Production and Characterization of a Soluble, Active Form of Tva, the Subgroup A Avian Sarcoma and Leukosis Virus Receptor

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Journal of Virology, April 1999, p. 3054-3061, Vol. 73, No. 4
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Production and Characterization of a Soluble, Active Form of Tva, the Subgroup A Avian Sarcoma and Leukosis Virus Receptor

John W. Balliet,¹ Joanne Berson,¹ Celina M. D'Cruz,¹ Julie Huang,¹ Joanne Crane,¹ Joanna M. Gilbert,² and Paul Bates¹^,^*

Department of Microbiology, School of Medicine, University of Pennsylvania, Philadelphia, Pennsylvania,¹ and Department of Pathology, Harvard Medical School, Boston, Massachusetts²

Received 3 September 1998/Accepted 23 December 1998

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The receptor for the subgroup A avian sarcoma and leukosis viruses [ASLV(A)] is the cellular glycoprotein Tva. A soluble formof Tva, sTva, was produced and purified with a baculovirus expressionsystem. Using this system, 7 to 10 mg of purified sTva per literof cultured Sf9 cells was obtained. Characterization of the carbohydratemodification of sTva revealed that the three N glycosylation sitesin sTva were differentially utilized; however, the O glycosylationcommon to Tva produced in mammalian and avian cells was not observed.Purified sTva demonstrates significant biological activity, specificallyblocking infection of avian cells by ASLV(A) with a 90% inhibitoryconcentration of ~25 pM. A quantitative enzyme-linked immunosorbentassay, developed to assess the binding of sTva to ASLV envelopeglycoprotein, demonstrates that sTva has a high affinity for EnvA,with an apparent dissociation constant of approximately 0.3 nM.Once they are bound, a very stable complex is formed between EnvAand sTva, with an estimated complex half-life of 6 h. The solublereceptor protein described here represents a valuable tool foranalysis of the receptor-envelope glycoprotein interaction andfor structural analysis ofTva.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The entry of enveloped viruses is determined by specific interactions between receptors on the cell surface and envelope glycoproteinson the virion. For most retroviruses, this process is pH independent,suggesting direct fusion between the viral and cell surface membranes(43). It has been hypothesized that the cellular receptor notonly provides a binding site for the virus but also induces conformationalchanges in the viral envelope proteins, ultimately leading tomembrane fusion and virus entry. The mechanism by which this occurs,however, is poorlyunderstood.

The avian sarcoma and leukosis virus (ASLV) family is an excellent model system for analyzing the mechanism of pH-independentvirus entry. There are five major subgroups (A to E) of ASLV basedon host range, infection interference, and immunological reactivityof the viral envelope glycoproteins. The five ASLV subgroups utilizecellular receptors encoded by three dominant autosomal loci, TVA,TVB, and TVC (16-18, 50), that allow for comparison of common,required features for virus entry. TVA and TVC confer susceptibilityto ASLV(A) and ASLV(C), respectively. The TVB locus is more complex,with various alleles determining infection by ASLV(B), ASLV(D),and ASLV(E). Several alleles of TVB have recently been cloned(1, 10).

Tva was the first ASLV receptor identified (7, 72) and has been mapped to the TVA locus (6). While it has been shownto function as a viral receptor, the cellular function of Tvaremains unknown. Due to alternative splicing, two isoforms ofTva (Tva₉₅₀ and Tva₈₀₀) that differ in their membrane anchoringdomains are expressed in avian cells. Both isoforms are functionalviral receptors (7), indicating that the determinants for receptorfunction are contained in the conserved, 83-amino-acid extracellulardomain. Within this domain is a 40-amino-acid, cysteine-rich motifhomologous to repeats (LDL-A modules) first identified in thehuman low-density lipoprotein receptor (hLDLR). The LDL-A modulein Tva, when appended to a heterologous membrane anchor, is sufficientto mediate ASLV(A) entry (51). Mutations within the LDL-A moduleseverely affect subgroup A envelope (EnvA) binding and virus entry,which suggests that the envelope binding site is composed of discontinuousregions within the LDL-A module (8, 54, 74, 75). Recentwork demonstrates that three amino acid substitutions in the hLDLRmodule A4 convert this module into an ASLV(A) receptor (53).In addition, since Tva contains a single LDL-A module, EnvA-Tvainteractions may serve as a model system for studying LDLR-ligandbinding in addition to dissecting determinants of virus entry(52).

Soluble receptors have been an effective tool for dissecting early entry events for several viruses. Preincubation of solubleCD4 (sCD4) with human immunodeficiency virus type 1 (HIV-1) enveloperesults in dissociation of gp120 from gp41 (47), acquisitionof protease sensitivity by HIV-1 Env (56), and alterations inmonoclonal antibody binding to HIV-1 Env (31, 41, 56) andpromotes the ability of Env to interact with coreceptors (4,33, 65, 71). A soluble form of the poliovirus receptor irreversiblyalters poliovirus to an intermediate similar to that identifiedduring poliovirus infection (38). sTva produced with stablytransfected quail cells was shown to inhibit ASLV(A) infection(15). However, the amount of receptor produced was not adequatefor rigorous biochemical analysis of the Tva-EnvA interactionor for structural determination of Tva by crystallography. Wetherefore chose to use a baculovirus expression system (BES) toproduce sTva. The BES produces high levels of secreted proteinthat retains biological activity as well as many of the posttranslationalmodifications.

