Multiple roles for protein phosphatase 1 in regulating the Xenopus early embryonic cell cycle.

Using cytostatic factor metaphase II-arrested extracts as a model system, we show that protein phosphatase 1 is regulated during early embryonic cell cycles in Xenopus. Phosphatase 1 activity peaks during interphase and decreases shortly before the onset of mitosis. A second peak of activity appears in mitosis at about the same time that cdc2 becomes active. If extracts are inhibited in S-phase with aphidicolin, then phosphatase 1 activity remains high. The activity of phosphatase 1 appears to determine the timing of exit from S-phase and entry into M-phase; inhibition of phosphatase 1 by the specific inhibitor, inhibitor 2 (Inh-2), causes premature entry into mitosis, whereas exogenously added phosphatase 1 lengthens the interphase period. Analysis of DNA synthesis in extracts treated with Inh-2, but lacking the A- and B-type cyclins, shows that phosphatase 1 is also required for the process of DNA replication. These data indicate that phosphatase 1 is a component of the signaling pathway that ensures that M-phase is not initiated until DNA synthesis is complete.

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Maturation promoting factor and cell cycle regulation

Development ◽

10.1242/dev.89.supplement.271 ◽

1985 ◽

Vol 89 (Supplement) ◽

pp. 271-284

Author(s):

C. C. Ford

Keyword(s):

Dna Synthesis ◽

Cell Cycle Regulation ◽

Nuclear Division ◽

S Phase ◽

Early Cleavage ◽

Cell Cycles ◽

Nuclear Envelope Breakdown ◽

Cytostatic Factor ◽

Cycle Regulation ◽

Maturation Promoting Factor

Cell cycles in early amphibian embryos are characterized by the absence of G1 and G2 phases. The simple cycle of S phase and mitosis does show similarities with other systems, particularly in the presence of cytoplasmic components advancing nuclei into DNA synthesis and mitosis. Maturation-promoting factor induces nuclear envelope breakdown and subsequent chromosome condensation. Cytoplasmic factors appear during maturation which are capable of inducing DNA synthesis, and arrest of the nuclear division cycle in metaphase (cytostatic factor). The timing of appearance of these activities is considered and their relationship in integrating DNA synthesis during early cleavage is discussed.

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Evolution of CDK1 paralog specializations in a lineage with fast developing planktonic embryos

10.1101/817783 ◽

2019 ◽

Author(s):

Xiaofei Ma ◽

Jan Inge Øvrebø ◽

Eric M Thompson

Keyword(s):

General Rule ◽

Embryonic Cell ◽

Cyclin B ◽

Gene Duplications ◽

Structural Elements ◽

Oikopleura Dioica ◽

Cell Cycles ◽

Protein Levels ◽

Binding Interface ◽

M Phase

AbstractThe active site of the essential, eukaryotic CDK1 kinase is generated by core structural elements, among which the PSTAIRE motif in the critical αC-helix, is universally conserved in metazoans. The CDK2 kinase, sharing the PSTAIRE, arose early in metazoan evolution and permitted subdivision of tasks along the S-M-phase axis. The marine chordate, Oikopleura dioica, is the only metazoan known to possess more than a single CDK1 ortholog, and all of its 5 paralogs show sequence divergences in the PSTAIRE. Through assessing CDK1 gene duplications in the appendicularian lineage, we show that the CDK1 activation loop substrate binding platform, ATP entrance site, hinge region, and main Cyclin binding interface, have all diversified under positive selection. Three of the 5 CDK1 paralogs are required for embryonic divisions and knockdown phenotypes illustrate further subdivision of functions along the S-M-phase axis. In parallel to CDK1 gene duplications, there has also been amplification in the Cyclin B complement. Among these, the CDK1d:Cyclin Ba pairing is required for oogenic meiosis and early embryogenesis and shows evidence of coevolution of an exclusive interaction. In an intriguing twist on the general rule that Cyclin B oscillations on a background of stable CDK1 levels regulate M-phase MPF activity, it is CDK1d protein levels that oscillate, rather than Cyclin Ba levels, to drive rapid, early embryonic cell cycles. Strikingly, the modified PSTAIRE of odCDK1d shows convergence over great evolutionary distance with plant CDKB, and in both O. dioica, and plants, these variants exhibit increased specialization to M-phase.

