 phosphatase, which regulates several microtubule-linked processes at the metaphase/anaphase transition and also drives mitotic exit. Here, we report that the SAC prevents separation of microtubule-organizing centers (spindle pole bodies [SPBs]) when spindle assembly is defective. Under these circumstances, failure of SAC activation causes unscheduled SPB separation, which requires Cdc20/APC, the FEAR pathway, cytoplasmic dynein, and the actin cytoskeleton. We propose that, besides inhibiting sister chromatid separation, the SAC preserves the accurate transmission of chromosomes also by preventing SPBs to migrate far apart until the conditions to assemble a bipolar spindle are satisfied.

Published

2009

23. The budding yeast PP2ACdc55 protein phosphatase prevents the onset of anaphase in response to morphogenetic defects

Author

Simonetta Piatti, Elena Chiroli, Giovanna Lucchini, Valentina Rossio, Chiroli, E, Rossio, V, Lucchini, G, and Piatti, S

Subjects

Saccharomyces cerevisiae Proteins, BIO/18 - GENETICA, Cell Cycle Proteins, Saccharomyces cerevisiae, Chromatids, Biology, Article, Phosphoprotein Phosphatases, Sister chromatids, budding yeast, Protein Phosphatase 2, Research Articles, Anaphase, Cohesin, Nuclear Proteins, Cell Biology, sister chromatid cohesion, PP2A, Cell biology, Securin, Establishment of sister chromatid cohesion, Biochemistry, Chromatid, biological phenomena, cell phenomena, and immunity, Separase, Cytokinesis

Abstract

Faithful chromosome transmission requires establishment of sister chromatid cohesion during S phase, followed by its removal at anaphase onset. Sister chromatids are tethered together by cohesin, which is displaced from chromosomes through cleavage of its Mcd1 subunit by the separase protease. Separase is in turn inhibited, up to this moment, by securin. Budding yeast cells respond to morphogenetic defects by a transient arrest in G2 with high securin levels and unseparated chromatids. We show that neither securin elimination nor forced cohesin cleavage is sufficient for anaphase in these conditions, suggesting that other factors contribute to cohesion maintainance in G2. We find that the protein phosphatase PP2A bound to its regulatory subunit Cdc55 plays a key role in this process, uncovering a new function for PP2ACdc55 in controlling a noncanonical pathway of chromatid cohesion removal.

Published

2007

24. The Saccharomyces cerevisiae 14-3-3 Proteins Are Required for the G1/S Transition, Actin Cytoskeleton Organization and Cell Wall Integrity

Author

Francisca Lottersberger, Giovanna Lucchini, Simonetta Piatti, Andrea Panza, Maria Pia Longhese, Lottersberger, F, Panza, A, Lucchini, G, Piatti, S, and Longhese, M

Subjects

Osmosis, Saccharomyces cerevisiae Proteins, actin cytoskeleton, Genes, Fungal, Saccharomyces cerevisiae, Gene Dosage, S. cerevisiae, BIO/18 - GENETICA, Investigations, Actin cytoskeleton organization, S Phase, Calcium-binding protein, Genetics, DNA, Fungal, Genes, Suppressor, Cytoskeleton, Protein Kinase C, 14-3-3, Membrane Glycoproteins, Base Sequence, biology, Calcium-Binding Proteins, G1 Phase, Intracellular Signaling Peptides and Proteins, Temperature, DNA replication, Membrane Proteins, G1/S transition, biology.organism_classification, Actin cytoskeleton, Actins, Cell biology, 14-3-3 Proteins, Membrane protein, Mutation, cell wall, cell cycle

Abstract

14-3-3 proteins are highly conserved polypeptides that participate in many biological processes by binding phosphorylated target proteins. The Saccharomyces cerevisiae BMH1 and BMH2 genes, whose concomitant deletion is lethal, encode two functionally redundant 14-3-3 isoforms. To gain insights into the essential function(s) shared by these proteins, we searched for high-dosage suppressors of the growth defects of temperature-sensitive bmh mutants. Both the protein kinase C1 (Pkc1) and its upstream regulators Wsc2 and Mid2 were found to act as high dosage suppressors of bmh mutants' temperature sensitivity, indicating a functional interaction between 14-3-3 and Pkc1. Consistent with a role of 14-3-3 proteins in Pkc1-dependent cellular processes, shift to the restrictive temperature of bmh mutants severely impaired initiation of DNA replication, polarization of the actin cytoskeleton, and budding, as well as cell wall integrity. Because Pkc1 acts in concert with the Swi4-Swi6 (SBF) transcriptional activator to control all these processes, the defective G1/S transition of bmh mutants might be linked to impaired SBF activity. Indeed, the levels of the G1 cyclin CLN2 transcripts, which are positively regulated by SBF, were dramatically reduced in bmh mutants. Remarkably, budding and DNA replication defects of bmh mutants were suppressed by CLN2 expression from an SBF-independent promoter, suggesting that 14-3-3 proteins might contribute to regulating the late G1 transcriptional program.

Published

2006

25. Disappearance of the budding yeast Bub2–Bfa1 complex from the mother-bound spindle pole contributes to mitotic exit

Author

Roberta Fraschini, Simonetta Piatti, Claudio D'Ambrosio, Marianna Venturetti, Giovanna Lucchini, Fraschini, R, D'Ambrosio, C, Venturetti, M, Lucchini, G, and Piatti, S

Subjects

Cell cycle checkpoint, Saccharomyces cerevisiae Proteins, Cyclin B, Reviews, Mitosis, Cell Cycle Proteins, Saccharomyces cerevisiae, Spindle Apparatus, Protein Serine-Threonine Kinases, Pheromones, Spindle pole body, Article, Methionine, Gene Expression Regulation, Fungal, CDC2 Protein Kinase, Guanine Nucleotide Exchange Factors, Alleles, Research Articles, Cyclin-Dependent Kinase Inhibitor Proteins, Genes, Dominant, Monomeric GTP-Binding Proteins, Anaphase, biology, Models, Genetic, Comment, GTPase-Activating Proteins, Cell Biology, Protein-Tyrosine Kinases, mitotic exit network, Tem1, spindle position checkpoint, Bub2, cytokinesis, Cyclin-Dependent Kinases, Cell biology, Cytoskeletal Proteins, Septin ring, Mitotic exit, Mutation, Microtubule Proteins, biology.protein, Protein Tyrosine Phosphatases, Protein Kinases, Cytokinesis

Abstract

Budding yeast spindle position checkpoint is engaged by misoriented spindles and prevents mitotic exit by inhibiting the G protein Tem1 through the GTPase-activating protein (GAP) Bub2/Bfa1. Bub2 and Bfa1 are found on both duplicated spindle pole bodies until anaphase onset, when they disappear from the mother-bound spindle pole under unperturbed conditions. In contrast, when spindles are misoriented they remain symmetrically localized at both SPBs. Thus, symmetric localization of Bub2/Bfa1 might lead to inhibition of Tem1, which is also present at SPBs. Consistent with this hypothesis, we show that a Bub2 version symmetrically localized on both SPBs throughout the cell cycle prevents mitotic exit in mutant backgrounds that partially impair it. This effect is Bfa1 dependent and can be suppressed by high Tem1 levels. Bub2 removal from the mother-bound SPB requires its GAP activity, which in contrast appears to be dispensable for Tem1 inhibition. Moreover, it correlates with the passage of one spindle pole through the bud neck because it needs septin ring formation and bud neck kinases. © The Rockefeller University Press.

