Correspondence to: Kyung S. Lee, Laboratory of Metabolism, Division of Basic Sciences, National Cancer Institute, National Institutes of Health, 9000 Rockville Pike, Bldg. 37, Rm. 3D25, Bethesda, MD 20892. Tel:(301) 496-9635 Fax:(301) 496-8419 E-mail:kyunglee{at}pop.nci.nih.gov.
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Abstract |
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Coordination of mitotic exit with timely initiation of cytokinesis is critical to ensure completion of mitotic events before cell division. The Saccharomyces cerevisiae polo kinase Cdc5 functions in a pathway leading to the degradation of mitotic cyclin Clb2, thereby permitting mitotic exit. Here we provide evidence that Cdc5 also plays a role in regulating cytokinesis and that an intact polo-box, a conserved motif in the noncatalytic COOH-terminal domain of Cdc5, is required for this event. Depletion of Cdc5 function leads to an arrest in cytokinesis. Overexpression of the COOH-terminal domain of Cdc5 (cdc5N), but not the corresponding polo-box mutant, resulted in connected cells. These cells shared cytoplasms with incomplete septa, and possessed aberrant septin ring structures. Provision of additional copies of endogenous CDC5 remedied this phenotype, suggesting a dominant-negative inhibition of cytokinesis. The polo-boxdependent interactions between Cdc5 and septins (Cdc11 and Cdc12) and genetic interactions between the dominant-negative cdc5
N and Cyk2/Hof1 or Myo1 suggest that direct interactions between cdc5
N and septins resulted in inhibition of Cyk2/Hof1- and Myo1-mediated cytokinetic pathways. Thus, we propose that Cdc5 may coordinate mitotic exit with cytokinesis by participating in both anaphase promoting complex activation and a polo-boxdependent cytokinetic pathway.
Key Words: Cdc5, polo-box, mitosis, cytokinesis, septin
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Introduction |
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Members of the polo subfamily of protein kinases have been identified in various eucaryotic organisms. These kinases are known to play pivotal roles in cell division and proliferation. The polo subfamily members are characterized by the presence of a distinct region of homology in the COOH-terminal noncatalytic domain, termed the polo-box (
Mammalian HeLa cells transfected with both wild-type and kinase-inactive Plk show an apparent cytokinetic defect with multiple nuclei, suggesting that overexpression of Plk interferes with cytokinesis in a manner independent of the kinase activity (
In budding yeast, the cleavage plane is specified early in the cell cycle and cleavage is achieved by a concerted process of membrane constriction by an actomyosin-based contractile ring followed by septum formation (
An actomyosin-based contractile ring forms in an ordered fashion in budding yeast (
In various organisms, it is widely appreciated that cytokinesis is preceded by inactivation of cyclin-dependent kinase Cdc2. In budding yeast, degradation of mitotic cyclins by the APC, thereby inactivating Cdc28 (functional homologue of Cdc2), is a prerequisite for cytokinesis, since cells overproducing mutant Clb2p lacking the destruction motif exhibit a mitotic exit defect with a telophase chromosome morphology (
Although the role of Cdc5 in the mitotic exit pathway is well established, it is not known whether Cdc5 activity is required for cytokinesis. This could be largely due to the lack of additional cdc5 mutants that exhibit a cytokinetic defect without inhibiting mitotic exit. We have previously shown that, in addition to spindle poles, Cdc5 localizes at cytokinetic neck filaments (
In this study, we investigated whether or not Cdc5 has an important role in cytokinesis. We demonstrate that cells depleted of Cdc5 function arrest at multiple points of M phase, including an arrest in cytokinesis. Consistent with this observation, inhibition of Cdc5 function by overexpressing the COOH-terminal domain of Cdc5 (cdc5N), but not the corresponding polo-box mutant, leads to a dominant-negative cytokinetic defect. Our data suggest that this defect is likely due to an inhibition of a direct interaction between endogenous Cdc5 and septins, Cdc11 and Cdc12, by the kinase activitydeficient cdc5
N. Remarkably, these cells appear to proceed through the cell cycle efficiently, as evidenced by cycling Cdc28/Clb2 activity, suggesting that an intact polo-box is critical for selective inhibition of cytokinesis without disturbing mitotic exit. Our data suggest that the polo-boxdependent localization of Cdc5 at cytokinetic neck filaments likely provides the temporal and spatial regulation of Cdc5, which may be important in coordinating the completion of mitosis with the initiation of cytokinesis.
