The Nup107-160 Nucleoporin Complex Is Required for Correct Bipolar Spindle Assembly

Arturo V. Orjalo^*, Alexei Arnaoutov, Zhouxin Shen^*, Yekaterina Boyarchuk, Samantha G. Zeitlin, Beatriz Fontoura, Steven Briggs^*, Mary Dasso, and Douglass J. Forbes^*

Sections of *Cell and Developmental Biology and Molecular Biology, Division of Biological Sciences, University of California-San Diego Medical School, La Jolla, CA 92093-0347; Laboratory of Gene Regulation and Development, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, MD 20892-5431; and Department of Cell Biology, University of Texas Southwestern Medical Center, Dallas, TX 75390-9039

Submitted November 18, 2005; Revised June 9, 2006; Accepted June 19, 2006
Monitoring Editor: Karsten Weis

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The Nup107-160 complex is a critical subunit of the nuclearpore. This complex localizes to kinetochores in mitotic mammaliancells, where its function is unknown. To examine Nup107-160complex recruitment to kinetochores, we stained human cellswith antisera to four complex components. Each antibody stainednot only kinetochores but also prometaphase spindle poles andproximal spindle fibers, mirroring the dual prometaphase localizationof the spindle checkpoint proteins Mad1, Mad2, Bub3, and Cdc20.Indeed, expanded crescents of the Nup107-160 complex encircledunattached kinetochores, similar to the hyperaccumulation observedof dynamic outer kinetochore checkpoint proteins and motorsat unattached kinetochores. In mitotic Xenopus egg extracts,the Nup107-160 complex localized throughout reconstituted spindles.When the Nup107-160 complex was depleted from extracts, thespindle checkpoint remained intact, but spindle assembly wasrendered strikingly defective. Microtubule nucleation aroundsperm centrosomes seemed normal, but the microtubules quicklydisassembled, leaving largely unattached sperm chromatin. Notably,Ran-GTP caused normal assembly of microtubule asters in depletedextracts, indicating that this defect was upstream of Ran orindependent of it. We conclude that the Nup107-160 complex isdynamic in mitosis and that it promotes spindle assembly ina manner that is distinct from its functions at interphase nuclearpores.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Communication between the nucleus and cytoplasm occurs throughthe nuclear pore complex (NPC; reviewed in Vasu and Forbes,2001; Suntharalingam and Wente, 2003; Hetzer et al., 2005).At mitosis the metazoan nuclear pore disassembles into approximatelya dozen subunits. The major subunit, both in size and complexity,is the nine-protein vertebrate Nup107-160 complex, which includesNup160, Nup133, Nup107, Nup96, Nup85, Nup43, Nup37, Sec13, andSeh1 (Belgareh et al., 2001; Vasu et al., 2001; Cronshaw etal., 2002; Harel et al., 2003b; Devos et al., 2004; Loiodiceet al., 2004). In yeast, a nearly identical complex exists (Siniossoglouet al., 1996, 2000; Teixeira et al., 1997; Lutzmann et al.,2002), lacking only the vertebrate Nup43 and Nup37 subunitsfor which there are no yeast counterparts.

Nuclear reconstitution in interphase Xenopus egg extracts depletedof the Nup107-160 complex produced nuclear envelopes with enclosedmembranes, but completely devoid of nuclear pores (Harel etal., 2003b; Walther et al., 2003a). These studies suggest thatthe Nup107-160 complex is a central and early determinant inNPC assembly. Genetic studies in yeast indicate the complexplays a critical role in mRNA export (Doye et al., 1994; Heathet al., 1995; Li et al., 1995; Pemberton et al., 1995; Goldsteinet al., 1996; Siniossoglou et al., 1996). In human cells, RNAinterference (RNAi) and transfection of dominant-negative fragmentsof individual complex members have revealed that vertebratemRNA export is similarly dependent upon this complex (Vasu etal., 2001; Boehmer et al., 2003; Harel et al., 2003b; Waltheret al., 2003a).

The Nup107-160 complex has been localized at kinetochores inmammalian cells during mitosis (Belgareh et al., 2001; Harelet al., 2003b; Loiodice et al., 2004), and one of its constituents,Nup96, has also been found at the spindles and spindle poles(Enninga et al., 2003). These studies used different antibodiesand experimental conditions. However, the function of this complexin these sites was not established. Deletion mutants in eitherSaccharomyces cerevisiae or Schizosaccharomyces pombe lackingthe homologues of vertebrate Nup160, show significant defectsin mitotic spindles (Aitchison et al., 1995; Bai et al., 2004).The mechanism through which the Nup107-160 complex may contributetoward spindle assembly is currently unknown.

Notably, other nucleoporins and transport factors also playa role in spindle assembly. The mammalian nucleoporin Nup358(also called RanBP2) is a component of the cytoplasmic filamentsof the interphase NPC (Vasu and Forbes, 2001; Suntharalingamand Wente, 2003). It is targeted to mitotic kinetochores withits binding partner, RanGAP1 (Joseph et al., 2002, 2004; Salinaet al., 2003). RNAi-mediated depletion of Nup358 induces mitoticarrest with defective spindles (Salina et al., 2003; Josephet al., 2004). Moreover, disruption of its targeting to kinetochorescauses defects in the microtubule fibers connecting kinetochoresto spindle poles (Arnaoutov et al., 2005). Additionally, themRNA transport factor Rae1 is associated with microtubules ininterphase HeLa cells and neurons (Kraemer et al., 2001). Duringmitosis, Rae1 localizes to the mitotic spindle, with enrichmentat the spindle poles (Blower et al., 2005). In Xenopus mitoticextracts, Rae1 binds to the spindle in an RNA-containing complex,whose depletion disrupts microtubule nucleation and aster formation,among the earliest steps in spindle assembly (Blower et al.,2005). Rae1 has also been implicated in both S. pombe and vertebratecells as a regulator of mitotic cell cycle progression (Whalenet al., 1997; Jeganathan et al., 2005). The extent to whichother NPC-associated proteins may be involved in spindle assemblyand function is an important question for future investigation.

Interestingly, some kinetochore proteins show a reciprocal localization:the Mad1, Mad2, and Mps1 proteins act at kinetochores duringmitosis, as part of the spindle checkpoint pathway that preventspremature anaphase onset until all chromosomes are attachedto the spindle and aligned on the metaphase plate. During interphase,however, these proteins associate with yeast and vertebratenuclear pores (Campbell et al., 2001; Iouk et al., 2002; Liuet al., 2003; Stukenberg and Macara, 2003). In budding yeast,there is evidence that nuclear pore association of Mad1 andMad2 is linked to the spindle checkpoint (Iouk et al., 2002),but not essential for checkpoint activation (Kastenmayer etal., 2005). This association seems to be controlled by the smallGTPase Ran in both yeast and vertebrate cells (Quimby et al.,2005).

Indeed, Ran may be a functional connector between many of theseevents. A chromatin-bound Ran-GEF (RCC1) produces Ran-GTP, whichplays a critical role in directing spindle assembly around chromosomesduring mitosis (Carazo-Salas et al., 1999; Kalab et al., 1999;Ohba et al., 1999; Wilde and Zheng, 1999; Zhang et al., 1999).Elevation of Ran-GTP levels in mitotic Xenopus egg extractscauses the assembly of microtubules in a chromosome-independentmanner, which in turn become rearranged over time into structuresresembling spindles. It is widely believed this effect resultsfrom the capacity of Ran-GTP to release inhibitory interactionsbetween mitotic spindle assembly factors and transport receptors(Gruss et al., 2001; Nachury et al., 2001; Wiese et al., 2001;Trieselmann et al., 2003; Tsai et al., 2003; Ems-McClung etal., 2004). Under normal circumstances, this function mightbe limited to the immediate vicinity of chromosomes due to therestricted localization of RCC1 (Askjaer et al., 2002; Kalabet al., 2002; Trieselmann and Wilde, 2002; Li and Zheng, 2004;Caudron et al., 2005; reviewed in Harel and Forbes, 2004; Clarke,2005). Ran-GTP also plays crucial roles in the spindle checkpoint(Arnaoutov and Dasso, 2003), centrosomal function (Di Fioreet al., 2003; Keryer et al., 2003; Di Fiore et al., 2004), postmitoticnuclear assembly (Zhang et al., 1999; Hetzer et al., 2000; Zhangand Clarke, 2000, 2001; Bamba et al., 2002; Hetzer et al., 2002;Harel et al., 2003a; Walther et al., 2003b), and interphasenuclear transport (Macara, 2001). It may well be that evolutionhas sought the most parsimonious option, using the dual localizationof nucleoporins and spindle checkpoint proteins, which are foundat pores and kinetochores, because both are subject to Ran control.

