NS1-Binding Protein (NS1-BP): a Novel Human Protein That Interacts with the Influenza A Virus Nonstructural NS1 Protein Is Relocalized in the Nuclei of Infected Cells

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Journal of Virology, September 1998, p. 7170-7180, Vol. 72, No. 9
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

NS1-Binding Protein (NS1-BP): a Novel Human Protein That Interacts with the Influenza A Virus Nonstructural NS1 Protein Is Relocalized in the Nuclei of Infected Cells

Thorsten Wolff,¹^,^* Robert E. O'Neill,² and Peter Palese²

Institut für Virologie, Philipps-Universität Marburg, 35037 Marburg, Germany,¹ and Department of Microbiology, Mount Sinai School of Medicine, New York, New York 10029²

Received 24 February 1998/Accepted 27 May 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

We used the yeast interaction trap system to identify a novel human 70-kDa protein, termed NS1-binding protein (NS1-BP), whichinteracts with the nonstructural NS1 protein of the influenzaA virus. The genetic interaction was confirmed by the specificcoprecipitation of the NS1 protein from solution by a glutathioneS-transferase-NS1-BP fusion protein and glutathione-Sepharose.NS1-BP contains an N-terminal BTB/POZ domain and five kelch-liketandem repeat elements of ~50 amino acids. In noninfected cells,affinity-purified antibodies localized NS1-BP in nuclear regionsenriched with the spliceosome assembly factor SC35, suggestingan association of NS1-BP with the cellular splicing apparatus.In influenza A virus-infected cells, NS1-BP relocalized throughoutthe nucleoplasm and appeared distinct from the SC35 domains, whichsuggests that NS1-BP function may be disturbed or altered. Theaddition of a truncated NS1-BP mutant protein to a HeLa cell nuclearextract efficiently inhibited pre-mRNA splicing but not spliceosomeassembly. This result could be explained by a possible dominant-negativeeffect of the NS1-BP mutant protein and suggests a role of thewild-type NS1-BP in promoting pre-mRNA splicing. These data suggestthat the inhibition of splicing by the NS1 protein may be mediatedby binding to NS1-BP.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Replication of viruses can induce drastic changes in the metabolism of the infected host cell. The analysis of the replicationcycle of viruses by molecular biological techniques has facilitatedthe identification and study of viral gene products which modulateand affect cellular functions (31). A well-studied example isthe NS1 protein of influenza A viruses. The NS1 protein is theonly nonstructural protein of the virus and is abundantly expressedin infected cells (35). Several regulatory functions of theNS1 protein have been identified. The NS1 protein influences multiplesteps of gene expression, including pre-mRNA splicing (19, 36),nucleocytoplasmic transport of poly(A) RNA (19, 48), and translation(9, 15). In addition, it was recently shown that NS1 canblock the activation of the double-stranded RNA-activated proteinkinase (PKR), presumably due to its double-stranded RNA bindingactivity (37). The activation of PKR results in a downregulationof translation and is part of the cellular antiviral defense mechanism.The NS1 protein may counteract this cellular response in orderto synthesize high levels of viral proteins in the infected cell(37). These pleiotropic effects may, singly or combined, providethe molecular basis for the role which the NS1 protein plays indetermining the host range and virulence of influenza virus strains(54, 61).

Despite the plethora of activities identified in NS1, little is known about the cellular factors that are recognized by theNS1 protein and that may therefore be central to NS1 functions.We have used the yeast interaction trap (26, 74) to screenfor cellular proteins that interact with the NS1 protein. Herewe report on the identification and characterization of a novelhuman 70-kDa protein, termed NS1-binding protein (NS1-BP). Innoninfected cells, NS1-BP was found to accumulate in discretenuclear domains which are enriched with pre-mRNA splicing factors.However, in influenza A virus-infected cells, NS1-BP relocalizedthroughout the nucleoplasm. The addition of a truncated NS1-BPinhibited pre-mRNA splicing in HeLa cell nuclear extracts in vitro,possibly as the result of a dominant-negative effect on the endogenousprotein. These results suggest a role for NS1-BP in pre-mRNA splicingand support a model in which the NS1-NS1-BP interaction has arole in mediating the splicing-inhibitory effect of the NS1 protein.

	MATERIALS AND METHODS

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Viruses, cells, and extracts. Influenza A/WSN/33 virus was grown in the allantoic cavities of 10-day-old embryonated chicken eggs. HeLa, HEp-2, and 293cells were passaged in Dulbecco's modified Eagle's tissue culturemedium (DMEM) containing 10% fetal calf serum. For immunoblotanalysis, confluent cell monolayers grown in 35-mm dishes werelysed in radioimmunoprecipitation assay buffer containing 150mM NaCl, 1.0% Nonidet P-40 (NP-40), 0.5% deoxycholate, 0.1% sodiumdodecyl sulfate (SDS), and 50 mM Tris-HCl (pH 8.0). Lysates wereclarified by centrifugation for 10 min at 13,000× g, and supernatantswere used for immunoblot analysis.

Yeast strains, E. coli strains, and plasmids. Escherichia coli strains used for cloning and expression were MH3 (trpC araD lacX hsdR galU galK), DH5 $alpha$ [F $Phi$ 80dlacZ $Delta$ M15 $Delta$ (lacZYA-argF)U169 deoR recA1 endA1 hsdR17 (r_K m_K⁺) supE44 $lambda$ thi-1 gyrA96 relA1], BL26 [F ompT hsdS_B (r_B m_B) gal dcm], and XL1-Blue recA1 endA1 gyrA96 thi-1 hsdR17 supE44relA1 lac [F' pro AB lacI^qZ $Delta$ M15 Tn10 (Tet^r)].