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Materials and Methods |
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Plasmid Construction
All plasmids and yeast strains used in this study are listed in Table 1. To generate a GAL1-cdc5-1 construct, a PCR-amplified cdc5-1 allele from strain KKY921-2BY was digested with PpuMI and BstEII to generate pSK877 (
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To visualize the subcellular structures of spindle, septin, or contractile rings, green fluorescent protein (GFP)tagged TUB1, CYK2, MYO1, or CDC3 constructs were integrated into the genome. To generate pUC19-TUB1-GFP::LEU2 (pSK1050) and pUC19-CYK2-GFP::LEU2 (pSK1051), KpnI-NotI fragments containing either TUB1-GFP (from pAFS125; a gift of Aaron F. Straight, Harvard Medical School, Boston, MA) or CYK2-GFP (from pLP2; a gift of Rong Li, Harvard Medical School) were inserted into YCplac111 vector digested with BglII and KpnI. The resulting constructs lack both ARS and CEN loci, but bear pUC19 backbone and LEU2 gene. pUC19-MYO1-GFP::LEU2 (pSK1052) was generated by inserting a PstI-NotI fragment of MYO1-GFP (from pLP8; a gift of Rong Li) into the PstI-BglII fragment of YCplac111 lacking both ARS and CEN loci. pUC19-YFP-CDC3::LEU2 (pSK1059) was created by inserting the SstI-SphI fragment of CDC3 tagged NH2 terminally with YFP (a yellow-green variant of GFP; CLONTECH Laboratories, Inc.) into a pUC19-LEU2 construct.
Gene disruption constructs for CYK2 (pSK1330), CDC10 (pSK1332), and MYO1 (pSK1348) were generated by inserting a 1.5-kb BglII-PmeI fragment of KanMX6 from pFA6a-13Myc-KanMX6 (
Several dominant-negative cdc5N constructs were used to inhibit the function of endogenous Cdc5. A fragment of GAL1-2X(EGFP)-cdc5
N or its FAA mutant (
N, a 0.75-kb SalI-XhoI fragment containing GST open reading frame was PCR amplified using pGEX-KG (Amersham Pharmacia Biotech) as a template. This fragment was inserted into pSK983 digested with XhoI digestion to replace GFP coding sequence.
To construct plasmids for two-hybrid analyses, CDC3, CDC10, CDC11, and CDC12 were PCR-amplified using genomic clones (gifts of John Chant, Harvard University, Cambridge, MA) as templates. The EcoRI-XhoI (artificially introduced restriction enzyme sites at the 5' and 3' ends of each open reading frame) fragments were ligated into pJG4-5 plasmid digested with corresponding enzymes. This results in in-frame fusion of full-length septins to activation domain. To generate a LexA DNA binding domainfused CDC5 construct, a 2-kb XbaI fragment from pSK1006 was inserted into EcoRI-digested, end-filled pEG202-NLS (Origene Technologies Inc.). Various forms of CDC5 mutants were constructed by PCR amplification or enzymatic deletion (see Table 1 and Fig 6 C). To construct LEU2-based GAL-SIC1 plasmid, pRDB608 (a gift of Raymond Deshaies, California Institute of Technology, Pasadena, CA) was digested with NaeI and AatII to swap a URA3 fragment for a LEU2 fragment of pRS305. The resulting pSK1996 was digested with BstXI to achieve a targeted integration of GAL-SIC1 at the LEU2 locus.
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Strain Construction
All strains constructed in this study were confirmed by PCR or Southern hybridization (data not shown). A cdc5::KanMX6 mutation was introduced into strain 1783 harboring either pSK877(GAL1-cdc5-1) or pSK1267(GAL1-Plk) by a one-step gene disruption method described previously (
N under GAL1 promoter control was achieved by the integrating pSK983, pSK984, or pSK1041 into strain 1783 at the URA3 locus.
Strain KLY1229 was generated by integrating two additional copies of GAL1-HA-2X(EGFP)-cdc5N/FAA::TRP1 (pSK929) into strain KLY1081. To generate a swe1
strain (KLY1439), a 2.3-kb XbaI fragment from pSWE1-10g (
and myo1
strains, 1.8- and 2-kb BamHI-SphI fragments from pSK1332 and pSK1348, respectively, were introduced into KLY1083 to yield KLY1589 and KLY1593, respectively.
To generate strains SKY1732 and SKY1734, the CDC11 locus in KLY1083 and KLY1229 strains, respectively, were COOH-terminally tagged with 9myc epitope that is bridged with a TEV protease (GIBCO BRL) cleavage site. To generate strain SKY1779 expressing GAL-SIC1, pSK1996 was digested with BstXI and integrated into the LEU2 locus in strain KLY1083.
Growth Conditions, Media, and Zymolyase Treatment
Yeast cell cultures and transformations were carried out by standard methods (-factor mating pheromone (Sigma-Aldrich). Treatment of the connected cells with zymolyase was performed as described previously (
Immunoprecipitation, Kinase Assays, and Western Analyses
Cell lysates were prepared in TED buffer (40 mM Tris-Cl, pH 7.5, 0.25 mM EDTA, 1 mM DTT, 1 mM AEBSF) (Pefabloc; Boehringer), 10 µM/ml pepstatin A, 10 µM/ml leupeptin, and 10 µM/ml aprotinin) with an equal volume of glass beads (Sigma-Aldrich). To measure Clb2-associated Cdc28 kinase activity, the obtained lysates were spun at 15,000 g for 10 min, and the resulting supernatants were subjected to immune complex kinase assays using an antiClb2 antibody (a gift of David Morgan, University of California, San Francisco, CA) as described previously (
To examine in vivo interactions between cdc5N and septins, coimmunoprecipitation experiments were carried out using strains bearing CDC11-TEV-9myc at the CDC11 locus and expressing either GAL1-EGFP-cdc5
N (SKY1732) or GAL1-EGFP-cdc5
N/FAA (SKY1734). An antiMyc antibody cross linked to sepharose beads (BabCO) was used to precipitate Cdc11-TEV-9Myc. Immunoprecipitates were digested with TEV protease (GIBCO-BRL) according to the manufacturer's instruction, and the resulting supernatants were subjected to further analyses.