Published

2006

26. Mad3/BubR1 Phosphorylation during Spindle Checkpoint Activation Depends on both Polo and Aurora Kinases in Budding Yeast

Author

Valentina Crispo, Giulia Rancati, Simonetta Piatti, Giovanna Lucchini, Rancati, G, Crispo, V, Lucchini, G, and Piatti, S

Subjects

Saccharomyces cerevisiae Proteins, Mad2, Mad1, BUB3, Molecular Sequence Data, BIO/18 - GENETICA, Cell Cycle Proteins, Spindle Apparatus, Mad3/BubR1, Protein Serine-Threonine Kinases, Biology, spindle assembly checkpoint, Fungal Proteins, Aurora Kinases, Serine, Polo kinase, Amino Acid Sequence, Phosphorylation, Kinetochores, Aurora kinase, Molecular Biology, Cells, Cultured, Anaphase, mitosi, Kinetochore, Nocodazole, Cell Cycle, Intracellular Signaling Peptides and Proteins, Cell Biology, Cyclin-Dependent Kinases, Spindle apparatus, Cell biology, Spindle checkpoint, Amino Acid Substitution, Mitotic exit, Saccharomycetales, Protein Kinases, Developmental Biology

Abstract

During mitosis the spindle assembly checkpoint ( SAC) delays the onset of anaphase and mitotic exit until all chromosomes are bipolarly attached to spindle fibers. Both lack of attachment due to spindle/kinetochore defects and lack of tension across kinetochores generate the "wait anaphase" signal transmitted by the SAC, which involves the evolutionarily conserved Mad1, Mad2, Mad3/BubR1, Bub1, Bub3 and Mps1 proteins, and inhibits the activity of the ubiquitin ligase Cdc20/APC, that promotes both sister chromatid dissociation in anaphase and mitotic exit. In particular, Mad3/BubR1 is directly implicated, together with Mad2, in Cdc20 inactivation in both human and yeast cells, suggesting that its activity is likely finely regulated. We show that budding yeast Mad3, like its human orthologue BubR1, is a phosphoprotein that is hyperphosphorylated during mitosis and when SAC activation is triggered by microtubule depolymerizing agents, kinetochore defects or lack of kinetochore tension. In vivo Mad3 phosphorylation depends on the Polo kinase Cdc5 and, to a minor extent, the Aurora B kinase Ipl1. Accordingly, replacing with alanines five serine residues belonging to Polo kinase-dependent putative phosphorylation sites dramatically reduces Mad3 phosphorylation, suggesting that Mad3 is likely an in vivo target of Cdc5

Published

2005

27. Budding yeast PAK kinases regulate mitotic exit by two different mechanisms

Author

Giovanna Lucchini, Mariagrazia Tonelli, Simonetta Piatti, Elena Chiroli, Alessia Beretta, Roberta Fraschini, Chiroli, E, Fraschini, R, Beretta, A, Tonelli, M, Lucchini, G, and Piatti, S

Subjects

Saccharomyces cerevisiae Proteins, Cyclin B, Mitosis, Cell Cycle Proteins, BIO/18 - GENETICA, Saccharomyces cerevisiae, CDC20, Protein Serine-Threonine Kinases, Anaphase-Promoting Complex-Cyclosome, Article, Ligases, cytokinesis, mitotic exit network, Cla4, spindle checkpoint, Swe1, p21-activated kinases, Cells, Cultured, Monomeric GTP-Binding Proteins, cytokinesis, Mitotic Exit Network, PAK kinases, spindle checkpoint, Swe1, biology, MAP kinase kinase kinase, Intracellular Signaling Peptides and Proteins, Nuclear Proteins, Ubiquitin-Protein Ligase Complexes, Cell Biology, Protein-Tyrosine Kinases, MAP Kinase Kinase Kinases, Cell biology, Genes, cdc, Securin, Mitotic exit, Mutation, biology.protein, Anaphase, Cytokinesis

Abstract

We report the characterization of the dominant-negative CLA4t allele of the budding yeast CLA4 gene, encoding a member of the p21-activated kinase (PAK) family of protein kinases, which, together with its homologue STE20, plays an essential role in promoting budding and cytokinesis. Overproduction of the Cla4t protein likely inhibits both endogenous Cla4 and Ste20 and causes a delay in the onset of anaphase that correlates with inactivation of Cdc20/anaphase-promoting complex (APC)–dependent proteolysis of both the cyclinB Clb2 and securin. Although the precise mechanism of APC inhibition by Cla4t remains to be elucidated, our results suggest that Cla4 and Ste20 may regulate the first wave of cyclinB proteolysis mediated by Cdc20/APC, which has been shown to be crucial for activation of the mitotic exit network (MEN). We show that the Cdk1-inhibitory kinase Swe1 is required for the Cla4t-dependent delay in cell cycle progression, suggesting that it might be required to prevent full Cdc20/APC and MEN activation. In addition, inhibition of PAK kinases by Cla4t prevents mitotic exit also by a Swe1-independent mechanism impinging directly on the MEN activator Tem1.

