The Nucleoporin Nup153 Plays a Critical Role in Multiple Types of Nuclear Export

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Vol. 10, Issue 3, 649-664, March 1999

The Nucleoporin Nup153 Plays a Critical Role in Multiple Types of Nuclear Export

Katharine S. Ullman,^* Sundeep Shah, Maureen A. Powers, and Douglass J. Forbes

Department of Biology, University of California at San Diego, La Jolla, California 92093-0347

Submitted October 20, 1998; Accepted December 17, 1998
Monitoring Editor: Pam Silver

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

The fundamental process of nucleocytoplasmic transport takes place through the nuclear pore. Peripheral pore structures arepresumably poised to interact with transport receptors and theircargo as these receptor complexes first encounter the pore. Onesuch peripheral structure likely to play an important role innuclear export is the basket structure located on the nuclearside of the pore. At present, Nup153 is the only nucleoporin knownto localize to the surface of this basket, suggesting that Nup153is potentially one of the first pore components an RNA or proteinencounters during export. In this study, anti-Nup153 antibodieswere used to probe the role of Nup153 in nuclear export in Xenopusoocytes. We found that Nup153 antibodies block three major classesof RNA export, that of snRNA, mRNA, and 5S rRNA. Nup153 antibodiesalso block the NES protein export pathway, specifically the exportof the HIV Rev protein, as well as Rev-dependent RNA export. Notall export was blocked; Nup153 antibodies did not impede the exportof tRNA or the recycling of importin $beta$ to the cytoplasm. The specificantibodies used here also did not affect nuclear import, whethermediated by importin $alpha$ / $beta$ or by transportin. Overall, the resultsindicate that Nup153 is crucial to multiple classes of RNA andprotein export, being involved at a vital juncture point in theirexport pathways. This juncture point appears to be one that isbypassed by tRNA during its export. We asked whether a physicalinteraction between RNA and Nup153 could be observed, using homoribopolymersas sequence-independent probes for interaction. Nup153, unlikefour other nucleoporins including Nup98, associated strongly withpoly(G) and significantly with poly(U). Thus, Nup153 is uniqueamong the nucleoporins tested in its ability to interact withRNA and must do so either directly or indirectly through an adaptorprotein. These results suggest a unique mechanistic role for Nup153in the export of multiplecargos.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Compartmentalization of genomic DNA within the nucleus provides a unique environment in which replication and expression ofthe genome can be tightly regulated. In turn, nucleocytoplasmictransport is critical to these fundamental processes. A majorchallenge in the field has been to determine how nuclear poresaccomplish the complicated task of selective, bidirectional trafficking.Initial steps in understanding nucleocytoplasmic transport haveinvolved characterization of the molecular nature of transportcargo traversing the pore. Much progress has been made not onlyin defining signals that direct nucleocytoplasmic traffic butalso in identifying cognate soluble receptors that ferry cargoto and through the pore (for review, see Corbett and Silver, 1997;Izaurralde and Adam, 1998). The first such receptor to be identifiedwas importin $alpha$ (also referred to as NLS receptor, karyopherin $alpha$ , PTAC58, and hSRP1), a protein that binds to the classical basicnuclear localization signal (NLS) (Adam and Gerace, 1991; Görlichet al., 1994; Imamoto et al., 1995; Moroianu et al., 1995; Weiset al., 1995). Importin $alpha$ directs import as part of a heterodimer;its partner importin $beta$ (p97, karyopherin $beta$ , and PTAC97) is primarilyresponsible for mediating contact with nucleoporins during transitof the receptor complex through the pore (Chi et al., 1995; Görlichet al., 1995; Radu et al., 1995a). Importin $beta$ is a member of alarge superfamily of related proteins (Fornerod et al., 1997b;Görlich et al., 1997). Recent results have implicated an increasingnumber of members of this family as specialized import receptors(Aitchison et al., 1996; Pollard et al., 1996; Pemberton et al.,1997; Rosenblum et al., 1997; Rout et al., 1997; Ferrigno et al.,1998; Jakel and Görlich, 1998; Senger et al., 1998). In mostcases these importin $beta$ -like receptor proteins have been foundto bind to specific transport substrates directly rather thanin conjunction with a partnerprotein.

Although numerous classes of RNA and a number of proteins are exported from the nucleus, less is known about the specificsignals and cognate receptors that direct their export. One importantstep forward was the identification of a short, leucine-rich aminoacid sequence termed the nuclear export signal or NES that, likethe NLS, mediates interaction with a soluble receptor, in thiscase exportin 1/Crm1 (Fornerod et al., 1997a interaction witha soluble receptor,; Fukuda et al., 1997; Neville et al., 1997;Ossareh-Nazari et al., 1997; Stade et al., 1997; Ullman et al.,1997). In fact, this export receptor was found to be a memberof the importin $beta$ superfamily. NESs were identified originallyin the human immunodeficiency virus (HIV) protein Rev and in thecellular protein PKI (protein kinase A inhibitor; Fischer et al.,1995; Wen et al., 1995). Competition analysis soon made it apparent,however, that an NES signal is involved in many types of nuclearexport including 5S RNA, U snRNA, and mRNA export (Fischer etal., 1995; Pasquinelli et al., 1997b). This implies that the NESreceptor exportin 1 is similarly multifunctional; however, therole of exportin 1 in the export of all of these cargo has notyet been entirelyelucidated.

tRNA export, although known to be an active export process (Zasloff, 1983; Jarmolowski et al., 1994), shows no dependenceon an NES signal in competition studies (Pasquinelli et al., 1997b).Recently, a soluble receptor termed exportin-t was identifiedand is proposed to guide tRNA from the nucleus to the cytoplasm(Arts et al., 1998; Hellmuth et al., 1998; Kutay et al., 1998).The protein sequence of exportin-t reveals that it too is a memberof the importin $beta$ superfamily. Interestingly, rather than recognizinga peptide signal sequence, exportin-t interacts directly withtRNA, illustrating another variation of cargo recognition in thisfamily.

In summary, evolution appears to have elegantly created a family of specialized receptors that fulfill myriad transport functions.Although each member has unique specificity, a common definingfeature shared by all members is a binding domain for the smallGTPase Ran, an important accessory factor for nuclear transport.The distinct roles of Ran in import and export are reflected inthe observation that Ran-GTP, predicted to be at high concentrationin the nucleus, stabilizes export receptor-cargo complexes butdissociates import receptor-cargo complexes (see Rexach and Blobel,1995; Fornerod et al., 1997a; Cole and Hammel, 1998; Kutay etal., 1998, and references therein). Transport is regulated furtherby additional accessory factors, such as the protein p10/NTF2(Moore and Blobel, 1994; Paschal and Gerace, 1995; Corbett andSilver, 1996; Clarkson et al., 1997; Feldherr et al., 1998).

With much of the groundwork laid in terms of identifying receptor-cargo transport complexes, one can now turn to the questionof how this traffic moves through the pore. Fundamental to ourunderstanding of nuclear pore function is the question of whetherthe importin $beta$ -related superfamily members have diverged in theircapacity to interact with the transport machinery of the pore.Transport receptors have been observed to interact with many nucleoporinswhen tested in vitro (Radu et al., 1995b; Aitchison et al., 1996;Bonifaci et al., 1997; Pemberton et al., 1997; Percipalle et al.,1997; Rosenblum et al., 1997; Rout et al., 1997). Although thisprovides information on a range of potential interactions, theissue of which interactions take place in vivo is at the cruxof understanding how transport of different substrates takes placemechanistically.

In vivo, interactions are constrained by several factors including accessibility, as well as relative affinities when multiplebinding choices are present. One way that in vivo interactionshave been studied has been by examining competition between transportreceptors for nuclear rim binding in permeabilized cells (Görlichet al., 1997; Kutay et al., 1997). Such studies have revealedthat importin $beta$ and several other import receptors potentiallybind overlapping sites at some point during transport. In vivomethods that focus on steady-state transport receptor-nucleoporininteractions have perhaps been more revealing of unique high-affinityinteractions between given receptors and nucleoporins. For example,exportin 1 has been found to be a major binding partner of nucleoporinNup214 in vivo (Fornerod et al., 1997b), whereas importin $beta$ isfound to interact stably with Nup358, Nup153, and Tpr but notother tested nucleoporins (Shah et al., 1998). In vivo interactionshave also been assessed genetically and biochemically in yeast(Belanger et al., 1994; Iovine et al., 1995; Simos et al., 1996;Bailer et al., 1998; Senger et al., 1998). Extrapolation of interactionsfound in yeast to the vertebrate pore is often difficult becauseof the divergence in pore proteins, but the results clearly lendfurther support to the conclusion that, in vivo, transport receptorsinteract preferentially with subsets of nucleoporins. Importantly,this indicates that different cargo-receptor complexes are likelyto have distinct modes of transport through the pore. However,with the limited amount of information at hand, it is not yetclear how many distinct routes there are. At one extreme, therecould be simply an import route and an export route. At the otherextreme, there could be a distinct route through the pore foreach class of cargo-receptorcomplex.

