Facilitated Nucleocytoplasmic Shuttling of the Ran Binding Protein RanBP1

doi:10.1128/MCB.20.10.3510-3521.2000

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Molecular and Cellular Biology, May 2000, p. 3510-3521, Vol. 20, No. 10
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Facilitated Nucleocytoplasmic Shuttling of the Ran Binding Protein RanBP1

Kendra Plafker and Ian G. Macara^*

Markey Center for Cell Signaling and Department of Pharmacology, University of Virginia, Charlottesville, Virginia 22908

Received 7 September 1999/Returned for modification 12 October 1999/Accepted 21 February 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Ran binding protein RanBP1 is localized to the cytosol of interphase cells. A leucine-rich nuclear export signal (NES)near the C terminus of RanBP1 is essential to maintain this distribution.We now show that RanBP1 accumulates in nuclei of cells treatedwith the export inhibitor, leptomycin B, and collapse of the nucleocytoplasmicRan:GTP gradient leads to equilibration of RanBP1 across the nuclearenvelope. Low temperature prevents nuclear accumulation of RanBP1,suggesting that import does not occur via simple diffusion. GlutathioneS-transferase (GST)-RanBP1(1-161), which lacks the NES, accumulatesin the nucleus after cytoplasmic microinjection. In permeabilizedcells, nuclear accumulation of GST-RanBP1(1-161) requires nuclearRan:GTP but is not inhibited by a dominant interfering G19V mutantof Ran. Nuclear accumulation is enhanced by addition of exogenouskaryopherins/importins or RCC1, both of which also enhance nuclearRan accumulation. Import correlates with Ran concentration. Remarkably,an E37K mutant of RanBP1 does not import into the nuclei underany conditions tested despite the fact that it can form a ternarycomplex with Ran and importin $beta$ . These data indicate that RanBP1translocates through the pores by an active, nonclassical mechanismand requires Ran:GTP for nuclear accumulation. Shuttling of RanBP1may function to clear nuclear pores of Ran:GTP, to prevent prematurerelease of import cargo from transportreceptors.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The defining feature of eukaryotic cells is the compartmentalization of DNA replication and transcription within the nucleus.Access to the nuclear compartment is provided by pores that areplugged through the double membrane of the nuclear envelope (forreviews, see references 15 and 66). A multitude of solubletransport receptors and accessory proteins controls the transitof protein and nucleic acid cargo through these pores (for recentreviews, see references 24, 40, 42, and 64). The vectorialityof cargo transport is in many cases dependent on the asymmetricdistribution of Ran, a small GTP binding protein, and of its regulatoryfactors (8, 17). Ran is predominantly nuclear and is believedto be maintained in the GTP-bound state (Ran:GTP) by a guaninenucleotide exchange factor, RCC1, which is associated with chromatinin the nucleus (7, 58). A Ran-specific GTPase-activatingprotein, RanGAP, which converts Ran to the GDP-bound state, isexcluded from the nucleus (5, 13, 30). This asymmetricarrangement of regulatory factors ensures that a steep Ran:GTPgradient exists across the nuclear pores, and the collapse ofthis gradient inhibits many forms of nuclear traffic (32, 52).

Proteins destined for import into the nucleus frequently possess a nuclear localization signal (NLS) containing multiple basicamino acid residues (16). The NLS is recognized by an adapterprotein called importin $alpha$ (also variously called karyopherin- $alpha$ ,p56, SRP1, PTAC58, and pendulin) which associates with a transportermodule, importin $beta$ (also called karyopherin- $beta$ and p97) (11,25, 31, 36, 48, 61). This complex can bind to nuclearpores and translocate from one side of the pore to the other,probably by a type of facilitated diffusion (18, 50). Ran:GTP,present within the nucleus, dissociates the complex from the poresand releases importin $alpha$ and its associated cargo from importin $beta$ (26, 49). Thus, it may be that the Ran gradient is not requiredfor translocation per se but can drive a net accumulation of thecargo in the nuclearcompartment.

The importin $beta$ is then believed to return to the cytosol as a complex with Ran:GTP (26, 28). There, the RanGAP must hydrolyzethe GTP to permit release of the importin $beta$ for another roundof import. However, RanGAP alone is unable to act on Ran:GTP thatis bound to importin $beta$ (19, 26). Another cytosolic factor,the Ran binding protein RanBP1, is required together with importin $alpha$ to permit efficient GTP hydrolysis by RanGAP (4, 20). Thegiant nucleoporin Nup358 can probably serve a similar function(65, 67). RanBP1 is a 23-kDa cytosolic protein that possessesa conserved Ran binding domain (RanBD) of about 135 amino acidresidues, which specifically recognizes Ran in the GTP-bound state(3, 14). The crystal structure of Ran in a complex with thesecond RanBD of Nup358 has been solved, and the two proteins forman unusually tight embrace in which the N terminus of the RanBDis wrapped around Ran, and the C terminus of Ran is wrapped aroundthe RanBD (62). Ran:GTP can form a ternary complex with RanBP1and importin $beta$ or with other members of the karyopherin family,and this complex is only weakly susceptible to RanGAP (4, 38).The presence of importin $alpha$ , which will sequester free importin $beta$ , increases the efficiency of the hydrolysis (4, 20). RanBP1is therefore predicted to be required for continued nuclear proteinimport, and this has been shown to be the case in yeast (57).RanBP1 and importin $beta$ have no measurable affinity for each otheror $---$ separately $---$ for Ran:GDP, but surprisingly they can form a stableternary complex with one another (12). The purpose of this RanBP1-importin $beta$ -Ran:GDP complex remainsobscure.

Proteins that need to be exported from the nucleus often possess a distinct, leucine-rich nuclear export signal (NES) (fora review, see reference 23). The NES can form a ternary complexwith an export receptor, called Crm1 (or exportin 1), and Ran:GTP(2, 21, 22, 44, 60). The formation of this complexwill therefore be favored in the nucleus. After translocationthrough the pores, RanGAP $---$ again with the likely assistance ofRanBP1 $---$ can hydrolyze the Ran:GTP and release the NES cargo intothe cytosol. Therefore, RanBP1 probably plays an essential rolein nuclear protein export. A similar mechanism can account forthe export of importin $alpha$ by the transport factor Cas (37).

