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© The Rockefeller University Press, 0021-9525/2001//425 $5.00
The Journal of Cell Biology, Volume 152, Number 3, , 2001 425-434

Chromosome Movement in Mitosis Requires Microtubule Anchorage at Spindle Poles

^a Department of Biochemistry, Dartmouth Medical School, Hanover, New Hampshire 03755
^b Rippel Electron Microscope Facility, Dartmouth College, Hanover, New Hampshire 03755
Department of Biochemistry, Dartmouth Medical School, Hanover, NH 03755.(603) 650-1128(603) 650-1990

duane.a.compton{at}dartmouth.edu

Anchorage of microtubule minus ends at spindle poles has been proposed to bear the load of poleward forces exerted by kinetochore-associated motors so that chromosomes move toward the poles rather than the poles toward the chromosomes. To test this hypothesis, we monitored chromosome movement during mitosis after perturbation of nuclear mitotic apparatus protein (NuMA) and the human homologue of the KIN C motor family (HSET), two noncentrosomal proteins involved in spindle pole organization in animal cells. Perturbation of NuMA alone disrupts spindle pole organization and delays anaphase onset, but does not alter the velocity of oscillatory chromosome movement in prometaphase. Perturbation of HSET alone increases the duration of prometaphase, but does not alter the velocity of chromosome movement in prometaphase or anaphase. In contrast, simultaneous perturbation of both HSET and NuMA severely suppresses directed chromosome movement in prometaphase. Chromosomes coalesce near the center of these cells on bi-oriented spindles that lack organized poles. Immunofluorescence and electron microscopy verify microtubule attachment to sister kinetochores, but this attachment fails to generate proper tension across sister kinetochores. These results demonstrate that anchorage of microtubule minus ends at spindle poles mediated by overlapping mechanisms involving both NuMA and HSET is essential for chromosome movement during mitosis.

Key Words: chromosome • kinetochore • spindle pole • NuMA • HSET

© 2001 The Rockefeller University Press

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

 
The spindle is a complex microtubule-based superstructure responsible for chromosome movement and segregation during mitosis and meiosis (McIntosh and Koonce 1989; Mitchison 1989a; Rieder 1991; Hyman and Karsenti 1996; Compton 2000). Chromosome movement on spindles during mitosis in cultured cells has been well documented (Gorbsky 1992; Rieder and Salmon 1994; Inoué and Salmon 1995; Rieder and Salmon 1998; Khodjakov et al. 1999) and is driven by three different force-generating mechanisms (Mitchison 1989b; Gorbsky 1992; Rieder and Salmon 1994; Khodjakov and Rieder 1996; Khodjakov et al. 1999). Poleward chromosome movement is driven by forces derived from kinetochore-associated microtubule motor proteins and the continuous poleward flux of tubulin subunits within the spindle lattice. Kinetic analyses indicate that a majority (60–70%) of poleward chromosome movement in cultured somatic cells is driven by forces generated by kinetochore-associated motors (Mitchison and Salmon 1992), and candidates for these motors are the kinesin-related proteins CENP-E and MCAK/XKCM1 as well as cytoplasmic dynein (Rieder and Alexander 1990; Pfarr et al. 1991; Steuer et al. 1991, Yen et al. 1991; Walczak et al. 1996; Schaar et al. 1997; Wood et al. 1997; Maney et al. 1998). Chromosome movement away from spindle poles during congression is driven by polar ejection forces (Rieder et al. 1986) that may be generated by chromosome-associated kinesin-related proteins (Antonio et al. 2000; Funabiki and Murray 2000).

An implicit assumption in how these force-generating mechanisms cause chromosome movement is that microtubule minus ends are firmly anchored at spindle poles. It has been suggested that this anchorage is necessary in anaphase to "bear the load when chromosomes move, so that the chromosomes move toward the poles rather than the poles toward the chromosome" (Nicklas 1989). In its extreme form, this idea posits that if the microtubule minus ends were not appropriately anchored at spindle poles, then the poleward forces generated by kinetochore-associated motors (coupled to microtubule depolymerization) would pull the microtubules in toward the chromosome rather than move the chromosome toward the pole. Indeed, direct observation of microtubule-chromosome interactions under defined in vitro conditions has demonstrated that microtubules are reeled in toward the chromosomes in the absence of anchorage at minus ends (Koshland et al. 1988). Likewise, the polar ejection forces would extrude the microtubules past the region of the spindle pole toward the cell cortex instead of pushing the chromosome toward the spindle equator.