In a complementary approach, individual components of the pore can be assessed for their involvement in different types oftransport. These experiments serve both to distinguish transportroutes as well as to functionally define the pore transport machineryin vivo. The vertebrate nuclear pore presents a formidable experimentalchallenge because of its large size (120 million daltons) andcomplexity. Electron microscopy has revealed several strikingfeatures of the pore (see Goldberg and Allen, 1995; Yang et al.,1998, and references therein). In addition to a central transporterregion held within a large ring of spokes, asymmetric structuresextend into the nucleus and cytoplasm. Filaments are found tetheredon the cytoplasmic face of the pore, whereas other fibers extendto form a basket-like structure on the nucleoplasmic side of thepore.

Several individual components of the vertebrate pore have been molecularly identified, and their locations have been mappedto these structural landmarks. Briefly, Nup358, Nup214, and Nup84(Nup88) are localized to the cytoplasmic filaments (Kraemer etal., 1994; Wu et al., 1995; Yokoyama et al., 1995; Bastos et al.,1997; Cordes et al., 1997), whereas Nup62 and its associated bindingpartners (Nup58, Nup54, and Nup45) are located centrally (Groteet al., 1995; Guan et al., 1995). Nup153 has been localized byimmunoelectron microscopy to the distal ring of the nuclear basketand intranuclear filaments (Cordes et al., 1993; Sukegawa andBlobel, 1993; Panté et al., 1994). Nup93, Nup98, and Nup205 arefound on the nuclear face of the pore (Powers et al., 1995; Raduet al., 1995b; Grandi et al., 1997), whereas the Tpr protein isfound on filaments that extend from the pore basket deeper intothe nucleus (Cordes et al., 1997; Zimowska et al., 1997). Althoughmany pore proteins have yet to be identified, valuable clues topore function can be gathered from studying the nucleoporins identifiedtodate.

Results of studies focusing on Nup153 have been particularly intriguing. Bastos et al. (1996) found that overexpression ofeither full-length or certain truncations of Nup153 results innuclear poly(A)+ RNA accumulation, suggesting that Nup153 playsa role in mRNA export. Studies in our laboratory, however, haverevealed that within assembled pores, Nup153 is a major bindingpartner for importin $beta$ , indicating a role for Nup153 in import.Indeed, addition of a fragment of Nup153 to a permeabilized cellassay completely blocks importin $beta$ -mediated import (Shah and Forbes,1998). To gain insight into the role of Nup153 in nuclear export,we have in this study probed numerous export, as well as import,pathways in Xenopus oocytes for defects following nuclear injectionof antibodies specific for Nup153. A dramatic effect on multipletypes of export is observed, while nuclear import and recyclingtake place normally. These results define a critical role forNup153 in specific nuclear export pathways, a role that is preventedby antibody binding. We further find that Nup153 associates, eitherdirectly or indirectly, with certain homoribopolymers in vitro,providing a clue to the role Nup153 plays in export and distinguishingNup153 mechanistically from other nucleoporins involved in RNAexport.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Plasmid Constructs and Oligos

Plasmids used as templates for the in vitro transcription of radiolabeled export substrates and the restriction enzyme usedto linearize the plasmid were as follows: pBSAd (adenoviral majorlate premRNA [see Powers et al., 1997]) and EcoRI; pT7-5S (providedby J. Gottesfeld [see You et al., 1991]) and DraI; pAd48 (Revresponse element [RRE]-containing adenoviral major late premRNA,provided by U. Fischer [see Fischer et al., 1994]) and BamHI;and pBS-DHFR and XbaI. The latter plasmid was constructed by placingthe cDNA sequence of DHFR (obtained from a construct providedby T. Hope, Salk Institute) into the BamHI site of Bluescript.PCR was used to generate DNA templates to be used to direct invitro transcription of tRNA, U1, and U6 snRNA transport substrates.The 5' oligos used for the PCR contained either a T7 or SP6 phagepolymerase promoter, and the genes were amplified from their respectiveplasmid DNAs. The oligonucleotides and corresponding plasmidsfor generating U6 and U1 snRNA templates were as described (Ternset al., 1992, 1993). The in vitro transcription template for humantRNA^met was generated with the following oligonucleotides: 5'-oligo (5'-TAATACGACTCACTATAGGGAGCAGAGTGGCGC-AGC)and 3'-oligo (5'-TAGCAGAGGATGGTT). M. Zasloff kindly provideda plasmid containing this tRNA gene (phH2D [Zasloff, 1983]).

A plasmid containing a T7-driven gene for pyruvate kinase (PK) fused at its C-terminal end to a bipartite NLS derived fromhnRNPK (Michael et al., 1995) was used to produce radiolabeledprotein. The NLS was deleted from this construct to generate aDNA template that produced control PK protein (kindly providedby S. Vasu, D. J. Forbes laboratory). The Xenopus hnRNPA1 gene(a kind gift from M. Michael) was cloned into the CS2MT+ vector(Turner and Weintraub, 1994) between the NcoI and XhoI sites togenerate an SP6-driven template for hnRNPA1 production. Finally,luciferase protein was made using a T7-luciferase control template(Promega, Madison,WI).

Bacterial expression constructs for Nup153 fragments are described in Shah et al. (1998) in which they are referred to asconstruct 3 (amino acids 53-334 of the partial Xenopus Nup153sequence) and construct 1 (amino acids 334-828). The Gst-Rev expressionconstruct used to produce Rev was the kind gift of M. Malim (Meyeret al., 1996); the importin $beta$ expression construct was generouslyprovided by D. Görlich (Kutay et al., 1997).

Generation and Affinity Purification of Anti-Nup153 Antibodies

Purified recombinant Nup153 fragments corresponding to amino acids 53-334 and 334-828 were used to immunize rabbits for Ab1(380)and Ab2(363), respectively (Shah et al., 1998). Neither antibodyrecognizes other FG repeat-containing nucleoporins, such as Nup358or Nup62, on immunoblots. To affinity purify and concentrate antibodiesfor the work described here, the respective antigen was coupledto CnBr-activated Sepharose (Amersham, Arlington Heights, IL).Serum was diluted with an equal volume of 1 M NaCl, 0.4% TritonX-100, and 50 mM Tris (pH 8) and passed over the appropriate affinitymatrix. The columns were washed with five volumes of 0.5 M NaCl,0.2% Triton X-100, and 50 mM Tris (pH 8), followed by five volumesof PBS. Antibodies were then eluted with up to 20 volumes of 100mM glycine (pH 2.5). The eluate was rapidly neutralized with a1:10 volume of 1 M Tris (pH 8) and concentrated in a spin concentrator(10,000 molecular weight [MW] cutoff; Millipore, Bedford, MA).The buffer was then exchanged by diluting and reconcentratingthree times with 10 volumes of PBS. Control preimmune antibodieswere purified following standard procedures using Protein A beads(Harlow and Lane, 1988).

Production and Purification of Recombinant Proteins

Bacteria (BL21/DE3) containing the Nup153 expression constructs were induced with 1 mM isopropyl- $beta$ -D-thiogalactopyranoside(IPTG) in LB media for 3 h at 37°C. After standard procedureswere followed for sonication and clarification, recombinant proteinwas purified on Ni-NTA-agarose according to the manufacturer'sprotocol (Novagen, Madison, WI). After dialysis into PBS, sucrosewas added to 0.25 M before freezing. Recombinant importin $beta$ wasexpressed and purified as above, using the M15 strain of Escherichiacoli (Qiagen, Santa Clara, CA), with growth and induction performedat room temperature. GST-Rev was produced according to Kellogget al. (1995) in bacteria grown in NZ media at room temperature.Protein expression was induced with 0.1 mM isopropyl- $beta$ -D-thiogalactopyranosidefor 3-4 h. Bacterial pellets were washed with cold PBS and sonicatedafter resuspension and a freeze/thaw cycle in cold PBS plus 0.5mM PMSF and 5 µg/ml aprotinin and leupeptin. The resulting suspensionwas clarified by centrifugation and incubated with glutathione-sepharose(Amersham) pre-equilibrated in PBS. After 60 min at 4°C, the beadswere washed extensively with PBS. Fusion protein was then elutedwith 20 mM glutathione in Tris (pH 8), 120 mM NaCl, and 10 mMDTT, followed by buffer exchange to PBS and concentration in aspin concentrator (5000 MW cutoff; Millipore). Glycerol was addedto 5% beforefreezing.

