A Third-Generation Lentivirus Vector with a Conditional Packaging System

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Journal of Virology, November 1998, p. 8463-8471, Vol. 72, No. 11
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

A Third-Generation Lentivirus Vector with a Conditional Packaging System

Tom Dull,¹ Romain Zufferey,² Michael Kelly,¹ R. J. Mandel,¹ Minh Nguyen,¹ Didier Trono,² and Luigi Naldini¹^,^*

Cell Genesys, Foster City, California,¹ and Department of Genetics and Microbiology, University of Geneva Medical School, Geneva, Switzerland²

Received 1 June 1998/Accepted 21 July 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Vectors derived from human immunodeficiency virus (HIV) are highly efficient vehicles for in vivo gene delivery. However,their biosafety is of major concern. Here we exploit the complexityof the HIV genome to provide lentivirus vectors with novel biosafetyfeatures. In addition to the structural genes, HIV contains tworegulatory genes, tat and rev, that are essential for HIV replication,and four accessory genes that encode critical virulence factors.We previously reported that the HIV type 1 accessory open readingframes are dispensable for efficient gene transduction by a lentivirusvector. We now demonstrate that the requirement for the tat genecan be offset by placing constitutive promoters upstream of thevector transcript. Vectors generated from constructs containingsuch a chimeric long terminal repeat (LTR) transduced neuronsin vivo at very high efficiency, whether or not they were producedin the presence of Tat. When the rev gene was also deleted fromthe packaging construct, expression of gag and pol was strictlydependent on Rev complementation in trans. By the combined useof a separate nonoverlapping Rev expression plasmid and a 5' LTRchimeric transfer construct, we achieved optimal yields of vectorof high transducing efficiency (up to 10⁷ transducing units [TU]/ml and 10⁴ TU/ng of p24). This third-generation lentivirus vector uses onlya fractional set of HIV genes: gag, pol, and rev. Moreover, theHIV-derived constructs, and any recombinant between them, arecontingent on upstream elements and trans complementation forexpression and thus are nonfunctional outside of the vector producercells. This split-genome, conditional packaging system is basedon existing viral sequences and acts as a built-in device againstthe generation of productive recombinants. While the actual biosafetyof the vector will ultimately be proven in vivo, the improveddesign presented here should facilitate testing of lentivirusvectors.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Lentiviruses have attracted the attention of gene therapy investigators (45) for their ability to integrate into nondividingcells (8, 15, 16, 25, 26). We previously developedreplication-defective vectors from the lentivirus human immunodeficiencyvirus (HIV) and showed that they transduce target cells independentof mitosis (32). The vectors proved highly efficient for invivo gene delivery and achieved stable long-term expression ofthe transgene in several target tissues, such as the brain (5,33), the retina (31), and the liver and muscle of adult rats(21). A major concern, however, is the biosafety of vectorsderived from a highly pathogenic human virus.

The complexity of the lentivirus genome may be exploited to build novel biosafety features in the design of a retrovirus vector.In addition to the structural gag, pol, and env genes common toall retroviruses, HIV contains two regulatory genes, tat and rev,essential for viral replication, and four accessory genes, vif,vpr, vpu, and nef, that are not crucial for viral growth in vitrobut are critical for in vivo replication and pathogenesis (27).

The Tat and Rev proteins regulate the levels of HIV gene expression at transcriptional and posttranscriptional levels, respectively.Due to the weak basal transcriptional activity of the HIV longterminal repeat (LTR), expression of the provirus initially resultsin small amounts of multiply spliced transcripts coding for theTat, Rev, and Nef proteins. Tat increases dramatically HIV transcriptionby binding to a stem-loop structure (transactivation responseelement [TAR]) in the nascent RNA, thereby recruiting a cyclin-kinasecomplex that stimulates transcriptional elongation by the polymeraseII complex (46). Once Rev reaches a threshold concentration,it promotes the cytoplasmic accumulation of unspliced and singlyspliced viral transcripts, leading to the production of the lateviral proteins. Rev accomplishes this effect by serving as a connectorbetween an RNA motif (the Rev-responsive element [RRE]), foundin the envelope coding region of the HIV transcript, and componentsof the cell nuclear export machinery. Only in the presence ofTat and Rev are the HIV structural genes expressed and new viralparticles produced (27).

In a first generation of HIV-derived vectors (32), viral particles were generated by expressing the HIV type 1 (HIV-1) coreproteins, enzymes, and accessory factors from heterologous transcriptionalsignals and the envelope of another virus, most often the G proteinof the vesicular stomatitis virus (VSV G) (9) from a separateplasmid. In a second version of the system, the HIV-derived packagingcomponent was reduced to the gag, pol, tat, and rev genes of HIV-1(51). In either case, the vector itself carried the HIV-derivedcis-acting sequences necessary for transcription, encapsidation,reverse transcription, and integration (2, 4, 22, 24,29, 30, 32, 35). It thus encompassed, from the 5' to 3'end, the HIV 5' LTR, the leader sequence and the 5' splice donorsite, approximately 360 bp of the gag gene (with the gag readingframe closed by a synthetic stop codon), 700 bp of the env genecontaining the RRE and a splice acceptor site, an internal promoter(typically the immediate-early enhancer/promoter of human cytomegalovirus[CMV] or that of the phosphoglycerokinase gene [PGK]), the transgene,and the HIV 3' LTR. Vector particles are produced by cotransfectionof the three constructs in 293T cells (32). In this design,significant levels of transcription from the vector LTR and ofaccumulation of unspliced genomic RNA occur only in the presenceof Tat and Rev.

