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J Virol, July 1998, p. 5441-5448, Vol. 72, No. 7
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Département de Microbiologie et Immunologie, Université de Montréal, Montréal, Québec, Canada H3C 3J7,1 and Division of Human Retrovirology, Dana-Farber Cancer Institute, Harvard Medical School, Boston, Massachusetts 021152
Received 8 December 1997/Accepted 25 March 1998
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ABSTRACT |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Inactivation of progeny virions with chimeric virion-associated proteins represents a novel therapeutic approach against human immunodeficiency virus (HIV) replication. The HIV type 1 (HIV-1) Vpr gene product, which is packaged into virions, is an attractive candidate for such a strategy. In this study, we developed Vpr-based fusion proteins that could be specifically targeted into mature HIV-1 virions to affect their structural organization and/or functional integrity. Two Vpr fusion proteins were constructed by fusing to the first 88 amino acids of HIV-1 Vpr the chloramphenicol acetyltransferase enzyme (VprCAT) or the last 18 C-terminal amino acids of the HIV-1 Vpu protein (VprIE). These Vpr fusion proteins were initially designed to quantify their efficiency of incorporation into HIV-1 virions when produced in cis from the provirus. Subsequently, CD4+ Jurkat T-cell lines constitutively expressing the VprCAT or the VprIE fusion protein were generated with retroviral vectors. Expression of the VprCAT or the VprIE fusion protein in CD4+ Jurkat T cells did not interfere with cellular viability or growth but conferred substantial resistance to HIV replication. The resistance to HIV replication was more pronounced in Jurkat-VprIE cells than in Jurkat-VprCAT cells. Moreover, the antiviral effect mediated by VprIE was dependent on an intact p6gag domain, indicating that the impairment of HIV-1 replication required the specific incorporation of Vpr fusion protein into virions. Gene expression, assembly, or release was not affected upon expression of these Vpr fusion proteins. Indeed, the VprIE and VprCAT fusion proteins were shown to affect the infectivity of progeny virus, since HIV virions containing the VprCAT or the VprIE fusion proteins were, respectively, 2 to 3 times and 10 to 30 times less infectious than the wild-type virus. Overall, this study demonstrated the successful transfer of resistance to HIV replication in tissue cultures by use of Vpr-based antiviral genes.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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The assembly and maturation of human immunodeficiency virus (HIV) particles constitute a complex process in which the structural gag, pol, and env gene products are expressed in the form of polyprotein precursors. The production of infectious viral particles requires incorporation of the Env glycoproteins gp120 and gp41 during viral budding and processing of the Gag and Gag-Pol polyproteins by the viral protease (12, 34). In addition to gag, pol, and env gene products, HIV type 1 (HIV-1) virions have been shown to contain several accessory proteins, including Vpr (7), Vif (15), and Nef (35). Vpr, a 14-kDa, 96-amino-acid nuclear protein, is packaged into HIV virions in amounts similar to those of Gag, while Vif and Nef appear to be incorporated in quantities comparable to that of Pol (5, 6, 35). The HIV-1 Vpr protein is incorporated in trans into viral particles through an interaction with the p6 domain of the Gag polyprotein precursors (20, 23).