Preparation of Radiolabeled Transport Substrates

Radiolabeled RNA export substrates were transcribed in vitro following standard procedures (Melton et al., 1984). To radiolabelimport substrates and control proteins, plasmids containing SP6-or T7-driven genes for hnRNPA1, PK-NLS, PK, and luciferase weretranscribed and translated using TnT rabbit reticulocyte lysate(Promega) in the presence of [³⁵S]-methionine (Dupont-New England Nuclear, Boston, MA). Unincorporatedmethionine was removed by twice diluting the sample in 500 µlof PBS and reconcentrating in a spin concentrator (5000 MW cutoff;Millipore). Glycerol was added to a 5% final concentration beforefreezing.

Injection and Harvest of Xenopus Oocytes

A small piece of ovary was surgically removed from a Xenopus frog and placed into modified Barth's solution. Stage V and VIoocytes were then selected and stored for up to 2 d at 18°C inmodified Barth's solution. Immediately before injection, the oocyteswere placed in a microwell miniplate (Nalge Nunc International,Naperville, IL), with animal poles oriented upward, and centrifugedat 1200 × g for 10 min at ~22°C. Microinjections were then performed,~10 nl if nuclear and 30-50 nl if cytoplasmic. Blue dextran 2000(18 mg/ml; Amersham) or, in some instances, rabbit reticulocytelysate (20%; Promega) was included with the injected materialto visually distinguish successful nuclear injections after dissection.Incubations were performed at 18°C for the duration indicatedin each experiment. The oocytes were then manually dissected undermineral oil into nuclei and cytoplasm (Lund and Paine, 1990),and each fraction was transferred into the appropriate bufferwith a microcapillary pipette. For isolation of RNA, the bufferused was 100 mM Tris (pH 7.5), 300 mM NaCl, 10 mM EDTA, and 2%SDS. For isolation of protein, the buffer used was 65 mM Tris(pH 7.5), 10 mM EGTA plus 1 mM DTT, and 1 mM PMSF. Generally,material from two to three oocytes was combined, and whereverpossible, samples were collected and analyzed induplicate.

Preparation and Analysis of Injected RNA

After dissection of oocytes, the RNA was prepared for gel analysis by protease K digestion for 60-90 min at 37°C (1 mg/ml;Worthington Biochemical, Lakewood, NJ), followed by extractionwith phenol/chloroform and precipitation with ethanol. Glycogen(30 µg; Boehringer Mannheim, Indianapolis, IN) was added to nuclearsamples as a carrier. The RNA pellets were resuspended in gel-loadingbuffer (80% formamide, 1× TBE buffer) and heated to 65-70°C for~10 min. The material equivalent to the amount found in one oocytenucleus or cytoplasm was loaded in each lane of a denaturing acrylamidegel (6% acrylamide, 6 M urea, TBE). After electrophoresis, thegel was fixed and dried. The results were analyzed by autoradiographyand quantitative phosphorimaging (Molecular Dynamics, Sunnyvale,CA).

Preparation and Analysis of Injected Proteins

To examine protein localization, we homogenized oocyte nuclei and cytoplasm samples either by repetitive pipetting or witha disposable mini pellet pestle (Fisher Scientific, Pittsburg,PA). After centrifugation in a horizontal microfuge rotor (5 min,4°C, 7500 × g), 75% of the material was transferred to a new tube,avoiding the yolk protein-containing pellet. Total protein wasprecipitated by the addition of three to four volumes of acetone,with 40 µg of soybean trypsin inhibitor added to nuclear fractionsas a carrier. After centrifugation, the resulting pellets werethoroughly dried at ~65°C, and then SDS-Laemmli sample bufferwas added to each tube. Protein was resuspended by warming to37°C for 60 min and gently vortexing. After a 10 min incubationat 99°C, the samples were electrophoresed on SDS-Laemmli gels.Material equivalent to 88% of one nucleus and 22% of one cytoplasmwas loaded on the gel, unless otherwise noted. This correspondsto 44 nl of nuclear material and 110 nl of cytoplasmic material,based on a 50- and 500-nl volume, respectively. When ³⁵S-labeled proteins were being monitored, gels were fixed, amplified(Amplify; Amersham), and dried, and the results were visualizedby autoradiography. Otherwise, the proteins were electrophoreticallytransferred to polyvinylidene fluoride membrane (PVDF; Millipore)for Western blot analysis. The filter was placed in blocking solution(5% dried nonfat milk, 2% BSA, 0.1% Tween in PBS for 60 min atroom temperature for anti-GST immunoblotting; and in 1% casein,0.1% Tween, PBS overnight at 4°C for anti-6XHis immunoblotting).Incubation with primary antibody was performed overnight (4°C)in 0.1% Tween and PBS (anti-GST) or in 1% casein, 0.1% Tween,and PBS for 2 h at room temperature (anti-6XHis; Tetra mAb; Qiagen).The primary antibody was detected using an HRP-conjugated secondaryantibody (Jackson ImmunoResearch Laboratories, West Grove, PA)and chemiluminescent substrate (Renaissance ECL; Dupont-New EnglandNuclear).

Identification of Polyribonucleotide-Binding Nucleoporins

High-speed extract prepared from Xenopus eggs (see Smythe and Newport, 1991) was diluted to 2 mg/ml in 25 mM HEPES, 100 mMKCl (or more, where indicated), and aprotinin/leupeptin (5 µg/ml).Nonidet P-40 (NP-40) was also included as indicated. Beads, eitheruncoupled or coupled to each of the homoribopolymers [poly(G),poly(C), and poly(A) (Sigma, St. Louis, MO) and poly(U) (Pharmacia)]were equilibrated (30 min) in the same buffer and then incubatedwith the diluted Xenopus extract for 45-60 min at 4°C. To reducenonspecific binding, BSA (10 mg/ml) was included in the pre-equilibrationand binding incubations where noted. The RNA resins and associatedproteins were separated from unbound proteins by centrifugation(14,000 × g, 30 sec, 4°C), and the beads were washed, first withbuffer containing heparin (2 mg/ml, 10 min, 4°C) and then withbuffer alone (five rapid washes, with KCl omitted from the lastwash). Proteins that remained associated with the resins wereeluted in SDS sample buffer and analyzed by SDS-gel electrophoresis,followed by Western blotting. Immunoblotting was performed asdescribed above, except 5% nonfat dried milk with 0.2% Tween inPBS was used as the blocking solution and either mAb414 (Babco,Berkeley, CA) or affinity-purified anti-Nup98 antibodies wereused as primaryantibodies.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Nup153 Plays a Key Role in the Export of Multiple RNA Cargo

To characterize the role of Nup153 in nuclear transport, we attempted to interfere with Nup153 activity in vivo by the injectionof specific antibodies. Affinity-purified anti-Nup153 antibodies,control buffer, or preimmune IgG were injected into the nucleiof Xenopus oocytes (Figure 1A). One hour later, radioactivelylabeled RNA export substrates were microinjected into the samenuclei. After a further 2 h incubation, the oocytes were dissectedinto nuclei and cytoplasm, and RNA was prepared from each fractionand analyzed by gel electrophoresis. In a first experiment, radiolabeledpre-mRNA, U1 snRNA, 5S RNA, and U6 snRNA were used (Figure 1B).U6 RNA typically is retained in the nucleus and serves as a controlfor accurate nuclear injection (Hamm and Mattaj, 1989). Here,U6 was found to be exclusively nuclear (Figure 1B, lanes 1, 3,and 5). The injected pre-mRNA transcript is normally processedin vivo into mature mRNA and an intron lariat. The intron lariatwas not transported to the cytoplasm in the buffer-injected controloocytes (Figure 1B, lanes 1 and 2); however, a substantial amountof the spliced mRNA was efficiently exported by the 2 h time point(Figure 1B, lane 2, mRNA). Similarly, significant amounts of U1and 5S RNA were exported to the cytoplasm in the buffer-injectedcontrol ooctyes (Figure 1B, lane 2). This overall pattern of exportwas also seen when IgG, isolated from preimmune serum, was injectedinto nuclei (Figure 1B, lanes 3 and 4). In contrast, when antibodiesdirected to Nup153 were injected into nuclei (Figure 1B, lanes5 and 6), the export of mRNA, U1 snRNA, and 5S RNA each was strikinglyinhibited.