Our understanding of the mechanisms for microtubule minus end anchorage at spindle poles has grown substantially in the past few years (Merdes and Cleveland 1997; Compton 1998). Centrosomes are the dominant site for microtubule nucleation and, when present, are located at spindle poles as a consequence of their function in microtubule nucleation. However, a variety of evidence demonstrates that centrosomes are neither necessary nor sufficient to act as functional spindle poles, and chromosome movement occurs normally in cells lacking centrosomes and in cells where centrosomes have been experimentally removed (Szollosi et al. 1972; Nicklas 1989; Heald et al. 1996; Gaglio et al. 1997; Khodjakov et al. 2000). These observations demonstrate that centrosomes cannot be the primary anchorage sites for microtubule minus ends at spindle poles in vertebrate cells. Thus, we hypothesize that noncentrosomal proteins provide the primary anchorage site for microtubule minus ends at poles to counterbalance the forces involved in chromosome movement. To test this hypothesis, we monitored chromosome movement in cultured cells after perturbation of nuclear mitotic apparatus protein (NuMA) and human homologue of the KIN C motor family (HSET), two noncentrosomal proteins involved in focusing microtubule minus ends at spindle poles (McDonald et al. 1990; Kallajoki et al. 1991; Hatsumi and Endow 1992; Yang and Snyder 1992; Endow et al. 1994; Gaglio et al. 1995; Kuriyama et al. 1995; Matthies et al. 1996; Merdes et al. 1996, Merdes et al. 2000; Walczak et al. 1997; Matuiene et al. 1999; Mountain et al. 1999). The results show that simultaneous perturbation of both NuMA and HSET virtually abolishes chromosome movement in cultured cells despite bi-oriented spindle assembly and microtubule attachment to kinetochores. These results indicate that NuMA and HSET act through overlapping mechanisms to hold microtubule minus ends at spindle poles and permit chromosome movement to be driven by kinetochore- and polar ejection–derived forces.

	Materials and Methods

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Cell Culture
CFPAC-1 cells were maintained at 37°C in a 5%-CO₂ atmosphere in Iscove's Modified Dulbecco's Medium containing 10% fetal bovine serum, 50 IU/ml penicillin, and 50 µg/ml streptomycin.

Antibodies
Rabbit polyclonal antibodies against NuMA were generated by immunization with the full-length recombinant NuMA protein (Gaglio et al. 1995). Rabbit polyclonal antibodies against HSET were generated by immunization with the recombinant protein representing the COOH-terminal 377 amino acids (Mountain et al. 1999). Tubulin was detected with the DM1 mouse monoclonal antibody (Sigma-Aldrich). Kinetochores were detected with the human anticentromere antibody ACA-m (provided by Kevin Sullivan, Scripps Research Institute, San Diego, CA), and CENP-E was detected using the mouse monoclonal antibody mAb177 (Yen et al. 1991; provided by Tim Yen, Fox Chase Cancer Center, Philadelphia, PA).

Antibody Microinjection
CFPAC-1 cells growing on photo-etched alphanumeric glass cover slips (Bellco Glass Co.) were microinjected following the procedures of Compton and Cleveland 1993 and Capecchi 1980. IgG was purified from whole serum for microinjection by affinity chromatography using protein A-conjugated agarose (Roche Molecular Biochemicals). PD-10 Sephadex G-25 columns (Amersham Pharmacia Biotech) were used for buffer exchange to microinjection buffer (100 mM KCl, 10 mM KPO₄, pH 7.0), followed by concentration using Centricon spin columns (Millipore). The following antibody concentrations refer to their concentrations in the microinjection needle: 20 mg/ml -NuMA, 10 mg/ml -HSET, and 19 mg/ml nonimmune IgG.