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N-Acetyl-β-D-glucopyranosylamine 6-phosphate is a specific inhibitor of glycogen-bound protein phosphatase 1

Biochemical Journal ◽

10.1042/bj3280695 ◽

1997 ◽

Vol 328 (2) ◽

pp. 695-700 ◽

Cited By ~ 3

Author(s):

Mary BOARD

Keyword(s):

Phosphatase Activity ◽

Protein Phosphatase ◽

Glycogen Phosphorylase ◽

Glycogen Synthase ◽

Specific Inhibitor ◽

Competitive Inhibitor ◽

Protein Phosphatase 1 ◽

P Concentration ◽

Glucose Analogue ◽

Stimulation Of

Previous work has shown that the C-1-substituted glucose-analogue N-acetyl-β-D-glucopyranosylamine (1-GlcNAc) is a competitive inhibitor of glycogen phosphorylase (GP) and stimulates the inactivation of this enzyme by GP phosphatase. In addition to its effects on GP, 1-GlcNAc also prevents the glucose-led activation of glycogen synthase (GS) in whole hepatocytes. Such an effect on GS was thought to be due to the formation of 1-GlcNAc-6-P by the action of glucokinase within the hepatocyte [Board, Bollen, Stalmans, Kim, Fleet and Johnson (1995) Biochem. J. 311, 845-852]. To investigate this possibility further, a pure preparation of 1-GlcNAc-6-P was synthesized. The effects of the phosphorylated glucose analogue on the activity of protein phosphatase 1 (PP1), the enzyme responsible for dephosphorylation and activation of GS, are reported. During the present study, 1-GlcNAc-6-P inhibited the activity of the glycogen-bound form of PP1, affecting both the GSb phosphatase and GPa phosphatase activities. A level of 50% inhibition of GSb phosphatase activity was achieved with 85 μM 1-GlcNAc-6-P in the absence of Glc-6-P and with 135 μM in the presence of 10 mM Glc-6-P. At either Glc-6-P concentration, 500 μM 1-GlcNAc-6-P completely inhibited activity. The Glc-6-P stimulation of the GPa phosphatase activity of PP1 was negated by 1-GlcNAc-6-P but there was no inhibition of the basal rate in the absence of Glc-6-P. 1-GlcNAc-6-P inhibition was specific for the glycogen-bound form of PP1 and did not inhibit the GSb phosphatase activity of the cytosolic form of the enzyme. The present work explains our previous observations on the inactivating effects on GS of incubating whole hepatocytes with 1-GlcNAc. These observations have their basis in the inhibition of glycogen-bound PP1 by 1-GlcNAc-6-P. A novel inhibitor of PP1, specific for the glycogen-bound form of the enzyme, is presented.

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Inhibition of protein phosphatase 1 reverses alcohol-induced ciliary dysfunction

AJP Lung Cellular and Molecular Physiology ◽

10.1152/ajplung.00336.2014 ◽

2015 ◽

Vol 308 (6) ◽

pp. L577-L585 ◽

Cited By ~ 15

Author(s):

Michael E. Price ◽

Jacqueline A. Pavlik ◽

Joseph H. Sisson ◽

Todd A. Wyatt

Keyword(s):