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Figure 1. Antibodies to Nup153 prevent the export of multiple classes of RNA. (A) The oocyte injection protocol is shown. First, antibodies were injected into the nucleus. After a 60 min incubation, a second nuclear injection was performed, delivering radioactively labeled RNA. The oocytes were incubated for periods of varying duration and then manually dissected. Nuclear (N) and cytoplasmic (C) RNA was prepared and analyzed by gel electrophoresis. (B) After initial injections either with buffer (BUF., lanes 1 and 2), preimmune IgG (PRE, lanes 3 and 4), or affinity-purified antibodies to Nup153 ( $alpha$ -153, lanes 5 and 6), oocytes were next injected with a mixture of RNA (pre-mRNA, U1 snRNA, 5S rRNA, and U6 snRNA). Two hours later, nuclear and cytoplasmic RNA was harvested. The pre-mRNA has been processed into mature mRNA and a lariat intron. The intron, as well as U6 snRNA, is not normally exported; their nuclear localization here confirms the accuracy of the injection and dissection. Nuclear export of mRNA, U1 snRNA, and 5S RNA is substantially underway at this 2 h time point (lanes 2 and 4) but is fully prevented in the presence of anti-Nup153 antibodies (lane 6).

The effect of anti-Nup153 antibodies on tRNA export was next addressed. Although once again the export of both mRNA and U1snRNA was disrupted by anti-Nup153 antibodies, tRNA export tookplace at its normally rapid rate in the presence of the Nup153antibodies (Figure 2A, compare lanes 3 and 4 with lanes 1 and2). Because anti-Nup153 antibodies clearly have an inhibitoryeffect on the export of mRNA, 5S RNA, and U1 snRNA, we next wantedto ascertain that this inhibitory phenotype was indeed attributableto the immunoreactivity of the antibodies and not attributableto any nonspecific inhibitor associated with the affinity-purifiedantibodies. Toward this end, we examined whether coinjection ofthe recombinant Nup153 protein fragment (amino acids [aa] 53-334)to which the antisera was raised could reverse the effect of antibodyinjection. When recombinant protein (10 ng) was mixed with anti-Nup153antibodies before injection, mRNA and snRNA export now took placenormally (Figure 2A, lane 8), demonstrating the specificity ofantibody inhibition. Another important observation is that inthis experiment the Nup153 fragment alone (Figure 2A, lane 6)had no dominant-negative effect on RNA export.

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Figure 2. Antibodies to Nup153 have a long-lasting and specific inhibitory effect on mRNA export but fail to block tRNA export. (A) An injection experiment was performed as described in Figure 1, except that, in some cases, a recombinant fragment of Nup153 was coinjected with the first injection of buffer or antibodies (lanes 5-8). The mix of RNAs in this experiment included tRNA in addition to pre-mRNA and U1 snRNA. Antibodies to Nup153 did not prevent tRNA export (compare lanes 2 and 4), whereas, as before, export of mRNA and U1 snRNA was blocked by these antibodies. When the Nup153 fragment was coinjected with anti-Nup153 antibodies (lanes 7 and 8), the effect of the antibody was neutralized (lane 8). (B) After injection of either buffer or antibodies, oocytes were injected with a mixture of pre-mRNA, U1 snRNA, 5S RNA, and U6 snRNA and then harvested after either 2 h (lanes 1-4) or 16 h (lanes 5-8) of incubation at 18°C. U6 snRNA is relatively less stable and is no longer detected at the later time point. Export of mRNA, U1 snRNA, and 5S RNA was inhibited at both early and late time points in oocytes preinjected with antibodies to Nup153.

A question that is raised by these results is whether the Nup153 antibodies actually block RNA export or whether they simplyslow the kinetics of export. To address this question, we harvestedRNA from oocytes incubated for 16 h after the injection of RNA.Even after this long incubation period, mRNA, 5S RNA, and U1 snRNAexport remained quantitatively inhibited by the anti-Nup153 antibodies(Figure 2B, compare lanes 4 and 8). This sustained block to exportindicates that the antibodies prevent an essential step in theexportprocess.

Nup153 Is Critical to NES-directed Export

We next wished to investigate directly the role of Nup153 in NES-directed protein export from the nucleus. In terms of theexport signal and corresponding soluble receptor, NES-directedprotein export is a relatively well-characterized export pathway,with the prototypical export cargo being the HIV Rev protein.When injected into the nucleus of a Xenopus oocyte, GST-Rev isnormally exported to the cytoplasm (Figure 3A, lane 2) (Fornerodet al., 1997a). Injection of anti-Nup153 antibodies before theinjection of GST-Rev, however, resulted in a significant blockto Rev export (Figure 3A, lane 4). Although the extent of thisinhibition varied somewhat, the inhibition was consistently observed.Thus, Nup153 must normally contribute to NES-directed proteinexport.

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Figure 3. Nup153 is required for Rev protein export and Rev-mediated RNA export. (A) After injection with either preimmune IgG (lanes 1 and 2) or antibodies to Nup153 (lanes 3 and 4), a recombinant form of the HIV protein Rev (GST-Rev) was injected into the oocyte nuclei. After 2 h, protein was harvested from dissected oocytes and analyzed by Western blot. Rev protein export was inhibited by anti-Nup153 antibodies (compare lanes 2 and 4). The preimmune and affinity-purified antibodies injected into the oocyte nuclei are detected by the secondary antibody (goat anti-rabbit IgG) used in the Western blot (lanes 1 and 3, Ab). (B) Control and antibody-injected oocytes were injected with a mixture of pre-mRNA, U1 snRNA, 5S RNA, U6 snRNA, and tRNA. The pre-mRNA used here contains a Rev response element (RRE) in the intron. Where indicated, GST-Rev was also included in the RNA mixture (lanes 3-6). In the presence of GST-Rev, the RRE-containing lariat intron as well as the pre-mRNA was exported (compare lanes 2 and 4). However, antibodies against Nup153 block Rev-mediated RRE export (lane 6).

The HIV Rev protein is critical to the viral life cycle because it facilitates the export of unspliced and partially splicedviral transcripts. This transport step is needed to express thefull complement of viral proteins, as well as to propagate theviral genome. Unspliced and partially spliced viral transcriptscontain an RNA recognition sequence known as the RRE. Rev proteinsbind to this sequence, and the resulting protein-RNA complexesare then exported, escaping nuclear retention typical for endogenoustranscripts that are only partially processed (for review, seeHope, 1997). In terms of the mechanism of transport through thepore, it is possible that there are differences between the exportof Rev alone, as opposed to a Rev-RNA complex. Certainly thesetwo export cargos are significantly different in terms of size,as well as the number of NESs per cargo complex. We thereforeused the Nup153 antibodies to address whether Nup153 also contributesto the Rev-mediated RNA exportpathway.

To assess an effect on Rev-mediated RNA export, a radiolabeled adenoviral premRNA engineered to contain an RRE in the intron(Fischer et al., 1994) was injected into oocyte nuclei in thepresence or absence of GST-Rev (Figure 3B). As had been demonstratedpreviously, Rev-mediated export was faithfully recapitulated inthe oocytes; the RRE-containing intron, as well as the pre-mRNA,was exported to the cytoplasm in the presence of Rev (Figure 3B,lane 4) but not in its absence (Figure 3B, lane 2). In contrast,coinjection of a mutant form of Rev (M10) that contains an inactiveNES (Malim et al., 1989) did not promote export of RRE-containingRNA (Fischer et al., 1994; our unpublished results). AlthoughRev-mediated export shares a limiting factor(s) with other exportpathways (Fischer et al., 1995; Pasquinelli et al., 1997b), atthe low levels of Rev used here Rev had no competitive effecton U1 snRNA, spliced mRNA, 5S RNA, or tRNA export (Figure 3B,compare lanes 2 and 4) (see also Fischer et al., 1994, 1995).When Rev-mediated RNA export was examined after injection of antibodiesto Nup153, Rev-RNA export was found to be markedly inhibited (Figure3B, lane 6, RRE-intron RNA and premRNA), indicating that Nup153plays an important role in the export of both Rev itself and aRev-RRE-RNAcomplex.