Published

2003

28. Budding Yeast Dma Proteins Control Septin Dynamics and the Spindle Position Checkpoint by Promoting the Recruitment of the Elm1 Kinase to the Bud Neck

Author

Yves Barral, Giovanna Lucchini, Barbara Boettcher, Roberta Fraschini, Laura Merlini, Simonetta Piatti, Merlini, L, Fraschini, R, Boettcher, B, Barral, Y, Lucchini, G, Piatti, S, Università degli Studi di Milano-Bicocca [Milano] (UNIMIB), Institute of Biochemistry, Eidgenössische Technische Hochschule - Swiss Federal Institute of Technology [Zürich] (ETH Zürich), Dipartimento di Biotecnologie e Bioscienze, Centre de recherche en Biologie Cellulaire (CRBM), and Université Montpellier 2 - Sciences et Techniques (UM2)-Centre National de la Recherche Scientifique (CNRS)-Université de Montpellier (UM)-Université Montpellier 1 (UM1)

Subjects

Cancer Research, Saccharomyces cerevisiae Proteins, lcsh:QH426-470, Saccharomyces cerevisiae, Elm1, Mitosis, BIO/18 - GENETICA, Cell Cycle Proteins, Protein Serine-Threonine Kinases, Septin, 03 medical and health sciences, Model Organisms, 0302 clinical medicine, Gene Expression Regulation, Fungal, Molecular Cell Biology, Genetics, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, Phosphorylation, Biology, Molecular Biology, Genetics (clinical), Ecology, Evolution, Behavior and Systematics, Cytokinesis, 030304 developmental biology, Anaphase, 0303 health sciences, biology, Fluorescence recovery after photobleaching, biology.organism_classification, Cell biology, lcsh:Genetics, Dma protein, Septin ring, septin dynamic, Mitotic exit, Mutation, M Phase Cell Cycle Checkpoints, biological phenomena, cell phenomena, and immunity, Protein Kinases, Septins, 030217 neurology & neurosurgery, spindle position checkpoint, Research Article, Signal Transduction

Abstract

The first step towards cytokinesis in budding yeast is the assembly of a septin ring at the future site of bud emergence. Integrity of this ring is crucial for cytokinesis, proper spindle positioning, and the spindle position checkpoint (SPOC). This checkpoint delays mitotic exit and cytokinesis as long as the anaphase spindle does not properly align with the division axis. SPOC signalling requires the Kin4 protein kinase and the Kin4-regulating Elm1 kinase, which also controls septin dynamics. Here, we show that the two redundant ubiquitin-ligases Dma1 and Dma2 control septin dynamics and the SPOC by promoting the efficient recruitment of Elm1 to the bud neck. Indeed, dma1 dma2 mutant cells show reduced levels of Elm1 at the bud neck and Elm1-dependent activation of Kin4. Artificial recruitment of Elm1 to the bud neck of the same cells is sufficient to re-establish a normal septin ring, proper spindle positioning, and a proficient SPOC response in dma1 dma2 cells. Altogether, our data indicate that septin dynamics and SPOC function are intimately linked and support the idea that integrity of the bud neck is crucial for SPOC signalling., PLoS Genetics, 8 (4), ISSN:1553-7390, ISSN:1553-7404

Published

2012

29. The RSC chromatin-remodelling complex influences mitotic exit and adaptation to the spindle assembly checkpoint by controlling Cdc14 phosphatase

Author

Matteo Ferrari, Katsuhiko Shirahige, Simonetta Piatti, Valentina Rossio, Elena Galati, Achille Pellicioli, Takashi Sutani, Giovanna Lucchini, Rossio, V, Galati, E, Ferrari, M, Pellicioli, A, Sutani, T, Shirahige, K, Lucchini, G, and Piatti, S

Subjects

Saccharomyces cerevisiae Proteins, cells, genetic processes, Mitosis, Cell Cycle Proteins, BIO/18 - GENETICA, macromolecular substances, Saccharomyces cerevisiae, Spindle Apparatus, Polo-like kinase, environment and public health, Article, mitotic checkpoints, adaptation, RSC, Cdc14,yeast, chemistry.chemical_compound, Phosphoprotein Phosphatases, Chromatin structure remodeling (RSC) complex, Research Articles, Anaphase, biology, Cdc14, Cell Biology, Chromatin Assembly and Disassembly, Cell biology, Genes, cdc, Nocodazole, Spindle checkpoint, chemistry, Mitotic exit, biology.protein, Protein Tyrosine Phosphatases, Signal Transduction

Abstract

Rsc2 promotes Cdc14 release from the nucleolus to free cells from mitotic arrest., Upon prolonged activation of the spindle assembly checkpoint, cells escape from mitosis through a mechanism called adaptation or mitotic slippage, which is thought to underlie the resistance of cancer cells to antimitotic drugs. We show that, in budding yeast, this mechanism depends on known essential and nonessential regulators of mitotic exit, such as the Cdc14 early anaphase release (FEAR) pathway for the release of the Cdc14 phosphatase from the nucleolus in early anaphase. Moreover, the RSC (remodel the structure of chromatin) chromatin-remodeling complex bound to its accessory subunit Rsc2 is involved in this process as a novel component of the FEAR pathway. We show that Rsc2 interacts physically with the polo kinase Cdc5 and is required for timely phosphorylation of the Cdc14 inhibitor Net1, which is important to free Cdc14 in the active form. Our data suggest that fine-tuning regulators of mitotic exit have important functions during mitotic progression in cells treated with microtubule poisons and might be promising targets for cancer treatment.

Published

2010

30. Alfalfa Mob1-like proteins are involved in cell proliferation and are localized in the cell division plane during cytokinesis

Author

Gianni Barcaccia, Sandra Citterio, Simonetta Piatti, R Aina, Serena Varotto, Emidio Albertini, Citterio, S, Piatti, S, Albertini, E, Aina, R, Varotto, S, and Barcaccia, G

Subjects

Saccharomyces cerevisiae Proteins, Molecular Sequence Data, Cell, Mitosis, Cell Cycle Proteins, cytokinesis, Saccharomyces cerevisiae, Biology, Septin, BIO/01 - BOTANICA GENERALE, Microtubule, medicago sativa l, Mps-one-binder, cell proliferation, programmed cell death, medicine, Protein Isoforms, Amino Acid Sequence, Plant Proteins, Medicago sativa L., Mitosis, Mps-one-binder, Cytokinesis, Cell proliferation, Programmed cell death, Cell Biology, Cell plate, Cell cycle, Phosphoproteins, Cell biology, medicine.anatomical_structure, Cytoplasm, Cell Division, Cytokinesis, Medicago sativa

Abstract

Mps-one-binder (Mob) proteins play a crucial role in yeast cytokinesis. After cloning two Mob1-like genes, MsMob1-A and MsMob1-B from alfalfa (Medicago sativa L.) we show that, although they are constitutively expressed in roots, stems, leaves, flowers and pods, their transcripts and proteins are mostly produced in actively proliferating tissues. A polyclonal antibody specifically raised against MsMob1 proteins was used for immunolocalization studies in synchronized root tip cells. The subcellular localization of MsMob1-like proteins is demonstrated to be cell cycle-regulated. Cytoplasmic localization is faint and diffused during G1 and S. It becomes concentrated in punctuate and fibrillar structures in G2 as well as M phase. At the stage of cytokinesis, the protein is found at the emerging cell plate marking the progressive formation of the septum. Mob1 proteins partially co-localize with microtubules structures functionally related to the spindles and important for cytokinesis in eukaryotic cells. The MsMob1 expression cannot rescue the lethality of the yeast mob1 mutant, suggesting that interaction of Mob1 proteins with their effectors may be species-specific. Localization of Mob1 proteins in the inner layer of the root cap indicates an additional function for this class of proteins in plants, which is likely related to the onset of programmed cell death.