Protein Phosphatase ◽

Mucociliary Clearance ◽

Specific Inhibitor ◽

Alcohol Exposure ◽

Inhibitory Effect ◽

Regulatory Proteins ◽

Protein Phosphatase 1 ◽

Tissue Cell ◽

Inhaled Particles ◽

Phosphatase Activation

Airway mucociliary clearance is a first-line defense of the lung against inhaled particles and debris. Among individuals with alcohol use disorders, there is an increase in lung diseases. We previously identified that prolonged alcohol exposure impairs mucociliary clearance, known as alcohol-induced ciliary dysfunction (AICD). Cilia-localized enzymes, known as the ciliary metabolon, are key to the pathogenesis of AICD. In AICD, cyclic nucleotide-dependent ciliary kinases, which modulate phosphorylation to regulate cilia beat, are desensitized. We hypothesized that alcohol activates cilia-associated protein phosphatase 1 (PP1) activity, driving phosphorylation changes of cilia motility regulatory proteins. To test this hypothesis we identified the effects of prolonged alcohol exposure on phosphatase activity, cilia beat, and kinase responsiveness and cilia-associated phosphorylation targets when stimulated by β-agonist or cAMP. Prolonged alcohol activated PP1 and blocked cAMP-dependent cilia beat and protein kinase A (PKA) responsiveness and phosphorylation of a 29-kDa substrate of PKA. Importantly, prolonged alcohol-induced phosphatase activation was inhibited by the PP1 specific inhibitor, inhibitor-2 (I-2), restoring cAMP-stimulated cilia beat and PKA responsiveness and phosphorylation of the 29-kDa substrate. The I-2 inhibitory effect persisted in tissue, cell, and isolated cilia-organelle models, highlighting the association of ciliary metabolon-localized enzymes to AICD. Prolonged alcohol exposure drives ciliary metabolon-localized PP1 activation. PP1 activation modifies phosphorylation of a 29-kDa protein related to PKA activity. These data reinforce our previous findings that alcohol is acting at the level of the ciliary metabolon to cause ciliary dysfunction and identifies PP1 as a therapeutic target to prevent or reverse AICD.

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Xenopus Cdc7 executes its essential function early in S phase and is counteracted by checkpoint-regulated protein phosphatase 1

Open Biology ◽

10.1098/rsob.130138 ◽

2014 ◽

Vol 4 (1) ◽

pp. 130138 ◽

Cited By ~ 18

Author(s):

Wei Theng Poh ◽

Gaganmeet Singh Chadha ◽

Peter J. Gillespie ◽

Philipp Kaldis ◽

J. Julian Blow

Keyword(s):

Protein Phosphatase ◽

Replication Timing ◽

S Phase ◽

Replication Initiation ◽

Protein Phosphatase 1 ◽

Checkpoint Kinases ◽

Anti Cancer ◽

Egg Extracts ◽

Mcm Proteins

The initiation of DNA replication requires two protein kinases: cyclin-dependent kinase (Cdk) and Cdc7. Although S phase Cdk activity has been intensively studied, relatively little is known about how Cdc7 regulates progression through S phase. We have used a Cdc7 inhibitor, PHA-767491, to dissect the role of Cdc7 in Xenopus egg extracts. We show that hyperphosphorylation of mini-chromosome maintenance (MCM) proteins by Cdc7 is required for the initiation, but not for the elongation, of replication forks. Unlike Cdks, we demonstrate that Cdc7 executes its essential functions by phosphorylating MCM proteins at virtually all replication origins early in S phase and is not limiting for progression through the Xenopus replication timing programme. We demonstrate that protein phosphatase 1 (PP1) is recruited to chromatin and rapidly reverses Cdc7-mediated MCM hyperphosphorylation. Checkpoint kinases induced by DNA damage or replication inhibition promote the association of PP1 with chromatin and increase the rate of MCM dephosphorylation, thereby counteracting the previously completed Cdc7 functions and inhibiting replication initiation. This novel mechanism for regulating Cdc7 function provides an explanation for previous contradictory results concerning the control of Cdc7 by checkpoint kinases and has implications for the use of Cdc7 inhibitors as anti-cancer agents.

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Aurora B kinase and protein phosphatase 1 have opposing roles in modulating kinetochore assembly

The Journal of Cell Biology ◽

10.1083/jcb.200710019 ◽

2008 ◽

Vol 181 (2) ◽

pp. 241-254 ◽

Cited By ~ 101

Author(s):

Michael J. Emanuele ◽

Weijie Lan ◽

Miri Jwa ◽

Stephanie A. Miller ◽

Clarence S.M. Chan ◽

...

Keyword(s):

Cell Cycle ◽

Protein Phosphatase ◽

Protein Phosphatase 1 ◽

Aurora B ◽

Aurora B Kinase ◽

Culture Cells ◽

Kinetochore Assembly ◽

M Phase ◽

Egg Extracts ◽

Cycle Dependent

The outer kinetochore binds microtubules to control chromosome movement. Outer kinetochore assembly is restricted to mitosis, whereas the inner kinetochore remains tethered to centromeres throughout the cell cycle. The cues that regulate this transient assembly are unknown. We find that inhibition of Aurora B kinase significantly reduces outer kinetochore assembly in Xenopus laevis and human tissue culture cells, frog egg extracts, and budding yeast. In X. leavis M phase extracts, preassembled kinetochores disassemble after inhibiting Aurora B activity with either drugs or antibodies. Kinetochore disassembly, induced by Aurora B inhibition, is rescued by restraining protein phosphatase 1 (PP1) activity. PP1 is necessary for kinetochores to disassemble at the exit from M phase, and purified enzyme is sufficient to cause disassembly on isolated mitotic nuclei. These data demonstrate that Aurora B activity is required for kinetochore maintenance and that PP1 is necessary and sufficient to disassemble kinetochores. We suggest that Aurora B and PP1 coordinate cell cycle–dependent changes in kinetochore assembly though phosphorylation of kinetochore substrates.