Here, we demonstrate that the trans-acting function of Tat becomes dispensable if part of the upstream LTR in the transfervector construct is replaced by constitutively active promotersequences. Furthermore, we show that the expression of rev intrans allows the production of high-titer HIV-derived vector stocksfrom a packaging construct which contains only gag and pol. Thisdesign makes the expression of the packaging functions conditionalon complementation available only in producer cells. The resultinggene delivery system, which conserves only three of the nine genesof HIV-1 and relies on four separate transcriptional units forthe production of transducing particles, offers significant advantagesfor its predicted biosafety.

	MATERIALS AND METHODS

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Transfer vector constructs. pHR'CMV-LacZ and pHR'CMV-Luciferase have been described elsewhere (32). pHR2 is a lentivirus transfer vector in which thepolylinker and downstream nef sequences up to the KpnI site ofpHR' have been replaced with a ClaI/SpeI/SnaBI/SmaI/BamHI/SacII/EcoRIpolylinker. pHR2 was generated by replacing the 3.7-kb ClaI-SacIfragment of pHR'CMVlacZ with a 607-bp ClaI-SacI fragment generatedby PCR using pHR'CMVlacZ as the template with oligonucleotideprimers 5'-CCATCGATGGACTAGTCCTACGTA TCCCCGGGGACGGGATCCGCGGAATTCCGTTTAAGACCAATGAC-3'and 5'-TTATAATGTCAAGGCCTCTC-3', followed by digestion with ClaIand SacI.

pHR2PGK-NGFR, pHR2CMV-NGFR, and pHR2MFG-NGFR are lentivirus transfer vectors in which the truncated low-affinity nerve growthfactor receptor (NGFR) (6) transgenes under the control ofthe murine PGK, human CMV, and Moloney leukemia virus (MLV) promoters,respectively, have been inserted into the polylinker of pHR2.The pHR2PGK-NGFR transgene encodes no intron sequences, the pHR2CMV-NGFRvector includes the intron from plasmid pMD (34), and the pHR2MFG-NGFRvector contains the MLV intron from MFG-S (34).

pRRL, pRLL, pCCL, and pCLL are lentivirus transfer vectors containing chimeric Rous sarcoma virus (RSV)-HIV or CMV-HIV 5'LTRs and vector backbones in which the simian virus 40 polyadenylationand (enhancerless) origin of replication sequences have been includeddownstream of the HIV 3' LTR, replacing most of the human sequenceremaining from the HIV integration site. In pRRL, the enhancerand promoter (nucleotides $-$ 233 to $-$ 1 relative to the transcriptionalstart site; GenBank accession no. J02342) from the U3 regionof RSV are joined to the R region of the HIV-1 LTR. In pRLL, theRSV enhancer (nucleotides $-$ 233 to $-$ 50) sequences are joined tothe promoter region (from position $-$ 78 relative to the transcriptionalstart site) of HIV-1. In pCCL, the enhancer and promoter (nucleotides $-$ 673 to $-$ 1 relative to the transcriptional start site; GenBankaccession no. K03104) of CMV were joined to the R region ofHIV-1. In pCLL, the CMV enhancer (nucleotides $-$ 673 to $-$ 220) wasjoined to the promoter region (position $-$ 78) of HIV-1. Exact sequencesand details of construction are available on request.

pHR2hPGK-GFP, pCCLhPGK-GFP, pCLLhPGK-GFP, pRRLhPGK-GFP, and pRLLhPGK.GFP are lentivirus transfer vectors containing the enhancedgreen fluorescent protein (eGFP) (750-bp BamHI-NotI fragment frompEGFP-1; Clontech) coding region, under the control of the humanPGK promoter (nucleotides 5 to 516; GenBank accession no. M11958),inserted into the polylinker region of each parental vector. pRRLGFPwas obtained by deletion of the XhoI-BamHI fragment containingthe PGK promoter from pRRLhPGK-GFP.

pRRLhPGK.GFP.SIN-18 is a vector in which 3' LTR sequences from $-$ 418 to $-$ 18 relative to the U3/R border have been deleted frompRLLhPGK.GFP (52).

Packaging constructs. The tat-defective packaging construct pCMV $Delta$ R8.93 was obtained by swapping an EcoRI-SacI fragment from plasmid R7/pneo( $-$ ) (12)with the corresponding fragment of pCMV $Delta$ R8.91, a previously describedplasmid expressing Gag, Pol, Tat, and Rev (51). This fragmenthas a deletion affecting the initiation codon of the tat geneand a frameshift created by the insertion of an MluI linker intothe Bsu36I site as described previously. pCMV $Delta$ R8.74 is a derivativeof pCMV $Delta$ R8.91 in which a 133-bp SacII fragment, containing a splicedonor site, has been deleted from the CMV-derived region upstreamof the HIV sequences to optimize expression.

