Regulation of the Anaphase-promoting Complex/Cyclosome by bimAAPC3 and Proteolysis of NIMA

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Vol. 9, Issue 11, 3019-3030, November 1998

Regulation of the Anaphase-promoting Complex/Cyclosome by bimA^APC3 and Proteolysis of NIMA

Xiang S. Ye,^* Russell R. Fincher, Alice Tang, Aysha H. Osmani, and Stephen A. Osmani

Henry Hood Research Program, Weis Center for Research, Pennsylvania State University College of Medicine, Danville, Pennsylvania 17822

Submitted June 16, 1998; Accepted August 19, 1998
Monitoring Editor: Marc W. Kirschner

	ABSTRACT

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Surprisingly, although highly temperature-sensitive, the bimA1^APC3 anaphase-promoting complex/cyclosome (APC/C) mutation does notcause arrest of mitotic exit. Instead, rapid inactivation of bimA1^APC3 is shown to promote repeating oscillations of chromosome condensationand decondensation, activation and inactivation of NIMA and p34^cdc2 kinases, and accumulation and degradation of NIMA, which allcoordinately cycle multiple times without causing nuclear division.These bimA1^APC3-induced cell cycle oscillations require active NIMA, becausea nimA5 + bimA1^APC3 double mutant arrests in a mitotic state with very high p34^cdc2 H1 kinase activity. NIMA protein instability during S phase andG2 was also found to be controlled by the APC/C. The bimA1^APC3 mutation therefore first inactivates the APC/C but then allowsits activation in a cyclic manner; these cycles depend on NIMA.We hypothesize that bimA^APC3 could be part of a cell cycle clock mechanism that is reset afterinactivation of bimA1^APC3. The bimA1^APC3 mutation may also make the APC/C resistant to activation by mitoticsubstrates of the APC/C, such as cyclin B, Polo, and NIMA, causingmitotic delay. Once these regulators accumulate, they activatethe APC/C, and cells exit from mitosis, which then allows thiscycle to repeat. The data indicate that bimA^APC3 regulates the APC/C in a NIMA-dependentmanner.

	INTRODUCTION

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The bimE and bimA genes were originally defined by temperature-sensitive mutations in functions required for normal progressionthrough mitosis in Aspergillus nidulans (Morris, 1976; Osmaniet al., 1988; Engle et al., 1990; O'Donnell et al., 1991) andwere subsequently found to encode highly conserved proteins whosehomologues have been isolated from many organisms ranging fromfungi to humans (Hirano et al., 1990, 1994; Mirabito and Morris,1993; Lamb et al., 1994; Starborg et al., 1994; King et al., 1995;Tugendreich et al., 1995). Most significantly, they were recentlyidentified as components of the anaphase-promoting complex (APC)(King et al., 1995; Peters et al., 1996; Zachariae et al., 1996).The APC is also known as the cyclosome (Sudakin et al., 1995)and is therefore abbreviated here to APC/C (see Townsley and Ruderman,1998, forreview).

bimE encodes the largest subunit of the APC/C and has recently been termed APC1 (Peters et al., 1996). We will use the designationbimE^APC1 for the gene and BIME^APC1 for the protein. bimA encodes a member of the tetratricopeptiderepeat family of proteins, being most similar to Schizosaccharomycespombe nuc2 (Hirano et al., 1990, 1994) and Saccharomyces cerevisiaeCDC27 (Sikorski et al., 1990; Lamb et al., 1994), which was recentlytermed APC3 (Peters et al., 1996). The APC/C functions as an E3ubiquitin ligase, which specifically targets proteins (such asmitotic cyclins) for degradation in a destruction box (D box)-dependentmanner (Glotzer et al., 1991; King et al., 1996b) through theubiquitin-proteasome pathway, to promote initiation of anaphaseand exit from mitosis into G1 (for reviews see Murray, 1995; Kinget al., 1996a; Hershko, 1997; Townsley and Ruderman, 1998).

APC/C activity is cell cycle regulated (Hershko et al., 1994; Zachariae and Nasmyth, 1996) potentially by reversible phosphorylation(Lahav-Baratz et al., 1995) of certain subunits (Peters et al.,1996). Recent data indicate that Polo-related kinases play a rolein the activation of the APC/C during mitosis (Charles et al.,1998; Descombes and Nigg, 1998; Shirayama et al., 1998). In S.cerevisiae, the APC/C is activated during the metaphase to anaphasetransition and remains active during G1 (Amon et al., 1994), asalso occurs in mammalian cells (Brandeis and Hunt, 1996). As cellsprogress into S phase from G1, mitosis-specific APC/C activityis turned off to allow accumulation of mitotic cyclins in preparationfor the nextmitosis.

It has been shown that the APC/C subunit BIME^APC1 also has an interphase function to negatively regulate mitosis, as loss of BIME^APC1 overrides the nimA5 G2 arrest and, in combination with non-tyrosinephosphorylatedp34^cdc2, promotes premature mitosis from S phase (Osmani et al., 1988;James et al., 1995; Ye et al., 1996). It has been proposed thatsome checkpoint controls over mitosis are switched from the APC/Cduring G1 to include tyrosine phosphorylation of p34^cdc2 upon initiation of DNA replication (Ye et al., 1997a). BIME^APC1 may therefore normally play a role to prevent activation of NIMAkinase, and other mitotic regulators, during interphase to preventprematuremitosis.

