Woodchuck Hepatitis Virus Posttranscriptional Regulatory Element Enhances Expression of Transgenes Delivered by Retroviral Vectors

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Journal of Virology, April 1999, p. 2886-2892, Vol. 73, No. 4
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Woodchuck Hepatitis Virus Posttranscriptional Regulatory Element Enhances Expression of Transgenes Delivered by Retroviral Vectors

Romain Zufferey,¹ John E. Donello,² Didier Trono,¹^,^* and Thomas J. Hope²^,^*

Department of Genetics and Microbiology, University of Geneva Medical School, CH-120 Geneva, Switzerland,¹ and Infectious Disease Laboratory, The Salk Institute for Biological Studies, La Jolla, California 92037²

Received 21 September 1998/Accepted 15 December 1998

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The expression of genes delivered by retroviral vectors is often inefficient, a potential obstacle for their widespread usein human gene therapy. Here, we explored the possibility thatthe posttranscriptional regulatory element of woodchuck hepatitisvirus (WPRE) might help resolve this problem. Insertion of theWPRE in the 3' untranslated region of coding sequences carriedby either oncoretroviral or lentiviral vectors substantially increasedtheir levels of expression in a transgene-, promoter- and vector-independentmanner. The WPRE thus increased either luciferase or green fluorescentprotein production five- to eightfold, and effects of a comparablemagnitude were observed with either the immediate-early cytomegalovirusor the herpesvirus thymidine kinase promoter and with both humanimmunodeficiency virus- and murine leukemia virus-based vectors.The WPRE exerted this influence only when placed in the senseorientation, consistent with its predicted posttranscriptionalmechanism of action. These results demonstrate that the WPRE significantlyimproves the performance of retroviral vectors and emphasize thatposttranscriptional regulation of gene expression should be takeninto account in the design of gene deliverysystems.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Retroviral vectors offer several characteristics of great value for a gene delivery system, including a large packaging capacity,an efficient integration machinery, and the absence of a vector-inducedcellular immune response. However, one shortcoming of retroviralvectors, whether based on oncoretroviruses or lentiviruses, istheir frequent inability to generate high levels of gene expression,particularly in vivo. Epigenetic phenomena, such as position effectsor silencing by DNA methylation, may partly account for thislimitation.

Many steps, both transcriptional and posttranscriptional, are involved in the regulation of gene expression. Therefore, itmay be possible to improve the expression of transgenes deliveredby retroviral vectors through the addition of elements known toincrease gene expression posttranscriptionally. The best knownexample of stimulation at this level is the inclusion of an intronwithin the expression cassette. Many gene transfer experiments,performed both in vitro and in vivo, have demonstrated that thepresence of an intron can facilitate gene expression (4). Inextreme cases, such as $beta$ -globin, expression is intron dependent.Expressed $beta$ -globin cDNAs are unstable in the nucleus and neveraccumulate in the cytoplasm. However, the addition of an introncauses the cytoplasmic accumulation of $beta$ -globin mRNA (2). Severalmechanisms can be responsible for this effect. Some introns havebeen found to contain regulatory sequences that enhance transcriptionor 3'-end processing (1, 5, 12, 22). More generally,however, splicing per se appears to stimulate gene expression,perhaps in part by promoting the nuclear stability, proper processing,and/or cytoplasmic localization of mRNAs (25).

This evidence has prompted the development of strategies to incorporate introns into retroviral vectors. This task is difficult,because retroviral genomic RNA is normally produced in the nucleusby the cellular transcriptional machinery and as such is exposedto the splicing machinery. To circumvent this difficulty, intron-containingtransgenes can be placed in an orientation opposite that of thevector genomic transcript (27). Unfortunately, this approachis complicated by the possibility of antisense effects. Alternatively,intron-containing retroviral vector genomic RNAs can be producedin the cytoplasm, for instance, through the use of an alphavirusvector (16). It remains to be seen whether the latter techniquewill gain broad acceptance for the production of clinical-graderetroviralvectors.

Other types of elements can also be used to stimulate $beta$ -globin cDNA expression posttranscriptionally. These elements havethe advantage of not requiring splicing events, thereby avoidingremoval during the viral life cycle. For instance, elements derivedfrom intronless viral messages can stimulate the cytoplasmic accumulationof $beta$ -globin cDNA transcripts. These include the posttranscriptionalprocessing element present within the thymidine kinase gene ofherpes simplex virus (17) and the posttranscriptional regulatoryelement (PRE) present in hepatitis B virus (HBV) (14).