In the present study, we have investigated the mitotic roleof the Nup107-160 nucleoporin complex. Immunofluorescence inmammalian cells and Xenopus egg mitotic extracts revealed thatthe Nup107-160 complex, in addition to localizing to kinetochores,localizes to the spindle poles and within the spindle. Nup107-160complex behavior in mammalian cells strikingly resembled thebehavior of a subset of spindle checkpoint proteins, as didthe accumulation of the Nup107-160 complex at unattached kinetochores.Although the complex did not seem to be essential for spindlecheckpoint signaling, the Nup107-160 complex was essential formitotic spindle assembly in vitro. These findings clearly indicatethat the Nup107-160 complex is highly dynamic during mitosisand that it has mitotic functions that are distinct from itsinterphase roles in NPC structure and nucleocytoplasmic trafficking.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Constructs, Immunoprecipitation, and Antibodies
A full-length cDNA encoding 375 aa of Xenopus Nup43 was preparedusing reverse transcription of XL177 total RNA. The oligonucleotidesused in the PCR amplification were derived using the extreme5' and 3' aa sequences of the GenBank Xenopus clones (GenBank/EMBL/DDBJaccession nos. BX843375 and BG016768). After the cDNA was clonedinto pET-28a, the recombinant protein was expressed in Escherichiacoli Rosetta (DE3), purified on Ni-NTA agarose (QIAGEN, Valencia,CA), and used to immunize a rabbit. Antibodies were affinitypurified against the same xNup43 protein coupled to CNBr-activatedSepharose (GE Healthcare, Little Chalfont, Buckinghamshire,United Kingdom).

A cDNA encoding of Xenopus Nup37 (aa 1–267) was reversetranscription-PCR cloned using 5' and 3' oligonucleotides derivedfrom GenBank/EMBL/DDBJ accession no. CA788183 and total XL177RNA. The cDNA was amplified by PCR, cloned into pET-28a, andexpressed. Antibodies were raised and affinity purified againstthe same Xenopus protein.

Expression of RanQ69L from pET-28a in E. coli Rosetta (DE3)was induced by the addition of 1 mM isopropyl- $beta$ -D-thiogalactopyranosidefor 5 h at 37°C. The cells were lysed by sonication, andthe protein was purified on Ni-NTA agarose. The eluted fractionscontaining RanQ69L were then dialyzed into phosphate-bufferedsaline (PBS) overnight at 4°C, concentrated using an AmiconUltra-4 centrifugal filter device (Millipore, Billerica, MA),and loaded with GTP as described previously (Kutay et al., 1997).RanQ69L loaded with GTP was finally dialyzed into PBS/5% glycerolfor 4 h and concentrated further using an Ultrafree-0.5 centrifugalfilter device (Millipore).

Immunoprecipitation was done using Xenopus egg cytosol preparedas described previously (Shah et al., 1998). Affinity-purifiedIgG against hNup133 and xNup43 or nonimmune rabbit IgG (5 µg;Calbiochem/EMD Biosciences, San Diego, CA) were coupled to 20µl of nProtein A-Sepharose (GE Healthcare). The beadswere incubated in egg extract (20 µl) added to 500 µlof PBS (2 h; 4°C), washed three times in PBS, eluted with0.1 M glycine, pH 2.5 (20 µl), and neutralized with 0.1volume of 1.0 M Tris, pH 8.0. Samples (5 µl) were loaded,resolved by SDS-PAGE, and immunoblotted.

Antibodies against the following proteins were used: rabbitpolyclonal antibodies against Bub1, BubR1, and Mad2 (kindlyprovided by R. H. Chen, Institute of Molecular Biology, AcademiaSinica, Taipei, Taiwan), monoclonal antibodies against humanCENP-B (kindly provided by D. Cleveland, Ludwig Institute forCancer Research, University of California-San Diego) and humanNup62 (BD Transduction Laboratories, Lexington, KY), and rabbitpolyclonal antibodies against Xenopus NuMA (kindly providedby D. Cleveland), hNup160, mNup85, hNup133 (Harel et al., 2003a),and human Nup96 (Fontoura et al., 1999).

Preparation of Mitotic Extracts for Spindle Assembly, Immunodepletion, and Antibody Addition
Frogs for mitotic (i.e., cytostatic factor [CSF] arrested) extractpreparation were primed with 100 U of pregnant mare serum gonadotropin(Calbiochem) and placed in water containing 2 g/l NaCl for atleast 48 h. Sixteen to 18 h before extract preparation, theprimed frogs were induced to ovulate with 500 U of human chorionicgonadotropin (Sigma-Aldrich, St. Louis, MO) and put into individualbuckets containing modified Ringer’s solution (MMR). Theylaid their eggs overnight at 16°C, which were then collectedin 250-ml beakers the next morning. After removing most of theMMR from the good batches of eggs, a 2% cysteine solution wasadded for dejellying. Eggs that seemed activated were constantlyremoved by a transfer pipette (Fisher Scientific, Pittsburgh,PA). The dejellied eggs were then washed three or four timeswith CSF-XB (Desai et al., 1999). Using a cut-tip transfer pipette,the eggs were drawn up and slowly dropped into a 14-ml polypropyleneround-bottomed tube (BD Biosciences Discovery Labware, Bedford,MA) containing 1 ml CSF-XB + aprotinin/leupeptin and cytochalasinB. After the excess buffer was removed from the top of the eggs,the tubes were spun for 20 s at setting 4 in a clinical centrifugeand then 15 s at setting 6. Buffer from the top of the eggswas gently removed, and the tubes were spun in the HB-6 rotorin the ultracentrifuge at 10,000 rpm for 15 min at 16°C.The cytoplasmic layer was removed with an 18-guage needle ona 3-ml syringe and gently drawn out. The needle was then removedand the extract transferred to a 14-ml polypropylene round-bottomedtube on ice. Finally, additional aprotinin/leupeptin and cytochalasinB was added as well an ATP energy mix.

Where indicated, rhodamine-labeled tubulin was added at a finalconcentration of 25 µg/ml. Checkpoint extracts were preparedby incubation with 20 µg/ml nocodazole for 40 min. Ranasters were generated by the addition of RanQ69L to extractsat a concentration of 25 µM. When used, sperm nuclei wereadded at a final concentration of 500 nuclei/µl.

For immunodepletion, a combined 400 µg of affinity-purifiedantibodies against hNup133 and xNup43 or an equal amount ofnonimmune rabbit IgG were bound to 60 µl of nProtein A-Sepharoseovernight. The bound antibody beads were blocked with 20 mg/mlbovine serum albumin in PBS buffer and washed twice with PBSand three times with CSF-XB. CSF-arrested extract (100 µl)was added to 30 µl of antibody or rabbit IgG beads andtumbled for 30 min (23°C) for two consecutive depletions.For the analysis of Ran asters and spindles in mock and depletedextracts, 20-µl reactions were fixed and spun onto coverslipsas described previously (Desai et al., 1999).