Published

2006

31. Sen34p depletion blocks tRNA splicing in vivo and delays rRNA processing

Author

Viviana Volta, David Tollervey, Pier Carlo Marchisio, Patrick Linder, Elisabeth Petfalski, Angela Bachi, Bertrand Emery, Stefano Biffo, Simonetta Piatti, Marcello Ceci, Volta, V, Ceci, M, Emery, B, Bachi, A, Petfalski, E, Tollervey, D, Linder, P, Marchisio, P, Piatti, S, and Biffo, S

Subjects

Ribosomal Proteins, RACK1, Saccharomyces cerevisiae Proteins, Translational efficiency, RNA Splicing, Biophysics, Saccharomyces cerevisiae, Biology, Biochemistry, Intermediate Filament Proteins, RNA, Transfer, 60S, Polysome, eIF6 (alias p27BBP), Gene Expression Regulation, Fungal, Endoribonucleases, RNA Precursors, RNA Processing, Post-Transcriptional, RRNA processing, Molecular Biology, Eukaryotic Large Ribosomal Subunit, Translation (biology), Cell Biology, Phosphoproteins, Molecular biology, Cell biology, Kinetics, RNA, Ribosomal, Transfer RNA, RNA splicing, Pre-rRNA, eIF3, Eukaryotic Ribosome, Carrier Proteins, Gene Deletion

Abstract

Tif6p (eIF6) is necessary for 60S biogenesis, rRNA maturation and must be released from 60S to permit 80S assembly and translation. We characterized Tif6p interactors. Tif6p is mostly on 66S-60S pre-ribosomes partly free. Tif6p complex(es) contain nucleo-ribosomal factors and Ase1p. Surprisingly, Tif6p particle contains the low-abundance endonuclease Sen34p. We analyzed Sen34p role on rRNA/tRNA synthesis, in vivo. Sen34p depletion impairs tRNA splicing and causes unexpected 80S accumulation. Accordingly, Sen34p overexpression causes 80S decrease and increased polysomes which suggest increased translational efficiency. With delayed kinetics, Sen34p depletion impairs rRNA processing. We conclude that Sen34p is absolutely required for tRNA splicing and that it is a rate-limiting element for efficient translation. Finally, we confirm that Tif6p accompanies 27S pre-rRNA maturation to 25S rRNA and we suggest that Sen34p endonuclease in Tif6p complex may affect also rRNA maturation. (c) 2005 Elsevier Inc. All rights reserved.

Published

2005

32. Functional characterization of Dma1 and Dma2, the budding yeast homologues of S. pombe Dma1 and human Chfr

Author

FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Bilotta, D, Fraschini, R, Bilotta, D, Lucchini, G, and Piatti, S

Subjects

BIO/18 - GENETICA, cytokinesis, spindle positioning, spindle position checkpoint, budding yeast, mitotic exit network

Abstract

Proper transmission of genetic information requires correct assembly and positioning of the mitotic spindle, responsible for driving each set of sister chromatids to the two daughter cells, followed by cytokinesis. In case of altered spindle orientation, the spindle position checkpoint inhibits Tem1-dependent activation of the Mitotic Exit Network (MEN), thus delaying mitotic exit and cytokinesis until errors are corrected. We report a functional analysis of two previously uncharacterized budding yeast proteins, Dma1 and Dma2, 58% identical to each other and homologous to human Chfr and S. pombe Dma1, both of which have been previously implicated in mitotic checkpoints. We show that Dma1 and Dma2 are involved in proper spindle positioning, likely regulating septin ring deposition at the bud neck. DMA2 overexpression causes defects in septin ring disassembly at the end of mitosis and in cytokinesis. The latter defects can be rescued by either eliminating the spindle position checkpoint protein Bub2 or overproducing its target Tem1, both leading to MEN hyperactivation. In addition, dma1Δ dma2Δ cells fail to activate the spindle position checkpoint in response to the lack of dynein, whereas ectopic expression of DMA2 prevents unscheduled mitotic exit of spindle checkpoint mutants treated with microtubule depolymerizing drugs. Although their primary functions remain to be defined, our data suggest that Dma1 and Dma2 might be required to ensure timely MEN activation in telophase.

Published

2004

33. Role of the kinetochore protein Ndc10 in mitotic checkpoint activation

Author

FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Beretta, A, Fraschini, R, Beretta, A, Lucchini, G, and Piatti, S

Subjects

anaphase, kinetochore, Mad2, mitotic checkpoint, Ndc10, BIO/18 - GENETICA

Abstract

Mitotic checkpoints delay cell cycle progression in response to alterations of the mitotic apparatus, thus ensuring correct chromosome segregation. While unproper spindle orientation activates a Bub2/Bfa1-dependent checkpoint delaying exit from mitosis, the lack of bipolar kinetochore-microtubule attachment activates a signal transduction cascade, preventing both anaphase onset and mitotic exit by inhibiting the Cdc20/APC-mediated proteolysis of securin and inactivation of mitotic CDKs, respectively. Proteolysis of the securin Pds1 is necessary to liberate the separase Esp1, which then triggers sister chromatid separation, whereas inactivation of mitotic CDKs is a pre-requisite for exiting mitosis and starting a new round of DNA replication in the next cell cycle. In budding yeast, this checkpoint response involves the Mad1, 2, 3, Bub1 and Bub3 proteins, whose vertebrate counterparts localize at unattached kinetochores. Unlike mutations altering other kinetochore proteins, which result in mitotic checkpoint activation, the ndc10-1 mutation impairs not only kinetochore function, but also proper checkpoint response, indicating a role for Ndc10 in this process. Here we present evidence that Ndc10 is not part of the Bub2/Bfa1-dependent pathway, and its role in checkpoint response might be different also from that of the other Mad and Bub proteins. In fact, Ndc10, unlike other mitotic checkpoint proteins, is not required for the mitotic block induced by overexpression of the Mps1 protein kinase, which is implicated in mitotic checkpoint control. Furthermore, the mitotic exit delay caused by non-degradable Pds1, which does not require Mad and Bub proteins, depends on Ndc10 function. We propose that a pathway involving Ndc10 might monitor defects in the mitotic apparatus independently of the Mad and Bub proteins. Since the Esp1 separase is required for exiting mitosis in both ndc10-1 and mad2Δ nocodazole-treated cells, the two signal transduction cascades might in the end converge in the inactivation of Esp1.

