Isolation of an Apoptosis Suppressor Gene of the Spodoptera littoralis Nucleopolyhedrovirus

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Journal of Virology, February 1999, p. 1278-1285, Vol. 73, No. 2
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Isolation of an Apoptosis Suppressor Gene of the Spodoptera littoralis Nucleopolyhedrovirus

Quansheng Du,¹^,² Dana Lehavi,¹ Ouriel Faktor,³ Yipeng Qi,² and Nor Chejanovsky¹^,^*

Entomology Department, Institute of Plant Protection, Agricultural Research Organization, The Volcani Center, Bet Dagan 50250,¹ and Department of Entomology, Faculty of Agriculture, The Hebrew University of Jerusalem, Rehovot 76100,³ Israel, and Institute of Virology, Wuhan University, Wuhan 430072, People's Republic of China²

Received 16 June 1998/Accepted 27 October 1998

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

Spodoptera frugiperda SF9 cells infected with mutants of the Autographa californica nucleopolyhedrovirus (AcMNPV) which lacka functional p35 gene undergo apoptosis, aborting the viral infection.The Spodoptera littoralis nucleopolyhedrovirus (SlNPV) was ableto suppress apoptosis triggered by v $Delta$ P35K/pol⁺, an AcMNPV p35 null mutant. To identify the putative apoptoticsuppressor gene of SlNPV, overlapping cosmid clones representingthe entire SlNPV genome were individually cotransfected alongwith genomic DNA of v $Delta$ P35K/pol⁺. Using this complementation assay, we isolated a SlNPV DNA fragmentthat was able to rescue the v $Delta$ P35K/pol⁺ infection in SF9 cells. By further subcloning and rescue, weidentified a novel SlNPV gene, Slp49. The Slp49 sequence predicteda 49-kDa polypeptide with about 48.8% identity to the AcMNPV apoptoticsuppressor P35. SLP49 displays a potential recognition site, TVTDG,for cleavage by death caspases. Recombinant AcMNPVs deficientin p35 bearing the Slp49 gene did not induce apoptosis and showedsuccessful productive infections in SF9 cells, indicating thatSlp49 is a functional homologue of p35. A 1.5-kbp Slp49-specifictranscript was identified in SF9 cells infected with SlNPV orwith vAc496, a v $Delta$ P35K/pol⁺-recombinant bearing Slp49. The discovery of Slp49 contributesto the identification of important functional motifs conservedin p35-like apoptotic suppressors and to the future isolationof p35-like genes from otherbaculoviruses.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Apoptosis is a normal physiological cell suicide program that is highly conserved among vertebrates and invertebrates (19,30, 38). This cell death program plays a critical role duringnormal development and tissue homeostasis, eliminating unwantedcells, including damaged and virus-infected cells, from the organism.Thus, animal viruses have evolved ways to evade, delay, or suppressthis important cell defense strategy (reviewed in reference 32).

Baculoviruses possess two type of genes with antiapoptotic activity, iap and p35, which can suppress apoptosis induced byvirus infection or by diverse stimuli in vertebrates or invertebrates(reviewed in reference 25). The iap genes from the baculovirusesCydia pomonella granulovirus and Orgia pseudotsugata nucleopolyhedrovirus,were isolated by their ability to block apoptosis of Spodopterafrugiperda SF21 cells induced by a p35 mutant of the Autographacalifornica nucleopolyhedrovirus (AcMNPV) (4, 10). Cellularhomologues of iap genes were identified in the genomes of insectsand vertebrates (12, 15, 23, 37).

The product of the p35 gene of AcMNPV inhibits a broad range of death proteases (caspases) (1, 3, 5, 39) activatedduring programmed cell death (reviewed in reference 35). p35is unique in gene databases (25), and the only homologue reportedso far is p35 of Bombyx mori NPV (BmNPV), a virus that has over90% nucleotide sequence identity with AcMNPV (20).

We have previously observed that AcMNPV induces apoptosis in Spodoptera littoralis SL2 cells, in contrast to S. littoralisNPV (SlNPV) (7), suggesting that the latter virus may containan antiapoptotic gene. To test this hypothesis, we first confirmedthat SlNPV was able to block apoptosis of S. frugiperda SF9 cellsinduced by either an AcMNPV p35 null mutant (16) or actinomycinD. This result provided the basis to search for the presence ofan apoptotic suppressor gene in the SlNPV genome. We report herethe identification of Slp49, a functional antiapoptotic gene ofSlNPV, isolated from an SlNPV cosmid library by complementingthe replication of an AcMNPV p35 null mutant in SF9 cells. Thepredicted amino acid sequence of SLP49 showed 48.8% identity toAcMNPV p35 and is the first gene isolated from a baculovirus distantfrom AcMNPV reported to be homologous to the p35 gene. RecombinantAcMNPVs defective in p35, bearing and expressing Slp49, did notinduce apoptosis in SF9, in contrast to their p35-deficientancestor.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Cell lines and viruses. S. frugiperda SF9 and Trichoplusia ni TN368 (18) cells were maintained and propagated in TNM-FH medium supplemented with10% heat-inactivated fetal bovine serum (31). Wild-type AcMNPVE-2 strain, SlNPV E-15 strain, and v $Delta$ 35K/LacZ were described previously(17, 29, 32) v $Delta$ P35K/pol⁺ was constructed by transfection of TN368 cells with v $Delta$ 35K/LacZand pI1 (8) DNAs by using Lipofectin (GIBCO-BRL). The polyhedron-positiverecombinant virus was isolated and purified by a standard plaqueassay (31).