A different protocol was used to analyze mitotic chromatin withoutpreserving the spindles. Twenty microliters of each reactionwas first diluted fivefold with 0.8x CSF-XB containing 250 mMsucrose and then mixed with 1 ml of fixation buffer (0.8x CSF-XB,250 mM sucrose, 4% paraformaldehyde) for 30 min at room temperature.The reactions were then layered onto a 40% glycerol cushionin 0.8x CSF-XB + 0.1% Triton X-100 and pelleted onto coverslipsfor 10 min at 18°C at 6000 x g. They were then processedfor immunofluorescence as described previously (Harel et al.,2003a). Cycling extracts were prepared as described previously(Desai et al., 1999).

For antibody addition experiments, sperm chromatin was firstadded to CSF extracts, which had been induced to enter interphaseby the addition calcium chloride (0.4 mM final). The chromatinpackages then formed nuclear structures. These extracts containingnuclei were then reconverted to mitosis by the addition of anequal volume of fresh CSF mitotic extract. This extract containedeither affinity-purified anti-Nup133 or -Nup43 antibodies ornonimmune rabbit IgG. The antibody concentration in the finalreactions was 1 mg/ml. To quantitate the relative density ofmicrotubules in the resultant spindles, images were acquiredusing a 63x objective and analyzed using Imaris imaging software(Bitplane, St. Paul, MN). The z-axis stacks of fluorescent images,corresponding to slices along the long axis of the spindle,were examined visually to determine the medial plane of thespindle, where microtubule density would be greatest. Withinthe appropriate stack, a 100 x 100 pixel region was chosen roughlyhalfway between the chromosomes and spindle poles. The fluorescencewithin this region was integrated. Background was determinedby measuring a corresponding 100 x 100 pixel region in an adjoiningarea of the same field lacking microtubules or chromatin. Thebackground was subtracted to provide the final measurement offluorescence intensity provided in Supplemental Table 3.

For assessing the chromatin recruitment of checkpoint proteinsunder spindle checkpoint conditions and the sensitivity of thisto RCC1/RanGEF, experiments were performed as described previously(Arnaoutov and Dasso, 2003).

Cell Culture and Immunofluorescence
HeLa cells were grown in DMEM supplemented with 10% fetal calfserum. In Figure 2, HeLa cells were first permeabilized forimmunofluorescence with PHEM buffer (60 mM PIPES, 20 mM HEPES,pH 6.9, 10 mM EGTA, 4 mM MgSO₄, 0.1% Triton X-100) for 5 minand then fixed with –20°C methanol for 10 min. Thecells were then processed for immunofluorescence as describedpreviously (Harel et al., 2003a) with the appropriate primaryand secondary antibodies. Coverslips were mounted with VECTASHIELD(Vector Laboratories, Burlingame, CA), and visualized with aZeiss Axioskop fluorescence microscope (Carl Zeiss, Thornwood,NY).

Images collection for Figure 4 was performed at the Universityof California-San Diego Cancer Facility in the laboratory ofDr. James Feramisco on a Deltavision deconvolution microscope(Applied Precision, Issaquah, WA).

Mass Spectroscopy Analysis of Mitotic and Interphase Nup107-160 Complex
To study the composition of the Nup107-160 complex in interphaseand mitotic Xenopus extract, the complex was immunoprecipitatedwith anti-hNup133 or anti-xNup43 antibodies as follows: affinity-purifiedantibodies (5 µg) or nonimmune rabbit IgG (5 µg;Calbiochem/EMD Biosciences) were covalently coupled to 20 µlof nProtein A-Sepharose (GE Healthcare) with dimethyl pimelimidate.Each set of antibody beads was incubated with mitotic CSF eggextract (20 µl in 500 µl of CSF-XB buffer) or theidentical extract converted to interphase by addition of calciumchloride and incubation for 1 h at room temperature (20 µlin 500 µl of CSF-XB buffer). The six immunoprecipitationreactions were incubated for 1 h at 23°C, washed three timesin CSF-XB buffer, and bound proteins eluted with 0.1 M glycine,pH 2.5 (20 µl). The mixtures were neutralized with 0.1volumes of 1.0 M Tris, pH 8.0. The immunoprecipitated proteinswere reduced and alkylated using 2 mM tris(2-carboxyethyl)phosphine(AC36383; Fisher Scientific) at 37°C for 30 min and 5 mMiodoacetamide (AC12227; Fisher Scientific) at 37°C in darkfor 30 min, respectively. The proteins were digested with 0.5mg of trypsin (03 708 969 001; Roche Diagnostics, Indianapolis,IN) overnight.

A reverse phase gradient from 0 to 80% acetonitrile at 300 nl/minflow rate was used to elute the peptides from a self-packedC18 capillary column (20 cm long x 100 mM i.d.) by using anAgilent 1100 quaternary high-performance liquid chromatographypump (Agilent Technologies, Palo Alto, CA). Eluted peptideswere directly analyzed by a Thermo Electron (Waltham, MA) LTQion trap mass spectrometer. About 20,000 tandem mass spectrometry(MS/MS) spectra were collected for each sample.

The raw data were extracted and searched using Spectrum Mill(version A.03.01.037a SR1; Agilent Technologies). MS/MS spectrawith a sequence tag length of 1 or more were searched againstthe National Center for Biotechnology Information (NCBI, Bethesda,MD) dbEST database (version 7/12/2005) limited to Xenopus taxonomy(1,344,320 expressed sequence tag [EST] sequences). The enzymeparameter was limited to full tryptic peptides with a maximummiscleavage of 2. All other search parameters were set to SpectrumMill’sdefault settings. Search results for individual spectra wereautomatically validated using the following filtering criteria:1) protein details mode: score >9 for 1+ and 2+ peptidesand score >11 for 3+ peptides; and 2) peptide mode: score>11 for 1+, >12 for 2+ and score >13 for 3+ peptides.The false-positive rate for such criteria was estimated by searchingthe same data set against a combined forward-reverse databaseof NCBI nonredundant protein database limited to human, fish,and reptile taxonomies. Among the autovalidated 97 proteinsand 314 peptides, two proteins were from the reverse sequencedatabase. And both of them are single-peptide hits. Thus, thefalse-positive rate of our filtering criteria is 1% spectraand 4% protein. Only proteins with at least two unique peptideswere selected for comparative analysis between different samples.

Quantitation of Kinetochore Staining with Anti-Nup133 Antibodies
Measurements of kinetochore fluorescence in Supplemental Table2 were obtained as described previously (Hoffman et al., 2001),by using Imaris imaging software. Images were acquired usinga 63x objective and analyzed without deconvolution. The bestin-focus images of individual kinetochore were determined bystepping through the z-axis stacks of corresponding fluorescenceimages visually. Computer-generated 9 x 9 and 13 x 13 pixelregions were centered over each kinetochore. The former regioncorresponded was typically large enough to contain essentiallyall kinetochore fluorescence. The outer region was chosen tobe more than double the area of the inner region but to excludesignificant fluorescence from adjacent kinetochores. The backgroundcomponent of the 9 x 9 pixel region was determined by subtractingthe integrated value of that region from the larger 13 x 13pixel region. The resulting measurement was scaled in proportionto the area of the 9 x 9 pixel region. The scaled measurementwas subtracted from the integrated value of the 9 x 9 pixelregion, to yield the final value for kinetochore fluorescence.Average values of kinetochore fluorescence were calculated from20 kinetochores for each experimental condition.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The Xenopus Nup107-160 Complex Contains New Members Nup43 and Nup37
The human Nup107-160 complex contains nine members, includingtwo recently identified members that have not been describedpreviously in Xenopus, Nup43 and Nup37 (Belgareh et al., 1998;Vasu et al., 2001; Cronshaw et al., 2002; Harel et al., 2003b;Loiodice et al., 2004). To better use the powerful biochemistryof the Xenopus egg extract system for investigation of Nup107-160complex function, we cloned and raised antibodies to Xenopusand human Nup43 and Nup37 (Figure 1, A–C; see Materialsand Methods). We found that the Xenopus Nup107-160 complex ineggs contains these proteins. Anti-xNup43 and anti-hNup133 antiseraeach coimmunoprecipitate Nup160, Nup133, Nup85, Sec13, Nup43,and Nup37 (Figure 1, E and F). Furthermore, mass spectroscopyanalysis of Nup43 and Nup133 immunoprecipitates indicate thatall nine Nup107-160 complex members are present (SupplementalTable 1).