The resistance of AIDS to traditional drug therapy has prompted a search for alternative treatments for this disease. One potential approach, termed intracellular inhibition or immunization, is designed to render cells resistant to viral replication and to limit the spread of virus in a cell culture or an individual (1, 14). Inhibition of HIV replication by such a strategy has now been established with different antiviral genes, including those directed at a nucleic acid or protein target (14). Virus-targeted inactivation represents a novel genetic approach to interfering with HIV replication. In this strategy, a deleterious amino acid sequence or sequence with enzymatic activity is fused to a virion-associated component to prevent the production of infectious viral particles and the subsequent spread of de novo infection (3). Several studies have demonstrated the efficient packaging of Vpr fused with a polypeptide sequence. The incorporation of Vpr fused to integrase (VprIN), reverse transcriptase (RT) (VprRT), enzymatically active staphylococcal nuclease, chloramphenicol acetyltransferase (CAT), and a trans-dominant negative mutant of the HIV-1 protease into HIV particles has been demonstrated (3, 13, 31, 37-39). Moreover, the expression of Vpr proteins fused to HIV-1 protease cleavage sites was recently shown to affect HIV-1 replication (33). However, the possibility that the stable transfer of genes encoding Vpr fusion proteins in HIV target cells could provide genetic resistance to viral replication remains to be demonstrated. In this paper, we report that a reporter enzyme (CAT) or a short peptide sequence derived from the HIV-1 Vpu protein fused to the carboxyl terminus of Vpr can be targeted specifically and efficiently into HIV particles. Using retroviral vectors, we demonstrate that the stable expression of these Vpr fusion proteins in CD4+ T cells can confer substantial resistance to HIV-1 replication by affecting the infectivity of progeny virions.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Site-directed mutagenesis and plasmid DNA constructions.
HxBRU (long terminal repeat [LTR]-gag+
pol+ vif+ vpr+ tat+
rev+ vpu
env+
nef-LTR) and HxBRU-R- (LTR-gag+
pol+ vif+ vpr tat+
rev+ vpu env+
nef-LTR) are two isogenic infectious molecular
clones of HIV-1 that differ only in their ability to express Vpr
(22). A unique XbaI site was inserted at position
5410 (position 1 is the site of transcription initiation of the HxBRU
molecular clone) in HxBRU by use of two-step PCR-based mutagenesis as
previously described (22). The nucleotide sequence of the
sense mutagenic oligonucleotide was as follows: 5'-CAG AGG AGA TCT AGA
AAT GGA GCC-3'. The resulting HxBRUXbaI mutant construct was confirmed
by sequencing with a Sequenase kit (United States Biochemical Co.).
Cells and DNA transfection.
MT4, Jurkat, COS-7, and 293T
cells (all from the American Type Culture Collection) and
HeLa-CD4-LTR/
-Gal indicator cells were maintained as described
previously (18, 22). MT4 (5 × 106) and
Jurkat (1 × 107) cells were transfected with 10 µg
of plasmid DNA by the DEAE-dextran transfection method as described
previously (22). COS-7 cells (106) were
transfected with 20 µg of proviral DNA and 293T cells
(106) were transfected with 20 µg of pCEP expression
vectors by the calcium phosphate method as described previously
(22).
Cell transduction and infection.
In order to generate Jurkat
cell lines expressing Vpr fusion proteins or RevM10, retroviral vector
technology was used. The 
CRIP packaging cell line was cultured as
described previously (10). Aliquots (10 µg) of pBabepuro,
pBabepuro-VprIE, pBabepuro-VprCAT, or pBabepuro-RevM10 vectors were
transfected into CRIP packaging cells by the calcium phosphate
method (22). CRIP cells that stably produced
amphotropically packaged pBabepuro, pBabepuro-VprIE, pBabepuro-VprCAT,
or pBabepuro-RevM10 vectors were obtained by selection with 1.2 µg of
puromycin (Calbiochem) per ml, generating CRIP-puro, CRIP-VprIE,
CRIP-VprCAT, or CRIP-RevM10 cell lines, respectively.
Transduction of Jurkat cells was performed as described previously
(36). Puromycin-resistant Jurkat cell populations were
isolated, characterized, and subsequently challenged with HIV-1.
Infections were performed as follows: 3 × 106
parental, control, or transduced Jurkat cells were absorbed for 2 h with different amounts of HIV in 1 ml of RPMI medium plus 10% fetal
calf serum. Following infection, the culture medium was changed every 3 days and cells were resuspended in 10 ml of fresh RPMI medium plus 10%
fetal calf serum at densities of 5 × 105 viable cells
per ml.
