Microtubule Flux Mediates Poleward Motion of Acentric Chromosome Fragments during Meiosis in Insect Spermatocytes

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Vol. 12, Issue 12, 4054-4065, December 2001

Microtubule Flux Mediates Poleward Motion of Acentric Chromosome Fragments during Meiosis in Insect Spermatocytes

James R. LaFountain Jr.,^* Rudolf Oldenbourg, Richard W. Cole,^§ and Conly L. Rieder^§

^*Department of Biological Sciences, University at Buffalo, Buffalo, New York 14260; Marine Biological Laboratory, Woods Hole, Massachusetts 02543; ^§Laboratory of Cell Regulation, Division of Molecular Medicine, Wadsworth Center, New York State Department of Health, Albany, New York 12201-0509; and Department of Biomedical Sciences, State University of New York, Albany, New York 12222

Submitted May 15, 2001; Revised July 27, 2001; Accepted September 10, 2001
Monitoring Editor: Ted Salmon

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

We applied a combination of laser microsurgery and quantitative polarization microscopy to study kinetochore-independent forcesthat act on chromosome arms during meiosis in crane fly spermatocytes.When chromosome arms located within one of the half-spindles duringprometa- or metaphase were cut with the laser, the acentric fragments(lacking kinetochores) that were generated moved poleward withvelocities similar to those of anaphase chromosomes (~0.5 µm/min).To determine the mechanism underlying this poleward motion ofdetached arms, we treated spermatocytes with the microtubule-stabilizingdrug taxol. Spindles in taxol-treated cells were noticeably short,yet with polarized light, the distribution and densities of microtubulesin domains where fragment movement occurred were not differentfrom those in control cells. When acentric fragments were generatedin taxol-treated spermatocytes, 22 of 24 fragments failed to exhibitpoleward motion, and the two that did move had velocities attenuatedby 80% (to ~0.1 µm/min). In these cells, taxol did not inhibitthe disjunction of chromosomes nor prevent their poleward segregationduring anaphase, but the velocity of anaphase was also decreased80% (~0.1 µm/min) relative to untreated controls. Together, thesedata reveal that microtubule flux exerts pole-directed forceson chromosome arms during meiosis in crane fly spermatocytes andstrongly suggest that the mechanism underlying microtubule fluxalso is used in the anaphase motion of kinetochores in thesecells.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

The poleward motion of a chromosome during mitosis or meiosis coincides with the shortening of its associated kinetochorefiber microtubules. Recent investigations on this motion havefocused on determining the site(s) where kinetochore microtubuledisassembly occurs, as well as on how the force for motion isgenerated. Two general models have arisen from these studies.In the "Pac-man" model, the kinetochore powers chromosome polewardmotion, which occurs along kinetochore microtubules that shortenby subunit removal at the kinetochore (reviewed in Rieder andSalmon, 1994). In this model kinetochore-associated minus end-directedmotors, such as cytoplasmic dynein, are envisioned to providethe force for chromosome movement, although it could also be generatedby the disassembly of kinetochore microtubule plus ends withinthe kinetochore (Inoue and Salmon, 1995). Such a model is supportedby the facts that dynein is present at kinetochores (Pfarr etal., 1990; Steurer et al., 1990; reviewed in Hoffman et al., 2001)and that its depletion attenuates the rate of poleward chromosomemotion (Savoian et al., 2000; Sharp et al., 2000).

Alternatively, in the "traction fiber" model, the chromosome is dragged poleward by the poleward motion of its associatedkinetochore microtubules that shorten by subunit removal at thepole (reviewed in Pickett-Heaps et al., 1996). In this model,force production is envisioned to occur, for example, as plusend-directed motors anchored within the spindle matrix interactwith and push all spindle microtubules poleward (Mitchison andSawin, 1990; Sawin and Mitchison, 1991). This model is supportedby microinjection (Mitchison et al., 1986) and photoactivationstudies (Mitchison, 1989), which reveal a "flux" of tubulin subunitsthat are constantly incorporated before anaphase into the plusends of microtubules while being removed from their minus endswithin the pole. The flux mechanism exerts a poleward force onthe chromosome when subunit incorporation at the kinetochore ceases,as occurs at anaphase onset (Waters et al., 1998).

The relative contribution that each of these mechanisms makes to the poleward motion of a chromosome appears to depend onthe system. The rate that kinetochore microtubules move polewardin spindles formed in Xenopus oocyte extracts is the same as therate exhibited by the chromosomes at anaphase (Desai et al., 1998).This suggests that poleward motion in this in vitro system ispowered entirely by flux. In contrast, in vertebrate somatic cells(Mitchison and Salmon, 1992; Zhai et al., 1995), both mechanismsappear to operate simultaneously, but the contribution made byflux is much less (~15-35%) than that made by the poleward movementofkinetochores.