The levels of NIME^cyclinB and NIMA proteins oscillate once each cell cycle in a strikingly similar manner (Evans et al., 1983; Alfaet al., 1990; Draetta et al., 1990; Ghiara et al., 1991; Huntet al., 1992; Richardson et al., 1992; Grandin and Reed, 1993;Pu and Osmani, 1995; Ye et al., 1995; Yamano et al., 1996). Bothproteins accumulate during late S to G2, peak at early M, andare rapidly degraded as cells progress out of mitosis with slightlydifferent kinetics (Pu and Osmani, 1995; Ye et al., 1995). Ifcells are arrested at mitosis, for instance by the bimE7^APC1 mutation or by addition of nocodazole, then both NIME^cyclinB and NIMA proteins remain stable (Ye et al., 1995). Additionally,degradation-deficient forms of either cyclin B (Murray et al.,1989; Luca et al., 1991; Gallant and Nigg, 1992; Surana et al.,1993) or NIMA (O'Connell et al., 1994; Pu and Osmani, 1995) preventnormal exit from mitosis. This raises the possibility that thedegradation of NIME^cyclinB and NIMA proteins may be mediated, at least partly, by the sameproteolytic pathway. Although the mitosis-specific proteolysisof cyclin B through D box-directed ubiquitination has been wellcharacterized in several systems (see Murray, 1995, for review),how NIMA kinase is specifically degraded during M phase progressionis not understood. The determinants for mitotic instability ofNIMA reside in its C-terminal domain, which contains PEST sequencesand p34^cdc2 phosphorylation sites (O'Connell et al., 1994; Pu and Osmani,1995).

In the present work, experiments using APC/C mutations and biochemical analysis of NIMA stability uncover a regulatory rolefor BIMA^APC3 involving APC/C-dependent instability ofNIMA.

	MATERIALS AND METHODS

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Aspergillus Strains and General Techniques

Strains of A. nidulans used in this study were R153 (pyroA4; wA3); GR5 (pyrG89; pyroA4; wA3); SO1 (bimE7; pyrG89; pyroA4;wA2); SO4 (bimE7; pabaA1; wA2); SO15 (nimA5; bimE7; pabaA1; riboB2;wA2); SO54 (nimA5; wA2); 5C (alcA::nimA, pyr4⁺; pyrG89; benA22; pabaA1; fwA1); RP5 (alcA::nimA; pyrG89, pyr4⁺; nicB8; riboA1; yA2); MAT68 (alcA::nimE at argB; pabaA1); AT62(bimA1; alcA::nimA, pyr4⁺; pyrG89; choA1; pabaA1); AT92 (alcA::nimE at argB; choA1; yA2);AT114 (bimE7; alcA::nimE at argB; yA2); AT120 (bimA1; alcA::nimEat argB; choA1; yA2); AT128 (bimE7; alcA::nimA, pyr4⁺ pyrG89; wA2); and PM156 (bimA1; pabaA1; wA2). Media and generaltechniques for culture, transformation, light microscopy, proteinextraction, immunoprecipitation, protein kinase assays, and Westernblotting were as previously described (Ye et al., 1995). NIMAand p34^cdc2 H1 kinase activities were quantified, based on incorporationof ³²P into their in vitro substrates $beta$ -casein and histone H1, usinga PhosphorImager (Molecular Dynamics, Sunnyvale, CA). The relativeamount of NIMA and NIME^cyclinB was measured after Western blotting with the use of a densitometerand ImageQuant software (MolecularDynamics).

nimA Deletion

A 5.0-kb KpnI fragment containing the nimA open reading frame was cloned into pGEM giving rise to plasmid pWC1. A PstI fragment,129 bp upstream of the start codon and 83 bp before the stop codonof nimA, was replaced with the PstI fragment of the pyr4 genefrom Neurospora crassa, which complements the pyrG89 mutationof A. nidulans. Two plasmids containing opposite orientationsof the pyr4⁺ gene were obtained called pnimA $Delta$ A and pnimA $Delta$ B. A linear KpnIfragment from pnimA $Delta$ B, as shown in Figure 7A, was used to deletenimA by transformation of GR5 andSO1.

Transformants were screened for heterokaryons (Osmani et al., 1988) by streaking conidiospores (conidia) onto selective YAGwithout uridine and uracil. If a transformant is maintained asa heterokaryon conidia derived from such a transformant, it willnot be able to grow in the absence of uridine and uracil. Thisis because conidia containing the parental nuclei (they are uninucleate)will not be able to germinate in the absence of uridine and uracilbecause of the pryG89 mutation. On the other hand, conidia containingdeleted nimA, which can germinate in the absence of uridine anduracil because of the pyr4⁺ gene, will not be able to undergo nuclear division and will ceasegrowth as a single nucleate germling (Osmani et al., 1988). Suspectedheterokaryons were maintained as mycelial colonies on selectivemedium.

Southern blot analysis of selected heterokaryons was carried out to confirm specific nimA deletion. Isolated DNA was digestedto completion with XhoI, separated by electrophoresis, and blottedonto nylon membranes. A 0.8-kb KpnI-PstI fragment was isolatedfrom pWC1 and was used as probe for random primer labeling. Hybridizationconditions were as previously described (Ye et al., 1996).

