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© The Rockefeller University Press,
0021-9525/1997//1055 $5.00
The Journal of Cell Biology, Volume 138, Number 5,
, 1997 1055-1066
Article |
Mitotic Spindle Poles are Organized by Structural and Motor Proteins in Addition to Centrosomes
The focusing of microtubules into mitotic spindle poles in vertebrate somatic cells has been assumed to be the consequence of their nucleation from centrosomes. Contrary to this simple view, in this article we show that an antibody recognizing the light intermediate chain of cytoplasmic dynein (70.1) disrupts both the focused organization of microtubule minus ends and the localization of the nuclear mitotic apparatus protein at spindle poles when injected into cultured cells during metaphase, despite the presence of centrosomes. Examination of the effects of this dynein-specific antibody both in vitro using a cell-free system for mitotic aster assembly and in vivo after injection into cultured cells reveals that in addition to its direct effect on cytoplasmic dynein this antibody reduces the efficiency with which dynactin associates with microtubules, indicating that the antibody perturbs the cooperative binding of dynein and dynactin to microtubules during spindle/aster assembly. These results indicate that microtubule minus ends are focused into spindle poles in vertebrate somatic cells through a mechanism that involves contributions from both centrosomes and structural and microtubule motor proteins. Furthermore, these findings, together with the recent observation that cytoplasmic dynein is required for the formation and maintenance of acentrosomal spindle poles in extracts prepared from Xenopus eggs (Heald, R., R. Tournebize, T. Blank, R. Sandaltzopoulos, P. Becker, A. Hyman, and E. Karsenti. 1996. Nature (Lond.). 382: 420–425) demonstrate that there is a common mechanism for focusing free microtubule minus ends in both centrosomal and acentrosomal spindles. We discuss these observations in the context of a search-capture-focus model for spindle assembly.
CHROMOSOME segregation during both mitosis and meiosis is mediated by a complex microtubule-based structure called the spindle (McIntosh and Koonce; 1989; Mitchison, 1989a; Rieder, 1991). The spindle is assembled in a spatially and temporally regulated manner during the cell cycle, and its assembly and function are intimately associated with microtubule dynamics (Inoué and Salmon, 1995; Hyman and Karsenti, 1996; Nicklas, 1997). The organization of microtubules into spindles is governed largely by the interaction of microtubules and microtubule ends with accessory proteins that regulate microtubule dynamics. These accessory proteins are located on the chromosomes (kinetochores), derived from the cytosol (some motor proteins), and/or found at the microtubule minus ends (centrosomes and peri-centrosomal region in somatic cells). The result of these complex interactions is a typical fusiform microtubule array in both mitotic and meiotic cells with microtubule plus ends attached to the chromosomes and minus ends focused into spindle poles.
One striking difference between spindles in vertebrate somatic cells and some types of meiotic and plant cells is that microtubules in vertebrate somatic cells are nucleated from centrosomes, whereas plant cells and some meiotic cells lack bonafide centrosomes. This single structural difference has spurred two different hypotheses regarding the mechanism by which microtubule minus ends are focused at spindle poles (for discussions see Wilson, 1925; Schrader, 1953; Rieder et al., 1993; Waters and Salmon, 1997). In acentrosomal spindles, microtubules associate with chromatin and are drawn into two focused poles through the action of minus end-directed microtubule motors (Bastmeyer et al., 1986; Steffen et al., 1986; Theurkauf and Hawley, 1992; McKim and Hawley, 1995; Vernos and Karsenti, 1995; Heald et al., 1996; Matthies et al., 1996; Merdes et al., 1996). In contrast, in mitotic spindles in vertebrate cells the predominant view holds that microtubule minus ends are focused at the poles as a consequence of their nucleation from the centrosomes (Kirschner and Mitchison, 1986; Hayden et al., 1990; Holy and Leibler, 1994; Rieder and Salmon, 1995). It is currently unclear, however, if mitotic spindles containing centrosomes, like acentrosomal spindles, also use minus end-directed motor activity to promote the focusing of microtubule minus ends at spindle poles despite the presence of centrosomes.