In addition to those forces that act on kinetochores, the chromosome arms are also subjected to spindle-mediated forces throughoutthe division process. In vertebrate somatic cells, when the armof a prometaphase chromosome positioned near a pole is severedfrom the kinetochore, it is ejected away from the pole (reviewedin Rieder and Salmon, 1994). The "polar wind" propelling thatmotion appears to be mediated by plus end-directed motors associatedwith the chromosome arms (i.e., chromokinesin; Antonio et al.,2000; Funabiki and Murray, 2000). In contrast, when a pole-directedarm of a metaphase chromosome during plant (Hemanthus) mitosisis similarly severed from its kinetochore, it is transported polewardat the same velocity exhibited by chromosomes during anaphase(Khodjakov et al., 1996). The force-producing mechanism behindthis motion remains to be determined, but candidates include microtubuleflux or chromosome-associated minus end-directedmotors.

Insect spermatocytes have long been a popular system for studying the forces that move and position chromosomes. In cranefly spermatocytes, chromosome arms sometimes become aligned parallelto the spindle long axis during spindle formation, and maintainthis alignment throughout anaphase (Adames and Forer, 1996). Thissuggests that in insect spermatocytes, as in plant mitosis, polewardforces act along the length of the chromosome independent of thoseacting on the kinetochore. To directly test this hypothesis weused laser microsurgery to sever chromosome fragments lackingkinetochores (i.e., acentric fragments) from pole-directed arms.As predicted, these fragments were invariably transported polewardat a velocity (~0.5 µm/min) similar to that exhibited by the kinetochoreregions on anaphase chromosomes. We then investigated the mechanismresponsible for this motion by repeating our experiments on cellstreated with paclitaxel (taxol), a drug that inhibits microtubuleflux (Derry et al., 1995; Waters et al., 1996) but not microtubule-dependentmotor activity (Vale et al., 1985). In taxol, the poleward movementof acentric fragments was dramatically inhibited: <10% of thefragments generated during metaphase exhibited motion, and inthose that did, velocity was greatly attenuated. From these findingswe conclude that the poleward force that acts on the chromosomearms in these spermatocytes is generated by microtubule flux andnot by molecular motors associated with the chromosome. Furthermore,because taxol treatment similarly attenuated the velocity of polewardchromosome motion during anaphase, it also is mediated largelyby flux, as originally suggested by Wilson et al. (1994).

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

Spermatocyte Culture and Drug Treatment

Spermatocytes were obtained from fourth instars of the crane fly, Nephrotoma suturalis, and were prepared for microscopy byrupturing the contents of testes, isolated in tricine insect (TI)buffer (Begg and Ellis, 1979), under oil on the surface of a coverslipattached to a well slide (Janicke and LaFountain, 1986).

Taxol (Sigma, St. Louis, MO) was dissolved in dimethyl sulfoxide (DMSO) at a concentration of 10 mM and stored at $-$ 20°C. Fortreatment of spermatocytes, the above-mentioned stock solutionwas diluted in TI buffer to obtain the desired concentration (100nM-50 µM), and isolated testes were incubated in the various dilutionsfor 15 min to 1 h. During that incubation, taxol was taken upinto the testicular fluid surrounding spermatocytes, as well asby spermatocytes that were suspended in that fluid. The concentrationof taxol in the testicular fluid was not known; however, the effectof taxol on spermatocytes was evident in the taxol phenotype (seeRESULTS) that was achieved. After incubation in taxol-TI buffer,testes were then ruptured under oil for microscopy. Under oil,spermatocytes remained suspended in testicular fluid that containedtaxol. Typically, it took 0.5-2 h after cells were prepared formicroscopy to find a cell suitable for either microsurgery oranalysis of anaphase velocities. Thus, in some cases, resultswere obtained from cells that had spindles before taxol exposure,and they shortened during exposure. In other cells, nuclear envelopebreakdown occurred during exposure to taxol and thus, short spindleswere assembled in the presence of taxol. Microsurgical operationswere performed on both types, and similar results were obtained

Fluorescence and Phase Contrast Microscopy

For analyzing the position of chromosome arms, testes were fixed with 3% paraformaldehyde, stained with Hoechst 33342 (Sigma)according to methods described previously (LaFountain et al.,1999), and then viewed with a Nikon Optiphot equipped with quadfluor optics and a SPOT 1 digital camera (Diagnostic Instruments,Sterling Heights, MI). For analysis of the progression of cellsthrough the first meiotic division after taxol treatment, livingspermatocyte cultures were prepared as described above and monitoredwith a Zeiss IM35 inverted microscope equipped with phase contrastoptics (40×/0.65 numerical apertureobjective).