Published

2001

34. Bub3 interaction with Mad1, Mad2, Mad3 and Cdc20 is mediated by WD40 repeats and does not require intact kinetochores

Author

FRASCHINI, ROBERTA, LUCCHINI, GIOVANNA, PIATTI, SIMONETTA, Beretta, A, Sironi, L, Musacchio, A, Fraschini, R, Beretta, A, Sironi, L, Musacchio, A, Lucchini, G, and Piatti, S

Subjects

BIO/18 - GENETICA, Bub3, Cdc20, kinetochore, mitotic checkpoint, WD40

Abstract

The kinetochore checkpoint pathway, involving the Mad1, Mad2, Mad3, Bub1, Bub3 and Mps1 proteins, prevents anaphase entry and mitotic exit by inhibiting the Anaphase Promoting Complex activator Cdc20 in response to monopolar attachment of sister kinetochores to spindle fibers. We show here that Cdc20, which had been previously shown to interact physically with Mad2 and Mad3, associates also with Bub3 and association is upregulated upon checkpoint activation. Moreover, co-fractionation experiments suggest that Mad2, Mad3 and Bub3 may be concomitantly present in protein complexes with Cdc20. Formation of the Bub3/Cdc20 complex requires all kinetochore checkpoint proteins but, surprisingly, not intact kinetochores. Conversely, point mutations altering the conserved WD40 motifs of Bub3, which might be involved in the formation of a β-propeller fold devoted to protein-protein interactions, disrupt its association with Mad2, Mad3 and Cdc20, as well as proper checkpoint response. We suggest that Bub3 could serve as a platform for interactions between kinetochore checkpoint proteins, and its association with Mad1, Mad2, Mad3 and Cdc20 might be instrumental for checkpoint activation

Published

2001

35. The spindle position checkpoint in budding yeast: the motherly care of MEN

Author

Piatti Simonetta, Venturetti Marianna, Chiroli Elena, Fraschini Roberta, Piatti, S, Venturetti, M, Chiroli, E, and Fraschini, R

Subjects

lcsh:Cytology, BIO/18 - GENETICA, Review, lcsh:QH573-671, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, lcsh:RC254-282, checkpoint, mitosis

Abstract

Mitotic exit and cytokinesis must be tightly coupled to nuclear division both in time and space in order to preserve genome stability and to ensure that daughter cells inherit the right set of chromosomes after cell division. This is achieved in budding yeast through control over a signal transduction cascade, the mitotic exit network (MEN), which is required for mitotic CDK inactivation in telophase and for cytokinesis. Current models of MEN activation emphasize on the bud as the place where most control is exerted. This review focuses on recent data that instead point to the mother cell as being the residence of key regulators of late mitotic events.

Published

2006

36. Comment on 'A centrosome-independent role for gamma-TuRC proteins in the spindle assembly checkpoint'

Author

Kevin G. Hardwick, Alexey Khodjakov, Kenneth E. Sawin, Conly L. Rieder, Simonetta Piatti, Andrea Musacchio, Stephen S. Taylor, Sue Biggins, Edward D. Salmon, Taylor, S, Hardwick, K, Sawin, K, Biggins, S, Piatti, S, Khodjakov, A, Rieder, C, Salmon, E, and Musacchio, A

Subjects

Centrosome, Multidisciplinary, Cell cycle checkpoint, Kinetochore, Mitosis, Spindle Apparatus, G2-M DNA damage checkpoint, Biology, Microtubules, Article, Spindle pole body, spindle assembly checkpoint, Spindle apparatus, Cell biology, Spindle checkpoint, Tubulin, Animals, Anaphase-promoting complex, Kinetochores, Microtubule-Associated Proteins, Signal Transduction

Abstract

Müller et al . (Reports, 27 October 2006, p. 654) showed that inhibition of the γ-tubulin ring complex (γ-TuRC) activates the spindle assembly checkpoint (SAC), which led them to suggest that γ-TuRC proteins play molecular roles in SAC activation. Because γ-TuRC inhibition leads to pleiotropic spindle defects, which are well known to activate kinetochore-derived checkpoint signaling, we believe that this conclusion is premature.

37. Septin Organization and Dynamics for Budding Yeast Cytokinesis.

Author

Varela Salgado M and Piatti S

Abstract

Cytokinesis, the process by which the cytoplasm divides to generate two daughter cells after mitosis, is a crucial stage of the cell cycle. Successful cytokinesis must be coordinated with chromosome segregation and requires the fine orchestration of several processes, such as constriction of the actomyosin ring, membrane reorganization, and, in fungi, cell wall deposition. In Saccharomyces cerevisiae , commonly known as budding yeast, septins play a pivotal role in the control of cytokinesis by assisting the assembly of the cytokinetic machinery at the division site and controlling its activity. Yeast septins form a collar at the division site that undergoes major dynamic transitions during the cell cycle. This review discusses the functions of septins in yeast cytokinesis, their regulation and the implications of their dynamic remodelling for cell division.

Published

2024

38. Phosphorylation of the F-BAR protein Hof1 drives septin ring splitting in budding yeast.

Author

Varela Salgado M, Adriaans IE, Touati SA, Ibanes S, Lai-Kee-Him J, Ancelin A, Cipelletti L, Picas L, and Piatti S

Subjects

Phosphorylation, Cell Cycle Proteins metabolism, Cell Cycle Proteins genetics, Actomyosin metabolism, Saccharomycetales metabolism, Saccharomycetales genetics, Mutation, Protein Binding, Saccharomyces cerevisiae Proteins metabolism, Saccharomyces cerevisiae Proteins genetics, Septins metabolism, Septins genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae genetics, Cytokinesis, Microtubule-Associated Proteins

Abstract

A double septin ring accompanies cytokinesis in yeasts and mammalian cells. In budding yeast, reorganisation of the septin collar at the bud neck into a dynamic double ring is essential for actomyosin ring constriction and cytokinesis. Septin reorganisation requires the Mitotic Exit Network (MEN), a kinase cascade essential for cytokinesis. However, the effectors of MEN in this process are unknown. Here we identify the F-BAR protein Hof1 as a critical target of MEN in septin remodelling. Phospho-mimicking HOF1 mutant alleles overcome the inability of MEN mutants to undergo septin reorganisation by decreasing Hof1 binding to septins and facilitating its translocation to the actomyosin ring. Hof1-mediated septin rearrangement requires its F-BAR domain, suggesting that it may involve a local membrane remodelling that leads to septin reorganisation. In vitro Hof1 can induce the formation of intertwined septin bundles, while a phosphomimetic Hof1 protein has impaired septin-bundling activity. Altogether, our data indicate that Hof1 modulates septin architecture in distinct ways depending on its phosphorylation status., (© 2024. The Author(s).)