Construction of a cosmid library of SlNPV, DNA cloning, and sequencing. SlNPV DNA was partially digested with Sau3AI and ligated into the vector Supercos 1 (Stratagene). Cosmid packaging and bacterialtransformation were performed as specified by the manufacturerinstructions. Cosmids, which encompassed the entire genome ofSlNPV, were selected from the library of clones after their analysisby digestion with restriction endonucleases and Southern blothybridization to SlNPV DNA. The cosmid DNA was purified on Qiagencolumns. Cosmid NotI-C was constructed by cloning the 30-kbp NotIfragment included in cosmid C50 intoSupercos.

Subclones of cosmid NotI-C were constructed in pBluescript SK-(Stratagene) by standard methods (24). pES2term was generatedby NdeI digestion of pES2 (bearing the EcoRI-SalI fragment ofSlNPV; map units 37.2 and 38.7, respectively) followed by endrepair with Klenow polymerase and blunt-end ligation. This generateda frameshift of the Slp49 open reading frame (ORF) at nucleotide1157, leading to premature termination at nucleotide 1196; thiswas confirmed by restriction analysis and DNA sequencing (27).

Plasmid clones were sequenced with specific synthetic primers. Sequence data were compiled and analyzed with Genetics ComputerGroup sequence analysis programs (11).

Marker rescue assay and isolation of recombinant viruses. Marker rescue assays were performed as described previously (4, 10, 33). Routinely, 1 µg of v $Delta$ P35K/pol⁺ DNA and 1 µg of test DNA (cosmid or plasmid DNA) were cotransfectedinto 4 × 10⁵ SF9 cells by lipofection. At 3 to 4 days after transfection,the cells were examined by light microscopy for the presence ofpolyhedra. Polyhedron-positive recombinant viruses were selectedfrom independent cotransfections and subjected to three roundsof plaque purification in SF9cells.

Extraction of fragmented DNA. DNA oligonucleosomes were extracted for 2 h at 37°C from virus-infected SF9 cells with a 10 mM Tris (pH 8.0)-1 mM EDTA-1%sodium dodecyl sulfate (SDS) buffer containing 70 µg of proteinaseK per ml, and NaCl (final concentration, 1 M) was added. The extractswere treated with phenol-chloroform and precipitated with ethanol,and resuspended DNA was analyzed by agarose gel electrophoresisas described previously (7).

Southern blot analysis. Viral DNA was digested with various restriction endonucleases as specified by the manufacturer and subjected to agarose gelelectrophoresis (0.8% agarose) for 16 h at 30 V. After photography,the gel was quick-blotted to a nitrocellulose membrane. Hybridizationwas performed as described previously (24), with the ³²P-labeled EcoRI-SalI fragment from pES2 bearing most of the Slp49codingsequence.

Western blot analysis. Wild-type AcMNPV-, v $Delta$ P35K/pol⁺-, or vAc496-infected cells were harvested and subjected to SDS-polyacrylamide gel electrophoresisand immunoblot analysis with either anti-P35 or anti-polyhedrinantiserum (7, 16).

Northern blot analysis. Total RNA was extracted from virus-infected SF9 cells at various times after infection by using TRI-reagent (Molecular ResearchCenter, Inc.) as specified by the manufacturer. RNA (20 µg) wasloaded onto a 1% agarose gel containing 6% formaldehyde and transferredto nitrocellulose membranes. Hybridization was performed in a50% formamide solution at 42°C with the same probe that was usedfor Southern blotanalysis.

Nucleotide sequence accession number. The nucleotide sequence presented in this report has been submitted to the EMBL Nucleotide Database and was assigned accessionno. AJ006751.

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

SlNPV infection inhibits apoptosis of SF9 cells. To search for potential SlNPV antiapoptotic genes, we first examined the ability of the virus to suppress apoptosis of SF9cells. Apoptosis was induced by infection of the cells with v $Delta$ P35K/pol⁺, an AcMNPV mutant lacking a functional p35 gene (16). At 24h, almost all the infected cells showed blebbing characteristicof apoptosis (data not shown) and DNA-fragmented oligonucleosomeladders were observed upon electrophoresis of extracted DNA (Fig.1A, lanes 2, 4, and 6). Infection of the cells with SlNPV at 24h prior to the addition of v $Delta$ P35K/pol⁺ inhibited apoptosis (lane 5). However, this result could be interpretedas interference of SlNPV with v $Delta$ P35K/pol⁺ infection, since addition of SlNPV to the cells 1 and 12 h priorto v $Delta$ P35K/pol⁺ infection did not block apoptosis completely (lanes 1 and 3,respectively). To confirm the ability of SlNPV infection to blockapoptosis, we induced apoptosis of SF9 cells by adding actinomycinD (9). Oligonucleosomes were detected in DNA extracted fromthe cells at 24 h after incubation with 250 ng of actinomycinD per ml (Fig. 1B, lane 5). SlNPV infection at 5, 24, and 48 h,prior to actinomycin D addition, blocked blebbing (data not shown)and oligonucleosome formation (lanes 2, 3, and 4, respectively).These results suggested that the SlNPV genome contained an antiapoptoticgene.

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FIG. 1. SlNPV infection of SF9 cells prevents induction of apoptosis by an AcMNPV p35 null mutant or by actinomycin D. DNA was extracted from 3 × 10⁵ SF9 cells infected with SlNPV at a multiplicity of infection of 5 (Sl + lanes indicated at the bottom of the figure). (A) v $Delta$ 35K/pol⁺ at a multiplicity of infection of 5 was added to the cells (Ac + lanes indicated at the bottom of the figure) at 0, 12, and 24 h after SlNPV infection (lanes 1 and 2, 3 and 4, and 5 and 6, respectively). At 24 h later, a sample for each pair of time points was extracted and analyzed by agarose electrophoresis. (B) Actinomycin D (250 ng/ml) was added at 1, 5, 24, and 48 h after SlNPV infection (lanes 1, 2, 3, and 4, respectively) or at 48 h for mock-infected cells (lane 5). The cells were harvested at 24 h after actinomycin D addition. Size markers in kilobase pairs are indicated on the right.