Saccharomyces cerevisiae EGY48 (MATa trp1 ura3 his3 LEU2::pLEX-Aop6-LEU2), plasmids pSH18-34 and pRFHM1, and the HeLacell cDNA expression library constructed in pJG4-5 were kindlyprovided by R. Brent (Harvard Medical School) and have been describedpreviously (26, 74). The constructions of plasmids pLexA-NS1,pcDNA3-NS1, and pGEX-NS1 have been described elsewhere (69).SP6-MINX (75) was used as a template for transcription of syntheticpre-mRNA. Construction of plasmids followed standard cloning procedures(2). Plasmid pGEX-NS1-BP was made by subcloning the HeLa cDNAfrom the library plasmid (see below) into pGEX-5X-1 (Pharmacia).The bacterial expression plasmids pGEX-NS1-BP-REP and pMAL-NS1-BP-REPwere generated by inserting NS1-BP cDNA corresponding to aminoacids 1 to 368 (nucleotide positions 1 to 1104) between the EcoRI/XhoIsites of pGEX-5X-1 and the EcoRI/SalI sites of pMAL-c2 (New EnglandBiolabs), respectively.

Identification and isolation of NS1-interacting cDNA clones using the yeast interaction trap. The yeast interaction trap was used to identify and to isolate HeLa cell cDNAs encoding NS1 binding factors as was previouslydescribed (69). In brief, EGY48 was transformed with the baitplasmid pLexA-NS1 and the lacZ reporter plasmid pSH18-34. Subsequently,this strain was transformed with a plasmid library in which HeLacell cDNAs were conditionally expressed as fusions with an acidicactivation domain from a GAL1 promoter. A total of 3.3 × 10⁵ primary transformants were screened for interaction, as determinedby their ability to grow on minimal synthetic medium in the absenceof leucine and to activate the lacZ reporter gene specificallyon plates containing galactose but not glucose. The library plasmidp59-1 was isolated from one selected clone by transformation inE. coli MH3 as described elsewhere (44). The specificity ofthe interaction was examined by retransformation of p59-1 intoEGY48 harboring pSH18-34 together with pLexA-NS1 or with pRFHM1,which expresses an unrelated fusion of LexA with the bicoid proteinof Drosophila melanogaster. p59-1 activated the lacZ reportergene specifically in the presence of galactose in combinationwith pLexA-NS1 but not in combination with pRFHM1. p59-1 was sequencedby using a standard chain termination protocol. p59-1 originatedfrom the same screen that led to the isolation of cDNA correspondingto another NS1-interacting protein, NS1-I, as described elsewhere(69).

Cloning of NS1-BP 5' end cDNA. cDNA corresponding to the 5' end of NS1-BP mRNA was obtained by a 5'-RACE (rapid amplification of cDNA ends) procedure usinga 5'-RACE kit (Gibco-BRL). The 59-1-specific DNA oligonucleotide59GSP1 (dCATTCCTCTCTGTTATAGCC, corresponding to positions 1123to 1142 of NS1-BP cDNA; 2.5 pmol) was hybridized to 1 µg of HeLapoly(A)⁺ RNA to prime first-strand cDNA synthesis by Moloney murine leukemiavirus reverse transcriptase. The cDNA was tailed with dC by usingterminal transferase. The product was used as a template to amplifydouble-stranded cDNA by PCR with the nested primer 59GSP2 (dCCACCTGCAGCTATGAG,positions 1108 to 1124) and the 5'-RACE anchor primer. The resultingproduct was subcloned into pGEM-T (Promega) to generate pGEM-NS1-BP-5'RACEplasmids. The NS1-BP cDNA was sequenced by the standard dideoxymethod.

Northern blot analysis. One microgram of HeLa cell poly(A)⁺ RNA was electrophoresed on a 1% agarose-formaldehyde gel, transferred onto a Nytran (Amersham)nylon membrane, and immobilized by UV cross-linking. A ³²P-labeled NS1-BP-specific probe comprising positions 1038 to 2215was used to detect NS1-BP mRNA by hybridization as described elsewhere(2).

Coprecipitation of NS1 protein with GST-NS1-BP by glutathione-Sepharose. NS1-BP (amino acids 347 to 619) was expressed from pGEX-NS1-BP as a glutathione S-transferase (GST) fusion protein in E. coliBL26. Synthesis of GST-NS1-BP was induced by the addition of 1mM isopropyl- $beta$ -D-galactopyranoside (IPTG). Bacterial cell lysatecontaining the GST-NS1-BP fusion protein was adsorbed to glutathione-Sepharose(Pharmacia) according to the protocol supplied by the manufacturer.Contaminating proteins were removed by three washes with phosphate-bufferedsaline (PBS). NS1 protein was synthesized and labeled with [³⁵S]methionine in coupled 50-µl transcription-translation reactions(TNT; Promega), programmed with pcDNA3-NS1. The translation reactionwas mixed with 10 µl of coated glutathione-Sepharose beads in750 µl of HN100 buffer (20 mM HEPES [pH 8.0], 100 mM NaCl, 0.01%NP-40) for 2 h at 4°C. The beads were washed three times withPBS-0.01% NP-40, and the precipitated proteins were separatedby SDS gel electrophoresis and visualized by autoradiography.

Anti-NS1-BP-serum and immunoblot analyses. The GST-NS1-BP-REP fusion protein, carrying amino acids 1 to 368 of NS1-BP, was expressed in E. coli BL26 transformed withpGEX-NS1-BP-REP and affinity purified on glutathione-Sepharoseresin (Pharmacia) as recommended by the manufacturer. A 6-month-oldfemale rabbit was immunized with 400 µg of purified GST-NS1-BP-REPfusion protein in complete Freund's adjuvant followed by boosterinjections of 250 µg of fusion protein in incomplete adjuvantat 4-week intervals. NS1-BP-specific antibodies were purifiedfrom serum by affinity chromatography using an antigen resin.For the construction of this matrix, a MAL-NS1-BP-REP fusion protein,in which the maltose-binding protein of E. coli was fused to aminoacids 1 to 368 of NS1-BP, was expressed in E. coli XL1-Blue cellsand affinity purified on an amylose affinity column (New EnglandBiolabs). The MAL-NS1-BP-REP fusion protein was immobilized onCNBr-activated Sepharose (Pharmacia), and the resulting resinwas used for the affinity purification of NS1-BP-specific antibodiesas described elsewhere (28). The purified antibodies were diluted1:200 for immunoblot experiments using standard procedures (28).