Previous studies have suggested that the HBV PRE (HPRE) and an intron are functionally equivalent. This model was a consequenceof the observation that the HPRE and $beta$ -globin intron II were interchangeable. $beta$ -Globin intron II could stimulate the expression of the HBV surfaceprotein, which is normally HPRE dependent, while the HPRE couldstimulate the expression of a $beta$ -globin cDNA (14). The proposedmechanism of HPRE function is the facilitation of the nuclearexport of PRE-containing transcripts (11, 13). Supportingthis model is evidence that the HPRE can functionally substitutefor the human immunodeficiency virus (HIV) type 1 (HIV-1) Rev-Rev-responsiveelement complex in a transient transfection reporter assay (7,13). Woodchuck hepatitis virus (WHV), a close relative of HBV,also harbors a PRE (WPRE) (8). We have previously shown thatthe WPRE is significantly more active than its HBV counterpart;the increased activity correlates with the presence of an additionalcis-acting sequence in the WPRE which is not found in the HPRE(8).

Because of the increased efficiency of this element, we examined whether the WPRE could stimulate the expression of intronlesstransgenes delivered by retroviral vectors. We found that theinsertion of this sequence in HIV-derived vectors resulted ina significant stimulation of expression of the reporter genesfor luciferase and green fluorescent protein (GFP) in a varietyof cells of human and rodent origins. Stimulation was irrespectiveof the cycling status of transduced cells. The WPRE effect wasnot promoter dependent and was also revealed within the contextof murine leukemia virus (MLV)-derived vectors. Interestingly,the WPRE acted on both intronless and spliced mRNAs, revealingthat the functions of the WPRE and splicing in gene expressionare not redundant. These data suggest that the inclusion of theWPRE in retroviral vectors will result in a significant improvementin their performance for gene therapy. Further, the WPRE may bea useful tool for stimulating gene expression in other vectorcontexts.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmids. (i) HIV-1 vector plasmids. Plasmids pHR'CMV-GFP and pHRCMV-Luc have been described previously (29). A PCR-amplified WPRE cassette (nucleotides 1093to 1684; GenBank accession no. J04514) was modified with ClaIor EcoRI ends and inserted into pHR'CMV-GFP either at the uniqueClaI site upstream of the cytomegalovirus (CMV) promoter or atthe unique EcoRI site downstream of the GFP stop codon, resultingin plasmids pHR'W-CMV-GFP and pHR'CMV-GFP-W, respectively. Subsequently,the BamHI-XhoI GFP coding sequence was replaced with a BamHI-XhoIluciferase coding sequence to generate pHR'CMV-Luc-W. PlasmidspMD.G and pCMV $Delta$ R8.91 have been described previously (29).

(ii) MLV vector plasmids. WPRE was inserted as a ClaI cassette into the unique ClaI site of plasmid pCLNCX (21). Subsequently, a BamHI-HindIII thymidinekinase (TK)-luciferase cassette was substituted for the CMV promoter,resulting in plasmid pCLNTluc-W. The ClaI WPRE cassette was deletedto generate control plasmidpCLNTluc.

Tissue culture and transfection. Dulbecco's modified Eagle's medium (Gibco) was supplemented with 10% fetal calf serum (Gibco), a combination of penicillinand streptomycin (Gibco), and glutamine (Gibco). 293T, HeLa, HeLa-tat,HOS, 208F, and NIH 3T3 cells were cultured in supplemented Dulbecco'smodified Eagle's medium in a 10% CO₂ atmosphere. Gamma irradiationwas delivered by a 3-min exposure to a ⁶⁰CO source. Vector stocks were prepared and cells were transducedas previously described (29).

To determine the titers of GFP-transducing vectors, five serial 1:2 dilutions of each filtered vector stock were used to transduceHeLa cells in six-well plates (2 × 10⁵ cells/well). The highest and lowest inocula corresponded to 100ml and 6.25 ml of undiluted supernatant, respectively. Vectorparticles were added to 2 ml of culture medium in the absenceof Polybrene and left on the cells for 48 to 60 h. At this time,the percentage of GFP-positive cells was determined with a fluorescence-activatedcell sorter on a Beckton Dickinson FACScan. To calculate titers(transducing units per milliliter), 2 × 10⁵ cells/well was multiplied by the percentage of GFP-positive cells,and this product was divided by the number of microliters in theinoculum. Numerous titer determinations have shown that the percentageof transduced cells correlates linearly with the vector inputwhen the percentage is lower than 12%. Therefore, all titers werebased on at least two values lower than 12% and showing the expectedlinearity.

