Ran-unassisted Nuclear Migration of a 97-kD Component of Nuclear Pore-targeting Complex

Shingo Kose, Naoko Imamoto, Taro Tachibana, Takuya Shimamoto, and Yoshihiro Yoneda

Department of Anatomy and Cell Biology, Osaka University Medical School, Suita, Osaka 565, Japan

Abstract
Materials and Methods
Results
Discussion
Footnotes
Acknowledgements
Abbreviations used in this paper
References


Abstract

A 97-kD component of nuclear pore-targeting complex (the beta -subunit of nuclear pore-targeting complex [PTAC]/importin/karyopherin) mediates the import of nuclear localization signal (NLS)-containing proteins by anchoring the NLS receptor protein (the alpha -subunit of PTAC/importin/karyopherin) to the nuclear pore complex (NPC). The import requires a small GTPase Ran, which interacts directly with the beta -subunit. The present study describes an examination of the behavior of the beta -subunit in living cells and in digitonin-permeabilized cells. In living cells, cytoplasmically injected beta -subunit rapidly migrates into the nucleus. The use of deletion mutants reveals that nuclear migration of the beta -subunit requires neither Ran- nor alpha -subunit-binding but only the NPC-binding domain of this molecule, which is also involved in NLS-mediated import. Furthermore, unlike NLS-mediated import, a dominant-negative Ran, defective in GTP-hydrolysis, did not inhibit nuclear migration of the beta -subunit. In the digitonin-permeabilized cell-free import assay, the beta -subunit transits rapidly through the NPC into the nucleus in a saturating manner in the absence of exogenous addition of soluble factors. These results show that the beta -subunit undergoes translocation at the NPC in a Ran-unassisted manner when it does not carry alpha -subunit/NLS substrate. Therefore, a requirement for Ran arises only when the beta -subunit undergoes a translocation reaction together with the alpha -subunit/NLS substrate. The results provide an insight to the yet unsolved question regarding the mechanism by which proteins are directionally transported through the NPC, and the role of Ran in this process.


NUCLEAR pore complexes (NPCs)1 mediate the bidirectional nucleocytoplasmic exchange of molecules via several different mechanisms. Ions, small metabolites, and proteins <20-40 kD in size can passively diffuse through 90-Å aqueous channels that span the NPC. Most macromolecules, which are too large to passively diffuse through the aqueous channels of the NPC, are thought to be transported through gated-channels of the NPC by active mechanisms (for reviews see Fabre and Hurt, 1994; Rout and Wente, 1994; Davis, 1995). These include the nuclear import of nuclear localization signal (NLS)-containing karyophiles and small nuclear RNPs (for reviews see Dingwall and Laskey, 1991; Garcia-Bustos et al., 1991; Goldfarb and Michaud, 1991; Görlich and Mattaj, 1996; Panté and Aebi, 1996), nuclear export of nuclear export signal-containing proteins (for reviews see Gerace, 1995; Görlich and Mattaj, 1996; Panté and Aebi, 1996; Yoneda, 1996) and RNAs (for reviews see Elliott et al., 1994; Izaurralde and Mattaj, 1995), and shuttling proteins, such as heat shock-related proteins (Mandell and Feldherr, 1990) and heterogeneous nuclear RNP A1 (Michael et al., 1995; for reviews see Laskey and Dingwall, 1993; Piñol-Roma and Dreyfuss, 1993). Based on sensitivity to chilling and WGA, the transport of calmodulin has been shown to be facilitated and to occur in an energy-independent manner (Pruschy et al., 1994).

The NLS-mediated import process involves a series of sequential steps, which are mediated by several soluble/ cytoplasmic factors. The import is initiated by NLS-dependent complex formation, termed the nuclear pore-targeting complex (PTAC), in the cytoplasm (Görlich et al., 1995a; Imamoto et al., 1995c). PTAC is a stable protein complex composed of a karyophilic protein and two cytosolic components, which we originally named PTAC58 and PTAC97, based on their molecular masses (Imamoto et al., 1995a,b). These components have also been referred to as importin alpha  and beta  (Görlich et al., 1994, 1995a,b), karyopherin alpha  and beta  (Moroianu et al., 1995a; Radu et al., 1995a), or hSRP1 alpha / NLS receptor (Adam and Gerace, 1991; Weis et al., 1995) as well as nuclear transport factor p97 (Adam and Adam, 1994; Chi et al., 1995). In this report, we will refer to the 58-kD component of PTAC as the alpha -subunit, and the 97-kD component as the beta -subunit. The alpha -subunit directly binds to the NLS of karyophile (Adam and Gerace, 1991; Imamoto et al., 1995b; Moroianu et al., 1995a; Weis et al., 1995) and the beta -subunit to the NH2-terminal portion of the alpha -subunit (Görlich et al., 1996a; Weis et al., 1996). The beta -subunit provides NPC-binding sites for PTAC, since this protein directly interacts with several FXFG or GLFG repeat-containing nucleoporins (Iovine et al., 1995; Kraemer et al., 1995; Radu et al., 1995b). NLS-containing karyophiles target the cytoplasmic face of the NPC with alpha - and beta -subunits as a single entity in the energy-independent stages of NLS-mediated nuclear import.