pMDLg/p is a CMV-driven expression plasmid that contains only the gag and pol coding sequences from HIV-1. First, pkat2Lg/pwas constructed by ligating a 4.2-kb ClaI-EcoRI fragment frompCMV $Delta$ R8.74 with a 3.3-kb EcoRI-HindIII fragment from pkat2 (14)and a 0.9-kb HindIII-NcoI fragment from pkat2 along with an NcoI-ClaIlinker consisting of synthetic oligonucleotides 5'-CATGGGTGCGAGAGCGTCAGTATTAAGCGGGGGAGAATTAGAT-3'and 5'-CG ATCTAATTCTCCCCCGCTTAATACTGACGCTCTCGCACC-3'. Next, pMDLg/pwas constructed by inserting the 4.25-kb EcoRI fragment from pkat2Lg/pinto the EcoRI site of pMD-2. pMD-2 is a derivative of pMD.G (34)in which the pXF3 plasmid backbone of pMD.G has been replacedwith a minimal pUC plasmid backbone and the 1.6-kb VSV G-encodingEcoRI fragment has been removed.

pMDLg/pRRE differs from pMDLg/p by the addition of a 374-bp RRE-containing sequence from HIV-1 (HXB2) immediately downstreamof the pol coding sequences. To generate pMDLg/pRRE, the 374-bpNotI-HindIII RRE-containing fragment from pHR3 was ligated intothe 9.3-kb NotI-BglII fragment of pVL1393 (Invitrogen) along witha HindIII-BglII oligonucleotide linker consisting of syntheticoligonucleotides 5'-AGCTTCCGCGGA-3' and 5'-GATCTCCGCGGA-3' togenerate pVL1393RRE (pHR3 was derived from pHR2 by the removalof HIV env coding sequences upstream of the RRE sequences in pHR2).A NotI site remains at the junction between the gag and RRE sequences.pMDLg/pRRE was then constructed by ligating the 380-bp EcoRI-SstIIfragment from pV1393RRE with the 3.15-kb SstII-NdeI fragment frompMD-2FIX (pMD-2FIX is a human factor IX-containing variant ofpMD-2 which has an SstII site at the 3' end of the factor IX insert),the 2.25-kb NdeI-AvrII fragment from pMDLg/p, and the 3.09-kbAvrII-EcoRI fragment from pkat1Lg/p (14).

pRSV-Rev and pTK-Rev (generous gifts of T. Hope, Salk Institute) are rev cDNA-expressing plasmids in which the joined secondand third exons of HIV-1 rev are under the transcriptional controlof the RSV U3 and herpes simplex virus type 1 thymidine kinase(TK) promoters, respectively. Both expression plasmids utilizepolyadenylation signal sequences from the HIV LTR in a pUC118plasmid backbone.

Vector production and assays. Vectors were produced by transient transfection into 293T cells as previously described (33), with the following modifications.A total of 5 × 10⁶ 293T cells were seeded in 10-cm-diameter dishes 24 h prior totransfection in Iscove modified Dulbecco culture medium (JRH Biosciences)with 10% fetal bovine serum, penicillin (100 IU/ml), and streptomycin(100 µg/ml) in a 5% CO₂ incubator, and the culture medium waschanged 2 h prior to transfection. A total of 20 µg of plasmidDNA was used for the transfection of one dish: 3.5 µg of the envelopeplasmid pMD.G, 6.5 µg of packaging plasmid, and 10 µg of transfervector plasmid. The precipitate was formed by adding the plasmidsto a final volume of 450 µl of 0.1× TE (1× TE is 10 mM Tris [pH8.0] plus 1 mM EDTA) and 50 µl of 2.5 M CaCl₂, mixing well, thenadding dropwise 500 µl of 2× HEPES-buffered saline (281 mM NaCl,100 mM HEPES, 1.5 mM Na₂HPO₄ [pH 7.12]) while vortexing and immediatelyadding the precipitate to the cultures. The medium (10 ml) wasreplaced after 14 to 16 h; the conditioned medium was collectedafter another 24 h, cleared by low-speed centrifugation, and filteredthrough 0.22-µm-pore-size cellulose acetate filters. For in vitroexperiments, serial dilutions of freshly harvested conditionedmedium were used to infect 10⁵ cells in a six-well plate in the presence of Polybrene (8 µg/ml).Viral p24 antigen concentration was determined by immunocapture(Alliance; DuPont-NEN). Vector batches were tested for the absenceof replication-competent virus by monitoring p24 antigen expressionin the culture medium of transduced SupT1 lymphocytes for 3 weeks.In all cases tested, p24 was undetectable (detection limit, 3pg/ml) once the input antigen had been eliminated from the culture.Transducing activity was expressed in transducing units (TU).

Northern blot analysis. Total RNA was isolated from 1 × 10⁷ to 2 × 10⁷ cells harvested at confluence by using RNAsol B as suggested by the manufacturer;10 to 20 µg of RNA was loaded per well on 1% agarose gels, usingNorthernMax (Ambion, Austin, Tex.) reagents as described by themanufacturer. Transfer was to Zetabind membranes (Cuno Inc., Meridien,Conn.) by either capillary transfer or pressure blotting (Stratagene).³²P-labeled probes were made by random priming.

