Proteolytic Processing and Assembly of gag and gag-pol Proteins of TED, a Baculovirus-Associated Retrotransposon of the Gypsy Family

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Journal of Virology, November 1998, p. 8718-8724, Vol. 72, No. 11
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Proteolytic Processing and Assembly of gag and gag-pol Proteins of TED, a Baculovirus-Associated Retrotransposon of the Gypsy Family

Kathryn L. Hajek¹^,²^, and Paul D. Friesen²^,³^,^*

Graduate Program in Cellular and Molecular Biology,¹ Institute for Molecular Virology,² and Department of Biochemistry,³ Graduate School and College of Agricultural and Life Sciences, University of Wisconsin $---$ Madison, Madison, Wisconsin 53706

Received 8 April 1998/Accepted 5 August 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

TED (transposable element D) is an env-containing member of the gypsy family of retrotransposons that represents a possibleretrovirus of invertebrates. This lepidopteran (moth) retroelementcontains gag and pol genes that encode proteins capable of formingviruslike particles (VLP) with reverse transcriptase. Since VLPare likely intermediates in TED transposition, we investigatedthe roles of gag and pol in TED capsid assembly and maturation.By using constructed baculovirus vectors and TED Gag-specificantiserum, we show that the principal translation product of gag(Pr55^gag) is cleaved to produce a single VLP structural protein, p37^gag. Replacement of Asp⁴³⁶ within the retrovirus-like active site of the pol-encoded protease(PR) abolished Pr55^gag cleavage and demonstrated the requirement for PR in capsid processing.As shown by expression of an in-frame fusion of TED gag and pol,PR is derived from the Gag-Pol polyprotein Pr195^gag-pol. The PR cleavage site within Pr55^gag was mapped to a position near the junction of a basic, nucleocapsid-likedomain and a C-terminal acidic domain. Once released by cleavage,the C-terminal fragment was not detected. This acidic fragmentwas dispensable for VLP assembly, as demonstrated by the formationof VLP by C-terminal Pr55^gag truncation proteins and replacement of the acidic domain witha heterologous protein. In contrast, C-terminal deletions thatextended into the adjacent nucleocapsid-like domain of Pr55^gag abolished VLP recovery and demonstrated that this central regioncontributes to VLP assembly or stability, or both. Collectively,these data suggest that the single TED protein p37^gag provides both capsid and nucleocapsid functions. TED may thereforeuse a simple processing strategy for VLP assembly and genome packaging.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

TED (transposable element D) is a 7.5-kb, middle-repetitive retrotransposon of the moth Trichoplusia ni. It was identifiedas a single-copy insertion (TED^FP-D) within the DNA genome of Autographa californica nucleopolyhedrovirus(AcMNPV), having transposed during infection of cultured T. nicells with this baculovirus (33). Comprised of gag, pol, andenv genes that are flanked by long terminal repeats (Fig. 1A),TED^FP-D was the first example of spontaneous, retroelement-mediated transferof functional host genes to an animal virus (11, 30, 33).On the basis of sequence similarity within pol, TED is most closelyrelated to the Drosophila retrotransposons 17.6, 297, tom, andgypsy (11, 18, 31, 37, 46) and thus is classified asa member of the gypsy family of retroelements (42). Recent studieshave indicated that TED, tom, and gypsy possess env-like genesthat encode membrane-associated glycoproteins with propertiesexpected of vertebrate retroviral envelope proteins (35, 40,45). These findings, combined with evidence that gypsy producesenveloped viruslike particles (VLP) that are infectious in Drosophilalarvae (19, 40, 41), suggest that the gypsy family transposonsmay be facultative retroviruses of insects (9, 38).

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FIG. 1. (A) TED genetic organization. TED (7.5 kb) contains gag, pol, and env genes flanked by 270-bp long terminal repeats (solid boxes). PR, RT, and IN are conserved retroviruslike domains within pol. (B) TED sequences expressed by baculovirus vectors. TED gag and pol were fused to the polyhedrin (polh) promoter (striped box) and inserted into the AcMNPV genome, replacing the polh gene. Expression of TED pol requires a $-$ 1 translational frameshift for all virus vectors except vGAG/POL.fs and vGAG/POL.PRfs, which contain in-frame gag-pol fusions due to 4-bp insertions ( $black-down-triangle$ ). The apparent masses (in kilodaltons) of TED proteins are indicated to the right of each virus. Symbols: ×, D⁴³⁶V mutation; arrow, transcriptional start site; $bullet$ , inserted stop codon. Restriction site abbreviations: B*, BamHI; R, EcoRI; H, HindIII; K, KpnI; N, NcoI; Nh, NheI; P, PstI; S, SalI; S3, Sau3AI, Sm, SmaI; Sp, SpeI. Only restriction sites used for cloning are indicated.

The assembly of VLP containing genomic RNA and the components necessary for reverse transcription is critical to the movementof retrotransposons and retroviruses (for reviews, see references4, 17, and 38). In the case of retrotransposons Ty1 andTy3 of Saccharomyces cerevisiae, synthesis of gag-encoded structuralproteins is required for transposition, suggesting that VLP assemblyis an important intermediate step in this process (2, 13).VLP may have multiple functions, including compartmentalizationof genomic RNA, along with reverse transcriptase (RT) and integrase(IN), protection of the genome from intracellular nucleases, andgenome transport to the nucleus, among others. In vertebrate retroviruses,distinct domains of the Gag precursor that are separated by proteolyticcleavage into matrix (MA), capsid (CA), and nucleocapsid (NC)proteins accomplish these functions (reviewed in references 5,7, 17, 49 and 50).