Metabolic labeling, immunoprecipitation, and CAT activity measurement. At 72 h posttransfection, COS-7 cells were starved in methionine-free Dulbecco modified Eagle medium for 30 min. The cells were then metabolically labeled with 50 µCi of [35S]methionine per ml for 16 h. For each sample, viral particles were pelleted by ultracentrifugation of an equal volume of supernatant fluid through a 20% sucrose cushion at 35,000 rpm for 2 h at 4°C in a Beckman 55.2 Ti rotor. The labeled pelleted virus and cells were lysed in radioimmunoprecipitation assay buffer and immunoprecipitated as previously described (22) with an HIV-1-positive human serum combined with either a rabbit anti-Vpr polyclonal serum (22), a rabbit anti-Vpu peptide serum (8), or a rabbit anti-CAT polyclonal serum (5' Prime 3' Prime) in a 1:1 ratio. HIV-associated proteins were separated on a sodium dodecyl sulfate-12.5% polyacrylamide gel and visualized by autoradiography. Quantitative analysis of immunoprecipitated proteins was performed by densitometric scanning of the autoradiographic signals on a Personal Densitometer (Molecular Dynamics) with ImageQuant software, version 3.22. In order to evaluate the level of VprCAT expressed in cells and incorporated into virions, CAT assays were performed (16). Cells and virus pelleted through a 20% sucrose cushion (see above) (virus was produced from HxBRU-VprCAT-transfected COS-7 cells) were harvested with 250 mM Tris-HCl (pH 7.4) and processed as previously described (16).
RNA extraction and Northern blot analysis.
Cytoplasmic and
nuclear RNAs were isolated from 107 parental or transduced
Jurkat cells with TRIzol reagent as described by the manufacturer
(GIBCO/BRL). Poly(A) RNA was then purified with a QuickPrep Micro mRNA
purification kit as instructed by the manufacturer (Pharmacia). RNA was
resolved on a 1% agarose gel containing formaldehyde and transferred
to a nitrocellulose membrane (Bio-Rad). The Vpr probe was generated by
PCR amplification with BamHI primers (see above) and pNL4.3
as a template. The purified DNA fragment was labeled with
[
-32P]dCTP by use of a random-primer DNA-labeling
system (Pharmacia). Prehybridization and hybridization were performed
as previously described (21).
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Construction of Vpr fusion proteins. Recent studies reported that the expression of the HIV-1 Vpr protein induced the accumulation of cells in the G2 phase of the cell cycle (17, 32). Mutational analysis revealed that the highly charged carboxy-terminal domain appears to be critical for Vpr stability and cell cycle arrest, while the integrity of the N-terminal amphipatic alpha helix is required for virion incorporation and nuclear localization (11, 24, 25). Since the expression of therapeutic molecules should not affect cell homeostasis in vitro and more importantly in vivo, we constructed Vpr fusion proteins by fusing antigens to the carboxyl-terminal end of a truncated Vpr mutant (88 amino acids). Two Vpr fusion proteins were initially generated to explore the possibility of targeting a sequence with enzymatic activity or an epitope tag into HIV-1 virions. For the first fusion partner, we used the C-terminal 18 amino acids of the Vpu protein, thus generating the VprIE protein. We selected this amino acid sequence because it contains an immunodominant epitope (IE) well recognized by a rabbit anti-Vpu peptide serum (8). Moreover, in order to study the efficiency of incorporation of larger proteins and to investigate whether an enzyme could be active in virions, we used the CAT protein as the second fusion partner (VprCAT). DNA fragments encoding the two Vpr fusion proteins were generated and subsequently cloned into the HxBRU infectious molecular clones as well as into the pBabepuro retroviral vector and the pCEP4 expression vector as described in Materials and Methods.