The dynein-specific monoclonal antibody 70.1 (Steuer et al., 1991) was recently shown to perturb the function of cytoplasmic dynein during spindle assembly in meiotic extracts prepared from Xenopus eggs (Heald et al., 1996). It blocked the formation of spindle poles as well as induced the disorganization of the polar regions of preassembled spindles, suggesting that dynein function was important to establish and maintain these spindle poles. Spindles assembled under those conditions, however, do not contain centrosomes, and the spindle poles are focused through an acentrosomal mechanism (Lohka and Maller, 1985; Sawin and Mitchison, 1991; Heald et al., 1996; Merdes et al., 1996). Thus, in this article we have used the 70.1 antibody to investigate whether the organization of microtubules at the polar ends of the mitotic spindle also relies on the action of cytoplasmic dynein despite the inherent focusing activity of centrosomes. We report that perturbation of cytoplasmic dynein function with the 70.1 antibody in somatic cells leads to the disruption of mitotic spindle poles and the separation of the centrosomes from the body of the spindle. Furthermore, the 70.1 antibody prevents the assembly of mitotic asters when added to a cell-free mitotic extract, and in both cases, reduces the efficiency with which dynactin associates with microtubules. These data indicate that microtubule minus ends are focused at mitotic spindle poles through contributions from both centrosomes and accessory proteins, including the minus end-directed motor cytoplasmic dynein and dynactin, and suggest that there are common aspects to the mechanism by which free microtubule minus ends are focused into poles in centrosomal and acentrosomal spindles. These results are discussed in the context of a search-capture-focus model for mitotic spindle assembly.
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Materials and Methods |
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Immunological Techniques
The control (mAb 154; Compton et al., 1991) and dynein-specific (mAb 70.1; Steuer et al., 1991) IgMs were purified from ascites fluid by mannose-binding protein affinity chromatography (Pierce, Rockford, IL). The purified antibodies were dialyzed into 0.1 M Tris, pH 7.4, and concentrated using centricon-30 concentrators (Amicon, Beverly, MA) to 8–16 mg/ml. The remaining antibodies used in this study were a rabbit anti- nuclear mitotic apparatus (NuMA)1 (Gaglio et al., 1995), mouse anti-tubulin (DM1A; Blose et al., 1984), rabbit anti-Eg5 stalk-tail (Sawin et al., 1992), mouse anti-Arp1 (45A; Schafer et al., 1994), mouse anti-p150 dynactin (150B; Gaglio et al., 1996), and mouse anti-dynein (74.1; Dillman and Pfister, 1994).
Indirect immunofluorescence microscopy was performed on cultured cells by immersion in microtubule stabilization buffer (MTSB: 4 M glycerol, 100 mM PIPES, pH 6.9, 1 mM EGTA, and 5 mM MgCl2) for 1 min at room temperature, extraction in MTSB plus 0.5% Triton X-100 for 2 min, followed by MTSB for 2 min. Cells were then fixed in –20°C methanol for 10 min. Indirect immunofluorescence microscopy on mitotic asters assembled in the cell-free mitotic extract was performed by dilution of 5 µl of the extract into 25 µl of KHM buffer (78 mM KCl, 50 mM Hepes, pH 7.0, 4 mM MgCl2, 2 mM EGTA, 1 mM DTT; Burke and Gerace, 1986). The diluted sample was then spotted onto a poly–L-lysine coated glass coverslip and fixed by immersion in –20°C methanol. Both the fixed cells and mitotic asters were rehydrated in TBS (10 mM Tris-HCl, pH 7.5, 150 mM NaCl) containing 1% albumin, and all antibody incubations and washes were performed in TBS plus 1% albumin. Each primary antibody was incubated on the coverslip for 30 min except for the 45A antibody against dynactin and the 74.1 antibody against cytoplasmic dynein, which were incubated on the coverslip for 2 h. After primary antibody treatment, the coverslips were washed for 5 min in TBS plus 1% albumin, and the bound antibodies were detected using either fluorescein- or Texas red-conjugated species- and antibody isotype-specific secondary antibodies at dilutions of 1:500 (Vector Labs, Burlingame, CA). DNA was detected using DAPI (4',6-diamidino-2-phenylindole) at 0.4 µg/ml (Sigma Chemical Co., St. Louis, MO). After a final wash the coverslips were mounted in FITC-guard mounting medium (Testog, Inc., Chicago, IL) and observed on a Nikon Optiphot microscope equipped for epifluorescence (Nikon, Inc., Meliville, NY).