Intracerebral injection of vectors. Twelve Fischer 344 male rats weighing approximately 220 g were obtained from Harlan Sprague-Dawley (Indianapolis, Ind.). Therats were housed with access to ad libitum food and water on a12-h light/dark cycle and were maintained and treated in accordancewith published National Institutes of Health guidelines. All surgicalprocedures were performed with the rats under isoflurane gas anesthesia,using aseptic procedures. After a rat was anesthetized in a sleepbox, it was placed in a small animal stereotaxic device (KopfInstruments, Tujunga, Calif.) using the earbars, which do notbreak the tympanic membrane. The rats were randomly divided intoone control and four treatment groups. After the rats were placedin the stereotaxic frame, 2 µl of lentivirus vector concentratedby ultracentrifugation at 50,000 × g for 140 min at 20°C (33)in phosphate-buffered saline (PBS) was injected consecutivelyinto the striatum in both hemispheres over 4 min at a rate of0.5 µl/min (coordinates, AP 0.0, LAT ±3.0, DV $-$ 5.5, $-$ 4.5, $-$ 3.5with the incisor bar set at 3.3 mm below the intra-aural line[36]), using a continuous-infusion system as described previouslyin detail (28). During the injection, the needle was slowlyraised 1 mm in the dorsal direction every 40 s (3-mm total withdrawal).One minute after cessation of the injection, the needle was retractedan additional 1 mm and then left in place for an additional 4min before being slowly withdrawn from the brain.

Histology. One month after vector injection, each animal was deeply anesthetized with intraperitoneal pentobarbital and perfused throughthe aorta with sterile PBS, followed by ice-cold 4% paraformaldehydeperfusion. The brains were removed from the skulls, postfixedin 4% paraformaldehyde by immersion for 24 h, and then transferredinto a 30% sucrose-PBS solution for 3 to 4 days, until the brainssank to the bottom of their containers. The brains were then frozenon dry ice, and 40-µm-thick coronal sections were cut on a slidingmicrotome. Sections were collected in series in microtiter wellplates that contained a glycerin-based antifreeze solution, andthey were kept at $-$ 30°C until further processing. Immunocytochemistrywas performed according to the general procedure described previously(44). After several PBS rinses and an incubation in 3% hydrogenperoxide, the sections were placed in a 3% normal goat serum.The sections were then incubated in the primary anti-GFP antibody(1:1,000; Clontech, Palo Alto, Calif.) in 1% normal goat serum-0.1%Triton X-100 overnight at room temperature. After rinsing, thesections were incubated in the biotinylated rabbit anti-goat secondaryantibody (Vector, Burlingame, Calif.) for 3 h. After rinsing,the sections were incubated with horseradish peroxidase-streptavidinand then reacted by using a purple chromagen kit (VIP; Vector),mounted, dried, dehydrated, and coverslipped.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Tat is required to produce a vector of efficient transducing activity. To investigate the role of Tat in the production of transducing particles, expression from lentivirus vectors was first examinedby Northern analysis (Fig. 1). The patterns of RNAs induced bytransfer vectors in which the transgene was driven by an internalPGK, CMV, or retrovirus MFG promoter were studied in both producerand target cells. In transfected 293T cells, expression occurredmainly from the internal promoter. When a packaging constructexpressing both Tat and Rev was cotransfected, a dramatic enhancementof transcription from the LTR was observed, with an accumulationof unspliced vector RNA. In cells transduced with the vectors,that is, in the absence of Tat and Rev, transcription from theLTR was almost completely suppressed, the residual transcriptsunderwent splicing, and the internal promoter was responsiblefor most of the expression.

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FIG. 1. Northern analysis of the RNA expression from lentivirus vectors. Three pHR2 vectors carrying an expression cassette for the same transgene (truncated low-affinity NGFR) and driven by three different promoters (PGK, CMV, and retroviral MFG) were analyzed in producer and transduced cells. Total RNA was extracted and analyzed by Northern blotting with a probe specific for the transgene sequence. (A) Schematic of the vector construct depicts the species of RNA driven by the internal promoter (Prom.; broken arrow, shorter transcript) and the viral LTR (solid arrows, longer transcripts; the two species differ for the splicing of the viral intron). The splice donor and acceptor sites (SD and SA), the packaging sequence ( $Psi$ ), the truncated gag sequence (GA), and the RRE are indicated. (B) The vector constructs were transfected in 293T cells without or with the packaging construct. (C) Vector particles produced by the 293T transfectants were used to transduce HeLa cells. In the absence of the viral transactivators, supplied by the core packaging construct only in the producer cells, vector expression occurs mainly from the internal promoter. Note the dramatic enhancement of the upstream transcription and the accumulation of unspliced RNA (carrying the $Psi$ sequence) in the presence of the packaging construct. In the transduced cells, the LTR is silenced. Note that the three expression cassettes differ in the size of the promoters and 5' untranslated sequence. In each case, the smallest RNA species represents transcripts initiated from the internal promoter, while the intermediate-size and larger species correspond to spliced and unspliced LTR-driven RNAs, respectively.

A packaging plasmid carrying two mutations in tat (pCMV $Delta$ R8.93) was then constructed. The first mutation is a deletion of theT in the ATG initiation codon of the tat gene; the second is aninsertion of a MluI linker producing a translation stop codonafter residue 46 of the Tat protein. These changes confer a tat-defectivephenotype to HIV-1 (12). After transfection of the control ortat-defective packaging constructs into 293T cells, comparableyields of vector particles were recovered in the culture medium,as assayed by using the Gag p24 antigen (see Table 3). Such Tatindependence was expected from the replacement of the HIV LTRby the constitutive CMV promoter in the packaging construct. However,the particles produced in the absence of Tat had a dramaticallyreduced transducing activity (Table 1): 5 to 15% of that of particlesproduced by the control Tat-positive packaging construct.