Despite the importance of gag in transposition, little is known about Gag protein processing and VLP assembly by the env-containingretrotransposons. Due to their striking resemblance to the vertebrateretroproviruses, these simple elements may provide useful modelsfor retrovirus CA assembly, morphogenesis, and evolution. An effectivemeans for investigation of TED Gag structure and function hasbeen the overexpression of TED by using baculovirus vectors (10).Infection of cultured lepidopteran cells with TED-containing AcMNPVrecombinants demonstrated that the primary translation productof TED gag is Pr55^gag (30). Consistent with Gag function, Pr55^gag assembles to produce 60-nm-diameter VLP. Expression of TED gag-pol,which requires a $-$ 1 ribosomal frameshift (Fig. 1A), yields VLPcomposed of the major CA protein p37^gag, traces of Pr55^gag, and RT activity. The appearance of p37^gag correlated with expression of the 5' portion of TED pol withsequence similarity to retroviral proteases (PR). Thus, it wasproposed that p37^gag is derived by PR-mediated processing of Pr55^gag (30). Moreover, PR cleavage of the TED Gag-Pol polyproteinPr195^gag-pol was predicted to yield RT and other functions necessary for transposition.

To examine the processing and assembly of TED Gag proteins, we have extended the use of baculovirus vectors to overexpressgag and pol in cultured Spodoptera frugiperda (SF21) cells thatlack endogenous copies of TED. By using polyclonal antisera raisedagainst TED Gag proteins, we confirmed that Pr55^gag is cleaved to produce the major VLP protein p37^gag. Moreover, we report here that cleavage is mediated by the TEDpol-encoded PR, which is generated from the frameshifted polyproteinPr195^gag-pol. The Gag cleavage site was mapped to the junction of a centralNC-like domain and a C-terminal acidic domain within Pr55^gag. Analogous acidic domains were identified at the C termini ofDrosophila retroelements 17.6, 297, and tom, suggesting that thefunction of the acidic domain is conserved. Nonetheless, the acidicdomain was dispensable for VLP assembly, whereas the adjacentNC-like domain was required. These findings suggested that p37^gag provides both CA and NC functions and that TED incorporates multiplefunctions into a single Gag protein. This feature distinguishesTED from those vertebrate retroviruses in which the gag productsare proteolytically separated.

	MATERIALS AND METHODS

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Cells and AcMNPV recombinants. S. frugiperda IPLB-SF21 cells (48) were cultured in TC100 growth medium (GIBCO Laboratories) supplemented with 2.6 mg oftryptose broth per ml and 10% heat-inactivated fetal bovine serum.Viruses vGAG and vGAG/POL (Fig. 1B) have been described previously(30). TED-containing recombinants derived from the wild-typeL1 strain of AcMNPV (28) were constructed and propagated bystandard methods (21, 34). For each virus, the polyhedringene (polh) was replaced with TED^FP-D sequences under the control of the polh promoter. In brief, SF21cells (2 × 10⁶ per plate) were transfected with Lipofectin (Bethesda ResearchLaboratories), 2 µg of NdeI-linearized transplacement plasmid,and 0.2 µg of Bsu36I-digested v $Delta$ p35/lacZ viral DNA (15). Extracellularbudded virus was collected 2 to 4 days later and plaque purifiedby using the non-apoptotic plaque phenotype conferred by acquisitionof the apoptotic suppressor gene p35 (29). Proper insertionof TED sequences was confirmed by PCR amplification and restrictionanalyses of viral DNA.

Recombinant plasmids. (i) Transplacement vector pEV/35K. AcMNPV p35 was inserted in the opposite orientation adjacent to polh of a modified form of plasmid pEVocc⁺/PA (8). An XhoI-KpnI fragment containing polh was replacedby the polh promoter fused to a polylinker. The resulting transplacementvector, pEV/35K, contained a modified polylinker for insertionof foreign genes downstream of a polh 5' noncoding leader identicalto that of pEV55 (34).

(ii) TED pol mutations. A Sau3AI fragment encoding TED PR (nucleotides 1943 to 2490) was inserted into the BamHI site of pBluescript KS(+) (Stratagene)to generate plasmid pTEDpr⁺. Asp⁴³⁶ in the putative PR active site was replaced with Val by usingthe oligonucleotide 5'-ATTCTTGATTGTCACTGCCAA-3' (A $right-arrow$ T at nucleotide1969 is underlined) (26) to generate pTEDpr. The D⁴³⁶V mutant sequence was inserted into TED pol by successive steps.First, TED nucleotides 1611 to 1951 were amplified by PCR (39)using primers 5'-CGTAAATCCGGGAATCCGCC-3' and 5'-GGTGGATCCGAAAATTCTATATAT-3'(T $right-arrow$ G at nucleotide 1942 introduced a BamHI site). After EcoRIand BamHI digestion, the amplified fragment (TED nucleotides 1672to 1943) was inserted at the corresponding sites of pGAG_tr (30)to generate pGag.2. A BamHI fragment of pTEDpr containing D⁴³⁶V was inserted at the BamHI site of pGag.2 to generate pGagpr. An XbaI/amber stop linker (New England Biolabs) was insertedat the XbaI site downstream of TED sequences to generate pGagpr.X. After treatment with T4 DNA polymerase, an XhoI-SstI fragmentfrom pGagpr.X was inserted into XhoI and SmaI sites of pEV/35K to generatepEV/35K/gagpr. An NcoI-SstII fragment (TED nucleotides 2418 to 6070) from pGAG/POL(30) was inserted into the corresponding sites of pEV/35K/gagpr to generate pEV/35K/gagpol.pr. The BamHI fragment of pTEDpr⁺ was used to replace the homologous fragment in pEV/35K/gagpr to generate pEV/35K/gagpr⁺. The sequence of nucleotides 1672 to 2490 was determined in orderto verify all mutations. The corresponding viruses vGAG/PR and vGAG/PR⁺ encoded 8 heterologous residues (PLVLASLD) at the 3' end of pol.