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Figure 1. xNup43 and xNup37 are components of the Xenopus Nup107-160 complex. (A) An antibody raised to amino acids 1–375 of Xenopus Nup43 recognizes two bands in Xenopus interphase extract. The lower band is Nup43, and the higher band labeled with the asterisk is a cross-reacting protein. (B) An antibody raised to amino acids 1–267 of Xenopus Nup37 recognizes two bands in Xenopus interphase extract. The higher band is Nup37, and the lower band labeled with the asterisk is a cross-reacting protein. (C) Immunofluorescence on interphase XL177 Xenopus cells was performed with anti-xNup37 antibody (left), which localizes in a punctate pattern on the nuclear rim, characteristic of a nuclear pore stain. Right, DNA stained with 4,6-diamidino-2-phenylindole (DAPI). Bar, 10 µm. (D) Schematic of the nine-member Xenopus Nup107-160 complex is shown. Because the nearest neighbors of Nup43 and Nup37 are unknown, they are placed arbitrarily in the subcomplex. (E) Nup37 and Nup43 are members of the Xenopus Nup107-160 nuclear pore subcomplex. Anti-Nup43 antibody immunoprecipitates Nup43 as well as the other members of the Nup107-160 complex, including Nup160, Nup133, and Nup37, from interphase extract (lane 3). Note that the cross-reacting band indicated by the asterisk does not coimmunoprecipitate with the Nup107-160 complex. (F) Anti-Nup133 antibody reciprocally immunoprecipitates Nup43 as well as other complex members, such as Nup160 and Nup37.

We conclude that, as in mammals, the Xenopus Nup107-160 complex,shown in Figure 1D, contains nine proteins: Nup160, Nup133,Nup107, Nup96, Nup85, Sec13, Seh1, Nup43, and Nup37. Interestingly,we see no major differences in the subunits immunoprecipitatedfrom interphase or mitotic Xenopus extracts (Supplemental Table1), suggesting that this represents a constitutive pore subcomplexthat is present throughout the cell cycle.

The mammalian Nup107-160 Complex Localizes to Prometaphase Spindles and Spindle Poles
Previous analysis observed that a small fraction of the Nup107-160complex ( $~$ 5%) localizes to kinetochores during mitosis (Belgarehet al., 2001; Harel et al., 2003b; Loiodice et al., 2004). Inthese studies, however, distribution of the remaining Nup107-160complex throughout the mitotic cell effectively obscured otherpotential sites of localization. To reveal additional sitesof localization, we performed immunofluorescence on mitoticHeLa cells, using a protocol designed to release soluble Nup107-160complexes. As expected, the Nup107-160 complex was present onkinetochores at all stages of mitosis (Figure 2A, left). However,immunofluorescence in the absence of soluble cytoplasmic proteinsalso showed clear localization of Nup133 to the spindle polesand proximal spindle microtubules (Figure 2A). Polar localizationwas similarly observed using antibodies against other Nup107-160complex members, including Nup85 (Figure 2B), Nup96 (Figure 2C),and Nup160 (Figure 2C). Antisera directed against nucleoporinsthat are not members of the Nup107-160 complex, i.e., Nup93and Nup62, did not stain kinetochores or spindles at any stageof mitosis (Figure 2C).

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Figure 2. The Nup107-160 complex localizes to kinetochores, spindle poles, and microtubules during prometaphase. (A and B) HeLa cells were prepared for immunofluorescence as described in Materials and Methods and stained with affinity-purified anti-hNup133 (red, A), affinity-purified anti-mNup85 (red, B), or an anti-hCENP-B monoclonal antibody (mAb) (green, A and B). A merge is shown in the right panels (A and B). Whereas CENP-B and the Nup107-160 complex were present throughout mitosis on centromeres and kinetochores, respectively, only the Nup107-160 complex was found at the spindle poles and proximal microtubules during prometaphase (A, prometaphase). Nup107-160 complex spindle pole localization was greatly diminished or absent after cells entered metaphase (A, metaphase and anaphase). Bar, 4 µm. (C) Immunofluorescence with anti-hNup160 and anti-hNup96 antibodies on HeLa cells stained the spindle poles during prometaphase (red, far left), identical to the localization seen for Nup133 and Nup85 in A and B. Immunofluorescence with affinity-purified anti-hNup93 polyclonal antibody or an anti-hNup62 mAb does not give a spindle stain. Affinity-purified antisera to Mad2, an outer kinetochore checkpoint protein found at the spindle poles and proximal microtubules during prometaphase (Howell et al., 2004

), shows localization identical to that of the Nup107-160 complex at that stage of the cell cycle (far right). Bar, 5 µm. (D) Nup133 colocalizes with NuMA in prometaphase HeLa cells. In cells prepared for immunofluorescence with affinity-purified anti-hNup133 and affinity-purified anti-xNuMA antisera, the localization of Nup133 and NuMA overlap in the spindle pole area in prometaphase cells. Nup133 is also found at the kinetochores and free in the cytoplasm. Bar, 5 µm.

Spindle pole staining could be seen specifically in prometaphase,as judged from the incomplete alignment of the chromosomes ontothe metaphase plate. This polar localization of the Nup107-160complex was not observed in metaphase or anaphase cells (Figure 2A).The narrow time window of Nup107-160 complex localization onspindles in mammalian cells suggested an explanation for whythe majority of these nucleoporins (Nup133, Nup85, and Nup160)had not been previously observed at the spindle poles by immunofluorescence(Belgareh et al., 2001

; Loiodice et al., 2004

) as well as anexplanation for why the spindle localization of Nup96 has beencontroversial (Enninga et al., 2003

; Loiodice et al., 2004

).The bulk of those studies concentrated on metaphase and anaphasecells, beyond the interval at which the complex is concentratedon spindles and poles; they would thus have found only negligiblelocalization of this complex on those structures.

To confirm definitively the localization of the Nup107-160 complexat spindle poles, we performed simultaneous immunofluorescencewith antisera to Nup133 and NuMA, a nuclear protein that isan established component of mitotic spindle poles (Merdes etal., 1996, and references therein). We found nearly identicallocalization of NuMA and Nup133 in prometaphase cells in theregion of the spindle poles (Figure 2D). Interestingly, thedistribution of the Nup107-160 complex is highly reminiscentof the behavior of a subset of the spindle checkpoint proteinsduring early mitosis. Specifically, Mad1, Mad2, Bub3, and Cdc20move along microtubules from the kinetochores, accumulatingon spindle poles at prometaphase (Howell et al., 2004). Theyare subsequently lost from kinetochores, spindles, and polesin metaphase. When we used anti-Mad2 antisera to stain HeLacells, we observed a prometaphase spindle pole stain (Figure 2C,right), identical to that seen with our anti-Nup107-160 complexantisera. We conclude that the Nup107-160 complex is much moredynamic in mitosis than had been thought and that it is foundat multiple locations within the mitotic spindle, correlatedwith the extent of spindle formation.