SlNPV contains an antiapoptotic gene. To identify the putative SlNPV antiapoptotic gene, we constructed a library of overlapping cosmid clones representing theentire SlNPV genome and assayed them for their ability to complementthe replication of v $Delta$ P35K/pol⁺. Cotransfection of the whole library and v $Delta$ P35K/pol⁺ DNA allowed replication of v $Delta$ P35K/pol⁺, resulting in formation of viral occluded bodies (polyhedra),detected by direct microscopic observation of the nuclei of thecells. v $Delta$ P35K/pol⁺ DNA transfected alone did not form polyhedra (data not shown).When the cosmids were individually cotransfected along with genomicDNA of v $Delta$ P35K/pol⁺, only one of them, C50, which corresponded to SlNPV map units25 to 54 (Fig. 2A), was positive. The fact that cosmids C80 andC6 (adjacent to C50) were negative for occluded virus rescue suggestedthat the complementing activity was present in the NotI-C fragmentof SlNPV (Fig. 2A). Further subcloning of smaller DNA fragmentsof C50 in Bluescript and their assay in cotransfections as describedabove (Fig. 2B and C), allowed us to assign the complementingactivity to a 2.4-kbp fragment, which corresponded to SlNPV mapunits 37.2 to 38.7 (Fig. 2C).

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FIG. 2. Rescue of occluded AcMNPV by cosmids and plasmids bearing SlNPV DNA fragments. (A) NotI linear restriction map of SlNPV. The scales above indicate SlNPV map units (mu) and kilobase pairs. The bars below (C80, C50, C3, and C50) represent the various overlapping cosmids of the genomic SlNPV cosmid library. (B) Restriction map of the cosmid C50 and individual plasmid subclones indicating their ability to rescue or not (+ and $-$ , respectively) the replication of v $Delta$ 35K/pol⁺, as detected by the presence of polyhedra in the nuclei of SF9 cells cotransfected with v $Delta$ 35K/pol⁺ and plasmid DNA. N, NotI; P, PstI; A, ApaI. (C) Restriction map of the ApaI-PstI region corresponding to SlNPV 31.0 to 39.6 map units. S, SalI; K, KpnI; E, EcoRI. Also, subclones able to rescue v $Delta$ 35K/pol⁺ polyhedron formation, as in panel B, are indicated.

Sequencing of this fragment revealed the existence of only one complete ORF, capable of encoding a polypeptide of 446 aminoacids and a molecular mass of about 49 kDa (Fig. 3). This ORFis preceded by a putative TATA box element and by the late motifinitiator sequence ATTAG (2) at positions $-$ 53 and $-$ 40 upstreamof the ORF start, respectively (Fig. 3B, boxes). Also, a putativepolyadenylation signal was found 28 bp 3' of the termination codon(Fig. 3B, underlined). We designated this putative SlNPV geneSlp49.

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FIG. 3. ORF analysis of the SlNPV genome, at map units 37.0 to 38.7, and sequence of the Slp49 gene. (A) Diagram of ORFs in six reading frames. Vertical bars indicate stop codons. The location of the 446-amino-acid (aa) product corresponding to SLP49 is labeled. ORFs encoding products longer than 100 amino acids are indicated by open arrows. (B) Nucleotide and predicted amino acid sequence of SLP49. The early TATA box and a late transcriptional start site are indicated (open squares). A polyadenylation signal is underlined.

The polypeptide encoded by Slp49 has 48.8% amino acid identity and 66.8% similarity to the product of p35, the apoptotic suppressorgene of AcMNPV. Alignment of SLP49 and P35 revealed two main homologyblocks at the N termini (amino acids 1 to 219 and 1 to 198, respectively)and at the C termini (amino acids 346 to 446 and 219 to 299, respectively)(Fig. 4).

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FIG. 4. Comparison of Slp49 and p35 predicted amino acid sequences. The alignment was performed with the GAP program (11). The P35 sequence was reported previously (13). Horizontal dots indicate gaps made to optimize the alignment. Vertical bars, identical amino acids; vertical dots, similar amino acids.

P35 of AcMNPV and BmNPV are polypeptides of 299 amino acids, in contrast to Slp49, which is 446 amino acids. To investigateif the intact 3' end of Slp49, including the putative SLP49 Cterminus, was required to rescue the infectivity of v $Delta$ P35K/pol⁺, we prepared two different deletion mutants (pKS $Delta$ S1-2 and pES $Delta$ S1-2)and one premature termination mutant (pES2term) with mutationsin the Slp49 ORF (Fig. 5). None of the mutants displayed occluded-virusrescue activity (Fig. 5), suggesting that the 3'-end of the genewas required for Slp49 function.

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FIG. 5. Contribution of the Slp49 3' end and SLP49 C terminus to the rescue of the replication of v $Delta$ 35K/pol⁺. The plasmids, pES2 bearing the complete Slp49 ORF, pES $Delta$ S1-2 and pKS $Delta$ S1-2, with the Slp49 3' end deleted, and pESterm, displaying a frameshift causing a mutation in SLP49 amino acid 352 resulting in termination of the peptide at amino acid 364, were cotransfected separately with v $Delta$ P35K/pol⁺ DNA. Success (+) or failure ( $-$ ) to rescue v $Delta$ 35K/pol⁺ replication was monitored as indicated in Fig. 2. S, SalI; K, KpnI; E, EcoRI; P, PstI.