A TED gag-pol in-frame fusion was created by inserting 4 bp (underlined) immediately after the $-$ 1 frameshift by using oligonucleotide5'-GTTTGGTCGATTGCTAGCAAATCCTGACTTTC-3' (TED nucleotides 1875 to1848) to generate plasmid pTEDfs. A 271-bp EcoRI-BamHI fragment from pTEDfs was inserted into the corresponding sites of pGagpr⁺.B2 (see below) to generate pGagpr⁺fs. The XhoI-NcoI fragment of pGagpr⁺fs was replaced with the analogous fragment of pEV/35K/gagpol.pr.

(iii) TED gag mutations. TED gag was truncated at either the EcoRI (nucleotide 1672) or the SalI (nucleotide 1705) site by EcoRI or SalI digestionof pGAG_tr (30), followed by digestion with XbaI. After end repairwith Klenow fragment, an XbaI/amber linker was inserted to generatepGag338 and pGag349, respectively. The gag sequences were insertedas XhoI-XbaI fragments into the transplacement vector pEV/35Kto generate pEV/35K/gag338 and pEV/35K/gag349. pEV/35K/gag338was digested with KpnI and XbaI, end repaired with Klenow fragment,and ligated to an XbaI/amber linker to generate pEV/35K/gag229.Virus vGAG²²⁹ encoded two heterologous residues (LV) at the 3' end of gag.The 1,024-bp EcoRI fragment from pPRM35K-ORF (16) with p35 was inserted into the EcoRI site of pEV/35K/gag338to generate pEV/35K/gag-P35. The gag-P35 hybrid encoded 6 heterologousresidues (DLYHSK) between gag and p35.

Sequences encoding the influenza hemagglutinin (HA) epitope YPYDVPDYA were inserted at TED nucleotide 1728 (Gag residue 355)by introducing an NheI site (underlined) into pGagpr⁺.X with oligonucleotide 5'-GTATAATAGTCGCAGCTAGCCCCTGGTTCGG-3'.Complementary oligonucleotides encoding the HA epitope (5'-CTAGCATGTACCCATACGACGTCCCAGACTACGCTG-3')were inserted to generate pGagpr⁺.HA. pGagpr⁺.X was partially digested with BamHI, Klenow repaired, and ligatedto a BglII linker, 5'-GAAGATCTTC-3', to generate pGagpr⁺.B2, in which a BglII site replaced the BamHI site at TED nucleotide2490. An EcoRI-BamHI fragment (nucleotides 1672 to 1943) frompGagpr⁺.HA was used to replace the analogous fragment of pGagpr⁺.B2 to generate pGagpr⁺.HAB. An XhoI-NcoI fragment (TED nucleotides 559 to 2418) from pGagpr⁺.HAB was used to replace the analogous fragment of pEV/35K/gagpolto generate pEV/35K/gagpol.HA.

Antiserum preparation. For anti-Pr55^gag ( $alpha$ -p55) antiserum, Triton X-100 lysate (see below) was prepared from SF21 cells 48 h after infection with vGAG.Particulate material was pelleted through a 30% (wt/vol) sucrosecushion by centrifugation (at 250,000 × g for 2.5 h) and sedimentedon a 20 to 70% (wt/vol) linear sucrose gradient (at 150,000 ×g for 16 h). Pr55^gag-containing gradient fractions were pooled for antigen preparation.For anti-TrpE-Gag ( $alpha$ -Tg) antiserum, an SpeI-PstI fragment containingTED gag nucleotides 765 to 1238 was inserted into the XbaI andPstI sites of vector pATH22 (22) to generate pATH22/TrpE-gag.Insoluble TrpE-Gag fusion protein was isolated from Escherichiacoli JM83 that contained pATH22/TrpE-Gag. After sodium dodecylsulfate (SDS)-polyacrylamide gel electrophoresis (27), gel slicescontaining either Pr55^gag or TrpE-Gag protein were crushed and emulsified with adjuvant.New Zealand White rabbits were immunized with 200 µg of antigenand boosted 2 weeks later with 100 µg of antigen. Immune and preimmunesera were collected and treated with an acetone powder from wild-typeAcMNPV-infected SF21 cells by standard methods (6, 14).

Analysis of virus-infected cell lysates and VLP. Except as noted, SF21 cells were inoculated with a multiplicity of infection (MOI) of 10 PFU per cell. Infected cells werewashed with phosphate-buffered saline 42 or 48 h later, suspendedin lysis buffer (1% SDS-2.5% $beta$ -mercaptoethanol), and boiled for5 min. For VLP isolation, cells were collected 42 h after infection,washed with TNE (10 mM Tris [pH 7.5], 150 mM NaCl, 1 mM EDTA),and suspended in TNE lysis buffer (TNE plus 250 mM sucrose-0.1%Triton X-100) for 15 min at 0°C to produce Triton X-100 lysates.After clarification by centrifugation (at 800 × g for 15 min),particulate material was collected by centrifugation through a30% (wt/vol) sucrose cushion (at 250,000 × g for 2.5 h). Pelletswere either suspended in lysis buffer and boiled for 5 min orsedimented on a 20 to 70% (wt/vol) sucrose gradient (at 150,000× g for 16 h). TED Gag-containing gradient fractions were pooled.