Subsequent energy-dependent steps of nuclear import, in which karyophiles translocate through gated channels of the NPC to the nuclear interior, have been shown to be mediated by small GTPase Ran, along with a dimeric protein called p10/NTF2 (Melchior et al., 1993; Moore and Blobel, 1993,1994; Paschal and Gerace, 1995). Ran, in its GTP form, has been shown to bind directly to the beta -subunit (Floer and Blobel, 1996; Paschal et al., 1996). Using an in vitro transport assay, it has been shown that the alpha - and beta -subunits dissociate upon NPC translocation and that the alpha -subunit accumulates in the nucleus along with the NLS substrate, while the beta -subunit remains bound to the nucleoplasmic face of the NPC (Görlich et al., 1995b; Moroianu et al., 1995b). Dissociation of the alpha -subunit from the beta -subunit is induced by the binding of GTP-Ran to the beta -subunit (Rexach and Blobel, 1995; Görlich et al., 1996b). Moreover, GTP-Ran causes the dissociation of beta -subunit from FXFG repeat-containing nucleoporins on binding to the beta -subunit (Rexach and Blobel, 1995).

The issue of how proteins actually directionally move through the NPC is not well understood. Several laboratories have carried out experiments directed at explaining the detailed translocation mechanism, and, as a result of these, different translocation models have been proposed. One model proposes that a repeated docking and undocking of PTAC, promoted by GTP-Ran, generates the vectorial movement through the NPC (Rexach and Blobel, 1995), and another proposes that a multi-complex formation between alpha -subunit, beta -subunit, GDP-Ran, and p10 at the central gate of NPC is required for vectorial movement (for reviews see Koepp and Silver, 1996; Nigg, 1997). More recently, Chi et al. (1996) proposed that multi-complex formation between alpha -subunit, beta -subunit, GDP-Ran, and RanBP1 at the central gate of the NPC is required for vectorial movement. Görlich et al. (1996b) proposed that the asymmetric distribution of GDP- and GTP-Ran in the cytoplasm and nucleoplasm contributes to the vectorial movement. In all cases, Ran has been proposed to play a key role in translocating the NLS-containing karyophile through the NPC with directionality, although its exact action remains to be elucidated.

Meanwhile, distantly related beta -subunit homologues have been identified from mammalian and yeast sources that mediate different transport pathways. One of these, termed transportin or karyopherin beta 2, has been shown to mediate the import of heterogeneous nuclear RNP A1, by binding directly to a novel NLS of this protein named the M9 sequence (Pollard et al., 1996; Bonifaci et al., 1997). Karyopherin beta 3 was shown to bind to ribosomal proteins, and it has been suggested that it mediates the nuclear transport of ribosomal proteins (Yaseen and Blobel, 1997). In yeast, three beta -subunit homologues have been identified from the yeast genome database. One of these, termed Kap104, was shown to bind directly to yeast mRNA binding proteins, termed Nab2p and Nab4p, and has been proposed to mediate the nuclear transport of these proteins (Aitchison et al., 1996). Neither of these beta -subunit homologues associates with the alpha -subunit. All of the beta -subunit homologues were shown to interact directly with NPC components, but not all of them bind directly to Ran (Yaseen and Blobel, 1997). Therefore, the issue of which of the interactions among transport factors is sufficient to exert the movement of molecules through NPC remains unclear.

In the present study, we examined the behavior of the beta -subunit and found that it can undergo NPC translocation in both a Ran-assisted and -unassisted manner. The beta -subunit, which is distributed throughout the cytoplasm and nucleus, rapidly migrates into the nucleus when injected into the cytoplasm of living cells. The use of deletion mutants, which lack the ability to bind alpha -subunit, GTP-Ran, or both, reveals that this protein migrates into the nucleus without binding to either alpha -subunit or GTP-Ran but requires its own NPC-binding domain, which possesses necessary and sufficient information to directionally translocate NPC. Moreover, dominant-negative Ran, defective in GTP hydrolysis, failed to inhibit nuclear migration of beta -subunit in living cells. In the digitonin-permeabilized cell-free transport assay, the beta -subunit moves rapidly through the NPC into the nucleus in the absence of exogenous addition of soluble factors. The data collected herein show that, in marked contrast to NLS-mediated import, which occurs when the beta -subunit carries alpha -subunit and bound NLS substrate, Ran is not required when the beta -subunit undergoes translocation through the NPC without carrying alpha -subunit/NLS substrate. Sensitivity to WGA and saturability of import show that the beta -subunit migrates into the nucleus through gated channels of the NPC via specific molecular interactions of the NPC-binding domain of the beta -subunit with NPC components.


Materials and Methods

Cell Culture

Madin-Darby bovine kidney (MDBK) cells and human embryonic lung (HEL) cells were incubated in DME containing 10% bovine serum. MDBK cells were plated on 8-well multi-test slides 12-24 h before use for cell-free import assays.

Microinjection

HEL cells were plated on marked coverslips, and microinjection experiments were performed as described previously (Yoneda et al., 1987). After injection and incubation, cells were fixed with 3.7% formaldehyde in PBS (137 mM NaCl, 2.7 mM KCl, 8.1 mM Na2HPO4, 1.5 mM KH2PO4, pH 7.2). The injected fluorescently labeled proteins were detected by fluorescent microscopy (Axiophot; Carl Zeiss, Inc., Thornwood, NY) or confocal laser scanning microscopy (Carl Zeiss, Inc.). Confocal images were collected using x63 objective, and the final figures were produced using Adobe Photoshop (Adobe Systems, Inc., Mountain View, CA).