A complete understanding of nuclear protein transport requires that we determine the mechanism by which essential factorssuch as RanBP1 maintain their specific locations within the cell.The role of RanBP1 as an accessory factor for RanGAP implies thatRanBP1 must be retained in the cytosol. Indeed, ectopic expressionof nuclear RanBP1 is toxic to cells, and microinjection of RanBP1into nuclei inhibits nuclear transport, probably because it sequestersnuclear Ran:GTP and effectively collapses the nucleocytoplasmicRan:GTP gradient (32, 53). It may also interfere with theformation of export complexes. This requirement for a cytoplasmiclocation presents a problem to the cell, because RanBP1 is inprinciple small enough to diffuse through the nuclear pores, andwithin the nucleus it will form a stable ternary complex withRan:GTP and importin $beta$ . Two distinct mechanisms may confer thecytoplasmic distribution of small proteins: (i) retention by bindingto a larger cytoplasmic protein and (ii) active export. RanBP1possesses a functional NES near its C terminus (54, 68). However,it also possesses an adjacent upstream sequence that may act incytoplasmic retention (54). Three other groups have providedindications that RanBP1 may shuttle between the cytosol and nucleus.Zolotukhin and Felber (68) found that the ectopic expressionof the Rev protein (which contains an NES) can lead to the nuclearaccumulation of RanBP1, presumably by competing for Crm1. Schlenstedtet al. (56), in a study of the Yrb4p importin in yeast, demonstratedthat a dominant interfering mutant of Yrb4p that blocks bidirectionalnuclear transport also caused the nuclear accumulation of Yrb1p,the yeast homologue of RanBP1. However, in both cases the inhibitoryprotein was expressed for a period greater than the cell cycletime. Thus, these results do not resolve whether RanBP1 continuallyshuttles across the nuclear pores or instead enters the nucleusonly at a specific time during cell division. For example, inmammalian cells an NES might be required to ensure that RanBP1is excluded from the nucleus after mitosis when the integrityof the nuclear envelope is reestablished. A third study examinedthe distribution of RanBP1 in Xenopus oocytes after microinjectionof an NES-peptide conjugate, which inhibits mRNA and snRNA transport(46). Oocytes were fractionated after 6.5 h, and the nuclearand cytosolic fractions were immunoblotted for RanBP1. These resultsdemonstrated that RanBP1 became partially associated with thenuclei $---$ either at the pores or within the nucleoplasm $---$ in the presenceof the competing NES-peptide. In all of these studies, however,it could be argued that the RanBP1 enters the nucleus only inresponse to a general perturbation in nucleartransport.

We now show that RanBP1 does continually shuttle quite rapidly between the nuclear and cytoplasmic compartments. LeptomycinB (LMB), which specifically inhibits NES-mediated export (63),causes a nuclear accumulation of endogenous RanBP1 and of a greenfluorescent protein (GFP)-RanBP1 fusion protein. MicroinjectedGST-RanBP1 lacking its C-terminal NES accumulates in the nucleusin the absence of any transport inhibitors. Collapse of the Ran:GTPgradient results in the equilibration of RanBP1 across the nuclearenvelope. The nuclear accumulation of a GST-RanBP1 mutant thatlacks the NES requires nuclear Ran:GTP. A point mutation in theN-terminal arm of the RanBD of RanBP1 completely blocks importinto nuclei under the conditions tested. Although this mutanthas a reduced affinity for Ran, it can form a ternary complexwith Ran:GTP and importin $beta$ or importin 5 (47). We propose thatthe RanBP1 can translocate through the nuclear pores by an activemechanism and, in the absence of functional export, accumulatewithin the nuclei in a complex with Ran:GTP.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Proteins. Recombinant proteins used in in vitro import assays and microinjection assays were overexpressed in Escherichia coli as glutathioneS-transferase (GST) fusions and affinity purified using glutathione(GSH)-Sepharose (Pharmacia catalog no. 17-0756-01). The proteinswere either eluted off the Sepharose with GSH or proteolyticallycleaved away from the GST using thrombin, as described previously(38, 39). RanBP1 mutants were isolated from mutant librariesgenerated either by template-limited PCR or by incorporation ofdoped oligonucleotides (47). Crm1 was partially purified asdescribed by Holaska and Paschal (29). Recombinant Ran was convertedto the GTP-bound state (Ran:GTP) by incubation with 1 mM GTP inthe presence of recombinant RCC1 (2.4 µg/ml) and 5 mM MgCl₂ (10min at 30°C) or by incubation with 1 mM GTP in 25 mM morpholinepropanesulfonicacid (MOPS; pH 7.1)-1 mM EDTA for 30 min on ice before the additionof 1 mM MgCl₂. Proteins were exchanged into import assay bufferor microinjection buffer, as needed, by size exclusion chromatographyusing Pharmacia PD10columns.

Plasmids. Various recombinant DNAs were used in transfections and transformations, some of which have been described previously (10,41, 53). The following constructs were made specifically forthis study. Vectors encoding a fusion of GFP to the N terminiof various RanBP1 mutants (E37K, G71C/K76E, R91S/K97T, and R92K/D93Y)were constructed by digesting the appropriate pGEX-RanBP1 plasmidswith BamHI and EcoRI and ligating the insert into the same restrictionsites of the pKGFP vector (10). pKGFP-GFP-RanBP1 was constructedby inserting a BamHI/EcoRI fragment encoding GFP-RanBP1 into pKGFP.A pGEX-importin- $beta$ (45-462) vector was constructed by amplificationof the required fragment of importin $beta$ by the PCR, using 5' and3' primers possessing BamHI and SacI sites, respectively. Theinsert was moved into pGEX-KG to produce a plasmid that encodesGST-importin $beta$ (45-462).

Microinjections. Baby hamster kidney (BHK-21) cells were plated onto Cellocate gridded coverslips (Eppendorf catalog no. 930002046); 48 h later,the growth medium was removed and replaced with Ringer's solution(25 mM HEPES [pH 7.2], 110 mM NaCl, 5 mM KCl, 2 mM CaCl₂, 1 mMMgSO₄, 10 mM glucose, 1 mM KH₂PO₄, 1 mg of bovine serum albumin(BSA)/ml), and the nuclei of the cells were injected with theindicated recombinant proteins and fluorescein isothiocyanate(FITC)-coupled dextran in microinjection buffer (10 mM NaPO₄,70 mM KCl, 1 mM MgCl₂ [pH 7.2]). Cells were then incubated at37°C for 10 to 30 min, fixed, permeabilized, and subjected toimmunofluorescence asdescribed.