Indirect immunofluorescence microscopy. HeLa cells were grown to 50% confluency on glass coverslips in D-MEM containing 10% fetal calf serum. Where indicated, cellswere infected at a multiplicity of 10 with influenza A/WSN/33virus diluted in PBS for 1 h at 37°C. Infection was continuedin tissue culture medium at 37°C. Cells were processed for immunofluorescenceanalysis by fixation in 2.5% methanol-free formaldehyde (PolysciencesInc.) diluted in PBS, and cells were permeabilized in 0.1% TritonX-100 as described elsewhere (69). Cells were stained with primaryantibodies diluted in PBS-3% bovine serum albumin. Affinity-purifiedanti-NS1-BP antibodies and the NS1-specific monoclonal antibodyIA7 (a kind gift of Jonathan Yewdell, National Institutes of Health)were used at 1:100 dilutions. The anti-SC35 antibody (21) waspurchased from Pharmingen Inc. and used at a dilution of 1:1,000.The cells were washed and incubated with fluorescein isothiocyanate(FITC)-conjugated sheep anti-rabbit immunoglobulin G (IgG) and/orTexas red-conjugated goat anti-mouse IgG. Subsequently, the coverslipswere washed and mounted in Mowiol 4-88 (Calbiochem) as describedelsewhere (28). For conventional immunofluorescence analysis,cells were viewed on a Zeiss Axiovert 100 fluorescence microscopewith a 63× objective, and photographs were captured by a CF8/10×video camera (Kappa GmbH). A Zeiss LSM 410 Invert microscope equippedwith a 100× objective lens was used for confocal laser scanningmicroscopy. Digitized images were pseudocolored by using Photoshopsoftware (Adobe Systems Inc.).

Spliceosome assembly and splicing of a ³²P-labeled pre-mRNA in the presence of GST proteins. GST, GST-NS1, and GST-NS1-BP fusion proteins were expressed in E. coli BL26 and affinity purified on glutathione-Sepharose(Pharmacia) columns as recommended by the manufacturer. GST proteinswere eluted with 20 mM glutathione in 50 mM Tris-HCl (pH 8.0),dialyzed against buffer D (20 mM HEPES [pH 8.0], 100 mM KCl, 20%glycerol, 0.2 mM EDTA, 0.5 mM dithiothreitol), and stored at $-$ 80°C.The purity of the prepared proteins was tested by SDS gel electrophoresisand staining with Coomassie blue. HeLa cell nuclear extract wasprepared as described elsewhere (12). ³²P-labeled MINX pre-mRNA (an artificial mini-exon construct derivedfrom the major late transcription unit of adenovirus 2) was synthesizedas described elsewhere (68). In a typical splicing reaction,4 ng of pre-mRNA was incubated in a 100-µl volume containing 40%HeLa cell nuclear extract, 3.2 mM MgCl₂, 0.5 mM ATP, 20 mM phosphocreatine,and 60 mM KCl. Eight micrograms of GST or equimolar amounts ofGST fusion proteins were added where indicated, and the reactionswere incubated at 30°C. The formation of splicing complexes wasanalyzed after treatment with heparin (1 mg/ml) by electrophoresison native acrylamide-agarose gels (43). For RNA analysis, splicingproducts were purified and analyzed by electrophoresis on denaturing13% acrylamide-urea gels.

Sequence comparisons. The NS1-BP cDNA and its derived amino acid sequence were compared to the GenBank and EMBL databases by using FASTA and TFASTAsoftware (10). The PILEUP and PRETTY programs of the GeneticsComputer Group (GCG) (University of Wisconsin, Madison) were usedto align the repeat elements of NS1-BP and to create a consensussequence.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Isolation of NS1 binding factors. The yeast interaction trap system (26, 74) was used to identify cellular proteins that bind to the NS1 protein of theinfluenza A virus (69). We used a constitutively expressed LexA-NS1fusion protein to screen a HeLa cell cDNA plasmid library, inwhich cDNA-encoded proteins were conditionally expressed as translationalfusions with an acidic activation domain from a GAL1 promoter.Expression of the acidic domain fusion proteins is induced inthe presence of galactose and repressed by glucose. A total of3.3 × 10⁵ primary yeast transformants were screened for the galactose-dependentactivation of LEU2 and lacZ reporter genes, which are regulatedby LexA-specific operator sites. Three library plasmids were isolatedfrom selected transformants that reproduced the interacting phenotypeupon retransformation with pLexA-NS1, but not with the controlplasmid pRFHM1. Here we report on the analysis of the human cDNAisolated through one of these library plasmids, p59-1, which encodesa novel human protein, NS1-BP.

Cloning and analysis of NS1-BP cDNA. p59-1 had a 1.2-kb cDNA insert containing one long open reading frame of 819 bp followed by 338 bp of an untranslated regionthat terminated in a run of 20 adenosines (Fig. 1). Northern blotanalysis of HeLa cell poly(A) RNA was used to determine if thesize of the isolated HeLa cDNA corresponded to a complete copyof NS1-BP mRNA. A ³²P-labeled NS1-BP-specific probe hybridized mainly to an RNA speciesof approximately 3.1 kb (Fig. 2). This result suggested that p59-1carried an incomplete copy of NS1-BP mRNA. We used a 5'-RACE procedureto generate cDNA derived from the 5' end of NS1-BP mRNA. The RACEproducts were subcloned, and six resulting plasmid clones wereisolated and sequenced. The longest 5'-RACE clone extended theNS1-BP cDNA to a total of 2,752 bp (Fig. 1). Sequence analysisrevealed the presence of one long open reading frame of 1,857nucleotides that encodes a 619-amino-acid protein with a predictedmolecular mass of 69.7 kDa. The initiator ATG codon of the openreading frame is in a sequence context which is compatible withbeing a translational start site (34). Analysis of the sequenceof NS1-BP revealed the presence of five imperfect repeat elementsof 47 to 49 amino acids at the C-terminal region between aminoacids 368 and 607 (Fig. 3). These tandem repeats are 18 to 41%identical to each other, and five positions are invariant betweendomains.