Expression and Purification of Recombinant Proteins

An epitope-tagged beta -subunit was constructed in a glutathione-S-transferase (GST) gene fusion vector pGEX-2T (Pharmacia Biotech, Inc., Piscataway, NJ) as described previously (Imamoto et al., 1995a). This vector is referred to as the pGEX HA-PTAC97. The expression vectors of the D769-876 and D644-876 mutants were constructed from the pGEX HA-PTAC97 by cutting out the HindIII-KpnI and EcoRI-KpnI fragments, respectively, followed by blunting and ligation. The expression vectors of the D3-145 and D3-447 mutants were constructed from pGEX HA-PTAC97 by cutting out the SacI-NdeI and SacI-AccI fragments, respectively, followed by blunting and ligation with the NotI linker (AGCGGCCGCT). To construct the expression vector of the D450-876 mutant, an NdeI-AccI (KpnI) fragment, which is 145-449 amino acids of beta -subunit, was amplified from the pGEX HA-PTAC97 by PCR using the synthetic oligonucleotides (5'-TTGGGGAGCTCGAGCATATGAAAGAGTCCACATTGG-3' and 5'-GAAAAGGTACCAGGTAGACATCGTTGATGGCGGCTTC-3') which incorporate a KpnI site after an AccI site. After digesting with NdeI and KpnI, this PCR product was inserted into NdeI and KpnI sites of pGEX HA-PTAC97. These resultant plasmids were sequenced to confirm the fidelity of the region of amplification by PCR and in-frame ligation of the fused region.

The green fluorescent protein (GFP) chimeras of recombinant beta -subunit or deletion mutants were generated as follows. The fragment encoding the entire amino acids of GFP and amino acids 1-3 of beta -subunit was amplified from pS65T-C1 (#6089-1; Clonetech Laboratories, Palo Alto, CA) by PCR using the synthetic oligonucleotides (5'-CCGTAAGATCTATGAGTAAAGGAGAAGAACTTTTC-3' and 5'-CCGTTGAGCTCCATGGATCCTTTGTATAGTTCATCCATGCC-3') which incorporate a BglII site in frame followed by a start codon of GFP. The amplified PCR product was digested with BglII and SacI, followed by incorporating into the BamHI and SacI sites of the pGEX HA-PTAC97 or the expression vector of GST-fused deletion mutants (D450-876 and D3-447) of beta -subunit described above.

The resultant expression vectors were transformed into Escherichia coli strain BL21(DE3). The E. coli cells were grown in LB medium containing 50 µg/ml ampicillin at 37°C to a density of 1.2 (OD550). Expression was induced by addition of 1 mM isopropyl-beta -D-thiogalactopyranoside (IPTG) and incubation for 14 h at 20°C, except that the D450-876 chimeras were induced by addition of 0.1 mM IPTG. Lysis of bacteria and purification of the fusion protein with glutathione-Sepharose were performed as described previously (Imamoto et al., 1995a). The GST portion of chimeras was cleaved off by a 2 h incubation at room temperature with 1 NIH unit of thrombin (Sigma Chemical Co., St. Louis, MO) per 100 µg of chimeras. GST and thrombin were separated from recombinant proteins on a MonoQ column (Pharmacia Biotech, Inc.) at flow rate of 0.5 ml/min with a linear gradient from 0.05 to 1.0 M NaCl in 20 mM Hepes, pH 7.3, 2 mM DTT, 1 µg/ml each of aprotinin, leupeptin, and pepstatin. The recombinant proteins were dialyzed against 20 mM Hepes, pH 7.3, 100 mM potassium acetate, 2 mM DTT, and 1 µg/ml each of aprotinin, leupeptin, and pepstatin.

E. coli strain BL21 (DE3) expressing human Ran was kindly provided by Dr. T. Nishimoto (Graduate School of Medical Science, Kyushu University, Fukuoka, Japan). The recombinant wild-type Ran and G19V Ran were expressed, purified, and charged with GTP or GDP based on methods described previously (Dasso et al., 1994; Sekimoto et al., 1996). The GST- alpha -subunit was expressed and purified as described previously (Imamoto et al., 1995b). Aliquots of each recombinant protein were frozen in liquid nitrogen and stored at -80°C.

Antibodies

The GST-beta -subunit, purified on a glutathione-Sepharose column, was used to immunize two rabbits. Immunizations were performed as described previously (Imamoto et al., 1995b). Anti-beta -subunit antibodies were performed independently from anti-serum of each rabbit, by first depleting the antiserum of anti-GST antibodies by passage over GST affinity columns and then on recombinant beta -subunit-conjugated Sepharose. Antibodies bound to beta -subunit-Sepharose were eluted with 0.1 M glycine-HCl (pH 2.5) and neutralized. After dialysis against phosphate buffer (pH 7.2) containing 0.3 M NaCl, the antibodies were further incubated with GST-Sepharose to absorb residual traces of anti-GST antibodies. Preimmune IgG fraction was obtained by two cycle precipitation with 40% saturated ammonium sulfate.

Indirect Immunofluorescence

HEL cells and MDBK cells, plated on coverslips, were washed twice in PBS and fixed with 3.7% formaldehyde in PBS (room temperature for 20 min). After permeabilization with 0.5% Triton X-100 in PBS (room temperature for 5 min), cells were incubated with 10 µg/ml of affinity-purified anti-beta -subunit antibodies for 1.5 h at room temperature. Rabbit antibodies were detected with FITC-conjugated goat antibodies to rabbit IgG (Tago Inc., Burlingame, CA). The samples were examined using an Axiophot microscope (Carl Zeiss, Inc.). For the confocal experiments, cells were treated identically. Images were collected using x63 objective on the Zeiss confocal laser scanning microscope (Carl Zeiss, Inc.), and the final figure was produced using Adobe Photoshop (Adobe Systems, Inc., Mountain View, CA).

Preparation of NLS-containing Transport Substrates

Allophycocyanin (APC; Calbiochem-Novabiochem Corp., La Jolla, CA) and biotinylated bovine serum albumin (bBSA) were chemically conjugated to synthetic peptide containing the amino acid sequence of SV40 large T-antigen NLS (CYGGPKKKRKVEDP), as described previously (Imamoto et al., 1995a).