Polarization Microscopy

Images of spindle birefringence were obtained with a polarization microscope, equipped with a universal compensator (CRI,Woburn, MA) that was constructed and operated as described byOldenbourg and Mei (1995) and then stored as TIFF files that wereimported into Image J for analysis (Image J is public-domain softwarefor image analysis available online from NIH Image http://rsb.info.nih.gov/ij/).For quantitative analysis of the birefringence of spindle microtubules,the magnitude of retardance was determined either 1) within selectedareas of images of half-spindles, nearby chromosome arms; or 2)from line scans that were made on images either parallel or perpendicularto the spindle axis, again within half-spindles in the vicinitiesof chromosome arms. With our system, retardance magnitude is proportionalto the gray scale (brightness) level within the area of interestof a captured image. To quantify retardance, we simply multipliedthe retardance maximum times the fraction of that maximum representedin the area of interest. For example, the line scan in Figure4G passes through three kinetochore bundles, the brightest ofwhich (left-most in the figure) had a brightness level of 201.That brightness corresponds to a retardance of 2.36 nm (201/255× 3 nm), because maximal retardance in this image was 3 nm witha maximum brightness value of 255. Student's t test (MicrosoftExcel) was used to compare retardance data obtained from taxol-treatedand controlcells.

Laser Microsurgery and Video Light Microscopy

All operations were conducted on a custom designed video-LM/laser microsurgery workstation described in detail elsewhere (Coleet al., 1995; Khodjakov et al., 1996). In brief, the 1064-nm outputof a Q-switched, pulsed (5-7 ns at 10 Hz) Nd:YAG laser (Continuum,Santa Clara, CA) was frequency doubled to 532 nm, filtered, attenuated,and then steered into the epi-port of a Nikon Diaphot 200 de Senarmontcompensation Nomarski DIC LM. Each pulse contained ~3 µJ of powerat the entry port of the microscope. Chromosome arms required2-3 s (20-30 laser pulses) to cut and there was no detectableadverse effect of the laser operation on cell viability. In fact,of the 13 spermatocytes monitored after surgery during metaphaseor anaphase of meiosis I, all progressed through interkinesisand completed meiosis II ~3 h afterirradiation.

Digital images were captured on the laser LM workstation with the use of a Micromax charge-coupled device camera (RSP PrincetonInstruments, Trenton, NJ), at 2 frames/min, and the illuminationwas shuttered between framing intervals. Time-lapse sequenceswere processed and stored as TIFF files on the hard drive withthe use of ImagePro software (Media Cybernetics, Silver Springs,MD) running on a PC. They were then imported into Image J formovie making and furtheranalyses.

Velocity Measurements

To determine the velocities of chromosomes and acentric fragments, Image J software was used to measure the distance fromeither the center of chromosome fragment or the leading kinetochoreof a segregating chromosome to a reference point at either thespindle pole or the spindle equator. These distances, obtainedfrom sequential images, were then plotted as a function of timewith the use of Microsoft Excel. Student's t test (Microsoft Excel)was used to compare velocities between control and taxol-treatedcells. The basal bodies of the polar flagella provided a well-definedreference at the spindle pole; when the plane of the spindle equatorwas used as the reference, the positions of chromosomes on themetaphase plate and the shape of the mitochondrial sheath outliningthe spindle provided the basis for defining thatplane.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

Among males of N. suturalis, the karyotype includes three pairs of metacentric autosomes and two small telocentric sex chromosomes(X and Y). The autosomes pair into three bivalents for meiosis;sex chromosome behavior during meiosis is complicated. X and Yinitially pair but then precociously separate into univalentsfor meiosis I; sex chromosomes behave normally as dyads duringmeiosis II. The spindle in spermatocytes is well defined, outlinedby a sheath, or mantle, of aligned mitochondria (LaFountain, 1972).

Chromosome Arms in Crane Fly Spermatocytes Frequently Become Aligned Parallel to Spindle Long Axis

During spindle formation in both primary and secondary spermatocytes, one of the arms of a chromosome sometimes appears toextend along the spindle toward a pole. This is a particularlyprevalent feature of meiosis II, when the arms of the two chromatidscomprising a dyad are no longer coherent (Figure 1A). In a surveyof fixed spermatocytes from eight testes one-third (78/222) ofthe metaphase II cells had one or more pole-directed arms. Althoughconsiderably less common, pole-directed arms are also found amongthe nonchiasmic arms of monochiasmic metaphase I bivalents (Figure2A): of the 277 monochiasmic bivalents in the 247 metaphase Ispermatocytes identified in the above-mentioned survey, 11 (4%)had a pole-directed arm (like that depicted in Figure 2A). Aspreviously noted by others (Adames and Forer, 1996), pole-directedarms seen during metaphase often remain pole-directed during anaphase.

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Figure 1. Chromosome fragments lacking kinetochores are transported poleward. Selected frames from a time-lapse recording of a secondary (meiosis II) spermatocyte in which one of the noncoherent pole-directed arms of a dyad (B, large arrowhead) was severed (B) from the kinetochore region (A, small arrowhead). This operation created a sniglet of denatured material (B-D, large arrow) and an acentric chromosome fragment (B-E, large arrowhead). Note that both the sniglet and the acentric fragment moved poleward, and their velocities were similar to those of the kinetochores during anaphase. Time in minutes:seconds. Bar (in E), 5 µm.