Time-Lapse Microscopy
Cells were injected in the cytoplasm during interphase and monitored by phase-contrast microscopy until they entered prophase (as judged by chromosome condensation). The coverslip was then mounted on a custom-built stainless steel modified Rose chamber containing growth medium and sealed with VALAP (Vaseline, lanolin, and paraffin wax in a 1:1:1 mass ratio). The chamber was placed on a heated stage, and differential interference contrast (DIC) images were acquired at 30-s intervals with a Hamamatsu Orca II cooled CCD camera using the Openlab software (Improvision Inc.) on an Axioplan 2 microscope using a Plan-Apochromat 63x (NA 1.4) objective (Carl Zeiss, Inc.). To minimize file sizes, the supplemental video sequences accompanying this article only contain images acquired every minute.

Chromosome velocities were obtained from the digital time-lapse record of each cell. The microscopy system used for time-lapse recordings was calibrated using a stage micrometer under the same conditions used for image acquisition. Individual chromosome movement was tracked by frame-by-frame analysis of digital images using Openlab software (Improvision, Inc.). The straight line calibration tool in the Openlab software package was used to determine the distance traveled by an individual chromosome between different time points. Velocities were then calculated by dividing the total distance traveled (microns) by the time interval in which the measurements were made (minutes). The spindle equator was used as a frame of reference in many images due to the lack of organized poles, and was assigned as the position where a bulk of the chromosomes were aligned. Chromosome movement was judged to be directed when the chromosome was displaced by >3 µm in a linear fashion. Displacement of this magnitude is easily distinguishable from Brownian motion (see Alexander and Rieder 1991).

Indirect Immunofluorescence Microscopy
Cells to be processed for immunofluorescence were first immersed in microtubule stabilizing buffer (MTSB: 4 M glycerol, 100 mM PIPES, pH 6.8, 1 mM EGTA, 5 mM MgCl₂) for 1 min. Cells were then extracted with MTSB/0.5% Triton X-100 for 2 min, followed by a 2-min rinse in MTSB. Cells were then fixed in 1% glutaraldehyde in PBS for 10 min, followed by two 10-min treatments with 0.5 mg/ml NaBH₄, and a 5-min wash in TBS (10 mM Tris, pH 7.5, 150 mM NaCl) containing 1% BSA (TBS-BSA). Primary antibody was diluted in TBS-BSA and added to the cells for 30 min in a humidified chamber. The cells were washed for 5 min in TBS-BSA and stained with the appropriate fluorochrome-conjugated, species-specific secondary antibodies in TBS-BSA along with 1 µg/ml DAPI (Sigma-Aldrich). Coverslips were washed for 5 min in TBS-BSA, and then mounted in Vectashield (Vector Laboratories).

Cells to be stained for kinetochore components were fixed in 3.5% paraformaldehyde in PBS for 5 min at room temperature, followed by extraction with TBS-BSA/0.5% Triton X-100 for 5 min and a 5-min wash in TBS-BSA. All subsequent antibody treatments were as described above.

Fluorescent images were captured with a Hamamatsu Orca II cooled CCD camera mounted on an Axioplan 2 microscope equipped for epifluorescence. A series of 0.5-µm optical sections were collected in the z plane for each channel (DAPI, fluorescein, and/or Texas red) and deconvolution using the Openlab software (Improvision Inc.) was used to eliminate extraneous fluorescence background. Selected planes from the z series were then overlayed to generate the final image.

Electron Microscopy
The position of injected CFPAC-1 cells on the alphanumeric coverslips was noted for subsequent selection for examination by electron microscopy. Cells were rinsed in MTSB for 1 min, extracted with MTSB/2% Triton X-100 for 5 min, and washed with MTSB for 2 min at room temperature. Cells were then fixed in 1% glutaraldehyde in 0.1 M Na-cacodylate buffer for at least 30 min. After fixation, the cells were rinsed twice with 0.1 M Na-cacodylate buffer, and then postfixed with 1% OsO₄ in Na-cacodylate buffer for 30 min at room temperature, and en bloc stained in 2% uranyl acetate for 30 min at room temperature. Cells were dehydrated through a graded series of ethanols and propylene oxide, and flat embedded in epon (LX112)/araldite(502). The glass coverslip was removed by etching in cold concentrated hydrofluoric acid, as described by Moore 1975 and Rieder and Bowser 1987. The area containing the injected cells was identified under a dissecting microscope, cut out of the flat embedded rectangle, and remounted onto epoxy blanks. Sections (90–200 nm) were stained with 2% aqueous uranyl acetate for 45 min at 50°C and with Reynold's lead citrate for 20 min at room temperature. Electron micrographs were taken at 80 or 100 kV on a JEOL 100CX.