Southern analysis. Genomic DNA was isolated from three 10-cm plates of each cell line. Cells were lysed, phenol extracted, and ethanol precipitatedby standard methods. Ten micrograms of genomic DNA was digestedovernight with BamHI, EcoRI, and XhoI restriction enzymes. DigestedDNA was ethanol precipitated and electrophoresed on a 0.9% agarosegel. DNA was visualized with ethidium bromide staining beforebeing transferred to a nylon membrane by standardmethods.

RNA isolation and analysis. Cells were washed with phosphate-buffered saline (PBS) and pelleted by centrifugation. For total RNA, the cell pellet wasresuspended in 250 µl of PBS, and 750 µl of RNA Stat LS-50 (Tel-Test)was added. For nuclear and cytoplasmic fractionation, cells wereresuspended in cytoplasmic lysis buffer (10 mM HEPES [pH 7.8],10 mM KCl, 0.1 mM EDTA, 20% glycerol, 0.5% Nonidet P-40). Thelysed cells were spun for 3 min at 8,000 × g, and the supernatantwas recovered and spun for an additional 5 min at 14,000 × g.The supernatant was transferred to 1 ml of RNA Stat LS-50. Thenuclear pellet from the first spin was resuspended in 1 ml ofcytoplasmic lysis buffer and then spun at 8,000 × g for 3 min.The supernatant was discarded, and the pellet was resuspendedin 800 µl of nuclear buffer (10 mM Tris [pH 8.4], 1.5 mM MgCl₂,140 mM NaCl, 20% glycerol). The sample was spun at 8,000 × g,and the supernatant was discarded. The pellet was resuspendedin 300 µl of nuclear buffer and lysed with 1 ml of RNA Stat LS-50.The RNA Stat LS-50 protocol wasfollowed.

For RNA half-life analysis, cells were grown to 70% confluency and treated with 5 mg of actinomycin D per ml. For each timepoint, two plates of cells were harvested. The cells were pelletedand resuspended in 250 µl of PBS, and 750 µl of RNA Stat LS-50was added. After RNA purification, the samples were treated withDNase for 15 min at 37°C. Five micrograms of nuclear RNA and 10µg of cytoplasmic RNA were separated on a 1% agarose-formaldehydegel, transferred to a nylon membrane, and hybridized with a GFPprobe by use of Quickhyb (Qiagen) and the manufacturer'sprotocol.

Nuclear run-on assays. For each experiment, 5 × 10⁷ cells were harvested. The nuclei were prepared by lysing the cells in cell lysis buffer (10 mMTris [pH 8.3], 10 mM NaCl, 5 mM MgCl₂). The nuclei were washedonce in cell lysis buffer and frozen overnight. The run-on reactionswere performed with 25 mM Tris (pH 8.0)-12.5 mM MgCl₂-750 mM KCl-1.25mM each ATP, CTP, and GTP-30 µl of UTP (800 Ci/mmol). The reactionmixtures were incubated for 30 min at 30°C. The nuclei were homogenizedin 750 µl of RNA Stat LS-50 (Tel-Test). The labeled RNA was purifiedin accordance with the manufacturer's specifications. The RNAsamples were treated with DNase, phenol extracted, and centrifugedthrough G-25 columns. The samples were ethanol precipitated andresuspended, and counts were determined with a scintillation counter.Equivalent counts were hybridized with nitrocellulose filterscontaining plasmid DNAs for histone H2B and glyceraldehyde-3-phosphatedehydrogenase (GAPDH) and PCR products derived from vector sequencesby use of Quickhyb and the manufacturer's protocol. Hybridizedfilters were treated with RNase A andanalyzed.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