Cell Staining and Immunofluorescence Microscopy
To visualize plasma membranes, cells were stained with DiI (Molecular Probes) as described previously (
Indirect immunofluorescence was performed as described previously (
Two-Hybrid Analyses
Two-hybrid analyses were performed using a system described by
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Results |
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Loss of CDC5 Function Results in Arrests in Multiple Points of M Phase
Although it has been shown that polo kinases play important roles in multiple stages of M phase in various eucaryotic organisms, it has not been clear whether budding yeast polo kinase Cdc5 has a role other than in the mitotic exit pathway. To address this issue, we investigated the terminal morphology of a cdc5 mutant. Since overexpression of Cdc5 inhibits cell growth (
strains were generated that were kept viable by expressing either its murine functional homologue Plk (KLY1046) or the less-stable cdc5-1encoded protein (
mutation (data not shown). Both strains grow well on YEP-galactose medium, but are unable to grow on YEP-glucose (Fig 1 A). When exponentially growing cells were transferred to YEP-glucose medium, Plk was undetectable after 10 h, whereas the cdc5-1 protein disappeared after 34 h (Fig 1 B). The fast removal of cdc5-1 protein, in comparison with Plk, may be due to the presence of two putative destruction boxes in the NH2-terminal sequence of Cdc5 (
6 h after depletion of Plk or 3 h after depletion of cdc5-1. As with cells with separated chromatids, cells with disassembled spindles increased and reached plateau in 8 h for KLY1046 or 4 h for KLY1047 (Fig 1 B). To determine the percentage of cells arrested at various phases of the cell cycle, both strains were depleted of the Plk or cdc5-1 proteins for 8 or 4 h, respectively, and counted using spindle structures as a cell-cycle marker. We observed that 65% of strain KLY1046 arrested at early anaphase with a short spindle elongated to, or extended just beyond, the mother-bud neck, whereas 25% of the population were arrested at cytokinesis with disassembled spindles (Fig 1 C). In the case of strain KLY1047, 53% of the cells were arrested in cytokinesis, whereas 3 and 44% of the cell population were arrested at early anaphase and late anaphase/telophase, respectively (Fig 1 C). The complete absence of unbudded (G1) cells suggests that cells were arrested in terminal phenotypes under these conditions. In contrast, consistent with a late mitosis arrest as reported previously (
cells with disassembled spindles in both strain KLY1046 and strain KLY1047 suggests that Cdc5 activity is required at a step in cytokinesis. In addition, our data suggest that Cdc5 function is required at multiple points of M phase, including cytokinesis.
The differences observed between cdc5-1 and Plk depletion may reflect the different capacity of these two proteins to replace the function of Cdc5. In addition, the relatively high percentage of cells arrested with elongated spindles in strain KLY1047 (44%), in comparison with that seen with KLY1046 (8%) (Fig 1 C), may be attributable to the specific defect of the cdc5-1 allele at this stage of the cell cycle. It is noteworthy that the population exhibiting a cytokinetic arrest is likely underrepresented, since cells escaping earlier arrests can only achieve arrests at later points.
To closely compare the cdc5 phenotype with that of the cdc5-1 mutation, TUB1-GFP, CDC3-YFP, CYK2-GFP, and MYO1-GFP constructs were integrated into the cdc5-1 mutant strain. When these cells cultured at 35°C for 3.5 h, they exhibited homogeneous arrest at late anaphase/telophase, as indicated by elongated spindles (Fig 1 D). In addition, Cdc3 was present as double rings at the mother-bud neck, before relocalization to the future budding sites. The Cyk2 ring was never seen as a single ring in these cells and the Myo1 ring appears to maintain normal size before contraction (Fig 1 D). Since the Cyk2 double ring merges to a single ring after the completion of spindle elongation and the contraction of the Cyk2 ring follows during spindle breakdown (
1015 min in the cell cycle between double Cyk2 ring stage with incompletely elongated spindle and initiation of contraction; see
cells arrested in cytokinesis, the cdc5-1 mutant arrests in late mitosis at a step before the initiation of cytokinesis.