In this report, we describe the production and purification of large quantities of sTva with a BES. The purified sTva is biologicallyactive; it specifically and potently blocks ASLV(A) infection,with a 90% inhibitory concentration (IC₉₀) of 26 pM. Additionally,we quantitatively evaluated sTva-EnvA interactions by enzyme-linkedimmunosorbent assay (ELISA). sTva has a high affinity for EnvA,with an apparent dissociation constant (K_d) of 0.3 nM, and oncebound, forms a very stable complex with an estimated half-lifeof 6h.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells, viruses, and reagents. Sf9 cells were routinely maintained in SF900II medium (Gibco BRL, Gaithersburg, Md.). Turkey embryo fibroblasts (TEF) weremaintained in TEF medium (1× M199, 10% tryptose phosphate broth,5% fetal calf serum, 1% chick serum, 2 mM L-glutamine, penicillin[100 U/ml], and streptomycin [100 µg/ml]). Stocks of the recombinantASLV(A) virus RCAS(A)AP (34), which expresses the histochemicalmarker alkaline phosphatase, were generated as described previously(72). The Baculogold baculovirus transfection kit was from Pharmingen(San Diego, Calif.).

Plasmid pSP73 was from Promega (Madison, Wis.). pVL1393 was from Pharmingen. pCB6 (7) and pVTBac (62) were describedpreviously.

Wheat germ agglutinin (WGA) agarose and concanavalin A (ConA) agarose were from Vector Laboratories, Inc. (Burlingame, Calif.).Peptide N-glycosidase F (PNGase F) was from New England Biolabs,Inc. (Beverly, Mass.). Neuraminidase, O-glycosidase, and tunicamycinwere from Boehringer Mannheim Biochemicals (Indianapolis, Ind.).ImmunoPure NHS-LC-biotin and 2,2'-azinobis(3-ethylbenzothiazoline)-6sulfonic acid diammonium salt were from Pierce (Rockford, Ill.).Rabbit polyclonal Tva antiserum 40 was previously described (7,72). Acrylamide was from National Diagnostics (Atlanta, Ga.).Ni²⁺-nitriloacetic acid (NTA) agarose was from Qiagen (Chatsworth,Calif.).

Construction of transfer vectors. The 968-bp fragment of pg950 (7) containing the complete open reading frame of quail Tva₉₅₀ was cloned into pSP73, whichwas digested with Asp718 and EcoRI to make pSP73-0.95. A six-histidinetail was appended to the carboxy terminus of the Tva ectodomainby digesting pSP73-0.95 with EagI and inserting a linker (OS9,5'-GGCCACCATCATCACCATCACTAGGAATTC-3', and OS10, 5'-GCCTGAATTCCTAGTGATGGATGATGATGGT-3'),encoding six histidine residues and containing a stop codon andan EcoRI site, to make pSP73-0.95H₆RI. This insertion deletedthe codon for the ultimate carboxy-terminal residue of the ectodomain,Arg83.

To generate a eukaryotic expression vector that expresses sTva, with a six-histidine carboxy terminus, pSP73-0.95H₆RI wasdigested with KpnI and ClaI (found in the polylinker of pSP73)and the resulting 830-bp fragment was cloned into pCB6 to makepCB6WT-Tva_HIS6.

Two baculovirus transfer vectors were used to generate recombinant baculovirus. The first construct preserves the Tva signalsequence. pSP73-0.95H₆RI was digested with BamHI (found in thepolylinker of pSP73) and EcoRI to yield a 790-bp fragment thatwas cloned into the baculovirus transfer vector pVL1393 to generatepVL1393Tva. The second baculovirus transfer vector contains themelittin leader sequence. pSP73-0.95H₆RI was digested with AgeIand EcoRI, and the 720-bp fragment was cloned into pVTBac digestedwith BamHI and EcoRI to make pVTTva by using a short oligonucleotideadaptor (OS13, 5'-GATCCGC-3', and OS14, 5'-CCGGGCG-3') to connectthe vector BamHI terminus to the insert AgeI terminus. Expressionof sTva from this construct was predicted to yield a protein withfour amino acids (AspProProGly) appended to the amino terminusby the linker (Fig. 1B).

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FIG. 1. Comparison of sTva and naturally occurring forms of quail Tva. (A) Diagram of sTva and quail Tva₉₅₀ and Tva₈₀₀. The arrow indicates the site of Tva leader peptide cleavage; the sTva melittin leader peptide is cross hatched, the LDL-A motif (residues 11 to 50) is hatched, transmembrane domain is solid, the glycosylphosphotidylinositiol linkage signal is vertically hatched, the cytoplasmic tail is shaded, and the six-histidine tail is stippled. The numbers on the right indicate the sizes (in amino acids) of the mature proteins. (B) Comparison of WT Tva and sTva amino and carboxy termini. The arrows indicate the signal peptide cleavage sites. The four additional N-terminal amino acids in sTva are marked with a line above. Potential N-linked glycosylation sites are underlined. MSD, start of the membrane-spanning domain.

Generation of recombinant baculovirus. Generation of recombinant baculovirus (Autographa californica nuclear polyhedrosis virus) (Baculogold; Pharmingen) was performedas described by the manufacturer. The recombinant baculovirusproduced from pVL1393Tva is designated bVL1393Tva. Likewise, pVTTvaproduced the recombinant virusbVTTva.