Transfections. Plasmid DNAs were transfected into BHK-21 cells by the calcium phosphate method. Cells were grown at 37°C in Dulbecco modifiedEagle medium containing 10% heat-inactivated calf serum and penicillin-streptomycin;24 h posttransfection, the medium was replaced with fresh mediumand incubated at 37°C for another 24 to 48 h. Transfected cellswere either untreated, placed on ice, or incubated in the presenceof 200 nM LMB. After the appropriate treatments, the cells werefixed and permeabilized with 4% paraformaldehyde in phosphate-bufferedsaline (PBS; 137 mM NaCl, 3 mM KCl, 10 mM Na₂HPO₄, 2 mM KH₂PO₄[pH 7.4]) and ice-cold methanol as described previously (10).Fixed cells were then prepared for viewing by fluorescencemicroscopy.

In vitro import assays. Assays using permeabilized cells were performed following established protocols (1), with some modification. BHK-21 cellswere plated onto glass coverslips coated with poly-L-lysine. At20 to 24 h after plating, cells were permeabilized with 0.008%digitonin in assay buffer (AB; 20 mM HEPES-KOH [pH 7.6], potassiumacetate, 80 mM 4 mM magnesium acetate, 250 mM sucrose, 1 mM dithiothreitol)for 5 min on ice. After permeabilization, cells were overlaidwith an energy-regenerating system (10 mM creatine phosphate,50 mg of creatine kinase/ml, 500 µM ATP, 500 µM GTP) and rabbitreticulocyte lysate (Promega catalog no. L4151) or HeLa cell lysateand/or purified recombinant factors, incubated at room temperaturefor 5 to 30 min, washed with AB, fixed with 4% paraformaldehydein PBS at room temperature for 15 min, permeabilized with $-$ 20°Cmethanol for 2 min, and prepared for fluorescence microscopy asdescribedbelow.

Fluorescence microscopy. After fixation and permeabilization, cells which contained GFP fusions were incubated with 10 ng of 4',6-diamidino-2-phenylindole(DAPI)/ml in 3% BSA in PBS for 30 min, mounted onto slides withGel/Mount (Biomeda catalog M01), and viewed with a 60× water immersionlens on a Nikon Diaphot 300 microscope. Images were captured witha Hamamatsu charge-coupled device camera and Openlab software.All other cells were blocked in 3% BSA-PBS; incubated with a 1:500dilution of anti-GST monoclonal antibody (MAb; Santa Cruz catalogSC138), a 1:200 dilution of anti-Ran or 1:200 dilution of anti-RanBP1polyclonal antibody (Santa Cruz catalog SC1159) as primary antibody,and Texas red-conjugated anti-mouse immunoglobulin G (IgG), Texasred-conjugated anti-goat IgG, or FITC-conjugated anti-rabbit IgG(all from Jackson ImmunoResearch Laboratories, diluted 1:500),with DAPI (10 ng/ml); and mounted and viewed as describedabove.

Affinity binding assays and immunoblots. Recombinant GST-importin $beta$ (165 pmol) was bound to GSH-Sepharose beads (55 µl) and incubated with RanBP1 (150 pmol) and Ran:GTP(150 pmol) for 90 min at 4°C, to form a ternary complex. Afterbeing washed with AB, the beads were divided into four aliquotsand incubated with 50 pmol of Crm1 and/or 50 pmol of Ran:GTP ina 12-µl volume for 1 h on ice. The supernatants and beads wereseparated by brief centrifugation. The beads were washed oncein AB. Proteins were denatured by boiling with sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE) buffer andseparated by electrophoresis on SDS-12% gels. After transfer tonitrocellulose, the proteins were detected by immunoblotting withanti-Crm1 (1:1,000), anti-RanBP1 (1:200), or anti-Ran (1:2,500)antibody and with horseradish peroxidase-coupled secondary antibodies.Detection was by enhancedchemiluminescence.

Recombinant GST-RanBP1 wild type or mutants (20 pmol) were bound to GSH-Sepharose (40 µl) and incubated with 20 pmol eachof Ran:GTP and importin $beta$ at 4°C for 90 min at 1,400 rpm. Beadswere then washed twice with Ran binding buffer (20 mM MOPS [pH7.1], 100 mM potassium acetate, 5 mM magnesium acetate, 5 mM dithiothreitol,0.5% BSA, 0.05% Tween 20). Bead-bound proteins were treated asabove, immunoblotted with anti-Ran (1:2,500) and anti-importin $beta$ (1:2,000) or anti-GST (1:4,000) with HRP-horseradish peroxidase-conjugatedanti-mouse IgG, and detected by enhanced chemiluminescence. Nucleoporinswere immunoblotted with MAb 414 (BAbCo, Richmond, Calif.), andimportin $beta$ was detected using an antibody from TransductionLaboratories.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Inhibition of nuclear export results in the nuclear accumulation of RanBP1 and GFP-RanBP1. LMB can bind to the karyopherin family member, Crm1, and specifically inhibit export from the nucleus of proteins that containleucine-rich NES sequences (21, 22, 34, 44). RanBP1 containssuch an NES near its C terminus (53, 68). If RanBP1 shuttlesconstitutively between the nuclear and cytoplasmic compartments,LMB should inhibit its export but not its import and cause nuclearaccumulation of the protein. However, if during interphase RanBP1were retained in the cytosol by association with a constitutivelycytosolic protein, LMB would have no effect on the subcellularlocation ofRanBP1.

We tested these alternate hypotheses in two ways. First, BHK cells were incubated for 30 min with or without 200 nM LMB andthen fixed and stained for endogenous RanBP1. The RanBP1 in controlcells was localized exclusively to the cytosol. LMB treatmentled to a substantial redistribution into the nuclei (Fig. 1a).As a second approach, BHK cells were transiently transfected witha vector encoding GFP-RanBP1. Treatment with LMB led to a significantredistribution of the GFP fluorescent signal from the cytosolto the nucleus (Fig. 1b). Importantly, this effect was not a nonspecificresult of LMB treatment, which under similar conditions (60-minpreincubation) did not inhibit import of a microinjected NLS cargo,GST-GFP-NLS (data not shown). Thus, inhibition of Crm1-mediatednuclear protein export results in the accumulation of RanBP1 withinthe nucleus. Moreover, the size of the GFP-RanBP1 fusion protein(approximately 50 kDa) is large enough that its nuclear importis unlikely to occur by simple diffusion within the time frameof the experiment. To confirm that import is not diffusive, weconstructed a GFP-GFP-RanBP1 fusion protein (approximately 75kDa), which also redistributed into the nuclei of cells treatedas above with LMB (Fig. 1c).