WPRE enhances the expression of transgenes delivered by HIV-based vectors. To test whether the WPRE enhances the expression of intronless reporter genes delivered by HIV-based vectors, a 600-nucleotide-longcassette containing the WPRE sequence was cloned into the previouslydescribed plasmids pHR'CMV-Luc and pHR'CMV-GFP (29). The WPREwas inserted in the 3' untranslated region (UTR) of the reportergenes between the stop codon and the polypurine tract (Fig. 1A).To produce vesicular stomatitis virus G protein (VSV-G)-pseudotypedtransducing particles, vector plasmids with or without the WPREwere cotransfected into 293T cells with the envelope plasmid pMD.Gand the packaging plasmid pCMV $Delta$ R8.91 by a published protocol (20).The resulting vectors were used to transduce in parallel differentcell lines. These experiments were done at a multiplicity of infection(MOI) of 0.1 to favor a single integration per cell. Dilutionanalysis of the vector stocks on 293T cells showed that the WPREdid not influence titers (data not shown). However, fluorescence-activatedcell sorter quantification of GFP expression in cells transducedwith HR'CMV-GFP or HR'CMV-GFP-W demonstrated that the presenceof the WPRE in the transgene 3' UTR (indicated by the suffix Win the plasmid name) increased the mean expression of the transducedpopulation by at least fivefold in 293T cells (Fig. 2A) and threefoldin HeLa cells (Fig. 2B). In contrast, the WPRE inserted in theopposite orientation (indicated by the suffix W(as) in the plasmidname) inhibited GFP expression in HeLa cells (Fig. 2C). Therefore,WPRE function is orientation dependent, as has been reported previously(8).

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FIG. 1. Schematic drawing of the vector constructs used in this study. (A) HIV-1-based vector constructs containing an internal CMV promoter driving transgene expression. (B) HIV-1-based vector constructs in which transgene expression is driven by the HIV LTR promoter. The transgene is expressed from a spliced message. (C) MLV constructs containing an internal herpes simplex virus TK promoter (Tk) driving the expression of luciferase. The WPRE is shown as a black box. W(as) designates the WPRE inserted in the antisense orientation. Orientation is designated by arrows. SD, splice donor; SA, splice acceptor; RRE, Rev-responsive element; R, repeat region.

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FIG. 2. WPRE enhances gene expression in cells transduced with HIV-based vectors. 293T (A) or HeLa (B) cells were transduced in parallel with HR'CMV-GFP or HR'CMV-GFP-W stocks matched for p24. Viral stocks were transduced at an MOI of 0.1 to 0.2. At 48 h postinfection, GFP expression was compared to that in noninfected cells (shaded histogram), in cells transduced with HR'CMV-GFP (thin line), and in cells transduced with HR'CMV-GFP-W (thick line). Average GFP expression per cell was determined for transduced cells contained in the M1 region. Values for average expression in the population are shown, designated by lines corresponding to the lines used in the histograms. In both cell lines, GFP expression per cell was increased by the presence of the WPRE. (C) WPRE function is orientation specific. HeLa cells were transduced with HR'CMV-GFP-W or HR'CMV-GFP-W(as). (D) WPRE functions in cis. HeLa cells were transduced with HR'W-CMV-GFP or HR'CMV-GFP. Average GFP expression per cell was equivalent for these two derivatives. Data in panels C and D were derived from a single experiment allowing direct comparison of mean GFP intensity. (E) The WPRE can stimulate the expression of luciferase in a variety of cell lines. Results are shown as the ratio of luciferase expression with a vector containing WPRE versus a normal vector for each cell line. The presence of the WPRE increased luciferase expression five- to sevenfold in each cell line.

Further studies revealed that the WPRE had to be present within the transgene transcript to function. When the WPRE was insertedupstream of the CMV promoter governing the transcription of theGFP gene (Fig. 1A), it was unable to stimulate GFP expressionin HeLa cells (Fig. 2D). This result demonstrates that the WPREmust be present within a transcript to stimulate expression, consistentwith a posttranscriptional mode ofaction.

To exclude the possibility that the WPRE effect was gene specific, we tested the ability of the WPRE to stimulate luciferaseexpression. The luciferase activities induced in various targetcells by either HR'CMV-Luc or HR'CMV-Luc-W were compared. Viralstocks were normalized for the amounts of HIV-1 p24 capsid antigenpresent in the inoculum (Fig. 2E). The WPRE in the 3' UTR of theluciferase cDNA increased luciferase production by a factor of5 to 6 (mean, 5.27) in all cell lines tested (293T, HeLa, HOS,208F, and NIH 3T3). The WPRE is thus active in both human androdent cell lines and in cells of epithelial, osteoblastic, orfibroblasticorigin.