Recombinant AcMNPVs expressing Slp49. Recombinant AcMNPVs exhibiting the occlusion-positive phenotype were isolated from the extracellular medium derived from cotransfectionsperformed with v $Delta$ P35K/pol⁺ DNA and either cosmid C50 or plasmids pKP and pKS2 (Fig. 2C).The recombinant viruses were designated vAcp491 and vAcp492, vAcp493and vAcp494, and vAcp495 and vAcp496 (two recombinants per transfection).Infection of SF9 cells with these viruses resulted in polyhedrinsynthesis at steady-state levels comparable to infection withwild-type AcMNPV, as detected by immunoblot analysis of extractsfrom infected cells (shown for the recombinant vAcp496 in Fig.6A, lanes 3 and 4). v $Delta$ P35K/pol⁺-infected cells showed much lower levels of polyhedrin, detectedafter prolonged incubation of the blot with the chromogenic substrate(lane 2). Also, as expected, no synthesis of P35 was detectedin v $Delta$ P35K/pol⁺- or vAcp496-infected cells (Fig. 6B, lanes 3, 4, 6, and 7) orin mock-infected cells (lanes 1 and 2), in contrast to wild-type-AcMNPV-infectedcells (lanes 5 and 8).

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FIG. 6. Infection of SF9 cells with a recombinant virus bearing the Slp49 gene. (A) Extracts from SF9 cells (4 × 10⁵) were mock infected (lane 1) or infected at a multiplicity of infection of 10 with v $Delta$ 35K/pol⁺, vAcp496, or AcMNPV (lanes 2, 3, and 4, respectively), harvested at 48 h after infection, and subjected to SDS-polyacrylamide gel electrophoresis and immunoblot analysis with anti-polyhedrin antiserum (7). (B) Extracts from SF9 cells were mock infected (lanes 1 and 2) or infected at a multiplicity of infection of 10 with v $Delta$ P35K/pol⁺ (lanes 3 and 6) or vAcp496 (lanes 4 and 7) or AcMNPV (lanes 5 and 8). The cells were harvested 12 and 24 h later (lanes 1 and 3 to 5 and lanes 2 and 6 to 8, respectively) and analyzed as in panel A with anti-P35 antiserum. Molecular mass markers are indicated on the right.

Genomic DNAs from the recombinants vAcp491 to vAcp496 were subjected to restriction enzyme digestion with HindIII and PstIfollowed by Southern blot hybridization (Fig. 7A and B, lanes4 to 9 and 10 to 15, respectively). All of them (vAcp491 to vAcp496)bore DNA fragments that hybridized to a ³²P-labeled Slp49 DNA probe (Fig. 7B, lanes 4 to 9 and 10 to 15).AcMNPV or v $Delta$ P35K/pol⁺-restricted DNAs did not react with that probe (Fig. 7A and B,lanes 1 and 18 and lanes 2 and 17, respectively). SlNPV genomicDNA was positive in the hybridization (Fig. 7A and B, lanes 3and 16). Moreover, BglII-SalI digestion of genomic DNA of theabove recombinants released an 856-bp fragment (Fig. 7C and D,lanes 6 to 11) characteristic of Slp49 (lanes 4 and 5). That fragmentwas absent in the genomes of wild-type AcMNPV, v $Delta$ P35K/LacZ, andv $Delta$ P35K/pol⁺ (lanes 1, 2 and 3, respectively).

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FIG. 7. vAc-Slp49 recombinants bear the Slp49 gene. Restriction enzyme digestion (A and C) and Southern blot analysis (B and D). (A and B) HindIII or PstI-digested DNA (indicated at the top of the figure) from AcMNPV (lanes 1 and 18), v $Delta$ 35K/pol⁺ (lanes 2 and 17), SlNPV (lanes 3 and 16), or polyhedron-positive-phenotype recombinants vAcp491 to vAcp496 (lanes 4 to 9 and lanes 10 to 15). (C and D) BglII-SalI-digested DNA from AcMNPV (lane 1), v $Delta$ 35K/LacZ (lane 2), v $Delta$ 35K/pol⁺ (lane 3), pES (lane 4), SlNPV (lane 5), or polyhedron-positive-phenotype recombinants vAcp491 to vAcp496 (lanes 6 to 11). A BglII-SalI 856-bp ³²P-labeled Slp49 fragment (Fig. 3A) was used for hybridization.

Infection of SF9 cells with v $Delta$ P35K/pol⁺ induced apoptosis displaying an oligonucleosome ladder characteristic of fragmentedDNA (Fig. 8, lane 1), in contrast to infection with recombinantvAcp496 bearing the Slp49 gene (lane 3) or wild-type AcMNPV (lane2). Control mock-infected cells did not show the oligonucleosomalladder (lane 5). Concomitantly, a transcript of 1.5 kbp that hybridizedto a Slp49-specific DNA-labeled probe was detected by Northernanalysis of RNA extracted from SF9 cells infected with vAcp496(Fig. 9, lanes 9 to 14). A similar transcript was present in SlNPV-infectedcells (lanes 6 to 8). Control RNA from AcMNPV- or v $Delta$ P35K/pol⁺-infected cells (lanes 2 and 3 and lanes 4 and 5, respectively)or from mock-infected cells (lane 1), did not react with the Slp49probe. Also, a larger transcript (about 2.9 kbp) reacted withthe Slp49 probe in vAcp496-infected cells (Fig. 9) and SlNPV-infectedcells showed a second Slp49 probe-positive transcript (about 2.6kbp). Slp49 transcripts were detected first at 3 h after vAcp496infection of SF9 cells (Fig. 9, lane 9) and 6 h after infectionwith SlNPV (data not shown).

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FIG. 8. vAcp496 suppresses apoptosis in SF9 cells. DNA extracted from the cells infected with v $Delta$ 35K/pol⁺, AcMNPV, or vAcp496 (indicated at the top of each lane) was analyzed by agarose gel electrophoresis. mi, mock-infected cells. Size markers are indicated on the left.

