The Interaction of Vpr with Uracil DNA Glycosylase Modulates the Human Immunodeficiency Virus Type 1 In Vivo Mutation Rate

doi:10.1128/JVI.74.15.7039-7047.2000

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Journal of Virology, August 2000, p. 7039-7047, Vol. 74, No. 15
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Interaction of Vpr with Uracil DNA Glycosylase Modulates the Human Immunodeficiency Virus Type 1 In Vivo Mutation Rate

Louis M. Mansky,¹^,^* Sandra Preveral,² Luc Selig,²^, Richard Benarous,² and Serge Benichou²

Department of Molecular Virology, Immunology, and Medical Genetics, Center for Retrovirus Research, and Comprehensive Cancer Center, Ohio State University Medical Center, Columbus, Ohio 43210,¹ and INSERM U529, ICGM, Université Paris V, Paris, France²

Received 8 March 2000/Accepted 1 May 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Vpr protein of human immunodeficiency virus type 1 (HIV-1) influences the in vivo mutation rate of the virus. Since Vprinteracts with a cellular protein implicated in the DNA repairprocess, uracil DNA glycosylase (UNG), we have explored the contributionof this interaction to the mutation rate of HIV-1. Single-amino-acidvariants of Vpr were characterized for their differential UNG-bindingproperties and used to trans complement vpr null mutant HIV-1.A striking correlation was established between the abilities ofVpr to interact with UNG and to influence the HIV-1 mutation rate.We demonstrate that Vpr incorporation into virus particles isrequired to influence the in vivo mutation rate and to mediatevirion packaging of the nuclear form of UNG. The recruitment ofUNG into virions indicates a mechanism for how Vpr can influencereverse transcription accuracy. Our data suggest that distinctmechanisms evolved in primate and nonprimate lentiviruses to reconcileuracil misincorporation into lentiviralDNA.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Retroviral RNA is copied into DNA by the virus-encoded enzyme reverse transcriptase via a process called reverse transcription(2, 42). The error-prone nature of reverse transcriptiongreatly contributes to the high level of genetic diversity observedwithin populations of retroviruses (4, 14, 18, 40, 41).Several variables define the diversity of human immunodeficiencyvirus type 1 (HIV-1) and retrovirus populations: (i) the rateof mutation per replication cycle, (ii) the number of replicationcycles, (iii) the fixation rate of mutations, and (iv) the rateof recombination (6, 26). The high rate of HIV-1 replicationis an important determinant in driving HIV-1 evolution (5,13, 47).

A genetically engineered system has been developed for HIV-1 to measure the in vivo rate of forward mutation per replicationcycle (27). The mutation rate of HIV-1 in this system was determinedto be 3 × 10⁵ to 4 × 10⁵ mutation per target base pair per cycle (24, 27), where basesubstitution mutations (G-to-A and C-to-T transitions) and frameshiftmutations ( $-$ 1 frameshifts in runs of T's and A's) were most commonlydetected. Replication of HIV-1 in the presence or absence of theauxiliary protein Vpr indicated that the mutation rate was asmuch as fourfold higher in the absence of Vpr (25, 27). Thisindicated that Vpr could influence the in vivo mutation rate ofHIV-1. The vpr gene encodes a 96-amino-acid (aa) nonstructuralprotein which is associated with HIV-1 particles at a level comparableto that of the Gag precursor and then accumulates in the nucleiof infected cells (7, 22, 30). Incorporation of Vpr intoparticles requires a direct interaction with the p6 region ofGag (1, 35). In addition to influencing the mutation rate,Vpr has been implicated in the nuclear translocation of the preintegrationcomplex and in cell arrest in the G₂ phase of the cell cycle (11,12, 17, 33). A recent report has indicated that Vpr alonecould decrease the frequency of deletion mutations which occurfollowing introduction of UV-damaged plasmid DNA into cells (16).This phenotype does not appear to be related to Vpr's role inthe process and accuracy of reverse transcription (25).