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TABLE 1. Transducing activities of lentivirus vectors made with and without a functional tat gene in the packaging construct^a

We also tested whether the Tat-defective phenotype could be rescued by complementation in target cells (Table 1). HeLa-tatcells, a cell line expressing Tat from the HIV-1 LTR (13), weretransduced by vectors produced with or without Tat. The expressionof Tat in target cells did not compensate for the loss in transductionefficiency of vector produced without Tat.

As expected from the Northern analysis, functional inactivation of the tat gene resulted in a lower abundance of vector RNAin producer cells. This was indicated by the decrease in luciferaseactivity in cells producing a luciferase vector without an internalpromoter. In this case, transgene expression directly reflectsthe abundance of transcripts originating from the LTR. 293T cellsproducing luciferase vectors without Tat had only 5% of the luciferasecontent of cells producing the same vector with Tat ([1.0 ± 0.2]× 10⁹ relative light units [RLU]/dish without Tat; [20.2 ± 0.7] × 10⁹ RLU/dish with Tat). This ratio corresponded very closely to thatobserved in cells transduced by either type of vector in the courseof the same experiment (Table 1), suggesting that the abundanceof vector RNA in producer cells is a rate-limiting factor in thetransduction by lentivirus vectors.

One could thus conclude that Tat is required in producer cells to activate transcription from the HIV LTR and to generatevector particles with a high transducing activity.

The tat requirement is offset by placing a constitutive promoter upstream of the transfer vector. If the only function of Tat is trans activation of vector transcription from the LTR, the tat-defective phenotype should berescued by placing a strong constitutive promoter upstream ofthe vector transcript. Three transcriptional domains have beenidentified in the HIV promoter in the U3 region of the LTR: thecore or basal domain, the enhancer, and the modulatory domain(27). Transcription starts at the U3/R boundary, the first nucleotideof R being numbered 1. The core promoter contains binding sitesfor the TATA-binding protein ( $-$ 28 to $-$ 24) and SP-1 (three bindingsites between $-$ 78 to $-$ 45). The enhancer contains two binding sitesfor NF- $kappa$ B which overlap with a binding site for NFATc ( $-$ 104 to $-$ 81). The modulatory domain contain binding sites for severalcellular factors, including AP-1 ( $-$ 350 to $-$ 293), NFAT-1 ( $-$ 256to $-$ 218), USF-1 ( $-$ 166 to $-$ 161), Ets-1 ( $-$ 149 to $-$ 141), and LEF( $-$ 136 to $-$ 125). A panel of 5' chimeric transfer constructs carryingsubstitutions of either all or part of the U3 region of the 5'LTR was generated. All substitutions were made to preserve thetranscription initiation site of HIV. Partial substitutions joinednew enhancer sequences to the core promoter of the HIV LTR ( $-$ 78to 1), while full substitutions replaced also the promoter. pRLLand pRRL vectors carried the enhancer and the enhancer/promoter,respectively, of RSV; pCLL and pCCL vectors carried the enhancerand the enhancer/promoter of human CMV.

Control pHR2 and 5' chimeric transfer constructs carrying a PGK-eGFP expression cassette were tested by transfection of 293Tcells with control or tat-defective packaging constructs, andthe expression of the eGFP transgene was analyzed by fluorescence-activatedcell sorting (FACS). The RRL chimeric construct yielded a higherlevel of eGFP expression than the pHR2 vector, reflecting theconstitutive transcriptional activity of the new sequence (Fig.2A). Interestingly, the chimeric vector also displayed upregulationby Tat, as shown by the increased eGFP expression of cells cotransfectedwith the control packaging construct. Tat upregulation was provento be a direct effect by transfecting a pRRL-eGFP vector lackingan internal promoter with control or tat-defective packaging constructsand analyzing GFP expression by FACS (Fig. 2B). Comparable resultswere obtained with the other chimeric LTR vectors (not illustrated).Vector particles were then collected from the transfected producercells and assayed for transduction of eGFP into HeLa cells andhuman primary lymphocytes (peripheral blood lymphocytes [PBL]).As shown in Table 2, all vectors had efficient transducing activity,as assessed by endpoint titration on HeLa cells or maximal transductionfrequency of PBL. The vector produced by the pRRL chimera wasas efficient as that produced by the pHR2 construct and was selectedto test transduction independent of Tat. As shown in Table 3,the pRRL construct yielded a vector of only slightly reduced transducingactivity (60%) when the packaging construct was tat defective.The residual effect of Tat on transduction was in agreement withthe ability of Tat to upregulate transcription from the chimericLTR.