Induction of Connected Cells by Overexpression of the COOH-terminal Domain of Cdc5, but Not the corresponding Polo-Box Mutant
We have previously shown that Cdc5 localizes at spindle poles and cytokinetic neck-filaments (N). To this end, strain 1783 was integrated with a single copy of GAL1-EGFP, GAL1-EGFP-cdc5
N, or GAL1-EGFP-cdc5
N/FAA. These cells grow normally without any detectable morphological defect on YEP-glucose (data not shown). However, when grown in YEP-galactose, expression of EGFP-cdc5
N (KLY1082) resulted in connected cells. In contrast, cells expressing either control EGFP (KLY1080) or EGFP-cdc5
N/FAA (KLY1081) did not yield any detectable morphological changes (Fig 2 A, top). Microscopic examinations revealed that cells expressing cdc5
N yield two fluorescent bands at the mother-bud neck and fluorescent dots in the cytoplasm, whereas the EGFP control and the corresponding FAA mutant yielded only diffuse signals (Fig 2 A, bottom). The apparent multiple dot signals in strain KLY1082 may be in part attributable to the ability of cdc5
N to induce multiple subcellular structures containing Spc42, a component of spindle pole bodies (
N; described below) do not possess any detectable growth defect in the presence of the antimicrotubule drug benomyl (data not shown), suggesting that these strains grow without a significant defect in the spindle checkpoint pathway. Both EGFP-cdc5
N and EGFP-cdc5
N/FAA were expressed at similar levels, indicating that the observed phenotype associated with EGFP-cdc5
N expression was not due to a difference in protein abundance (Fig 2 B).
The Connected Cell Phenotype Is the Result of a Dominant-Negative Function of cdc5N
The observed chained cell phenotype led us to speculate that overexpression of the kinase-activitydeficient COOH-terminal domain (cdc5N) may have resulted in a dominant-negative inhibition of a cytokinetic event that is regulated by endogenous Cdc5. Thus, we examined whether provision of endogenous CDC5 in a low copy centromeric plasmid could alleviate the apparent chained cell phenotype. Cells expressing EGFP-cdc5
N under the control of GAL1 promoter (KLY1082) were transformed with wild-type and various mutant forms of Cdc5. When cultured under induction conditions for 12 h, KLY1082 cells transformed with control vector showed typical connected cell morphology in 48% of the total population (Fig 2 C). In contrast, provision of wild-type CDC5 into strain KLY1082 efficiently restored this phenotype to a wild-type morphology. However, neither the polo-box mutated cdc5/FAA nor the kinase-inactive cdc5/NA (the N209A mutation that inactivates Cdc5 kinase activity;
N overexpression is due specifically to the inhibition of endogenous Cdc5 function, and both the kinase activity and the intact polo-box are required to remedy this phenotype. Thus, it appears that the observed connected cell phenotype is the result of dominant-negative inhibition of endogenous Cdc5 function important for normal cell division. In addition, cells possessing three copies of EGFP-cdc5
N (KLY1083) exhibited a uniformly connected cell morphology in almost all cells, whereas cells expressing the same three copies of EGFP-cdc5
N/FAA (KLY1229) did not (see below). Provision of multiple copies of CDC5 into strain KLY1083 alleviated the chained cell morphology (data not shown). Thus, these cells were used for further characterization of the chained cell phenotype.
Inhibition of Cytokinesis by a Dominant-Negative COOH-Terminal Domain of Cdc5
To examine the phenotype associated with the overexpression of EGFP-cdc5N, strain KLY1083 was cultured under induction conditions in YEP-galactose. Control strains expressing either EGFP alone (KLY1080) or an equal dosage of EGFP-cdc5
N/FAA (KLY1229) were grown under the same conditions. When induced, KLY 1083 cells yielded a connected cell phenotype in a time-dependent manner, whereas cells expressing the corresponding FAA mutant appear to divide normally with wild-type morphology (Fig 3A and Fig B). Upon inducing for 9 h, 98% of the population exhibited this phenotype, and 30% of them possess >10 connected cell bodies. In contrast, cells expressing the FAA mutant did not show this morphology (Fig 3 C). In addition, the cell number of strain KLY1083 (when counting the connected cells as one cell) did not increase after shifting to the induction conditions (Fig 3 D), indicating that cells remained unseparated. However, these cells continued to grow, although slowly, as indicated by an increase in optical density of the cell culture. Under the same conditions, cells expressing either control EGFP (KLY1080) or EGFP-cdc5
N/FAA (KLY1229) exhibited a normal increase in both cell number and optical density (Fig 3 D). Western analyses revealed that both EGFP-cdc5
N and EGFP-cdc5
N/FAA were expressed at similar levels, and that they were slightly more abundant than that of a single copy EGFP-cdc5
N integrant (Fig 3 E).