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Figure 2. Chromosome fragments lacking kinetochores are transported poleward. (A-D) Selected frames from a time-lapse recording of a primary (meiosis I) spermatocyte in which a pole-directed arm (A, large arrowhead) was severed (B) from the kinetochore region (A and B, small arrowheads) of a monochiasmic bivalent. This operation created a sniglet (B-D, large arrow) and an acentric chromosome fragment (B-D, large arrowhead). As in metaphase II (Figure 1), both the sniglet and acentric fragment moved poleward (D). Time in minutes:seconds. Bar (in D), 5 µm. (E) Distance from the equator versus time for the acentric fragment ( $open circle$ ) depicted by the arrowhead in B-D, and also for the lower left half-bivalent (

) in D as it moved poleward during anaphase. Note that each moved with a similar kinetic profile.

Acentric Chromosome Fragments Generated Near the Spindle Equator during Metaphase and Anaphase Are Transported Poleward

To test the hypothesis that the extension of a chromosome arm along the interpolar spindle axis in crane fly spermatocytesis due to a poleward force acting along the arms, we severed thearms from metaphase I and II chromosomes between their kinetochoreand telomere regions (Figures 1B and 2B, large arrowheads). Inall cases, the resultant acentric fragment was transported polewardwith a relatively constant and uniform velocity (Figure 2E), averaging~0.5 µm/min (range 0.3-0.7 µm/min; n = 23; Table 1). It shouldbe noted here that the kinetochore regions also moved polewardat a similar constant velocity averaging ~0.5 µm/min during anaphaseI and II (Figure 2E and Table 1).

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Table 1. Comparison of spindle organization, transport velocities, and the duration of meiosis 1 in control and taxol-treated spermatocytes

A thin linear ribbon of highly refractive material is generated in the cutting plane as the specimen is translated slowlythrough the focused laser beam (Figure 1B and 2B). These "sniglets"(Cole et al., 1995) can be formed at will, anywhere within thespindle or cell, and presumably consist of material denaturedby the laser pulses. As chromosome arms were severed, conspicuoussniglets were formed, and these were also always transported polewardwith a velocity similar to that exhibited by the adjacent acentricfragment (Figures 1, C-E, and 2, C and D, arrows; Table 1). Whensniglets were formed by irradiating a region of the half-spindlethat lacked chromosomes, they were also transported poleward witha velocity similar to that exhibited by acentric fragments andanaphase chromosomes (our unpublisheddata).

When acentric chromosome fragments were generated at metaphase in a fully formed spindle, they moved in a linear manner intothe proximal pole (Figures 1, B-E, and 2, C and D). When generatedin early- to mid-prometaphase cells, fragments frequently exhibiteda gradual lateral displacement toward the sheath of mitochondriasurrounding the spindle as they moved poleward (Figure 3). Thus,in addition to experiencing pole-directed forces, during spindleformation the chromosomes are also subjected to forces directedperpendicular to the spindle long axis that tend to eliminatethem laterally from the central domain of the spindle. These so-called"transverse equilibrium forces" were originally described by Östergren(1945), and likely represent the tendency of highly ordered dynamicmicrotubule arrays to sterically eliminate larger inclusions asthey form (see examples in Tucker, 1977).

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Figure 3. As the spindle forms during meiosis I and II, acentric fragments also experience a transverse force that eliminates them to the spindle periphery even as they are moving poleward. (A-D) Mid-prometaphase II cell in which a fragment, originally located near the spindle equator along the pole-to-pole axis (vertical line in B-D), moved laterally toward the spindle periphery as it migrated poleward. (E-H) Similar to A-D, except this fragment (F-H, arrow) was created near the spindle pole during prometaphase I. The fragment was slowly translated laterally toward the spindle periphery, which is outlined by a sheath of mitochondria. Bar (in H), 5 µm.

Taxol Treatment Induces Spindle Shortening, but Does not Prevent Either Anaphase Onset or Poleward Chromosome Motion in Crane Fly Spermatocytes

To investigate the possible contribution made by microtubule flux to the poleward motion of acentric fragments, we treatedtestes with various concentrations of taxol before making spermatocytepreparations (see MATERIALS AND METHODS). Incubating testes in5 or 10 µM taxol for 15 min before making cell preparations producedspermatocytes containing spindles that were ~40% shorter thannormal (Figure 4C and Table 2), and their spindle poles werebroader than normal. This characteristically occurs when spindlesfrom various animal cells are treated with concentrations of taxolgreater than threshold values (Snyder and Mullins, 1993; Waterset al., 1998), and we used it as a criterion when selecting cellsfor the laser microsurgical operations described below.