Solution Binding Assay

The ability of the deletion mutant proteins to form a complex with the alpha -subunit and biotin-labeled SV40 T-antigen NLS conjugate (T-bBSA; Imamoto et al., 1995a) was examined in the solution binding assay. The amounts of mutant proteins incorporated into the complex correspond to those that directly bind to the alpha -subunit, since beta -subunit does not directly associate with the NLS substrate (Imamoto et al., 1995a). Binding assays were performed in transport buffer (TB: 20 mM Hepes, pH 7.3, 110 mM potassium acetate, 2 mM magnesium acetate, 5 mM sodium acetate, 1 mM glycoletherdiaminetetraacetic acid [EGTA], 2 mM DTT, and 1 µg/ml each of aprotinin, leupeptin, and pepstatin) in a final volume of 100 µl. Recombinant GST chimeras of beta -subunit or deletion mutants were incubated with alpha -subunit and T-bBSA (0.25 mg/ml) for 1 h on ice. The solution was then incubated for 1 h at 4°C with 30 µl of immobilized avidin (Pierce, Rockford, IL), which was washed with TB and resuspended in a 50% slurry. The immobilized avidin was collected by centrifugation and washed five times by resuspension in 0.5 ml of TB. The bound proteins were eluted from immobilized avidin by a 30-min incubation at 37°C with 30 µl of the elution buffer (0.2% SDS, TE, pH 8.0). The eluted proteins were resolved by SDS-PAGE. The intensity of protein bands, stained with coomassie brilliant blue, was quantified by densitometric scanning (CS-930; Shimazu, Kyoto, Japan). The molar ratio of beta -subunit or deletion mutant proteins bound to alpha -subunit was estimated by dividing the intensity of the protein bands by the molecular mass of each protein.

Ran Overlay Assay

Direct binding of beta -subunit to GTP-Ran was performed using an overlay assay, based on methodology described by Lounsbury et al. (1994). Recombinant wild-type beta -subunit and its deletions were separated by 12.5% SDS-PAGE and transferred to nitrocellulose and then incubated, first in buffer containing 20 mM Hepes, pH 7.3, 100 mM sodium acetate, 5 mM magnesium acetate, 0.25% Tween 20, 0.5% BSA, and 5 mM DTT, and then preincubated for 30 min at room temperature in binding buffer (20 mM Hepes, pH 7.3, 100 mM potassium acetate, 5 mM magnesium acetate, 0.05% tween 20, 0.5% BSA, and 5 mM DTT) in the presence of 100 µM GTP. Blots were rinsed with binding buffer and then overlaid with 0.126 pmol/µl [gamma -32P]GTP-Ran (sp act, 15,400 cpm/pmol) in binding buffer for 30 min at room temperature. Binding ability to Ran was also examined in the solution binding assay using GST chimeras of wild-type beta -subunit and its deletions, which gave the same results that were obtained in the overlay assay.

Cell-free Import Assay

Digitonin-permeabilized MDBK cells were prepared as described previously (Adam et al., 1990; Imamoto et al., 1995a). Digitonin-permeabilized cells were incubated with TB containing testing proteins, in 10 µl, under each condition indicated in the respective figure legends. After incubation, cells were fixed with 3.7% formaldehyde in TB. T-APC and GFP fusion proteins were detected by Axiophot microscopy (Carl Zeiss, Inc.).


Results

beta -Subunit Is Localized Both in the Cytoplasm and within the Nucleus

We initially examined the intracellular localization of a 97-kD component of the PTAC (beta -subunit) by using affinity-purified antibodies raised against recombinant beta -subunit. The affinity-purified anti-beta -subunit antibodies recognized a single protein band that corresponds to endogenous beta -subunit from cytosol prepared from Ehrlich ascites tumor cells, as well as total extracts prepared from human embryonic lung (HEL) cells, and MDBK cells (Fig. 1 A). Staining with these antibodies showed that the beta -subunit is located not only in the cytoplasm but also within the nucleus in these tissue-cultured mammalian cells (Fig. 1 B, a and c). Intranuclear staining was further confirmed by confocal microscopy (Fig. 2, a and b). These staining patterns were abolished on incubation of the antibodies with recombinant beta -subunit (Fig. 1 B, b and d), confirming that they represent a subcellular localization of endogenous beta -subunit.



Fig. 1. Subcellular localization of beta -subunit in tissue-cultured mammalian cells. (A) SDS-PAGE profiles of proteins stained by coomassie brilliant blue staining (indicated as C) of Ehrlich ascites tumor cells cytosol, or total extracts of HEL cells, and MDBK cells, and Western blots of the corresponding proteins incubated with affinity-purified anti-beta -subunit antibodies (indicated as i) or preimmune IgG (indicated as p). (B) HEL cells (a and b) and MDBK cells (c and d) were stained with affinity-purified anti- beta -subunit antibodies preincubated with recombinant GST (a and c) or GST-beta -subunit (b and d) trapped in glutathione-Sepharose.
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Fig. 2. Confocal microscopy reveals that beta -subunit is localized inside the nucleus. HEL cells (a) and MDBK cells (b) stained with affinity-purified anti-beta -subunit antibodies, as in Fig. 1, or subcellular localization of GFP-wild-type beta -subunit that was microinjected into the cytoplasm of HEL cells (c) as in Fig. 4, was examined with a confocal laser scanning microscope (Carl Zeiss, Inc.). 0.5-µm sections, corresponding to the equator of the nucleus, are shown.
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Fig. 4. The NPC-binding domain of beta -subunit is necessary and sufficient for its nuclear migration. HEL cells injected with 1.5 mg/ml GFP-wild-type beta -subunit (a and b), GFP-D450-876 (c and d), FITC-D3-145 (e and f), or GFP-D3-447 (g) were incubated for 30 min at 37°C. b, d, and f show cells co-injected with 1 mg/ml WGA. After incubation, cells were fixed with 3.7% formaldehyde in PBS, and the localization of proteins was examined by Axiophot microscopy (Carl Zeiss Inc.).
[View Larger Version of this Image (86K GIF file)]