The observed connected cell morphology could be achieved by various defects, such as a defect in cytokinesis, septum formation, or cell separation. To distinguish among these possibilities, KLY1083 cells cultured under induction conditions for 12 h were treated with zymolyase to remove the cell wall, and the cell number was counted. Even after an extensive zymolyase treatment, cells largely remained as clumps and unseparated cells without a significant increase in number (data not shown). These data suggest that the connected cell phenotype is the result of a cytokinetic defect, as defined by the criteria described previously (
To confirm a cytokinetic defect in strain KLY1083, cells induced for 9 h were stained with calcofluor to examine chitin deposition in cell walls and septum. Strong calcofluor bands were observed between connected cell bodies (Fig 4 A). To examine whether septum formation is completed in these cells, we performed serial optical sectioning using a confocal microscope. In most of the mother-bud necks examined, calcofluor signals were discontinuous in focal planes bisecting the cell bodies longitudinally, indicating that septa were not completely formed between the connected cell bodies (Fig 4 A). Interestingly, among the connected cells examined (n = 56), only one cell body, either in center or at one edge of the chains, possessed bud scars (revealed as fluorescent chitin rings), indicating that other cell bodies did not generate daughter cells. Since these cells do not increase in number under the induction conditions (Fig 3 D), the bud scars on the presumed mother cells are likely to be the result of previous budding events before transferring into induction conditions.
To reveal cytoplasmic membrane structures of the connected cells, the same cells used for calcofluor staining were stained with DiI. We observed that most of connected cell bodies share cytoplasm. However, it was also apparent that a fraction of mother-bud necks have closed membranes (Fig 4 B). These data suggest that some mother-bud necks overcame the cytokinetic defect imposed by overexpression of EGFP-cdc5N, but failed to complete cell division.
Cell Cycle Is Not Significantly Affected in an Early Stage of Connected Cells
To investigate whether the cell cycle is altered in connected cells, flow cytometry analyses were carried out for the cells expressing control EGFP (KLY1080), EGFP-cdc5N (KLY1083), or EGFP-cdc5
N/FAA (KLY1229). Cells arrested with
-factor were transferred into YEP-galactose medium to induce protein expression upon release from a G1 arrest. Strains KLY1080 and KLY1229 appeared to progress through the cell cycle normally, regenerating the 1C DNA-containing (G1) population
120 min after release. In contrast, strain KLY1083 expressing EGFP-cdc5
N failed to regenerate a distinct 1C (G1) peak, and continued to accumulate a DNA content greater than 2C (G2/M) peak (Fig 5 A). To further investigate whether these cells go through the cell cycle normally, the levels of Clb2 protein and Cdc28/Clb2-associated kinase activities were examined. Control strain KLY1080 achieved the maximum Cdc28/Clb2 activity (onset of M phase) in 60 and 150 min after release. Strain KLY1229 exhibited a slight delay in the cell cycle in comparison with EGFP control, whereas strain KLY1083 had a 20-min delay. However, in all cases, Clb2 protein levels and Clb2-associated kinase activities appeared to fluctuate normally with similar kinetics (Fig 5 B), suggesting that overexpression of cdc5
N did not efficiently prevent endogenous Cdc5 from activating APC. Upon induction after release, approximately equal amounts of EGFP control, EGFP-cdc5
N, and EGFP-cdc5
N/FAA proteins were expressed in these cells (Fig 5 B). These data suggest that overexpression of EGFP-cdc5
N appears to selectively inhibit cytokinesis without significantly perturbing the nuclear division cycle during the early stage of connected cells.
Disturbed Septin Structures Leads to the Cytokinetic Defect in the Connected Cells
The chained cell phenotype could be achieved by continuous division of peripheral cells in the absence of cytokinesis. To reveal the cell cycle stage of individual cell bodies in the connected cells, a wild-type strain expressing a GST-fused cdc5N (GST-cdc5
N) under control of the GAL1 promoter (KLY1053) was additionally integrated with a copy of a TUB1-GFP fusion to create strain KLY1069. Strain KLY1069 grew normally and exhibited normal spindle structures in YEP-glucose (data not shown). When these cells were cultured under induction conditions for 12 h, either a dot or short line of fluorescent signal was observed in most of internal cell bodies, indicating that these cell bodies were arrested at a point after spindle disassembly. In contrast, mitotic spindle structures were often observed in cell bodies present at the periphery of chained cells (Fig 6 A), suggesting that cells at the edges are active in cell division. A similar observation was made when connected cells observed with strain KL1083 were immunostained with an antitubulin antibody (data not shown). The fact that most internal cell bodies possess disassembled spindles and do not bear buds suggests that a prolonged inhibition of cytokinesis in these cell bodies may have resulted in an inhibition of the next round of the cell cycle.