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Endoreduplication in Maize Endosperm: An Approach for Increasing Crop Productivity

10.32747/2000.7575285.bard ◽

2000 ◽

Author(s):

Gideon Grafi ◽

Brian Larkins

Keyword(s):

Cell Cycle ◽

Dna Synthesis ◽

Storage Protein ◽

Molecular Mechanisms ◽

S Phase ◽

Cyclin B ◽

Regulatory Subunit ◽

Maize Endosperm ◽

M Phase

The focus of this research project is to investigate the role of endoreduplication in maize endosperm development and the extent to which this process contributes to high levels of starch and storage protein synthesis. Although endoreduplication has been widely observed in many cells and tissues, especially those with high levels of metabolic activity, the molecular mechanisms through which the cell cycle is altered to produce consecutive cycles of S-phase without an intervening M-phase are unknown. Our previous research has shown that changes in the expression of several cell cycle regulatory genes coincide with the onset of endoreduplication. During this process, there is a sharp reduction in the activity of the mitotic cyclin-dependent kinase (CDK) and activation of the S-phase CDK. It appears the M-phase CDK is stable, but its activity is blocked by a proteinaceous inhibitor. Coincidentally, the S-phase checkpoint protein, retinoblastoma (ZmRb), becomes phosphorylated, presumably releasing an E2F-type transcriptional regulator which promotes the expression of genes responsible for DNA synthesis. To investigate the role of these cell cycle proteins in endoreduplication, we have created transgenic maize plants that express various genes in an endosperm-specific manner using a storage protein (g-zein) promoter. During the first year of the grant, we constructed point mutations of the maize M-phase kinase, p34cdc2. One alteration replaced aspartic acid at position 146 with asparagine (p3630-CdcD146N), while another changed threonine 161 to alanine (p3630-CdcT161A). These mutations abolish the activity of the CDK. We hypothesized that expression of the mutant forms of p34cdc2 in endoreduplicating endosperm, compared to a control p34cdc2, would lead to extra cycles of DNA synthesis. We also fused the gene encoding the regulatory subunit of the M- phase kinase, cyclin B, under the g-zein promoter. Normally, cyclin B is expected to be destroyed prior to the onset of endoreduplication. By producing high levels of this protein in developing endosperm, we hypothesized that the M-phase would be extended, potentially reducing the number of cycles of endoreduplication. Finally, we genetically engineered the wheat dwarf virus RepA protein for endosperm-specific expression. RepA binds to the maize retinoblastoma protein and presumably releases E2F-like transcription factors that activate DNA synthesis. We anticipated that inactivation of ZmRb by RepA would lead to additional cycles of DNA synthesis.

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Protein phosphatase 2A (PP2A) promotes anaphase entry after DNA replication stress in budding yeast

Molecular Biology of the Cell ◽

10.1091/mbc.e21-04-0222 ◽

2021 ◽

Author(s):

Cory Haluska ◽

Fengzhi Jin ◽

Yanchang Wang

Keyword(s):