Temperature Shifts

We usually do temperature upshift to 42°C by vigorously shaking the culture in a 60°C water bath. In this study, we also harvestedAspergillus cells by vacuum filtration through a layer of Miracloth(Calbiochem-Novabiochem, La Jolla, CA) and then transferred thecells directly to prewarmed medium at 42°C to cause instant temperaturechange of theculture.

Induction and Repression of NIME^cyclinB and NIMA Expression from the alcA Promoter

Induction and repression of NIMA and NIME^cyclinB expression from the alcA promoter were as previously described (Pu and Osmani, 1995).In this study, we also incorporated hydroxyurea (100 mM) intothe medium to cause S phase arrest before ethanolinduction.

	RESULTS

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Unsuccessful Cell Cycle Oscillations Are Induced by Rapid Inactivation of bimA^APC3

Temperature-sensitive mutations in two genes, bimA^APC3 and bimE^APC1, which both encode components of the APC/C, have been previouslyidentified in A. nidulans (Morris, 1976; Engle et al., 1990; O'Donnellet al., 1991; King et al., 1995; Tugendreich et al., 1995; Peterset al., 1996; Zachariae et al., 1996). When shifted to restrictivetemperature, the bimE7^APC1 mutation causes a rapid cell cycle arrest in mitosis (Morris,1976; Osmani et al., 1988; James et al., 1995), consistent withthis mutation causing inactivation of APC/C function and preventingmitotic exit. However, the bimA1^APC3 mutation takes much longer to cause a mitotic arrest (O'Donnellet al., 1991), even though this allele is more temperature sensitivethan bimE7^APC1 (Figure 1). The extreme temperature sensitivity caused by bimA1^APC3, and the lack of first cell cycle arrest in mitosis caused bythis mutation, indicate that irreversible loss of APC/C functionis not caused by the bimA1^APC3 allele at restrictive temperature.

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Figure 1. Temperature sensitivity of bimA1^APC3 and bimE7^APC1 strains. Strains containing no temperature-sensitive mutation (R153) or bimA1^APC3 (PM156) or bimE7^APC1 (SO4) were replica plated and incubated at permissive temperature (30°C) or semirestrictive temperature (35°C) for 3 d. Greater temperature sensitivity caused by bimA1^APC3 when compared with bimE7^APC1 is apparent.

In an attempt to generate a more effective mitotic block with bimA1^APC3, we transferred cells, after filtration from 32°C medium, directlyinto medium prewarmed to 42°C with the expectation that this maymore immediately inactivate APC/C function. This shortened theperiod to attain restrictive temperature from several minutes,using our standard technique, to a matter of a second or so. Toour surprise, the instant temperature shift induced multiple synchronizedmitotic oscillations, of increasing magnitude, with four peaksof chromosome mitotic index (CMI) occurring over 12 h (Figure2A). This was specific for the bimA1^APC3 mutation, as such synchronized mitotic oscillations were absentin wild-type and bimE7^APC1 mutant cells when treated identically (our unpublished results).When bimA1^APC3 mutant cultures were shifted to 42°C by shaking in a 60°C waterbath (our standard temperature shift regimen), no cell cycle synchronywas apparent, but instead the CMI increased slowly to ~70% by8 h after temperature shift.

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Figure 2. Mitotic oscillations induced by bimA1^APC3 upon rapid temperature shift. (A) CMI of a bimA1^APC3 mutant strain after rapid temperature shift. (B) Autoradiograms of p34^cdc2 H1 and NIMA kinase activities and Western blot analysis of NIMA, NIME^cyclinB, and p34^cdc2. (C) Nuclear division and germling growth of the nimA5+ bimA1^APC3 mutant cells after rapid temperature upshift. Spores were first germinated at 32°C for 7.5 h, and, after harvesting by centrifugation, the germlings were rapidly transferred to new medium prewarmed to 42°C and incubated at 42°C for 8 h. The number of nuclei and germling length were measured before and 8 h after temperature shift.

As rapid temperature-shifted bimA1^APC3 cultures underwent repeated rounds of chromosome condensation, we followed biochemicallythe abundance and activities of several mitotic regulators duringthese apparent cell cycle oscillations (Figure 2B). Both the activitiesof p34^cdc2 and NIMA mitotic-promoting kinases oscillated in the same manneras the CMI values. When the CMI was low, the mitotic kinase activitieswere low, and when the CMI was high, so were the kinase activities,most noticeably for NIMA kinase activity (Figure 2B). The chromosomemitotic oscillations caused by rapid inactivation of bimA1^APC3 are therefore clearly cell cycle oscillations driven by activationand inactivation of mitosis-promoting protein kinases. This conclusionwas further ratified by the dramatic periodic accumulation andhyperphosphorylation, followed by degradation, of the NIMA proteinrevealed by Western blot analysis (Figures 2B and 4B, NIMA). Nosuch oscillation in p34^cdc2 abundance was detected, and only minor oscillations of NIME^cyclinB protein could be detected (Figure 2B).

The oscillations in cell cycle parameters caused by rapid inactivation of bimA1^APC3 did not lead to successful nuclear division. If relatively youngcultures, which contained germlings having two to four nucleiper cell, were shifted rapidly to restrictive temperature, virtuallyno increase in nuclear number was observed (Figure 2C). The germlingsdid continue to grow, but they were unable to complete successfulmitotic division over a period in which at least two divisionswould be expected to have taken place. In addition, it shouldbe noted that no obvious increase in DNA ploidy occurred, basedon DAPI staining, during the bimA1-induced cell cycle oscillations.During incubation at 42°C for 13 h (e.g., Figure 2) the normal1n ploidy of A. nidulans should have increased to 16n if DNA synthesiswas occurring without division. However, no such large nucleiwere observed during these experiments (our unpublishedresults).