To explore if WPRE function is sensitive to the proliferation status of transduced cells, we analyzed the level of luciferaseexpression in dividing and gamma-irradiated 293T cells. Cellswere transduced with HIV-based luciferase vectors carrying theWPRE sequence in either the sense or the antisense orientation(Table 1). When a vector without the WPRE was used as a reference,the WPRE in the sense orientation resulted in a eightfold increasein luciferase expression in both dividing and arrested 293T cells.The WPRE in the antisense orientation was nonfunctional. Thisexperiment reveals that the proliferation status of the targetcells has no impact on WPRE function, an important feature forin vivo expression in terminally differentiated tissues.

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TABLE 1. Stimulation of transgene expression by the WPRE in arrested cells

WPRE enhances the expression of transgenes carried by MLV-based vectors. Since the WPRE is functional in settings as different as those of WHV and HIV-based vectors, it was considered likely thatit would also be functional when incorporated into a vector derivedfrom a simple retrovirus. To test this hypothesis, the WPRE wasinserted in the 3' UTR of the luciferase cDNA delivered by anMLV-based vector (21). Instead of the CMV promoter, the promoterfrom the human herpes simplex virus TK gene was chosen to demonstratethat WPRE action is not dependent on a particular promoter (Fig.1C). Stocks of VSV-G-pseudotyped MLV-based vectors were generatedby cotransfection of 293T cells with three plasmids, pMD.G, pCMVGagPol,and pCLNTluc or pCLNTluc-W, and used to transduce 293T cells.The induction of luciferase activity in these targets was measuredand normalized for the amount of reverse transcriptase activitypresent in the inoculum. The results revealed that the presenceof the WPRE increased the levels of expression of luciferase deliveredby MLV-based vector-mediated transduction more than fourfold (relativelight units with CLNTluc and CLNTluc-W [mean ± standard errorof the mean for triplicate batches of each vector in two independentexperiments], 139,518 ± 11,349 and 571,887 ± 7,319,respectively).

WPRE also acts on spliced mRNAs. In its natural context, the WPRE is located within intronless mRNAs. To test whether this element could facilitate the expressionof spliced mRNAs, the WPRE was inserted in HIV-based vectors expressingGFP or luciferase but devoid of the internal CMV promoter (Fig.1B). In these vectors, the reporter-encoding RNAs are producedby the 5' HIV long terminal repeat (LTR). Transgene expressionmeasured in this system is from the spliced message. It is notexpected that unspliced messages will substantially contributeto transgene expression because 10 ATG triplets present in theintron sequence may act as aberrant translational start sites.Since the HIV LTR is a weak promoter unless stimulated by theHIV Tat protein or the adenovirus early protein E1A, we used HeLa-tatand 293T cells as targets. As shown in Table 2, the WPRE enhancedluciferase expression in 293T cells eightfold. This level of stimulationby the WPRE is comparable to that observed for intronless mRNAs.In HeLa and HeLa-tat cells, the WPRE increased luciferase expressionby factors of 4 and 5, respectively. The similar levels of enhancementobserved in HeLa and HeLa-tat cells indicated that the WPRE iseffective over a wide range of promoter activities, since theLTR is 30 times more active in HeLa-tat cells than in HeLa cells.Comparable results were obtained with the GFP gene (data not shown).As noted for intronless transcripts, the action of the WPRE onspliced mRNAs was orientation dependent.

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TABLE 2. Expression of a transgene containing an intron is enhanced by the WPRE

Mechanism of WPRE action. It was previously established that HPRE and WPRE act at a posttranscriptional level (7, 11, 13). To explore the mechanismof WPRE action in a lentivirus context, 293T cells were transducedwith HR'CMV-GFP and HR'CMV-GFP-W at an MOI of 0.2. Fluorescentcells were sorted, expanded, and used for comparative DNA andRNA analyses (Fig. 3). Southern blot analysis demonstrated thatthe GFP transgene was present at comparable copy numbers in bothpopulations (Fig. 3A). Nuclear run-on analysis (Fig. 3B) demonstratedthat the WPRE did not influence the rate of transcription of vector-basedmessages. The observation that the WPRE does not function by stimulatingtranscription is consistent with previous reports indicating thatWHV does not have an enhancer within the WPRE (6, 8, 10,26).