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FIG. 1. Nucleotide sequence of NS1-BP cDNA and derived amino acid sequence. The sequence of 2,752 nucleotides was determined by sequencing of two overlapping clones. Nucleotides at positions +1038 to +2215 are derived from the HeLa cDNA insert of the library plasmid p59-1. The 5' end of the library cDNA is indicated by an arrow. Nucleotides $-$ 537 to +1037 were determined by sequencing cloned HeLa cDNA that was generated by 5'-RACE. The open reading frame of 619 amino acids spans positions +1 to +1857. The stop codon is marked by a star.

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FIG. 2. Northern blot analysis of poly(A)-selected HeLa cell RNA with an NS1-BP-specific probe. One microgram of HeLa cell poly(A) RNA was separated by formaldehyde-agarose gel electrophoresis and immobilized on a nylon membrane. A ³²P-labeled probe derived from p59-1 was used to detect NS1-BP mRNA by hybridization. RNA size markers are indicated to the left.

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FIG. 3. Alignment of the five tandem repeat elements of NS1-BP. The PILEUP program of the GCG was used to align repetitive sequences between amino acids 368 and 607 of NS1-BP. The PRETTY program of the GCG was used to determine a consensus sequence (Consens.). Capital letters, conserved amino acids; boldface letters, invariant residues.

The cDNA and the deduced amino acid sequence of NS1-BP were compared to sequences in the GenBank and EMBL databases by usingthe FASTA and TFASTA algorithms (10). Two regions of NS1-BPwhich had homology to other proteins were identified. First, theN-terminal ~120 amino acids of NS1-BP are homologous to the BTB(bric-a-brac, tramtrack, broad complex)/POZ (poxviruses and zincfingers) domain that has been identified in several zinc fingerproteins known to act as transcriptional regulators (3, 76).Second, the five tandem repeats located between NS1-BP residues368 and 607 are homologous to the 50-amino-acid kelch motif thatwas originally found in the Drosophila Kelch protein (5, 71).The Kelch protein is a component of the intercellular ring canalsin the Drosophila egg chamber. Its function is required for thedevelopment of fertile oocytes, since mutations in the kelch genecan cause a sterile phenotype in females (71). Interestingly,the Kelch protein also contains a predicted BTB/POZ domain. Intotal, the amino acid sequence of NS1-BP is 31% identical to thatof Kelch.

Several other proteins which have both kelch and BTB/POZ domains were identified. These include the murine ENC-1 protein,which is specifically expressed in the nervous system (29),human and bovine calicin, which are components of the mammaliansperm head (65), the predicted product of the human KIAA0132gene (42), and the proteins encoded by genes of vaccinia virus(A55R, C2L, and F3L) (22), the Shope fibroma virus (T6, T8,and T9) (62), variola major virus (D16L, C7L, J6R, and B20R)(40), and swinepox virus (C4L and C13L) (39). The functionsof the viral gene products are not known. Several cellular kelchrepeat proteins containing no BTB/POZ domains were found, includingthe $alpha$ - and $beta$ -scruin proteins, which are expressed in the spermof the horseshoe crab Limulus polyphemus (66, 67), and theproducts of the mouse intracisternal A particle-promoted placenta(MIPP) gene (7) and the spe-26 gene of Caenorhabditis elegans(64).

The NS1 protein binds to NS1-BP in vitro. To confirm the interaction of NS1 and NS1-BP, in vitro binding assays were performed. NS1-BP cDNA isolated through the libraryplasmid in the interaction trap screen (corresponding to NS1-BPamino acids 347 to 619) was fused to the GST gene in a bacterialexpression vector. GST-NS1-BP fusion protein was expressed inE. coli and adsorbed to glutathione-Sepharose beads. As a control,we prepared glutathione-Sepharose beads complexed with GST proteinalone. The NS1 protein was synthesized in vitro and labeled with[³⁵S]methionine through coupled transcription-translation reactionsin reticulocyte lysates. The coated glutathione-Sepharose beadswere incubated with the radiolabeled NS1 protein. The NS1 proteinwas efficiently precipitated by the GST-NS1-BP fusion proteinbut not by GST (Fig. 4, lanes GST and GST-NS1-BP). This resultconfirms the yeast two-hybrid data and shows that the viral NS1protein can also physically interact with the cellular NS1-BP.

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FIG. 4. Precipitation of ³⁵S-labeled NS1 protein by GST-NS1-BP fusion protein. Radiolabeled NS1 protein was synthesized in coupled transcription-translation reactions in the presence of [³⁵S]methionine by using pcDNA3-NS1 as a template. The NS1 protein was precipitated by glutathione-Sepharose beads coated with GST (lane GST) or GST-NS1-BP, which carries amino acids 347 to 619 of NS1-BP (lane GST-NS1-BP). The precipitates were analyzed by SDS-polyacrylamide gel electrophoresis and autoradiography. A 10% aliquot of the total reaction was separated in parallel (lane T). The positions of molecular weight markers (in thousands) are indicated to the left.