Protein expression and replication potential of HIV-1 virions carrying VprCAT and VprIE fusion proteins. To test the expression and incorporation of the Vpr fusion proteins into HIV-1 virions, HxBRU-VprIE, HxBRU-VprCAT and, as a control, HxBRU were transfected into COS-7 cells. At 72 h posttransfection, labeled cell lysates and pelleted virus were immunoprecipitated with an HIV-1-positive human serum combined with specific anti-Vpr, anti-Vpu, or anti-CAT antibodies. Results indicated that antibodies directed against Vpr or Vpu immunoprecipitated the predicted 18-kDa VprIE protein from virions and cell lysates (Fig. 1, lanes 3, 4, 9, and 10). Similarly, antibodies directed against Vpr or CAT detected the predicted 35-kDa VprCAT protein in virions and cell lysates (Fig. 1, lanes 5, 6, 11, and 12). This result indicates that VprIE and VprCAT fusion proteins are expressed from recombinant proviruses in transfected COS-7 cells. We observed with HxBRU-VprIE a second band corresponding to the molecular mass of the 16-kDa Vpr protein. This Vpr-related product appears to result from a deletion of the Vpu-derived sequences, possibly by recombination rearrangement in COS-7 cells, since the product comigrated with Vpr and was immunoprecipitated with the anti-Vpr antibody but not with the anti-Vpu antibody (Fig. 1, lanes 9 and 10). Under our conditions, low-molecular-mass products derived from VprCAT were not detected in significant amounts (Fig. 1, lanes 11 and 12).
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Generation and characterization of Jurkat CD4+ T-cell
lines expressing Vpr fusion proteins.
Amphotropic murine
retroviruses carrying pBabepuro, pBabepuro-VprIE, and pBabepuro-VprCAT
were used to transduce Jurkat cells. Following puromycin selection,
populations of cells consisting of a pool of, respectively,
Jurkat-puro, Jurkat-VprIE, and Jurkat-VprCAT puromycin-resistant cell
clones were isolated and amplified. To evaluate the level of VprIE or
VprCAT gene expression in transduced Jurkat cell lines, we performed
Northern blot analysis of purified total mRNAs by using a
vpr-specific probe as described in Materials and Methods.
Figure 2A shows the expected 2.5- and
2.6-kb vprIE- and vprCAT-specific mRNAs, detected
only in Jurkat-VprIE and Jurkat-VprCAT cell lines, respectively (lanes
2 and 3). All attempts to detect VprIE and VprCAT protein expression by
immunoprecipitation or Western blot analysis were unsuccessful,
indicating that the level of expression of both Vpr fusion proteins in
transduced Jurkat cells was low. We also attempted to demonstrate the
expression and virion incorporation of the VprCAT fusion protein in
HIV-1-infected Jurkat-VprCAT cell lines by CAT activity measurements.
Briefly, 3 × 106 parental or Jurkat-VprCAT cells were
infected with equivalent amounts (106 cpm of RT activity)
of HxBRU and HxBRU-R-. At 6 days postinfection, cells and
virus-containing supernatants were collected, and virions were pelleted
by ultracentrifugation through a 20% sucrose cushion. CAT activity was
undetectable in infected and uninfected Jurkat-VprCAT cells (data not
shown). In contrast, CAT activity associated with Vpr+ and
Vpr HIV-1 virions was detected (Fig. 2B), indirectly
indicating that VprCAT proteins were expressed in Jurkat-VprCAT cells.
These results also suggest that trans incorporation
concentrated VprCAT in the virions to detectable levels. Importantly,
virion incorporation of VprCAT appeared less efficient in HxBRU than in
HxBRU-R-, since the level of CAT activity associated with the
Vpr+ virus was lower than the level of CAT activity
associated with the Vpr virus. This result suggests that
competition for virion incorporation occurred between the
virus-expressed Vpr and the VprCAT fusion protein.