To determine the role of NIMA in the cell cycle oscillations caused by inactivation of bimA^APC3, a double bimA1^APC3 + nimA5 mutant strain was constructed and subjected to the rapidtemperature shift protocol. In this double mutant no significantoscillation of p34^cdc2 kinase activity was apparent, but instead p34^cdc2 kinase activity dramatically increased 10-fold, and the chromosomemitotic index also increased to a high sustained level with onlyminor variations (Figure 3A). Additionally, no oscillations wereobserved in the level or phosphorylation state of NIMA or NIME^cyclinB; rather, these two proteins accumulated after the temperatureshift (Figure 3B). These data indicate that active NIMA is requiredto generate the cell cycle oscillations observed after rapid inactivationof bimA^APC3. The data also indicate that rapid inactivation of bimA^APC3 can apparently override the G2 arrest caused by nimA5 in a mannerreminiscent of how bimE7^APC1 also overrides the nimA5 G2 arrest (Osmani et al., 1988, 1991b;James et al., 1995) (see below).

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Figure 3. nimA dependence of the mitotic oscillations induced by bimA1^APC3. (A) CMI of a nimA5 + bimA1 double mutant strain after rapid temperature shift. (B) Autoradiogram of p34^cdc2 H1 kinase activity and Western blots of NIMA, NIME^cyclinB, and p34^cdc2 after rapid temperature shift.

The mitotic oscillations promoted by rapid temperature shift of bimA1^APC3-containing cells were also tested for sensitivity to checkpointcontrol mechanisms. Mitotic oscillations were instigated by rapidtemperature shift to 42°C. After 4 h incubation, cells were testedfor the DNA damage checkpoint by using methyl methanesulfonate(MMS) and were also treated with the microtubule poison nocodazole,which is known to generate a pseudomitotic arrest. No effect wasobserved on the oscillations of either the CMI or NIMA or p34^cdc2 kinase activities after treatment with MMS (Figure 4, A and B),whereas, as noted previously, the wild-type delays the cell cycleafter sustaining DNA damage by inactivating p34^cdc2 (Ye et al., 1997b). Again the oscillations observed after MMStreatment were particularly apparent for the abundance and phosphorylationstate of NIMA. In contrast, addition of nocodazole largely suppressedthe cell cycle oscillations, and these cells arrested with highCMI values (Figure 4A) and also high levels of NIMA, NIME^cyclinB, and NIMA and p34^cdc2 kinase activities (our unpublished results). These results suggestthat, after rapid temperature shift, the bimA1^APC3 mutant cells have lost the DNA damage checkpoint but still havean intact spindle assembly checkpoint. The ability of nocodazoleto trap bimA1^APC3 cells in mitosis also confirms that this mutation causes a reversibledelay to mitotic progression and not an arrest in mitosis.

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Figure 4. Effects of addition of nocodazole and MMS on the bimA1^APC3-induced mitotic oscillations. Nocodazole or MMS was added to bimA1^APC3 mutant cells 4 h after temperature shift and remained in the culture during the duration of the experiment. (A) CMI. (B) Autoradiograms of p34^cdc2 H1 and NIMA kinase activities and NIMA Western blot in the MMS-treated bimA1^APC3 cells.

NIMA and NIME^cyclinB Are Stabilized in Cells with Inactive bimE^APC1 and bimA^APC3

Previous work has demonstrated that NIMA protein abundance is regulated in a cell cycle-dependent manner, being low duringS phase and maximal at mitosis, similar to cyclin B (Ye et al.,1995). Additionally, degradation of NIMA, also like cyclin B,is required for exit from mitosis (O'Connell et al., 1994; Puand Osmani, 1995), and the APC/C is known to regulate the stabilityof other mitotically unstable proteins (for review see Cohen-Fixand Koshland, 1997; Townsley and Ruderman, 1998). These observations,and the dramatic oscillations in NIMA abundance caused by rapidinactivation of the APC/C subunit bimA^APC3 (Figures 2B and 4B), prompted us to investigate the potentialrole of the APC/C in the regulation of NIMAstability.

To directly assess the role of the APC/C in NIMA degradation, we measured the stability of NIMA expressed from the heterologousalcA promoter in S phase-arrested cells, as we have shown previouslythat NIMA is very unstable during S phase arrest (Ye et al., 1995;Ye et al., 1996). The stability of NIME^cyclinB when expressed from the alcA promoter was similarly determined.Three conditions were used: stability with normal APC/C function,stability with bimA^APC3 inactivated, and stability with bimE^APC1 inactivated. As shown in Figure 5, A and B, in the presence ofAPC/C function both NIME^cyclinB and NIMA are unstable in the hydroxyurea (HU)-arrested S phasecells with a half-life of <20 min. In contrast, both NIME^cyclinB and NIMA are greatly stabilized when the APC/C subunit BIMA^APC3 was inactive, and their half lives were increased to >60 min.Similar results were obtained when the BIME^APC1 APC/C component was inactivated and both NIME^cyclinB and NIMA proteins were both highly stabilized (our unpublishedresults). These results provide strong biochemical evidence fora role of the APC/C in NIMA degradation at a point in the cellcycle where NIMA is known to be unstable.