beta -Subunit Rapidly Migrates into the Nucleus in Living Cells

We examined whether the beta -subunit migrates into the nucleus by using tissue-cultured cell microinjection. To visualize the injected recombinant beta -subunit, we modified this protein in three different ways: tagging with influenza virus hemagglutinin (HA) epitope, tagging with GFP to the NH2 terminus of beta -subunit, or labeling with FITC. None of these modifications affected the activity of the beta -subunit in terms of supporting nuclear import in the digitonin-permeabilized cell-free transport assay (data not shown). We found that all these modified recombinant beta -subunits rapidly migrated into the nucleus within 30 min after injection into the cytoplasm. Intranuclear localization of cytoplasmically injected GFP-beta -subunit, observed by confocal microscopy, is shown in Fig. 2 c.

In the digitonin-permeabilized cell-free transport assay, it was shown that the beta -subunit does not accumulate in the nucleus, while alpha -subunit does so with NLS substrate during NLS-mediated nuclear import. In the following studies, we attempted to analyze whether nuclear import of the beta -subunit is related to NLS-mediated nuclear import.

Nuclear Migration of beta -Subunit Occurs without Binding to alpha -Subunit and Ran in Living Cells

To determine the functional domain of the beta -subunit, which is required for its nuclear locating ability, deletion mutants were generated, permitting an initial mapping of the alpha -subunit-, Ran-, and NPC-binding domains of the beta -subunit. Deletion mutants that were generated and used in this study are shown in Fig. 3 A. In the solution binding assay, COOH-terminal deletions, such as D769-876 and D644-876, showed a decreased binding activity for the alpha -subunit, and D450-876 completely lost binding affinity (Fig. 3 B). In contrast, NH2-terminal deletions, such as D3-145 and D3-447, showed binding activity to the alpha -subunit that was equivalent to the wild-type beta -subunit. These results show that the alpha -subunit binding domain is located in the COOH-terminal portion of the molecule.



Fig. 3. Mapping of the alpha -subunit-, Ran-, and NPC-binding domains of beta -subunit. (A) The constructions of the deletion mutants of beta -subunit. (B) alpha -Subunit-binding activity of deletion mutants of beta -subunit. GST-beta -subunit or its deletion mutants were incubated with 30 pmol GST-alpha -subunit and T-bBSA (0.25 mg/ ml) for 30 min at 37°C and then trapped in immobilized avidin. The bound proteins were resolved by SDS-PAGE and quantified by densitometric scanning, and molar ratios of beta -subunit or its deletion mutants bound to alpha -subunit were determined. (C) Ran-binding activity of deletion mutants of beta -subunit was determined by overlay assay. 100 pmol of wild-type beta -subunit and its deletions, or RanBP1, were subjected to SDS-PAGE, transferred to nitrocellulose sheet, and incubated with [gamma -32P]GTP-Ran as described under experimental procedures. [gamma -32P]GTP-Ran bound to the recombinant proteins were detected by autoradiography. (D) NH2-terminal portion of beta -subunit competitively inhibits NPC docking of PTAC. Digitonin-permeabilized cells were incubated with 10 µl testing solution containing 12 pmol GST-beta -subunit, 12 pmol GST-alpha -subunit, and T-APC (0.1 mg/ml) in the presence (b) or absence (a) of 144 pmol D450-876 mutant for 20 min on ice. After incubation, the cells were fixed with 3.7% formaldehyde in TB, and T-APC was detected by Axiophot microscopy (Carl Zeiss Inc.).
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It is noteworthy that, D450-876 specifically binds to GTP-Ran (Fig. 3 C). This portion of the beta -subunit also contains a domain that interacts directly with the NPC, since D450-876 competitively inhibited the NPC docking of PTAC, when examined in the digitonin-permeabilized cells (Fig. 3 D). D3-447, which lacks the entire NH2-terminal portion of the beta -subunit, neither binds to Ran (Fig. 3 C) nor NPC (see Figs. 4 and 7). A deletion mutant lacking the NH2-terminal 143 amino acids (D3-145) did not bind to Ran (Fig. 3 C). Since neither amino acids 1-300 and 145- 449 beta -subunit fragments bound to GTP-Ran in overlay assay, two stretches of NH2- and COOH-terminal amino acids of D450-876 appear to be necessary for efficient Ran binding (data not shown). These mapping results are consistent with recently published reports by other groups (Chi et al., 1997; Kutay et al., 1997).


Fig. 7. Nuclear migration of beta -subunit is saturable. Digitonin-permeabilized cells were incubated with 10 µl of testing solution containing 3 pmol GFP-beta -subunit (a-d) or GFP-D450-876 (e-h) in the absence (a and e) or presence of either 24 pmol GST- beta -subunit (b and f), GST-D450-876 (c and g), or GST-D3-447 (d and h) for 15 min on ice. Localization of GFP-chimeras was examined after fixation of the permeabilized cells as in Fig. 3 D.
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Having established which of the beta -subunit mutant proteins cannot bind to the alpha -subunit (D450-876), Ran (D3-145), or to both Ran and NPC (D3-447), we examined which of these proteins are capable of migrating into the nucleus in living cells. As shown in Fig. 4, cytoplasmically injected D450-876 and D3-145 rapidly migrated into the nucleus, while D3-447 did not. As with the wild-type beta -subunit, nuclear migration of D450-876 and D3-145 was inhibited by WGA, indicating that all of these proteins migrate through the gated channels of the NPC. These results show that the nuclear migration of beta -subunit does not require alpha -subunit and Ran binding, but only the NPC-binding domain, which is involved in PTAC docking.

