CaMKIIγ-mediated inactivation of the Kin I kinesin MCAK is essential for bipolar spindle formation
2005; Springer Nature; Volume: 24; Issue: 6 Linguagem: Inglês
10.1038/sj.emboj.7600601
ISSN1460-2075
AutoresPer Holmfeldt, Xin Zhang, Sonja Stenmark, Claire Walczak, Martin Gullberg,
Tópico(s)Ubiquitin and proteasome pathways
ResumoArticle3 March 2005free access CaMKIIγ-mediated inactivation of the Kin I kinesin MCAK is essential for bipolar spindle formation Per Holmfeldt Per Holmfeldt Department of Molecular Biology, Umeå University, Umeå, Sweden Search for more papers by this author Xin Zhang Xin Zhang Department of Biology, Indiana University, Bloomington, IN, USA Search for more papers by this author Sonja Stenmark Sonja Stenmark Department of Molecular Biology, Umeå University, Umeå, Sweden Search for more papers by this author Claire E Walczak Claire E Walczak Departments of Biochemistry and Molecular Biology,Indiana University, Bloomington, IN, USA Search for more papers by this author Martin Gullberg Corresponding Author Martin Gullberg Department of Molecular Biology, Umeå University, Umeå, Sweden Search for more papers by this author Per Holmfeldt Per Holmfeldt Department of Molecular Biology, Umeå University, Umeå, Sweden Search for more papers by this author Xin Zhang Xin Zhang Department of Biology, Indiana University, Bloomington, IN, USA Search for more papers by this author Sonja Stenmark Sonja Stenmark Department of Molecular Biology, Umeå University, Umeå, Sweden Search for more papers by this author Claire E Walczak Claire E Walczak Departments of Biochemistry and Molecular Biology,Indiana University, Bloomington, IN, USA Search for more papers by this author Martin Gullberg Corresponding Author Martin Gullberg Department of Molecular Biology, Umeå University, Umeå, Sweden Search for more papers by this author Author Information Per Holmfeldt1, Xin Zhang2, Sonja Stenmark1, Claire E Walczak3 and Martin Gullberg 1 1Department of Molecular Biology, Umeå University, Umeå, Sweden 2Department of Biology, Indiana University, Bloomington, IN, USA 3Departments of Biochemistry and Molecular Biology,Indiana University, Bloomington, IN, USA *Corresponding author. Department of Molecular Biology, Umeå University, S-901 87 Umeå, Sweden. Tel.: +46 90 785 67 03; Fax: +46 90 77 14 20; E-mail: [email protected] The EMBO Journal (2005)24:1256-1266https://doi.org/10.1038/sj.emboj.7600601 PDFDownload PDF of article text and main figures. ToolsAdd to favoritesDownload CitationsTrack CitationsPermissions Figures & Info MCAK, a member of the kinesin-13 family, is a microtubule (MT) depolymerase that is necessary to ensure proper kinetochore MT attachment during spindle formation. Regulation of MCAK activity and localization is controlled in part by Aurora B kinase at the centromere. Here we analyzed human cells depleted of the ubiquitous Ca2+/calmodulin-dependent protein kinase IIγ isoform (CaMKIIγ) by RNA interference and found that CaMKIIγ was necessary to suppress MCAK depolymerase activity in vivo. A functional overlap with TOGp, a MT regulator known to counteract MCAK, was suggested by similar CaMKIIγ- and TOGp-depletion phenotypes, namely disorganized multipolar spindles. A replicating vector system, which permits inducible overexpression in cells that simultaneously synthesize interfering short hairpin RNAs, was used to dissect the functional interplay between CaMKIIγ, TOGp, and MCAK. Our results revealed two distinct but functionally overlapping mechanisms for negative regulation of the cytosolic/centrosomal pool of MCAK. These two mechanisms, involving CaMKIIγ and TOGp, respectively, are both essential for spindle bipolarity in a normal physiological context, but not in MCAK-depleted cells. Introduction The bipolar mitotic spindle segregates duplicated chromosomes during cell division. Generation of a functional spindle requires both the inherent dynamic instability of microtubules (MTs), which are polar polymers comprised of α/β tubulin heterodimers, and regulatory proteins that alter MT dynamics (reviewed in Desai and Mitchison, 1997). Spindle MTs attach to sister chromatids at kinetochores, which are protein complexes that assemble onto centromeres (reviewed in Biggins and Walczak, 2003). Chromosome movement is powered by a