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FIG. 2. Transcriptional activities of wild-type and 5' chimeric vector constructs in the absence and presence of Tat. (A) Control pHR2 and the 5' chimeric pRRL transfer construct carrying a PGK-eGFP expression cassette were transfected into 293T cells with a packaging construct having a functional (pCMV $Delta$ R8.91; grey line) or inactive (pCMV $Delta$ R8.93; black line) tat gene. GFP expression was analyzed by FACS. The filled area represents nontransfected cells. In the absence of Tat, the chimeric construct yielded a level of GFP expression higher than that achieved by the pHR2 construct. Both constructs were further upregulated by Tat. (B) A pRRL construct carrying the eGFP gene without an internal promoter was transfected with a packaging construct carrying a functional (grey line, open area) or inactive (black line, open area) tat gene. Direct upregulation of the chimeric promoter by Tat was observed. The filled area represents nontransfected cells.

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TABLE 2. GFP transduction by lentivirus vectors made by transfer constructs with a wild-type or 5' chimeric LTR

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TABLE 3. GFP transduction into HeLa cells by lentivirus vectors made by transfer constructs with a wild-type or 5' chimeric LTR and packaging constructs with or without a functional tat gene^a

The use of the chimeric LTR construct allowed removal of Tat from the packaging system with a minimal loss in the transductionefficiency of the vector in vitro. To test vector performancein the more challenging setting of in vivo delivery into brainneurons, high-titer vector stocks were generated from the pHR2and pRRL constructs with and without Tat. The four stocks of eGFPvector were matched for particle content by p24 antigen and injectedbilaterally in the neostriata of groups of three adult rats. Theanimals were sacrificed after 1 month, and serial sections ofthe brain were analyzed for eGFP fluorescence (not shown) andimmunostained by antibodies against eGFP (Fig. 3). The resultsobtained in vivo matched the in vitro data. Vector produced bythe pHR2 construct only achieved significant transduction of theneurons when packaged in the presence of Tat. Vector producedby the pRRL chimera was as efficient when made with or withoutTat. The transduction extended throughout most of the striatumand reached a very high density of positive cells in the sectionsclosest to the injection site. No signs of pathology were detectablein the injected tissue, except for a small linear scar markingthe needle track, by hematoxylin and eosin staining of the sections(data not shown).

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FIG. 3. In vivo transduction of eGFP into brain cells by lentivirus vectors produced with and without Tat. Vectors carrying a PGK-eGFP expression cassette were produced by the pHR2 (A and B) or the 5' chimeric pRRL (C and D) transfer construct and a packaging construct with (pCMV $Delta$ R8.91; A and C) or without (pCMV $Delta$ R8.93; B and D) a functional tat gene, concentrated by ultracentrifugation, and normalized for particle content prior to injection into the corpora striata of adult rats. One month after injection, brain sections were stained for immunoreactivity to the GFP protein. While both types of vectors transduced neurons very efficiently when made with Tat, only the vector made by the chimeric transfer construct worked as well when produced without Tat. Representative sections close to the injection site are shown for one of six striata injected per each type of vector. The bar in panel B represents 1 mm; that in the inset in panel A represents 100 µm.

These results provide evidence that Tat is dispensable for efficient transduction by a lentivirus vector.

A new split-genome conditional packaging system. The possibility of deleting the tat gene prompted us to explore a new design of the packaging component of the HIV vectorsystem, in which two separate nonoverlapping expression plasmids,one for the gag and pol genes and the other for the rev gene,were used. The gag and pol reading frames were expressed withinthe context of the MD cassette, which employs the CMV promoterand intervening sequence and the human $beta$ -globin poly(A) site (34).All HIV sequences upstream of the gag initiation codon were removed,and the leader was modified for optimal fit to the Kozak consensusfor translation. This construct, however, expressed almost nop24 antigen when transfected alone in 293T cells. This observationis in agreement with the previously reported presence of cis-repressiveor inhibitory sequences in the gag and pol genes (40, 41).The HIV RRE was then inserted downstream of the pol gene, andthe resulting plasmid was cotransfected with a rev expressionvector (Table 4). High levels of p24 antigen production wereobserved in this case, the highest yields being obtained whenrev was driven by an RSV promoter. When the gag-pol and the revconstructs were cotransfected with the pRRL chimeric transfervector and the VSV G-expressing plasmid, high-titer vector wasobtained in the culture medium. Both the yield of particles andtheir transducing efficiency were similar to those obtained withprevious versions of the system. Northern analysis of producercells confirmed that unspliced vector genomic RNA accumulatedonly in the presence of Rev (data not shown). Thus, both the expressionof the gag and pol genes and the accumulation of packageable vectortranscripts are dependent on trans complementation by a separateRev expression construct. Such a conditional packaging systemprovides an important safety feature unavailable to oncoretrovirusvectors.

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TABLE 4. GFP transduction into HeLa cells by lentivirus vectors made by linked or split packaging constructs and a pRRL transfer construct^a

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The predicted biosafety of a viral vector depends in part on how much segregation of the cis- and trans-acting functions ofthe viral genome is achieved by the vector design and is maintainedduring vector production. A vector particle is assembled by viralproteins expressed in the producer cell from a construct(s) strippedof the cis-acting sequences required for the transfer of the viralgenome to target cells (packaging construct). These cis-actingsequences are instead linked to the transgene in the transfervector. As the vector particle packages only the genetic informationcontained in this latter construct, the infection process is limitedto a single round without spreading. Through recombination, itis possible that sequences encoding viral proteins rejoin thecis-acting elements of the transfer vector. If the resulting recombinantexpresses all required functions, it is able to replicate (i.e.,it is a replication-competent retrovirus [RCR]) and presents arisk to the recipient. The formation of heterozygous vector particlescontaining RNAs from both the packaging and transfer vectors,followed by homologous recombination during reverse transcription,is the mechanism most often incriminated in the emergence of RCRduring the production of retroviral vectors. The likelihood ofthis type of recombination is dependent on residual cis-actingsequences in the packaging plasmid, allowing some level of encapsidation,and on the extent of homology between packaging and vector constructs(10).