Immunoblot analysis. Protein samples were subjected to SDS-polyacrylamide gel electrophoresis and transferred to nitrocellulose membranes (47).The membranes were incubated in 5% nonfat dry milk or 3% bovineserum albumin in TBST (50 mM Tris [pH 7.4], 150 mM NaCl, 0.05%Tween 20), followed by a 5 × 10⁴ dilution of $alpha$ -Tg, a 10³ dilution of $alpha$ -p55, or a 10³ dilution of anti-HA 12CA5 monoclonal serum (BAbCO) in 5% nonfatmilk- or 3% bovine serum albumin-containing TBST by standard methods(6). Immune complexes were detected with horseradish peroxidase-conjugatedgoat or mouse anti-rabbit immunoglobulin G (Jackson Laboratories)and developed by enhanced chemiluminescence according to the manufacturer'sinstructions (Amersham).

Pulse-chase analysis. The medium from SF21 cells infected 42 h previously was replaced with phosphate-buffered saline containing 200 µCi of Tran³⁵S-label (>1,000 Ci/mmol; ICN Biomedicals, Inc.)/ml. After 20 minat 27°C, the radiolabel was replaced with growth medium containinga 50-fold excess of unlabeled methionine and cysteine. SDS celllysates were prepared at the indicated times. For immunoprecipitations,the lysates were clarified by centrifugation (at 6,000 × g for2 min), diluted in Nonidet P-40 (NP-40) buffer (50 mM Tris [pH8.0], 1% NP-40, 150 mM NaCl, 5 mM EDTA), and incubated with $alpha$ -p55for 30 min at 0°C. Protein A-Sepharose beads were added, and themixture was incubated for 1 h at 7°C. Immune complexes were washedthree times with NP-40 buffer, boiled in lysis buffer, and subjectedto SDS-polyacrylamide gel electrophoresis and fluorography (En³Hance; DuPont).

Image processing. Films were scanned at a resolution of 300 dpi by using a Microtek Scanmaker III equipped with a transparency adapter. Theresulting files were printed from Adobe Photoshop 3.0 by usinga Kodak 8650 PS dye sublimation printer.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Identity of TED gag proteins. To establish and verify the precursor-product relationships of TED Gag and Gag-Pol polyproteins, we first generated polyclonalantisera to TED gag-specific proteins. $alpha$ -Tg serum was raised againstan E. coli-generated TrpE protein fused to TED gag amino acidresidues 35 to 192. Immunoblot analysis with $alpha$ -Tg detected Pr55^gag (Fig. 2, lanes 2 and 8), the primary translation product of TEDgag that is synthesized in cultured SF21 cells infected with AcMNPVrecombinant vGAG (Fig. 1B). The TED-related protein p77, of unknownfunction, was also recognized (30). In addition, p37^gag was detected (Fig. 2, lanes 6 and 12) upon expression of TEDgag and pol by recombinant vGAG/POL (Fig. 1B). As demonstratedby the failure to recognize proteins from wild-type AcMNPV-infectedSF21 cells (Fig. 2, lanes 1 and 7), $alpha$ -Tg was specific for TEDproteins. A different antiserum, $alpha$ -p55 (see below), which wasraised against full-length Pr55^gag isolated from purified TED VLP, exhibited similar specificity.

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FIG. 2. Effect of D⁴³⁶V mutant pol on proteolytic processing of TED Gag proteins. Triton X-100 (TX-100) extracts were prepared from SF21 cells 42 h after infection with the indicated AcMNPV recombinants (MOI of 10). Samples (10⁴ cell equivalents) of Triton X-100 extract (lanes 1 to 6) or the VLP collected from 10⁴ cells (lanes 7 to 12) were subjected to immunoblot analysis by using $alpha$ -Tg serum. Positions of molecular mass standards (in kilodaltons), TED proteins, and degradation products (arrows) are indicated. WT, wild type.

Requirement of Asp⁴³⁶ for PR activity and Pr55^gag cleavage. The active-site hexapeptide (hydrophobic residue)₂-D-(T/S)-G-(A/S) is conserved among pol-encoded aspartyl PR of retroelements(25). To assess the role of TED PR in Gag processing, we substituteda valine for aspartate residue 436 within the predicted activesite (LID⁴³⁶TGA) of TED PR and generated AcMNPV recombinants vGAG/POL.PR and vGAG/PR, containing gag and all or part of the D⁴³⁶V-mutated pol gene (Fig. 1B). Immunoblot analysis of infectedcells revealed that vGAG/PR and vGAG/POL.PR produced little or no p37^gag (Fig. 2, lanes 3 and 5). Moreover, the steady-state level ofPr55^gag was higher than that in cells infected with the wild-type PR-containingvirus vGAG/PR⁺ or vGAG/POL (lanes 4 and 6). The active-site D⁴³⁶V substitution also caused an accumulation of the larger gag-relatedproteins p80 and Pr195^gag-pol in cells infected with vGAG/PR (lane 3) and vGAG/POL.PR (lane 5), respectively.

The requirement for Asp⁴³⁶ in Gag processing was confirmed by an analysis of TED VLP. As measured by recovery of particulatematerial by centrifugation through 30% sucrose cushions, Pr55^gag was the major gag-related protein of VLP isolated from cellsinfected with PR-mutated vGAG/PR and vGAG/POL.PR (Fig. 2, lanes 9 and 11). p37^gag was not detected in VLP produced by the viruses with the D⁴³⁶V substitution. In contrast, p37^gag was the major VLP protein produced by vGAG/PR⁺ or vGAG/POL (Fig. 2, lanes 10 and 12). Smaller gag-related proteinswere detected in cells infected with TED gag-containing viruses(Fig. 2, lanes 2 to 6). Because these proteins were not detectedin VLP preparations (Fig. 2, lanes 8 to 12) and their abundancevaried between experiments, it is likely that they representedPr55^gag breakdown products.