The HIV-1 Vpr protein has been found to interact with several cellular partners (32, 51), in particular with two proteinsinvolved in the DNA repair process, uracil DNA glycosylase (UNG)and the human homologue of the yeast RAD23 protein (HHR23A) (3,10, 49). UNG is an enzyme involved in the base excision repairpathway which specifically removes the RNA base uracil from DNA(19). Uracil appears in DNA by misincorporation during its synthesiswhen the dUTP pool level is high or by cytosine deamination ofdCMP. When cytosine deamination occurs and is not repaired, theresult is a C-to-T transition mutation in that DNA strand (anda G-to-A transition in the opposite strand) in the next roundof replication. The human ung gene contains two promoters thatare required for generation of the mitochondrial (UNG1) and nuclear(UNG2) forms of the enzyme by alternative splicing (28). UNG1and UNG2 have 35 and 44 unique N-terminal aa, respectively, whilethe C-terminal 269 aa are identical and contain the catalyticdomain. The Vpr-binding site was mapped within the common C-terminalpart of UNG, but the interaction did not perturb in vitro UNGenzymatic activity (3). While recent results suggest that theHHR23A protein is a mediator of Vpr-induced cell cycle arrest(10, 34), a detailed mutational analysis of Vpr revealed thatthe interaction with UNG is genetically separable from the abilityof Vpr to perturb the cell cycle (49). A Trp residue locatedin position 54 of Vpr was found to be critical for the interactionwith UNG, but replacement of this residue did not disrupt theG₂ arrest activity. It has been observed that Vpr from simianimmunodeficiency virus of sooty mangabeys, but not Vpx, associateswith UNG (36).

Based on these observations, we tested the hypothesis that the interaction of Vpr with UNG could influence the in vivo mutationrate of HIV-1. We found that binding of Vpr to UNG correlateswith the influence of Vpr on the mutation rate. We demonstratethat Vpr recruits the nuclear form of UNG into HIV-1 virions toinfluence the in vivo mutation rate. These data indicate a mechanismby which Vpr can influence reverse transcription accuracy andsuggest the evolution of distinct mechanisms in primate and nonprimatelentiviruses to reconcile uracil misincorporation into lentiviralDNA.

	MATERIALS AND METHODS

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HIV-1 vectors and expression plasmids used for mutation rate studies. The HIV-1 vector used in the in vivo forward mutation rate assay (Fig. 1A) was constructed as previously described (27).A vpr null mutant derivative of this vector was made by a primary-combinatorialtwo-step PCR protocol (25). Plasmids pSVgagpol-rre-r and pSV-A-MLV-envhave been previously described (25). The vectors used for expressionof wild-type (wt) Vpr or Vpr variants (pCMVvpr) were constructedby amplifying the wt or mutated vpr gene by PCR and insertingit into plasmid pCR3 (Invitrogen). The Vpr variants (Vpr*W54Rand Vpr*R90K) were selected by two-hybrid screening from an HIV-1Vpr mutant library generated by random error-prone PCR (34).

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FIG. 1. HIV-1 vector used for in vivo forward mutation rate studies. (A) vpr null mutant HIV-1 vector. The vector is shown in the proviral DNA form and has been previously described (25). (B) Protocol for one cycle of HIV-1 vector replication. The steps going from a parental shuttle vector provirus in the step 2 cell to a vector provirus in the step 3 cell constitute a single cycle of replication. LTR, long terminal repeat; SV, simian virus 40; ampho MLV, amphotropic murine leukemia virus.

Cell culture, transfections, infections, and cocultivations. HeLa and COS-1 cells were maintained in Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% calf serum or 10%fetal bovine serum, respectively. HIV-1 vectors and expressionplasmids were transfected into COS-1 or HeLa cells by use of dimethylsulfoxide-Polybrene (27). HeLa cells were infected in the presenceof Polybrene. Infection of HeLa target cells was done by cocultivationof virus-producing cells with target cells (25). The 293T cellsused in the virion packaging assay were maintained in DMEM supplementedwith 10% fetal calf serum, and 25 mM HEPES was added during virusproduction. They were transfected with the 22-kDa polyethylenimine(Euromedex) as previously described (35).

Cell culture strategy used to generate a single cycle of HIV-1 replication. The experimental protocol developed to assay a single cycle of HIV-1 shuttle vector replication is shown in Fig. 1 (25).Step 2 clones were tested by Southern analysis to ensure thatonly a single vector proviral DNA was present. The lacZ $alpha$ peptidegene in the vector proviral DNA of step 2 clones was sequencedto confirm that no mutation wasintroduced.