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Figure 4. Taxol treatment induces the formation of short, broad spindles, but taxol does not inhibit anaphase onset or prevent the subsequent poleward motion of chromosomes. (A-D) Differential interference contrast micrographs of living DMSO (0.05%) control (A and B) and taxol (5 µM for 15 min)-treated (C and D) spermatocytes during meiosis I at metaphase (A and C) and near the completion of anaphase A (B and D). Positions of the basal bodies of the polar flagella are marked with arrowheads in A and C. Note that anaphase takes ~3 times longer in the shortened taxol spindle than in the DMSO control. Another noteworthy point, illustrated in C, is that mitochondria (normally restricted to the periphery of the spindle) often are found within the central domain of spindles formed in taxol. In this case, the mitochondrion appears as a highly refractile rod extending from pole to pole and between two bivalents. Time in minutes:seconds. Bar (in D), 5 µm. (E-H) Images generated with polarization microscopy depicting birefringence (bright contrast) due to spindle microtubules in untreated control (E and G) and taxol-treated (F and H) spermatocytes at metaphase. (E and F) Retardance magnitude was measured within areas 0.55 µm²; kinetochore fiber retardance appears reduced after 5 µM taxol treatment (2.0 vs. 2.35 nm in the control; refer to Table 2 for summary), but nonkinetochore domains appear less affected by taxol (1.5 vs. 1.62 nm in the control). (G and H) Similar results were obtained from line scans made perpendicular to the spindle axis. The top of the line scan in H (10 µM taxol) is on the left of the plot. Bar (in F), 5 µm.

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Table 2. Comparison of retardance magnitude in three spindle domains of control and taxol-treated spermatocytes

The effect of taxol on distribution of microtubules in the spindle was best resolved with polarized light (Figure 4, E-H).For the interpretation of images made with polarized light, white(maximal brightness) represents maximal retardance or birefringence;black represents no retardance or the absence of birefringence.Our images demonstrated that the taxol-induced broadening of thespindle poles correlated with greatly increased numbers and densitiesof microtubules that extended short distances (~2-3 µm) from thepoles toward the equator. Microtubule densities in subpolar andequatorial domains after taxol treatment, however, did not appearto be different from those of controls. Spindle structure in thoseregions was especially important to this study. If taxol treatmenthad greatly altered the distribution of microtubules in thosedomains into which fragments were released after they had beensevered from their chromosomes then any interpretation of fragmentbehavior would have to take those alterations into account. Becausewith the instrumentation we used the retardance magnitude withina given domain of the spindle is directly dependent on its microtubulenumber/density, we were able to quantify microtubules in thosedomains based on their retardance. We quantified retardance twoways: 1) within 0.55-µm² areas that were made within regions of interest (Figure 4, Eand F), and 2) from line scans that were made along planes ofinterest (Figure 4, G and H). Taking those approaches, we foundthat retardance in central spindle domains (in the vicinitiesof chromosomes that could have been cut had we been performingoperations) in taxol-treated spindles was not significantly different(Student's t test, p = 0.19; differences were regarded significantat p < .001) from those in control spindles (Table 2). Our quantitativeanalysis revealed that retardance at spindle poles was clearlyincreased after taxol treatment, and a taxol effect also was manifestedin reduced retardance of kinetochore fibers (Table 2). The lattersuggests there are fewer microtubules per kinetochore in taxol,an effect also apparent from the data presented by Wilson andForer (1997). The cause of this effect of taxol on kinetochorefibers is not known. One of the reviewers raised the possibilitythat the birefringence of kinetochore fibers in taxol is due tofewer than normal associated nonkinetochore microtubules in kinetochorefibers (Wise et al., 1991). Data needed to confirm that, however,will require serial section electron microscopic analysis, suchas that performed on untreated and cold-treated spermatocytesby Scarcello et al. (1986).

A final point regarding taxol effects on spermatocytes is that the doses of taxol that were effective in producing the taxolphenotype did not prevent entry into, or progression through,anaphase. For similar effects on spermatocytes from Drosophila,see Savoian et al. (2000). This was true for both meiosis I andII, but to obtain quantitative data on these points, analysiswas restricted to spermatocytes in meiosis I. In the 83 untreatedcells that we monitored, it took ~83 min on average to reach anaphaseI onset after the breakdown of the nuclear envelope (NEB) at theend of diakinesis (Table 1). Spermatocytes from testes that hadbeen incubated in 5 or 10 µM taxol for 15 min (see MATERIALS ANDMETHODS) progressed through meiosis in taxol, and the durationbetween NEB to anaphase I onset lasted somewhat longer, averaging112 min over a range between 78 and 166 min (Table 1), yet inall 167 cells analyzed, the onset of anaphase was not prevented.In the time between NEB and anaphase, events usually seen in untreatedcells, including congression of autosomes to the equator and metakineticmovements of sex univalents, were also observed in taxol-treatedcells. We analyzed anaphase I in taxol-treated cells and foundthat segregating half-bivalents exhibited very slow (average velocity= 0.1 µm/min; range 0.1-0.3 µm/min; n = 20) poleward motion (Table1). This was true in the cases of spindles that existed beforetaxol exposure and then shortened during exposure, as well asspindles that were assembled in taxol. Because this velocity wassignificantly less (Student's t test, p < .0001) than in untreatedspermatocytes (0.5 µm/min; see above), anaphase A in taxol-shortenedspindles lasted 30-40 min compared with 15 min in the longer spindlesof controls (Figure 4, A-D).