Nuclear Import Occurs Normally in the Presence of Anti-Nup153 Antibodies

Having established that anti-Nup153 antibodies specifically inhibit multiple export pathways, we wished to assess the effectof these antibodies on nuclear import. For this, we again injectedanti-Nup153 antibodies into the nucleus and, after a 60 min incubation,injected radioactively labeled import substrate into the cytoplasm(Figure 4A). To test import directed by a classical NLS, we useda chimeric protein containing pyruvate kinase (PK) fused to abasic bipartite NLS derived from hnRNPK (Matunis et al., 1992;Michael et al., 1995). Although wild-type PK remained in the cytoplasmwhen examined 4 h after injection (Figure 4B, lanes 1 and 2),the PK-NLS protein was found in both compartments at 4 h (Figure4B, lanes 3 and 4). Notably, this NLS-directed import took placeequally well when the oocytes had been injected with antibodiesagainst Nup153 (Figure 4B, lanes 5 and 6).

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Figure 4. Nuclear import occurs in the presence of antibodies to Nup153. (A) The oocyte injection protocol is shown. Antibodies were injected into the nucleus, and after a 60 min incubation, radioactively labeled import substrates were injected into the cytoplasm. After 4 h of incubation, oocytes were manually dissected, and nuclear and cytoplasmic protein was prepared and analyzed by gel electrophoresis. (B) After cytoplasmic injection, pyruvate kinase (PK) remains primarily cytoplasmic (lanes 1 and 2). In contrast, a substantial amount of an NLS-containing form of PK migrates to the nucleus after cytoplasmic injection (lanes 3 and 4). This NLS-directed import continues in the presence of anti-Nup153 antibodies (lanes 5 and 6). (C) M9-directed import of hnRNPA1 also took place in the presence of antibodies to Nup153 (lanes 3 and 4 vs. lanes 1 and 2). Luciferase, coinjected into the cytoplasm with hnRNPA1, remained primarily cytoplasmic, serving as a control for the specificity of nuclear accumulation.

Importin $alpha$ and $beta$ mediate the import of NLS-containing proteins, such as the test substrate above. However, there are otherdistinct import pathways mediated by different import receptors.To examine a second, independent import pathway, we injected hnRNPA1.hnRNPA1 has a nonclassical nuclear import signal termed M9 thatinteracts with the import receptor transportin (Pollard et al.,1996). After cytoplasmic injection of hnRNPA1, a significant amountwas imported into nuclei by 4 h (Figure 4C, lanes 1 and 2). Coinjectedluciferase control protein remained primarily cytoplasmic (lane2). When anti-Nup153 antibodies were injected, the nuclear importof hnRNPA1 took place with equal efficiency (Figure 4C, comparelanes 1 and 3). Thus, under conditions in which multiple exportpathways are inhibited, both NLS- and M9-mediated transport intothe nucleus occursnormally.

Importin $beta$ Recycles in the Presence of Anti-Nup153 Antibodies

After a round of import has taken place, soluble import receptors must be recycled back to the cytoplasm. To examine whetherthe recycling phase of import occurs when anti-Nup153 antibodiesare present, we examined the export of importin $beta$ . Recombinantimportin $beta$ , tagged with a 6XHis epitope, was injected into oocytenuclei. Oocytes were incubated for 2 or 17 h and then dissectedand examined by Western blotting. At a relatively early time point(2 h), a substantial portion of importin $beta$ injected into the nucleiof control oocytes had already been exported to the cytoplasm(Figure 5A, lane 2). Significantly, an equal proportion of importin $beta$ was found in the cytoplasm of oocytes injected with anti-Nup153antibodies (Figure 5A, lane 4), indicating that importin $beta$ wasexporting with identical kinetics in the absence or presence ofthe antibodies. At a later time point (17 h), importin $beta$ was foundto have equilibrated predominantly to the cytoplasm, in oocytesinjected either with control antibodies (Figure 5B, lane 2) orwith Nup153-specific antibodies (Figure 5B, lane 4). Endogenousimportin $beta$ also had a predominantly cytoplasmic localization incontrol, as well as in anti-Nup153-injected oocytes (our unpublishedresults). These results indicate that importin $beta$ is efficientlyrecycled to the cytoplasm in the presence of the Nup153 antibodiesused here.

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Figure 5. Importin $beta$ exports in the presence of anti-Nup153 antibodies. (A) After either no treatment or antibody injection, recombinant 6XHis-importin $beta$ (Imp.- $beta$ ) was injected into the oocyte nuclei. The localization of His-tagged importin $beta$ was then examined at an early time point (2 h) when its export was still underway. The nucleocytoplasmic distribution of 6XHis-importin $beta$ was similar in oocytes that were either untreated (lanes 1 and 2) or injected with anti-Nup153 antibodies (lanes 3 and 4) before the injection of importin $beta$ . This indicates that the kinetics of importin $beta$ recycling are unaltered by the presence of antibodies to Nup153. (B) In an independent experiment, recombinant importin $beta$ was injected into nuclei after injection of either preimmune IgG or anti-Nup153 antibodies. Protein was harvested from nuclear and cytoplasmic fractions 17 h later. His-tagged importin $beta$ equilibrated to the cytoplasm even in the presence of Nup153-specific antibodies (lanes 2 and 4).

Antibodies Directed to Distinct Regions of Nup153 Have Differential Effects on Export

The data indicate that the export of very different substrates shares a requirement for access to Nup153, access that is blockedby the presence of anti-Nup153 antibodies. These different exportcomplexes are likely to interact with Nup153 $---$ directly or indirectly $---$ intheir progression through the nuclear pore. This leads to theinteresting question as to whether the antibodies disrupt an interactionshared by each of the export substrates or whether each substrate(or subsets thereof) has a unique interaction with Nup153. Todelineate further the requirements for Nup153 in export and toask whether differences between the routes of different exportsubstrates can be detected, we used a second set of anti-Nup153antibodies raised to a different region ofNup153.

The antibodies in the previous experiments (now referred to as Ab1) were raised against a fragment of Nup153 that includesa unique N-terminal region and one zinc finger (Figure 6A, fragment1; referred to as "Construct 3" in Shah et al. [1998]). A secondantiserum (Ab2) was generated to fragment 2 (Figure 6A; "Construct1" in Shah et al. [1998]) that includes the zinc fingers of Nup153and part of the C-terminal FG domain located downstream of fragment1. Affinity-purified Ab1 or Ab2 antibodies were injected intooocyte nuclei, followed by the injection of RNA export substratesU1 and tRNA and an additional class of RNA export substrate DHFRmRNA, made as an intronless transcript and therefore not processedin vivo. The export pathway of this latter type of mRNA has beenshown to have some features distinct from that of spliced mRNA(Pasquinelli, et al., 1997a,b; Saavedra et al., 1997). In thisexperiment, DHFR RNA export proved to share a requirement withspliced mRNA for functional Nup153 in the pore; DHFR RNA exportwas strongly blocked by both Ab1 and Ab2 (Figure 6B, lanes 4 and6; 90 and 96% inhibition, respectively, for DHFR export). In contrast,U1 RNA export was differentially affected by the anti-Nup153 antibodies.Although Ab1, as seen in previous experiments, was a potent inhibitorof U1 export (Figure 6, lane 4), Ab2 was not as effective at blockingU1 export (Figure 6B, lane 6; 85 and 40% inhibition in the presenceof Ab1 and Ab2, respectively). tRNA export was robust in the presenceof both Ab1 and Ab2 (Figure 6, lanes 4 and 6). The results ofseveral experiments in which Ab1 and Ab2 were tested are shownin Figure 6C. Although spliced adenoviral mRNA and 5S RNA arecomparably inhibited by both antibody types, U1 snRNA export wasconsistently less sensitive to Ab2 than to Ab1. This reveals thatthe export route of U1 has distinct requirements for Nup153 (seeDISCUSSION).

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Figure 6. Antibodies to distinct regions of Nup153 affect export differentially. (A) The domain structure of Xenopus Nup153 is represented schematically, showing the unique N-terminal region, the five zinc fingers, and the FG-containing C-terminal region. Antibody 1 (Ab1) was raised against a fragment containing part of the N-terminal region and one zinc finger (amino acids 53-334). Antibody 2 (Ab2) was raised against the remaining four zinc fingers and part of the FG region (amino acids 334-828). (B) Oocytes were injected as described in Figure 1, first with buffer or antibodies and then with radiolabeled RNA. The RNA mixture used here contained DHFR mRNA (an intronless mRNA), U1 snRNA, U6 snRNA, and tRNA. RNA localization was analyzed after a 4 h incubation. DHFR mRNA export was inhibited equally by Ab1 and Ab2, whereas U1 RNA export is significantly less sensitive to Ab2 (compare lanes 2, 4, and 6). (C) The effects of Ab1 and Ab2 are depicted in this bar chart in which data from multiple experiments are summarized. Inhibitory profiles of antibodies to distinct regions of Nup153 are shown here for the adenoviral mRNA (spliced), U1 snRNA, 5S rRNA, and tRNA.

Nup153 Associates with Poly(G) and Poly(U) Homoribopolymers

The central role of Nup153 in RNA export led us to ask whether Nup153 could associate, either directly or indirectly, withRNA. One method that has proven useful in detecting the affinityof a protein for RNA is to test its affinity for homoribopolymers.We therefore examined whether Nup153 could associate with poly(G),poly(C), poly(U), or poly(A) when the ribopolymer was coupledto a gel matrix. Extracts made from Xenopus eggs were incubatedwith each of the affinity matrices, as well as with control resinthat had no nucleotide attached. Binding was performed in thepresence or absence of the nonionic detergent NP-40. After a washcontaining heparin to reduce nonspecific binding, the proteinsassociated with each affinity matrix were subjected to gel electrophoresisand analyzed by immunoblotting using antisera to nucleoporins.Although several nucleoporins associated with the different ribopolymerbeads in the absence of NP-40 (Figure 7A, lanes 1, 3, 5, and 7),a substantial amount of the observed binding could be accountedfor by the background levels of association with control beads(Figure 7A, lane 9). In most cases, this binding activity waslost when NP-40 was added to the extract before incubation withthe resin (Figure 7A, lanes 2, 4, 6, and 8). However, Nup153 exhibiteda high level of association with poly(G) in the presence of NP-40(0.5%) (Figure 7A, lane 2) and a lesser but significant associationwith poly(U) under these conditions (Figure 7A, lane 8).

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Figure 7. Nup153 interacts, directly or indirectly, with poly(G) and poly(U). (A) Affinity resins bearing the homoribopolymer indicated (lanes 1-8) or resin alone (lanes 9 and 10; control [C]) were incubated with Xenopus egg extract in the absence (lanes 1, 3, 5, 7, and 9) or presence (lanes 2, 4, 6, 8, and 10) of 0.5% NP-40. After the beads were washed (see MATERIALS AND METHODS), proteins that remained associated were eluted in SDS sample buffer and analyzed by Western blot. mAb414 and antibodies specific for Nup98 were used to detect a panel of nucleoporins. Nup358, Nup214, Nup153, Nup98, and Nup60 are all detected in egg extract (Ext. [left], an amount equivalent to 28% of the material included in each incubation is loaded). Some nonspecific binding of Nup98 and Nup60 is found in the absence of NP-40 when the nucleoporins recovered with the control beads are examined (lane 9). Levels over this background binding are clearly detected for Nup153 with poly(G) (lane 1), and this binding is greatly augmented by the presence of NP-40 (lane 2). Nup153 also associated with poly(U) in the presence of NP-40 (lane 8). (B) A binding experiment similar to that described above was performed with a matrix bearing the poly(G) ribopolymer and an identical control matrix lacking ribopolymer. Nucleoporin recovery was examined in the presence of increasing amounts of KCl and with NP-40 (0.2%) present. Nup153 remained associated with poly(G) when the KCl concentration was as high as 300 mM (lane 3). The left panel of egg extract represents 16% of the loaded material.

This binding of Nup153 to poly(G) and poly(U) far exceeded that of the other nucleoporins. To be specific, Nup358 and Nup214did not appear to associate with any of the homoribopolymers evenin the absence of NP-40. Nup60 had binding levels marginally overbackground to poly(G) and poly(U) (Figure 7A, compare controllane 9 with lanes 1 and 7). Nup98 appeared to have low levelsof association with poly(G) and poly(U) compared with background,but for both Nup98 and Nup60, binding was disrupted by the presenceof NP-40.

To look further at the stringency of the interaction between Nup153 and poly(G), the association was examined in buffer containing0.2% NP-40 with increasing amounts of KCl. BSA (10 mg/ml) wasincluded to reduce any nonspecific association with the beads.Nup153 was detected bound to poly(G) at concentrations of saltup to 300 mM (Figure 7B, lanes 1-3), whereas the low levels ofNup98 and Nup60 binding to poly(G) were highly sensitive to salt(Figure 7B, lanes 1 and 2). These experiments demonstrate a significantassociation of Nup153 with poly(G) and suggest that Nup153 maylikewise associate with certain cellular RNAs, either by directbinding or indirectly by interacting with an adaptor or receptorprotein involved in export. Such a protein is likely to be presentin egg cytosol and would therefore be available if needed to bridgethe binding of Nup153 toRNA.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

To understand the process of nucleocytoplasmic trafficking, a major question that must be addressed is how traffic moves throughthe nuclear pore in a regulated, bidirectional manner. Littleis known of the way in which individual proteins of the pore contributeto this complex process, yet this information is key to dissectingthe mechanisms of transport. In this study, we have analyzed nuclearexport and the role of the nucleoporin Nup153, the only nucleoporinknown to be located on the distal ring of the pore basket, a locationencountered very early in the export process. Our results indicatethat Nup153 is a central component of the export machinery formultiple types of RNA and protein cargo. Specifically, antibodiesto Nup153 block the export of U1 snRNA, 5S RNA, spliced mRNA,and intronless mRNA. We find that Nup153 does not play the samecritical role in the export of tRNA. Thus, Nup153 plays a keyrole in specific paths of RNA export. Equally importantly, antibodiesagainst Nup153 were used to examine Rev protein export, as wellas Rev-mediated RNA export. In both cases, export was inhibited,demonstrating that Nup153 plays a role in NES protein export andNES-mediated RNA export. These results indicate that althoughthere may be mechanistic differences between NES protein exportand NES-mediated RNA export, Nup153 is critical to the exportof both types ofcargo.

To assess further whether other transport pathways through the pore are disrupted by antibodies bound to Nup153, we examinedtwo distinct routes of nuclear import. In this case, both NLS-and M9-mediated import pathways were found to be unperturbed bythe anti-Nup153 antibodies used here. We also examined the recyclingphase of nuclear import by analyzing the export of importin $beta$ to the cytoplasm. This factor was found to export normally inthe presence of our Nup153-specific antibodies. Consistent withthis observation, endogenous importin $beta$ remained in its primarilycytoplasmic location in the presence of the anti-Nup153 antibodies(our unpublished results); the antibodies would have caused relocalizationof importin $beta$ to nuclei if recycling had been inhibited. Our experimentsclearly demonstrate that, although antibodies disrupt a crucialfunction of Nup153 with respect to a number of export pathways,several modes of traffic through the pore continue to take placenormally. This underscores the specificity of the export blockwe see in the presence of anti-Nup153antibodies.

Nup153 has been found to be a major in vivo binding partner of importin $beta$ (Shah et al., 1998). A fragment of Nup153 containingthe first half of the FG region of Nup153 (equivalent to hNup153aa 976-1198), when added in excess, completely blocks importin $beta$ -mediated import in permeabilized cells. Moreover, a more N-terminalfragment of Nup153 (equivalent to hNup153 aa 431-723), when addedin excess, blocks transportin-mediated import (Shah and Forbes,1998). Both Nup153 fragments bind the respective receptors invitro. As such, Nup153 appears to play a role in the last stepsof import. The experiments here do not address the in vivo roleof the Nup153-import receptor interactions, because the Nup153antibodies used here do not interfere with the Nup153-importin $beta$ or Nup153-transportin interactions. This is clear from the findingthat the Nup153 antibodies coimmunoprecipitate importin $beta$ andtransportin (Shah and Forbes, 1998; Shah et al., 1998), indicatingthat the antibodies do not displace the import receptors fromNup153. Moreover, when the levels of Nup153 associated with exogenousimportin $beta$ in Xenopus extract were compared in the absence orpresence of our Nup153 antibodies, no significant differenceswere observed (our unpublished results). This was the case withboth Ab1 and Ab2, providing unequivocal evidence that the antibodiesdo not interfere with the Nup153-importin $beta$ interaction in eggextract. This is likely attributable to the fact that there aremultiple importin $beta$ -binding sites in the FG-repeat region of Nup153(Shah et al., 1998). Ab2 was raised to the proximal half of theFG region and is likely to bind exclusively to it, leaving thedownstream importin $beta$ -binding site accessible and functional forroles in $beta$ -mediated import and/or $beta$ recycling. Thus, the resultsillustrate that not only do the antibodies affect Nup153 specifically,they target only certain interactions involving this nucleoporin,those involved in the export of a specific subset ofcargo.