Proteins from the mitotic extracts were solubilized directly with SDS-PAGE sample buffer. The proteins were then separated by size using SDS-PAGE and transferred to PVDF (polyvinylidene difluoride) membrane (Millipore Corp., Bedford, MA). The membranes were blocked in TBS containing 5% nonfat milk for 30 min at room temperature and the primary antibody incubated for 6 h at room temperature in TBS containing 1% nonfat milk. Nonbound primary antibody was removed by washing five times for 3 min each in TBS, and the bound antibody was detected using either horseradish peroxidase-conjugated protein A or horseradish peroxidase-conjugated goat anti–mouse (Bio Rad, Hercules, CA). The nonbound secondary reagent was removed by washing five times for 3 min each in TBS and the signal detected using enhanced chemiluminescence (Amersham Corp., Arlington Heights, IL).
Microinjection
CV-1 cells growing on photo-etched 
-numeric glass cover slips (Bellco Glass Co., Vineland, NJ) were microinjected following the procedures of Compton and Cleveland (1993) and Capecchi (1980). Interphase cells were microinjected in the cytoplasm with either the control antibody or the dynein-specific antibody and followed by phase contrast microscopy as they progressed into mitosis. Metaphase cells were selected for injection by phase contrast microscopy by virtue of a clearly identifiable bipolar mitotic spindle. Injected cells were followed for up to 4 h after injection unless otherwise stated in the text and were processed for immunofluorescence microscopy as described above.
Mitotic Extracts
Mitotic extracts from HeLa cells were prepared according to Gaglio et al. (1995). HeLa cells were synchronized in the cell cycle by double block with 2 mM thymidine. After release from thymidine block the cells were allowed to grow for 6 h, and then nocodazole was added to a final concentration of 40 ng/ml. The mitotic cells that accumulated over the next 4 h were collected by mitotic shake off and incubated for 30 min at 37°C with 20 µg/ml cytochalasin B. The cells were then collected by centrifugation at 1,500 rpm and washed twice with cold PBS containing 20 µg/ml cytochalasin B. Cells were washed one last time in cold KHM buffer containing 20 µg/ml cytochalasin B and finally Dounce homogenized (tight pestle) at a concentration of 
3 x 107 cells/ml in KHM buffer containing 20 µg/ml cytochalasin B, 20 µg/ml phenylmethylsulfonyl fluoride, and 1 µg/ml each of chymostatin, leupeptin, antipain, and pepstatin. The crude cell extract was then subjected to sedimentation at 100,000 g for 15 min at 4°C. The supernatant was recovered and supplemented with 2.5 mM ATP (prepared as Mg2+ salts in KHM buffer) and 10 µM taxol, and the mitotic asters were stimulated to assemble by incubation at 30°C for 30–60 min. After incubation, samples were processed for indirect immunofluorescence microscopy as described above, and the remainder of the extract containing the assembled mitotic asters was subjected to sedimentation at 10,000 g for 15 min at 4°C. The supernatant and pellet fractions were both recovered and solubilized in SDS-PAGE sample buffer for immunoblot analysis.