Recovery of HIV-1 vector proviral DNA and sequence analysis of the lacZ $alpha$ peptide region. Purified genomic DNA from pools of step 3 clones was digested with the restriction enzymes StuI and XhoI to release the neo,pACYC origin of replication, and lacZ $alpha$ peptide gene sequencesfrom the HIV-1 vector. Proviral DNA was purified with the Lacrepressor protein as previously described (25). The ratio ofthe number of white plus light blue bacterial colonies to thetotal number of colonies observed provided the forward mutationrate for a single retroviral replication cycle. Plasmid DNA waspurified and sequenced in the lacZ $alpha$ peptide gene region by anautomated DNA sequencer (Applied Biosystems). Mutation rates werecalculated as previously described (25).

Yeast two-hybrid assay. The construction of the HIV-1 Vpr mutant library fused to the DNA-binding domain of the LexA repressor (LexABD) and the two-hybridscreening procedure of the library have already been described(34). Vectors for expression of wt Vpr or the Vpr*W54R and Vpr*R90Kvariants fused to LexABD were described previously (34), whilevectors for expression of UNG1, UNG2, and a truncated form ofUNG without the N-terminal part of the protein (UNG57/66) fusedto the Gal4 activation domain (Gal4AD) were constructed in thepGAD1318 plasmids (3). The L40 yeast strain was cotransformedwith the indicated LexABD and Gal4AD hybrid expression vectorsand plated on selective medium. Double transformants were thenassayed for $beta$ -galactosidase activity and histidine auxotrophyas previously described (34).

Analysis of Vpr and UNG incorporation into HIV-1 virions. Incorporation of Vpr and UNG was analyzed using a packaging assay in which Vpr and UNG were expressed in trans and incorporatedinto virions (35). The HIV-1-based packaging vectors pCMV $Delta$ R8.9(lacking the env and auxiliary genes) and pCMV $Delta$ R8.2 (lacking onlythe env gene) and the pMD.G plasmid for expression of the vesicularstomatitis virus G protein were kindly provided by D. Trono (Geneva,Switzerland) (53). Vectors for expression of wt or mutated Vprand UNG1, UNG2, and UNG57/66 fused to the epitope tag from theinfluenza virus hemagglutinin (HA) were constructed in pAS1B aspreviously described (35). For analysis of Vpr-dependent incorporationof UNG, cells were cotransfected with 10 µg of pCMV $Delta$ R8.9, 5 µgof pMD.G, 10 µg of pAS1B-UNG57/66, and the indicated amounts ofpAS1B-Vpr (wt or mutated). For incorporation analysis of the distinctUNG forms, cells were cotransfected with 10 µg of pCMV $Delta$ R8.2, 5µg of pMD.G, and 10 µg of either pAS1B-UNG1, -UNG2, or -UNG57/66.Cell culture supernatants were collected 48 h after transfectionand filtered through 0.45-µm-pore-size filters, and an aliquotwas assayed for CAp24 antigen. Virions were collected by ultracentrifugationfor 1 h at 100,000 × g and suspended in ice-cold lysis buffer(10 mM Tris [pH 7.6], 150 mM NaCl, 2 mM EDTA, 0.5% Triton X-100).For preparation of cell lysates, cells were trypsinized, collectedby centrifugation, and suspended in ice-cold lysis buffer. Celland virion lysates were incubated on ice for 5 min and clarifiedby centrifugation. The protein concentration of the cell lysateswas measured (Bio-Rad). Proteins from cell (50 µg of total protein)and virion (50 ng of CAp24) lysates were separated by sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and analyzedby Western blotting with anti-HA 3F10 (Boehringer) or anti-CAp24antibodies (39).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Replication of a vpr null mutant HIV-1 vector and genetic trans complementation with Vpr. The vpr null mutant HIV-1 vector (25) used in these studies was derived from the HIV-1 shuttle vector 3.12 (Fig. 1A). Inorder to complement this vpr null mutant HIV-1 vector, a plasmidexpressing wt Vpr or a Vpr variant was transiently transfectedalong with gag-pol and env expression plasmids (25). The HIV-1vector produced from either COS-1 or HeLa cells was used to infectfresh HeLa target cells (Fig. 1B). Cocultivation of mitomycinC-treated step 2 cells with fresh HeLa target cells to producestep 3 cells led to titers that were typically about 8 × 10² to 3 × 10³ CFU/2.5 × 10⁵ HeLa target cells. The steps going from a parental shuttle vectorprovirus in step 2 cells to a vector provirus in step 3 cellsconstitute a single cycle of replication (Fig. 1B). Southern analysisof total DNA from each step 2 cell clone was done to ensure thateach clone contained only one provirus copy (data not shown).Proviral DNA from at least 5 × 10⁵ cells of each step 2 cell clone was purified using the Lac repressorprotein and introduced into Escherichia coli to screen for mutationsin the lacZ $alpha$ generegion.