The ultimate outcome of anaphase in the presence of taxol varied. In some cells chromosome poleward motion (anaphase A) wasfollowed by elongation of the previously shortened spindle; thosecells usually initiated, and sometimes completed, cytokinesis.In contrast, in other cells, the spindle poles moved progressivelycloser to one another during anaphase A, and this gradual collapseof the spindle inhibited the initiation of cytokinesis. It isnoteworthy that neither congression nor anaphase was inhibitedeven when testes were incubated in 50 µM taxol for >30 min beforespreading underoil.

Taxol Inhibits Poleward Transport of Acentric Chromosome Fragments during Metaphase

This part of our study was conducted only on meiosis I spermatocytes because, at the concentrations we used, taxol inducedmetaphase II half-spindles to become so short that meaningfulstudies were practically impossible. We found that the transportproperties of meiosis I spindles were clearly and dramaticallyinhibited by taxol (Figure 5, C and D). Of the 24 acentric fragmentsgenerated in 24 prometaphase or metaphase I spermatocytes (Table1), only two exhibited any pole-directed motion and the velocityof that motion (~0.1 µm/min) was greatly attenuated relative tocontrols. In those cells where the fragment exhibited no polewardmotion, it was often slowly but progressively eliminated laterallytoward the spindle periphery (Figure 5). In some cases the fragmentwas still contained within the spindle at anaphase onset and wasobserved to move poleward during anaphase within the interzone,usually trailing behind the segregating half-bivalents (Figure5, E and G). When such poleward motion of fragments was observedduring anaphase in taxol, their velocities, of course, were veryslow (~0.1 µm/min).

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Figure 5. Acentric fragments, generated near the spindle equator in taxol-treated spermatocytes, are not transported poleward as they are in control spermatocytes. (A-H) Selected frames from a time-lapse sequence of a taxol-treated primary spermatocyte that contained a pole-directed achiasmic arm (A-D, arrowhead). After it was severed with the laser (B), this arm remained relatively motionless over the next 47 min until it began to disintegrate before anaphase onset. (E-H) During anaphase, the fragment disintegrated further as it moved poleward (E and G), trailing behind the segregating half-bivalents (F and H), which moved poleward with a velocity of ~ 0.1 µm/min. Time in minutes:seconds. Bar (in D), 5 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

The original goal of our study was to test the hypothesis that spindles in crane fly spermatocytes exert a pole-directed forceon chromosomes independent of kinetochores. To do this we usedlaser microsurgery to sever the arms from metaphase chromosomes,between their kinetochore and telomere regions. We found thatthe resultant acentric fragments invariably moved poleward witha uniform velocity similar to that exhibited by kinetochores duringanaphase. We also found that ribbons or sniglets of denaturedmaterial, generated anywhere within a half-spindle by laser irradiation,also moved poleward with the same kinetics. From these data weconclude that the production of kinetochore-independent, polewardforces is a general feature of crane fly spermatocyte half-spindles.

Poleward Transport of Acentric Fragments Is Mediated by Microtubule Flux

To uncover the mechanism underlying these forces, we treated spermatocytes with taxol before severing chromosome arms. Inso doing, we have developed an indirect assay for microtubuleflux. This approach should be useful on other cell types, forexample, spermatocytes from other insect species or plant endospermcells, which are not amenable to microinjection and thereforeare precluded from direct analysis of flux by photoactivationof fluorescence (Mitchison, 1989) or fluorescent speckle microscopy(Waterman-Storer et al., 1998).

Taxol rapidly inhibits microtubule flux within spindles. It does not affect the activity of microtubule-based motors (Valeet al., 1985), and thus it provided the means for distinguishingbetween possible flux-based and motor-based mechanisms of armfragment transport. At low concentrations taxol preferentiallyinhibits microtubule plus end dynamics in vitro and in vivo, whereasat higher concentrations both plus and minus ends are affected(Jordan et al., 1993; Derry et al., 1995). When vertebrate somaticcells are treated with 10 µM taxol during metaphase, microtubulesubunit incorporation at the kinetochores is inhibited well beforeremoval at the poles (Waters et al. 1996). Because of this differentialinhibition, the kinetochore microtubules shorten as subunits arelost at the poles, and the spindle shortens as the poles holdon to shortening microtubules attached to the chromosomes (Waterset al., 1996; Derry et al., 1998).