The Nup107-160 Complex Localizes to Spindles and Ran Asters in Mitotic Xenopus Extracts
To address Nup107-160 complex mitotic function in a system moreamenable to manipulation, we next used Xenopus mitotic extracts.Xenopus eggs are naturally arrested in meiotic metaphase. Whenlysed in the presence of the calcium chelator EGTA, the resultinglow Ca²⁺ concentration maintains the extract, termed a CSF-arrestedextract, within metaphase (Murray, 1991; Heald et al., 1996;Desai et al., 1999). When sperm chromatin is added to a CSFextract, microtubules assemble around each set of sperm chromosomesto form bipolar spindles within $~$ 60 min. If rhodamine-labeledtubulin is present during the reaction, microtubules can beeasily observed organized into bipolar spindles. Alternatively,spindles can be formed around fully replicated chromosomes withduplicated centrosome pairs in "cycled" extracts. In this case,CSF extracts are converted to interphase through the additionof calcium, and added sperm chromatin is allowed to form nucleiand undergo DNA replication for 60 min. When replication iscomplete, the extracts are induced to reenter mitosis throughthe addition of an equal volume of fresh CSF extract. The additionof CSF extract under these conditions normally promotes nuclearenvelope breakdown, chromatin condensation, and spindle formation.

We first determined whether the Nup107-160 complex associatedwith in vitro assembled Xenopus spindles in cycled egg extractscontaining added sperm chromatin and rhodamine-labeled tubulin.After fixation, the spindles were centrifuged onto coverslips.Immunofluorescence was performed with affinity-purified antibodiesto hNup133, xNup43, hNup62 (a noncomplex nucleoporin) as wellas control rabbit IgG antibodies. Both Nup133 and Nup43 wereclearly detected throughout the assembled spindles (Figure 3A).Neither anti-Nup62 nor control rabbit IgG antibodies, however,stained Xenopus spindles (Figure 3A). Similar to these spindlelocalization results, the Nup107-160 complex localized at fociof RanGTP-induced microtubule asters formed directly in CSFextracts (Supplemental Figure 1). Together, our results suggestthat the Nup107-160 complex is localized to mitotic spindlesin both human somatic cells and Xenopus egg extracts. Moreover,these findings show that Nup107-160 recruitment to asters isnot dependent upon their association with chromosomes.

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Figure 3. The Nup107-160 complex localizes to in vitro-assembled mitotic spindles. (A) Demembranated sperm chromatin and rhodamine-labeled tubulin were added to Xenopus CSF extracts. The reactions were induced to enter interphase through addition of 0.4 mM calcium chloride. After 1 h, the reactions were returned to mitosis by the addition of an equal volume of fresh CSF extract, and allowed to form spindles for 60 min. Reactions were fixed with formaldehyde, then the spindles were centrifuged onto coverslips, postfixed in methanol, and processed for immunofluorescence. The presence or absence of Nup133 (green, first row), Nup43 (green, second row), Nup62 (green, third row), or IgG (green, bottom row) on spindles was detected with the same affinity-purified antisera used in Figure 1. Presence of rhodamine-labeled tubulin (red, all rows), and DAPI-stained chromosomes (blue, all rows) is also shown. The right-most panels contain the merged images. Bar, 10 µm. (B) The staining of the in vitro assembled spindles by anti-Nup133 and Nup43 shown in A most often obscures concurrent kinetochore staining. However, occasional views reveal bright foci of kinetochore staining (indicated by arrowheads). An anti-Nup133 stain is shown. Bar, 10 µm.

Because of the high concentration of Nup107-160 complex proteinson spindles (Figure 3A), it was difficult to observe kinetochorestaining above the bright spindle stain. However, in the occasionalspindle with fainter anti-Nup133 stain, we clearly observedbright foci at the midplane of the spindle (Figure 3B). Forpurely technical reasons, it was not possible to confirm theidentity of these foci as kinetochores by immunostaining. However,given their localization, paired appearance, and the high degreeof conservation between the Xenopus and human Nup107-160 complexes,these sites are likely to be Xenopus kinetochores (also seeFigure 4A) Together, the data indicate that the Nup107-160 complexis present throughout in vitro reconstituted spindles, in amanner that may be analogous to its localization on mammalianprometaphase spindles.

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Figure 4. The Nup107-160 complex shows increased accumulation on unattached kinetochores. (A) Mitotic (CSF) extract was incubated with demembranated sperm chromatin for 40 min at 23°C with (bottom) or without (top) nocodazole. Mitotic chromosomes were collected and spread by centrifugation onto coverslips and then analyzed by indirect immunofluorescence with antibodies to Xenopus Nup37 (green) and Bub1 (red). The chromosomal DNA was stained with DAPI. Note that these conditions do not maintain spindle structure. Both Nup37 and BubR1 staining of kinetochores increases greatly. Bar, 10 µm. (B) HeLa cells were treated with nocodazole for 2 h before performing immunofluorescence by using affinity-purified anti-hNup133 antisera. The amount of the Nup107-160 complex, visualized with affinity-purified anti-hNup133 antisera, increased greatly giving large crescents, and ring structures typical of those outer kinetochore proteins that are affected by microtubule disassembly. Bar, 5 µm.

Recruitment of the Nup107-160 Complex to Unattached Kinetochores
Given the dynamic nature of Nup107-160 complex localizationthrough mitosis, we wished to determine whether the amount ofNup107-160 complex on kinetochores is dependent upon microtubuleattachment. We addressed this question by assembling kinetochoresin vitro using sperm chromatin in Xenopus CSF extract plus orminus the microtubule depolymerizing agent, nocodazole (seeHoffman et al., 2001

), and references therein). After 40 min,the chromatin was centrifuged onto coverslips and immunofluorescencewas performed with antisera directed against Nup37 and againstcheckpoint protein Bub1. As expected, significantly more Bub1was recruited to kinetochores in the presence of nocodazolethan in untreated extracts (Figure 4A, top and bottom centerpanels). Nup37 also showed an increase in intensity at kinetochoresin nocodazole-treated extracts (Figure 4A, top and bottom left).Although it is formally possible that this increased stainingintensity may result from conformational changes within thecomplex that allow better antibody recognition, we do not believethat this is the case; very similar increases in staining intensitywere consistently observed using multiple independent antiseradirected against different complex members. Rather, we believethat the increased staining in nocodazole-treated extracts suggestsincreased Nup107-160 complex recruitment to unattached kinetochoresin vitro.

To examine Nup107-160 complex recruitment onto unattached kinetochoresin somatic cells, we treated HeLa cells for 2 h with nocodazoleand stained with antibodies directed against Nup133. We foundthat more Nup133 was recruited to kinetochores in nocodazole-treatedcells (Figure 4B, right) than in untreated cells (Figure 4B,left). Analysis of untreated and nocodazole-treated mitoticcells by using methods described by Hoffman et al. (2001) indicateda measurable (1.8-fold) increase in kinetochore staining intensitywith nocodazole (Supplemental Table 2). Similar to the in vitroobservations, this finding indicates that the Nup107-160 complexassociation to kinetochores is sensitive to microtubule attachment.Notably, nocodazole also caused Nup133, and presumably the entireNup107-160 complex, to assemble as expanded crescents and ringswere observed around kinetochores (Figure 4B, right, also seeinset). A similar morphological change at unattached kinetochoresof nocodazole-treated cells is characteristic of a subset ofdynamic outer kinetochore proteins, including BubR1, Mad2, dynein,and CENP-E (Hoffman et al., 2001; Maiato et al., 2004).

The Xenopus Nup107-160 Complex Is Not Required for Spindle Checkpoint Activation
Given the similarities between Nup107-160 complex and spindlecheckpoint proteins in their recruitment to unattached kinetochores,we wished to determine whether this complex plays a role inthe checkpoint. To address this question, sperm chromatin andnocodazole were added to mock-depleted or Nup107-160 complex-depletedCSF extracts (Figure 5). After 40 min, the mitotic chromosomesand associated structures were centrifuged onto coverslips byusing conditions that spread the DNA for better kinetochoreanalysis (Arnaoutov and Dasso, 2003). It should be noted thatunder these conditions, mitotic spindles and related microtubulestructures are not well maintained.