Published

2024

39. The Syp1/FCHo2 protein induces septin filament bundling through its intrinsically disordered domain.

Author

Ibanes S, El-Alaoui F, Lai-Kee-Him J, Cazevieille C, Hoh F, Lyonnais S, Bron P, Cipelletti L, Picas L, and Piatti S

Subjects

Septins, Microscopy

Abstract

The septin collar of budding yeast is an ordered array of septin filaments that serves a scaffolding function for the cytokinetic machinery at the bud neck and compartmentalizes the membrane between mother and daughter cell. How septin architecture is aided by septin-binding proteins is largely unknown. Syp1 is an endocytic protein that was implicated in the timely recruitment of septins to the newly forming collar through an unknown mechanism. Using advanced microscopy and in vitro reconstitution assays, we show that Syp1 is able to align laterally and tightly pack septin filaments, thereby forming flat bundles or sheets. This property is shared by the Syp1 mammalian counterpart FCHo2, thus emphasizing conserved protein functions. Interestingly, the septin-bundling activity of Syp1 resides mainly in its intrinsically disordered region. Our data uncover the mechanism through which Syp1 promotes septin collar assembly and offer another example of functional diversity of unstructured protein domains., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

40. Downregulation of the Tem1 GTPase by Amn1 after cytokinesis involves both nuclear import and SCF-mediated degradation.

Author

Devault A and Piatti S

Subjects

Active Transport, Cell Nucleus, Cell Cycle Proteins genetics, Cell Cycle Proteins metabolism, Cytokinesis, Down-Regulation genetics, Humans, Mitosis, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Spindle Apparatus metabolism, Monomeric GTP-Binding Proteins genetics, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism

Abstract

At mitotic exit the cell cycle engine is reset to allow crucial processes, such as cytokinesis and replication origin licensing, to take place before a new cell cycle begins. In budding yeast, the cell cycle clock is reset by a Hippo-like kinase cascade called the mitotic exit network (MEN), whose activation is triggered at spindle pole bodies (SPBs) by the Tem1 GTPase. Yet, MEN activity must be extinguished once MEN-dependent processes have been accomplished. One factor contributing to switching off the MEN is the Amn1 protein, which binds Tem1 and inhibits it through an unknown mechanism. Here, we show that Amn1 downregulates Tem1 through a dual mode of action. On one side, it evicts Tem1 from SPBs and escorts it into the nucleus. On the other, it promotes Tem1 degradation as part of a Skp, Cullin and F-box-containing (SCF) ubiquitin ligase. Tem1 inhibition by Amn1 takes place after cytokinesis in the bud-derived daughter cell, consistent with its asymmetric appearance in the daughter cell versus the mother cell. This dual mechanism of Tem1 inhibition by Amn1 may contribute to the rapid extinguishing of MEN activity once it has fulfilled its functions., Competing Interests: Competing interests The authors declare no competing or financial interests., (© 2021. Published by The Company of Biologists Ltd.)

Published

2021

41. Silencing the spindle assembly checkpoint: Let's play Polo!

Author

Benzi G and Piatti S

Subjects

Cell Cycle Proteins genetics, Phosphoric Monoester Hydrolases, Protein Serine-Threonine Kinases, Proto-Oncogene Proteins, Polo-Like Kinase 1, Kinetochores, M Phase Cell Cycle Checkpoints

Abstract

Silencing of the spindle assembly checkpoint involves two protein phosphatases, PP1 and PP2A-B56, that are thought to extinguish checkpoint signaling through dephosphorylation of a checkpoint scaffold at kinetochores. In this issue, Cordeiro et al. (2020. J. Cell Biol.https://doi.org/10.1083/jcb.202002020) now show that a critical function of these phosphatases in checkpoint silencing is removal of Polo kinase at kinetochores, which would otherwise autonomously sustain the checkpoint., (© 2020 Benzi and Piatti.)

Published

2020

42. Killing two birds with one stone: how budding yeast Mps1 controls chromosome segregation and spindle assembly checkpoint through phosphorylation of a single kinetochore protein.

Author

Benzi G and Piatti S

Subjects

Humans, Kinetochores metabolism, Phosphorylation genetics, Saccharomycetales genetics, Aurora Kinase B genetics, Chromosome Segregation genetics, M Phase Cell Cycle Checkpoints genetics, Microtubule-Associated Proteins genetics, Protein Serine-Threonine Kinases genetics, Saccharomyces cerevisiae Proteins genetics

Abstract

During mitosis, the identical sister chromatids of each chromosome must attach through their kinetochores to microtubules emanating from opposite spindle poles. This process, referred to as chromosome biorientation, is essential for equal partitioning of the genetic information to the two daughter cells. Defects in chromosome biorientation can give rise to aneuploidy, a hallmark of cancer and genetic diseases. A conserved surveillance mechanism called spindle assembly checkpoint (SAC) prevents the onset of anaphase until biorientation is attained. Key to chromosome biorientation is an error correction mechanism that allows kinetochores to establish proper bipolar attachments by disengaging faulty kinetochore-microtubule connections. Error correction relies on the Aurora B and Mps1 kinases that also promote SAC signaling, raising the possibility that they are part of a single sensory device responding to improper attachments and concomitantly controlling both their disengagement and a temporary mitotic arrest. In budding yeast, Aurora B and Mps1 promote error correction independently from one another, but while the substrates of Aurora B in this process are at least partially known, the mechanism underlying the involvement of Mps1 in the error correction pathway is unknown. Through the characterization of a novel mps1 mutant and an unbiased genetic screen for extragenic suppressors, we recently gained evidence that a common mechanism based on Mps1-dependent phosphorylation of the Knl1/Spc105 kinetochore scaffold and subsequent recruitment of the Bub1 kinase is critical for the function of Mps1 in chromosome biorientation as well as for SAC activation (Benzi et al. EMBO Rep, 2020).