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Figure 5. APC/C-dependent stabilization of NIME^cyclinB and NIMA. (A) Cells of the wild-type (wt = R153) and bimA1^APC3 cells containing a copy of alcA-driven nimE^cyclinB were grown at 32°C to early log phase in acetate media (repressing for alcA). HU (100 mM) was added to the cells for 2 h to cause S phase arrest before rapid transfer to inducing medium (ethanol) also containing 100 mM HU but at 42°C. One hour after transfer to inducing medium at 42°C, glucose was added to repress expression from the alcA promoter. The abundance of NIME^cyclinB was determined by Western blotting. The same blots were also subsequently detected for p34^cdc2 as loading control. (B) The experimental procedures for NIMA induction and repression in HU-arrested cells were as described in A by using a strain with alcA inducible nimA. NIMA was detected by Western blot after immunoprecipitation. No general proteolysis was observed in the samples from which NIMA was isolated, and the level of p34^cdc2 was found by Western blotting to be constant. However, in addition to full-length NIMA (top band) numerous smaller NIMA degradation products were observed.

Mutations of the APC/C Override the nimA5 G2 Arrest by Elevating p34^cdc2 H1 Kinase Activity and Making nimA5 Leaky

The nimA5 mutation arrests cells in G2 at restrictive temperature even though p34^cdc2 kinase activity increases to mitotic levels (Osmani et al., 1991a;Ye et al., 1995). Our current data (Figure 3A) and previous studies(Osmani et al., 1991b; James et al., 1995) indicate that mutationof the APC/C allows cells to bypass the nimA5 G2 arrest and entermitosis, albeit a defective mitosis (Osmani et al., 1991b). Tofurther understand this phenomenon we have carried out two typesof experiment. First, biochemical analysis was completed to seewhether mitosis was occurring without NIMA kinase activity inAPC + nimA5 double mutant strains. Second, nimA was deleted frombimE7^APC1 cells to see whether an APC/C mutation could override completelack of NIMAfunction.

Strains containing single nimA5, bimA1^APC3, or bimE7^APC1 mutations, and those containing nimA5 + bimA1^APC3 and nimA5 + bimE7^APC1 were subjected to temperature shift and analyzed for CMI, NIMA,and p34^cdc2 H1 kinase activities (Figure 6). Two features of the analysisare particularly interesting. First, it is clear that both thebimA1^APC3 and bimE7^APC1 mutations allow some activation of the mutant NIMA kinase toa level higher than that observed in the single nimA5 mutant strain(Figure 6B). This partial activation could contribute to the defectivemitosis seen in bimE7^APC1 + nimA5 mutant strains. Second, dramatic activation of the p34^cdc2 H1 kinase was promoted in both bimE7^APC1 + nimA5 and bimA1^APC3 + nimA5 strains to a level much higher than that observed innormal mitosis and greater than that recorded in cells blockedin mitosis by the bimE7^APC1 mutation or at the restrictive temperature for bimA1^APC3 or nimA5 (Figure 6C). Such high activation of p34^cdc2 H1 kinase is likely to play a role in the ability of bimE7^APC1 and bimA1^APC3 mutations to override the nimA5 G2 arrest (Figure 6A).

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Figure 6. APC/C mutations override the nimA5 G2 arrest with very high p34^cdc2 H1 kinase activity. (A) Mutant cells, as indicated, were grown to early log phase at 32°C and shifted to 42°C at time 0. At the times indicated the CMI was determined after DAPI staining and fluorescent microscopy. p34^cdc2 H1 (B) and NIMA kinase (C) activities were assayed after immunoprecipitation with specific antibodies.

Deletion of nimA Prevents an APC/C Mutant from Entering Mitosis

To see whether some NIMA activity is required to allow mitotic events when bimE^APC1 is inactivated, we removed nimA by targeted deletion in botha wild-type strain and a bimE7^APC1 strain. A linear DNA deletion strategy was used (Figure 7A) inwhich nimA was replaced with the pyr4 nutritional marker fromNeurospora crasser, which encodes orotidine-5'-phosphate decarboxylaseand complements the pyrG89 mutation in A. nidulans. The deletedallele in the homokaryotic state is lethal (see below) and wastherefore maintained in heterokaryons as previously described(Osmani et al., 1988; Oakley and Osmani, 1993).