Infections for protein expression. A suspension culture of 1.2 × 10⁷ Sf9 cells/ml in an Erlenmeyer flask was infected with the recombinant baculovirus at a multiplicityof infection of 2 and incubated in a rotary shaker at 90 rpm and28°C for 1 h. The cells were diluted 1:2, and infection was allowedto proceed for between 48 and 96 h postinfection (p.i.), dependingon the experiment. To harvest the recombinant protein, the mediumwas clarified by two-step centrifugation at 430 × g and then at2,300 ×g. The clarified medium was used directly for biochemicalanalysis of sTva or for protein purification. The cell cultureviability was determined by trypan blue exclusion. The percentageof viable cells was equal to the number of unstained cells dividedby the total number ofcells.

Characterization of sTva. (i) Western immunoblotting. Detection of sTva was performed by Western blotting with polyclonal Tva antiserum 40 as described previously (51).

(ii) Lectin binding. WGA agarose and ConA agarose were washed with Triton lysis buffer (50 mM Tris [pH 8], 5 mM EDTA [pH 8], 150 mM NaCl, 1% TritonX-100) containing 10 mM MnCl₂. sTva from infected cell lysateswas incubated with 1/20 volume of lectins, rocked 1 to 2 h at4°C, and then washed three times with Triton lysis buffer containing10 mM MnCl₂. The lectin-bound protein was eluted with Laemmlibuffer and analyzed by sodium dodecyl sulfate-polyacrylamide gelelectrophoresis (SDS-PAGE) (12.5% acrylamide) and Western blotting.sTva precipitation from media of infected cells with WGA and ConAwas performed as described above, except the washes were performedwith phosphate-buffered saline (PBS) containing 10 mM MnCl₂.

(iii) Enzymatic analysis of carbohydrates. sTva was precipitated from medium with 10% trichloroacetic acid and incubated at 0°C for 15 min. The precipitate was washedonce with ice-cold acetone and resuspended in a minimal volumeof 20 mM NaH₂PO₄ (pH 7.2)-1% SDS. NaOH (2 N) was used to adjustthe sample to a pH of ~9, and the sample was heated to 95°C for5 min to completely denature sTva. The sample was then diluted10-fold in 20 mM NaH₂PO₄ (pH 7.2) plus 0.5% Triton X-100 to yielda final SDS concentration of 0.1%. The pH was adjusted to ~7.5with 6 N HCl. The denatured sTva was digested overnight at 37°Cwith the endoglycosidases PNGase F (0.4 U/Rx), O-glycosidase (2.5mU/Rx), and neuraminidase (0.5 U/Rx), individually or in combination.The digested products were analyzed by SDS-PAGE (12.5% acrylamide)and Western blotting as previously described (51).

To produce deglycosylated sTva for the ASLV inhibition assay (see below), purified sTva in 20 mM NaH₂PO₄ (pH 7.2) was incubatedwith PNGase F (10 µg of sTva/0.09 U of PNGase F) overnight at37°C. The deglycosylated protein was purified from PNGase F ona Ni²⁺-NTA agarosecolumn.

(iv) Tunicamycin treatment of infected cells. Sf9 cells were infected with bVTTva as described above with the addition of 4 µg of tunicamycin/ml. The infections were allowedto proceed in the presence of tunicamycin for 48 h, and then theinsect cell medium was clarified and analyzed by SDS-PAGE andWestern blotting as describedabove.

Purification of sTva. An Ni²⁺-NTA agarose column was washed with one bed volume of wash buffer 1 (100 mM NaH₂PO₄, 10 mM Tris, pH 7.0). sTva-containingmedium that was dialyzed with 3,000-molecular-weight-cutoff dialysistubing overnight in PBS was passed through the column twice at~0.5 ml/min. The column was washed with 10 bed volumes of washbuffer 1, 5 bed volumes of wash buffer 2 (initial experimentsused 100 mM NaH₂PO₄-10 mM Tris-60 mM imidazole [pH 7.0]; subsequentexperiments used 20 mM imidazole), and eluted with 2 bed volumesof elution buffer (100 mM NaH₂PO₄, 10 mM Tris, 500 mM imidazole,pH 7.9). Removal of imidazole, buffer exchange, and concentrationof purified sTva was performed with a 3K Macrosep concentrator(Filtron, Northborough, Mass.) as described by the manufacturer,initially with 20 mM NaH₂PO₄ (pH 7.2) and subsequently with 10mM HEPES (pH 7.0). The purity of sTva was evaluated by SDS-PAGE(12.5% acrylamide) followed by Coomassie blue staining. The sTvaconcentration was determined by spectrophotometry (1A₂₈₀ unit= 0.70 mg/ml, as calculated from the molar extinction coefficientdetermined by the computer program Protean [DNA $star$ , Madison, Wis.]).The concentration was verified by SDS-PAGE (12.5% acrylamide)and Coomassie blue staining of sTva compared with those of bovineserum albuminstandards.