Online Supplemental Material
Quicktime videos to accompany Fig. 1Fig. 2Fig. 3Fig. 4 are available at http//:www.jcb.org/cgi/content/full/152/3/425/DC1.

View larger version (89K): [in this window] [in a new window] [Download PPT slide]   Figure 1 Chromosome movement in a CFPAC-1 cell microinjected with antibodies to NuMA. (A) Selected DIC images from the video record of a mitotic cell that has been microinjected with an antibody to NuMA. Times are indicated in hours:minutes:seconds. The arrow highlights a chromosome that makes a pronounced movement toward the cell equator. (B and C) The cell featured in A (B) and a second, unrelated injected mitotic CFPAC-1 cell (C) were fixed and processed for immunofluorescence microscopy using antibodies specific for tubulin, the injected NuMA antibody, and the DNA-specific dye DAPI, as indicated. Arrows indicate centrosomes and arrowheads indicate sites of microtubule convergence (see Video 1 in online supplement). Bar: 20 µm.

View larger version (74K): [in this window] [in a new window] [Download PPT slide]   Figure 2 Chromosome movement in a cell microinjected with antibodies to HSET. (A) Selected DIC images from the video record of a mitotic cell that has been microinjected with an antibody to HSET. Times are indicated in hours:minutes:seconds. (B and C) The cell featured in A (B) and a second, unrelated injected mitotic CFPAC-1 cell (C) were fixed and processed for immunofluorescence microscopy using antibodies specific for tubulin, the injected HSET antibody, and the DNA-specific dye DAPI, as indicated. The arrowhead highlights a microtubule bundle protruding from the main body of the spindle (see Video 2 in online supplement). Bar: 20 µm.

View larger version (72K): [in this window] [in a new window] [Download PPT slide]   Figure 3 Chromosome movement in a cell microinjected with antibodies to both NuMA and HSET. (A) Selected DIC images from the video record of a mitotic cell that has been microinjected with antibodies to both NuMA and HSET. Times are indicated in hours:minutes:seconds. (B) The cell featured in A was fixed and processed for immunofluorescence microscopy using antibodies specific for tubulin, the injected antibodies (since both the NuMA- and HSET-specific antibodies were generated in rabbits, this panel shows the location of both), and the DNA specific dye DAPI, as indicated. (C) Merged image of the tubulin and injected antibody signals (see Video 3 in online supplement). Bar: 20 µm.

View larger version (116K): [in this window] [in a new window] [Download PPT slide]   Figure 4 Chromosome movement in a cell treated with nocodazole. (A) Selected DIC images from the video record of a mitotic cell cultured in the presence of 200 nM nocodazole. Times are indicated in hours:minutes:seconds. (B) The cell featured in A was fixed and processed for immunofluorescence microscopy using antibodies specific for tubulin and the DNA-specific dye DAPI, as indicated (see Video 4 in online supplement). Bar: 20 µm.