Synthesis of in-frame TED gag-pol fusions. Synthesis of the PR-containing Gag-Pol polyprotein Pr195^gag-pol requires a ribosomal frameshift in the $-$ 1 direction within the 43-bpoverlap between TED gag and pol (Fig. 1A). The abundance of Gagproteins relative to Gag-Pol proteins produced by the PR-deficientbaculovirus vectors (Fig. 2) suggested that the frameshift affectsthe stoichiometry of TED structural and enzymatic proteins, includingPR. Thus, to investigate the potential regulatory role of theframeshift, we inserted 4 nucleotides immediately adjacent tothe predicted site of ribosomal slippage (GGAUUUU), creating anin-frame gag-pol fusion (fs) that eliminated the synthesis of Pr55^gag. Recombinant viruses vGAG/POL.fs and vGAG/POL.PRfs, with and without active PR, respectively, were generated (Fig.1B). Consistent with an in-frame fusion, vGAG/POL.fs produced p37^gag but not the precursor, Pr55^gag, as indicated by analysis of the particulate fraction of infectedcells (Fig. 3, lane 5). The level of p37^gag derived from vGAG/POL.fs was comparable to that of vGAG/POL (Fig. 3, lane 3), containingthe natural $-$ 1 frameshift, and similar to that of vGAG³⁴⁹ (lane 2), containing a C-terminal truncation of Pr55^gag (see below). D⁴³⁶V inactivation of PR within the in-frame gag-pol fusion causedhigh levels of accumulation of Pr195^gag-pol (Fig. 3, lane 6) and yielded a smaller gag-related protein ofunknown origin. The loss of p37^gag and the appearance of Pr195^gag-pol upon PR inactivation demonstrated that PR is active within theGag-Pol polyprotein. Moreover, p37^gag can be derived by PR-mediated cleavage of Pr195^gag-pol.

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FIG. 3. Expression of TED gag-pol in-frame fusions. Triton X-100 extracts were prepared from SF21 cells 42 h after infection (MOI of 10) with recombinant vGAG, vGAG³⁴⁹, vGAG/POL, vGAG/POL.PR, vGAG/POL.fs, or vGAG/POL.PRfs. Particulate material was collected by centrifugation through a 30% (wt/vol) sucrose cushion, and samples (7.5 × 10⁴ cell equivalents) were subjected to immunoblot analysis by using $alpha$ -Tg. Molecular mass markers (in kilodaltons) and TED proteins are indicated.

Kinetics of PR-mediated cleavages. To validate the precursor-product relationships of TED gag proteins and confirm the requirement of TED PR in proteolytic processing,we conducted pulse-chase analyses in which immunoprecipitationwith $alpha$ -p55 antiserum monitored the fate of radiolabeled Gag proteins.Pr55^gag synthesized in cells infected with either vGAG (Fig. 4, lanes1 to 3) or D⁴³⁶V-mutated vGAG/PR or vGAG/POL.PR (lanes 9 to 14) was relatively stable during the chase. Moreover,at no time was p37^gag detected. Polyproteins p80 and Pr195^gag-pol, synthesized by the PR-deficient viruses, were also detected(Fig. 4, lanes 9 to 14). When functional PR was synthesized byviruses vGAG/PR⁺ (Fig. 4, lanes 4 to 8) and vGAG/POL (lanes 15 to 19), Pr55^gag levels decreased whereas p37^gag levels increased. Although the level of immunoprecipitated Pr55^gag was reduced in PR-synthesizing cells, the rate of p37^gag appearance indicated that Pr55^gag had a half-life of ~15 min, consistent with our previous findings(30). Collectively, these data demonstrated that p37^gag is derived from Pr55^gag. However, the smaller, sister fragment to p37^gag was not detected by immunoprecipitation with $alpha$ -p55, despite thepresence of Cys and Met residues for radiolabeling (see below).

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FIG. 4. Pulse-chase analysis of TED Gag processing. Cells infected 42 h previously with the indicated AcMNPV recombinants (MOI of 10) were radiolabeled for 20 min with [³⁵S]methionine-cysteine. The radiolabel was replaced with medium containing excess unlabeled methionine-cysteine, and cell lysates were prepared 0, 0.25, 0.5, 1, and 3 h thereafter. TED gag-related proteins were immunoprecipitated by using $alpha$ -p55 and were subjected to polyacrylamide gel electrophoresis and fluorography. Molecular mass standards (in kilodaltons) and TED-specific proteins are indicated.

Pr55^gag $right-arrow$ p37^gag cleavage site. Inspection of the predicted amino acid sequence of Pr55^gag revealed a C-terminal region (residues 332 to 386) that is highlyacidic and devoid of basic residues (Fig. 5A). This unusual domainis conserved among the gypsy retroelements tom and 17.6. The acidicdomain of TED is joined to an NC-like region (residues 199 to314) that is basic and proline rich and that lacks acidic residues.Since proteolytic cleavage between the NC-like region and theacidic domain would yield a protein similar in size to p37^gag, we predicted that processing occurs at or near the predictedjunction of these dissimilar segments. To test this possibility,we first inserted the 9-amino-acid HA epitope from influenza virusHA at residue 355 within the acidic domain of Pr55^gag (Fig. 5A). The presence of the HA tag in Pr55^gag was verified by immunoblot analysis (with HA-specific serum)of cells infected with the resulting AcMNPV recombinant vGAG^HA/POL (data not shown). However, p37^gag was not detected by the HA-specific serum after cleavage, norwere smaller HA-containing cleavage products detected. These findingssuggested that the acidic domain was proteolytically removed fromthe C terminus of Pr55^gag and that the sister cleavage fragment was unstable.