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Figure 7. Targeted nimA deletion. (A) Restriction maps of the nimA locus and nimA $Delta$ locus after targeted deletion. The PstI fragment of nimA was replaced with a PstI fragment containing the pyr4 gene. The linear genomic KpnI fragment containing the pyr4 insert was used for transformation in a wild-type (wt = GR5) and a bimE7^APC1 strain. Diagnostic XhoI fragments of 4.0 kb (wt) and 4.5 kb (nimA $Delta$ ) when probed with the PstI-KpnI fragment are indicated. (B) Autoradiogram of a Southern blot of XhoI-digested genomicDNA isolated from putative heterokaryons after deletion of nimA probed with the radiolabled PstI-KpnI fragment indicated in A. 10, 13, 32, 76, 109, and 131 are deletions in GR5, and 19R and 30R indicate deletions in a bimE7^APC1 strain. Heterokaryons 10, 13, 109, 19R, and 30R all contain both a specific deletion and the wild-type allele. (C) Micrographs of DAPI-stained germlings. The wild-type germling is from an 8-h sample and contains eight interphase nuclei. The nimA $Delta$ germlings are derived from a heterokaryon germinated for 8 and 15 h, respectively, at 32°C. (D) Representative micrographs of DAPI-stained germlings from strains with the indicated pertinent genotypes. Spores were first allowed to germinate at 32°C for 7 h before shifting to 42°C for 4 h. The nimA5 mutant germling was grown at 42°C directly for 7 h. It is to be noted that the single nucleus of the large nimA $Delta$ + bimE7^APC1 germling remained at interphase upon shift to 42°C for 4 h, whereas nuclei in the bimE7^APC1 or nimA5 + bimE7^APC1 mutant germlings all became condensed. The arrow indicates an ungerminated spore carrying the parental genotype (GR5 = pyrg89) derived from the nimA $Delta$ + bimE7^APC1 heterokaryon.

After transformation with the linear deletion construct and preliminary screening of transformants for heterokaryons (seeMATERIALS AND METHODS), Southern blot analysis identified severalheterokaryons containing both a wild-type allele and a clean deletedallele (Figure 7, A and B) termed nimA $Delta$ . It was noticeable thatall deleted heterokaryons contained much lower levels of the deletedallele. This is most likely due to selection for the wild-typeallele, as NIMA is expressed at a low level, is cell cycle regulated,and is very unstable. It is therefore likely that a 50:50 ratioof nimA to nimA $Delta$ nuclei in a heterokaryon would not supply enoughNIMA to enable normal cell cycle progression within that heterokaryon.This therefore leads to the selection for high ratios of the wild-typeallele.

The ability to maintain nuclei containing a deletion of an essential gene in the heterokaryotic state in A. nidulans allowsthe analysis of the null phenotype because the heterokaryoticstate is broken when conidia are formed, as they are uninucleate(Osmani et al., 1988). Phenotypic analysis of germinated conidiaderived from heterokaryons having a clean deletion of nimA identifieda low percentage of conidia (~3.0%) that germinated to producepolarized germlings with a single interphase nucleus (Figure 7C),which is the classic nim (never in mitosis) phenotype of A. nidulans.These cells clearly contain the deleted allele, as they are pyr4⁺. They also showed the expected phenotype for deletion of an essentialcell cycle gene. All other conidia from the heterokaryon are parentalpyrG89-containing cells because they did not form germlings onmedia lacking uridine and uracil. The low recovery of the nimA $Delta$ allele in conidia from the heterokaryons confirms the Southernblot analysis, indicating that there is selection for the wild-typeallele in these heterokaryons. We conclude that the nimA5 phenotypeis very similar to the nimA $Delta$ null allele and that nimA is an essentialgene.

Phenotypic analysis of conidia derived from a heterokaryon containing a clean deletion of nimA in a bimE7^APC1 background was used to determine whether inactivation of bimE^APC1 could cause mitosis in the absence of nimA. Conidia were platedon media lacking uridine and uracil and were germinated at 32°Cfor a period to allow identification of those containing the nimA $Delta$ allele. After temperature shift to 42°C to inactivate BIME^APC1, DAPI staining revealed that all the nimA $Delta$ + bimE7^APC1 cells (>150) remained arrested in interphase (Figure 7D). Theexperiment was repeated by germinating directly at 42°C, but thenimA $Delta$ allele still prevented bimE7^APC1 from promoting cells into mitosis. It is therefore necessaryto have some NIMA activity or cells remain arrested before mitosiswhen the APC/C is inactivated by bimE7^APC1.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The abundance of the NIMA kinase is regulated through the cell cycle, and its degradation is required for exit from mitosis(Osmani and Ye, 1996). Mitotic degradation of other regulatoryproteins (Cohen-Fix et al., 1996; Funabiki et al., 1996; Juanget al., 1997; Michaelis et al., 1997; Charles et al., 1998; Shirayamaet al., 1998) is also required for normal exit from mitosis, andthese proteins are targeted by the APC/C for degradation. In thecurrent work we provide evidence that BIMA^APC3 plays a regulatory role in APC/C function and show that NIMAkinase is likely a target of the APC/C.

Although the bimA1^APC3 allele causes tight temperature sensitivity, it does not cause an irreversible arrest in mitosis, whichwould be expected for a mutation causing inactivation of the APC/Cat restrictive temperature. Remarkably, we demonstrate that inactivationof bimA1^APC3 instead induces repeating rounds of mitotic events characterizedby chromosome condensation and decondensation, activation andinactivation of the p34^cdc2 and NIMA protein kinases, accumulation and degradation of NIMA,and cyclic rounds of phosphorylation of NIMA. The tight correlationobserved between these events strongly indicates that rapid inactivationof bimA1^APC3 promotes cyclic activation and inactivation of the mitosis-promotingkinases, which then drive nuclei in and out of a mitoticstate.

How does inactivation of an APC/C subunit cause cell cycle oscillations of the mitosis-promoting kinases? Some insight intothis phenomenon is provided by data indicating that NIMA couldbe a target of the APC/C.