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Figure 5. Extracts lacking the Nup107-160 complex have an intact spindle checkpoint. (A) Nup107-160 complex depleted ( ${Delta}$ 107-160) or mock depleted (mock) CSF extracts plus sperm chromatin and nocodazole were incubated for 40 min at 23°C. Mitotic chromosomes were analyzed by indirect immunofluorescence by using antibodies to the checkpoint proteins Bub1, BubR1, and Mad2, which accumulated at kinetochores even in the absence of the Nup107-160 complex. (B) The checkpoint was checked for responsiveness to Ran by the addition of the RanGEF RCC1 (lanes 2 and 4). The checkpoint protein Bub1 and Mad2 were released normally in both extracts. (C) CSF extracts with nuclei were treated with DMSO (top) or nocodazole (bottom). After incubation for 40 min, extracts were stimulated with 0.6 mM Ca²⁺ to destroy CSF. At 45 min after calcium addition, Hoechst 33258 dye was added for the examination of DNA morphology. (D) At the indicated times after calcium addition aliquots were removed for Western blot analysis with anti-cyclin B2 antibodies. (E) Anti-Nup133 immunodepletion of mitotic CSF extract removes all visible Nup133 (lanes 2 and 4; 0.2 and 0.4 µl of extract was loaded, respectively). Mock depletion of extract with control IgG antibodies did not (lanes 1 and 3; 0.2 and 0.4 µl). Levels of noncomplex nucleoporins, such as Nup62, were not altered. (F) An immunoblot of mock- and Nup107-160 complex-depleted extracts is shown probed with antibodies to Nup160, Nup133, Importin- ${alpha}$ , the AAA ATPase p97, dynein, and Nup43. Lanes 1 and 2 contain 0.2 µl of extract; lanes 3 and 4 contain 0.4 µl of extract. Nup160, Nup133, and Nup43, all members of the complex, were depleted. Levels of Importins and noncomplex kinetochore components tested were not altered by Nup107-160 deletion.

Immunofluorescence on chromatin showed that the Bub1, BubR1,and Mad2 spindle checkpoint proteins were present on kinetochoresin mock-depleted, nocodazole-treated egg extracts (Figure 5A,Noc/Mock). Strikingly, an identical pattern of checkpoint proteinloading onto kinetochores was seen in Nup107-160 complex-depletedmitotic extracts (Figure 5A, Noc/D107-160). This loading couldalso be observed by biochemically analyzing centrifuged chromatinderived from mitotic reactions performed under the same experimentalconditions. Immunoblotting of such chromatin with anti-Bub1and anti-Mad2 antisera revealed that both mock- and Nup107-160-depletedextracts loaded spindle checkpoints onto chromatin/kinetochoresin identical amounts (Figure 5B, lanes 1 and 3).

The addition of nocodazole to CSF extracts containing high concentrationsof sperm chromatin results in the presence of unattached kinetochores,which are detected by the spindle checkpoint pathway and inducemitotic arrest (Minshull et al., 1994). As a result, such checkpointarrested extracts do not exit from mitosis when CSF arrest isreleased with Ca²⁺. The maintenance of this arrest can be monitoredboth through chromosome morphology and through the degradationof key mitotic regulators, such a cyclin B. We examined whethercheckpoint arrest was induced normally in the absence of theNup107-160 complex (Figure 5, C and D). Both control and Nup107-160complex-depleted extracts treated with dimethyl sulfoxide (DMSO)exited mitosis normally, as demonstrated by the degradationof cyclin B protein. Control extracts formed nuclei in the subsequentinterphase, whereas the depleted extracts showed defects innuclear assembly similar to those demonstrated previously (Harelet al., 2003b; Walther et al., 2003a). Notably, both controland Nup107-160 complex-depleted extracts showed mitotic arrestin response to the addition of nocodazole, with no evident changein condensed chromatin morphology or degradation of cyclin B.These results clearly indicate that the spindle assembly checkpointdoes not absolutely require the Nup107-160 complex for its activation.

Finally, elevated levels of Ran-GTP can inactivate the spindlecheckpoint in nocodazole treated extracts and release Mad2 andBub1 from kinetochores (Arnaoutov and Dasso, 2003). This effectcan be observed through the addition of exogenous RCC1, whichpromotes increased nucleotide exchange on Ran. Given the relationshipbetween Ran and the NPC during interphase, we wondered whetherthis mechanism was still functional in the absence of the Nup107-160complex. To address this question, we added RCC1 protein tonocodazole-treated mock- and Nup107-160 complex-depleted extractsand monitored release of the checkpoint proteins from the kinetochores.As shown in Figure 5B, release of Bub1 and Mad2 from chromatinwas identical in the presence (lane 2) or absence (lane 4) ofthe Nup107-160 complex. Although we cannot rule out the possibilitythat the very small amount of Nup107-160 complex remaining indepleted extracts is sufficient for normal spindle checkpointactivity, our current observations indicate that Nup107-160complex is not required in large amounts for recruitment ofcheckpoint proteins to unattached kinetochores, for the activationof the spindle checkpoint, or for the response of this checkpointto elevated levels of Ran-GTP.

The Nup107-160 Complex Is Required for a Normal Spindle Assembly
Because the Nup107-160 complex did not seem to be required atkinetochores for the spindle checkpoint, we wondered whetherit might play a role in spindle assembly. We used two experimentalapproaches to address this question. First, we assayed spindleassembly around sperm chromatin in Nup107-160 complex-depletedCSF extracts. Note that under these conditions, sperm chromatinhas not undergone DNA replication before spindle assembly, sothat it contains only unreplicated centromeres. Also, the spermchromatin brings only one centriole pair into the reaction,so only a single pole is formed around a centrosome. The otherpole is spontaneously formed in this reaction through the Ran-dependentnucleation of microtubules in the vicinity of the sperm chromatin(Mitchison et al., 2004). We added sperm chromatin and rhodamine-labeledtubulin to mock- and Nup107-160 complex-depleted extracts andallowed spindle formation for 60 min. Abundant bipolar spindlesformed throughout the mock-depleted mitotic extract at 60 min(Figure 6A, mock depleted). In strong contrast, only around15% of the sperm chromatin in the depleted extracts was associatedwith spindles. Instead, most chromatin seemed rounded with fewor no associated microtubules at 60 min (Figure 6A, ${Delta}$ 107-160).The rare bipolar spindles that we observed were faint and containedmany fewer microtubules (Figure 6A, ${Delta}$ 107-160, right). These dataindicate that the absence of the Nup107-160 complex severelydisrupts spindle assembly.

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Figure 6. Disruption of the Nup107-160 complex severely compromises spindle assembly. (A) Spindles were assembled for 60 min in vitro by adding sperm chromatin and rhodamine-labeled tubulin to mitotic CSF extracts that were either mock-depleted (top) or Nup107-160 complex-depleted (bottom). Aliquots were examined for spindle assembly by fixation, centrifugation, and a second fixation, before examination with a Zeiss Axioskop fluorescence microscope. In both A and B, DNA was stained with DAPI DNA dye (blue, all rows). Absence of the Nup107-160 complex produced a much reduced number of bipolar spindles and those that were seen were small and contained many fewer microtubules. (B) Nuclei were assembled in interphase Xenopus extract for 60 min. At that time, an equal volume of CSF extract was added to convert the interphase extract to mitosis, via the cyclin B present in the CSF extract. Five minutes later rhodamine-labeled tubulin and either control IgG (left), affinity-purified anti-Nup133 antibody (middle), or affinity-purified anti-Nup43 antibody (right) were added. Spindle assembly was assessed 60 min later, as in A. Both antibodies to the Nup107-160 complex significantly interfered with correct spindle assembly, mirroring the depletion defect of A. Bar, 10 µm.