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Effect of Vpr fusion protein expression on HIV-1 replication. We next evaluated the ability of HIV-1 to replicate in Jurkat-VprIE and Jurkat-VprCAT cell lines. The Jurkat-puro cell line was used as a control. The replication kinetics were analyzed by monitoring viral production in the culture supernatant (determined by RT activity measurements) every 3 days over time. Briefly, each Jurkat cell line was infected with increasing amounts (25,000, 100,000, and 300,000 cpm, as determined by RT activity) of HxBRU and HxBRU-R- viruses produced from transfected MT4 cells. Figure 3A shows the replication kinetics obtained when Jurkat-VprCAT and Jurkat-puro cells were infected with 100,000 cpm of HxBRU or HxBRU-R-. Maximum replication of HxBRU and HxBRU-R- was delayed by 2 to 3 days in Jurkat-VprCAT cells relative to control cells. Interestingly, in the same experiment, when Jurkat-VprIE cells were infected with 100,000 cpm of virus, a more pronounced delay of viral replication was observed (Fig. 3B). Peak viral replication was detected at day 15 in control cells infected with both HxBRU and HxBRU-R-. In contrast, maximum replication in Jurkat-VprIE cells was detected between days 21 and 24 for HxBRU and at approximately day 27 for HxBRU-R- (Fig. 3B). This result reveals that the replication of HxBRU and HxBRU-R- was delayed by 6 and 12 days, respectively, in Jurkat-VprIE cells relative to control cells. This result also indicates that HxBRU-R-, which does not express a native Vpr protein, replicates less efficiently than HxBRU in Jurkat-VprIE cells. The delay in the replication of HxBRU-R- in Jurkat-VprIE cultures also varied according to the input virus. Figure 3C and D show the replication kinetics obtained when Jurkat-VprIE and control cells were infected with 300,000 (Fig. 3C) or 25,000 (Fig. 3D) cpm of HxBRU or HxBRU-R-. When cells were infected with 300,000 cpm of virus, maximum replication of HxBRU and HxBRU-R- was delayed, respectively, by 6 and 9 days (Fig. 3C). However, when cells were infected with 25,000 cpm of virus, delays of approximately 6 and 18 days, respectively, were observed with HxBRU and HxBRU-R- (Fig. 3D). The appearance of virus-associated cytotoxic effects was also delayed in Jurkat cells expressing Vpr fusion proteins relative to control cells (data not shown). These results demonstrate that Jurkat-VprIE cells were less permissive for HIV-1 replication than Jurkat-puro control cells. They also exhibited a higher degree of resistance to cell killing mediated by HxBRU and HxBRU-R- than control cells.
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virus (HxBRU-R-) more
effectively than RevM10.
Impairment of HIV-1 replication by VprIE is dependent on an intact
p6gag domain.
Several studies have shown
that Vpr is incorporated into HIV-1 particles through a specific
interaction with the p6gag domain (20,
23). Mutational analysis of the p6gag
domain demonstrated that the integrity of the LXXLF motif at the
carboxy terminus of p6 was essential for Vpr incorporation into virions
(19). To determine whether the delayed HIV-1 replication in
transduced Jurkat cells was due to the specific incorporation of Vpr
fusion proteins into virions, Jurkat-VprIE cells were challenged with
p6gag mutants that do not incorporate Vpr. Two
mutations targeting the LXXLF motif of p6gag,
L44P and F45S, were introduced into the vpr
HIV-1 infectious molecular clone HxB89-R-, generating HxB89LF-PS-R-, as
described in Materials and Methods. Cotransfection of HxB89LF-PS-R- and
pCEPVpr into COS-7 cells revealed that Vpr was highly expressed in
cells but not incorporated into virions (data not shown). Stocks of
HxB89LF-PS-R- and the isogenic p6 wild-type counterpart HxB89-R- were
generated by transfection into MT4 cells, and 300,000 cpm was used to
infect Jurkat-puro or Jurkat-VprIE cell lines. As shown in Fig.