A first strategy to improve the biosafety of a vector is to use nonoverlapping split-genome packaging constructs that requiremultiple recombination events with the transfer vector for RCRgeneration. Earlier studies described several approaches to generatereplication-defective HIV vectors (7, 35, 38, 42). However,these vectors could be produced only to low infectious titers,were restricted to CD4-positive cellular targets, and carriedthe risk of generating wild-type HIV by recombination of the components.A major advance was achieved when an improved vector design wascombined with the use of the envelope of another virus (32,33, 39). The lentivirus vector that we describe here is packagedby three nonoverlapping expression constructs, two expressingHIV proteins and the other expressing the envelope of a differentvirus. Moreover, all HIV sequences known to be required for encapsidationand reverse transcription (2, 22, 24, 27, 29, 30,35) are absent from these constructs, with the exception ofthe portion of the gag gene that contributes to the stem-loopstructure of the HIV-1 packaging motif (29).

A second strategy to improve vector biosafety took advantage of the complexity of the lentivirus genome. The minimal set ofHIV-1 genes required to generate an efficient vector was identified,and all other HIV reading frames were eliminated from the system.As the products of the removed genes are important for the completionof the virus life cycle and for pathogenesis, no recombinant canacquire the pathogenetic features of the parental virus. We previouslydemonstrated that all four accessory genes of HIV could be deletedfrom the packaging construct without compromising gene transduction(51). In this work, we went further by deleting another factorcrucial for HIV replication, the tat gene. Its product is oneof the most powerful transcriptional activators known and playsa pivotal role in the exceedingly high replication rates thatcharacterize HIV-induced disease (18, 19, 47).

It was found that Tat was required in producer cells to generate vector of efficient transducing activity but that this requirementwas offset by inducing constitutive high-level expression of vectorRNA. Due to the low basal transcription from the HIV LTR, Tatwas necessary to increase the abundance of vector transcriptsand allow their efficient encapsidation by the vector particles.When made in the absence of Tat, vector particles had 10- to 20-fold-reducedtransducing activity. However, when strong constitutive promotersreplaced the HIV sequence in the 5' LTR of the transfer construct,vectors made without Tat exhibited a less than twofold reductionin transducing activity. As Tat strongly upregulated transcriptionfrom the chimeric LTR, the transducing activity of the outputparticles must reach saturation. The abundance of vector RNA inproducer cells thus appears to be a rate-limiting factor for transductionuntil it reaches a threshold. Conceivably, an upper limit is setby the total output of particles available to encapsidate vectorRNA. As the total particle output varied with the types of vectorand internal promoter used, this may explain the quantitativedifferences obtained in response to tat deletion.

Successful deletion of the tat gene was unexpected in view of a reported additional role for Tat in reverse transcription(17, 20). While the reasons for this discrepancy are not obvious,it should be noted that the transduction pathway of the lentivirusvector mimics only in part the infection pathway of HIV. The vectoris pseudotyped by the envelope of an unrelated virus and containsonly the core proteins of HIV, without any accessory gene product.The VSV envelope targets the vector to the endocytic pathway,and it has been shown that redirection of HIV-1 from its normalroute of entry by fusion at the plasma membrane significantlychanges the biology of the infection. For example, Nef and cyclophilinA are required for the optimal infectivity of wild-type HIV-1but not of a (VSV G) HIV pseudotype (1). It is also possiblethat the kinetics of reverse transcription are more critical forthe establishment of viral infection than for gene transduction,given the differences in size and sequence between the virus andvector genome.

Tat-independent transduction by an HIV-based vector was recently reported by Kim et al. for in vitro cellular targets (23).In the vector designed by these authors, however, Tat and Revwere expressed from the transfer vector and thus were also presentin target cells. A CMV-HIV hybrid LTR was used; this constructyielded vector titers approximately 30% of that obtained withan intact LTR. When the tat gene was inactivated, the titer didnot change. Srinivasakumar et al. (43) previously reported arather low (5- to 10-fold) dependence on Tat of an HIV-based vectorproduced by cells stably expressing the HIV structural proteins.In this case, titers of 5 × 10³ TU/ml with Tat and 7 × 10² TU/ml without Tat were obtained on HeLa-CD4 cells. Although thesetiters are much lower than those reported here, the vector particlescarried the HIV envelope, an indication that Tat is not absolutelyrequired for transduction by vector particles which in that casemirror more closely the wild-type virus. It remained possible,however, that a dependence on Tat may be revealed in more challenginggene deliveries into the body tissues that are the actual targetsof gene therapy. This could have been due to a stricter Tat requirementfor optimal transduction efficiency or for the production of high-titervector stocks or to differences in cell-type-specific factors.Our results now establish that Tat is fully dispensable for lentivirusvector transduction even when high titers are achieved and, mostimportantly, for gene delivery in vivo into terminally differentiatedneurons of an adult rat brain.