It is known that inhibition of DNA synthesis by addition of hydroxyurea to dividing A. nidulans cells causes S phase arrestand disappearance of NIMA protein (Ye et al., 1996). By expressionof nimA from an inducible promoter after S phase arrest, we haveshown that, like NIME^cyclinB, NIMA is rendered unstable in an APC/C-dependent manner. We haveno direct evidence that this involves the E3 ubiquitin ligaseactivity of the APC/C, but this is an obviouspossibility.

We have also found that the APC/C plays a role in NIMA stability at G2 because the previously reported ability of the bimE7^APC1 mutation to override the nimA5 G2 arrest (Osmani et al., 1988)was found to be shared with the bimA1^APC3 mutation. Thus mutations of subunits of the APC/C allow entryinto mitosis when NIMA is defective. Biochemical analysis wasused to reveal the molecular basis for this effect. First, thekinase activity of p34^cdc2 is greatly increased in nimA5 + bimE7^APC1 and nimA5 + bimA1^APC3 double mutant strains to a level much higher than that foundduring normal mitosis. This increased level of p34^cdc2 activity is at least in part because NIME^cyclinB accumulates to higher levels in these double mutants. Increasesin NIME^cyclinB at the G2 arrest point of nimA5 can cause immediate elevationof p34^cdc2 H1 kinase activity, as p34^cdc2 is not subjected to inhibitory tyrosine phosphorylation at thispoint in the cell cycle (Osmani et al., 1991a). Second, inactivationof bimA^APC3 or bimE^APC1 renders the nimA5 mutation slightly leaky, giving rise to marginallyelevated levels of NIMA kinase activity. This is, at least inpart, due to an accumulation of NIMA protein to higher levelsbut could also be caused by the marked elevation of p34^cdc2 H1 kinase activity observed in these strains. The data indicatethat at G2 NIMA and NIME^cyclinB proteins are held in check via an APC/C-dependent mechanism.Therefore, APC/C mutations make the nimA5 mutation leaky and alsosuperinduce p34^cdc2 H1 kinase activity to promote defective mitotic events. Mutationof the APC/C cannot, however, override complete loss of NIMA function,as deletion of nimA arrests cells in G2 even after inactivationof bimE7^APC1.

While this work was in preparation, it has been reported that promoter rundown of nimA, which causes a G2 arrest, can be overriddenby inactivation of bimA1^APC3 in cells containing "insignificant levels" of NIMA kinase. Thisexperiment has been interpreted to mean that APC/C mutations canpromote mitotic events in the complete absence of NIMA function(Lies et al., 1998). This apparent discrepancy with our data maybe due to the different experimental approaches used. However,deletion of nimA from the genome generates a true null phenotype.Additionally, the insignificant levels of NIMA kinase reported(Lies et al., 1998) may be significant, because when NIMA andthe APC/C are inhibited, p34^cdc2 H1 kinase levels are induced to higher than mitotic levels (Figure6). Additionally, as NIMA is likely a substrate of the APC/C (seebelow), promoter rundown of NIMA is probably less effective whenthe turnover rate of NIMA is reduced by inactivation of the APC/C.

The fact that mutation of APC/C subunits causes elevation of NIMA at the nimA5 arrest point and also renders NIMA more stableduring S-phase arrest suggests that NIMA requires the APC/C forinstability during interphase and indicates that NIMA is a substrateof the APC/C. In further support of this contention, we note thatNIMA is degraded during mitosis and that it is stabilized whenthe spindle assembly checkpoint is engaged, which is thought tobe imposed by inhibition of the APC/C (Osmani and Ye, 1996). Additionally,we have previously shown that forced expression of NIMA enhancesthe bimE^APC1 mutation, which is also consistent with NIMA being a substrateof the APC/C (Ye et al., 1996). We now show that the bimA1^APC3 mutation causes amazing oscillations in the abundance of NIMAprotein, indicating that this APC/C mutation promotes repeatedrounds of inactivation and then activation of the APC/C towardNIMA. With these observations in mind we propose the followingto help explain the oscillatory effects caused by bimA1^APC3.

The bimA1^APC3 mutation may uncouple an oscillatory clock mechanism that controls the APC/C and thus cell cycle progression. Byrapid inactivation of bimA1^APC3, perhaps this regulatory clock is reset to a base level. By restartingthe clock from the same regulatory point in the cell cycle, allcells would then proceed through the cell cycle in a synchronousmanner, resulting in the observed cell cycle-specific changeswe documented regarding chromosome condensation, kinase activities,and proteinabundance.

Second, to help explain why multiple oscillations occur, we suggest that the bimA1^APC3 mutation makes the APC/C partially resistant to activation byits substrates, such as cyclin B, Polo, and NIMA, during mitosis.This would cause cells to delay in mitosis and accumulate APC/Csubstrates until a critical threshold level could accumulate andeventually activate the partially defective APC/C. After APC/Cactivation, cyclin B, Polo, and NIMA would be degraded and allowexit from mitosis. In this manner an extended mitotic delay wouldbe imposed followed by progression through interphase into anothermitotic delay until the defective APC/C could be activated againafter accumulation of substrates, and so on. In this manner multiplecell cycle oscillations could be generated between interphaseand mitoticstates.