Inhibition of cytokinesis in connected cells could be the result of a failure either in recruitment of cytokinetic materials or in the function of cytokinetic structures. To investigate these possibilities, strain KLY1053 was additionally integrated with CDC3-YFP (KLY1075), CYK2-GFP (KLY1071), or MYO1-GFP (KLY1073) under control of their own promoters. These strains grew normally with apparently normal ring structures when cultured in YEP-glucose (data not shown). Upon induction of GST-cdc5N, cells were then examined to determine whether these components formed normal ring structures. (Fig 6 B and 7 A). At an early stage of induction, distinct septin ring structures were observed at all the mother-bud necks of connected cells, indicating that continuous budding events have occurred in the absence of cytokinesis at the previous mother-bud necks. Upon inducing for 12 h, double YFP-Cdc3 rings were found to be distantly placed at the mother-bud neck or remnants of YFP-Cdc3 were placed at one side of the mother-bud neck, suggesting a disturbance in maintaining properly organized septin ring structures or a defect in septin ring disassembly and relocalization. In addition, unusually wide or tiny rings of Cdc3 were occasionally observed at the axial position of incipient budding site without formation of a noticeable bud (Fig 6 B), suggesting that a fraction of cell bodies were capable of relocalizing septins to the future budding sites but failed to assemble or maintain proper septin ring structures. Taken together, in the presence of dominant-negative cdc5
N, septin rings appear to be assembled normally at the growing edge of the connected cells, thereby permitting continuous budding events. However, these ring structures are cytokinesis incompetent, resulting in the generation of connected cell morphology. As with septin ring structures persisting at most of the mother-bud necks of connected cells, both Cyk2-GFP and Myo1-GFP ring structures were also remained at these sites (Fig 7 A). This observation further supports the notion that cytokinetic processes have failed in these cells.
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In contrast to double Cyk2-GFP rings observed with the cdc5-1 mutant at the restrictive temperature (Fig 1 D), it was apparent that connected cells possess single Cyk2-GFP rings between cell bodies. Since double Cyk2 rings becomes a single ring structure at the time of cytokinesis (
Polo-Boxdependent Interactions between Cdc5 and Septins
Since Cdc5 localizes at cytokinetic neck filaments and overexpression of cdc5N induces aberrant septin ring structures with a connected cell morphology, we investigated whether Cdc5 directly interacts with septins in a yeast two-hybrid system. To increase protein stability, a destruction-boxdeficient form of Cdc5 (
N, but not the cdc5
N/FAA, interacted strongly with both Cdc11 and Cdc12 (Fig 6 C). No interaction was detected between the NH2-terminal domain of Cdc5 (cdc5
C) and septins. Western blot analyses revealed that septins and various forms of Cdc5 were expressed at similar levels (data not shown).
To examine whether Cdc5 interacts with septins in vivo, coimmunoprecipitation experiments were carried out using strains bearing a TEV-9myc tag at the CDC11 locus and expressing either GAL1-EGFP-cdc5N (SKY1732) or GAL1-EGFP-cdc5
N/FAA (SKY1734). Our data show that
30% of cdc5
N present in the S15 lysates were coimmunoprecipitated with Cdc11. However, no such interaction was observed with cdc5
N/FAA (Fig 6 D). Similar results were also obtained with Cdc12-TEV-Myc precipitates (data not shown). These data along with two-hybrid interaction analyses strongly suggest that the polo-box domain is critical for the interactions between Cdc5 and the septins, Cdc11 and Cdc12. These observations further suggest that the connected cell morphology could be the result of a disturbance in septin ring structure through direct interactions between cdc5
N and septins.
Enhancement of Cytokinetic Defects by Overexpression of cdc5N in cyk2
or myo1
Mutants
Although septin ring structures are largely disturbed in the connected cells, the presence of contraction size Cyk2 or Myo1 rings (Fig 7 A) suggests that overexpression of cdc5N did not completely eliminate the function of septin rings in these cells. Vallen et al. (2000) suggest that two cytokinetically important components, Myo1 and Cyk2, function in parallel pathways (see Discussion). Since both of these components localize at neck-filaments in a septin-dependent manner (
N partially inhibits septin function, introduction of either the cyk2
or the myo1
mutation into the connected cells may enhance the severity of the chained cell phenotype. To test this idea, strain KLY1083 was modified with an additional cyk2
(KLY1591), myo1
(KLY1593), or cdc10
(KLY1589) mutation and examined under induction conditions. Introduction of additional cyk2
or myo1
into KLY1083 strain resulted in a synthetic growth defect. However, introduction of cdc10
did not reveal this phenomenon (Fig 7 C), most likely because septin ring structures are already impaired by overexpression of cdc5
N. During the initial stage of induction (up to 6 h), both KLY1591 and KLY1593 cells yielded a significantly enhanced connected cell morphology, in comparison with those of the corresponding cyk2
or myo1
single mutants or the cells overexpressing cdc5
N alone (data not shown). These results indicate that the synthetic growth defect is the result of the synthetic cytokinetic defect between cdc5
N and either cyk2
or myo1
. In contrast, introduction of either cyk2
or myo1
mutation into the cdc5-1 mutant failed to reveal any synthetic defect under various conditions tested (data not shown). These data further support our notion that the dominant-negative cytokinetic defect observed with strain KLY1083 differs from the mitotic exit defect in cdc5-1 mutant. In addition, our data support the argument that the cytokinetic pathways regulated by Cyk2 and Myo1 are mediated by septins.