NS1-BP is concentrated in intranuclear domains enriched with splicing factors. Polyclonal rabbit antibodies were raised against recombinant NS1-BP and used to analyze the concentration and intracellularlocalization of NS1-BP in mammalian cells. Immunoblot analysesof the human epithelium-derived HEp-2, 293, and HeLa cell linesby NS1-BP-specific antibodies detected a protein doublet bandwith a molecular mass of about 70 kDa (Fig. 5). This is the predictedsize for a protein derived from the NS1-BP open reading frame.Two minor protein bands migrating at 65 and 50 kDa were stainedat variable intensities and may correspond to NS1-BP breakdownproducts. NS1-BP-specific antibodies were affinity purified fromimmune serum and used for immunofluorescence analysis. In HeLacells, a punctate nuclear staining pattern that excluded the nucleoliwas observed (Fig. 6). In addition, a weak, diffuse staining ofthe cytoplasm was reproducibly seen. The nuclear staining of NS1-BPwas similar in appearance to the "speckled" pattern that was obtainedby immunofluorescence staining of cells with antibodies directedagainst factors involved in pre-mRNA splicing (59). The speckledomains correspond ultrastructurally to interchromatin granulesand perichromatin fibrils and are enriched with splicing snRNPsand non-snRNP splicing factors like SC35 and other serine-arginine-rich(SR) proteins (reviewed in reference 58). To determine how NS1-BPlocalization relates to speckle domains, we double-immunostainedHeLa cells with NS1-BP-specific antibodies and a monoclonal antibodyraised against the spliceosome assembly factor SC35, which isa known component of speckle domains (21). Confocal laser scanningmicroscopy demonstrated that the dot-like nuclear NS1-BP signalcolocalized with the SC35 signal (Fig. 7A through C). The concentrationof multiple proteins involved in pre-mRNA processing in thesenuclear regions suggests an important role of this compartmentfor cellular RNA biogenesis (55). The accumulation of NS1-BPin the same compartment suggests that NS1-BP may be a componentof the cellular splicing machinery.

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FIG. 5. Immunoblot analysis of NS1-BP. Confluent monolayers of HEp-2, 293, and HeLa cells were lysed in radioimmunoprecipitation assay buffer. Soluble proteins from equivalent volumes of extract corresponding to 5 × 10⁴ cells were separated by SDS gel electrophoresis, transferred to a nitrocellulose membrane, and probed with affinity-purified NS1-BP-specific antibodies. The positions of marker proteins (in kilodaltons) are indicated to the left.

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FIG. 6. Intracellular localization of NS1-BP as determined by indirect immunofluorescence analysis of HeLa cells. Subconfluent HeLa cells were fixed and stained with affinity-purified NS1-BP-specific rabbit antibodies, followed by visualization using FITC-conjugated secondary antibodies.

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FIG. 7. Intracellular distribution of cellular NS1-BP, the SC35 protein, and the viral NS1 protein in noninfected or influenza A virus-infected HeLa cells. Confocal micrographs show noninfected (A through C) or influenza A/WSN/33 virus-infected HeLa cells at 10 h postinfection (D through I). The intranuclear localization of NS1-BP was visualized by staining with NS1-BP-specific primary rabbit antibodies and FITC-conjugated secondary antibodies (A, D, and G). The cellular SC35 protein (B and H) and the viral NS1 protein (E) were labeled by monoclonal mouse antibodies and visualized by Texas red-conjugated anti-mouse IgG. Micrographs in the right column (C, F, and I) show confocal overlays of the FITC and Texas red signals from the left and middle columns.

NS1-BP relocalizes to the entire nucleoplasm in influenza A virus-infected cells. The viral NS1 protein accumulates in the nuclei of cells infected with influenza A virus (24, 72). We examined whetherthe speckled nuclear localization of cellular NS1-BP would beaffected in virus-infected cells expressing the NS1 protein. InfluenzaA virus-infected cells were double-immunostained with antibodiesdirected against NS1-BP and either the viral NS1 or the cellularSC35 protein (Fig. 7). As expected, the NS1 protein localizedpredominantly to the nucleoplasm, with some additional nucleolarsignal (Fig. 7E). For the NS1-BP staining, a remarkable changewas observed after infection by influenza virus. The cellularNS1-BP was no longer found concentrated in the nuclear specklesbut was instead distributed throughout the nucleoplasm. Its distributionpattern was similar to that of the viral NS1 protein except thatthere was no nucleolar signal (Fig. 7D and F). This redistributionof NS1-BP was observed in a few cells as early as 4 h postinfection.With ongoing infection, most of the cells expressing the viralNS1 protein had an NS1-BP staining pattern similar to that shownin Fig. 7D. The intensity of the nuclear NS1-BP signal appearedto increase slightly in infected cells. However, we did not detectan increase in the amount of NS1-BP in virus-infected cells byimmunoblotting (data not shown). This suggests that NS1-BP epitopesare more easily accessible to antibodies in the nuclei of infectedcells.

The intranuclear relocalization of NS1-BP in infected cells raised the question of whether the distribution of other proteinswhich normally localize to speckles would also change. Gross redistributionof proteins might occur if speckles break down during influenzavirus infection. However, the staining of virus-infected cellswith anti-SC35 antibody at 10 h postinfection (Fig. 7H) showedonly a small change from the normal pattern. The average sizeof the speckles appeared to be slightly decreased, with a concomitantincrease in the number of these domains. Essentially the sameobservation was made in a previous study that examined the distributionof splicing factors in influenza A virus-infected cells (20).These findings suggest that the redistribution of NS1-BP to thenucleoplasm in infected cells is not merely a consequence of speckledisintegration. It is tempting to speculate that cellular NS1-BPis relocalized via the binding to the viral NS1 protein. The intracellularrelocalization is likely to have an impact on NS1-BP functionin virus-infected cells.

A truncated NS1-BP protein inhibits pre-mRNA splicing at a step after spliceosome assembly. It has been demonstrated that the NS1 protein can inhibit pre-mRNA splicing in vivo and in vitro (19, 36). The block insplicing was assigned to a step after the assembly of spliceosomes,but before the first catalytic event (36). We hypothesized thatthe binding of the NS1 protein to a cellular protein(s) whosefunction is essential for splicing leads to the observed blockin splicing. Given the intranuclear colocalization of NS1-BP withwell-known factors of the mRNA splicing apparatus, we wonderedif NS1-BP could play a role in pre-mRNA splicing, as analyzedby in vitro splicing assays using HeLa cell nuclear extracts.We decided to use a truncated NS1-BP (amino acid positions 347to 619) in the form of a GST-NS1-BP fusion protein as a potentialdominant-negative inhibitor of the endogenous NS1-BP. Such a strategyhas been used previously to examine a functional role of a proteinin RNA splicing (73).