Immunodepletions from the extract before aster assembly was carried out using 20–50 µg of either an anti-Eg5 affinity-purified rabbit polyclonal IgG or the monoclonal antibody 70.1, which is an IgM specific for the IC74 intermediate chain of cytoplasmic dynein. Each antibody was adsorbed onto 25 µl of either protein A- or protein G-conjugated agarose (Boehringer Mannheim, Indianapolis, IN). The 70.1 monoclonal antibody against cytoplasmic dynein intermediate chain was coupled to protein G-conjugated agarose using goat anti–murine IgM specific antibody (Vector Lab. Burlingame, CA). The antibody-coupled agarose was washed in KHM buffer and then packed by centrifugation to remove the excess fluid. Efficient depletion of each target protein was routinely achieved by sequential depletion reactions in which the total quantity of packed agarose did not exceed 15 µl per 100 µl of extract. First, half of the antibody-coupled agarose was resuspended with the mitotic extract and incubated with agitation for 1 h at 4°C. After this incubation the agarose was removed from the extract by sedimentation at 15,000 g for 10 s and saved. Next, the extract was recovered and used to resuspend the other half of the antibody-coupled agarose and another incubation performed with agitation for 1 h at 4°C. After this incubation the agarose was removed by sedimentation at 15,000 g for 10 s and pooled with the agarose pellet from the initial depletion reaction. In all cases, immunoblot analysis indicates that this depletion protocol results in nearly 100% efficient depletion of the target protein as described previously (Gaglio et al., 1996). The depleted extract was recovered and microtubule polymerization induced by the addition of taxol and ATP and incubation at 30°C. Each depletion experiment was performed at least two times and in all cases the efficiency of mitotic aster formation (as determined by counting the average number of asters per microscope field) was not significantly different from the values determined previously (Gaglio et al., 1996).
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-tubulin (data not shown) and were nucleating microtubules normally forming small astral microtubule arrays, but were separated from the body of the spindle (Fig. 3, C and D, arrowheads). Thus, despite the presence of functional centrosomes, the minus ends of the microtubules became unfocused and were displaced from the centrosomes after the injection of this dynein-specific antibody into metaphase cells.
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The alteration in the efficiency with which dynactin associates with microtubules in the presence of the dynein-specific antibody suggests that addition of this dynein-specific antibody to the extract may have functional consequences that are different from inactivation of cytoplasmic dynein alone. To determine if the reduction of dynactin association with microtubules induced by the addition of the dynein-specific antibody is functionally involved in the disruption of mitotic aster formation, we compared the effects of the addition of the dynein-specific antibody to the depletion of cytoplasmic dynein (Fig. 6). In this experiment, it was necessary to either deplete cytoplasmic dynein or add the 70.1 antibody to extracts depleted of the plus end-directed kinesin-related protein Eg5. The formation of mitotic asters in this system requires cytoplasmic dynein, and asters fail to organize in the absence of cytoplasmic dynein alone due to the imbalance in forces generated by microtubule motors during aster assembly. Mitotic asters will form in the absence of cytoplasmic dynein, however, if the forces generated by microtubule motors are partially equilibrated by the simultaneous depletion of the plus end-directed motor Eg5 (Gaglio et al., 1996). Thus, if the depletion of cytoplasmic dynein is functionally equivalent to the addition of the dynein-specific 70.1 antibody, then mitotic asters should be observed after either the simultaneous depletion of cytoplasmic dynein and Eg5 or addition of the 70.1 antibody to an Eg5-depleted extract. Fig. 6 shows that in the absence of Eg5 alone, microtubules organize into astral arrays that are larger than typical mitotic asters, they lack a well formed central core, and NuMA is diffusely localized at the center (Fig. 6 B; Gaglio et al., 1996). In the absence of both Eg5 and cytoplasmic dynein, mitotic asters form that resemble those formed in the absence of Eg5 alone, although they are somewhat less well organized (Fig. 6 C; Gaglio et al., 1996). Thus, if the 70.1 antibody only affects the function of cytoplasmic dynein, then addition of the 70.1 antibody to an Eg5-depleted extract should also yield asters. Contrary to this prediction, mitotic asters did not form when the 70.1 antibody was added to an Eg5-depleted extract, while addition of the control antibody had no observable effect on the formation of astral microtubule arrays (Fig. 6, D and E). Thus, in this cell-free system the depletion of cytoplasmic dynein is not functionally equivalent to the addition of this dynein-specific antibody. The most likely explanation for this difference is that the dynein-specific antibody both directly affects cytoplasmic dynein and indirectly affects dynactin such that the presence of the 70.1 antibody is analogous to the simultaneous disruption of dynein and dynactin. While we can not rule out the possibility that this antibody has additional deleterious effects beyond the perturbation of cytoplasmic dynein and dynactin, this interpretation is consistent with our previous results showing that the depletion of dynactin is more deleterious to mitotic aster formation than the depletion of cytoplasmic dynein (Gaglio et al., 1996).