Inhibition of ASLV infection. Serial dilutions of purified sTva (or the deglycosylated form) were added to 2.1 × 10³ infectious units of RCAS(A)AP in 1 ml (final volume) of completeTEF medium and incubated for 30 min at 22°C. Following incubation,the sTva-virus mixture was added to 1.5 × 10⁵ TEF/well of a six-well plate and placed in an incubator for 4h. To limit virus diffusion and allow foci of infected cells toform, the cells were washed three times with PBS and overlaidwith 3 ml of complete TEF medium containing 0.5% agarose. After72 h at 37°C, the overlays were removed and the cells were fixedand stained for alkaline phosphatase activity as described previously(51). The stained foci were enumerated, and these values wereplotted against the concentration of sTva. Linear regression analysiswith the Cricket graph program (Computer Associates International,Inc., Islandia, N.Y.) was used to determine the IC₅₀ and IC₉₀for sTva. Experiments were done in triplicate with two independentpreparations ofsTva.

Envelope binding assay. A 96-well ELISA plate was coated overnight at 4°C with 100 µl of saturating concentrations (1:1,000 ascites fluid) of $alpha$ -gDmonoclonal antibody 1D3 (provided by Gary Cohen and Roselyn Eisenberg,University of Pennsylvania)/well in 20 mM Tris HCl, pH 8.5, and0.1 M NaCl. The following morning, the plate was washed threetimes with 200 µl of ELISA wash buffer (1× PBS, 0.05% Tween 20)/wellwith agitation for 15 s between washes. To reduce nonspecificbinding, the plate was subsequently blocked for 45 min at roomtemperature with 200 µl of ELISA block solution (1× PBS, 0.5%gelatin, 0.05% Tween 20, 0.05% NaN₃)/well. 100 µl of gD-EnvA (52)cell lysates/well in ELISA blocking buffer was added, and thesolution was incubated for 1 h at 4°C. The volume of lysates usedwas predetermined to be sufficient to saturate the 1D3 antibodyon the plate. The plate was then washed three times with ELISAwash buffer. Various concentrations of purified, biotinylatedsTva (see below) in a total of 100 µl of ELISA blocking buffer/wellwere added and incubated at either 4, 22, or 37°C. After 1 h ofincubation, the wells were washed with ELISA wash buffer threetimes. The bound biotinylated sTva was detected with 100 µl ofavidin-horseradish peroxidase (1:2,500 dilution in 1× PBS-0.5%gelatin-0.05% Tween 20)/well for 30 min at 4°C, followed by threewashes with 2× ELISA wash buffer. 2,2'-Azinobis(3-ethylbenzothiazoline)-6sulfonic acid diammonium salt (100 µl/well) dissolved in 10 mlof ELISA substrate solution (0.1 M NaOAc, 0.1% Tween-20 [pH 4.2],5 µl of 3% H₂O₂) was added to visualize the horseradish peroxidaseactivity. The plates were read with a Vmax ELISA reader (MolecularDynamics, Sunnyvale, Calif.) at 405 nm. All experiments were performedin triplicate and repeated several times with comparable results.The data was plotted as maximum optical density as a functionof sTva concentration and analyzed by nonlinear least-squaresfitting with Cricket graph. The coefficients of correlation forthe fitted lines were 0.97, 0.96, and 1.0 for 37, 22, and 4°C,respectively. The apparent K_d was estimated from half-maximalbinding as described previously (45).

EnvA-sTva complex stability assay. To analyze the stability of the EnvA-sTva complex, the ELISA was modified as follows: 5 nmol of biotinylated sTva in a totalof 100 µl of ELISA blocking buffer was added to each well andincubated for 1 h at 4°C. After being washed three times withELISA wash buffer, 5 nmol of unlabeled sTva in a total of 100µl of ELISA blocking buffer was added to each well and incubatedfor 0, 15, 30, 60, 120, and 240 min at either 4 or 22°C. The wellswere washed three times, and then bound, labeled sTva was detectedas described above. The data was plotted as the percent of labeledsTva bound (maximum optical density) as a function of time. Allexperiments were performed in triplicate and repeated severaltimes with comparableresults.

Biotinylation of purified sTva. Twenty micrograms of sTva was added to a 1 mg/ml stock of Sulfo-NHS-LC-biotin in PBS to yield a 400-µl reaction solution.This was incubated at 4°C for 45 min. The reaction was quenchedwith 40 µl of 1 M glycine for 5 min at 4°C. The biotin-labeledsTva was dialyzed against PBS for 24 h with several buffer changes.The concentration of labeled sTva was subsequently determinedbyspectroscopy.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Vector construction. To express the subgroup A ASLV receptor protein (Tva) in a form and quantity sufficient for biochemical and structural analysis,we used a BES to produce secreted sTva. The region encoding theTva signal sequence and extracellular domain was PCR amplifiedand cloned into the A. californica nuclear polyhedrosis transfervector pVL1393. To aid in protein purification, six histidineresidues were appended to the carboxyl-terminal end of the Tvaextracellular domain to generate pVL1393Tva. This His₆ tag replacedone residue at the boundary of the membrane-spanning domain (Fig.1B). A second construct, pVTTva, was generated by using the A.californica nuclear polyhedrosis transfer vector pVT-Bac (62).This vector substitutes the honeybee mellitin signal peptide,which substantially increases the secretion of proteins from insectcells, for the Tva signal peptide (58, 62). The amino terminusof the mature form of the sTva protein produced from pVTTva waspredicted to contain four additional amino acids (AspProProGly)from the mellitin signal sequence and an oligonucleotide adaptor(Fig. 1B). A comparison of sTva with the two alternatively splicedforms of Tva is shown in Fig. 1A. The pVTTva and pVL1393Tva transfervectors were used to generate recombinant baculoviruses, whichwere cloned by three rounds of plaque purification. Finally, toallow expression of secreted receptor protein in mammalian andavian cells, the tva sequence from the pVL1393 vector was clonedinto an expression vector under control of the cytomegalovirusimmediate-earlypromoter.