Vpr virion incorporation is required to influence the in vivo mutation rate. The virion incorporation of Vpr into HIV-1 particles requires direct interaction with the p6 region of the Gag precursor (1,35). In order to extend the observation that Vpr virion incorporationis required to influence the HIV-1 mutation rate, we used theassay described in Fig. 1B to compare the effects of Vpr transcomplementation on the mutation frequencies of vpr null mutantHIV-1 (expressing a wt gag gene) and p6 vpr null mutant HIV-1 (expressing a mutant gag gene lacking thep6-encoding region). As indicated in Table 1, complementationwith Vpr had no influence on the mutation rate of p6 vpr null mutant HIV-1 and resulted in an average mutation frequencycomparable to that of noncomplemented vpr null mutant HIV-1 (chisquare, 0.009; P >0.95) but significantly higher (chi square,20; P <0.01) than that of vpr null mutant HIV-1 complemented withVpr. Levels of Vpr expression were comparable in cells expressingthe wt and p6-truncated forms of the Gag precursor (data not shown).These data support the requirement of Vpr incorporation into virionsin order for Vpr to influence the HIV-1 mutation rate.

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TABLE 1. Incorporation of Vpr into virions is required to influence the mutation frequency of HIV-1 vectors^a

To test whether trans complementation of Vpr could be provided in the infected target cells rather than in the virus-producingcells, vpr null mutant HIV-1 was replicated with trans complementationof Vpr in step 3 target cells. Complementation of target cellswith Vpr resulted in a mutation frequency significantly higher(chi square, 15; P <0.01) than that observed by complementationin virus-producing cells and equivalent (chi square, 0.033; P>0.5) to the mutation frequency of noncomplemented vpr null mutantHIV-1 (Table 1). Expression of Vpr in target cells was comparableto that in the virus-producing cells (not shown). These data indicatethat trans complementation with Vpr in the target cells does notcomplement vpr null mutant HIV-1 in the mutation rate assay. Thisfurther supports the conclusion that Vpr virion incorporationis required to influence the HIV-1 mutationrate.

Vpr binding to UNG correlates with the influence on the HIV-1 in vivo mutation rate. In order to analyze the potential correlation between the Vpr influence on the HIV-1 mutation frequency and the interactionwith UNG, the effect of Vpr variants was analyzed in the mutationrate assay. We had previously reported that a single substitutionof the Trp residue in position 54 (Vpr*W54R variant) was sufficientto abolish binding to UNG but did not disrupt the Vpr-inducedG₂ arrest activity. These data demonstrated the critical roleof this residue in the maintenance of Vpr binding to UNG and indicatedthat this interaction is not involved in the perturbations ofthe cell cycle (34). The Vpr*R90K variant, containing a conservativesubstitution of Arg90 located in the C-terminal basic domain ofthe protein, was included in our analysis to study the relationshipbetween the G₂ arrest activity and the influence on the HIV-1mutation rate. This mutant interacted with UNG as efficientlyas wt Vpr but was unable to induce G₂ arrest in HeLa cells (34).

Vpr*W54R and Vpr*R90K were analyzed in parallel for their influence on the HIV-1 mutation rate. The vpr null mutant HIV-1vector was replicated in the absence of Vpr or trans complementedwith a wt Vpr, Vpr*W54R, or Vpr*R90K expression plasmid. The proviralDNA from pooled step 3 cells, representing over 50,000 differentclones for each experiment, was purified and introduced into E.coli to screen for mutations in the lacZ $alpha$ gene.