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FIG. 5. PR-mediated cleavage of C-terminal TED Gag truncations. (A) Comparison of gypsy element Gag precursors. The predicted N-terminal CA-like (CA), basic NC-like (NC) (shaded), and C-terminal acidic (striped) domains of TED (11) and analogous domains of the predicted Gag proteins of Drosophila gypsy elements tom and 17.6 (37, 46) are shown. Tick marks indicate basic or acidic amino acid residues. The HA epitope ( $black-down-triangle$ ) was inserted at residue 355 within the acidic domain of TED Pr55^gag. Predicted PR cleavage sites are indicated (vertical arrows). (B) TED gag sequences. AcMNPV vectors contain the full-length gag open reading frame (vGAG) or 3' truncations that are designated by the number of codons extending from the initiation codon to the introduced stop codon ( $bullet$ ). Synthesized Gag proteins are indicated on the right. Restriction site abbreviations are listed in the legend to Fig. 1. (C) Immunoblot analysis. Cells were infected with wild-type (WT) AcMNPV (lane 1), vGAG²²⁹ (lane 2), vGAG³³⁸ (lane 3), vGAG³⁴⁹ (lane 4), vGAG/POL (lane 5), or vGAG/POL.PR (lane 9) alone. Cells infected with vGAG²²⁹, vGAG³³⁸, and vGAG³⁴⁹ were also coinfected with vGAG/POL (lanes 6 to 8) or vGAG/POL.PR (lanes 10 to 12). SDS lysates were prepared 42 h after infection and subjected to immunoblot analysis (3 × 10⁴ cell equivalents) by using $alpha$ -Tg. Molecular mass standards (in kilodaltons), TED-specific proteins, and gag-related degradation proteins ( $star$ ) are indicated.

To map the location of the Pr55^gag cleavage site, recombinant viruses with 3' deletions of TED gag were constructed (Fig. 5B).Since cleavage occurred near the Pr55^gag C terminus, we predicted that removal of these residues wouldeliminate processing by PR and thereby provide the location ofthe cleavage site. Immunoblot analysis of infected cells demonstratedthat vGAG²²⁹, vGAG³³⁸, and vGAG³⁴⁹ produced gag truncation proteins p25, p38, and p40, respectively(Fig. 5C, lanes 2 to 4). When provided in trans, functional PRhad no effect on the size or accumulation of p25, as shown bycoinfection of vGAG²²⁹ with PR-containing vGAG/POL or PR-deficient vGAG/POL.PR (Fig. 5C, lanes 6 and 10). Thus, cleavage occurs on the C-terminalside of residue 229. In contrast, coinfection of vGAG³⁴⁹ with vGAG/POL reduced the intracellular level of truncation proteinp40 and yielded p37^gag (Fig. 5C; compare lanes 4 and 8). Since p40 cleavage was notdetected upon coinfection with vGAG/POL.PR (Fig. 5C, lane 12), PR was responsible for the cleavage of p40.Little, if any, change in the size or level of truncation proteinp38 was detected upon coinfection with either vGAG/POL or vGAG/POL.PR (Fig. 5C, lanes 7 and 11). Taken together, these findings indicatethat Pr55^gag cleavage occurred on the N-terminal side of residue 349 at ornear residue 338.

Dispensability of the acidic domain for Pr55^gag cleavage. To determine whether the C-terminal acidic domain was required for Gag cleavage, we constructed an AcMNPV vector, vGAG-P35,in which a portion of TED gag was fused in frame with the heterologousgene p35 and placed under the control of the polh promoter. Expressionof the gag-p35 chimera produced Gag-P35 (Fig. 6A), which containedthe first 338 residues of Pr55^gag (p38) fused to P35, a 35-kDa cytosolic protein encoded by AcMNPV(16). Infection with vGAG-P35 yielded the full-length Gag-P35fusion, as detected by using Gag-specific $alpha$ -Tg and P35-specific $alpha$ -P35NF antisera (Fig. 6A, lanes 3 and 8). Upon infection of vGAG-P35with PR-expressing vGAG/POL, Gag-P35 was cleaved to produce P35',a protein detected exclusively by $alpha$ -P35NF (Fig. 6A, lane 9). Dueto the presence of Gag-derived residues, P35' was larger thanwild-type P35 detected in all recombinant AcMNPV-infected cells(Fig. 6A, lanes 6 to 10). The absence of P35' in cells coinfectedwith vGAG-P35 and PR-deficient vGAG/POL.PR (Fig. 6A, lane 10) verified that P35' was generated by PR-mediatedcleavage of Gag-P35. However, the abundance of the Gag-P35 fusionprotein in PR-synthesizing cells (Fig. 6A, lanes 4 and 9) suggestedthat cleavage of Gag-P35 was less efficient than that of Pr55^gag. These data demonstrated that PR can cleave a heterologous Gagfusion protein lacking the acidic domain and indicated that cleavageis N terminal to Gag residue 338.