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FIG. 1. RanBP1 is able to accumulate in the nucleus in the presence of LMB. BHK-21 cells were either untransfected (a panels) or transfected with pKGFP-RanBP1 (b panels) or pKGFP-GFP-RanBP1 (c panels); 72 h posttransfection, cells were either untreated or incubated with 200 nM LMB for 30 min at 37°C. Cells expressing GFP fusion proteins were fixed, permeabilized, and stained with DAPI. Untransfected cell cultures were fixed, permeabilized, and stained with anti-RanBP1 and Texas red-conjugated secondary antibody as described in Materials and Methods.

Low temperatures inhibit RanBP1 nuclear import. The estimated upper bound for the passive diffusion of proteins through the nuclear pores has been estimated to be about 50kDa. Therefore, RanBP1 at 23 kDa is in principle small enoughto diffuse into the nucleus. However, other proteins of similarsize, such as ribosomal proteins, histones, and Ran, have beenfound to be transported as complexes with other factors (9,33, 51, 59). Passive diffusion rates vary linearly withthe absolute temperature and so are relatively insensitive tothe effect of cooling on ice. Therefore, we tested whether chillingwould abrogate the nuclear accumulation of RanBP1 in the absenceor presence of LMB. BHK-21 cells were cooled on ice for 30 minand then incubated with or without 200 nM LMB for a further 30min on ice. LMB did not cause nuclear accumulation of endogenousRanBP1 (Fig. 2b) or of GFP-RanBP1 (Fig. 2d) under these conditions,suggesting that RanBP1 import does not occur by a process of passivediffusion through the nuclear pores. In interpreting these data,it should be appreciated that chilling the cells will reduce therates of both Ran:GTP formation and consumption. Therefore, inhibitionof RanBP1 import by cooling is unlikely to result from reducedlevels of nuclear Ran:GTP. In this context, it is also importantto note that chilling to 4°C completely inhibits export of a microinjectedGST-GFP-NES cargo (data not shown) so that even in the absenceof LMB, RanBP1 that entered the nuclei by simple diffusion wouldnot be reexported.

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FIG. 2. Nuclear import of RanBP1 is inhibited by incubation on ice. BHK-21 cells were either mock transfected (a and b) or transfected with pKGFP-RanBP1 (c and d); 72 h posttransfection, cells were either incubated on ice for 1 h or incubated on ice for 30 min and then treated with 200 nM LMB for an additional 30 min on ice. Cells expressing GFP fusion proteins were stained with DAPI. Mock-transfected cell cultures were stained with anti-RanBP1 and Texas red-conjugated secondary antibody as described in Materials and Methods.

Collapse of the Ran gradient causes equilibration of RanBP1 across the nuclear envelope. The nucleocytoplasmic Ran:GTP gradient is essential for many types of traffic through the nuclear pores, including proteinimport and export. Collapse of the Ran gradient might thereforebe predicted to curtail RanBP1 export and permit its accumulationin the nucleus. However, if Ran:GTP were required for import,the loss of nuclear Ran:GTP could conceivably prevent such accumulation.To distinguish between these possibilities, we collapsed the Ran:GTPgradient by microinjecting nuclei of BHK cells with recombinantRanGAP. At high concentrations, the GAP can destroy Ran:GTP fasterthan it is produced by RCC1 and thus inhibit nuclear protein export(32). As shown in Fig. 3b, this treatment also resulted in theequilibration of RanBP1 across the nuclear envelope. RecombinantRan, injected as a negative control, had no effect on RanBP1 localization(Fig. 3a) and demonstrated that the nuclear fluorescence in cellsinjected with RanGAP is not a result of bleed-through into thered channel of emission from the FITC-dextran marker. Togetherwith the previous results, these data confirm that RanBP1 canshuttle between the cytoplasmic and nuclear compartments and thatthe import of RanBP1 is Ran independent while export is Ran dependent.

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FIG. 3. Collapse of the nucleocytoplasmic Ran gradient causes an equilibration of RanBP1 across the nuclear envelope. The nuclei of BHK-21 cells were microinjected with FITC-dextran (0.2 mg/ml) as a site-of-injection marker (left) along with either wild-type (WT) Ran (1.0 mg/ml; a panels) or RanGAP (0.4 mg/ml; b panels) and incubated for 10 min at 37°C. The intracellular distribution of endogenous RanBP1 was assessed by indirect immunofluorescence (IF) with anti-RanBP1 and Texas red-conjugated to anti-goat IgG (right) as described in Materials and Methods. Arrows are drawn to help distinguish injected cells from uninjected cells.

Microinjected GST-RanBP1 lacking an NES can accumulate in the nucleus. The previous experiments to demonstrate nuclear import of RanBP1 depended on perturbations in normal cell function $---$ eitherinhibition of the protein export pathway or collapse of the Rangradient. One might argue, therefore, that RanBP1 does not usuallyenter the nucleus but is induced to do so only in response toa disruption in the normal nucleocytoplasmic traffic. To testthis possibility, we microinjected into the cytosol of BHK-21cells a GST-RanBP1(1-161) fusion protein that contains an intactRanBD but lacks the C-terminal NES (53). Within 15 min, accumulationof this protein was visible within the nuclei of a significantfraction of the injected cells (Fig. 4).

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FIG. 4. GST-RanBP1(1-161) is imported into the nucleus. The C-terminal truncation mutant of RanBP1, which lacks the NES, was expressed as a GST fusion protein and injected at a concentration of 1.0 mg/ml into the cytosol of BHK-21 cells, together with FITC-dextran (2.0 mg/ml) as an injection site marker. After 15 min incubation at 37°C, the cells were fixed and stained for GST. A gallery of injected cells is shown.

Therefore, the RanBP1 RanBD is capable of nuclear entry and accumulation even in cells in which nuclear transport has notbeen perturbed. Taken together with results of the other experimentsdescribed above, these data suggest that nuclear import of RanBP1is an ongoing process in interphase cells and that the steady-statecytoplasmic distribution of RanBP1 requires activeexport.