Three thousand seven hundred thirty-four bacterial colonies were screened in three replicates where vpr null mutant HIV-1was trans complemented with Vpr*W54R. Fifty-nine of these colonieshad a white or light blue colony color phenotype (Table 2). Theaverage mutation frequency in these experiments was 59 to 3,734or 0.016 mutation per cycle. The mutation frequency of vpr nullmutant HIV-1 complemented with Vpr*W54R was significantly differentfrom that found when it was complemented with wt Vpr (chi square,17; P <0.01) but not from the mutation frequency of noncomplementedvpr null mutant HIV-1 (chi-square, 0.4; P > 0.5). This indicatesthat expression of Vpr*W54R leads to a mutation frequency phenotypecomparable to that of vpr null mutant HIV-1 alone and thereforedoes not influence the in vivo mutation rate. Vpr*W54R interactedwith the Gag precursor (data not shown) and was incorporated intoHIV-1 particles as efficiently as wt Vpr (see Fig. 3C and reference35), indicating that the mutation frequency phenotype of Vpr*W54Rwas not related to inefficient virion incorporation.

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TABLE 2. Mutation frequency in recovered proviruses of vpr null mutant HIV-1 complemented in trans with Vpr variants with differential binding to UNG^a

Three thousand two hundred eighty-two bacterial colonies were screened in three replicates where vpr null mutant HIV-1 wascomplemented with Vpr*R90K. Twenty-two of these colonies had awhite or light blue colony color phenotype (Table 2). The averagemutation frequency was thus 22 to 3,282 or 0.007 mutation percycle. The mutation frequency of vpr null mutant HIV-1 complementedwith Vpr*R90K was not significantly different from that of vprnull mutant HIV-1 complemented with wt Vpr (chi square, 0.02;P >0.5) but was significantly different from the mutation frequencyof noncom- plemented vpr null mutant HIV-1 (chi square, 15; P< 0.01). We have previously shown that Vpr*R90K bound to the Gagprecursor and was efficiently incorporated into HIV-1 particles(35). These results indicate that the expression of Vpr*R90Kinfluences the in vivo mutation rate in a manner comparable tothat of wt Vpr. Since Vpr*R90K completely fails to induce a G₂arrest (34), they indicate that the effects of Vpr on the cellcycle are genetically separable from those on the reverse transcriptionprocess.

Complementation of vpr mutant HIV-1 with a Vpr*W54R UNG binding-deficient mutant protein leads to a mutation phenotype similar to that observed with vpr null mutant HIV-1 alone. In order to compare the mutation phenotype of vpr mutant HIV-1 complemented with Vpr*W54R to that of noncomplemented vpr nullmutant HIV-1, the types of mutations that led to the white orlight blue colony color phenotype were determined by DNA sequencingof the lacZ $alpha$ gene (Fig. 2). Twenty (34%) of the 59 mutants sequencedfrom vpr null mutant HIV-1 complemented with Vpr*W54R had a singleG-to-A base pair transition mutation, which was the predominantsubstitution observed. This percentage is comparable to what wasobserved for single G-to-A substitution mutations in vpr nullmutant HIV-1 alone (11 [37%] of 30). Six hypermutants that eachcontained multiple mutations were observed for vpr null mutantHIV-1 complemented with Vpr*W54R (Fig. 2), and five of them containedat least one G-to-A transition. Therefore, 25 (44%) of the 59mutants sequenced for vpr null mutant HIV-1 complemented withVpr*W54R had G-to-A mutations. In comparison, two hypermutants(Fig. 2) were observed for vpr null mutant HIV-1 alone and bothhad at least one G-to-A mutation, indicating that 13 (43%) ofthe 30 mutants had G-to-A mutations. These data indicate thatthe rates of G-to-A mutation in both vpr null mutant HIV-1 complementedwith Vpr*W54R and vpr null mutant HIV-1 alone are comparable andthree- to fourfold higher than that of vpr null mutant HIV-1 complementedwith wt Vpr (data not shown).