Expression of Tva in insect cells. Monolayer cultures of Sf9 cells were infected with either the recombinant virus bVTTva or bVL1393Tva or with the parentalbaculovirus. To address the possibility of clonal variation inexpression of Tva, three recombinant virus clones for both bVTTvaand bVL1393Tva were examined. Lysates and media from infectedcells were analyzed for Tva expression with a rabbit antiserumto the receptor protein (7). SDS-PAGE and Western blottingof lysates and media with the polyclonal Tva antiserum revealedthat cells infected with any of the bVTTva recombinant clonesexpressed very high levels of Tva. Greatly reduced levels of aprotein of similar size were detected in the bVL1393Tva-infectedcells (data not shown). No Tva protein was detected in lysatesor media from cells infected with the parent virus (data not shown).This data supports previous work suggesting that the mellitinleader aids in expression of foreign glycoproteins in insect cells(58, 62). Based on these results, one of the bVTTva recombinantvirus clones was selected for large-scale production ofsTva.

Optimization of sTva production. In order to determine the optimal time for harvesting the sTva protein from the supernatant of infected Sf9 cells, a timecourse analysis was performed (data not shown). Sf9 cells in suspensionwere infected with bVTTva at a multiplicity of infection of 2,and medium was removed at various time points for analysis byWestern blotting. sTva could be readily detected in the culturesupernatant as early as 24 h p.i. (data not shown). Maximum levelsof sTva in the medium were observed at 48 h p.i. At 72 h p.i.,significant amounts of sTva were observed in the medium; however,degradation products were also apparent. By 96 h p.i., littlesTva was detected. The level of sTva in the supernatant correlatedwith the viability of the infected cell culture. As determinedby trypan blue exclusion, the infected cell culture remained >95%viable up to 50 h p.i. (data not shown). By 72 h p.i., the viabilitydropped to nearly 40%, suggesting that the sTva proteolytic productsseen in the culture supernatant are due to cleavage by cellularor viral proteases released from dead cells. This expression patternwas highly reproducible; therefore, the 48-h p.i. time point wasused for sTvaproduction.

Characterization of sTva. To begin characterizing the soluble receptor protein, sTva produced in insect cells was compared with Tva₉₅₀ and sTva (wild-type[WT] Tva_His6) expressed in human 293T cells. sTva produced ininsect cells infected with bVTTva migrates significantly fasteron SDS-PAGE than Tva₉₅₀ expressed in human cells (Fig. 2A). sTvaappears as a group of four bands approximately 18 to 26 kDa inmass, while Tva₉₅₀ from human cells produces a characteristicheterogeneous population of bands migrating with apparent molecularmasses between 29 and 43 kDa. The discrepancy in size betweenthe insect cell-produced sTva and Tva₉₅₀ expressed in human cellssuggested that sTva was modified differently than membrane-anchoredTva₉₅₀. Consistent with this hypothesis, expression of sTva (WTTva_His6) in murine (data not shown) or human (Fig. 2A) cells resultsin a series of bands with apparent molecular masses ranging from18 to 29 kDa (additional protein bands due to nonspecific antibodycross-reactivity [32 to 43 kDa] and proteolytic degradation [14to 18 kDa] are also observed).

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FIG. 2. Comparison of Tvas from mammalian and insect cells and analysis of purified sTva. (A) Cell lysates from human 293T cells transiently expressing either Tva₉₅₀ or sTva and lysates from Sf9 cells infected with bVTTva were subjected to SDS-PAGE (12.5% acrylamide), and Western blotting was performed with a polyclonal $alpha$ -Tva serum. (B) Analysis of purified sTva. To assess the purity of sTva, 0.5 (left) and 10 (right) µg of the same preparation were analyzed by SDS-PAGE (12.5% acrylamide) and Coomassie blue staining. Molecular mass standards (in kilodaltons) are indicated.

sTva contains three potential N-linked glycosylation sites as well as a region rich in serine and threonine residues thatcould be modified by O-linked carbohydrates. To determine if thefour bands observed when sTva is produced in insect cells representdifferential carbohydrate modifications, sTva was precipitatedfrom Sf9 cell lysates with lectin-agarose beads. Both WGA- (datanot shown) and ConA-agarose precipitated the three largest speciesof sTva from infected Sf9 cell lysates but not the fastest-migratingspecies (Fig. 3A). WGA binds to N-acetylglucosamine residues inboth N- and O-linked oligosaccharides, whereas ConA binds to $alpha$ -linkedmannose residues in the N-linked core oligosaccharide. Thus, theseresults suggest that the upper three slower-migrating bands ofsTva represent forms of the soluble receptor with one, two, orthree N-linked oligosaccharides, and because sTva was precipitatedby WGA, it may contain O-linked glycosylation.

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FIG. 3. sTva is modified by asparagine-linked glycosylation. (A) sTva binds to ConA. Lysates of Sf9 cells infected with bVTTva were incubated with ConA sepharose. After extensive washing, ConA-bound proteins were eluted and analyzed by Western blotting as described in the legend to Fig. 2. (B) Analysis of sTva glycosylation by glycosidase digestion. sTva was acid precipitated from the medium of bVTTva-infected Sf9 cells. Pelleted sTva was resuspended in the appropriate glycosidase buffer and digested with PNGase F (F; lanes 2 and 5), neuraminidase (N; lanes 3, 4, and 5), and O-glycosidase (lanes 4 and 5). Following glycosidase digestion the samples were analyzed by SDS-PAGE and Western blotting as described in Fig. 2. Molecular mass standards (in kilodaltons) are indicated on the left.