It has been shown that in the digitonin-permeabilized transport assay, both alpha -subunit and Ran binding to the beta -subunit is essential for NLS-mediated import (Chi et al., 1996; Görlich et al., 1996b; Kutay et al., 1997). In contrast, the above microinjection results show that the beta -subunit is capable of migrating into the nucleus of living cells in the absence of these interactions. These findings indicate that the beta -subunit migrates into the nucleus alone, independent of NLS-mediated nuclear import. We refer to such behavior as the "unassisted" nuclear migration of the beta -subunit.

beta -Subunit Migrates into the Nucleus of Digitonin-permeabilized Cells in the Absence of Exogenous Addition of Soluble Factors

In further investigations, we examined the behavior of the beta -subunit using the digitonin-permeabilized cell-free transport assay. In the presence of alpha -subunit/NLS substrate, the beta -subunit accumulated at the nuclear rim, as reported previously (Imamoto et al., 1995a; Görlich et al., 1995b; Moroianu et al., 1995b). However, wild-type beta -subunit was found to efficiently accumulate in the nucleus in the absence of added soluble factors. Consistently, D450-876, lacking the alpha -subunit-binding domain, efficiently migrated into the nucleus, irrespective of the presence or absence of alpha -subunit/NLS substrate (Fig. 5 A).



Fig. 5. Unassisted nuclear migration of beta -subunit occurs in the absence of exogenous addition of soluble factors in digitonin-permeabilized cell-free transport assay. (A) Digitonin-permeabilized MDBK cells were incubated with 10 µl of testing solution containing 3 pmol GFP-beta -subunit (a and b) or GFP-D450-876 (c and d) in the presence (a and c) or absence (b and d) of 3 pmol GST- alpha -subunit and T-APC (0.1 mg/ml) for 20 min. (B) Digitonin-permeabilized MDBK cells were incubated with 10 µl testing solution containing 4 pmol of GFP-beta -subunit (a-c), GFP-D450-876 (d-f), or FITC-D3-145 (g-i) in the absence (a, d, and g) or presence of either 20 pmol GTP-Ran (b, e, and h) or GDP-Ran (c, f, and i) for 15 min. After incubation, localization of beta -subunit and its mutant proteins was examined after fixation of the permeabilized cells as in Fig. 3 D.
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We next examined the effect of small GTPase Ran on the nuclear accumulation of beta -subunit. As shown in Fig. 5 B, wild-type beta -subunit and D450-876 significantly accumulated at the nuclear rim, but did not enter the nucleus in the presence of GTP-Ran. GDP-Ran had a much less inhibitory effect on the nuclear accumulation of both proteins. The effect of Ran on the nuclear migration of beta -subunit is likely to be the result of its direct binding to the beta -subunit, since the nuclear accumulation of D3-145, which lacks Ran-binding ability, was not affected by GTP-Ran.

These results show that the nuclear migration of beta -subunit occurs in the absence of added soluble factors, when it is not bound to either alpha -subunit or GTP-Ran, and that the beta -subunit itself possesses the necessary and sufficient information to translocate the NPC.

The Unassisted Nuclear Migration of beta -Subunit Occurs without the Support of GTP-Hydrolysis of Ran

The above results indicate that the beta -subunit, when it does not carry alpha -subunit with NLS substrate, is capable of migrating into the nucleus in the absence of Ran. To further verify that the movement of the beta -subunit through the NPC is not supported by Ran, we examined the effect of GTP-G19V Ran, a point-mutated Ran, defective in GTP hydrolysis, on the unassisted nuclear migration of beta -subunit. This dominant-negative Ran, defective in GTP hydrolysis, has been demonstrated to strongly inhibit the Ran-dependent import of known substrates in living cells (Dickmanns et al., 1996; Sekimoto et al., 1996). In contrast, in living cells, it was found that co-injection of GTP-G19V Ran did not affect the nuclear migration of either wild-type beta -subunit or D3-145, while it strongly inhibited the nuclear migration of SV40 T-antigen NLS-containing karyophile (Fig. 6 A). These in vivo results further confirm that GTP hydrolysis of Ran is not required for movement of the beta -subunit through the NPC.



Fig. 6. The import of beta -subunit occurs without the support of GTP hydrolysis of Ran. (A) 1 mg/ml SV40 T-antigen NLS substrate (a and b), 1 mg/ml GFP-wild-type beta -subunit (c and d), or 0.7 mg/ml FITC-D3-145 (e and f) were injected with (b, d, and f) or without (a, c, and e) 3 mg/ml GTP-G19V Ran in the cytoplasm of HEL cells. After incubation for 30 min at 37°C, localization of beta -subunit or D3-145 was examined after fixation of the cells as in Fig. 4. (B) Digitonin-permeabilized MDBK cells were incubated with 10 µl of testing solution containing 3 pmol GFP-beta -subunit (a-c) or FITC-D3-145 (d-f) in the absence (a and d) or presence of 40 pmol G19V GTP-Ran (b and e) for 15 min. c and f show the import assay performed with permeabilized cells pretreated with 0.2 mg/ml WGA for 15 min. Localization of beta -subunit or its mutant proteins was examined after fixation of the permeabilized cells as in Fig. 3 D.
[View Larger Versions of these Images (93 + 96K GIF file)]

It should be noted, however, that in the digitonin-permeabilized cell-free transport assay, GTP-G19V Ran showed an inhibitory effect on the nuclear import of wild-type beta -subunit, but failed to inhibit the import of D3-145 (Fig. 6 B). These in vitro results are consistent with those obtained with GTP-Ran, described above, and indicate that the inhibitory effect of GTP-G19V Ran appears to be due to the direct binding of this molecule to the beta -subunit but not the inhibition of GTP hydrolysis. Moreover, different results, obtained in in vitro and in vivo studies, indicate that GTP-G19V Ran cannot stably bind to the beta -subunit in the cytoplasm of living cells (discussed below).