	Results

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In many of the -NuMA–injected cells, we noticed that microtubule minus ends were loosely focused into pole-like regions (Fig. 1 B, arrowheads). In some cases, nearly bipolar spindles formed with two focused poles, although the centrosomes were not associated with those pole-like regions (Fig. 1 C, see also Figure 9 F in Gaglio et al. 1995). This suggests that other factors promote microtubule focusing at poles in the absence of NuMA activity. A strong candidate for this activity is the minus end–directed KIN C motor, which has been shown to play a role in spindle pole organization in numerous different systems (McDonald et al. 1990; Hatsumi and Endow 1992; Endow et al. 1994; Kuriyama et al. 1995; Matthies et al. 1996; Walczak et al. 1997; Matuiene et al. 1999; Mountain et al. 1999). To determine whether perturbation of HSET affects chromosome movement, we microinjected interphase cells in the cytoplasm with antibodies against HSET and monitored chromosome dynamics in those cells that subsequently entered mitosis (Fig. 2). Time-lapse DIC microscopy of a cell injected with HSET-specific antibodies showed that chromosome movement resembles control cells (Fig. 2 A) with the rates of poleward, away from the pole, and anaphase movements being not significantly different from uninjected control cells (t test, P = 0.40, 0.46, and 0.27 for poleward, away from the pole, and anaphase motion, respectively; Table ). We are confident that these antibodies block HSET function for several reasons. First, these antibodies have previously been shown to block microtubule organization into poles under acentrosomal conditions in mitotic extracts and in mouse oocytes (Mountain et al. 1999). Second, the injected antibody is concentrated near the spindle poles, suggesting it interacts with HSET and displaces it from its typical localization throughout the spindle (Fig. 2B and Fig. C). Third, the duration of prometaphase in -HSET–injected cells increased to 77.5 ± 30.0 min compared with control cells that complete prometaphase, on average, in 38.5 ± 10.3 min, consistent with previous results showing that perturbation of KIN C motor proteins causes a decrease in spindle assembly efficiency and increases the duration of prometaphase (Matthies et al. 1996; Walczak et al. 1997; Matuiene et al. 1999). Finally, examination of spindle structure in injected cells during metaphase frequently showed microtubule bundles protruding from the main body of the spindle (Fig. 2 C, arrowhead), a hallmark of the loss of KIN C motor function (Endow et al. 1994; Hatsumi and Endow 1992; Matthies et al. 1996; Walczak et al. 1997; Matuiene et al. 1999; Mountain et al. 1999). Thus, the perturbation of the KIN C motor HSET perturbs spindle structure prolonging prometaphase, but there is no detectable effect on the rates of chromosome movement.

That microtubule minus ends were loosely organized at poles after perturbation of NuMA and tightly focused at poles after perturbation of HSET raised the possibility that these proteins play redundant roles in spindle pole function. To test this idea, we injected cells with antibodies to both NuMA and HSET and monitored chromosome dynamics by time-lapse DIC microscopy (Fig. 3). Chromosomes in cells injected with antibodies to both NuMA and HSET appeared to experience Brownian motion, but failed to undergo detectable directed movement (Fig. 3 A). Instead, the chromosomes remained loosely arranged near the cell center. In some cases (e.g., Fig. 3), chromosomes coalesced into a metaphase-like arrangement, but in other cases the chromosomes formed a loose group in the cell center and did not align efficiently (e.g., see Fig. 6 B). Spindles in cells injected with both antibodies were bi-oriented but lacked organized poles, and centrosomes were dissociated from the bulk of the microtubules connected to the chromosomes (Fig. 3 B). The injected antibody was concentrated around the centrosomes as well as in aggregates in the cytoplasm, consistent with the sequestration of NuMA and HSET away from their normal sites of localization (Fig. 3 C). Many of the chromosomes appeared to have K fibers associated with each sister kinetochore, and the K fibers extend normally toward opposite sides of the cell, but K fibers of different chromosomes did not focus at poles. These cells did not enter anaphase, similar to when cells were injected with NuMA-specific antibodies alone.

View larger version (64K): [in this window] [in a new window] [Download PPT slide]   Figure 6 CENP-E localizes normally to kinetochores in cells lacking organized spindle poles. CFPAC-1 cells that were uninjected (A) or microinjected with antibodies to both NuMA and HSET (B) were fixed and processed for immunofluorescence microscopy using antibodies to the kinetochore-associated motor protein CENP-E and the DNA-specific dye DAPI, as indicated. Bar: 20 µm.