To confirm whether the Sf9-produced sTva was modified by N and/or O glycosylation, we subjected sTva to digestion with specificglycosidases. Neither neuraminidase nor O-glycosidase treatmentaffected the mobility of sTva (Fig. 3B, lanes 3 and 4), suggestingthat the protein is not significantly modified by O-linked sugarsor sialic acid. In contrast, treatment of sTva with PNGase F,which specifically removes N-linked carbohydrates, condensed thecharacteristic four bands of sTva to a single species that comigratedwith the fastest-migrating form (18 kDa) seen in cell lysates(Fig. 3B, lanes 2 and 5). The PNGase F-treated sTva was incompetentto bind to either WGA or ConA (data not shown). Additionally,when bVTTva-infected cells are grown in the presence of tunicamycin,which inhibits N-linked glycosylation, only a single form of secretedsTva could be detected by Western blot analysis, migrating at18 kDa (data not shown). Taken together, these results are consistentwith N-linked modification but not O glycosylation of sTva, withthe upper three forms of sTva representing proteins with one,two, or three N-linked sugars and the fastest-migrating speciesrepresenting an unmodified form of the receptor.

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FIG. 4. ELISA analysis of sTva-ASLV(A) envelope binding. (A) Titration of sTva. Increasing concentrations of purified sTva were incubated with captured gD-EnvA at the indicated temperature ( $open circle$ , 37°C; $diamond$ , 25°C;

, 4°C) in an ELISA as described in Materials and Methods. The percent of sTva bound for each concentration is the average of three experiments. The error bars indicate standard deviations. The apparent K_ds for sTva-EnvA were estimated from the half-maximal binding and are 0.3, 0.2, and 0.5 nM at 37, 25, and 4°C, respectively. (B) Analysis of sTva-EnvA complex stability. The relative dissociation rate of the sTva-EnvA complex was determined by preincubating excess biotinylated sTva with gD-EnvA which was captured on an ELISA plate. After extensive washing, excess unlabeled sTva was incubated at 4°C for the indicated times. The percentage of labeled sTva bound is the average of three experiments. The error bars indicate standard deviations. The sTva-EnvA dissociation rates at 22 ( $open circle$ ) and 4°C (

) are ~5.5 and >6 h, respectively.

Purification of sTva. His₆-tagged sTva protein can be rapidly and quantitatively purified from culture supernatants of bVTTva-infected cells byusing the protocol outlined in Materials and Methods. The mainfeatures of this protocol are an initial dialysis step followedby binding to metal-chelating resin (NTA), a low-concentrationimidazole wash to remove contaminating proteins adsorbed to thecolumn, and, finally, elution of sTva with a high concentrationof imidazole. The dialysis step was added to the protocol forall cultures larger than 100 ml, since it appeared that compoundsin the insect cell growth medium remove the nickel from the NTAcolumn, interfering with sTva purification. The eluted solublereceptor protein is >95% pure as judged by staining with Coomassieblue following SDS-PAGE analysis of overloaded sTva samples (Fig.2B, right). Furthermore, three glycosylated forms of sTva arepresent in the purified protein when the purified protein is analyzedby SDS-PAGE and Coomassie blue staining (Fig. 2B, left). The extinctioncoefficient predicted from the sTva primary amino acid sequencewas used to estimate the yield of purified protein from variouspreparations at 7 to 10 mg/liter of infected Sf9 cells. This estimatewas confirmed by SDS-PAGE by comparing purified sTva to bovineserum albumin concentration standards (data notshown).

Inhibition of ASLV infection by sTva. To determine if the purified sTva retained biological activity, we assessed the ability of the purified protein to inhibitinfection by ASLV(A). A subgroup A Rous sarcoma virus vector carryingan alkaline phosphatase reporter gene, RCAS(A)AP, was preincubatedwith various concentrations of purified sTva and then added toTEF. Following removal of the virus inoculum, the cells were overlaidwith soft agar to allow foci to develop. Two days after infection,the overlay was removed, the cells were stained for alkaline phosphataseactivity, and the alkaline phosphatase-positive foci were enumerated.sTva inhibited infection by RCAS(A)AP in a dose-dependent manner(data not shown). The IC₅₀ for sTva inhibition of RCAS(A)AP infectionwas found to vary between 6 and 25 pM in numerous experiments,with an average of 14 pM (Table 1). A PNGase F-treated form ofsTva similarly inhibited RCAS(A)AP, indicating that saccharidemoieties are not required for envelope-receptor interactions (datanot shown). As expected, infection by subgroup C ASLV, which doesnot utilize Tva, was unaffected by sTva (data not shown). Thus,it appears that sTva retains specific biological activity effectivelyneutralizing ASLV(A).

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TABLE 1. Inhibition of ASLV(A) infection by sTva^a

Analysis of sTva binding to ASLV envelope protein. Neutralization of RCAS(A)AP by sTva suggested that the soluble, baculovirus-produced receptor was capable of binding to thesubgroup A envelope glycoprotein, EnvA. To directly address thisquestion and to quantitatively analyze the interaction betweensTva and EnvA, an ELISA-based binding assay was developed. Thisassay is similar to an assay used to measure HIV-1 glycoproteinbinding to a soluble form of the cellular receptor CD4 (45).