Cell Cycle ◽

Dna Replication ◽

Dna Synthesis ◽

Protein Phosphatase ◽

Budding Yeast ◽

Replication Stress ◽

S Phase ◽

Viability Loss ◽

Phosphatase 2A ◽

Dna Replication Stress

DNA replication stress activates the S-phase checkpoint that arrests the cell cycle, but it is poorly understood how cells recover from this arrest. Cyclin-dependent kinase (CDK) and Protein Phosphatase 2A (PP2A) are key cell cycle regulators, and Cdc55 is a regulatory subunit of PP2A in budding yeast. We found that yeast cells lacking functional PP2ACdc55 showed slow growth in the presence of hydroxyurea (HU), a DNA synthesis inhibitor, without obvious viability loss. Moreover, PP2A mutants exhibited delayed anaphase entry and sustained levels of anaphase inhibitor Pds1 after HU treatment. A DNA damage checkpoint Chk1 phosphorylates and stabilizes Pds1. We showed that chk1Δ and mutation of the Chk1 phosphorylation sites in Pds1 largely restored efficient anaphase entry in PP2A mutants after HU treatment. In addition, deletion of SWE1 that encodes the inhibitory kinase for CDK or mutation of the Swe1 phosphorylation site in CDK ( cdc28F19) also suppressed the anaphase entry delay in PP2A mutants after HU treatment. Our genetic data suggest that Swe1/CDK acts upstream of Pds1. Surprisingly, cdc55Δ showed significant suppression to the viability loss of S-phase checkpoint mutants during DNA synthesis block. Together, our results uncover a PP2A-Swe1-CDK-Chk1-Pds1 axis that promotes recovery from DNA replication stress.

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The protein phosphatase inhibitor okadaic acid induces defects in cytokinesis and organellar genome segregation in Trypanosoma brucei

Journal of Cell Science ◽

10.1242/jcs.107.12.3477 ◽

1994 ◽

Vol 107 (12) ◽

pp. 3477-3483 ◽

Cited By ~ 6

Author(s):

A. Das ◽

M. Gale ◽

V. Carter ◽

M. Parsons

Keyword(s):

Cell Cycle ◽

Mitochondrial Dna ◽

Okadaic Acid ◽

Protein Phosphatase ◽

Specific Inhibitor ◽

Eukaryotic Cell ◽

Cell Cycles ◽

African Trypanosomes ◽

20 Nm

Mitosis and cytokinesis are events that are highly coordinated in most eukaryotic cell cycles. African trypanosomes possess a single mitochondrion and must additionally coordinate the organellar division cycle. Here we report that okadaic acid, a potent and specific inhibitor of protein phosphatases PP1and PP2A, uncouples these cycles in living trypanosomes. Cell cycle analysis of treated cells revealed elevated DNA content. Microscopic examination indicated that okadaic acid treatment yielded multinucleate cells with a single mitochondrial network indicating these cells have undergone mitosis but failed to complete cytokinesis. Immunofluorescence analysis of 5-bromo-2-deoxyuridine incorporation demonstrated that the mitochondrial DNA was replicated but did not segregate. The dose response curve for inhibition of the normal cell cycle paralleled that for the in vitro inhibition of protein phosphatase activities with IC50s of approximately 20 nM okadaic acid. These results suggest the involvement of a PP1/PP2A-like activity in coordinating mitosis, mitochondrial DNA division and cytokinesis in trypanosomes.

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Inhibiting proteasome activity causes overreplication of DNA and blocks entry into mitosis in sea urchin embryos

Journal of Cell Science ◽

10.1242/jcs.113.15.2659 ◽

2000 ◽

Vol 113 (15) ◽

pp. 2659-2670 ◽

Cited By ~ 1

Author(s):

H. Kawahara ◽

R. Philipova ◽

H. Yokosawa ◽

R. Patel ◽

K. Tanaka ◽

...

Keyword(s):

Sea Urchin ◽

Embryonic Cell ◽

S Phase ◽

Cdc2 Kinase ◽

Replication Checkpoint ◽

Kinase Activation ◽

Peptide Aldehydes ◽

M Phase ◽

Dna Replication Checkpoint ◽

P34 Cdc2

The proteasome has been shown to be involved in exit from mitosis by bringing about destruction of mitotic cyclins. Here, we present evidence that the proteasome is also required for proper completion of S phase and for entry into mitosis in the sea urchin embryonic cleavage cycle. A series of structurally related peptide-aldehydes prevent nuclear envelope breakdown in their order of inhibitory efficacies against the proteasome. Their efficacies in blocking exit from S phase and exit from mitosis correlate well, indicating that the proteasome is involved at both these steps. Mitotic histone HI kinase activation and tyrosine dephosphorylation of p34(cdc2) kinase are blocked by inhibition of the proteasome, indicating that the proteasome plays an important role in the pathway that leads to embryonic p34(cdc2)kinase activation. Arrested embryos continued to incorporate [(3)H]thymidine and characteristically developed large nuclei. Pre-mitotic arrest can be overcome by treatment with caffeine, a manoeuvre that is known to override the DNA replication checkpoint. These data demonstrate that the proteasome is involved in the control of termination of S phase and consequently in the initiation of M phase of the first embryonic cell cycle.

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