combination of motor proteins at the kinetochore and balanced MT dynamics in the spindle. Kinetochores lacking attached MTs also serve as the signal generators for the mitotic checkpoint, which arrests mitosis until all kinetochores are correctly attached. Defects in the mitotic checkpoint results in aneuploidy, which is one of the hallmarks for cancer cells. Entry into mitosis triggers global changes in MT dynamics including an increased catastrophe frequency, that is, the transition from MT growth to shrinkage (reviewed in Kline-Smith and Walczak, 2004). In Xenopus egg extracts, the kinesin-13 family member MCAK mediates increased catastrophe frequency at the onset of mitosis (Tournebize et al, 2000; Lawrence et al, 2004). The mechanism of MCAK-mediated catastrophe promotion involves binding to both ends of the MT polymer and catalytically depolymerizing protofilament ends (Desai et al, 1999; Hunter et al, 2003). In Xenopus egg extracts (Tournebize et al, 2000) and in an in vitro MT assembly system consisting of purified components (Kinoshita et al, 2001), the potent catastrophe-promoting activity of MCAK is counteracted by the XMAP215 protein. Human cells differ from Xenopus egg extracts in that the counteractive activities of MCAK and the human homolog of XMAP215, TOGp, are not clearly manifested at the level of stability of MT plus ends. Instead, the phenotype of cells depleted of TOGp by RNA interference has highlighted an essential function of TOGp at the centrosome (Gergely et al, 2003). Bipolar spindles can form in cells depleted of either MCAK alone or doubly depleted of MCAK and TOGp, but not in cells depleted of TOGp alone (Cassimeris and Morabito, 2004; Holmfeldt et al, 2004). Given that endogenous MCAK is required for manifestation of the characteristic TOGp-depletion phenotype of disorganized multipolar spindles, we proposed that centrosomal TOGp has an essential role in protecting spindle MTs from MCAK activity at the centrosome (Holmfeldt et al, 2004). For accurate chromosome segregation during anaphase, it is essential that each kinetochore of a pair of sister chromatids attaches to spindle MTs from opposing poles, such that all chromosomes are bioriented. MCAK is necessary for proper chromosome segregation (Maney et al, 1998) by mediating proper MT attachments during congression (Walczak et al, 2002; Kline-Smith et al, 2004). Recent studies have shown that the Aurora B kinase and the inner centromere Kin I stimulator ICIS function with MCAK at the centromere to regulate proper MT attachment (Ohi et al, 2003, 2004; Andrews et al, 2004; Lan et al, 2004). The emerging model implies that Aurora B and ICIS regulate MCAK activity at specific regions within the centromere, such that the depolymerizing activity of MCAK is directed towards incorrectly orientated kinetochore MTs. Spatial and temporal regulation of MCAK by the Aurora B kinase involves phosphorylation on multiple Ser residues, which suppresses and thereby controls the potent MT-destabilizing activity of MCAK at the centromere (Andrews et al, 2004; Lan et al, 2004; Ohi et al, 2004). However, MCAK is also abundant in the cytosol and at the centrosome, and it is unclear how its activity is controlled at these locations. In contrast to what could be expected from the original studies of Xenopus egg extracts (Walczak et al, 1996; Tournebize et al, 2000), it was recently shown that MCAK depletion in human cells by RNA interference has only a minor effect on the level of spindle MT polymer content and no effect on the density of the interphase MT array (Cassimeris and Morabito, 2004; Holmfeldt et al, 2004). This surprisingly modest depletion phenotype suggests that cytosolic/centrosomally located MCAK is also subject to negative regulation, but the mechanism is unknown. Ca2+/calmodulin-dependent protein kinase II (CaMKII) is a multifunctional enzyme that has been implicated in a multitude of Ca2+-regulated biological processes, including synaptic transmission, gene transcription, and growth control (reviewed in Hudmon and Schulman, 2002). There are four isoforms of CaMKII encoded by separate genes; the γ and δ isoforms are ubiquitously expressed, while the α and β isoforms are neural specific. Here we have investigated functions of CaMKIIγ in human cell lines, either