Epitope-tagged EnvA (gD-EnvA) was captured on the ELISA plate with a monoclonal antibody to the gD tag. sTva was labeled bybiotinylation with a primary amine-reactive reagent. Since sTvacontains no lysine residues, labeling with this reagent shouldattach a single biotin molecule only to the amino terminus ofthe protein. Labeled sTva was added at various concentrationsto wells containing captured gD-EnvA and incubated for 30 minat the indicated temperature (Fig. 4A). After washing, bound sTvawas detected with peroxidase-conjugated avidin. In numerous experiments,sTva bound to the captured gD-EnvA in a concentration-dependentmanner, achieving saturable binding at concentrations in excessof 2 to 4 nM. Moreover, the data in Fig. 4A fits a simple bimolecularnoncooperative-binding curve. From this data, the binding affinityof sTva was estimated to have an apparent K_d of 0.3 nM at 37°C.The apparent K_ds at 4 and 22°C were very similar, indicating thatsTva binding to EnvA is temperatureindependent.

The ELISA was also used to analyze the stability of the sTva-EnvA interaction (Fig. 4B). A saturating amount (5 nM $congruent$ 18 × K_d)of biotinylated sTva was added to captured gD-EnvA and allowedto achieve equilibrium. After removal of the unbound labeled sTvaand washing, excess unlabeled sTva (5 nM) was added and incubatedfor the indicated times at 4 or 22°C (Fig. 4B). Even after 6 hat 4°C, 50% of the labeled sTva remained bound to EnvA, suggestinga complex half-life of ~6 h. Similar results were obtained at22°C. This extremely slow off rate attests to the stability ofthe sTva-EnvAcomplex.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this report, we describe the construction, expression, and characterization of a soluble form of Tva using a BES. sTvasecreted into the medium of infected insect cells is differentiallymodified by N-linked glycosylation but does not appear to containsignificant O link modifications. Large quantities of sTva canbe purified from the medium of infected insect cells, and thispurified protein is capable of efficiently and specifically neutralizingASLV(A). In addition, using an ELISA-based binding assay, sTva-EnvAinteractions were investigated and an apparent K_d of 0.3 nM anda complex half-life of 6 h weredemonstrated.

Four different protein species of sTva from infected Sf9 cell lysates were identified, with masses of 18 to 26 kDa, suggestingthat the three N-linked glycosylation sites in sTva are differentlyutilized. In contrast, expression of the same truncated form ofTva, as well as Tva₉₅₀, in mammalian cells resulted in additionalprotein bands, indicating differences in posttranslational processingof insect- and mammalian-derived proteins (Fig. 2A). Indeed, lectinbinding and glycosidase digestion of sTva as well as tunicamycintreatment of infected insect cells confirmed that sTva containsN-linked glycans but does not appear to be O glycosylated (Fig.3). This is in agreement with previous data demonstrating thatproteins expressed in Spodoptera frugiperda cells are N link modifiedbut are either not O glycosylated or are underglycosylated witheither the monosaccharide N-acetylglucosamine (69) or N-acetylgalactosamine(63) or the disaccharide galactose( $beta$ 1-3)N-acetylgalactosamine(29, 36, 63).

Using chimeric Tva-CD8 proteins, we have previously shown that there is no requirement for specific N or O glycosylation forASLV(A) receptor function (51). The results with sTva confirmthis observation. A PNGase F-treated form of sTva, in which thereis no detectable remaining N-linked glycosylation, was fully competentto neutralize ASLV(A) infection of primary turkey cells, indicatingthat saccharide moieties have no apparent role in Tva viral receptorfunction.

Soluble forms of viral receptors for HIV (14, 22, 27, 35, 59, 64), Epstein-Barr virus (48), mouse hepatitisvirus (55), poliovirus (38), and rhinovirus (42) have beenshown to be biologically active by inhibition of virus infection,and therefore are most likely correctly folded. Previous experimentswith media from mammalian cells expressing a secreted form ofTva suggested it also could block ASLV(A) infection (15). Todetermine whether purified sTva retained biological activity,we evaluated the ability of sTva to block ASLV(A) infection. Preincubationof sTva with virus potently inhibited virus infection of primaryavian cells, with an IC₉₀ of 26 pM (Table 1), indicating thatthe protein is biologically active and therefore likely correctlyfolded. Moreover, sTva is a significantly more potent inhibitorof virus infection, with an IC₉₀ nearly 10³-fold lower than that of sCD4 for laboratory-adapted HIV-1 infection(14, 27, 35) and 10⁶-fold lower than that of soluble intercellular adhesion molecule1 (sICAM-1) for rhinovirus infection (42). The differences amongthe antiviral activities of the three soluble receptors are likelydue to mechanistic differences in the way the receptors neutralizetheir cognate viruses. sICAM-1 inhibits rhinovirus infection primarilyby saturating the receptor binding sites on the virus (30).Similarly, sCD4 neutralization of HIV-1 appears to be mediatedby receptor binding to virions; however, gp120-induced sheddingfrom the virion may contribute to viral neutralization (23,49).