It is interesting that this subset of export pathways is blocked by two different anti-Nup153 antibodies, one raised to aunique proximal region of Nup153 plus the first of the Zn fingersand a second antibody raised to a more distal fragment consistingof a nonoverlapping portion of the Zn finger domain and the firsthalf of the FG region (Figure 6). Ab1 and Ab2 both inhibit theexport of multiple RNAs. However, one striking difference betweenthe antibodies is the relative refractory nature of the U1 exportpathway to Ab2 inhibition. Specifically, spliced adenoviral mRNA,intronless DHFR mRNA, and 5S RNA export were all inhibited comparablyby the two antibodies, but U1 snRNA export was only partiallyinhibited by Ab2. One straightforward interpretation of this resultis that the more C-terminal portion of Nup153 that is recognizedby Ab2 is not as important for the U1 export pathway as it isfor the mRNA and 5S export pathways. Alternately, some other propertyof Ab2, such as its overall affinity for Nup153, may result inan inefficient block of a Nup153 interaction needed for U1 export.Importantly, in either case, this suggests that Nup153 is eithernot as critical for U1 export or in fact plays different mechanisticroles in different paths ofexport.

How do the anti-Nup153 antibodies block export? A concern has been raised previously that any antibodies bound to the nuclearpore complex could cause a nonspecific steric inhibition to theexport (or import) of the large transport complexes (Ohno et al.,1998). The results here argue that the Nup153 antibodies in facthave a very specific effect on transport and that this effectis clearly independent of cargo size. For example, Rev proteinexport is inhibited although this is a small export substratebound to exportin 1 and the associated transport factor Ran-GTP(Fornerod et al., 1997a). However, the export of the tRNA-exportin-t-Ran-GTPcomplex, in the same size range as the Rev export complex, ishighly efficient in the presence of anti-Nup153 antibodies, asis the export of importin $beta$ . The antibodies therefore do not causegeneral steric interference at the pore but rather selectivelydisrupt interactions with Nup153 that are essential to the affectedcargo.

One probable candidate for the protein that must interact with Nup153 is the export receptor exportin 1. Exportin 1 (or Crm1)has been identified as a cognate receptor for leucine-rich NESs(Fornerod et al., 1997a; Fukuda et al., 1997; Neville et al.,1997; Ossareh-Nazari et al., 1997; Stade et al., 1997; Ullmanet al., 1997). Recent results have indicated that the export ofmany RNA classes, but not tRNA, is blocked by injection of excessleucine-rich NES sequences (Fischer et al., 1995; Pasquinelliet al., 1997b). This suggests that the 5S RNA, U snRNA, and likelymRNA export pathways use exportin 1. In turn, the anti-Nup153inhibition results reported here are consistent with a centralrole for an interaction between exportin and Nup153, an interactionthat is disrupted by anti-Nup153 antibodies. However, it remainsan open question as to whether an essential interaction of Nup153and exportin 1 or a different export factor is disrupted by theanti-Nup153 antibodies usedhere.

The export of tRNA is known to be mediated by a different export receptor, exportin-t (Arts et al., 1998; Hellmuth et al.,1998; Kutay et al., 1998). One would predict from the many differencesbetween tRNA export and the export of mRNA, snRNA, and 5S RNAthat exportin-t traverses the pore via a distinct route. Thisroute is clearly not disrupted by Nup153 antibodies (presentedhere) or by Nup98 antibodies (Powers et al., 1997). Presumably,exportin-t interacts with different nucleoporins. An alternatebut interesting possibility is that our Nup153 antibodies do notdisrupt some as yet undiscovered interaction of exportin-t withNup153. Precedence for receptor-Nup153 interactions that are notdisrupted by the Nup153 antibodies exists, as discussed above,between importin $beta$ and Nup153 (Shah et al., 1998) and betweentransportin and Nup153 (Shah and Forbes, 1998).

Limited data exist on which subdomains of Nup153 are required for participation in the export of RNA and protein cargos. Inan earlier study, Bastos et al. (1996) found that overexpressionof the FG domain of Nup153 in mammalian tissue culture cells causednuclear accumulation of poly(A)+ RNA, whereas transfection andexpression of the N-terminal or Zn finger domains did not. Theobserved effect on poly(A)+ RNA accumulation occurred despitethe fact that the overexpressed Nup153 FG domain was localizedto the cytoplasm. Although this suggested a role for the FG domainin export, because of the complex nature of the transfection approachand the delay before the phenotype could be assessed, it is notclear whether the poly(A)+ RNA accumulation observed was attributableto 1) a block in mRNA export, 2) inhibition of an earlier stepin mRNA biogenesis, such as splicing, or 3) an indirect effectcaused by blocking a specific, required import pathway. Furthermore,if accumulation was caused by a direct effect on mRNA export,it remained unanswered whether the effect was specific to mRNAor extended to other export substrates. We have now determinedthat Nup153 is in fact central to U1 snRNA, 5S rRNA, and splicedand intronless mRNA export, as well as to Rev and Rev-mediatedRNA export. The role of the FG domain was not specifically assessedin our experiments. Indeed, the inhibitory antibodies Ab1 andAb2 overlap in their reactivity with the Zn finger domain of Nup153,raising the new possibility that the Zn finger domain contributesto the export function of Nup153. However, because these antibodiesmay well exert their inhibitory effects by interfering with thefunction of other domains, detailed functional mapping of Nup153subregions will be essential in illuminating which Nup153 domain(s)actually interacts with exportcomplexes.

In the nucleus, Nup153 is found on the distal ring of the pore basket and also on intranuclear, pore-associated filaments(Cordes et al., 1993; Sukegawa and Blobel, 1993; Panté et al.,1994). An interesting consideration is whether Nup153 functionis different at these two locations. For example, Nup153 localizedto the intranuclear filaments might play a role in initiatingthe export process, whereas basket-associated Nup153 might functionprimarily in import. The provocative question as to whether suchfunctional distinctions exist between subpopulations of Nup153molecules is difficult to approach experimentally and awaits thedevelopment of specialized techniques foranalysis.

To search for clues to the mechanistic role that Nup153 plays in RNA export, we asked whether Nup153 could in fact associatewith RNA, either directly or indirectly. Toward this end, we testedwhether Nup153 in Xenopus egg extracts was able to bind RNA homopolymers.This approach is advantageous for two reasons: 1) an affinityfor RNA can be assessed without making assumptions about sequencepreference, and 2) the egg extract is likely to contain any adaptorproteins that may be needed to bridge the interaction of exportcomplexes with Nup153. In addition, this approach allowed us tocompare Nup153 simultaneously with several other nucleoporinspresent in the extract. We found that nucleoporins Nup358 andNup214 did not detectably bind to any of the RNA homopolymers.Nup60 bound marginally over background to poly(G) and poly(U),and low levels of Nup98 bound weakly over background to poly(G)and poly(U). In sharp contrast, Nup153 associated at a high levelwith poly(G) and to a lesser extent with poly(U). Interestingly,the nonionic detergent NP-40 significantly enhanced the Nup153binding observed, suggesting that a binding site could be furtherunmasked under theseconditions.

The yeast GLFG nucleoporins Nup145p and Nup116p have been reported to bind poly(G) and poly(U) (Fabre et al., 1994). The RNP1-likedomains thought to confer the RNA-binding property on yeast GLFGnucleoporins are also present in Nup98, the vertebrate homologueof the GLFG family, and are not present in Nup153. Yet, underthe conditions examined here Nup153 clearly associates much moretightly with RNA than does Nup98 and does so under more stringentconditions. There exists no obvious homologue of Nup153 for comparisonin yeast. It is possible that a role played by the GLFG familyof nucleoporins in yeast pores has been assumed by Nup153 in themuch larger and complex vertebrate pore. However, even in thecase of yeast Nup116p and Nup145p, only a small fraction of theinput nucleoporins bound to polyribonucleotide columns (Fabreet al., 1994), similar to the results seen here for the XenopusGLFG protein Nup98 (Figure 7). Thus, it is likely that the GLFGnucleoporins have only a low affinity for RNA in both lower andhigher eukaryotes. In contrast, up to ~30% of the Nup153 presentin the extract associated with poly(G) under the conditions usedhere (Figure 7A, lane 2). Nup153 contains several zinc fingers(five in Xenopus), which could potentially mediate a direct interactionwith RNA. Nup153 has, in fact, been found to interact with DNAin vitro in a Zn-dependent manner (Sukegawa and Blobel, 1993),although the implication of this DNA binding is unclear. Futurework will focus on determining whether Nup153 binds to RNA directlyor indirectly. At present, however, the RNA binding reveals animportant distinguishing property ofNup153.