by depleting the γ isoform by RNA interference or by overexpressing a constitutively active derivative. These studies revealed an essential function of CaMKIIγ as a negative regulator of MCAK that is required for suppression of cytosolic/centrosomal MCAK activity during spindle assembly. CaMKIIγ depletion resulted in the same type of disorganized multipolar spindles that were previously observed in TOGp-depleted cells. By examining the functional interplay between CaMKIIγ, TOGp, and MCAK, we propose a model in which this interplay is essential for protection of MTs from uncontrolled MCAK activity at the centrosome. Results CaMKIIγ is essential for bipolar spindle formation To explore a potential cell cycle regulatory role of the ubiquitously expressed CaMKIIγ isoform, CaMKIIγ levels were reduced in human K562 leukemia cells by RNA interference by using an short hairpin RNA (shRNA) expression vector. Our approach relies on an EBV-based replicating vector system that confers hygromycin resistance and thus allows selection of cells within 3 days, all of which express the transfected shRNA (Holmfeldt et al, 2004). Graded shRNA expression levels were achieved by premixing the specific shRNA derivative at different ratios with a control vector. As these vectors have a stringent replication control, the relative proportion of transfected DNA is maintained (Melander Gradin et al, 1997). Transfection of a shuttle vector directing expression of CaMKIIγ-specific shRNA (shRNA-CaMKIIγ)-depleted CaMKIIγ, while TOGp and tubulin levels were unaltered (Figure 1A). Quantification of immunoblots by serial dilutions of cell lysates revealed more than 90% specific depletion at all shRNA-CaMKIIγ dilutions. It should be noted that >95% reduction of CaMKIIγ was below the limit of detection. Figure 1.Phenotype of K562 cells expressing CaMKIIγ-specific interfering shRNA. Cells were transfected with a total of 18 μg DNA comprising the indicated percentage of shRNA-scrambled or shRNA-CaMKIIγ made up of Vector-Co. Cells were counter-selected for 5 days with hygromycin to kill off nontransfected cells. (A) Immunoblots of total cellular lysates using the indicated antibody for detection. (B) Cells were triple-stained for DNA, MTs, and the MT minus-end marker NUMA. Representative examples of each spindle type are shown below the histogram. Spindles of mitotic cells were categorized into four groups, namely, bipolar, monastral, and multipolar types A and B, as indicated by the subdivision of bars. The data in this and subsequent figures are presented as percentage of total cells and represent the means of duplicate determinations of coded samples (n=300 mitotic cells). The most notable difference between type A and type B multipolar spindles is that the chromosomes of type B spindles are completely disorganized and appear aggregated (two representative examples shown). Bar: 10 μm. (C) Cells were transfected with 100% shRNA-CaMKIIγ and counter-selected for 5 days with hygromycin. The histogram depicts the distribution of the number of spindle poles in individual cells with type B multipolar spindles, as determined by pericentrin-labeled dots positioned at the spindle pole (n=40). The data represent the means of duplicate determinations. A representative epifluorescence image of a type B multipolar spindle of a shRNA-CaMKIIγ-expressing cell stained with anti-α-tubulin (green) and anti-pericentrin (red) is also shown. The data in this and subsequent figures are representative of at least three independent transfection experiments. Download figure Download PowerPoint Analysis of CaMKIIγ-depleted cells revealed no detectable phenotype on the level of MT polymer in interphase cells, suggesting that endogenous CaMKIIγ is not important for regulating the density of the interphase MT array (data not shown). However, whereas cells harboring a control vector (Vector-Co) or cells expressing a control shRNA with a scrambled sequence (shRNA-Co) were unaffected, analysis of cell cycle profiles after 5 days of CaMKIIγ depletion revealed an increased fraction of cells with G2/M DNA content (data not shown) and accumulation of mitotic cells with multipolar spindles (see subdivision of bars in Figure 1B). This phenotype became increasingly pronounced at increasing shRNA-CaMKIIγ concentrations. The multipolar spindles observed could be divided into two categories: (1) multipolar spindles with chromosomes that appear well organized between three or more spindle poles (type A), which are also observed among Vector-Co cells, and (2) disorganized multipolar spindles with multiple MT asters of various sizes and with disorganized chromosomes aggregated around each aster (type B) (see images in Figure 1B). The organization of MTs at the minus end in the type B multipolar spindles was not defective, as evidenced by NUMA staining. We found that the type B multipolar spindles were not observed among control cells and are therefore a hallmark of CaMKIIγ-depleted cells. The shRNA-CaMKIIγ derivative used here depletes its target more efficiently than the shRNA-CaMKIIγ derivative that was used as a negative control in a previous study (Holmfeldt et al, 2004). This observation, as well as a comparison of immunoblot analysis (Figure 1A) and the finding of accumulation of defective mitotic cells (Figure 1B), emphasizes the requirement of efficiently depleting CaMKIIγ in order to detect a phenotype. To ascertain that the phenotype observed was specific for CaMKIIγ depletion, we also analyzed the effect of an independent CaMKIIγ-specific shRNA derivative and the CaMKII inhibitory drug KN93. In both cases, type B multipolar spindles were generated (data not shown). This spindle phenotype was also observed as a major phenotype in the Jurkat T-cell leukemia and the DG 75 Burkitt lymphoma cell lines expressing either of two distinct shRNA-CaMKIIγ derivatives (data not shown). Thus, the ubiquitously expressed CaMKIIγ appears to be necessary for efficient bipolar spindle formation in human cells. To look more closely at the organization of poles in CaMKIIγ-depleted cells, the type B multipolar spindles of CaMKIIγ-depleted cells were further characterized by dual labeling of tubulin and the centrosomal protein pericentrin. We found that the majority of these abnormal spindles in shRNA-CaMKIIγ-expressing cells contained centrosomes at only two of the multiple spindle poles (Figure 1C), which shows that type B multipolar spindles are not caused by nucleation from multiple centrosomes. The CaMKIIγ-depletion phenotype is dependent on MCAK It is notable that the type B multipolar spindles observed among CaMKIIγ-depleted cells appear indistinguishable from the multipolar spindles observed after depletion of TOGp (Gergely et al, 2003). It has previously been shown that the type B multipolar spindles caused by depletion of TOGp are dependent on MCAK (Cassimeris and Morabito, 2004; Holmfeldt et al, 2004). To determine if MCAK is also involved in generating the CaMKIIγ-depletion phenotype, cells were either singly or doubly depleted of CaMKIIγ and MCAK by expressing specific interfering shRNAs. Cell proliferation and mitotic figures were followed over 10 days and compared to cells transfected with Vector-Co or a scrambled control derivative (shRNA-Co). As an additional control for the specificity of phenotypes, we also included shRNA-MAP4 to deplete the MT-associated MAP4 protein, which is not required for spindle assembly (Wang et al, 1996). It is shown in Figure 2A that the present system for RNA interference allows depletion of the specific gene product for prolonged culture periods and, as expected, depletion of MAP4 did not cause interference with cell proliferation (Figure 2B) or spindle assembly (Figure 2C). Moreover, depletion of MCAK caused a modest inhibition of cell proliferation, which is consistent with our previous report (Holmfeldt et al, 2004), whereas depletion of CaMKIIγ caused an almost complete growth arrest. Most importantly, simultaneous depletion of MCAK and CaMKIIγ greatly reduced the cell proliferation defect caused by depletion of CaMKIIγ alone and proliferation of doubly depleted cells was very similar to that observed after depletion of MCAK alone. These results suggest that MCAK is involved in growth inhibition of CaMKIIγ-depleted cells. Figure 2.The essential function of CaMKIIγ during cell division is dependent on MCAK. Cells were co-transfected, as in Figure 1, with DNA mixtures containing either 50% of each shRNA, or individually with 50% Vector-Co. Nontransfected cells were counter-selected by culturing in the