Curiously, the rate of import of GST-RanBP1(1-161) was not uniform. Within a group of cells injected within several secondsof one another, there were often single cells that did not accumulatethe fusion protein within their nuclei, at least within the shortincubation times permitted (e.g., Fig. 4, top panel). The reasonfor this heterogeneity of response is unclear atpresent.

Nuclear accumulation of RanBP1 requires energy and soluble factors. To determine the mechanism by which RanBP1 enters the nucleus, we used digitonin-permeabilized cells that were competent fornuclear protein transport. As a substrate we used GST-RanBP1(1-161).After incubation with the cells, the fusion protein was detectedby immunofluorescence with anti-GST antibodies. GST-RanBP1(1-161),either alone or with an ATP/GTP-regenerating system, did not accumulatein the nuclei (Fig. 5A, panel a). Similarly, the addition of reticulocytelysate as a source of soluble factors did not, in the absenceof energy, lead to accumulation of the RanBP1 construct (panelb). However, rapid accumulation did occur when both reticulocytelysate and energy were provided (panel c). A similar result wasobtained when full-length GST-RanBP1 was used in this assay, inthe presence of LMB to inhibit export, although some nuclear accumulationof the GST-RanBP1 was detectable even in the absence of energy(data not shown).

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FIG. 5. Nuclear accumulation of GST-RanBP1(1-161) requires addition of energy and soluble factors. (A) BHK-21 cells were permeabilized with 0.008% digitonin and overlaid with 3 µM GST-RanBP1(1-161) and either an ATP/GTP-regenerating system (a), reticulocyte lysate (Retic; b), or reticulocyte lysate and ATP/GTP-regenerating system (c). The cells were incubated at room temperature for 30 min and then fixed and stained for GST. Nuclei were stained with DAPI (right). (B) Import of GST-RanBP1(1-161) is not an artifact of damaged nuclear envelopes. Import was performed as for panel A, using either digitonin-permeabilized (a and c) or Triton X-100-extracted (b) cells. Following fixation, the cells were either incubated directly with anti-GST antibody (c) or first incubated with methanol ( $-$ 20°C) to dissolve the nuclear membrane (a and b).

These data indicate that the nuclear accumulation of RanBP1 is an active process. However, in vitro nuclear transport assaysdepend critically on the integrity of the nuclear envelope. Ifthe envelope is damaged and the import substrate binds to insolublenuclear components, then false positives can arise. To validateour import assay, we added GST-RanBP1(1-161), plus energy andreticulocyte lysate, to cells that had been deliberately damagedby addition of 0.2% Triton X-100, which dissolves the nuclearenvelope. As shown in Fig. 5B (panels a and b), this treatmentdid not result in the binding of the RanBP1 to insoluble nuclearcomponents. Second, we tested whether the nuclei of the digitonin-permeabilizedcells were accessible to antibodies by performing an import assayusing GST-RanBP1(1-161) as described above except that after fixation,the membranes were not dissolved with methanol. Under these conditions,the anti-GST antibody could not gain access to the nuclei to stainthe substrate (panel c), whereas staining was efficient when thecells were treated with methanol (panel a). These tests demonstratethat the digitonin-permeabilized cells used in the assay possessintact nuclear envelopes and that damage to the envelopes doesnot result in a falsepositive.

To determine which soluble factors are required for nuclear accumulation of the GST-RanBP1(1-161), the fusion protein wasadded to permeabilized cells together with various combinationsof recombinant transport factors. As shown in Fig. 6A, the additionof Ran plus an energy source led to a small amount of nuclearaccumulation (panel e), which was substantially increased by theaddition of the transport receptor, importin $beta$ (panel h). Thereare at least two possible interpretations of this result. First,RanBP1 may be imported like a more classical transport substrate,in a complex with importin $beta$ and Ran:GDP (12). Second, RanBP1may translocate across the nuclear pores by itself, or with Ran,and accumulate in the nucleus as a ternary complex with Ran:GTPand importin $beta$ .

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FIG. 6. Nuclear accumulation of GST-RanBP1(1-161) requires energy, Ran plus importin $beta$ , or RCC1. (A) BHK-21 cells were permeabilized with digitonin and overlaid with an energy-regenerating system and different combinations of the following factors: 3 µM GST-RanBP1(1-161), 3 µM wild-type (WT) Ran, 3 µM importin (imp) $beta$ , and 3 µM RCC1. Cells were incubated at room temperature for 30 min and then fixed and stained for GST. (B) Loss of importin $beta$ from permeabilized cells. Cells were solubilized in SDS buffer either before or after permeabilization with digitonin, and samples were analyzed by SDS-PAGE followed by immunoblotting with antibodies against either importin $beta$ or glycosylated nucleoporins (MAb 414).

To begin to distinguish between these possibilities, we tested whether the Ran exchange factor, RCC1, could stimulate RanBP1import in the absence of exogenous importin- $beta$ (Fig. 6A, paneli). We chose RCC1 because it is rapidly accumulated within nuclei(M. E. Nemergut and I. G. Macara, submitted for publication),where it efficiently drives the formation of Ran:GTP. It doesnot bind RanBP1 directly, although RanBP1 can inhibit catalysisof nucleotide exchange by RCC1 (6). Interestingly, the RCC1did significantly elevate the nuclear accumulation of GST-RanBP1(1-161)(panel i). Neither importin $beta$ nor RCC1 in the absence of Ran wasable to mediate import to a significant level (panels f and g).Note that during preparation, the permeabilized cells are depletedof the majority of their endogenous importin $beta$ , compared to thelevel of nucleoporins detected by MAb 414 (Fig. 6B), and the residualimportin $beta$ is insufficient to drive the nuclear accumulation ofa classical NLS (data not shown). Therefore, nuclear accumulationof RanBP1 in vitro may require Ran:GTP, but the addition of akaryopherin such as importin $beta$ is not essential (although importin- $beta$ can enhanceaccumulation).

Taken together, these results suggest that RanBP1 can enter the nucleus either as a complex with Ran or by a factor-independentmechanism and is then sequestered within the nucleus by bindingRan:GTP or by the formation of a ternary complex with Ran andimportin $beta$ (or otherkaryopherins).