4, peak viral production appeared at
approximately day 17 for HxB89FS-PS-R- in both Jurkat-puro and
Jurkat-VprIE cell lines, indicating that the replication of this virus,
which had lost its ability to incorporate Vpr, was not affected by
VprIE expression. In contrast, the replication of HxB89-R- was delayed by approximately 9 days in Jurkat-VprIE cells relative to Jurkat-puro cells (Fig. 4). These results indicate that the antiviral effect of
VprIE is mediated by the incorporation of the fusion protein into HIV-1
virions.
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Incorporation of VprIE and VprCAT into HIV virions impairs viral
infectivity but not viral production.
The results presented above
indicate that VprIE and, to a lesser extent, VprCAT interfere with
viral replication by affecting viral production and/or infectivity. To
evaluate whether VprCAT or VprIE expression affected viral production,
Jurkat-VprCAT and Jurkat-VprIE cell lines were transfected with HxBRU
or HxBRU-R- infectious molecular clones. Measurements of viral
production were obtained with a p24 enzyme-linked immunosorbent assay
24 h posttransfection to detect mainly viruses resulting from the first round of replication. The levels of p24 antigen were found to be
similar in all samples (data not shown), indicating that there was no
impairment at the levels of viral gene expression, assembly, and
release of viral particles. This result suggests that the infectivity
potential of the released viral particles that incorporated Vpr fusion
molecules might be affected. To evaluate the infectious potential of
HIV-1 virions containing VprCAT or VprIE fusion proteins, we performed
multinuclear activation of galactosidase indicator cell (MAGI) assays
(18). Viruses containing Vpr fusion proteins or control
virus produced from infected transduced Jurkat cells (Fig. 3A and B)
was harvested at the peak of viral production and titrated by RT
activity measurements. In three experiments performed with three
different virus stocks, MAGI cells were infected with 300,000 cpm of
each virus. Figure 5 shows that HIV-1
released from Jurkat-VprCAT cells (HxBRU/VprCAT and HxBRU-R-/VprCAT)
was two to three times less infectious than control vpr+ or vpr virus
produced from Jurkat-puro cells. However, HIV-1 released from
Jurkat-VprIE cells (HxBRU/VprIE and HxBRU-R-/VprIE) was 10 to 30 times
less infectious than control virus produced from Jurkat-puro cells
(Fig. 5). Furthermore, HxBRU-R-/VprCAT or HxBRU-R-/VprIE viruses
exhibited a larger impairment of viral infectivity than HxBRU/VprCAT or
HxBRU/VprIE viruses, again suggesting that competition between
HIV-1-encoded Vpr and Vpr fusion proteins for virion incorporation occurred. Although less quantitative, the negative effect of Vpr fusion
proteins on viral infectivity was also observed in transient experiments. Indeed, virus produced by transient cotransfection of
pCEPVprCAT or pCEPVprIE and HxBRU-R- in COS-7 cells exhibited two- and
fourfold inhibition of infectivity in a MAGI cell assay, respectively
(data not shown). Overall, these results strongly suggest that the
impairment of viral infectivity is the consequence of Vpr fusion
protein incorporation into HIV-1 virions.
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Recent progress in our understanding of the structural and functional domains of Vpr makes the design of very efficient Vpr-based antiviral genes possible. To address the question of whether Vpr could be used as a shuttle to target foreign amino acid sequences of different sizes into HIV-1 virions, an XbaI restriction site was inserted at the 3' end of vpr in the infectious molecular clone HxBRU (22). The resulting construct, which replicates as efficiently as wild-type HxBRU (unpublished data), had the advantage of providing a simple means to screen several Vpr fusion proteins for their ability to be packaged into HIV-1 virions. Moreover, HxBRUXbaI provided a quantitative and physiological assay for Vpr fusion protein incorporation into HIV particles. Indeed, our results revealed that the first 88 amino acids of Vpr were sufficient to incorporate the 18-amino-acid Vpu C-terminal immunodominant epitope and the 218-amino-acid CAT enzyme into HIV-1 virions. Importantly, the packaging efficiency of the VprCAT and VprIE fusion proteins was comparable to that obtained with wild-type Vpr (Fig. 1).