We also monitored chromosome movement in mitosis in cells treated with nocodazole (Fig. 4). Nocodazole prevents the assembly of spindle microtubules, thereby eliminating any microtubule-dependent chromosome movement. Upon nuclear envelope breakdown in the presence of 200 nM nocodazole, chromosomes displayed Brownian motion and coalesced near the center of the cell, but did not show detectable directed movement (Fig. 4 A). Immunofluorescence microscopy verified the lack of a spindle in this cell and the presence of only small clumps of short residual microtubules (Fig. 4 B). Thus, chromosome behavior in nocodazole-treated cells is similar to cells lacking both HSET and NuMA activities despite the fact that nocodazole-treated cells lack spindle microtubules and cells injected with both NuMA- and HSET-specific antibodies have bi-oriented spindle-like structures. Chromosomes may coalesce near the cell center under both these conditions because that is the thickest part of the cell.

Microtubule Attachment to Kinetochores in Cells Lacking Organized Poles
To verify that microtubules were attached to kinetochores in cells injected with antibodies to both NuMA and HSET, we examined injected cells by transmission electron microscopy (Fig. 5). Uninjected control cells showed organized spindles with tightly focused spindle poles (Fig. 5 A). In contrast, cells injected with antibodies to both NuMA and HSET lacked organized spindle poles (Fig. 5 B), consistent with images obtained by fluorescence microscopy (Fig. 3 B). At high magnification, many of the chromosomes had identifiable kinetochores and multiple microtubules were observed attached to both kinetochores, consistent with the formation of bi-oriented K fibers (Fig. 5 C). These data demonstrate that the lack of directed chromosome movement in the absence of organized spindle poles does not arise from a lack of microtubule binding to kinetochores or formation of K fibers, although this limited analysis does not permit us to determine whether each kinetochore has obtained a full complement of microtubules.

View larger version (109K): [in this window] [in a new window] [Download PPT slide]   Figure 5 Microtubule attachment to kinetochores in microinjected cells. CFPAC-1 cells that were uninjected (A) or microinjected with antibodies to both NuMA and HSET (B) were processed for transmission electron microscopy. Arrows in A and B point to centrosomes. The electron-dense material detected in B near the centrosomes is most likely the antibody-induced aggregates of NuMA and HSET, which are prominently detected by immunofluorescence microscopy. (C) High magnification views to highlight kinetochore-microtubule interactions in the chromosomes identified as 1–4 in B. The kinetochore regions of chromosome 2 were located in the adjacent serial section from that shown in B. Bars: (A and B) 3 µm; (C) 100 nm.

Tension Across Sister Kinetochores Is Reduced upon Disruption of Spindle Poles
Forces acting to move chromosomes during mitosis also generate tension between sister kinetochores during prometaphase and metaphase (Nicklas et al. 1995; Waters et al. 1998). To test whether proper tension was generated across sister kinetochores in cells lacking organized spindle poles, we fixed and processed control and injected cells for immunofluorescence analysis using a human autoimmune sera that specifically recognizes centromeric antigens. We then measured the distances between sister kinetochores (Fig. 7 and Table ). Uninjected cells, control injected cells, and cells injected with antibodies to either NuMA or HSET each showed an average interkinetochore distance slightly >3 µm. Cells that entered mitosis in the presence of 10 µM nocodazole lack spindle microtubules and showed an average interkinetochore distance of only 1.6 µm, consistent with previously published results showing that microtubule-dependent forces are involved in generating tension between sister kinetochores. The relaxed interkinetochore distance observed in the presence of nocodazole was similar to that observed in untreated early prometaphase cells before chromosome–microtubule interactions (data not shown). Mitotic cells injected with both NuMA- and HSET-specific antibodies displayed interkinetochore distances of 2.5 µm. This 20% reduction in interkinetochore distance is significant (t test, P < 0.0001), and demonstrates that full tension is not generated across sister kinetochores in the absence of organized spindle poles despite microtubule attachment to kinetochores.