We found that the spermatocytes obtained from testes treated with 5 or 10 µM taxol for 15 min contained significantly shortenedspindles characteristic of the taxol phenotype (Table 2; Wilsonand Forer, 1997). When we generated acentric chromosome fragmentsnear the spindle equator in these cells, they failed to move poleward,or they displayed significantly attenuated poleward motion (~0.1µm/min vs. ~0.5 µm/min in controls). The two fragments that exhibitedthis motion were likely generated in spindles in which the effectsof taxol had not yet been fullyreached.

Taxol promotes microtubule assembly (Schiff et al., 1979), and it was possible that an increase in microtubule density withineach half-spindle impeded the poleward motion of acentric fragments.To evaluate this, we used quantitative polarization microscopyto determine the density of microtubules within those areas oftaxol-treated spindles where fragments were released by our cuttingoperations. We found that taxol treatment did not significantlyincrease the density of microtubules in those regions, althoughit did enhance microtubule density near the spindlepoles.

From these results, we conclude that the force for transporting acentric chromosome fragments and the other material polewardin crane fly spermatocytes is produced by microtubule flux. Chromosomearms must simply become trapped by the dense arrays of microtubulesin the half-spindle (LaFountain 1974, 1976; Scarcello et al.,1986) and then are directed poleward as their surfaces interactwith fluxing microtubules. This conclusion provides a ready explanationfor why areas of reduced birefringence, created on crane fly spermatocytekinetochore fibers by UV irradiation, move poleward (Forer, 1966).It also reveals that the transport properties of crane fly spermtocytespindles are similar to metaphase spindles in plant endosperm(Khodjakov et al., 1996) but differ from those of animal somaticcells in which a polar wind is generated by microtubule plus end-directedmotors associated with chromosome arms (Rieder and Salmon, 1994).

During Anaphase, Kinetochore Microtubules Depolymerize at Their Minus Ends

Our assay reveals that acentric chromosome fragments also moved poleward during anaphase with the same velocities exhibitedby chromosomes (~0.5 µm/min). Because the rate of flux duringmetaphase is similar to the rate of chromosomes during anaphase,a flux-based mechanism, involving shortening of kinetochore microtubulesat their minus ends, is implicated for anaphase. Thus, our dataindependently confirm the conclusion of Wilson et al. (1994).By taking advantage of the fact that kinetochore microtubulesin crane fly spermatocytes are acetylated, except for an unacetylated"gap" near kinetochores (Wilson and Forer, 1989), they were ableto show that at least 80% of the shortening of kinetochore fibersduring anaphase is due to subunit removal at thepole.

Although the rate at which kinetochores move poleward during anaphase in taxol-treated spermatocytes is reduced by 80% (from0.5 µm/min to only ~0.1 µm/min), the chromosomes invariably completedthis migration. Why and how this occurs is unclear. It is possiblethat our taxol treatment did not eliminate flux. That is, it didnot completely inhibit the incorporation of microtubule subunitsat kinetochores and their removal at the poles. However, our observationthat the majority of acentric fragments generated in metaphasecells failed to exhibit poleward motion suggests that in mostcases flux is shut down completely by the time of anaphase onset.The idea that subunit incorporation into kinetochore microtubulesis inhibited, but that some residual removal at the pole continues,is not consistent with our finding that taxol-treated spindlesreached an equilibrium length after which they no longer shortened.In their study on the sites of microtubule disassembly duringanaphase in crane fly spermatocytes, Wilson et al. (1994) concludedthat although 80% of kinetochore fiber shortening occurs by subunitremoval at the pole, 20% can be attributed to subunit removalat the kinetochore. Thus, it is possible that the stability ofkinetochore microtubule plus ends is suddenly modified at anaphaseonset in taxol-treated cells by, for example, the rapid inactivationof the CDK1 kinase, which then allows them to shorten by subunitremoval at thekinetochore.

Our conclusion that anaphase chromosome motion in crane fly spermatocytes is driven primarily by flux differs from Nicklas'(1989) finding that in grasshopper spermatocytes the force forpoleward chromosome motion during anaphase is generated at ornear the kinetochores and that during this motion microtubulesshorten primarily by subunit removal at kinetochores. Recent workon zw10 and rod mutants also suggests that the force for anaphasemotion in Drosophila spermatocytes is generated primarily at thekinetochore (Savoian et al., 2000; Sharp et al., 2000). Together,these studies imply that the relative contribution that each (redundant)force-producing mechanism contributes to moving chromosomes polewardduring meiosis in insect spermatocytes varies betweenorganisms.

	CONCLUSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION CONCLUSION REFERENCES

Our findings add to the growing body of evidence in support of the conclusion that both kinetochore-based and flux-based mechanismsexist and that the mechanism that is emphasized depends on theparticular system. Although flux is a contributor in animal somaticcells, forces produced by kinetochore-associated motors, or disassemblingmicrotubule plus ends, appear to dominate (Mitchison and Salmon,1992; Zhai et al., 1995). Here we show that each of the two opposinghalf-spindles in crane fly spermatocytes are "flux machines" thattransport kinetochores, acentric chromosome fragments, and otherinclusions poleward as they adhere to the surfaces or plus endsof microtubules. These spindles are therefore similar to thoseformed in Xenopus oocyte extracts (Murray et al., 1996; Desaiet al., 1998) in that the force for poleward chromosome motionis also produced by microtubule flux as kinetochore microtubulesshorten by subunit removal at thepole.