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FIG. 3. DNA contents and transcription levels are not affected by the WPRE. 293T cells were transduced with HR'CMV-GFP and HR'CMV-GFP-W vectors at an MOI of 0.2. GFP-positive cells were sorted, expanded, and used for comparative DNA and RNA analyses. (A) Southern blot. Genomic DNA extracted from HR'CMV-GFP-transduced cells (lanes 1 and 3) or HR'CMV-GFP-W-transduced cells (lanes 2 and 4) were hybridized with a GFP-specific probe (lanes 1 and 2). The membrane was stripped and rehybridized with a GAPDH-specific probe (lanes 3 and 4). (B) WPRE does not increase transcription initiation frequency. Radiolabeled transcripts produced by nuclear run-on transcription were hybridized to plasmid DNA encoding GAPDH or histone 2B or PCR-derived DNA.

To determine the effects of the WPRE on GFP transcripts, RNA from cytosolic and nuclear fractions of transduced cells wasanalyzed by Northern blotting with a GFP-specific probe (Fig.4B). Three RNA species can be detected by this probe; the twolarger ones correspond to unspliced and spliced transcripts initiatedat the 5' HIV LTR, and the smaller one corresponds to RNAs originatingfrom the internal CMV promoter. All GFP transcripts extractedfrom HR'CMV-GFP-W-transduced cells were larger than their counterpartsextracted from HR'CMV-GFP-transduced cells due to the presenceof the WPRE. The levels of expression of all three classes ofWPRE-containing transcripts were six times higher than those inthe respective controls in both nuclear and cytosolic fractions.

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FIG. 4. RNA analysis of transduced cell lines. (A) Schematic drawing of vectors showing the three classes of generated messages that contain GFP. SD, splice donor; SA, splice acceptor; RRE, Rev-responsive element. (B) Northern blot analysis of nuclear (N) and cytoplasmic (C) RNAs derived from HR'CMV-GFP- and HR'CMV-GFP-W-transduced populations. Analysis for GAPDH expression of the same filter after stripping and reprobing is shown at the bottom. (C) Half-life analysis of total RNA. Actinomycin D was added, and cells were harvested at the times shown. Controls for the unstable histone 2B (H2B) message and the stable GAPDH message are shown below. sp., spliced. (D) Phosphorimager analysis of the Northern blot shown in panel C. Quantitation of GFP and histone 2B levels is shown in the upper panel. Quantitation of GAPDH is shown in the lower panel. Data are expressed as a percentage of levels of expression at time zero over time.

To determine if the WPRE altered the RNA half-life, populations transduced with either HR'CMV-GFP or HR'CMV-GFP-W were incubatedwith actinomycin D. Total RNA was extracted at different timesand analyzed by Northern blotting (Fig. 4C). From the earliesttime, all the WPRE-containing transcripts were much more abundantthan the respective controls. However, the half-life of the WPRE-containingGFP RNA was increased less than twofold compared to that of theGFP RNA, as determined by phosphorimager analysis (Fig. 4D). Takentogether, these results suggest that the WPRE acts very earlyduring the biogenesis of RNA transcripts, perhaps by directingtheir efficient processing as soon as they emerge from the transcriptionalmachinery.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Retroviral vectors can transduce efficiently a variety of cells, but the expression of the integrated transgene is usuallylow. In this study, we demonstrate that a cis-acting RNA elementfrom WHV substantially increases the expression of transgenesdelivered by retroviral vectors. The WPRE was active when insertedin vectors derived from both HIV-1 and MLV. Further, WPRE functionwas not cell type or species dependent, because it could stimulatetransgene expression in several cell lines of human and rodentorigins. The WPRE effect was not influenced by the cycling statusof the transduced cells. The WPRE was only functional when presentwithin a transcript in the sense orientation. The antisense WPREhad a significant inhibitory effect, reducing GFP and luciferaseactivities by a factor of 4 (Fig. 1D and Table 1). The inhibitionseen in the antisense derivative is most likely due to the X promoterof WHV which is present in the WPRE cassette. This promoter couldgenerate antisense RNA complementary to the transgene mRNA. Functionalanalysis revealed that the stimulation of transgene expressionby the WPRE isposttranscriptional.