Published

2020

43. A common molecular mechanism underlies the role of Mps1 in chromosome biorientation and the spindle assembly checkpoint.

Author

Benzi G, Camasses A, Atsunori Y, Katou Y, Shirahige K, and Piatti S

Subjects

Cell Cycle Proteins genetics, Kinetochores, M Phase Cell Cycle Checkpoints genetics, Spindle Apparatus genetics, Chromosome Segregation, Saccharomyces cerevisiae Proteins genetics

Abstract

The Mps1 kinase corrects improper kinetochore-microtubule attachments, thereby ensuring chromosome biorientation. Yet, its critical phosphorylation targets in this process remain largely elusive. Mps1 also controls the spindle assembly checkpoint (SAC), which halts chromosome segregation until biorientation is attained. Its role in SAC activation is antagonised by the PP1 phosphatase and involves phosphorylation of the kinetochore scaffold Knl1/Spc105, which in turn recruits the Bub1 kinase to promote assembly of SAC effector complexes. A crucial question is whether error correction and SAC activation are part of a single or separable pathways. Here, we isolate and characterise a new yeast mutant, mps1-3, that is severely defective in chromosome biorientation and SAC signalling. Through an unbiased screen for extragenic suppressors, we found that mutations lowering PP1 levels at Spc105 or forced association of Bub1 with Spc105 reinstate both chromosome biorientation and SAC signalling in mps1-3 cells. Our data argue that a common mechanism based on Knl1/Spc105 phosphorylation is critical for Mps1 function in error correction and SAC signalling, thus supporting the idea that a single sensory apparatus simultaneously elicits both pathways., (© 2020 The Authors.)

Published

2020

44. Cytokinesis: An Anillin-RhoGEF Module Sets the Stage for Septin Double Ring Assembly.

Author

Piatti S

Subjects

Contractile Proteins metabolism, Rho Guanine Nucleotide Exchange Factors, Cytokinesis, Septins metabolism

Abstract

In many eukaryotes septin filaments form an hourglass-like structure at the division site that rearranges into a double ring at cytokinesis. A new study elucidates how an anillin-RhoGEF complex guides the assembly of the septin double ring in budding yeast., (Copyright © 2020 Elsevier Inc. All rights reserved.)

Published

2020

45. The Phosphatase PP1 Promotes Mitotic Slippage through Mad3 Dephosphorylation.

Author

Ruggiero A, Katou Y, Shirahige K, Séveno M, and Piatti S

Subjects

Cell Cycle Proteins metabolism, Nuclear Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism, Cell Cycle Proteins genetics, Chromosome Segregation, M Phase Cell Cycle Checkpoints genetics, Mitosis genetics, Nuclear Proteins genetics, Protein Phosphatase 1 metabolism, Saccharomyces cerevisiae physiology, Saccharomyces cerevisiae Proteins genetics

Abstract

Accurate chromosome segregation requires bipolar attachment of kinetochores to spindle microtubules. A conserved surveillance mechanism, the spindle assembly checkpoint (SAC), responds to lack of kinetochore-microtubule connections and delays anaphase onset until all chromosomes are bipolarly attached [1]. SAC signaling fires at kinetochores and involves a soluble mitotic checkpoint complex (MCC) that inhibits the anaphase-promoting complex (APC) [2, 3]. The mitotic delay imposed by SAC, however, is not everlasting. If kinetochores fail to establish bipolar connections, cells can escape from the SAC-induced mitotic arrest through a process called mitotic slippage [4]. Mitotic slippage occurs in the presence of SAC signaling at kinetochores [5, 6], but whether and how MCC stability and APC inhibition are actively controlled during slippage is unknown. The PP1 phosphatase has emerged as a key factor in SAC silencing once all kinetochores are bipolarly attached [7, 8]. PP1 turns off SAC signaling through dephosphorylation of the SAC scaffold Knl1/Blinkin at kinetochores [9-11]. Here, we show that, in budding yeast, PP1 is also required for mitotic slippage. However, its involvement in this process is not linked to kinetochores but rather to MCC stability. We identify S268 of Mad3 as a critical target of PP1 in this process. Mad3 S268 dephosphorylation destabilizes the MCC without affecting the initial SAC-induced mitotic arrest. Conversely, it accelerates mitotic slippage and overcomes the slippage defect of PP1 mutants. Thus, slippage is not the mere consequence of incomplete APC inactivation that brings about mitotic exit, as originally proposed, but involves the exertive antagonism between kinases and phosphatases., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2020

46. Septin clearance from the division site triggers cytokinesis in budding yeast.

Author

Tamborrini D and Piatti S

Abstract

In many eukaryotic cells cytokinesis involves a contractile actomyosin ring (CAR) that drives cleavage furrow ingression. What triggers CAR constriction at a precise time of the cell cycle and how constriction is coupled to chromosome segregation are fundamental questions. In the budding yeast Saccharomyces cerevisiae , CAR assembly strictly requires a rigid septin collar that forms at the bud neck early during the cell cycle. At the time of cytokinesis, a sudden remodelling of the septin collar occurs, leading to its splitting into two separate rings that sandwich the CAR. We have shown that septin displacement during splitting is an essential prerequisite for CAR constriction [Tamborrini et al ., Nat Commun. 9(1):4308]. Thus, cytokinesis in budding yeast is a two-step mechanism: during the first step, the septin collar organizes the assembly of the cytokinetic machinery at the right place while restraining CAR-driven membrane ingression; during the second step, a confined eviction of septins from the division site during septin ring splitting triggers CAR constriction. Our data further indicate that septin ring splitting is prompted by the Mitotic Exit Network (MEN), and in particular by its downstream phosphatase Cdc14, independently of its mitotic exit function. Surprisingly, MEN signalling at spindle pole bodies (SPBs) is critical for septin ring splitting and cytokinesis. Ubiquitination of the MEN anchor at SPBs by the Dma1/2 ubiquitin ligase attenuates MEN signalling and could have a decisive role in coupling cytokinesis to chromosome and organelle segregation. Altogether, our data emphasize the importance of septin ring splitting, which has been mysterious so far, and highlight a novel mechanism to prevent CAR constriction and cytokinesis in unpropitious conditions., Competing Interests: Conflict of interest: The authors declare no conflict of interest.