presence of hygromycin, which killed off most nontransfected cells within 3 days. (A) Total cellular lysates were analyzed by immunoblotting using the indicated antibodies for detection. (B) Viable cells grown in the presence of hygromycin were determined on the days indicated. The graph represents the mean±s.d. of data from three independent transfection experiments, each of which was performed in duplicate. (C) Mitotic figures were categorized after 6 days of depletion, as described under Figure 1B. Download figure Download PowerPoint Consistent with our previous study (Holmfeldt et al, 2004), analysis of mitotic figures revealed a relatively mild MCAK-depletion phenotype in which there was a slight increase in the number of cells with monastral spindles (Figure 2C). We also observed the expected accumulation of mitotic cells in the CaMKIIγ-depleted population, many of which contained multipolar spindles (Figure 2C). It should be noted that the shRNA-CaMKIIγ has to be diluted with vector control DNA to allow direct comparisons with doubly depleted cells (i.e., 50% of each shRNA in the transfection mix); therefore, the mitotic CaMKIIγ-depletion phenotype is not as dramatic as for maximally depleted cells (i.e., 100% shRNA-CaMKIIγ DNA, Figure 1). Most importantly, double depletion of MCAK and CaMKIIγ significantly reduced the mitotic index and spindle abnormalities caused by depletion of CaMKIIγ alone. In fact, the defects in the doubly depleted cells appeared similar to the relatively mild mitotic phenotype of MCAK depletion alone. Consistent with the cell proliferation assays, these data show that the presence of MCAK is necessary for the mitotic phenotypes caused by depletion of CaMKIIγ, perhaps by a mechanism in which CaMKIIγ downregulates MCAK activity. The mitotic phenotype of CaMKIIγ depletion includes not only type B multipolar spindles, but also an increased population of bipolar spindles (see subdivision of bars in Figure 2C). Classification of these bipolar spindles revealed an accumulation of prometaphase/metaphase cells, which we found in CaMKIIγ-depleted cells but not in cells depleted of MCAK or doubly depleted of CaMKIIγ and MCAK (Supplementary Figure S1). Many of the prometaphase spindles found in CaMKIIγ-depleted cell populations appeared unusually small, but these features were not distinctive enough to allow a clear-cut classification into a specific subgroup. Nevertheless, given that accumulation of prometaphase/metaphase cells in the CaMKIIγ-depleted population is dependent on MCAK, and that excessive cytosolic MCAK activity is likely to cause accumulation of prometaphase/metaphase cells, these results suggest that CaMKIIγ depletion results in uncontrolled cytosolic MCAK activity. Excessive MCAK levels cause type B multipolar spindles besides other spindle abnormalities If uncontrolled MCAK activity is the direct cause of the type B multipolar spindle abnormality, we would expect that increasing the levels of cytosolic and/or centrosomal MCAK will at some point out-titrate the negative regulation by CaMKIIγ, and thereby generate type B multipolar spindles in addition to other mitotic abnormalities. To test this model, we created a pMEP-xMCAK derivate that lacks the N-terminal centromere-targeting domain and, consequently, will only act in the cytosol and at the centrosome (Walczak et al, 2002). In addition, to increase the expression level, the coding region of xMCAK was fused with a 5′ untranslated region that directs high-level protein expression in human cells. The resulting xMCAK(187–732) derivative was expressed four- to eight-fold higher than the intact xMCAK derivative (Figure 3A). At these high levels, interphase MTs were almost completely depolymerized within 8 h (Figure 3B). Consistent with increased expression levels, cells expressing xMCAK(187–732) for 24 h showed a much higher mitotic index than cells expressing xMCAK (Figure 3C). Figure 3.MT depolymerization and mitotic defects caused by high levels of xMCAK active in the cytosol and/or the centrosome. K562 cells were transfected with the pMEP derivative indicated (18 μg) and counter-selected with hygromycin for 5 days. Cd2+ was added to induce ectopic xMCAK from the hMTIIa promoter for the indicated time period. (A) To compare expression of