It was surprising to observe that the WPRE stimulated the expression of spliced mRNAs to the same extent as intronless transcripts.Previous studies had suggested that the HPRE and an intron werefunctionally equivalent (14). However, the studies presentedhere show that the WPRE stimulated the expression of a splicedRNA, suggesting that splicing and the PRE are not functionallyredundant. This observation does not exclude the possibility thatsome functions of the WPRE and splicing of an intron in stimulatinggene expression overlap. It is also possible that the intron withinthe vector does not act to facilitate the expression of transcriptsaftersplicing.

Several observations are consistent with a model in which the WPRE functions within the nucleus to stimulate gene expressionposttranscriptionally. The WPRE increases the levels of nucleartranscripts. The WPRE also does not greatly influence RNA half-life.Further, the observed increase in protein expression roughly correlateswith an increase in RNA levels. It has previously been proposedthat the PRE functions by facilitating RNA export. Although theWPRE does not greatly alter the nucleocytoplasmic ratio of affectedRNAs generated by vector messages, this observation does not excludea role for export in the function of the WPRE. Recent studieshave revealed that the disruption of Rev function by the drugleptomycin B causes a decrease in the amount of nuclear Rev-responsiveelement-containing RNA (23). This observation and the observationthat Rev can increase the nuclear half-life of HIV messages (18)suggest that engagement of an export pathway may simultaneouslyincrease both the nuclear and the cytoplasmic pools of a specificRNA.

Alternatively, the WPRE may facilitate another step in RNA processing, directing RNAs that would normally be degraded withinthe nucleus to be efficiently expressed. This processing couldbe facilitated at the level of 3' cleavage and polyadenylation.It has previously been shown that increasing the efficiency of3' processing can stimulate gene expression (3). The WPRE couldalso function to facilitate the generation of RNA-protein complexeswhich would protect newly synthesized transcripts from degradationin the nucleus. Increasing the efficiency of any one step in RNAprocessing could increase the efficiency of gene expression. Thesepossible modes of action for the WPRE are not mutually exclusive,especially considering that the WPRE contains at least three distinctcis-acting subelements required for maximal function. For instance,one subelement could influence export, while another could increasethe efficiency of 3'processing.

Retroviral vectors have recently become more attractive as delivery systems for use in gene therapy. Lentivirus vectors allownondividing cells to be transduced (20). HIV-based vectors canthus efficiently govern in vivo transgene delivery, integration,and long-term expression in nonmitotic cells, such as neurons,myocytes, and hepatocytes (15, 19). The initially low clinicalacceptance of lentivirus vectors has been considerably increasedby the development of multiply attenuated and self-inactivating(9, 28, 29) HIV-based vectors while, in parallel, analogousvectors have been derived from nonhuman lentiviruses (24). Ourstudies demonstrate that the WPRE can significantly improve theperformance of retroviral vectors for use both in gene therapyprotocols and in basic research. It is likely that the WPRE willalso stimulate the expression of transgenes delivered by othervector systems. This improvement in the expression of genes deliveredby retroviral vectors helps to bring the promise of gene therapyone step closer tofruition.

	ACKNOWLEDGMENTS

We thank Allison Bocksrucker for assistance in preparing the manuscript and Matthew Weitzman for critical reading of themanuscript.

This work was supported by a grant from the Swiss National Science Foundation and from the Berger Foundation and by a professorshipfrom the Giorgi-Cavaglieri Foundation to D.T. and by grants fromthe Gene and Ruth Posner Foundation and by a gift from ArthurKramer and Larry Kramer to T.J.H. R.Z. was the recipient of afellowship from the Swiss National Science Foundation, and J.E.D.was supported by NCI training grant T32CA64041.

	FOOTNOTES

^* Corresponding author. Mailing address for Didier Trono: Department of Genetics and Microbiology, CMU, 1 rue Michel-Servet,CH-1211 Geneva 4, Switzerland. Phone: (41 22) 702 5720. Fax: (4122) 702 5721. E-mail: didier.trono{at}medecine.unige.ch. Mailingaddress for Thomas J. Hope: Infectious Disease Laboratory, SalkInstitute, P.O. Box 85800, San Diego, CA 92186-5800. Phone: (619)453-4100, ext. 1559. Fax: (619) 554-0341. E-mail: hope{at}salk.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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