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Based on these data, we propose that mitotic spindle formation in somatic cells proceeds through a search-capture-focus mechanism (Fig. 8). This model expands on the search-capture model (Kirschner and Mitchison, 1986) and begins with the nucleation of microtubule asters from centrosomes. The plus ends of these microtubules "search" the cytoplasm by rapidly converting between growing and shrinking states and are "captured" and stabilized by kinetochores. At some point during the search and capture process microtubules are released (or severed) from the centrosome, and these microtubules become "focused" by structural and motor proteins into a spindle pole with their free minus ends near the centrosome (Fig. 8). The centrosome remains tethered to this newly focused array through a lateral interaction between microtubules within this array and astral microtubules that continue to emanate from the centrosome (Fig. 8).
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-tubulin ring complexes (Zheng et al., 1996). These short microtubules associate randomly with chromatin in disorganized arrays and are then organized into parallel bundles (Steffen et al., 1986; Theurkauf and Hawley, 1992; Heald et al., 1996). In somatic cells, microtubules are nucleated from -tubulin ring complexes that are associated with centrosomes (Moritz et al., 1996), which establishes an oriented microtubule array (mitotic asters) with microtubule plus ends that search the cytoplasm and are captured by kinetochores. Despite these differences in the initial search and capture stages of spindle formation, both systems appear to use a common mechanism to "focus" the free microtubule minus ends into spindle poles. The parallel bundles of microtubules in acentrosomal spindles are focused at their minus ends (Theurkauf and Hawley, 1992; Matthies et al., 1996; Merdes et al., 1996; Heald et al., 1996), while in centrosomal spindles free microtubule minus ends are focused onto the astral microtubule array. This process of focusing free microtubule minus ends is much more pronounced in acentrosomal meiotic systems, because unlike mitotic systems in which microtubules are inherently focused from centrosomes, microtubules in acentrosomal meiotic systems have no organization before the focusing activity exerted by the noncentrosomal components. According to this search-capture-focus model for spindle assembly it may be possible to separate the microtubule nucleating activity associated with centrosomes in somatic cells from the focusing activity exerted by the noncentrosomal structural and motor proteins. In fact, this possibility has already been confirmed under a variety of different experimental conditions. First, there are several reports in the literature that centrosomes have detached from the body of the spindle while the microtubule minus ends remain focused in a pole (Rieder and Hard, 1990; Mitchison and Salmon, 1992; Murray et al., 1996). These poles are functional because they support chromosome segregation, and in one case it was observed that the microtubule turnover associated with poleward microtubule flux continued to converge towards this pole (Mitchison and Salmon, 1992). Second, centrosomes can be mechanically detached from the body of the mitotic spindle at metaphase, and the minus ends of the mitotic spindle remain focused; and in some cases the chromosomes still migrate toward that focused collection of microtubule minus ends despite the removal of the centrosome (Hiramoto and Nakano, 1988; Nicklas, 1989; Nicklas et al., 1989). Third, in rare cases where microtubules associate with chromosomes in the absence of centrosomes and/or centrioles in cultured cells (Brenner et al., 1977; Keyer et al., 1984; Debec et al., 1995), or if the requirement for centrosomes in microtubule nucleation is bypassed by the addition of taxol both in vivo during mitosis (DeBrabander et al., 1981) and in vitro in mitotic extracts (Gaglio et al., 1995, 1996), then microtubules are still organized into astral and polar arrays. The focusing of microtubule minus ends under these conditions is likely the manifestation of the microtubule minus end focusing activity exerted by the noncentrosomal components. Fourth, electron microscopy has shown that many microtubule minus ends within both mitotic and centrosome-containing meiotic spindles are not associated with centrosomes (Wolf and Bastmeyer, 1991; Mastronarde et al., 1993). Fifth, microtubule release from centrosomes has been documented in cell-free extracts (Belmont et al., 1990) as well as under nonmitotic circumstances in living cells (Keating et al., 1997). Finally, free microtubule minus ends within the mitotic spindle are necessary for tubulin subunit loss during poleward microtubule flux (Mitchison, 1989b). Taken together, these results clearly discriminate between the processes of microtubule nucleation and minus end focusing during mitosis in somatic cells, and demonstrate that noncentrosomal structural and motor proteins will focus microtubule minus ends independently of centrosomes in somatic cells through a mechanism that is probably related to spindle pole formation in acentrosomal systems.