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FIG. 6. PR-mediated cleavage of TED Gag-P35. (A) Immunoblot analysis of cell lysates. Cells were infected with vGAG/POL (POL) (lanes 1 and 6), vGAG/POL.PR (PR) (lanes 2 and 7), or vGAG-P35 ( $-$ ) (lanes 3 and 8) alone. In addition, cells were coinfected with vGAG-P35 and vGAG/POL (lanes 4 and 9) or with vGAG-P35 and vGAG/POL.PR (lanes 5 and 10). SDS lysates (3 × 10⁴ cell equivalents) were subjected to immunoblot analysis by using $alpha$ -Tg or $alpha$ -P35NF. (B) VLP analysis. The VLP from cells 42 h after infection with vGAG-P35 were collected by centrifugation through a 30% sucrose cushion. Triton X-100 (TX-100) extract from 2 × 10⁴ cells (lane 1) and VLP from 6 × 10⁴ cells (lane 2) were subjected to immunoblot analysis by using $alpha$ -P35NF.

Dispensability of the acidic domain for VLP assembly. Examination of the particulate fraction derived from vGAG-P35-infected cells (Fig. 6B) indicated that the Gag-P35 fusion proteinretained the capacity to assemble VLP. This finding suggestedthat the acidic domain is not required for particle assembly.To define Pr55^gag residues involved in VLP assembly and to further investigateTED gag functions, we tested the effects of the 3' gag truncations(Fig. 5B) on VLP yields produced by AcMNPV vectors. Deletion of61 (vGAG³⁴⁹) or 72 (vGAG³³⁸) residues at the Pr55^gag C terminus had no effect on particle assembly, since the yieldof p40-containing VLP (Fig. 7, lane 12) or p38-containing VLP(lane 11) was comparable to that of vGAG/POL-infected cells (lane9). VLP composed of either p38 (vGAG³³⁸) or p40 (vGAG³⁴⁹) were stable to sucrose gradient purification (Fig. 7, lanes15 and 16) and exhibited a density (1.19 g/ml) comparable to thatof VLP composed of full-length Pr55^gag. Electron microscopic examination also indicated that negativelystained VLP from vGAG³⁴⁹ resembled negatively stained Pr55^gag-containing VLP (data not shown). In contrast, removal of 181residues (vGAG²²⁹) that included residues within the basic, NC-like domain eliminatedrecovery of VLP (Fig. 7, lane 10) without altering protein (p25)stability (lane 4). Thus, Pr55^gag residues from 229 to 338 contribute to VLP assembly or stability,or both.

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FIG. 7. Effect of TED gag truncations on VLP assembly. SF21 cells were harvested 42 h after infection (MOI of 10) with wild-type (WT) AcMNPV, vGAG, vGAG/POL (POL), vGAG²²⁹ (229), vGAG³³⁸ (338), or vGAG³⁴⁹ (349). Triton X-100 (T X-100) extract (2.5 × 10⁴ cell equivalents) (lanes 1 to 6) and the VLP-containing (particulate) fraction (7.5 × 10⁴ cell equivalents) collected from extracts by centrifugation through a 30% sucrose cushion (lanes 7 to 12) were subjected to immunoblot analysis by using $alpha$ -Tg. Threefold less sample was used from vGAG-infected cells (lanes 2 and 8). VLP from equivalent numbers of vGAG/POL-, vGAG²²⁹-, vGAG³³⁸-, and vGAG³⁴⁹-infected cells were sedimented on 20 to 70% (wt/vol) sucrose density gradients and analyzed similarly (lanes 13 to 16).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Model for TED VLP assembly and maturation. Our data indicate that the assembly and maturation of TED Gag and Gag-Pol proteins resemble those of the simple vertebrateretroviruses. The primary translation product of TED gag, Pr55^gag, first assembles with the less abundant Gag-Pol polyprotein Pr195^gag-pol to yield immature particles. PR-mediated processing of both precursorsthen generates mature VLP containing the major CA protein p37^gag, the pol-encoded enzymes RT and IN, and genomic RNA. By analogyto other retroelements (20, 23, 32, 36, 44), it is expectedthat the maturation process activates RT and IN for reverse transcriptionand subsequent integration of TED sequences into the host T. nigenome. Thus, proper proteolytic processing of VLP is an essentialstep in transposition. The intracellular site for assembly andprocessing of TED VLP and whether VLP bud from the plasma membraneremain to be determined.

PR processing of Pr55^gag and Pr195^gag-pol. By using baculovirus vectors and TED gag-specific antisera, we have demonstrated that the major VLP structural protein p37^gag of TED is derived from precursor Pr55^gag, confirming earlier studies (30). As expected, p37^gag is also generated from Pr195^gag-pol (Fig. 3). On the basis of the fact that replacement of the criticalaspartate (D⁴³⁶V) within the consensus active site of PR abolished processing(Fig. 2), TED PR is responsible for these cleavages. Althoughthe D⁴³⁶V loss-of-function mutation did not affect VLP formation (Fig.2), it is likely that loss of PR disrupts TED transposition, sincePR is required for retrotransposition and retrovirus replication(20, 23, 43, 51). Interestingly, coexpression of TED gag-poland PR-deficient gag-pol inhibited Pr55^gag processing by the wild-type PR (12). This dominant inhibitionof PR by PR-deficient Pr195^gag-pol is consistent with the requirement of Gag-Pol polyprotein dimerizationfor PR activity in a manner analogous to that of the vertebrateretroviruses (reviewed in references 5 and 49).

CA and NC functions of TED p37^gag. For the retroviruses, proteolytic cleavage releases the MA, CA, and NC domains from the Gag precursor, thereby irreversiblypreparing the virus particle for reverse transcription and subsequentuncoating (reviewed in references 7, 49 and 50). In thecase of TED, our studies indicated that Gag precursor Pr55^gag is cleaved to yield the single structural protein p37^gag, which may provide both CA and NC functions. PR-mediated cleavageoccurred between Gag residues 305 and 325, as shown by the useof C-terminal Gag truncations (Fig. 5) and PR cleavage of thefusion protein Gag-P35 (Fig. 6). Cleavage removed the 9-kDa acidicdomain from the C terminus of Pr55^gag and placed the basic, proline-rich NC domain at the C terminusof p37^gag (Fig. 5A). Thus, the position of the predicted NC (residues 199to 314) of TED is analogous to that of the NC of other retroelements(reviewed in references 5, 7 and 38).