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FIG. 9. Temporal analysis of Slp49 transcription in SlNPV- and vAcp496-infected SF9 cells. A Northern blot of total RNA extracted from mock-infected cells (lane 1) or cells infected with AcMNPV (lanes 2 and 3), v $Delta$ 35K/pol⁺ (lanes 4 and 5), SlNPV (lanes 6 to 8), or vAcp496 (lanes 9 to 14) is shown. RNA was extracted at 3 h (lane 9), 6 h (lane 10), 9 h (lane 11), 12 h (lanes 2, 4, 6, and 12), 18 h (lanes 7 and 13), and 24 h (lanes 3, 5, 8, and 14) after infection. The ³²P-labeled Slp49 fragment used for hybridization was the same as in Fig. 7. Size markers (in kilobase pairs) are indicated on the right.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

We identified a gene of SlNPV, Slp49, which blocks apoptosis induced by infection of SF9 cells with v $Delta$ P35K/pol⁺, a p35-deficient mutant of AcMNPV. Slp49-bearing plasmids wereable to rescue the replication of v $Delta$ P35K/pol⁺ (Fig. 2) and donate the Slp49 gene to v $Delta$ P35K/pol⁺ recombinants, blocking apoptosis of SF9 cells (Fig. 7 and 9).

Slp49 encodes a predicted 49-kDa polypeptide, SLP49. The SLP49 amino acid sequence has 48.8% identity and 66.8% similaritywith P35, the apoptotic suppressor of AcMNPV. The homology betweenSLP49 and P35 is concentrated in two major blocks located at theN termini (amino acids 1 to 219 and 1 to 198, respectively) andat the C termini (amino acids 346 to 446 and 219 to 299, respectively)of the polypeptides (Fig. 4). Interestingly the N-terminal halfof P35, between amino acids 1 and 130, was very sensitive to insertionalmutagenesis, resulting in loss of the ability to rescue a p35-deficientmutant of AcMNPV (3).

SLP49 is larger than P35 from AcMNPV (13) or BmNPV (20). A shorter SLP49, obtained by frame shift mutation of SLP49 atamino acid 352, failed to complement the replication of v $Delta$ P35K/pol⁺ (Fig. 5), indicating that the predicted C terminus of the proteinis important for its function. The amino acid sequence betweenSLP49 amino acids 268 and 345 is not present in P35, and its contributionto SLP49 function remains to be elucidated. It may confer specificityto the protein in its interaction with other viral or hostproteins.

SLP49 displays the motif TVTDX (X = G; N-terminal sequence underlined) at amino acids 90 to 94, similar to the P4 to P1 sequenceN'-terminal to the D-X peptide cleavage site recognized by deathcaspases (26, 39). Similar sequence motifs are present incaspase inhibitors like P35 (DQMDG in A. californica P35; DKIDGin B. mori P35) (3, 5, 28, 34, 39) or short peptides(YVADG in interleukin-1 $beta$ ) (34) in S. frugiperda caspase-1-processingsites (TETDG) (1) and in caspase targets (6, 22). Althoughother putative caspase recognition sites (reviewed in reference26) such as SRGDX (X = L) at amino acids 112 to 115 are presentin SLP49, the SLP49-P35 alignment (Fig. 4) suggests that TVTDGmay be the preferred caspase-cleavable site, given that it isin a conserved position with respect to the P35 recognition site.Experiments designed to assess that assumption are in progress(seebelow).

Taken together, the above data suggest that SLP49 may block apoptosis by inhibiting death caspases. An intriguing questionis if SLP49 will show wide apoptosis suppression ability by beingan inhibitor of a broad spectrum of caspases like P35. We willaddress this question by (i) overexpressing Slp49 and studyingits ability to compete with various caspase-specific substrates(3, 5, 39) and (ii) studying caspase-mediated cleavageofSLP49.

An Slp49 1.5-kbp transcript was present in SlNPV- and vAc496-infected SF9 cells (Fig. 9). This transcript was prominent 12h after SlNPV infection, suggesting that the inhibitory functionof Slp49 may coincide with caspase activation, detectable at theonset of viral DNA replication. It was shown that higher steady-statelevels of P35 and caspase inhibition by P35 cleavage coincidewith the initiation of AcMNPV DNA synthesis (14, 21). Also,a 2.6-kbp transcript and a 2.9-kbp transcript were detected bythe Slp49 probe, in SlNPV- and vAc496-infected SF9 cells, respectively.Since a double-stranded DNA-labeled probe was used for hybridization,it is conceivable that larger transcripts corresponding to adjacentgenes (like the cathepsin gene for SlNPV, located 5' upstreamof Slp49 [11a]) were reacting withit.

Is Slp49 essential for SlNPV replication? To answer this question, we will attempt to isolate Slp49-deficient viablemutants.

Finally, the discovery of Slp49 suggests that more p35-like genes may exist in baculoviruses and probably in the animal kingdom.The sequence similarities found between p35 and Slp49 may provideclues that will enable the design of degenerate primers to attemptthe identification of those p35-like genes, e.g., by PCR-mediatedapproaches.

	ACKNOWLEDGMENTS

We thank Gennadii Polubessov, Plant Genetics Department, The Weizmann Institute of Science, for assistance with computeranalysis.

We acknowledge support for this research by the Israel Science Foundation under grant 398/96-1 to N.C.

	FOOTNOTES

^* Corresponding author. Mailing address: Entomology Department, Institute of Plant Protection, The Volcani Center, POB 6, BetDagan 50250, Israel. Phone: (972)-3-9683694. Fax: (972)-3-9604180.E-mail: ninar{at}netvision.net.il.

Contribution 525/98 from the Agricultural Research Organization, The Volcani Center, Bet Dagan,Israel.