View larger version (39K): [in this window] [in a new window] [Download PPT slide]   Figure 7 Interkinetochore distances in cells with disorganized spindle poles. Four representative pairs of kinetochores are shown for an uninjected control mitotic cell, a mitotic cell injected with antibodies to both NuMA and HSET, and a cell treated with 10 µM nocodazole, as indicated. Centromere regions were visualized by staining with an anticentromere-specific autoimmune serum. Bar: 2.5 µm.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

A prediction from these data is that chromosome movement during anaphase A should be inhibited in the absence of HSET and NuMA function. Unfortunately, we were unable to examine that possibility due to the activity of the checkpoint that prevents anaphase onset. The checkpoint may remain active in these cells for a variety of reasons including the reduced tension across sister kinetochores, the potential role of spindle poles in regulating Mad2 activity (Howell et al. 2000), or the possibility that spindle pole integrity is necessary for proper cyclin B proteolysis (Clute and Pines 1999; Wakefield et al. 2000). We are currently investigating how specific components of the checkpoint (i.e., Mad2) are affected by spindle pole disruption and whether inactivation of the checkpoint permits us to follow chromosome movement during anaphase in cells lacking organized poles.

A striking feature of cells lacking both NuMA and HSET function is that bi-oriented spindle-like structures formed with well organized K fibers. This suggests that many of the constituent parts of the spindle function normally despite the absence of pole organization. For example, the paired sister kinetochores may dictate bi-orientation, and cross-linking proteins such as Eg5 may bundle microtubules into K fibers despite the fact that those K-fibers do not focus tightly at poles. Moreover, steric interactions between K fibers may inhibit the diffusion of chromosomes contributing to a metaphase plate-like arrangement of chromosomes in some of these cells. It is also striking that interkinetochore distances were only reduced by 20% under conditions where chromosome motion was suppressed. The most likely explanation for this is that the force needed to stretch kinetochores is smaller than the force needed for chromosome movement, and our experiments caused a reduction in poleward forces sufficient to suppress chromosome movement while only minimally reducing sister kinetochore stretching. Support for this interpretation comes from the work of Waters et al. 1996, who demonstrated that the force generated from poleward microtubule flux alone was sufficient to maintain kinetochores in a fully stretched configuration in the absence of forces generated by kinetochore-associated motors. Thus, the fact that many aspects of spindle assembly appear normal in cells injected with antibodies to both NuMA and HSET lends support to the conclusion that the only aspect of spindle function perturbed in these cells is the organization of microtubule ends at spindle poles.

Models for Microtubule Anchorage at Spindle Poles
Two models are most plausible to explain how microtubule anchorage at spindle poles contributes to chromosome movement, and both of these ideas have been proposed previously in alternate forms. One model involves the anchorage of microtubule minus ends in a matrix (McIntosh 1980; Pickett-Heaps et al. 1982; Rebhun and Palazzo 1988; Nicklas 1989). This matrix would bind to microtubules and hold the minus ends so that poleward forces generated at kinetochores would cause chromosomes to move relative to the poles rather than the poles relative to the chromosomes (Fig. 8 A). If the interaction between this matrix and microtubules were disrupted, then the drag the matrix imposes on microtubules would be relieved and chromosome movement would stall due to the lack of resistance on kinetochore microtubules.

View larger version (28K): [in this window] [in a new window] [Download PPT slide]   Figure 8 Models for the NuMA- and HSET-dependent anchorage of microtubules at spindle poles. (A) The matrix model posits that NuMA and an unidentified matrix element associated with HSET anchor microtubule ends at spindle poles. This anchorage creates drag on microtubules that provides the necessary resistance for forces generated by kinetochore-associated motors (large solid arrows) to create chromosome movement. (B) The microtubule cross-linking model posits that the cross-linking and minus end–directed motility (small arrows) of HSET and NuMA (in association with dynein) involved in focusing microtubules at spindle poles also creates physical linkages between kinetochore and nonkinetochore microtubules. This connects microtubules involved in poleward forces (large solid arrows) with microtubules involved in polar ejection forces (large open arrows), as well as interdigitating microtubules emanating from opposite poles, which constrains the positions of the spindle poles and permits chromosomes to move relative to the poles.