Previous studies reported that Vpr fusion proteins could severely
impair HIV replication in CD4+ T cells when expressed in
cis from the provirus (28, 33). All of our
attempts to express Vpr fusion proteins in the context of the HxBRUXbaI
proviral construct revealed that this biological system was not
reliable for the evaluation of the viral replication potential. Indeed,
we found that the introduction of foreign DNA sequences between the Tat
splice acceptor site and the Tat initiation codon had a
cis-acting negative effect on HIV protein expression (data
not shown). On the other hand, transient expression experiments in
which a vpr+ or a vpr
provirus was cotransfected with a Vpr fusion protein expressor did not
allow for the sensitive measurement of antiviral activity, since the
different transfection efficiencies of the two plasmids gave highly
variable results. For quantitative measurement of antiviral activity,
T-cell lines that express Vpr fusion proteins constitute a more
reliable system. In addition, the stable expression of therapeutic
genes in cell lines is essential to evaluate their possible effect on
cell homeostasis as well as their effectiveness in a gene therapy
approach.
Consequently, we generated CD4+ Jurkat cell populations constitutively expressing Vpr fusion proteins by using retroviral vectors. This system provided a reliable method to evaluate the effect of Vpr fusion proteins on viral replication and spread in vitro, since the ideal situation, in which 100% of HIV-1 target cells carried the therapeutic gene, was achieved. We first investigated the expression of VprIE and VprCAT in selected transduced Jurkat cell populations. The expression of vprIE- and vprCAT-specific mRNAs was demonstrated by Northern blot analysis (Fig. 2B). Moreover, CAT enzymatic activity associated with the VprCAT fusion protein was efficiently incorporated in trans into HIV-1 virions (Fig. 2C). However, we failed to detect the expression of the transgenes by immunoprecipitation and Western blot analysis. It has been shown that proteins are poorly expressed from the Moloney murine leukemia virus LTR in human-derived CD4+ T-cell lines (29).
The effect of VprCAT and VprIE fusion proteins on cell division was quantitatively evaluated with 293T cells. The results indicated that cells expressing VprCAT or VprIE fusion proteins proliferated and formed colonies with the same efficiency as the pCEPVpr-R- positive control, which did not express Vpr (Fig. 2C). The first 88 amino acids of Vpr therefore appeared sufficient to achieve Vpr fusion protein virion incorporation without any negative effect on cellular growth. This finding allowed us to isolate Jurkat-puromycin-resistant clones that expressed Vpr fusion proteins and that were later pooled to obtain a stable cell population representative of the parental Jurkat cell line. Infection of transduced Jurkat-VprCAT or Jurkat-VprIE cell lines resulted in partial inhibition of HIV-1 replication compared to that for control cells (Fig. 3A and B). To confirm that the delays in viral replication observed when we challenged the different Jurkat cell lines were not an artifact arising from cell line selection, we analyzed CD4 expression at the cell surface. Fluorescence-activated cell sorter analysis demonstrated that CD4 expression at the plasma membrane of both Jurkat-VprCAT and Jurkat-VprIE cells was similar to that of parental Jurkat cells (data not shown). Moreover, a p6gag mutant of HIV-1 that did not incorporate Vpr replicated as efficiently in Jurkat-VprIE cells as in Jurkat-puro control cells (Fig. 4), indicating that the impairment of viral replication in Jurkat-VprIE cells was the consequence of VprIE fusion protein incorporation into virions. Overall, these results argue strongly against a clonal effect resulting from cell population selection as a major contributor to the impairment of viral replication.