In the second approach, we used "cycled" extracts, where chromosomeswere fully replicated and centrosomes duplicated during interphase.The reactions were then driven back into M phase through theaddition of fresh CSF extract, as in Figure 3. Notably, it wasnot possible to perform this type of experiment using immunodepletedextracts, because both nuclear pore assembly and DNA replicationare dependent upon the intact Nup107-160 complex (Harel et al.,2003b

). Instead, we added rhodamine-labeled tubulin 5 min afterthe induction of reentry into mitosis, along with a controlIgG, affinity-purified anti-Nup133 antibody, or affinity-purifiedanti-Nup43 antibody (Figure 6B). Addition of antibodies at thispoint allowed us to restrict our analysis of Nup107-160 complexfunction strictly to mitosis. As before, the samples were fixedand centrifuged onto coverslips.

The control IgG-treated reaction showed normal, bipolar spindleformation (Figure 6B, left). By contrast, antibodies directedagainst either Nup133 and Nup43 significantly interfered withcorrect spindle assembly (Figure 6B; Supplemental Table 3).In this case, we found that faint spindles bipolar spindleswere more common than chromatin completely devoid of microtubules.These spindles were greatly reduced in overall size and hada maximal density of spindle microtubules that was only one-halfof the density found in IgG-treated controls. Together, bothapproaches lead us to conclude than the Nup107-160 complex isessential for robust mitotic spindle formation.

The Nup107-160 Complex Is Not Required for Ran Aster Assembly
Logically, the defects observed after Nup107-160 complex depletioncould reflect disruption of several distinct processes requiredfor spindle formation. These processes include microtubule polymerization,initial aster assembly around sperm centrioles, and kinetochoreattachment. Under normal circumstances, increased levels ofRan-GTP cause massive polymerization of microtubules in mitoticXenopus extracts, even in the absence of added chromatin (Kalabet al., 1999; Ohba et al., 1999; Wilde and Zheng, 1999; Zhanget al., 1999). These asters spontaneously rearrange into spindle-likestructures (microspindles) through the action of multiple microtubulemotor proteins within extracts. To test whether Ran-mediatedmicrotubule assembly pathways are disrupted by the absence ofthe Nup107-160 complex, we measured the capacity of Nup107-160-depletedmitotic extracts (Figure 5, E and F) to form microtubule astersand spindle-like structures in response to a constitutivelyGTP-bound form of Ran (Ran-Q69L; 25 µM, final). We addedrhodamine-tubulin at the start of the reaction to visualizemicrotubule assembly and assayed aster assembly microscopicallyafter 30 min.

As shown in Supplemental Figure 2, RanQ69L-induced asters formedequivalently in both mock- and Nup107-160 complex-depleted extracts(top). The morphology of asters in both reactions was very similar,and the number of asters in the Nup107-160-depleted extract(13 ± 6 asters/field) was comparable with or greaterthan the number in mock-depleted control reactions (11 ±6 asters/field). Similarly, microspindles formed at least aswell in Nup107-160-depleted extracts as in mock-depleted extracts(Supplemental Figure 2, bottom). We conclude that the Nup107-160complex is not required for microtubule polymerization in responseto elevated Ran-GTP levels.

The Nup107-160 Complex Is Required for Formation of a Stable Mitotic Spindle In Vitro
We next wished to ascertain whether formation of asters aroundsperm centrioles occurred normally as well as to determine whena clear spindle assembly defect could first be observed. Todo this, we examined the time-course spindle assembly aroundsperm chromatin in control and Nup107-160-depleted CSF extracts(Figure 7).

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Figure 7. Absence of the Nup107-160 complex causes an increasing regression in spindle assembly and stability. (A) Mock-depleted and Nup107-160 complex-depleted Xenopus mitotic (CSF) extracts were supplemented with rhodamine-labeled tubulin and sperm chromatin at t = 0'. Aliquots were withdrawn at 15, 25, and 60 min, prefixed with formaldehyde, spun down onto coverslips, postfixed with methanol, and examined with a Zeiss Axioskop 2 microscope. Bar, 10 µm. (B) Quantitation of in vitro spindle defects observed upon depletion of the Nup107-160 complex. The data from the 60-min time point in Figure 7A is shown graphically.

After 15 min, each group of sperm chromosomes in both mock anddepleted extracts was associated with a microtubule aster (Figure 7A).The size and morphology of these asters was comparable betweenthe depleted and control reactions, although the size was perhapsslightly less in depleted reactions. This observation suggeststhat sperm aster formation initially occurs relatively normallyin the absence of the Nup107-160 complex. After 25 min, themajority (87%) of chromatin figures in the mock-depleted extracthad advanced to very robust half-spindles, and 13% were alreadybipolar (Figure 7, mock, 25'). However, the asters that hadformed on chromatin in the Nup107-160-depleted extract at 15min had deteriorated, such that 19% of the chromatin lackedany microtubules and 59% had few microtubules (Figure 7A, ${Delta}$ 107-160,25').

After 1 h, fully one-half of the sperm chromatin in the mock-depletedextract had formed robust bipolar spindles (Figure 7, A andB). In the depleted extract, however, the deterioration in microtubuleshad progressed further, such that a large fraction of the chromatinfigures (62%) lacked any associated microtubules whatsoever.A small fraction of the sperm chromatin ( $~$ 6%) was associatedwith bipolar spindles at this point. Interestingly, an increasedintensity of DNA staining in most of these cases suggested thatthe few bipolar spindles found in depleted egg extracts mayhave formed predominately from fusion of two chromatin massesand their associated half-spindles. The data from the chromatinfigures at the 60-min time point is summarized in Figure 7B.The endpoint of this kinetic experiment was entirely consistentwith what we had observed in depletion of the Nup107-160 complexfrom mitotic extract (Figure 6A). Specifically, the majorityof structures observed in Nup107-160 complex-depleted extractswere extremely thin in density of microtubules.

Together, our results argue that the Nup107-160 complex playsan important role in mitotic spindle assembly. Its functionis not critical to microtubule nucleation around sperm centrosomesor for microtubule assembly in response to exogenous Ran-GTP.Rather, the defects in spindle assembly that we observe in theabsence of the Nup107-160 complex arise at later times; thesephenotypes are consistent with the notion that this complexis important for the assembly or maintenance of microtubulefibers between the spindle poles and chromosomes.

DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have examined the localization and role of the Nup107-160complex during mitosis. The Nup107-160 complex resembles a subsetof checkpoint proteins in its bimodal distribution on spindlesand kinetochores as well as in its dramatic accumulation onunattached kinetochores in nocodazole-treated cells. However,the Nup107-160 complex was not required for any aspect of spindlecheckpoint function that we tested. Rather, depletion or inhibitionof the Nup107-160 complex rendered spindle assembly strikinglydefective. Together, these observations offer a global pictureof the dynamics of the Nup107-160 complex during mitosis aswell as the first evidence for its mitotic function that canbe clearly distinguished from its interphase roles in NPC structureand nuclear transport.

Antibodies to four different members of the Nup107-160 complexstained spindle poles and proximal spindle microtubules in mammaliancells during prometaphase (Figure 2). This spindle pole localizationdiminished significantly in metaphase, suggesting that complexlocalization is dynamic. The strong staining of spindles inXenopus mitotic extracts using antisera to multiple membersof the Nup107-160 complex (Figure 3) is consistent with ourresults in mammalian cells. The disparity of Nup107-160 complexdistribution in prometaphase mammalian cells and Xenopus extractsmay reflect differing mechanisms of spindle assembly in thesetwo systems as well as the meiotic nature of CSF extracts. Inparticular, Xenopus spindles rely more upon self-organization(i.e., chromatin-induced microtubules) than search-and-capturemechanisms that are essential in somatic cells (i.e., centrosome-nucleatedmicrotubules) (Karsenti and Vernos, 2001; Gadde and Heald, 2004;Mitchison, 2005).