In this context it is noteworthy that Jarmolowski et al. (1994) found that the nuclear injection of poly(G) into oocytes inhibitsmRNA, U1, and 5S RNA export, while tRNA export continues normally.In addition, poly(U) was found to have a small inhibitory effecton mRNA export. These homoribopolymers could well inhibit exportby disrupting a critical interaction, direct or indirect, betweenNup153 and RNA. The homoribopolymers might sequester adaptor proteinsthat are required to bridge the interaction of RNA and Nup153.Or, if Nup153 interacts directly with RNA, this nucleoporin coulditself be the target of inhibitory RNA homopolymers injected intooocytes. However, if Nup153 does interact directly with RNA, itmust have additional interactions with receptor-cargo export complexes,because Rev protein export is also inhibited by the Nup153antibodies.

To date, functional dissection of the vertebrate nuclear pore has been limited. A monoclonal antibody RL1 that recognizesa subset of nucleoporins containing N-acetylglucosamine was foundto inhibit NLS-directed nuclear import, as well as 5S and tRNAexport (Dabauvalle et al., 1988; Featherstone et al., 1988; Ternsand Dahlberg, 1994). Wheat germ agglutinin, a lectin that bindsto the same set of glycosylated nucleoporins, broadly inhibitsboth import and export (Finlay et al., 1987; Featherstone et al.,1988; Bataille et al., 1990; Neuman de Vegvar and Dahlberg, 1990).Interestingly, anti-Nup98 antibodies have a strong inhibitoryeffect on export (Powers et al., 1997), similar to that of theanti-Nup153 antibodies tested here. Specifically, mRNA, U1 snRNA,and 5S RNA export are inhibited by both anti-Nup98 and anti-Nup153antibodies, while tRNA export and nuclear import take place unabatedby the antibodies. These results suggest that Nup153 and Nup98are functionally linked as components of the export machinerythat is used by a subset of important export cargos. However,we have as yet found no indication that the two nucleoporins physicallyinteract with one another. Significantly, the RNA homopolymer-bindingexperiments indicate that Nup153 and Nup98 are likely to makevery different mechanistic contributions to nuclear export. Thus,Nup153 plays an important role as part of the export machineryof the pore and contributes in a specialized manner to the exportof multiple export substrates. It is now clear from the resultsof import studies (Shah and Forbes, 1998) and from the resultspresented here that multiple pathways of nuclear import and exportall converge on the basket of the nuclear pore atNup153.

	ACKNOWLEDGMENTS

The authors thank those mentioned in the MATERIALS AND METHODS for the gifts of plasmids, as well as Dr. Elsebet Lund forhelpful advice regarding oocyte microinjection, Dr. Sarah Guadagnofor the gift of anti-GST antibodies, and members of the Forbeslaboratory for insightful suggestions and discussions. This workwas supported by grants from the National Institutes of Health(2R01GM-33279) and American Cancer Society (RPG-96-086-03-CCG)to D.J.F., a Gann predoctoral fellowship grant to S.S., and aBurroughs Wellcome Career Award in Biomedical Sciences to K.S.U.

	FOOTNOTES

^* Corresponding author. E-mail address: katharine.ullman{at}hci.utah.edu.

Present addresses: Department of Oncological Sciences, Huntsman Cancer Institute, University of Utah, Salt Lake City, UT 84108; Department of Cell Biology, Emory University, Atlanta, GA30322.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERNCES

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The nucleoporin Nup60p functions as a Gsp1p-GTP-sensitive tether for Nup2p at the nuclear pore complex
J. Cell Biol., September 3, 2001; 154(5): 937 - 950.
[Abstract] [Full Text] [PDF]

N. Daigle, J. Beaudouin, L. Hartnell, G. Imreh, E. Hallberg, J. Lippincott-Schwartz, and J. Ellenberg
Nuclear pore complexes form immobile networks and have a very low turnover in live mammalian cells
J. Cell Biol., July 9, 2001; 154(1): 71 - 84.
[Abstract] [Full Text] [PDF]

W. Hofmann, B. Reichart, A. Ewald, E. Muller, I. Schmitt, R. H. Stauber, F. Lottspeich, B. M. Jockusch, U. Scheer, J. Hauber, et al.
Cofactor Requirements for Nuclear Export of Rev Response Element (Rre)-And Constitutive Transport Element (Cte)-Containing Retroviral Rnas: An Unexpected Role for Actin
J. Cell Biol., March 5, 2001; 152(5): 895 - 910.
[Abstract] [Full Text] [PDF]

J. M. Petersen, L.-S. Her, V. Varvel, E. Lund, and J. E. Dahlberg
The Matrix Protein of Vesicular Stomatitis Virus Inhibits Nucleocytoplasmic Transport When It Is in the Nucleus and Associated with Nuclear Pore Complexes
Mol. Cell. Biol., November 15, 2000; 20(22): 8590 - 8601.
[Abstract] [Full Text] [PDF]

B. Fahrenkrog, W. Hübner, A. Mandinova, N. Panté, W. Keller, and U. Aebi
The Yeast Nucleoporin Nup53p Specifically Interacts with Nic96p and Is Directly Involved in Nuclear Protein Import
Mol. Biol. Cell, November 1, 2000; 11(11): 3885 - 3896.
[Abstract] [Full Text]

C. M. Lane, I. Cushman, and M. S. Moore
Selective Disruption of Nuclear Import by a Functional Mutant Nuclear Transport Carrier
J. Cell Biol., October 16, 2000; 151(2): 321 - 332.
[Abstract] [Full Text] [PDF]

T. Guan, R. H. Kehlenbach, E. C. Schirmer, A. Kehlenbach, F. Fan, B. E. Clurman, N. Arnheim, and L. Gerace
Nup50, a Nucleoplasmically Oriented Nucleoporin with a Role in Nuclear Protein Export
Mol. Cell. Biol., August 1, 2000; 20(15): 5619 - 5630.
[Abstract] [Full Text] [PDF]

M. Smitherman, K. Lee, J. Swanger, R. Kapur, and B. E. Clurman
Characterization and Targeted Disruption of Murine Nup50, a p27Kip1-Interacting Component of the Nuclear Pore Complex
Mol. Cell. Biol., August 1, 2000; 20(15): 5631 - 5642.
[Abstract] [Full Text] [PDF]

T Haraguchi, T Koujin, T Hayakawa, T Kaneda, C Tsutsumi, N Imamoto, C Akazawa, J Sukegawa, Y Yoneda, and Y Hiraoka
Live fluorescence imaging reveals early recruitment of emerin, LBR, RanBP2, and Nup153 to reforming functional nuclear envelopes
J. Cell Sci., January 3, 2000; 113(5): 779 - 794.
[Abstract] [PDF]

M.-j. Luo and R. Reed
From the Cover: Splicing is required for rapid and efficient mRNA export in metazoans
PNAS, December 21, 1999; 96(26): 14937 - 14942.
[Abstract] [Full Text] [PDF]

C. Dimaano, J. R. Ball, A. J. Prunuske, and K. S. Ullman
RNA Association Defines a Functionally Conserved Domain in the Nuclear Pore Protein Nup153
J. Biol. Chem., November 21, 2001; 276(48): 45349 - 45357.
[Abstract] [Full Text] [PDF]

J. P. Rodrigues, M. Rode, D. Gatfield, B. J. Blencowe, M. Carmo-Fonseca, and E. Izaurralde
REF proteins mediate the export of spliced and unspliced mRNAs from the nucleus
PNAS, January 30, 2001; 98(3): 1030 - 1035.
[Abstract] [Full Text] [PDF]

J. M. Petersen, L.-S. Her, and J. E. Dahlberg
Multiple vesiculoviral matrix proteins inhibit both nuclear export and import
PNAS, July 17, 2001; 98(15): 8590 - 8595.
[Abstract] [Full Text] [PDF]

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				M.-j. Luo and R. Reed From the Cover: Splicing is required for rapid and efficient mRNA export in metazoans PNAS, December 21, 1999; 96(26): 14937 - 14942. [Abstract] [Full Text] [PDF]

				C. Dimaano, J. R. Ball, A. J. Prunuske, and K. S. Ullman RNA Association Defines a Functionally Conserved Domain in the Nuclear Pore Protein Nup153 J. Biol. Chem., November 21, 2001; 276(48): 45349 - 45357. [Abstract] [Full Text] [PDF]

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