Virion infectivity has been shown to correlate with proper viral assembly and maturation (12, 34). The presence of a nonrelevant amino acid sequence fused to Vpr during assembly and budding may affect viral morphogenesis, resulting in the production of virus with a drastically reduced infectious potential. Indeed, as shown in Fig. 3B, the introduction of 18 amino acids derived from HIV-1 Vpu at the C-terminal end of Vpr affected considerably the replication of HIV-1 in tissue cultures. This antiviral effect of VprIE was shown to be as efficient as that exerted by a transdominant mutant of Rev, the RevM10 protein, which inhibits HIV-1 replication through a distinct mechanism (Fig. 3E). In contrast, the 35-kDa VprCAT fusion protein delayed HIV-1 replication less efficiently (Fig. 3A). Analysis of virus produced from transduced Jurkat cells revealed that virus released from Jurkat-VprCAT cells was two to three times less infectious than the control virus, whereas virus produced from Jurkat-VprIE cells exhibited a 10- to 30-fold decrease in viral infectivity (Fig. 5). We currently assume that the highly hydrophilic Vpu sequence fused to Vpr may provoke an important steric hindrance, which in turn affects normal viral morphogenesis. Indeed, electron microscopy revealed a strong morphological alteration of virions containing VprIE fusion proteins (unpublished data). However, at this point we cannot rule out the possibility that early events following the entry of wild-type virus into VprIE-expressing cells may be affected.
From a therapeutical point of view, an efficient Vpr fusion protein
should impair the replication of a large range of HIV isolates, which
could be vpr+ or vpr.
Figure 2B shows that the vpr+ HxBRU virus
incorporated less VprCAT fusion protein than the vpr HxBRU-R- virus. Moreover, HxBRU-R- was
less infectious than HxBRU when produced in Jurkat-VprIE or
Jurkat-VprCAT cell lines (Fig. 5). These results suggest competition
for virion incorporation between wild-type Vpr expressed from HxBRU and
Vpr fusion proteins provided in trans by the transduced cell
lines. Consequently, it was not surprising to observe a greater delay
in viral replication in Jurkat-VprIE cells infected with HxBRU-R- than
in Jurkat-VprIE cells infected with HxBRU (Fig. 3B, C, and D). No such
difference was observed in Jurkat-VprCAT cells. This finding likely
reflects the weak antiviral effect of VprCAT on HIV replication (Fig.
3A). The competition for virion incorporation between Vpr fusion
proteins and wild-type Vpr expressed by the virus remains a
critical point. Indeed, an increased delay in viral
replication was observed with decreasing amounts of HxBRU-R- virus
in Jurkat-VprIE cells, an effect that was not observed with the HxBRU
virus (compare Fig. 3B, C, and D). Therefore, the development of Vpr
fusion proteins that could target both HIV-1 production and infectivity
and that could efficiently compete with wild-type Vpr for virion
incorporation remains an essential and promising goal.
This report presents, for the first time, proof of principal experiments showing that virion-targeted viral inactivation with Vpr fusion proteins can delay HIV-1 replication in transduced CD4+ T cells. Therefore, the development of more efficient Vpr-based fusion proteins represents a promising approach that may contribute to efficient strategies against HIV infection.
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ACKNOWLEDGMENTS |
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We thank Richard Mulligan for the CRIP packaging cell line,
Bryan Cullen for the pM10 construct (containing RevM10), and Andrew J. Mouland for critical reading of the manuscript.
G.P.K. is the recipient of a studentship from the National Health Research and Development Program (NHRDP) of Canada. E.A.C. is the recipient of a National Health Research Scholar award from NHRDP. This work was supported by grants from the Medical Research Council of Canada, the Pharmaceutical Manufacturers Association of Canada, and Theratechnologies Inc. to E.A.C.
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FOOTNOTES |
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* Corresponding author. Mailing address: Laboratoire de Rétrovirologie Humaine, Département de Microbiologie et Immunologie, Faculté de Médecine, Université de Montréal, CP 6128, succursale Centre-ville, Montréal, Québec, Canada H3C 3J7. Phone: (514) 343-5967. Fax: (514) 343-5995. E-mail: cohenea{at}ere.umontreal.ca.
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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