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FIG. 2. Plus strand nucleotide sequence of the lacZ $alpha$ gene region in a vpr null mutant HIV-1 vector complemented with Vpr*W54R. The start for nucleotide numbering is the beginning of the 5' long terminal repeat of the HIV-1 vector. The locations of base substitution, frameshift, and deletion mutations in vpr null mutant HIV-1 vectors from parallel experiments that were complemented with Vpr*W54R or noncomplemented are shown above and below the nucleotide sequence, respectively. The start and stop codons of the lacZ $alpha$ open reading frame and the lac operator sequence are boxed. Nucleotide positions of base pair substitutions (letters above or below the sequence), +1 frameshifts (letters with $black-down-triangle$ ), $-$ 1 frameshifts ( $down-triangle$ ) and deletions (solid black lines with arrows and adjacent to the deletion names) are indicated. Mutations from the same mutant are designated with a Greek letter adjacent to each mutation; identical Greek letters indicate mutations from the same mutant.

C-to-T transition mutations were the second most common type of mutation detected for both vpr null mutant HIV-1 complementedwith Vpr*W54R and vpr null mutant HIV-1 alone (Fig. 2). For vprnull mutant HIV-1 complemented with Vpr*W54R, 10 (17%) of 59 mutantscontained a single C-to-T mutation. Two of the six hypermutantshad one C-to-T transition, for a total of 12 (20%) of 59 mutantshaving C-to-T transitions. For vpr null mutant HIV-1 alone, 6(20%) of 30 mutants had single C-to-T transitions, both hypermutantshad C-to-T transitions, and thus a total of 8 (27%) of the 30mutants had C-to-T transitions. This indicates that the ratesof C-to-T transitions are similar for both vpr null mutant HIV-1complemented with Vpr*W54R and vpr null mutant HIV-1 alone andare over twofold higher than that of vpr null mutant HIV-1 complementedwith wt Vpr (data notshown).

Single frameshift mutations as an entire group of mutations (but primarily $-$ 1 or +1 frameshifts in runs of T's and A's) wereidentified in 14 (24%) of 59 mutants for vpr null mutant HIV-1complemented with Vpr*W54R, and 8 (27%) of 30 for vpr null mutantHIV-1 alone. One hypermutant from vpr null mutant HIV-1 complementedwith Vpr*W54R had two $-$ 1 frameshifts in runs of A's. The ratesof frameshift mutations observed for vpr null mutant HIV-1 complementedwith Vpr*W54R and for vpr null mutant HIV-1 alone are comparableto what was observed in vpr null mutant HIV-1 complemented withwt Vpr (not shown). Similarly, the rates of deletion mutationsdetected for both vpr null mutant HIV-1 complemented with Vpr*W54R(1 [2%] of 59) and for vpr null mutant HIV-1 alone (1 [3%] of30) are comparable to that observed in vpr null mutant HIV-1 complementedwith wt Vpr (not shown). These data confirm that these two typesof mutations are not influenced by expression of Vpr (25).

Based upon the characterization of the types of mutations that occurred, the calculated in vivo mutation rate for vpr nullmutant HIV-1 complemented with Vpr*W54R is 13 × 10⁵ mutation per target base pair per cycle, which is fourfold higherthan that of vpr null mutant HIV-1 complemented with wtVpr.

UNG is recruited into HIV-1 particles through Vpr incorporation. Since virion incorporation of Vpr is required to influence the in vivo mutation rate, we have explored whether UNG could berecruited into virus particles. Incorporation into virions wasanalyzed using a packaging assay in which UNG fused to the HAepitope (HA-tagged UNG) was expressed in trans in virus-producingcells (35). We first analyzed the incorporation of a truncatedform of UNG containing a deletion of the N-terminal part of theprotein (UNG $Delta$ 57/66) because it corresponded to the UNG clone initiallyisolated in the two-hybrid screening performed to identify Vpr-interactingproteins (3). 293T cells were transfected with the HA-taggedUNG expression vector in combination with a HIV-1-based packagingvector (pCMV $Delta$ R8.2) containing an intact vpr gene (53), and thevirion- and cell-associated UNG was then assessed by Western blotanalysis using an anti-HA monoclonal antibody (MAb) (Fig. 3A).The HA-tagged version of UNG57/66 was detected in the supernatantof transfected cells (lower panel), indicating that it is incorporatedinto virions. To determine if the recruitment of UNG into virionsis dependent on Vpr incorporation, we used the same virion packagingassay described above but HA-tagged Vpr and UNG57/66 were bothexpressed in trans in virus-producing cells transfected with aHIV-1 packaging vector lacking the auxiliary genes (pCMV $Delta$ R8.9).Parallel experiments were performed in which 293T cells were cotransfectedwith pCMV $Delta$ R8.9 and a constant amount of the HA-tagged UNG57/66expression vector, in combination with increasing amounts of theHA-tagged Vpr vector. The virion- and cell-associated UNG andVpr were then assessed by Western blot analysis with the anti-HAMAb (Fig. 3B). No HA-UNG57/66 was detected in virions when Vprwas not expressed in virus-producing cells, indicating that UNGis incorporated in a Vpr-dependent manner. In contrast, UNG57/66was found in virions when the amount of Vpr expressed in cellswas increased. Both HA-Vpr and UNG were simultaneously detectedin a range of 10 to 20 µg of Vpr plasmid that was transfectedinto cells. The same blots were probed with an anti-CAp24 MAbto verify that similar amounts of virions were produced in allof the transfections. These results demonstrate that Vpr incorporationis required to recruit UNG into HIV-1 particles.