The Northern analysis of producer and target cells shows that the Tat dependence of LTR-driven expression restricts the productionof vector genomic RNA to producer cells. This applies as wellto vectors made by the 5' chimeric constructs, as the U3 sequencesof both LTRs of the resulting provirus are derived from the vector3' LTR. However, the functional replacement of the tat gene inthe packaging construct by promoter sequences upstream of thetransfer construct makes the generation of a transcriptionallyactive recombinant much more unlikely. This will be even moresignificant in stable producer cell lines that avoid the riskof plasmid recombination during cotransfection.

We also exploited the Rev dependence of gag-pol expression and of the accumulation of unspliced, packageable transcripts.Yu et al. (50) previously showed that the dependence on Revcan be used to make expression of HIV genes inducible. We describea core packaging system split in two separate nonoverlapping expressionconstructs, one for the gag and pol reading frames optimized forRev-dependent expression and the other for the rev cDNA. Thisthird-generation packaging system matches the performance of itspredecessors in terms of both yield and transducing efficiency.However, it increases significantly the predicted biosafety ofthe vector. It has been suggested that the Rev-RRE axis couldbe replaced by the use of constitutive RNA transport elementsof other viruses, although at the price of decreased efficiency(11, 23, 43). We would suggest that maintaining the Revdependence of the system allows for an additional level of biosafetythrough the splitting of the HIV-derived components of the packagingsystem.

The conditional packaging system described here can be combined with a self-inactivating vector construct carrying a majordeletion in the 3' LTR (52). This vector design (Fig. 4) offerssignificant biosafety features. The contribution of HIV is reducedto a fraction of cis-acting sequences in the vector, leaving outin particular most of the LTR, and to only three genes, gag, pol,and rev, in the packaging constructs, compared with the nine genesnecessary for the in vivo replication and pathogenesis of wild-typeHIV-1 (3, 18, 27, 49). The actual biosafety of a vectormust be proven in vivo. However, given the serious limitationsof the available animal models of HIV-induced disease, the biosafetyof HIV-derived vectors will ultimately be proven only in humanhosts. Therefore, the vector design must ensure the highest predictablebiosafety for clinical testing to be acceptable.

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FIG. 4. Schematic drawing of the HIV provirus and the four constructs used to make a lentivirus vector of the third generation. The viral LTRs, the reading frames of the viral genes, the major 5' splice donor site (SD), the packaging sequence ( $Psi$ ), and the RRE are boxed and indicated in bold type. The conditional packaging construct, pMDLg/pRRE, expresses the gag and pol genes from the CMV promoter and intervening sequences and polyadenylation site of the human $beta$ -globin gene. As the transcripts of the gag and pol genes contain cis-repressive sequences, they are expressed only if Rev promotes their nuclear export by binding to the RRE. All tat and rev exons have been deleted, and the viral sequences upstream of the gag gene have been replaced. A nonoverlapping construct, RSV-Rev, expresses the rev cDNA. The transfer construct, pRRL.SIN-18, contains HIV-1 cis-acting sequences and an expression cassette for the transgene. It is the only portion transferred to the target cells and does not contain wild-type copies of the HIV LTR. The 5' LTR is chimeric, with the enhancer/promoter of RSV replacing the U3 region (RRL) to rescue the transcriptional dependence on Tat. The 3' LTR has an almost complete deletion of the U3 region, which includes the TATA box (from nucleotides $-$ 418 to $-$ 18 relative to the U3/R border). As the latter is the template used to generate both copies of the LTR in the integrated provirus, transduction of this vector results in transcriptional inactivation of both LTRs; thus, it is a self-inactivating vector (SIN-18). The fourth construct, pMD.G, encodes a heterologous envelope to pseudotype the vector, here shown coding for VSV G. Only the relevant parts of the constructs are shown.

It is noteworthy that the fraction of the HIV-1 genome that is left in the vector is probably smaller than could be achievedwith any of the nonprimate lentiviruses, the genomic complexityof which is lower than that of HIV-1 (37). Also, the risks associatedwith the introduction in humans of a recombinant arising froma nonprimate lentivirus, even in a form that in its cognate animalspecies appears to be attenuated, are very difficult to assess,as illustrated by the ongoing debate on xenotransplantation (48).In contrast, the almost two decades spent studying a virus thathas now spread in tens of millions of people worldwide have revealeda considerable amount of information on the pathogenic featuresof HIV-1, in particular on the dependence of virulence on a crucialset of viral genes. Based on these data, we would like to suggestthat the HIV-based vectors described here are good candidatesfor the clinical trial of lentivirus vectors in human gene therapy.

	ACKNOWLEDGMENTS

We are indebted to Tom Hope for providing the Rev expression plasmids, to Melinda Van Roey and Heidi Oline for help with theanimal experiments, and to Jennifer Davis and Mitch Finer forsuggestions and critical reading of the manuscript.

This work was partly supported by a grant and by a fellowship from the Swiss National Science Foundation to D.T. and R.Z.,respectively.

	FOOTNOTES

^* Corresponding author. Mailing address: Cell Genesys, 342 Lakeside Dr., Foster City, CA 94404. Phone: (650) 425-4474. Fax:(650) 358-8636. E-mail: luigin{at}cellgenesys.com.

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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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