In such flux machines, "slippage" must occur between the plus ends of kinetochore microtubules and the kinetochores duringmetaphase, when poleward motion is prevented by the cohesion ofhomologs (or sister chromatids). As the machine continues to flux,this slippage, which in vertebrate somatic cells produces a "neutral"kinetochore state (Khodjakov and Rieder, 1996), could still maintainthe tension on the kinetochores needed to stabilize attachmentto the spindle (Nicklas, 1997). Then, when the chromosomes disjoinat anaphase onset, the sudden decrease in tension could releasethe clutch on the opposing kinetochores, engage the gears (i.e.,stop slippage), and allow the force produced by flux to move thechromosomepoleward.

Although the molecular basis for flux is unknown, it has been proposed that microtubule plus end-directed motors, anchoredwithin the spindle matrix, could push the microtubule latticetoward the spindle pole (Sawin and Mitchison, 1991). An actin/myosinsystem located within the kinetochore fiber and spindle matrixcould act in a similar manner (Waterman-Storer and Salmon, 1997;Silverman-Gavrila and Forer, 2000). Regardless of the mechanism,the flux-mediated production of forces for kinetochore polewardmotion is compatible with traction fiber models (reviewed by Haysand Salmon, 1990) for chromosome positioning. In this view chromosomesbecome aligned on the spindle equator because the opposing poleward"pulling" forces, acting on sister kinetochores, are proportionalto the length of the kinetochore fibers. Challenges for the futurewill be to determine whether chromosome congression in flux machinesis indeed mediated by traction fibers and how poleward forcesthat act on the chromosome arm influence thisprocess.

	ACKNOWLEDGMENTS

We gratefully acknowledge the contributions made to this study by A. Khodjakov, G. Rickards, S. Inoué, K. LaFountain, D.LaFountain, and A. Siegel. We also thank the reviewers who recommendedrevisions that improved the final version of this report. Thisresearch was supported by grants from the National Science Foundation(MCB-9808290 to J.L.) and National Institutes of Health (GM-40198to C.R. and GM-49210 to R.O). Much of the work was completed inthe Video LM Core Facility of the WadsworthCenter.

	FOOTNOTES

Online version of this article contains video material for certain figures. Online version available at www.molbiolcell.org.

Corresponding author: E-mail address: jrl{at}acsu.buffalo.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
CONCLUSION
REFERENCES

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This Article

Abstract

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				G. C. Rogers, S. L. Rogers, and D. J. Sharp Spindle microtubules in flux J. Cell Sci., March 15, 2005; 118(6): 1105 - 1116. [Abstract] [Full Text] [PDF]

				J. R. LaFountain Jr. and R. Oldenbourg Maloriented Bivalents Have Metaphase Positions at the Spindle Equator with More Kinetochore Microtubules to One Pole than to the Other Mol. Biol. Cell, December 1, 2004; 15(12): 5346 - 5355. [Abstract] [Full Text] [PDF]

				J. R. LaFountain Jr., C. S. Cohan, A. J. Siegel, and D. J. LaFountain Direct Visualization of Microtubule Flux during Metaphase and Anaphase in Crane-Fly Spermatocytes Mol. Biol. Cell, December 1, 2004; 15(12): 5724 - 5732. [Abstract] [Full Text] [PDF]

				H. Maiato, J. DeLuca, E. D. Salmon, and W. C. Earnshaw The dynamic kinetochore-microtubule interface J. Cell Sci., November 1, 2004; 117(23): 5461 - 5477. [Abstract] [Full Text] [PDF]

				A. A. Levesque, L. Howard, M. B. Gordon, and D. A. Compton A Functional Relationship between NuMA and Kid Is Involved in Both Spindle Organization and Chromosome Alignment in Vertebrate Cells Mol. Biol. Cell, September 1, 2003; 14(9): 3541 - 3552. [Abstract] [Full Text] [PDF]

				I. Brust-Mascher and J. M. Scholey Microtubule Flux and Sliding in Mitotic Spindles of Drosophila Embryos Mol. Biol. Cell, November 1, 2002; 13(11): 3967 - 3975. [Abstract] [Full Text] [PDF]

				J. R. LaFountain Jr, R. W. Cole, and C. L. Rieder Partner telomeres during anaphase in crane-fly spermatocytes are connected by an elastic tether that exerts a backward force and resists poleward motion J. Cell Sci., January 4, 2002; 115(7): 1541 - 1549. [Abstract] [Full Text] [PDF]