REFERENCES

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Abstract
Introduction
Materials and methods
Results
Discussion
References

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5. Bump, N. J., M. Hackett, M. Hugunin, S. Seshagiri, K. Brady, P. Chen, C. Ferenz, S. Franklin, T. Ghayur, P. Li, P. Licari, J. Mankovich, L. F. Shi, A. H. Greenberg, L. K. Miller, and W. W. Wong. 1995. Inhibition of ice family proteases by baculovirus antiapoptotic protein p35. Science 269:1885-1888[Abstract/Free Full Text].

6. Casciola-Rosen, L., D. W. Nicholson, T. Chong, K. R. Rowan, N. A. Thornberry, D. K. Miller, and A. Rosen. 1996. Apopain/CPP32 cleaves proteins that are essential for cellular repair: a fundamental principle of apoptotic death. J. Exp. Med. 183:1957-1964[Abstract/Free Full Text].

7. Chejanovsky, N., and E. Gershburg. 1995. The wild-type Autographa californica nuclear polyhedrosis virus induces apoptosis of Spodoptera littoralis cells. Virology 209:519-525[Medline].

8. Chejanovsky, N., N. Zilberberg, H. Rivkin, E. Zlotkin, and M. Gurevitz. 1995. Functional expression of an alpha anti-insect scorpion neurotoxin in insect cells and lepidopterous larvae. FEBS Lett. 376:181-184[Medline].

9. Clem, R. J., and L. K. Miller. 1994. Control of programmed cell death by the baculovirus genes p35 and iap. Mol. Cell. Biol. 14:5212-5222[Abstract/Free Full Text].

10. Crook, N. E., R. J. Clem, and L. K. Miller. 1993. An apoptosis-inhibiting baculovirus gene with a zinc finger-like motif. J. Virol. 67:2168-2174[Abstract/Free Full Text].

11. Devereux, J. D., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395.

11a. Du, Q., and N. Chejanovsky. Unpublished data.

12. Duckett, C. S., V. E. Nava, R. W. Gedrich, R. J. Clem, J. L. Vandongen, M. C. Gilfillan, H. Shiels, J. M. Hardwick, and C. B. Thompson. 1996. A conserved family of cellular genes related to the baculovirus iap gene and encoding apoptosis inhibitors. EMBO J. 15:2685-2694[Medline].

13. Friesen, P. D., and L. K. Miller. 1987. Divergent transcription of early 35- and 94-kilodalton protein genes encoded by the HindIII K genome fragment of the baculovirus Autographa californica nuclear polyhedrosis virus. J. Virol. 61:2264-2272[Abstract/Free Full Text].

14. Gershburg, E., H. Rivkin, and N. Chejanovsky. 1997. Expression of the Autographa californica M nuclear polyhedrosis virus apoptotic suppressor gene p35 in nonpermissive Spodoptera littoralis cells. J. Virol. 71:7593-7599[Abstract].

15. Hay, B. A., D. A. Wassarman, and G. M. Rubin. 1995. Drosophila homologs of baculovirus inhibitor of apoptosis proteins function to block cell death. Cell 83:1253-1262[Medline].

16. Hershberger, P. A., J. A. Dickson, and P. D. Friesen. 1992. Site-specific mutagenesis of the 35-kilodalton protein gene encoded by Autographa californica nuclear polyhedrosis virus: cell line-specific effects on virus replication. J. Virol. 66:5525-5533[Abstract/Free Full Text].

17. Hershberger, P. A., D. J. LaCount, and P. D. Friesen. 1994. The apoptotic suppressor P35 is required early during baculovirus replication and is targeted to the cytosol of infected cells. J. Virol. 68:3467-3477[Abstract/Free Full Text].

18. Hink, W. F. 1970. Established insect cell line from cabbage looper, Trichoplusia ni. Nature (London) 225:466-467.

19. Jacobson, M. D., M. Weill, and M. C. Raff. 1997. Programmed cell death in animal development. Cell 88:347-354[Medline].

20. Kamita, S. G., K. Majima, and S. Maeda. 1993. Identification and characterization of the p35 gene of Bombyx mori nuclear polyhedrosis virus that prevents virus-induced apoptosis. J. Virol. 64:455-463.

21. LaCount, D. J., and P. D. Friesen. 1997. Role of early and late replication events in induction of apoptosis by baculoviruses. J. Virol. 71:1530-1537[Abstract].

22. Lazebnik, Y. A., S. H. Kaufmann, S. Desnoyers, G. G. Poirier, and W. C. Earnshaw. 1994. Cleavage of poly(ADP-ribose) polymerase by a proteinase with properties like ICE. Nature (London) 371:346-347[Medline].

23. LIston, P., N. Roy, K. Tamai, C. Lefebvre, S. Baird, G. Chertonhorvat, R. Farahani, M. Mclean, J. E. Ikeda, A. Mackenzie, and R. G. Korneluk. 1996. Suppression of apoptosis in mammalian cells by NAIP and a related family of iap genes. Nature (London) 379:349-353[Medline].

24. Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

25. Miller, L. K. 1997. Baculovirus interaction with host apoptotic pathways. J. Cell. Physiol. 173:178-182[Medline].

26. Nicholson, D. W., and N. A. Thornberry. 1997. Caspases: killer proteases. Trends Biochem. Sci. 22:299-306[Medline].

27. Sanger, F., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain-terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].

28. Seshagiri, S., and L. K. Miller. 1997. Baculovirus inhibitors of apoptosis (IAPs) block activation of Sf-caspase-1. Proc. Natl. Acad. Sci. USA 94:13606-13611[Abstract/Free Full Text].

29. Smith, G. E., and M. D. Summers. 1978. Analysis of baculovirus genomes with restriction endonucleases. Virology 98:517-527.

30. Steller, H. 1995. Mechanisms and genes of cellular suicide. Science 267:1445-1449[Abstract/Free Full Text].

31. Summers, M. D., and G. E. Smith. 1978. A manual of methods for baculovirus vectors and insect cell culture procedures. Texas Agricultural Experiment Station bulletin 1555. Texas Agricultural Experiment Station, College Station, Tex.