The splicing of a ³²P-labeled pre-mRNA in HeLa cell nuclear extracts was analyzed in the presence of GST-NS1-BP, GST-NS1, orcontrol GST protein (Fig. 8). We also examined the formation ofheparin-resistent splicing complexes in the same reactions bynative gel electrophoresis. In the control reaction, the intronlariat-exon 2 splicing intermediate was easily detected aftera 1-h incubation. At the 2-h time point, the accumulation of splicedmRNA and the intron lariat was observed (Fig. 8A, lanes NE). Nativegel electrophoresis showed that both A- and B-type spliceosomeswere formed normally at 20, 40, and 60 min, with a higher proportionof radiolabeled mRNAs shifting into B-complex bands at later timepoints (Fig. 8B, lanes NE). The A complex contains U2 snRNP, andthe B complex, which represents the fully assembled spliceosome,contains the U2, U4/U6, and U5 snRNPs (32). H represents a heterogenousclass of RNA-protein complexes, some of which may be precursorsof A- and B-type spliceosomes (Fig. 8B) (32). The addition ofGST protein to nuclear extracts did not change the splicing ofthe pre-mRNA, nor did it interfere with the assembly of spliceosomes(Fig. 8, lanes GST). However, no splicing intermediates or productsaccumulated in the presence of equimolar amounts of affinity-purifiedGST-NS1 protein (Fig. 8A, lanes GST-NS1). This effect was notdue to a defect in spliceosome assembly, because both A- and B-typecomplexes assembled, although B bands formed at a slightly reducedrate (Fig. 8B, lanes GST-NS1). Interestingly, an almost identicalresult was obtained in splicing reactions complemented with thesame concentration of purified GST-NS1-BP. There were no splicingproducts detectable after 1 h of incubation, and only trace amountsof the exon 1 and intron lariat-exon 2 splicing intermediateswere detected at the 2-h time point (Fig. 8, lanes GST-NS1-BP).The RNP gel analysis showed that the formation of B-type splicingcomplexes occurred in the presence of GST-NS1-BP (Fig. 8B, lanesGST-NS1-BP and GST-NS1). This result demonstrates that truncatedNS1-BP and the viral NS1 proteins block a cellular activity requiredat the same step of pre-mRNA splicing. We suggest that the observedsplicing inhibition by truncated NS1-BP is the result of a dominant-negativeeffect on the splicing function of the endogenous wild-type protein.

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FIG. 8. Pre-mRNA splicing, but not spliceosome assembly, is inhibited by truncated NS1-BP. ³²P-labeled MINX pre-mRNA, which is an artificial mini-exon construct derived from the major late transcription unit of adenovirus 2 (75), was incubated in HeLa cell nuclear extracts under splicing-compatible conditions in the absence (lanes NE) or presence of 80 ng of affinity-purified GST/µl (lanes GST) or equimolar amounts of affinity-purified GST-NS1 (lanes GST-NS1) or GST-NS1-BP fusion protein, which carries amino acids 347 to 619 of NS1-BP (lanes GST-NS1-BP). (A) RNA analysis. RNAs were purified from aliquots of the reactions after a 1-h (lanes 1) or 2-h (lanes 2) incubation period and were analyzed by electrophoresis on denaturing 13% polyacrylamide-urea gels. The positions of the pre-mRNA, the intron-exon 2 and exon 1 intermediates, and the spliced mRNA and lariat products are indicated to the right. The lower panel shows a longer exposure of the gel. M, ³²P-labeled size marker DNA fragments. (B) Splicing complex analysis. Aliquots of the splicing reactions were taken after 20, 40, and 60 min, and heparin was added to a final concentration of 1 mg/ml. The samples were analyzed by electrophoresis on a native agarose-polyacrylamide gel. The positions of the H-, A-, and B-type splicing complexes (32) are indicated on the left.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

NS1 is the only nonstructural protein of influenza A viruses which is expressed in infected cells. Although the NS1 proteinhas been implicated in several different processes, includingpre-mRNA splicing and mRNA transport and translation, little isknown about specific cellular factors that are recognized by NS1.Since NS1 has pleiotropic effects, it may interact with a varietyof proteins in infected cells, thereby affecting different stepsof cell metabolism. In order to identify such cellular proteins,we have used the yeast interaction trap to screen a human cDNAexpression library, using a LexA-NS1 fusion protein as bait. Wehave previously characterized NS1-I (NS1-interactor), which isa cytoplasmic 55-kDa protein that binds to the divergent NS1 proteinsexpressed by influenza A and B viruses (69). NS1-I is derivedfrom the precursor protein of an estradiol 17 $beta$ -dehydrogenase,and its binding to NS1 may have a function in modulating steroidhormone levels in virus-infected cells (69). Here we reporton the identification of NS1-BP through its specific interactionwith the NS1 protein. This interaction was confirmed by the useof an in vitro binding assay. The NS1 protein coprecipitated witha GST-NS1-BP fusion protein but not with GST alone, demonstratingthat NS1 also physically binds to NS1-BP. We did not detect coimmunoprecipitationof radiolabeled NS1 protein from extracts of virus-infected cellswith NS1-BP specific antibodies (data not shown). This resultmay indicate that NS1-NS1-BP complexes are disrupted by the antibodypreparation used or that the interaction of the two proteins islabile in the immunoprecipitation buffer.

The analysis of the primary structure of NS1-BP identified two regions with considerable homology to known proteins. The amino-terminal120 amino acids of NS1-BP are homologous to the BTB/POZ domainoriginally identified in a group of proteins that primarily regulatetranscription (3, 76). This includes the human proto-oncogenesLAZ3/BCL6 and PLZF and the Drosophila Tramtrack, GAGA, and BroadComplex proteins (for a review, see reference 1). It has beenshown that the isolated BTB/POZ domains of bric-a-brac (bab),ZID, LAZ3/BCL6, and Kelch can mediate homo- and/or heterodimerization,suggesting that BTB/POZ domains are a conserved protein-proteininteraction motif (3, 8, 11, 13, 50). In the bab protein,the first 51 amino acids of the BTB/POZ domain were found to besufficient for dimerization (8). Another function of this modulemay be protein targeting to specific nuclear domains, since theappearance of ZID, LAZ3/BCL6, and hZF5 proteins in "nuclear dots"depended on the integrity of their BTB/POZ domains (3, 8,11, 13, 60). The nature of the nuclear regions in whichthese BTB/POZ domain-containing proteins accumulate has not beenanalyzed so far. We are currently examining how the speckled regionsin which the NS1-BP is localized relate to the nuclear dots recognizedby antibodies directed against other BTB/POZ proteins.