RanBP1 accumulation in the nucleus requires Ran:GTP. To further distinguish between these possibilities, we tested whether import of GST-RanBP1(1-161) was inhibitable by dominantinterfering mutants of Ran and importin $beta$ or wheat germ agglutinin(WGA), each of which blocks classical, receptor-mediated transportthrough the nuclear pores. WGA and the dominant interfering mutantof importin $beta$ both substantially reduced the extent of import(Fig. 7A panels h and j), and consistent with previous results,the removal of energy by addition of apyrase also prevented accumulationof the GST-RanBP1(1-161), indicating that it is an active process(panel g). However, the addition of Ran(G19V) had no inhibitoryeffect, although it completely blocked import of the control substrate,GST-GFP-NLS (Fig. 7A, panel i; Fig. 7B). This result suggeststhat RanBP1 does not enter the nucleus as a complex with Ran:GDPand importin $beta$ .

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FIG. 7. Inhibitors of the NLS pathway do not inhibit GST-RanBP1(1-161) import. (A) BHK-21 cells were permeabilized with 0.008% digitonin and overlaid with either 1.5 µM GST-GFP-NLS (a to e) or 3 µM GST-RanBP1(1-161) (f to j) in the presence of an energy-regenerating system, reticulocyte lysate (Retic), 100 U of apyrase/ml, 2 µM importin (imp) $beta$ (45-462)), 100 mg of RanG19V/ml, or 200 mg of WGA/ml. Cells were incubated at 23°C for 30 min and then fixed. GST-GFP-NLS and GST-RanBP1(1-161) were detected by epifluorescence and by indirect immunofluorescence with anti-GST MAb, respectively. (B) The average total fluorescence per cell of GST-RanBP1(1-161) was quantitated using Openlab software. Error bars represent the standard error of the mean (n > 20 cells per treatment).

It is important to note that WGA and importin $beta$ (45-462) also block Ran import (51, 59) and do not, therefore, distinguishwhether the observed inhibition is of RanBP1 translocation acrossthe nuclear pores or of RanBP1 accumulation within the nucleus.It is also of note that although Ran normally enters the nucleusas a complex with GDP, the Ran(G19V) mutant, which is predominantlyGTP bound, can accumulate both within the nucleoplasm and at thenuclear pores (39).

Taken together, these data support the idea that Ran:GTP is required for nuclear accumulation of GST-RanBP1(1-161). To testthis hypothesis further, we performed in vitro import assays usingvarious concentrations of Ran at a fixed concentration of GST-RanBP1(1-161)and RCC1. After fixation, the cells were stained for both GSTand Ran. We observed that the fluorescence intensity of the nuclearGST-RanBP1(1-161) correlated quite well with the nuclear Ran fluorescence(Fig. 8A). We then quantitated the relative nuclear fluorescencelevels of GST-RanBP1(1-161) in individual cells and plotted themean values against the Ran concentration added to the cells (Fig.8B). The GST-RanBP1(1-161) levels show a strong linear correlationwith the Ran concentration (linear correlation coefficient [r]= 0.967). The most likely explanation of this result is that GST-RanBP1(1-161)enters the nucleus alone, by a process of facilitated diffusion,and that association with Ran:GTP within the nucleus preventsits export. Alternatively, the RanBP1 may enter as a complex withRan:GTP, and become trapped within the nucleus by associationwith other factors.

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FIG. 8. Nuclear accumulation of GST-RanBP1(1-161) is mediated by Ran:GTP. (A) Digitonin-permeabilized BHK-21 cells were incubated with Ran, RCC1, and an energy-regenerating system as for Fig. 6. GST-RanBP1(1-161) was detected using anti-GST and an anti-mouse conjugated to Texas red; Ran was detected with anti-Ran and an anti-rabbit antibody conjugated to FITC. WT, wild type. (B) Import assays were performed at a variety of Ran concentrations as in panel A. Images were captured; the average total fluorescence per cell of GST-RanBP1(1-161) was quantitated for different assays using Openlab software as described in Materials and Methods and plotted against the Ran concentration. Values are shown ± standard error of the mean (n = 20). The line was drawn using a least squares algorithm. Correlation coefficient, r = 0.967.

A RanBP1 mutant is defective in nuclear import. To distinguish between these two hypotheses, we examined a number of RanBP1 variants that we had previously generated usinga random mutagenesis approach (47). We chose two mutants thateach exhibit a substantially reduced affinity for Ran:GTP (Fig.9A). One mutant contains a single residue substitution, E37K,and the other is a double mutant, G71C/K76E. Both mutants possessthe unusual property that they can form stable ternary complexeswith Ran:GTP plus either importin 5 (47) or importin $beta$ (Fig.9B).

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FIG. 9. An E37K mutant of RanBP1 does not import into nuclei but can form a ternary complex with Ran:GTP and importin $beta$ . (A) Equimolar amounts of recombinant wild-type or mutant GST-RanBP1s were spotted onto nitrocellulose and incubated with Ran (8 nM) loaded with [ $gamma$ -³²P]GTP for 30 min as described in Materials and Methods, washed, and exposed to film with an intensifying screen at $-$ 80°C for 1 h. (B) GST-RanBP1 fusion proteins on GSH-Sepharose beads were incubated with importin $beta$ plus Ran. Bound proteins were washed, separated by SDS-PAGE, and immunoblotted for Ran and importin $beta$ or GST to show that equivalent amounts of the RanBP1 mutants bound to GSH-Sepharose. Molecular weight markers (in kilodaltons) are shown on the left. (C) BHK-21 cells were transfected with wild-type or mutant GFP-RanBP1 plasmids and treated with 200 nM LMB for 30 min, as in Fig. 1, prior to fixation. (D) GFP-BP1(E37K) was transfected into BHK-21 cells. The cells were then either incubated on ice for 1 h or incubated on ice for 30 min and then treated with 200 nM LMB for an additional 30 min on ice. Fixed cells were stained with DAPI. (E) The C-terminal truncation mutant of Ran BP1(E37K), which lacks the NES, was expressed as a GST fusion protein and injected into the cytosol of BHK-21 cells at a concentration of 1.0 mg/ml along with 2.0 mg of FITC-dextran/ml as a site-of-injection marker. After 15 min of incubation at 37°C, the cells fixed and stained for GST.