32. Teodoro, J. G., and P. Branton. 1997. Regulation of apoptosis by viral gene products. J. Virol. 71:1739-1746[Medline].

33. Thiem, S. M., X. L. Du, M. E. Quentin, and M. M. Berner. 1996. Identification of a baculovirus gene that promotes Autographa californica nuclear polyhedrosis virus replication in a nonpermissive insect cell line. J. Virol. 70:2221-2229[Abstract].

34. Thornberry, N. A., and S. M. Molineaux. 1995. Interleukin-1 $beta$ converting enzyme: a novel cystein protease required for IL-1 $beta$ production and implicated in programmed cell death. Protein Sci. 4:3-12[Abstract].

35. Thornberry, N. A., A. Rosen, and D. W. Nicholson. 1997. Control of apoptosis by proteases. Adv. Pharmacol. 41:155-177.

36. Toister-Achituv, M., and O. Faktor. 1997. Transcriptional analysis and promoter activity of the Spodoptera littoralis multicapsid nucleopolyhedrovirus ecdysteroid UDP-glucosyltransferase gene. J. Gen. Virol. 78:487-491[Abstract].

37. Uren, A. G., M. Pakusch, C. J. Hawkins, K. L. Puls, and D. L. Vaux. 1996. Cloning and expression of apoptosis inhibitory protein homologs that function to inhibit apoptosis and/or bind tumor necrosis factor receptor-associated factors. Proc. Natl. Acad. Sci. USA 93:4974-4978[Abstract/Free Full Text].

38. Vaux, D. L., and A. Strasser. 1996. The molecular biology of apoptosis. Proc. Natl. Acad. Sci. USA 93:2239-2244[Abstract/Free Full Text].

39. Xue, D., and H. R. Horvitz. 1995. Inhibition of the Caenorhabditis elegans cell-death protease CED-3 by a CED-3 cleavage site in baculovirus p35 protein. Nature (London) 377:248-251[Medline].

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J. Bacteriol.	Mol. Cell. Biol.	Microbiol. Mol. Biol. Rev.