pMEP-xMCAK(187–732), which contains an optimized 5′ untranslated sequence, and pMEP-xMCAK, serially diluted lysates from Cd2+-induced (8 h) transfected cells were analyzed by immunoblotting (1/1: 25 μg/lane; 1/2: 12.5 μg/lane; 1/4: 6.3 μg/lane; 1/8: 3.1 μg/lane). To allow comparison of full-length and N-terminal truncated xMCAK proteins, an antiserum raised against the C-terminus of xMCAK was used for detection. (B) MT content expressed as percentage polymerized tubulin after 0 and 8 h of induced expression. (C) After 24 h of induced expression, mitotic figures were categorized as described in Figure 1B. Representative examples of each spindle type found among xMCAK(187–732)-expressing cells are shown below. Characteristic features of type I bipolar spindles as compared to normal spindles include the observation that most kinetochore MTs are absent and MTs appear as two dense star-like asters. Bar: 10 μm. Download figure Download PowerPoint Analysis of mitotic figures revealed that essentially all xMCAK(187–732)-expressing mitotic cells had some type of distinctive abnormality, which were categorized into five distinct types (Figure 3C). We found that expression of either xMCAK derivative caused a major increase in the percentage of the previously described type I bipolar spindle (see subdivision of bars in Figure 3C), which has characteristic small MT asters that are indicative of excess catastrophe promotion (Holmfeldt et al, 2004). Moreover, in cells expressing high levels of xMCAK(187–732), many mitotic cells were completely devoid of detectable MTs, which indicates complete depolymerization (termed type II). Importantly, while analysis of mitotic figures revealed very few type B multipolar spindles among cells expressing the full-length xMCAK derivative, essentially all multipolar spindles in cells expressing xMCAK(187–732) were the disorganized type B, and this spindle type comprised ∼20 % of the accumulated mitotic cells. Thus, MCAK has, at sufficiently high levels, the potential to generate a fraction of type B multipolar spindles. This is consistent with a model in which unregulated MCAK activity is the cause of the multipolar spindle phenotype seen when CaMKIIγ is inhibited. Ectopic CaMKIIγ suppresses the MT-depolymerizing activity of ectopic xMCAK If CaMKIIγ is responsible for downregulating MCAK activity, then we would also expect that overexpressing active CaMKIIγ would suppress the defects seen upon overexpression of xMCAK. To test this idea, we coexpressed xMCAK with a constitutively active CaMKIIγB derivative (CaMKIIγB(c)). To allow selection of cell populations that coexpress two potentially growth-inhibitory gene products, we used a previously described system for inducible coexpression of genes encoding a substrate and a cognate kinase carried on pMEP vectors under the control of the tightly regulatable hMTIIa promotor (Gradin et al, 1998). We found that stimulation of the hMTIIa promotor for 8 h resulted in a six- to 10-fold overexpression of CaMKIIγB(c) and xMCAK proteins as compared to the cognate endogenous gene products (Figure 4A). Figure 4.Constitutively active CaMKIIγB(c) suppresses the activity of ectopic xMCAK during both interphase and mitosis. K562 cells were co-transfected (18 μg in total, DNA ratio 1:1) as indicated, with either Vector-Co or pMEP-xMCAK combined with either Vector-Co (−) or pMEP-CaMKIIγB(c) (+). After 5 days of counter-selection with hygromycin, Cd2+ was added to induce ectopic expression from the hMTIIa promoter of the pMEP vector. (A) Immunoblots of total cellular lysates from Cd2+-induced cells (8 h) using the indicated antibody for detection. (B) MT content in interphase cells expressed as percentage of polymerized tubulin prior to (0 h) or after Cd2+-induced expression (8 h). (C) After 24 h of induced expression, mitotic cells were categorized as described in Figure 1B, into the six groups depicted in Figure 3C. Download figure Download PowerPoint Analysis of the total MT content in interphase cells prior to induced expression (0 h) revealed similar tubulin polymer levels in all four transfected cell populations (Figure 4B), which reflects the tight regulation from the hMTIIa promoter. Expression of CaMKIIγB(c) alone caused no changes in the MT polymer level after 8 h, while expression of