The localization of the Nup107-160 complex (Figure 2) was reminiscentof the behavior of spindle checkpoint proteins Mad1, Mad2, andBub3 (Howell et al., 2004; Maiato et al., 2004). Moreover, likethe checkpoint proteins, accumulation of the Nup107-160 complexat kinetochores responded dynamically to cell cycle conditions.On disruption of kinetochore–microtubule attachment withnocodazole, we observed increased amounts of the Nup107-160complex on kinetochores (Figure 4). Indeed, the Nup107-160 complexassembles into expanded crescents and rings around each kinetochore.This increase mirrors the behavior of BubR1 and Mad2 as wellas the outer kinetochore motor proteins dynein and CENP E (Hoffmanet al., 2001; Maiato et al., 2004). A notable difference, however,is that the Nup107-160 complex remains on kinetochores throughanaphase (Figure 2A; Loiodice et al., 2004), whereas Mad1, Mad2,and Bub3 all become drastically reduced after kinetochore–microtubuleattachment (Taylor et al., 1998; Shannon et al., 2002; Howellet al., 2004). Therefore, checkpoint proteins and the Nup107-160complex diverge in their behavior during later stages of mitosis.

Despite similarities in behavior of checkpoint proteins andof the Nup107-160 complex, we did not find that this complexis essential for the correct localization of checkpoint proteinsto kinetochores in egg extracts, for the activation of the spindlecheckpoint or for the regulation of this checkpoint by Ran-GTP(Figure 5). Our findings cannot not rule out, however, the possibilitythat a very small amount of Nup107-160 complex remains in thedepleted extract, sufficient for activation of the highly sensitivespindle checkpoint.

The Nup107-160 complex was similarly dispensable for formationof microtubule asters around sperm centrioles (Figure 7A), andfor formation of asters in response to exogenous Ran-GTP (SupplementalFigure 2). By contrast to the Nup107-160 complex, the mRNA exportfactor Rae1 is essential in Xenopus extracts for assembly ofRan-GTP asters and spindles associated with sperm chromatin(Blower et al., 2005). This difference between Rae1- and Nup107-160–depletedextracts suggests that the Nup107-160 complex acts either distinctlyfrom or upstream of Rae1. Ran-GTP-induced asters in extractsdepleted of the Nup107-160 complex eventually organized intomicrospindles (Supplemental Figure 2), further indicating thatthis complex is not required for motor activities involved inmicrospindles formation (Karsenti and Vernos, 2001; Gadde andHeald, 2004; Mitchison, 2005).

However, our study revealed that the Nup107-160 complex is criticalfor later events in spindle assembly around chromatin in bothCSF extracts (Figures 6 and 7) and cycled extracts (Figure 6).Our data would be consistent with the possibility that the Nup107-160complex acts directly in these later steps of spindle assembly.Possibly more likely, however, the complex might also functionindirectly, through intimate association to or regulatory interactionwith other spindle- or kinetochore-associated proteins. Interestingly,the defects observed in Nup107-160-depleted egg extracts werereminiscent of defects in egg extracts depleted of the chromosomalpassenger complex (CPC), which also show aster assembly aroundsperm centrioles, but do not progress to formation of bipolarspindles (Sampath et al., 2004). The possible relationship ofthe Nup107-160 complex to the CPC and other established spindleassembly factors will be an interesting topic for future investigation.

Our results do not provide a definitive point of action forthe complex at later stages of spindle assembly. However, detailedreports on spindle assembly in egg extracts allow some speculationon this topic. Each group of sperm chromosomes initially formsa pole around their single centrosome when added to CSF eggextracts, and the second pole is subsequently derived from chromosomallystabilized microtubules (Mitchison et al., 2004). It has beenwell established that the localized production of Ran-GTP byRCC1 contributes substantially to chromatin-induced microtubuleassembly (Hetzer et al., 2002). The flux of spindle microtubulescommences when bipolarity is achieved in this manner, presumablyin response to the assembly of antiparallel, overlapping microtubulesoriginating at the opposite poles (Mitchison et al., 2004).Notably, sequestration of Ran pathway targets by exogenous Importin- ${alpha}$ causes a loss of microtubule density in preformed spindles andblocks spindle microtubule flux. Based upon these observationsand findings in other systems, we can imagine two possible rolesfor the Nup107-160 complex, which are not mutually exclusive.

In the first model, the absence of the Nup107-160 complex onkinetochores may be causative for the defects we observed. Inthis case, depletion of the Nup107-160 complex may prevent effectivecapture of centrosome-initiated microtubules, which is knownto be required for production of stable spindle fibers. Indeed,both the kinetochore localization of the Nup107-160 complexand the normal initiation but subsequent decay of centrosome-inducedasters in Nup107-160 complex-depleted extracts might be consistentwith an inability of kinetochores to capture and stabilize microtubules.Alternatively, the Nup107-160 complex may play a general rolein stabilizing spindle microtubules around sperm chromatin,perhaps by acting as an upstream regulator of the Ran pathway.In this case, monopolar spindles would fail to mature into bipolarstructures around chromatin added to CSF extracts and wouldnot develop networks of antiparallel microtubules required topromote flux within the spindle. This model might account forthe persistence of weak bipolar spindles in the cycled extracts;each group of chromosomes in this situation would form spindlescontaining two centrosomes and might therefore be less dependentupon chromatin-mediated stabilization of microtubules for achievingbipolar organization.

In summary, Nup107-160 complex localization on spindles mirrorsthe behavior of a subset of spindle checkpoint proteins, bothin occurring transiently in the spindle pole at prometaphaseand in responding dynamically to spindle checkpoint conditionsat the kinetochore. Within mitosis, this complex has a rolein spindle assembly that can be clearly distinguished from interphasenuclear envelope assembly and NPC function. This complex istherefore likely to be important for accurate mitotic segregationof vertebrate chromosomes.

ACKNOWLEDGMENTS

We thank A. Desai and D. Cleveland for helpful comments. Thiswork was supported by National Institutes of Health Grant R01GM-33279 to D. F. and by Intramural National Institute of ChildHealth and Human Development funds to M. D.

Footnotes

The online version of this contains supplemental material at MBC Online (http://www.molbiolcell.org).

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E05-11-1061)on June 28, 2006.

Address correspondence to: Douglass Forbes (DForbes{at}UCSD.edu)

Abbreviations used: NPC, nuclear pore complex

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aitchison, J. D., Blobel, G., Rout, M. P. (1995). Nup120p: a yeast nucleoporin required for NPC distribution and mRNA transport. J. Cell Biol 131, 1659–1675.[Abstract/Free Full Text]

Arnaoutov, A., Azuma, Y., Ribbeck, K., Joseph, J., Boyarchuk, Y., Karpova, T., McNally, J., Dasso, M. (2005). Crm1 is a mitotic effector of Ran-GTP in somatic cells. Nat. Cell Biol 7, 626–632.[CrossRef][Medline]

Arnaoutov, A. and Dasso, M. (2003). The Ran GTPase regulates kinetochore function. Dev. Cell 5, 99–111.[CrossRef][Medline]

Askjaer, P., Galy, V., Hannak, E., Mattaj, I. W. (2002). Ran GTPase cycle and importins alpha and beta are essential for spindle formation and nuclear envelope assembly in living Caenorhabditis elegans embryos. Mol. Biol. Cell 13, 4355–4370.[Abstract/Free Full Text]

Bai, S. W., Rouquette, J., Umeda, M., Faigle, W., Loew, D., Sazer, S., Doye, V. (2004). The fission yeast Nup107-120 complex functionally interacts with the small GTPase Ran/Spi1 and is required for mRNA export, nuclear pore distribution, and proper cell division. Mol. Cell. Biol 24, 6379–6392.[Abstract/Free Full Text]

Bamba, C., Bobinnec, Y., Fukuda, M., Nishida, E. (2002). The GTPase Ran regulates chromosome positioning and nuclear envelope assembly in vivo. Curr. Biol 12, 503–507.[CrossRef][Medline]