An alternative model involves the interaction of kinetochore and nonkinetochore (interpolar) microtubules at spindle poles (Fig. 8 B). In this model, NuMA and HSET cross link kinetochore microtubules to interpolar microtubules. This creates direct physical connections between microtubules experiencing compressive forces (kinetochore microtubules) with microtubules that could either passively resist those compressive forces (antiparallel interacting interpolar microtubules) or directly oppose those compressive forces through repulsive forces (polar ejection forces). In the absence of both NuMA and HSET activities, the linkages between interpolar and kinetochore microtubules are broken and chromosome movement stalls due to a lack of resistance on the kinetochore microtubules. We note, however, that while the specific subset of interpolar microtubules forming antiparallel interactions between the poles probably participate in this model, they cannot provide the primary resistance to poleward forces acting on kinetochore microtubules. This is evident from the fact that chromosome movement occurs normally on monopolar spindles and during anaphase-like prometaphase, two circumstances where antiparallel interactions between microtubules emanating from opposite poles are completely absent (Bajer 1982; Rieder et al. 1986; Rieder and Alexander 1990).

This model is supported by a variety of observations in the literature. First, micromanipulation experiments in grasshopper spermatocytes have demonstrated that physical associations exist among kinetochore and nonkinetochore spindle microtubules (Nicklas et al. 1982). These physical associations were shown to be tightest near the spindle poles, although some nonkinetochore microtubules were observed linked to kinetochore microtubules a substantial distance from the poles. Moreover, examination of spindles in PtK1 cells by electron microscopy has shown that a large percentage of interpolar microtubules have their minus ends associated with K fibers, and that these linkages occur an appreciable distance away from the centrosome (Mastronarde et al. 1993). Next, interactions between kinetochore and nonkinetochore microtubules has been argued to generate forces driving chromosome movement in several systems, including plant cells, as well as crane fly, grasshopper, and flatworm spermatocytes (Molè-Bajer 1969; Salmon and Begg 1980; Steffen and Fuge 1982; Bajer and Molè-Bajer 1986; Steffen 1986; Bajer 1990; Fuge and Falke 1991; Smirnova and Bajer 1992). In some of these cell types, the velocity of chromosome movement was positively correlated with the density of nonkinetochore microtubules interacting with the kinetochore microtubules. In other cases, it was shown that treatments that selectively disassemble nonkinetochore microtubules halt chromosome movement, which was only restored upon reestablishment of nonkinetochore microtubules after removal of the offending treatment. Finally, both HSET and NuMA (in association with cytoplasmic dynein) have microtubule cross-linking and minus end–directed motor activities (Merdes et al. 1996; Mountain et al. 1999). These two minus end–directed motors act redundantly in organizing microtubule minus ends at spindle poles (Walczak et al. 1998; Mountain et al. 1999), and that redundancy may be related to the functional redundancy we show here for HSET and NuMA during chromosome movement. This raises the possibility that the functional role that HSET and NuMA play in organizing microtubules at spindle poles may directly relate to how they create connections between interpolar and kinetochore microtubules to support chromosome movement as proposed in Fig. 8 B.

In summary, we provide evidence that NuMA and HSET cooperate to anchor microtubule minus ends at spindle poles to support chromosome movement. These data begin to define the specific proteins involved in the mechanics of chromosome movement and indicates that a common mechanism provides the microtubule anchorage necessary for chromosome movement in all vertebrate cells regardless of whether centrosomes are present or not. The models proposed to explain this mechanism are not mutually exclusive and it is possible that some combination of the spindle matrix and microtubule cross-linking models participate in this essential process. Further, these models imply that spindle poles are not only the sites to which microtubule minus ends converge physically, but they also act as sites for integration of different forces generated within the spindle.

	Acknowledgments

 
The authors thank Kevin Sullivan and Tim Yen for providing antibodies. We also thank Roger Sloboda and Gary Mack for providing comments on the manuscript and Conly Rieder for helpful discussions.

This work was supported by a grant from the National Institutes of Health (GM51542). The time-lapse microscopy equipment was purchased using a grant from the Fannie E. Rippel Foundation.

Submitted: 2 October 2000

Revised: 5 December 2000

Accepted: 8 December 2000

The online version of this article contains supplemental material.

Abbreviations used in this paper: DIC, differential interference contrast; HSET, human homologue of the KIN C motor family; MTSB, microtubule stabilizing buffer; NuMA, nuclear mitotic apparatus protein.

	References

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