We have shown that NIMA is likely a substrate of the APC/C and that its level and activity oscillate widely after rapid inactivationof bimA1^APC3. For this reason it is possible that NIMA accumulation playsa key role in the activation of the APC/C seen after rapid inactivationof bimA1^APC3 (Figure 8). This possibility is further supported by the factthat in a nimA5 + bimA1^APC3 double mutant the APC/C is not activated, and cells remain inan extended mitotic state with elevated levels of both NIMA andNIME^cyclinB. Thus, nimA is required for the activation of the APC/C afterinhibition of bimA^APC3. This then explains why the nimA5 + bimA1^APC3 double mutant arrests in mitosis but the single bimA1^APC3 mutant oscillates in and out of mitosis. In bimA1^APC3 strains, NIMA protein could accumulate with normal activity andhelp activate the APC/C to allow degradation of mitotic substratesand promote exit from mitosis (Figure 8B). By contrast, in nimA5+ bimA1^APC3 strains, although NIMA5 protein accumulates and has enough activityto allow cells into mitosis, it does not properly activate theAPC/C, thus causing the extended mitotic arrest observed (Figure8C).

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Figure 8. Relationship between NIMA and BIMA1^APC3. To help explain why the nimA5 mutation in combination with bimA1^APC3 causes an effective mitotic arrest phenotype, whereas the bimA1^APC3 mutation generates repeating rounds of mitotic oscillation, we propose the following. (A) Substrates of the APC/C, such as cyclin B, Polo-like kinases, and NIMA, accumulate to a threshold during mitosis, which activates the APC/C to trigger their demise and also to exit from mitosis. (B) The bimA1^APC3 mutation increases the threshold of activation of the APC/C. This results in a mitotic delay during which NIMA protein and activity accumulate. When NIMA activity reaches the higher threshold level of activation, the APC/C is activated, and cells can exit mitosis. (C) In the bimA1 + nimA5 double mutant, although p34^cdc2 H1 kinase activity and NIMA5 activity are increased to allow entry into mitosis, the level of NIMA5 activity stays below that required to activate the APC/C. This then causes an extended mitotic arrest, because cells cannot exit mitosis.

Of course it is possible that both p34^cdc2/cyclin B and NIMA are involved in the activation of the APC/C at mitosis, along withother regulators such as Polo-like kinases (Charles et al., 1998;Descombes and Nigg, 1998; Shirayama et al., 1998). The importantpoint is that bimA^APC3 apparently plays a regulatory role in APC/C function. We proposethat bimA^APC3 could be part of a cell cycle clock mechanism and, additionally,that it is required for normal activation of the APC/C at mitosisin response to accumulation and activation of APC/C substratesduringmitosis.

Finally, it should be noted that the cyclic oscillations of cell cycle events caused by inactivation of bimA1^APC3 are unusual in several respects. Most noticeably they are notsuccessful in dividing nuclei, despite repeated rounds of activationand inactivation of p34^cdc2 and NIMA. Perhaps some APC/C substrates, such as Pds1 (Cohen-Fixet al., 1996), Cut2 (Funabiki et al., 1996), Scc1 (Michaelis etal., 1997), and Ase1 (Juang et al., 1997), that need to be removedto allow normal progression out of mitosis are not destroyed whenbimA^APC3 is inhibited. The cell cycle oscillations are also not responsiveto the DNA damage checkpoint. They are, however, responsive tothe spindle assembly checkpoint activated by microtubule depolymerization.Because the bimA1^APC3-induced cyclic oscillations are arrested at mitosis after microtubuledepolymerization, it is indicated that the APC/C is still inhibitedby Mad2p, which mediates this checkpoint arrest (He et al., 1997;Li et al., 1997).

Our data therefore indicate that bimA^APC3 inactivation prevents degradation of anaphase substrates of the APC/C while allowingnormal regulation of the APC/C during the spindle checkpoint.This suggests that the regulation of the APC/C is disturbed ina relatively specific manner by the bimA1^APC3 mutation. Perhaps the cyclic rounds of chromosome condensationand decondensation promoted by bimA1^APC3 inactivation are driven primarily by cycles of NIMA activity,with most other cell cycle-specific events remaining unchanged.This could occur if the bimA1^APC3 mutation interferes with the activation of the APC/C toward NIMAbut not toward substrates required for anaphase progression andpassage through other phases of the cell cycle. Future experimentswill be aimed at validating our proposed regulatory role for bimA^APC3, which should further our understanding of the regulation ofthe APC/C, particularly with regard to its substrate specificityduring cell cycle progression and checkpointcontrol.

	ACKNOWLEDGMENTS

We thank the members of our laboratory for constructive suggestions on this work and Drs. Peter Mirabito and Matthew O'Connellfor A. nidulans strains. This work was supported in part by agrant from the National Institutes of Health (GM-42564) to S.A.O.

	FOOTNOTES

^* Present address: Infectious Diseases Research, Lilly Research Laboratories, Eli Lilly & Company, Lilly Corporate Center, Indianapolis,IN46285.

Present address: Johns Hopkins School of Medicine, Department of Molecular Biology and Genetics, Baltimore, MD21205.

Correspondingauthor.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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Potential Link between the NIMA Mitotic Kinase and Nuclear Membrane Fission during Mitotic Exit in Aspergillus nidulans
Eukaryot. Cell, December 1, 2004; 3(6): 1433 - 1444.

				A. H. Osmani, J. Davies, H.-L. Liu, A. Nile, and S. A. Osmani Systematic Deletion and Mitotic Localization of the Nuclear Pore Complex Proteins of Aspergillus nidulans Mol. Biol. Cell, December 1, 2006; 17(12): 4946 - 4961. [Abstract] [Full Text] [PDF]