The human cDNA isolated through the interaction trap encoded amino acids 347 to 619 of NS1-BP, which suggests that this regioncontains the binding site for the NS1 protein. This part of theNS1-BP consists almost entirely of five imperfect repeats of 47to 49 amino acids that are homologous to the kelch repeat motif(5). Based on phylogenetic sequence comparisons, it was suggestedthat kelch repeats take on a conserved three-dimensional foldthat was previously identified in procaryotic and eucaryotic enzymes(5). A high-resolution X-ray diffraction analysis for one ofthese enzymes, galactose oxidase of Dactylium dendroides, revealedthat each repeat element folds into a blade-like domain of four-strandedantiparallel $beta$ sheets. The blade-like domains are circularly arranged,resulting in a $beta$ propeller structure (30). The sequence homologysuggests that the five repeats of NS1-BP may also adopt a similarthree-dimensional fold.

In spite of the conservation on the sequence level, kelch repeats appear to have divergent functions in the homologous proteins.In galactose oxidase of D. dendroides, the kelch repeat fold containsthe catalytic center of the enzyme (30). On the other hand,the kelch elements of the $beta$ -scruin protein of L. polyphemus havebeen shown to bind to actin, which leads to the proposal thatkelch repeats may constitute an actin-binding domain (52, 67).However, other proteins that contain kelch repeats, such as the $alpha$ -scruin or the calicin proteins, are localized to intracellularregions that appear to be devoid of actin (65, 66).

The proteins encoded by different poxviruses that are homologous to NS1-BP have not been studied. The genes of the vacciniavirus A55R, C2L, and F3L open reading frame products could bedeleted without affecting viral replication in tissue cultureand are therefore considered nonessential (33, 45). However,the presence of homologous proteins in different poxviruses arguesfor important roles of these proteins. For example, these geneproducts may increase virus virulence or otherwise play a rolein infected animals.

By immunolocalization studies, we discovered that NS1-BP is concentrated in discrete regions in the nuclei of noninfectedcells. This intracellular distribution is compatible with a functionof NS1-BP in gene regulation. Confocal double-immunostaining analysesof cells demonstrated that NS1-BP colocalized in a speckled patternwith the spliceosome assembly factor SC35 (21). Several immunolocalizationstudies have shown that a number of other factors involved inpre-mRNA splicing, among them the spliceosomal snRNPs, also accumulatein the 20 to 50 irregularly shaped SC35 domains termed speckles(reviewed in reference 58). As shown by electron-microscopicanalysis, the speckle domains correspond to interchromatin granulesand perichromatin fibrils (17, 59). Different conclusionshave been drawn about the functional significance of the accumulationof splicing factors in specific subnuclear compartments. Sincespeckle domains localize near genes that are transcribed and spliced,it was suggested that speckles constitute a compartment in whichpre-mRNA is actively spliced (70). However, nascent RNA polymeraseII transcripts were detected by Br-UTP labeling in a random distributionthroughout the nucleoplasm (18). Since splicing is thought tooccur cotranscriptionally, it was concluded by this group thatpre-mRNA is processed throughout the nucleoplasm. For the speckledomains, a role as a storage or recycling compartment that suppliessplicing factors to transcription sites was also proposed (reviewedin reference 55). In any case, the important role of speckledomains for cellular RNA biogenesis is emphasized by their dynamicappearance in response to alterations of cellular gene expression.Stress conditions such as heat shock that result in inhibitionof RNA splicing also induce apparent changes in the distributionof splicing factors (4, 59). The localization of NS1-BP innuclear regions that contain high concentrations of pre-mRNA splicingfactors suggests a role for NS1-BP in mRNA splicing.

The intranuclear localization of NS1-BP was drastically altered in influenza A virus-infected cells that expressed the NS1protein. The speckled pattern was replaced by a rather homogeneousdistribution of NS1-BP throughout the nucleoplasm in a fashionsimilar to that observed for the viral NS1 protein. In contrast,only subtle changes were detected in the appearance of the SC35protein in influenza A virus-infected cells. This finding arguesthat the relocalization of NS1-BP is a specific effect and notthe result of a disintegration of the SC35-enriched domains. Thisnotion is further supported by our observations that stress conditionssuch as heat shock, serum starvation, or the addition of actinomycinD, which inhibits RNA polymerase II transcription, did not disruptthe colocalization of NS1-BP with SC35 (67a). It is conceivablethat local changes in NS1-BP concentration in response to an influenzaA virus infection also influence its function. We did not detectNS1-BP redistribution in cells that transiently expressed theNS1 protein from an RNA polymerase II-driven plasmid vector (datanot shown). This result may indicate that NS1-BP redistributionrequires intracellular concentrations of the NS1 protein thatare not achievable by the expression system used. Alternatively,another viral gene product or spliced viral mRNA may be neededfor the effect to be observed.