xMCAK caused ∼2-fold reduction in the MT content. We found that the MT depolymerization caused by xMCAK overexpression was efficiently suppressed by coexpressed CaMKIIγB(c), which is consistent with our model wherein MCAK activity is downregulated by CaMKIIγ. To explore the functional interactions between ectopic CaMKIIγB(c) and xMCAK during spindle formation, the mitotic index and the appearance of mitotic cells were analyzed after 24 h of induced expression. CaMKIIγB(c) overexpression caused only a very subtle phenotype (Figure 4C). In contrast, high levels of xMCAK expression caused the expected accumulation of mitotic cells, which frequently displayed the bipolar type I abnormality described above (Figure 3). Most significantly, if xMCAK was coexpressed with CaMKIIγB(c), the frequency of mitotic cells was close to normal, and the percentage of cells with type I abnormal spindles was reduced to control levels. These data show that, similar to the observed suppression of MT depolymerization by ectopic xMCAK activity in interphase cells shown in panel B, CaMKIIγB(c) efficiently suppresses the spindle disruptive effect of excessive xMCAK levels during mitosis. It should be noted that we aimed for an expression level of CaMKIIγB(c) that by itself causes a minimal phenotype, which was restricted to a limited increase in monastral spindles. Under these conditions, the observed suppression of MCAK-dependent abnormalities appears remarkably specific. To evaluate the specificity of CaMKIIγB(c)-mediated suppression further, we analyzed mechanistically distinct types of MT destabilization. We found that ectopic CaMKIIγB(c) neither modulated the potency by which the drug nocodazole destabilizes interphase MTs (Supplementary Figure S2), nor suppressed the activity of the MT-destabilizing protein Op18/Stathmin during interphase and mitosis (Supplementary Figure S3). These results show that CaMKIIγB(c) does not support MT stability against any depolymerizer, and they are consistent with a model in which CaMKIIγB(c) suppresses MT destabilization through MCAK suppression. This implies that ectopic CaMKIIγB(c) should have the same effect on the MT system as MCAK depletion, which indeed appears to be the case since either ectopic CaMKIIγB(c) or MCAK depletion caused a small accumulation of monastral spindles without having an effect on the MT density of interphase cells (Figure 4; Holmfeldt et al, 2004). It was shown previously that MCAK is phosphorylated by Aurora B, which inhibits the depolymerization activity of MCAK (Andrews et al, 2004; Lan et al, 2004; Ohi et al, 2004). To determine if the previously identified Aurora B kinase phosphorylation sites were the regulatory sites used by CaMKII, CaMKIIγB(c) was coexpressed with an N-terminal truncated xMCAK(187–732) derivative with or without Ala substitutions at Ser-196, which is the only major negative regulatory Aurora B phosphorylation site that remains after N-terminal truncation (Lan et al, 2004). We found that CaMKIIγB(c) suppressed the potent destabilization of the interphase MT array caused by either xMCAK(187–732) or xMCAK(187–732)-S196A overexpression (Figure 5B). Moreover, analysis of mitotic figures revealed that CaMKIIγB(c) also mediated suppression of the potent mitotic block and accumulation of all characteristic spindle aberrancies (Figure 5C). Consistent with our data on interphase cells, suppression of overexpressed MCAK was unaltered by Ala substitution at Ser-196. These data show that suppression of MCAK activity by CaMKIIγ does not require phosphorylation of any of the previously identified Aurora B sites. Figure 5.CaMKIIγB(c) suppresses MCAK-dependent generation of defective spindles independently of the major negative Aurora B phosphorylation site. K562 cells were co-transfected as in Figure 4 with either Vector-Co or the indicated pMEP-xMCAK(187–732) derivative combined with either Vector-Co (−) or pMEP- CaMKIIγB(c) (+). After 5 days of counter-selection with hygromycin, Cd2+ was added to induce ectopic expression from the hMTIIa promoter of the pMEP vector. (A) Immunoblots of total cellular lysates from Cd2+-induced cells (8 h) using the indicated antibody for detection. The migration of endogenous MCAK is indicated by
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