Nuclear Migration of beta -Subunit Is Saturable

The unassisted beta -subunit import was promoted by amino acid residues 1-447 of this molecule. To confirm that the import is promoted through specific interaction(s), we examined the saturability of the import. In the digitonin-permeabilized cell-free system, the nuclear migration of GFP-tagged beta -subunit and D450-876 decreased on the addition of an eightfold excess of nonlabeled beta -subunit or D450-876 (Fig. 7). Addition of the NH2-terminal deletion, D3-447, which lacks the NPC-binding domain, had no effect on nuclear migration of the beta -subunit. Since nuclear migration of the beta -subunit occurs in the absence of added soluble factors, it is likely that the beta -subunit transits through the NPC, from the cytoplasmic face toward the nuclear interior, by interacting directly with saturable site(s) within the NPC.


Discussion

Our present study shows that a 97-kD component of the nuclear pore-targeting complex (beta -subunit) can behave in two different ways in cells. One is to support NLS-mediated import and the other is to migrate into the nucleus in an unassisted manner. The former reaction, in which the beta -subunit carries the alpha -subunit with NLS substrate, is absolutely dependent on the presence of Ran and requires the Ran-binding domain of the beta -subunit to exert a translocation reaction. The latter reaction, when beta -subunit is alone, does not require Ran for the translocation through the NPC. Therefore, the beta -subunit can exert protein translocation reaction through NPC via two contrasting mechanisms, namely, "Ran-assisted" versus "Ran-unassisted" import.

The Ran-unassisted nuclear migration of the beta -subunit was strongly inhibited by WGA, both in living cells and in the digitonin-permeabilized cells (Figs. 4 and 6 B). Therefore, it is most likely that this protein migrates into the nucleus through gated channels of the NPC, similar to NLS-mediated import. Nuclear migration of the beta -subunit is not the result of protein degradation, which was confirmed by judging the integrity of the GFP-beta -subunit, which migrated into the nucleus of permeabilized cells by SDS-PAGE, followed by immunoblotting (data not shown).

The unassisted nuclear migration of the beta -subunit was promoted by its NPC-interacting domain, which is located within its NH2-terminal portion and which is also involved in the NPC docking of PTAC. A competition study, showing that the unassisted nuclear migration of beta -subunit occurs in a saturating manner (Fig. 7), indicates that the beta -subunit is translocated through the NPC via specific interaction(s) with saturable site(s) of the NPC. Since D3-145 migrated into the nucleus in a manner similar to the wild-type beta -subunit and D450-876, a structure necessary for the nuclear migration of the beta -subunit through interaction with NPC components, would be predicted to be located within amino acids 146-447 of this protein.

Unlike NLS-mediated import, the beta -subunit import was observed without the exogenous addition of ATP/GTP. Also, nuclear accumulation of beta -subunit occurred even on ice (see Fig. 7), although the rate of import was reduced compared to the reaction performed at 30°C. Pretreatment of permeabilized cells with apyrase or hexokinase/glucose reduced but did not abolish the import (Imamoto, N., S. Kose, and Y. Yoneda, manuscript in preparation). Meanwhile, sensitivity to WGA and saturability of import provide strong support for the view that the unassisted nuclear migration of beta -subunit through NPC occurs via a mechanism that involves specific molecular interactions of the NPC-binding domain of the beta -subunit with NPC components. Differences in the level of requirement of ATP/ GTP may be due to differences in the requirement of Ran, although this must be addressed in further studies.

It was shown in previous studies that the beta -subunit binds directly with several yeast nucleoporins, containing FXFG repeats (NUP1, NUP2, NUP36, NUP156, and NUP96) and GLFG repeat (NUP116) (Iovine et al., 1995; Kraemer et al., 1995; Radu et al., 1995b). However, in a solution-binding assay, it was shown that the beta -subunit, when bound to GTP-Ran, cannot access the repeat-containing nucleoporins. Our present data show that the beta -subunit is stably complexed at the nuclear rim when it is bound to alpha -subunit/NLS substrate but transits rapidly through the NPC when it is not bound to these factors (Fig. 5 A). NPC docking of PTAC was significantly reduced, but was not completely inhibited in the presence of 12-fold excess of D450-876 beta -subunit fragment, which may indicate that the mode of interaction of the beta -subunit with NPC is different when it is alone or complexed with the alpha -subunit/NLS substrate (see Fig. 3 D). The rim binding of the beta -subunit that occurs in the presence of alpha -subunit/NLS substrate can be thought of as an intermediate state of NLS-mediated import, probably through repeat-containing nucleoporins. It is possible, however, that the beta -subunit could be complexed with different site(s) of the NPC in the presence of GTP-Ran, in contrast to those in the presence of alpha -subunit/NLS substrate. By analogy with the finding that the beta -subunit forms a stable complex with Ran and its binding protein RanBP1 (Chi et al., 1996; Imamoto, N., S. Kose, T. Tachibana, and Y. Yoneda, unpublished observation), one such candidate might be a 358-kD Ran-binding NPC protein (RanBP2/NUP358), which contains four Ran-binding domains similar to RanBP1 (Yokoyama et al., 1995; Wu et al., 1995). The rim binding of the beta -subunit that occurs in the presence of GTP-Ran will require further studies to understand the physiological significance.