Finally, prevailing evidence indicates that the mechanism for focusing free microtubule minus ends into spindle poles in both centrosomal and acentrosomal spindles is driven by a common group of noncentrosomal accessory proteins including NuMA, cytoplasmic dynein, dynactin, Eg5, and a minus end-directed kinesin-related protein (Verde et al., 1991; Sawin et al., 1993; Endow et al., 1994; Gaglio et al., 1995, 1996; Blangy et al., 1996; Heald et al., 1996; Matthies et al., 1996; Merdes et al., 1996; Walczak et al., 1997). Experimental data indicate that all of these proteins participate in the organization of spindle poles in both centrosomal and acentrosomal systems. Despite the complex nature of this process and the involvement of numerous components, recent evidence suggests that a trimolecular complex composed of NuMA, cytoplasmic dynein, and dynactin may be crucial for focusing free microtubule minus ends at spindle poles. These three proteins form a stable complex in extracts prepared from Xenopus eggs, and this complex of proteins is essential for the organization of spindle poles in that system (Merdes et al., 1996). While no evidence exists for a stable complex between these proteins in extracts prepared from somatic cells, we show that NuMA fails to concentrate near microtubule minus ends in the absence of dynein and/or dynactin under both in vitro and in vivo conditions, consistent with a dynein/dynactin-dependent movement of NuMA to microtubule minus ends (Figs. 3 and 5, and Gaglio et al., 1996). Indeed, in a striking group of experiments, the perturbation of either cytoplasmic dynein (mAb 70.1 microinjection; present work), dynactin (dynamitin over expression; Echeverri et al., 1996; Gaglio et al., 1996), or NuMA (antibody microinjection; Gaglio et al., 1995) in cultured cells all produced a similar effect on the spindle pole organization characterized by splaying of microtubule minus ends and detachment of centrosomes. Given that the interaction of NuMA with cytoplasmic dynein and dynactin is mitosis-specific in somatic cells (NuMA is nuclear during interphase), it is possible that NuMA confers a unique mitosis-specific property to the minus end-directed motor activity of cytoplasmic dynein and dynactin, which contributes to the essential function of this trimolecular complex during spindle formation.
In the end, we speculate that free microtubule minus ends are necessary for proper spindle function, because they are necessary for the mechanism of poleward microtubule flux, which exerts force through the spindle (Waters et al., 1996) and (depending on the cell type) contributes to poleward chromosome movement (Salmon, 1992; Wilson et al., 1994; Mitchison and Salmon, 1992; Zhai et al., 1995). Free microtubule minus ends are inherently produced in acentrosomal spindles, whereas in centrosomal spindles they must be generated by microtubule release from centrosomes. In both cases, a common pole-forming activity focuses the free microtubule ends. In somatic cells, these free microtubule minus ends that are obligatory to poleward microtubule flux remain attached to the astral microtubules emanating from the centrosome, thus allowing the centrosome-associated astral array to convey positional cues derived from the cell cortex to the body of the spindle.
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Acknowledgments |
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Submitted: 19 June 1997
Revised: 14 July 1997
1. Abbreviation used in this paper: NuMA, nuclear mitotic apparatus. -tubulin antibody, and Dr. Trina Schroer (Johns Hopkins University, Baltimore, MD) for donating the dynactin-specific antibodies. We would also like to recognize the tolerance of Leslie Henderson and Bob Maue during microinjections and thank Alejandro Saredi, Vicki Mountain, Arijit Chakravarty, and Roger Sloboda for stimulating discussion during the preparation of this manuscript.
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