Unlike many retroelements, including the gypsy-related retrotransposon Ty3, TED Gag lacks retroviruslike major homology regionand zinc finger (C-X₂-C-X₄-H-X₄-C) motifs, located within CA andNC domains, respectively. In this respect, TED Gag resembles theGag protein of the retroviral foamy viruses (spumavirus genus),which also undergoes limited proteolysis at the C terminus only(reviewed in references 24 and 52). The predicted NC of TEDis distinguished by its unusually high proline content (23%),lack of acidic residues, and abundance of basic residues (pI,12.7). We have noted a striking similarity between the NC of TEDand the corresponding region within gag of Drosophila elementstom and 17.6 (Fig. 5A). The abundance of proline (22 and 14% intom and 17.6, respectively) and basic residues (pI values, 11.4and 11.6, respectively), plus the absence of a zinc finger, suggeststhat NC function is conserved among these insect gypsy elements.The potential role of the basic residues in the NC for RNA packagingby TED remains to be determined. Nonetheless, the proline-richNC also contributes to VLP assembly or stability. Stable VLP werenot recovered when a C-terminal deletion removed a large portionof the TED NC-producing truncation protein p25 (Fig. 7). In contrast,selective deletion of the C-terminal acidic domain, which produceda p37^gag-like protein, had no effect on VLP yields. Collectively, thesefindings suggest that TED p37^gag has both NC and CA properties.

Function of the TED acidic domain. Gypsy retroelements TED, tom, and 17.6 each contain acidic domains (Fig. 5A) analogous in size and charge (pI values, 3.4,3.3, and 3.3, respectively). This striking similarity also suggeststhat the function of the acidic domain is conserved. Due to itsacidic nature, it is unlikely that this domain participates directlyin RNA binding. Although this domain is not required for TED VLPassembly or PR-mediated proteolysis, it may regulate these events.Alternatively, since the acidic domain is adjacent to PR withinPr195^gag-pol, it may contribute to PR function from within the Gag-Pol precursor.Interestingly, by using immunoprecipitations with $alpha$ -p55 serum(Fig. 4) or epitope tagging (data not shown), we have failed todetect a separate acidic-domain-containing fragment. Thus, uponrelease by cleavage, the domain may have a short half-life ormay no longer be recognized by these sera.

MA function for TED Gag? As a potential retrovirus, TED gag is expected to encode an MA domain that promotes interaction between Gag proteins and thehost cell membrane for virus budding (reviewed in reference 5).Indeed, TED env encodes a 75-kDa glycoprotein (gp75^env) that localizes to membrane fractions of env-expressing cells(35). In T. ni cells, resident copies of TED actively producespliced, polyadenylated RNAs that encode gp75^env (12). Thus, TED VLP could generate enveloped, gp75^env-containing particles upon budding. However, due to low levelsof TED expression in T. ni, we have not yet detected budded VLP,with or without gp75^env. Thus, the role of TED Gag proteins in promoting membrane associationremains to be determined.

Production of TED Gag fusion proteins in insect cells. When fused to the heterologous protein P35, TED Gag retained the capacity to form VLP (Fig. 6). Moreover, baculovirus-directedexpression produced high yields of hybrid VLP that were readilypurified by single-step centrifugation. In yeast, the retrotransposonTy1 has been used to express Gag fusion proteins that self-assemble,facilitating the purification of recombinant proteins (1, 3).The efficiency of VLP assembly of TED Gag fusion proteins in insectculture, combined with the convenience and high level of expressionafforded by the baculovirus vector system (34), provides anotheradvantageous strategy for production of biologically importantproteins in eukaryotes.

	ACKNOWLEDGMENTS

We thank Doug LaCount for the design and construction of recombinant virus vGAG-P35 and for helpful comments during this study.We also thank Robert Lerch for the construction of several TED-containingviruses and plasmids and Jean Engelke for technical help in antibodyproduction.

This work was supported in part by Public Health Service grant AI25557 from the National Institute of Allergy and InfectiousDiseases (P.D.F.) and by NIH Predoctoral Traineeship GM07215 (K.L.H.).

	FOOTNOTES

^* Corresponding author. Mailing address: Institute for Molecular Virology, Bock Laboratories, University of Wisconsin $---$ Madison,1525 Linden Dr., Madison, WI 53706-1596. Phone: (608) 262-7774.Fax: (608) 262-7414. E-mail: pfriesen{at}facstaff.wisc.edu.

Present address: Department of Biological and Environmental Sciences, University of Tennessee, Chattanooga, TN 37403-2598.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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1.	Adams, S. E., K. M. Dawson, K. Gull, S. M. Kingsman, and A. J. Kingsman. 1987. The expression of hybrid HIV:Ty virus-like particles in yeast. Nature (London) 329:68-70[Medline].
2.	Adams, S. E., J. Mellor, K. Gull, R. B. Sim, M. F. Tuite, S. M. Kingsman, and A. J. Kingsman. 1987. The functions and relationships of Ty-VLP proteins in yeast reflect those of mammalian retroviral proteins. Cell 49:111-119[Medline].
3.	Adams, S. E., S. M. Richardson, S. M. Kingsman, and A. J. Kingsman. 1994. Expression vectors for the construction of hybrid Ty-VLPs. Mol. Biotechnol. 1:125-135[Medline].
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