The mechanism of sTva inhibition of ASLV(A) infection appears to be by irreversible inactivation of the ASLV virion. In sharpcontrast to CD4, which requires a coreceptor for HIV-1 infectivity,Tva appears to be necessary and sufficient to mediate ASLV(A)entry (3, 7, 72). Binding of sTva to EnvA induces a conformationalchange in the SU subunit, exposing previously inaccessible proteasesites (28), and leads to the formation of stable, higher-orderoligomers of the TM subunit (3a) reminiscent of structures forthe putative fusogenic forms of influenza HA2 (11, 13), Ebolavirus GP2 subunits (67), and the murine leukemia virus (MLV)(26) and HIV-1 TM subunits (12, 60, 68). In addition,sTva binding to a soluble, oligomeric form of EnvA converts theenvelope glycoprotein to a membrane-associated form consistentwith activation of EnvA to a fusogenic state (21, 32). Inthis case, upon EnvA activation, sTva dissociates (21, 32),perhaps permitting it to reassociate with a new EnvA molecule.The extremely low IC₅₀ seen for sTva would suggest the soluble-receptorneutralization is mediated by a hit-and-run mechanism, where sTvainduces irreversible conformational changes that inactivate EnvAand then dissociates to inactivate additional envelope molecules.Taken together, these results confirm the biological activityof sTva and demonstrate the utility of this reagent for dissectingthe early events in ASLV(A)entry.

sTva inactivation of ASLV(A) is initiated by binding to EnvA, since it had no effect on ASLV(C) infection. To further evaluatethe interaction between EnvA and sTva, we developed a sensitiveELISA. Half-maximal binding is a function of the equilibrium dissociationconstant (K_d); however, because equilibrium was not maintainedby the addition of sTva during wash and detection steps, the K_dvalue obtained is an approximation. With this caveat, the apparentK_d for sTva-EnvA is 0.3 nM at 37°C (Fig. 4A). The magnitude ofthe apparent K_d suggests that any dissociation is negligible.In addition, the apparent K_d for sTva-EnvA is temperature independent.While the K_ds for sCD4-gp120 at different temperatures are similar,the kinetics of binding vary with temperature (23). The kineticparameters for EnvA-Tva will need to be defined to determine whethera similar situation exists. Table 2 summarizes the K_d valuesdetermined for a number of viruses. As Table 2 illustrates, theapparent K_d determined for the sTva-EnvA system is similar tothat determined with a fluorescence-activated cell sorter-basedassay (75). Moreover, it is within the range of many other virus-receptorK_ds, implying that strong affinity between viral glycoproteinsand their cognate receptors is a common, conserved feature ofa number of viruses, regardless of whether they are enveloped(e.g., HIV-1 and ASLV) or nonenveloped (e.g., poliovirus and reovirus).

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TABLE 2. Comparison of virus-receptor binding constants

Consistent with the low apparent K_d, the sTva-EnvA complex is extremely stable. Complex half-life estimations indicate that50% of the purified receptor is still bound to EnvA after up to6 h and the binding is not significantly affected by temperature(Fig. 4B). In contrast, after 90 min, 50% of ecotropic MLV boundto the cell surface dissociates at 25°C (73). The differencein complex stability is even more striking considering the multivalentinteractions between MLV and the cell surface versus the monovalentinteraction between sTva and EnvA. Analysis of HIV-1 binding suggeststhis interaction is also relatively less stable, since 50% ofthe HIV-1 gp120-CD4 complex dissociates within ~30 min at 37°C(44). A possible reason for the high stability of the Tva-EnvAinteraction is that avian cells express levels of Tva on theirsurface that are too low to be detected by fluorescence-activatedcell sorter, immunofluorescence, or Western blot analysis (7).Since cooperative binding appears to be required for EnvA activation(21), an extremely stable Env-receptor complex may be requiredto ensure enough envelope glycoproteins are bound for activationof membrane fusion. Interestingly, once Env is activated, receptorreadily dissociates (21, 32), confirming the intimate relationshipof Tva and EnvA in coordinating virusentry.

The quality and quantity of sTva produced from Sf9 cells has allowed us to begin structural analysis of the receptor. Fromcrystal trials, we have identified conditions that produce crystalsof sufficient size and quality to be competent to diffract X rays.Mapping of mutations in Tva that affect viral receptor functiononto the structure will assist in understanding envelope-receptorinteractions as well as LDLR-ligand interactions. Additionally,this will be the first structure of an LDL-A module in which biologicalactivity can be demonstrated. It will be interesting to compareit to previously determined structures of hLDLR modules refoldedfrom Escherichia coli-produced proteins (19, 20, 25).

	ACKNOWLEDGMENTS

We acknowledge the generosity of Roselyn Eisenberg and Gary Cohen for supplying $alpha$ -gD monoclonal antibody. We also thank CarrieL. Rokos, Rouven Wool-Lewis, and Lijun Rong for critical readingof the manuscript and useful discussions, as well as the othermembers of the Bateslaboratory.

This work was supported by grants to P.B. from the National Institutes of Health (CA63531) and the American Heart Association(95015200). J.W.B. is a trainee under grant T32-AI-07325 fromthe National Institutes ofHealth.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, University of Pennsylvania School of Medicine, 225 JohnsonPavilion, 3610 Hamilton Walk, Philadelphia, PA 19104-6076. Phone:(215) 573-3509. Fax: (215) 573-4184. E-mail: pbates{at}mail.med.upenn.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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