Previous published results did not detect the nuclear accumulation of beta -subunit in the digitonin-permeabilized cell-free import assay (Görlich et al., 1995; Moroianu et al., 1995b; Kutay et al., 1997). However, our present data show that the beta -subunit transits rapidly through NPC in the permeabilized cell-free import assay. Although we cannot clearly explain reasons for such contradictions, the nuclear migration of beta -subunit would not be detected in the import assay when carried out in the presence of either alpha -subunit, GTP-Ran, or crude cytosol. In our experiments, nuclear migration of the beta -subunit in the in vitro system can be observed only in the absence of exogenous addition of soluble factors. alpha -Subunit and GTP-Ran prevent the nuclear migration of beta -subunit, and crude cytosol, in all probability, contains these and other soluble factor(s) that prevent the nuclear migration of the beta -subunit in vitro. Also, nuclear migration of beta -subunit might be affected by factor(s) that could be differently retained in the permeabilized cells upon preparation.

In living cells, cytoplasmically injected beta -subunit rapidly migrated into the nuclei, irrespective of the protein concentration in the needle (from 0.5 mg/ml; corresponding, approximately, to 0.2-fold of endogenous beta -subunit to 10 mg/ml protein; corresponding, approximately, to fourfold of the endogenous beta -subunit). Further, GTP-G19V Ran did not prevent the nuclear migration of beta -subunit in living cells, while it prevented nuclear migration of the beta -subunit in vitro. These observations suggest that there may be factor(s) in the cytoplasm of living cells that actively dissociate beta -subunit from GTP-Ran. We speculate that a cellular mechanism, which remains to be elucidated, exists by which the unassisted nuclear migration of beta -subunit occurs, even in the presence of endogenous alpha -subunit and Ran.

Indirect immunofluorescence studies using affinity-purified antibodies against recombinant beta -subunit demonstrated that a significant amount of endogenous beta -subunit is located within the nucleus in tissue-cultured mammalian cells (Figs. 1 and 2), while previous reports indicated that it is located in the cytoplasm and on the nuclear envelope, but not within the nucleus (Chi et al., 1995). In yeast, Koepp et al. (1996), using affinity-purified anti-Kap95p antibodies, detected Kap95p (yeast beta -subunit) on the nuclear envelope but not within the nucleus. However, Iovine and Wente (1997) very recently demonstrated that Kap95p recycles between the cytoplasm and nucleus by showing that nuclear export signal-mutated Kap95p accumulates in the nucleus. Our preliminary results indicate that the beta -subunit shuttles between the nucleus and cytoplasm, since nucleoplasmically injected beta -subunit rapidly exits the nucleus. The tagging of GFP to the NH2 terminus of the beta -subunit did not affect its nuclear export, indicating that the nuclear accumulation of the beta -subunit observed in this study is not due to its inability to exit the nucleus caused by the tagging (data not shown). We presume that discrepancies between previous and present studies regarding the detection of nuclear beta -subunit are due to differences in antibodies used, or, alternatively, differences in cellular and/ or fixation conditions that may affect the equilibrium of beta -subunit between the cytoplasm and nucleus.

The present data, which show that the beta -subunit migrates into the nuclear interior independently from the NLS-containing substrate, provide an intriguing possibility that this protein possesses another role in cells, in addition to supporting NLS-mediated import. The extent of nuclear migration of injected beta -subunit, as well as the distribution of endogenous beta -subunit, differed among cells, indicating that its unassisted import could be regulated by cellular physical conditions. The intracellular distribution of endogenous beta -subunit should also be affected by its export. Whether the export of the beta -subunit occurs in a Ran- assisted or -unassisted manner is now under investigation. The intranuclear amount of beta -subunit may affect the ratio of alpha - to beta -subunit in the cytoplasm or the GTPase cycle of Ran, both in the nucleus and cytoplasm, which, in turn, could lead to the regulation of NLS-mediated nuclear import. Further studies are required to explore these and other possibilities.


Footnotes

Received for publication 16 June 1997 and in revised form 14 August 1997.

   S. Kose and N. Imamoto contributed equally to this work.
   Address all correspondence to Yoshihiro Yoneda, Department of Anatomy and Cell Biology, Osaka University Medical School, 2-2 Yamada-oka, Suita, Osaka 565, Japan. Tel.: (81) 6 879 3211. Fax: (81) 6 879 3219.
   Takuya Shimamoto's present address is Department of Microbiology, Osaka University Medical School, Suita, Osaka 565, Japan.

We thank Drs. T. Ohba and T. Nishimoto for E. coli strain expressing human Ran, and Dr. S. Yuba for helpful discussions.

This work was supported by a Grant-in-Aid for Scientific Research on Priority Areas (No. 07282103), Grant-in-Aid for Scientific Research (B) (No. 08458229), Grant-in-Aid for Scientific Research (C) (No. 08680764), and Grant-in-Aid for COE Research (No. 07CE2006) from the Japanese Ministry of Education, Science, Sports and Culture, the Nissan Science Foundation, and the Naito Foundation.


Abbreviations used in this paper

GFP, green fluorescent protein: GST, glutathione-S-transferase; MDBK, Madin-Darby bovine kidney; NLS, nuclear localization signal; NPC, nuclear pore complex; PTAC, nuclear pore-targeting complex.


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