The NS1 protein has previously been shown to inhibit pre-mRNA splicing in vitro and in vivo (19, 36). It was speculatedthat the inhibition of splicing would result in the retentionof pre-mRNA in the nuclei of infected cells, thereby increasingthe concentration of mRNA cap structures available for cap snatchingby the viral RNA polymerase (36). Alternatively, the activityof the NS1 protein may contribute to the observed regulated splicingof the viral mRNAs derived from segments 7 and 8 (56, 63).Because cellular NS1-BP is concentrated in nuclear regions enrichedwith pre-mRNA splicing factors and because it relocalizes in virus-infectedcells, we examined whether NS1-BP has a role in pre-mRNA splicingin vitro. A truncated NS1-BP was used as a potential nonfunctionalcompetitor of the endogenous protein in HeLa cell nuclear extract,and the effects of this probe were compared to the known inhibitionof pre-mRNA splicing by the NS1 protein. A similar experimentaldesign has been used before by others to examine the role of thelarge subunit of RNA polymerase II in pre-mRNA splicing (14,73). In the present study, we demonstrated that the truncatedNS1-BP blocks the splicing of a ³²P-labeled pre-mRNA in HeLa cell nuclear extracts at the same stepas the NS1 protein does. Splicing complexes formed at only slightlyreduced rates in the presence of each of the two proteins. However,the conversion of the pre-mRNA into splicing intermediates orproducts was greatly reduced. This finding suggests that bothproteins act on the same stage of the spliceosome pathway, i.e.,they block an activity required for the first catalytic step.The shortened NS1-BP we used lacks the 346 N-terminal amino acidsof the wild-type protein and was fused to the 26-kDa GST protein.This mutant NS1-BP protein is therefore unlikely to retain thefull activity of the wild-type protein. However, the truncatedNS1-BP may still be able to interact with other essential splicingfactors, thereby preventing their association with the wild-typeNS1-BP. The bacterially expressed full-length NS1-BP was insoluble(data not shown). Therefore, we were unable to assess whetherthe full-length NS1-BP had an effect on pre-mRNA splicing similarto that of the truncated protein. Nevertheless, our results arecompatible with a role of the wild-type NS1-BP in pre-mRNA splicing.

How does the observed inhibition of splicing by the viral NS1 protein relate to these findings? In normal cells, NS1-BP isconcentrated in intranuclear domains that are enriched with multiplesplicing factors. We have demonstrated that cellular NS1-BP isspecifically relocalized in influenza A virus-infected cells thatexpress the NS1 protein. Redistribution of NS1-BP is likely toalter its function or activity. We propose a model in which theinfluenza A virus inhibits host cell splicing in infected cellsby the association of the viral NS1 protein with cellular NS1-BP.The NS1 protein may downregulate NS1-BP activity directly by blockingits normal association with spliceosomes. Alternatively, a mechanismcan be envisioned in which the viral NS1 protein removes cellularNS1-BP from centers of active splicing, thereby lowering its availabilityfor participation in cellular mRNA splicing processes. In bothmodels, the relocalization of NS1-BP may reflect its disruptedfunction. It has previously been suggested that the NS1 proteininhibits splicing by binding to U6 snRNA (36, 49), which isa key component of the catalytic core within the spliceosome (25,53). Our proposal to explain the inhibition of splicing by theNS1 protein through the binding to NS1-BP does not exclude anNS1-U6 interaction. It is estimated that at least 80 to 100 differentfactors are involved in pre-mRNA splicing (23, 53). For thatreason it has been difficult to dissect their dynamic and complexinteractions during the assembly of a spliceosome and the catalysisof the splicing reaction. It is possible that interactions ofthe NS1 protein with both NS1-BP and U6 snRNA contribute to theinhibition of pre-mRNA splicing.

Like the influenza A virus NS1 protein, the essential ICP27 protein of herpes simplex virus type 1 (HSV-1) has been implicatedin impairing cellular pre-mRNA splicing, possibly as part of ahost cell shutoff mechanism (27). One could therefore ask ifthere are parallels between lytic infections by influenza A virusand HSV-1. As has been shown for the NS1 protein, the ICP27 proteinhas been found to have pleiotropic regulatory effects. Roles forICP27 in mRNA 3'-end processing (6, 41) and in mRNA export(47, 57) have been suggested in addition to an inhibitoryeffect on pre-mRNA splicing. Interestingly, the expression ofICP27 induces the redistribution of SC35 and spliceosomal snRNPsfrom the known speckled pattern to a few condensed intranuclearstructures, in which they colocalize with the ICP27 protein (46,51). This pattern is basically the opposite of the situationobserved in influenza A virus-infected cells. In the present study,the number of SC35 domains appears to increase, with a concomitantdecrease in size (reference 20 and this study), and in contrastto ICP27, the NS1 protein is localized throughout the nucleusin a diffuse pattern.

We will need further analyses to explore the precise function of NS1-BP in pre-mRNA splicing and the role of the NS1-NS1-BPinteraction in virus-infected cells. For example, we will examineif other splicing factors that associate with NS1-BP during thecourse of splicing can be identified. Influenza A viruses withtemperature sensitivity (ts) mutations in the NS1 gene have beenisolated (summarized in reference 38). We want to examine ifany of the identified ts lesions in NS1 have an effect on thebinding to NS1-BP. These experiments will reveal if it is feasibleto correlate a weakened interaction between NS1 and NS1-BP witha ts phenotype and if this is paralleled by a lack of NS1-BP relocalizationat the nonpermissive temperature. Since the NS1 gene of the influenzaA virus is now amenable to genetic manipulation (16), it shouldalso be possible to mutate the NS1-BP binding site within theNS1 protein and to study the consequences for virus infection.These studies will expand our knowledge of how viruses interactwith cellular components and will also help us to learn more aboutthe cellular splicing apparatus.

	ACKNOWLEDGMENTS

We thank R. Brent (Massachusetts General Hospital) for providing yeast strains and two-hybrid vectors and J. Gyuris for theacidic domain-HeLa cell cDNA library. T.W. thanks H.-D. Klenk(Institute of Virology, Philipps-University Marburg) for his generoussupport and help in the immunization of rabbits.

This work was supported by a fellowship of the AIDS-Stipendienprogramm of the German Ministry for Education, Science, Research,and Technology (T.W.) and by a grant from the Deutsche Forschungsgemeinschaft(SFB286).

	FOOTNOTES

^* Corresponding author. Mailing address: Institut für Virologie, Philipps-Universität Marburg, Robert-Koch-Str. 17, 35037Marburg, Germany. Phone: 49-6421-286692. Fax: 49-6421-285482.E-mail: wolfft{at}mailer.uni-marburg.de.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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