Induction of Cytokinetic Defects by a Dominant-Negative cdc5 Is Not the Result of a Swe1-dependent Cell Cycle Delay
It has been shown that defects in septin assembly cause a G2 delay in a Swe1-dependent manner, resulting in a filamentous phenotype (, kcc4
, gin4
mutant require the Swe1 kinase (
into KLY1083 strain (KLY1439) did not influence cell growth or the chained cell phenotype associated with overexpression of cdc5
N (Fig 7c and Fig D). In addition, overexpression of cdc5
N induced a connected cell morphology in a strain possessing an activated CDC28 allele (CDC28/Y19F) as the sole CDC28 locus (data not shown). These observations indicate that the cytokinetic defect associated with overexpression of cdc5
N differs from the phenotype associated with Cdc28 inactivation.
When cultured under the induction conditions, strain KLY1083 exhibited defects in septin ring structure with a 20-min delay in the cell cycle (Fig 5 B and 6 B). Since it is possible that this delay may have contributed to the cytokinetic defect induced by overexpression of cdc5N, we closely monitored the cell cycle progression of strain KLY1083 and the corresponding swe1
strain (KLY1439) by analyzing the Clb2 levels. Control strain KLY1229, which expresses cdc5
N/FAA without cytokinetic defect, achieved the maximum Clb2 level
70 min after release from
-factor block, whereas the Clb2 level peaked at 80 min in strain KLY1083. Introduction of swe1
into strain KLY1083 (KLY1439) abolished the delay in Clb2 accumulation and restored the cell cycle to a degree similar to that of strain KLY1229 (Fig 7 E). These data suggest that disruption of septin ring structures by overexpression of cdc5
N (Fig 6 B) may have induced a Swe1-dependent cell cycle delay through activation of a septin assembly checkpoint pathway. However, restoration of the cell cycle by introducing swe1
did not influence the chained cell phenotype of strain KLY1083 [96% (153/160) after culturing under the induction conditions for 10 h; Fig 7 D].
Since it is generally believed that inactivation of Cdc28/Clb2 is required for the initiation of cytokinesis, a delayed inactivation of Cdc28/Clb2 itself may have prevented the onset of cytokinesis or contributed to the cytokinetic defect induced by overexpression of cdc5N. To eliminate this possibility, GAL-SIC1, a Cdc28/Clb2 inhibitor, was introduced at the LEU2 locus of strain KLY1083 (SKY1779), and cultured under the induction conditions. However, overexpression of GAL-SIC1 did not influence the capacity of cdc5
N to induce chained cells [97% (145/150) after culturing under the induction conditions for 10 h; Fig 7 D]. Overexpression of GAL-SIC1 itself did not induce chained cell morphology in an isogenic wild-type strain (data not shown). The GAL-SIC1 appears to be functional since it inhibited the Cdc28/Clb2 activity of strain SKY1779 (40% inhibition after 4-h induction), as determined by antiClb2 immunocomplex kinase assays using cells arrested in M phase with nocodazole treatment for 4 h (data not shown). In addition, it was able to suppress the mitotic-exit defect associated with the cdc5-1 mutation (data not shown), as previously reported (
Taken together, the dominant-negative cytokinetic defect associated with overexpression of cdc5N is apparently the result of a specific inhibition of cytokinesis, but not of the Swe1-dependent cell cycle delay or the delayed inactivation of Cdc28/Clb2 activity.
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Discussion |
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The Role of Cdc5 in Cytokinesis
Cytokinesis is a highly coordinated cellular and biochemical process by which a eucaryotic cell assures the equipartition of its chromosomes and cytosolic contents. It comprises a complex set of motile events, such as reorganization of microtubules and formation of cytokinetic ring structures. Data obtained from Drosophila suggest that polo plays a role in cytokinesis (
Our data demonstrates that overexpression of cdc5N, but not the corresponding polo-box mutant, results in dominant-negative inhibition of cytokinesis without interfering with mitotic exit. Overexpression of cdc5
N induces a disturbance in septin ring structures and Cdc5 interacts with two septins, Cdc11 and Cdc12, in a polo-boxdependent manner. In addition, in strain KLY1053 expressing GST-cdc5
N under the GAL1 control, the bud-neck localization of ADH1-EGFP-CDC5/N209A was greatly diminished (data not shown). Taken together, the dominant-negative cytokinetic defect is likely the result of overexpressed cdc5
N that may have prevented endogenous Cdc5 from interacting with septins and carrying out its cytokinetic function.
The septins are thought to be the major structural components of the neck filaments (N at the mother-bud neck may require septins and higher-order cytokinetic neck filaments. Since a cdc10
mutant grows normally at 23°C, but does not possess detectable neck filaments (
mutation was introduced into KLY1083 strain (KLY1589). When strain KLY1589 was cultured under the induction conditions, localization of EGFP-cdc5
N was greatly diminished, but was not completely eliminated (data not shown). These data suggest that intact neck filaments are likely to be important for the localization of cdc5
N. Septins (Cdc3 and Cdc11) still localize at the mother-bud necks in the absence of Cdc10 (
N localized at these sites may reflect inefficient interactions with other septins or other components at the neck filaments in the absence of Cdc10. Although our data suggest that septins are likely the targets of cdc5
N binding, we cannot rule out the possibility that cdc5
N also interacts with additional component(s) other than septins at the mother-bud necks.