The two mutants were expressed ectopically as GFP fusions in BHK-21 cells, and their ability to enter the nucleus was testedby the addition of LMB, to block export. In the absence of LMB,both mutants localized exclusively to the cytosol (Fig. 9C, panelsb and c). Surprisingly, however, they behaved differently in thepresence of LMB. The G71C/K76E mutant accumulated within the nucleusto a degree similar to that of the wild-type protein, but theE37K mutant remained excluded from the nucleus (panels e and f).Importantly, at 4°C in the presence of LMB, the GFP-RanBP1(E37K)did not equilibrate across the nuclear envelope, as would be expectedif accumulation, rather than transport, were defective (Fig. 9D,panel b). Additionally, a GST-RanBP1(1-161,E37K) recombinant proteinwas excluded from the nucleus when microinjected into the cytoplasmof BHK-21 cells (Fig. 9E), unlike the control GST-RanBP1(1-161)protein (Fig. 4). Four other mutants of RanBP1 that were testedall behaved like the G71E/K76E mutant and wild-type RanBP1, accumulatingin the nuclei of LMB-treated cells (data notshown).

These results suggest that the translocation of RanBP1 into the nucleus most likely occurs in the absence of association withRan:GTP and confirm that import occurs by a specific, facilitatedpathway rather than by simple diffusion. The E37K mutation liesin the N-terminal arm of the RanBD, which embraces Ran:GTP, whilethe other mutations are located in different regions of the bindingdomain. Thus, these results implicate the N-terminal arm of theRanBD in the nuclear transport mechanism ofRanBP1.

Crm1 dissociates RanBP1 from a RanBP1-Ran:GTP-importin $beta$ ternary complex. If RanBP1 can accumulate in the nucleus as a ternary complex with Ran:GTP and importin $beta$ , how is it efficiently exported backto the cytosol? One possibility is that Crm1 exports the entirecomplex; another is that Crm1 displaces importin $beta$ from the complexand exports only the RanBP1. To distinguish between these differentmechanisms, recombinant GST-importin $beta$ was attached to GSH-Sepharosebeads and mixed with Ran:GTP and RanBP1 to form a tethered ternarycomplex on the beads. After washing to remove free Ran and RanBP1,the beads were incubated either with buffer or with purified Crm1(29). The beads and eluate were then analyzed by immunoblottingfor Ran, RanBP1, and Crm1. As shown in Fig. 10, incubation withCrm1 led to release into the eluate of a substantial fractionof the RanBP1 and of the Ran from the GST-importin $beta$ . No Crm1was found to be associated with the complex on the Sepharose beads.Therefore, we conclude that Crm1 promotes the dissociation ofRan and RanBP1 from importin $beta$ , or sequesters free Ran and RanBP1,which drives dissociation from the importin $beta$ by mass action.In either case, the Crm1 appears unable to form a complex withRan and RanBP1 that includes importin $beta$ .

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FIG. 10. Crm1 dissociates RanBP1 and Ran from a RanBP1-Ran-importin $beta$ complex. GST-importin $beta$ was bound to GSH-Sepharose and incubated with RanBP1 and Ran. Uncomplexed proteins were washed away. The bead-bound complex was then incubated on ice with either buffer, Ran, or Crm1 (29). The eluate and beads were collected separately, subjected to SDS-PAGE, transferred to nitrocellulose, and immunoblotted for Crm1 (top), RanBP1 (middle), and Ran (bottom). Purified proteins were run alongside the beads and eluates as standards.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

One of the hallmarks of the nuclear transport machinery is the asymmetric distribution of its soluble components. The Ran:GTPgradient across the nuclear pores is critical to many forms ofprotein and nucleic acid transport, and the dissociation of transportcomplexes in the cytosol requires both RanGAP and RanBP1. It istherefore essential to understand how the asymmetric distributionof transport factors is initiated and maintained. Ran:GDP importhas been demonstrated to be mediated by NTF2 (51, 59). Importin $beta$ and transportin appear able to cross the nuclear pores in theabsence of other factors (35, 43). Importin $alpha$ is recycledback to the cytosol by CAS (37). We now present evidence thatRanBP1 import also occurs via a specific, facilitatedmechanism.

RanBP1 functions as a coactivator of RanGAP and thereby mediates the dissociation of complexes between Ran:GTP and transportreceptors of the importin $beta$ superfamily. This function requiresthat RanBP1 be localized to the cytosol. However, RanBP1 is smallenough, in principle at least, to be able to enter the nucleusby passive diffusion (although the protein behaves in solutionas a dimer [6]). Because RanBP1 binds with nanomolar affinityto Ran:GTP, which is concentrated within the nucleus, and canform a ternary complex with importin $beta$ , which is also predominantlynuclear, a mechanism must exist either to sequester the RanBP1in the cytosol or to actively export it from the nucleus. RanBP1does contain a leucine-rich NES near its C terminus but also containsadjacent sequences that may function in cytosolic retention (53).

We now show that RanBP1 shuttles constitutively between the cytosolic and nuclear compartments and that its cytosolic distributionis actively maintained by nuclear export. It is likely that thisprocess is conserved through evolution, because Yrb1p, the yeasthomologue of RanBP1, though lacking a C-terminal NES, has beenshown to accumulate in the nucleus under conditions in which exportis likely inhibited (27, 56). GST-RanBP1 lacking an NES accumulatesin the nuclei both of intact cells when the protein is microinjectedinto the cytosol and of permeabilized cells in a Ran- and importin $beta$ -dependent fashion that requiresenergy.

Based on the observations that accumulation of RanBP1 in nuclei of intact cells was blocked by cooling the cells on ice, andthat both GFP-GFP-RanBP1 (~75 kDa) and GST-RanBP1(1-161) (~50-kDamonomer; ~100-kDa dimer) were capable of nuclear import, we considerit highly unlikely that RanBP1 transits the pores by simple diffusion.In vitro assays demonstrated that nuclear accumulation of GST-RanBP1(1-161)is active. Accumulation required energy and Ran. However, it isimportant to distinguish the mechanism of translocation throughthe pores from that of the net accumulation of a substrate withinthe nucleoplasm. These are entirely separate processes. Most importassays do not distinguish between them, however. A protein thatcan transit the pores by facilitated diffusion may accumulateagainst a concentration gradient if it binds to a nuclear proteinor is covalently modified $---$ for instance, by phosphorylation $---$ withinthe nucleus in a manner that prevents reexport. If the nuclearprotein partner is imported via a classical pathway, then in vitroassays will display a dependence on energy and soluble factorseven though these are not required for the translocation of thesubstrate itself. In the present case, the in vitro assays showeda strong dependence on Ran:GTP. This factor could be suppliedeither as a constitutively GTP-bound mutant [Ran(G19V)] or byaddition of wild-type Ran plus RCC1. Factors that enhance nuclearaccumulation of Ran, such as importin $beta$ , also enhanced RanBP1accumulation. Factors that inhibit Ran accumulation, such as WGAor a dominant interfering mutant of importin $beta$ , also inhibitedRanBP1 accumulation. Therefore, these assays could not distinguishwhether the GST-RanBP1(1-161) transits the nuclear pores aloneand becomes trapped within the nucleoplasm by binding to Ran:GTPor, alternatively, transits the pores in a complex with Ran:GTP.