Clin. Vaccine Immunol.	ALL ASM JOURNALS

1.	Ahmad, M., S. M. Srinivasula, L. Wang, G. Litwack, T. Fernandes-Alnemri, and E. S. Almemri. 1997. Spodoptera frugiperda caspase-1, a novel insect death protease that cleaves the nuclear immunophilin FKBP46, is the target of the baculovirus antiapoptotic protein p35. J. Biol. Chem. 272:1421-1424[Abstract/Free Full Text].
2.	Ayres, M. D., S. C. Howard, J. Kuzio, M. Lopez-Ferber, and R. D. Possee. 1994. The complete DNA sequence of Autographa californica nuclear polyhedrosis virus. Virology 202:586-605[Medline].
3.	Bertin, J., S. M. Mendrysa, D. J. Lacount, S. Gaur, J. F. Krebs, R. C. Armstrong, K. J. Tomaselli, and P. D. Friesen. 1996. Apoptotic suppression by baculovirus p35 involves cleavage by and inhibition of a virus-induced ced-3/ice-like protease. J. Virol. 70:6251-6259[Abstract].
4.	Birnbaum, M. J., R. J. Clem, and L. K. Miller. 1994. An apoptosis-inhibiting gene from a nuclear polyhedrosis virus encoding a polypeptide with Cys/His sequence motif. J. Virol. 68:2521-2528[Abstract/Free Full Text].
5.	Bump, N. J., M. Hackett, M. Hugunin, S. Seshagiri, K. Brady, P. Chen, C. Ferenz, S. Franklin, T. Ghayur, P. Li, P. Licari, J. Mankovich, L. F. Shi, A. H. Greenberg, L. K. Miller, and W. W. Wong. 1995. Inhibition of ice family proteases by baculovirus antiapoptotic protein p35. Science 269:1885-1888[Abstract/Free Full Text].
6.	Casciola-Rosen, L., D. W. Nicholson, T. Chong, K. R. Rowan, N. A. Thornberry, D. K. Miller, and A. Rosen. 1996. Apopain/CPP32 cleaves proteins that are essential for cellular repair: a fundamental principle of apoptotic death. J. Exp. Med. 183:1957-1964[Abstract/Free Full Text].
7.	Chejanovsky, N., and E. Gershburg. 1995. The wild-type Autographa californica nuclear polyhedrosis virus induces apoptosis of Spodoptera littoralis cells. Virology 209:519-525[Medline].
8.	Chejanovsky, N., N. Zilberberg, H. Rivkin, E. Zlotkin, and M. Gurevitz. 1995. Functional expression of an alpha anti-insect scorpion neurotoxin in insect cells and lepidopterous larvae. FEBS Lett. 376:181-184[Medline].
9.	Clem, R. J., and L. K. Miller. 1994. Control of programmed cell death by the baculovirus genes p35 and iap. Mol. Cell. Biol. 14:5212-5222[Abstract/Free Full Text].
10.	Crook, N. E., R. J. Clem, and L. K. Miller. 1993. An apoptosis-inhibiting baculovirus gene with a zinc finger-like motif. J. Virol. 67:2168-2174[Abstract/Free Full Text].
11.	Devereux, J. D., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395.
11a.	Du, Q., and N. Chejanovsky. Unpublished data.
12.	Duckett, C. S., V. E. Nava, R. W. Gedrich, R. J. Clem, J. L. Vandongen, M. C. Gilfillan, H. Shiels, J. M. Hardwick, and C. B. Thompson. 1996. A conserved family of cellular genes related to the baculovirus iap gene and encoding apoptosis inhibitors. EMBO J. 15:2685-2694[Medline].
13.	Friesen, P. D., and L. K. Miller. 1987. Divergent transcription of early 35- and 94-kilodalton protein genes encoded by the HindIII K genome fragment of the baculovirus Autographa californica nuclear polyhedrosis virus. J. Virol. 61:2264-2272[Abstract/Free Full Text].
14.	Gershburg, E., H. Rivkin, and N. Chejanovsky. 1997. Expression of the Autographa californica M nuclear polyhedrosis virus apoptotic suppressor gene p35 in nonpermissive Spodoptera littoralis cells. J. Virol. 71:7593-7599[Abstract].
15.	Hay, B. A., D. A. Wassarman, and G. M. Rubin. 1995. Drosophila homologs of baculovirus inhibitor of apoptosis proteins function to block cell death. Cell 83:1253-1262[Medline].
16.	Hershberger, P. A., J. A. Dickson, and P. D. Friesen. 1992. Site-specific mutagenesis of the 35-kilodalton protein gene encoded by Autographa californica nuclear polyhedrosis virus: cell line-specific effects on virus replication. J. Virol. 66:5525-5533[Abstract/Free Full Text].
17.	Hershberger, P. A., D. J. LaCount, and P. D. Friesen. 1994. The apoptotic suppressor P35 is required early during baculovirus replication and is targeted to the cytosol of infected cells. J. Virol. 68:3467-3477[Abstract/Free Full Text].
18.	Hink, W. F. 1970. Established insect cell line from cabbage looper, Trichoplusia ni. Nature (London) 225:466-467.
19.	Jacobson, M. D., M. Weill, and M. C. Raff. 1997. Programmed cell death in animal development. Cell 88:347-354[Medline].
20.	Kamita, S. G., K. Majima, and S. Maeda. 1993. Identification and characterization of the p35 gene of Bombyx mori nuclear polyhedrosis virus that prevents virus-induced apoptosis. J. Virol. 64:455-463.
21.	LaCount, D. J., and P. D. Friesen. 1997. Role of early and late replication events in induction of apoptosis by baculoviruses. J. Virol. 71:1530-1537[Abstract].
22.	Lazebnik, Y. A., S. H. Kaufmann, S. Desnoyers, G. G. Poirier, and W. C. Earnshaw. 1994. Cleavage of poly(ADP-ribose) polymerase by a proteinase with properties like ICE. Nature (London) 371:346-347[Medline].
23.	LIston, P., N. Roy, K. Tamai, C. Lefebvre, S. Baird, G. Chertonhorvat, R. Farahani, M. Mclean, J. E. Ikeda, A. Mackenzie, and R. G. Korneluk. 1996. Suppression of apoptosis in mammalian cells by NAIP and a related family of iap genes. Nature (London) 379:349-353[Medline].
24.	Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
25.	Miller, L. K. 1997. Baculovirus interaction with host apoptotic pathways. J. Cell. Physiol. 173:178-182[Medline].
26.	Nicholson, D. W., and N. A. Thornberry. 1997. Caspases: killer proteases. Trends Biochem. Sci. 22:299-306[Medline].
27.	Sanger, F., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain-terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].
28.	Seshagiri, S., and L. K. Miller. 1997. Baculovirus inhibitors of apoptosis (IAPs) block activation of Sf-caspase-1. Proc. Natl. Acad. Sci. USA 94:13606-13611[Abstract/Free Full Text].
29.	Smith, G. E., and M. D. Summers. 1978. Analysis of baculovirus genomes with restriction endonucleases. Virology 98:517-527.
30.	Steller, H. 1995. Mechanisms and genes of cellular suicide. Science 267:1445-1449[Abstract/Free Full Text].
31.	Summers, M. D., and G. E. Smith. 1978. A manual of methods for baculovirus vectors and insect cell culture procedures. Texas Agricultural Experiment Station bulletin 1555. Texas Agricultural Experiment Station, College Station, Tex.
32.	Teodoro, J. G., and P. Branton. 1997. Regulation of apoptosis by viral gene products. J. Virol. 71:1739-1746[Medline].
33.	Thiem, S. M., X. L. Du, M. E. Quentin, and M. M. Berner. 1996. Identification of a baculovirus gene that promotes Autographa californica nuclear polyhedrosis virus replication in a nonpermissive insect cell line. J. Virol. 70:2221-2229[Abstract].
34.	Thornberry, N. A., and S. M. Molineaux. 1995. Interleukin-1 $beta$ converting enzyme: a novel cystein protease required for IL-1 $beta$ production and implicated in programmed cell death. Protein Sci. 4:3-12[Abstract].
35.	Thornberry, N. A., A. Rosen, and D. W. Nicholson. 1997. Control of apoptosis by proteases. Adv. Pharmacol. 41:155-177.
36.	Toister-Achituv, M., and O. Faktor. 1997. Transcriptional analysis and promoter activity of the Spodoptera littoralis multicapsid nucleopolyhedrovirus ecdysteroid UDP-glucosyltransferase gene. J. Gen. Virol. 78:487-491[Abstract].
37.	Uren, A. G., M. Pakusch, C. J. Hawkins, K. L. Puls, and D. L. Vaux. 1996. Cloning and expression of apoptosis inhibitory protein homologs that function to inhibit apoptosis and/or bind tumor necrosis factor receptor-associated factors. Proc. Natl. Acad. Sci. USA 93:4974-4978[Abstract/Free Full Text].
38.	Vaux, D. L., and A. Strasser. 1996. The molecular biology of apoptosis. Proc. Natl. Acad. Sci. USA 93:2239-2244[Abstract/Free Full Text].
39.	Xue, D., and H. R. Horvitz. 1995. Inhibition of the Caenorhabditis elegans cell-death protease CED-3 by a CED-3 cleavage site in baculovirus p35 protein. Nature (London) 377:248-251[Medline].