What role does Cdc5 play after localizing at cytokinetic neck filaments in a polo-boxdependent manner? Since Cdc5 is expressed in a late phase of the cell cycle and its kinase activity peaks in mitosis ( cells were depleted of Plk protein for 10 h, a large fraction of cells (51%, 227/442 cells counted) possessed severely disturbed septin rings. Taken together, Cdc5 activity may not be required for the assembly of septin rings into a higher-order structure (
N. Since remnants of septin materials are found between mother-bud necks without proper relocalization to the future budding sites, overexpression of cdc5
N may also have disturbed a step or steps important for disassembly of septin ring structures.
Our data suggest that overexpression of a dominant-negative cdc5N induces a partial inhibition of cytokinesis as demonstrated by the presence of contractile ring size Cyk2 and Myo1 rings and occasional membrane closures. In budding yeast, cytokinesis is carried out by at least two separate pathways: an actomyosin ring-dependent pathway and an alternative pathway mediated by localized chitin depositions and cell-wall synthesis (
or cyk2
into the strain overexpressing cdc5
N results in enhanced cytokinetic defects (Fig 7 C). These data strengthen the view that septins play a critical role in mediating both actomyosin-based and alternative cytokinetic pathways.
Dominant-Negative cdc5N Mutant Versus Septin Mutants
Loss of septin function results in a cytokinetic defect with a chained-cell morphology (N. However, these phenotypes differ from each other in several important aspects. At the restrictive temperature, septin mutants accumulate multinucleated cells with hyperpolarized buds (
N exhibit round cell bodies in connected cells and form colonies on YEP-galactose medium. These cells go through the cell cycle efficiently with cycling Cdc28/Clb2 activity. In the absence of cell division, these cells continue to increase the cell mass by continuous budding events at the periphery of the chained cells.
Mutations in septins have been shown to result in a defect in bud-site selection (
One interesting observation is that most internal cells possess short spindles (Fig 6 A), indicating that cells arrested at a point after spindle disassembly. In addition, these cell bodies failed to generate buds, suggesting an arrest in G1. Our data also show that inactivation of Cdc28, thereby mitotic exit, occurs normally in these cells in an early stage of the cell cycle (Fig 5 B and 7 E). Taken together, these observations allow for an intriguing possibility that a failure in cytokinesis may be detected by an unknown mechanism that leads to the cell cycle arrest in G1.
Temporal and Spatial Regulation of Mitotic Exit and Cytokinesis
Although a growing body of evidence suggests that members of the polo kinase subfamily play multiple roles such as centrosome maturation, bipolar spindle formation, activation of APC, and cytokinesis during M phase progression, it is also apparent that their roles are disparate in different organisms. For instance, studies with fission yeast Plo1 revealed that its function is important for bipolar spindle formation and cytokinesis. However, there is to date no indication of Plo1 function in the activation of APC. In budding yeast, even though polo kinase has a role in the mitotic exit pathway leading to the activation of APC, it is not known whether Cdc5 plays a role in spindle function or cytokinesis. These apparent discrepancies may be in part due to the specialization of polo kinase function among evolutionarily distant organisms, and their roles may have remained largely unchanged throughout evolution.
Our data suggest that Cdc5 plays dual roles in a late stage of M phase. We propose that, in addition to activation of APC, Cdc5 activity is required for proper function of septin ring structures during cytokinesis (Fig 8). In this scenario, during or shortly after activation of APC, a fraction of Cdc5 relocalizes to bud-neck to carry out its cytokinetic function, an event that requires an intact polo-box. A dominant-negative cdc5N, which localizes at the neck-filament, does not interfere with APC activation and mitotic exit pathway. However, it inhibits Cdc5 localization at the neck filaments, thereby impairing septin functions critical for cytokinesis. Our model also helps explain the phenotypes associated with overexpression of Cdc5 (
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Footnotes |
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1 Abbreviations used in this paper: APC, anaphase promoting complex; GFP, green fluorescent protein; HA, hemagglutinin.
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Acknowledgements |
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We are grateful to Raymond Deshaies, Orna Cohen-Fix, Philip Lee, Rong Li, and Michael Lichten for critical reading of this manuscript, and Erie Lee and Dan Ilkovitch for technical support. We also thank Sue Jaspersen and David Morgan for the provision of antiClb2 antibody and Raymond Deshaies for antiCdc28 antibody and the GAL-SIC1 construct, Aaron Straight for a Tub1-GFP construct, Rong Li and John Lippincott for a GFP-Cyk2 and a GFP-Myo1 construct, and Mark Longtine for KanMX6 construct. We also acknowledge Susan Garfield for help with confocal microscopy and Jim McNally and Tatiana Kapova for processing confocal images obtained at the LRBGE Fluorescence Imaging Facility in NCI/DBS.
Submitted: 12 April 2000
Revised: 5 December 2000
Accepted: 12 December 2000
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References |
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