Published

2019

47. Recruitment of the mitotic exit network to yeast centrosomes couples septin displacement to actomyosin constriction.

Author

Tamborrini D, Juanes MA, Ibanes S, Rancati G, and Piatti S

Subjects

Cell Cycle Proteins metabolism, Centrosome metabolism, Deoxyribonucleases metabolism, Protein Tyrosine Phosphatases metabolism, Saccharomyces cerevisiae Proteins metabolism, Ubiquitination, Yeasts, tRNA Methyltransferases metabolism, Actomyosin metabolism, Cytokinesis, Saccharomyces cerevisiae enzymology, Septins metabolism, Spindle Pole Bodies metabolism

Abstract

In many eukaryotic organisms cytokinesis is driven by a contractile actomyosin ring (CAR) that guides membrane invagination. What triggers CAR constriction at a precise time of the cell cycle is a fundamental question. In budding yeast CAR is assembled via a septin scaffold at the division site. A Hippo-like kinase cascade, the Mitotic Exit Network (MEN), promotes mitotic exit and cytokinesis, but whether and how these two processes are independently controlled by MEN is poorly understood. Here we show that a critical function of MEN is to promote displacement of the septin ring from the division site, which in turn is essential for CAR constriction. This is independent of MEN control over mitotic exit and involves recruitment of MEN components to the spindle pole body (SPB). Ubiquitination of the SPB scaffold Nud1 inhibits MEN signaling at the end of mitosis and prevents septin ring splitting, thus silencing the cytokinetic machinery.

Published

2018

48. Asymmetric Localization of Components and Regulators of the Mitotic Exit Network at Spindle Pole Bodies.

Author

Scarfone I and Piatti S

Subjects

Fixatives, Fluorescent Antibody Technique methods, GTP-Binding Proteins analysis, Green Fluorescent Proteins analysis, M Phase Cell Cycle Checkpoints, Mitosis, Yeasts ultrastructure, Cell Cycle Proteins analysis, Fungal Proteins analysis, Microscopy, Fluorescence methods, Spindle Pole Bodies ultrastructure, Yeasts cytology

Abstract

Most proteins of the Mitotic Exit Network (MEN) and their upstream regulators localize at spindle pole bodies (SPBs) at least in some stages of the cell cycle. Studying the SPB localization of MEN factors has been extremely useful to elucidate their biological roles, organize them in a hierarchical pathway, and define their dynamics under different conditions.Recruitment to SPBs of the small GTPase Tem1 and the downstream kinases Cdc15 and Mob1/Dbf2 is thought to be essential for Cdc14 activation and mitotic exit, while that of the upstream Tem1 regulators (the Kin4 kinase and the GTPase activating protein Bub2-Bfa1) is important for MEN inhibition upon spindle mispositioning. Here, we describe the detailed fluorescence microscopy procedures that we use in our lab to analyze the localization at SPBs of Mitotic Exit Network (MEN) components tagged with GFP or HA epitopes.

Published

2017

49. Control of Formin Distribution and Actin Cable Assembly by the E3 Ubiquitin Ligases Dma1 and Dma2.

Author

Juanes MA and Piatti S

Subjects

Actin Cytoskeleton genetics, Actins genetics, Actins metabolism, Cell Cycle physiology, Cell Cycle Proteins genetics, Cell Polarity physiology, Cytoskeletal Proteins biosynthesis, Cytoskeletal Proteins genetics, Cytoskeletal Proteins metabolism, Cytoskeleton metabolism, Microfilament Proteins biosynthesis, Microfilament Proteins genetics, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins biosynthesis, Saccharomyces cerevisiae Proteins genetics, Ubiquitin-Protein Ligases genetics, Ubiquitination, Actin Cytoskeleton metabolism, Cell Cycle Proteins metabolism, Microfilament Proteins metabolism, Saccharomyces cerevisiae Proteins metabolism, Ubiquitin-Protein Ligases metabolism

Abstract

Formins are widespread actin-polymerizing proteins that play pivotal roles in a number of processes, such as cell polarity, morphogenesis, cytokinesis, and cell migration. In agreement with their crucial function, formins are prone to a variety of regulatory mechanisms that include autoinhibition, post-translational modifications, and interaction with formin modulators. Furthermore, activation and function of formins is intimately linked to their ability to interact with membranes. In the budding yeast Saccharomyces cerevisiae, the two formins Bni1 and Bnr1 play both separate and overlapping functions in the organization of the actin cytoskeleton. In addition, they are controlled by both common and different regulatory mechanisms. Here we show that proper localization of both formins requires the redundant E3 ubiquitin ligases Dma1 and Dma2, which were previously involved in spindle positioning and septin organization. In dma1 dma2 double mutants, formin distribution at polarity sites is impaired, thus causing defects in the organization of the actin cable network and hypersensitivity to the actin depolymerizer latrunculin B. Expression of a hyperactive variant of Bni1 (Bni1-V360D) rescues these defects and partially restores proper spindle positioning in the mutant, suggesting that the failure of dma1 dma2 mutant cells to position the spindle is partly due to faulty formin activity. Strikingly, Dma1/2 interact physically with both formins, while their ubiquitin-ligase activity is required for formin function and polarized localization. Thus, ubiquitylation of formin or a formin interactor(s) could promote formin binding to membrane and its ability to nucleate actin. Altogether, our data highlight a novel level of formin regulation that further expands our knowledge of the complex and multilayered controls of these key cytoskeleton organizers., (Copyright © 2016 by the Genetics Society of America.)

Published

2016

50. The final cut: cell polarity meets cytokinesis at the bud neck in S. cerevisiae.

Author

Juanes MA and Piatti S

Subjects

Actins metabolism, Actomyosin metabolism, Cell Polarity, Microfilament Proteins metabolism, Saccharomyces cerevisiae metabolism, Septins metabolism, rho GTP-Binding Proteins metabolism, Cytokinesis, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae growth & development, Saccharomyces cerevisiae Proteins metabolism

Abstract

Cell division is a fundamental but complex process that gives rise to two daughter cells. It includes an ordered set of events, altogether called "the cell cycle", that culminate with cytokinesis, the final stage of mitosis leading to the physical separation of the two daughter cells. Symmetric cell division equally partitions cellular components between the two daughter cells, which are therefore identical to one another and often share the same fate. In many cases, however, cell division is asymmetrical and generates two daughter cells that differ in specific protein inheritance, cell size, or developmental potential. The budding yeast Saccharomyces cerevisiae has proven to be an excellent system to investigate the molecular mechanisms governing asymmetric cell division and cytokinesis. Budding yeast is highly polarized during the cell cycle and divides asymmetrically, producing two cells with distinct sizes and fates. Many components of the machinery establishing cell polarization during budding are relocalized to the division site (i.e., the bud neck) for cytokinesis. In this review we recapitulate how budding yeast cells undergo polarized processes at the bud neck for cell division.

Published

2016