We were able to distinguish between these two hypotheses, however, by the use of point mutants of RanBP1. We chose two mutantswith impaired affinity for Ran:GTP, E37K and G71C/K76E (47).Importantly, both of these proteins, which contain altered residueswithin the RanBD, retain the ability to form stable ternary complexeswith karyopherins such as importin $beta$ plus Ran:GTP. Thus, if capableof entering the nucleus, they could in principle become trappedin such a ternary complex and accumulate within the nucleoplasm.When expressed in cells as a GFP fusion protein, the G71C/K76Emutant accumulated within nuclei upon addition of LMB to blockexport. This result is consistent with a model in which RanBP1transits the nuclear pores alone, not as a complex with Ran:GTP.Several other mutants with altered residues within the RanBD werealso capable of nuclear import in the presence of LMB (data notshown). Additionally, Zolotukhin and Felber found that a mutantRanBP1 which is defective in Ran binding and lacks an NES couldstill accumulate in the nucleus of transfected cells (68). Theability of this mutant to form ternary complexes with Ran:GTPand importin $beta$ was not tested, however, and so the mechanism ofnuclear accumulation remains to be determined in thiscase.

Interestingly, we discovered one mutant, E37K, that was incapable of nuclear import under the conditions of the assay anddid not even equilibrate across the nuclear envelope when thecells were held at 4°C. This result confirms that RanBP1 cannotenter the nucleus by passive diffusion but must use a facilitatedmechanism. The E37K mutation lies in the N-terminal arm of theRanBD, and the side chain faces outward into the solvent (62).Therefore, the unique transport defect of RanBP1(E37K) suggeststhat the N-terminal arm of the protein may be involved in nuclearimport, perhaps by binding to nuclear pore components. In an independentstudy, a different group has identified another mutation withinthe RanBP1 of budding yeast (Yrb1p) that is unable to accumulatein nuclei when export is inhibited (Ed Hurt, personal communication).Their data support our conclusion that RanBP1 import does notoccur by simple diffusion and that its nuclear accumulation isenergydependent.

Within the nucleoplasm, RanBP1 probably forms a ternary complex with Ran:GTP and karyopherins such as importin $beta$ or otherbinding proteins. We therefore asked how the RanBP1 could be efficientlyexported. We found that Crm1 cannot bind with measurable affinityto the RanBP1-Ran-importin $beta$ ternary complex, but it facilitatesthe dissociation of RanBP1 and Ran from the complex. This mechanismmay be required to prevent the RanBP1 from being sequestered withinthenucleus.

Based on the data described above, we propose that RanBP1 is continually cycling between the cytosol and nucleus in interphasecells and that import occurs via a specific, nondiffusive pathwaythat does not require soluble factors such as the karyopherinsand that involves the N-terminal arm of the RanBD. Accumulationwithin the nucleus against a concentration gradient can occurif the NES of RanBP1 is deleted or if export is inactivated. Accumulationis driven by binding to nuclear Ran:GTP, and most likely by theformation of ternary complexes with Ran:GTP and karyopherins.Endogenous RanBP1, however, binds to the exportin, Crm1, whichprevents association with other karyopherins. Rapid export ofthe RanBP1 by Crm1 terminates the transportcycle.

The purpose of RanBP1 shuttling remains to be further investigated. However, we speculate that RanBP1 import may help clearthe nuclear pores of Ran:GTP. Ran is sufficiently small that inprinciple it could diffuse through the pores (55, 62). Indeed,NTF2 (the nuclear import receptor for Ran:GDP) is not requiredfor survival of yeast if the expression of Ran is elevated, andthe requirement for NTF2 in nuclear import assays performed onpermeabilized cells can be eliminated by the inclusion of a highRan concentration in the assay buffer (45). Ran:GTP possessesan average molecular size that is very similar to that of Ran:GDP.Therefore Ran:GTP is expected to slowly diffuse out through thenuclear pores at about the same rate that it can diffuse in. Incomingnuclear transport complexes will be dissociated by interactionwith any molecule of Ran:GTP that is encountered within the pore,and such a premature dissociation would most likely cause terminationof the translocation process. By sweeping the pores free of Ran:GTP,RanBP1 may reduce the likelihood that this processoccurs.

	ACKNOWLEDGMENTS

We thank Bryce Paschal and Jim Holaska (University of Virginia) for the kind gifts of purified Crm1 protein and anti-Crm1antiserum, Steve Adam (Northwestern University) for the importin $beta$ cDNA, and Barbara Wolff-Winiski (Novartis) for theLMB.

This work was supported by grant GM 50526 from the National Institutes of Health,DHHS.

	FOOTNOTES

^* Corresponding author. Mailing address: Room 7191 Hospital West, P.O. Box 800577, HSC, University of Virginia School of Medicine,Charlottesville, VA 22908. Phone: (804) 982-0074. Fax: (804) 924-1236.E-mail: imacara{at}virginia.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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45. Paschal, B. M., C. Fritze, T. Guan, and L. Gerace. 1997. High levels of the GTPase Ran/TC4 relieve the requirement for nuclear protein transport factor 2. J. Biol. Chem. 272:21534-21539[Abstract/Free Full Text].

46. Pasquinelli, A. E., M. A. Powers, E. Lund, D. Forbes, and J. E. Dahlberg. 1997. Inhibition of mRNA export in vertebrate cells by nuclear export signal conjugates. Proc. Natl. Acad. Sci. USA 94:14394-14399[Abstract/Free Full Text].

47. Petersen, C., N. Orem, J. Trueheart, J. Thorner, and I. G. Macara. 2000. Random mutagenesis and functional analysis of the Ran binding protein, RanBP1. J. Biol. Chem. 275:4081-4091[Abstract/Free Full Text].

48. Radu, A., G. Blobel, and M. S. Moore. 1995. Identification of a protein complex that is required for nuclear protein import and mediates docking of import substrate to distinct nucleoporins. Proc. Natl. Acad. Sci. USA 92:1769-1773[Abstract/Free Full Text].

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