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FIG. 3. Vpr-dependent recruitment of UNG into HIV-1 particles. (A) Virion incorporation of UNG57/66. 293T cells were cotransfected with pCMV $Delta$ R8.2 (containing an intact vpr gene), pMD.G, and either pAS1B-UNG57/66 (+) or pAS1B without an insert ( $-$ ). (B) Vpr dose-dependent incorporation of UNG. Cells were cotransfected with pCMV $Delta$ R8.9 (lacking vpr) and pMD.G in combination with 10 µg of pAS1B-UNG57/66 and the indicated increasing amounts of pAS1B-Vprwt. NT, nontransfected cells. (C) Failure of Vpr*W54R to recruit UNG into virions. Cells were cotransfected with pCMV $Delta$ R8.9 and pMD.G with or without 10 µg of pAS1B-UNG57/66 in combination with 20 µg of either pAS1B-Vprwt, pAS1B-Vpr*W54R, or pAS1B without an insert ( $-$ ). Proteins from cell and virion lysates were separated by SDS-PAGE and analyzed by Western blotting with anti-HA (cells and virions, upper panels) or anti-CAp24 (cells and virions, lower panels) antibody.

We then analyzed whether the mutation frequency phenotype of the Vpr*W54R UNG binding-deficient variant was related to a defectin UNG incorporation into virions. Cells were thus transfectedwith pCMV $Delta$ R8.9 and the HA-tagged UNG57/66 expression vectors,in combination with the HA-tagged wt Vpr or Vpr*W54R expressionplasmid (Fig. 3C). As previously, UNG57/66 was detectable in virionsonly when wt Vpr was coexpressed in virus-producing cells, andboth UNG and wt Vpr were thus incorporated. In contrast, no UNGwas detected in virions produced from cells expressing high levelsof Vpr*W54R, even though this variant was incorporated as efficientlyas wt Vpr. These data demonstrate that a UNG binding-deficientVpr variant does not recruit UNG into virions, suggesting thatthe mutation frequency phenotype of Vpr*W54R results from itsinability to allow the recruitment of UNG into HIV-1particles.

The nuclear form of UNG is preferentially incorporated into HIV-1 particles. Since UNG exists as mitochondrial (UNG1) and nuclear (UNG2) isoforms whose N-terminal sequences differ (see Fig. 4A), we haveexplored whether both forms of UNG could be recruited into virions.Each of these UNG forms fused to Gal4AD bound to LexABD-Vpr asefficiently as did UNG57/66 in a yeast two-hybrid assay (Fig.4A), confirming that the N-terminal portions of UNG1 and UNG2do not influence Vpr binding. The incorporation of UNG1 and UNG2into virions was analyzed by transfection of 293T cells with theHIV-1 pCMV $Delta$ R8.2 vector and the HA-tagged UNG1, UNG2, or UNG57/66expression vector. Virion- and cell-associated UNGs were thenassessed by Western blot analysis using the anti-HA MAb (Fig.4B). UNG2 and UNG57/66 were efficiently incorporated into virions,since the HA-tagged version of each form was detected in the supernatantsof transfected cells (lower panel). In contrast, mitochondrialUNG1 was not incorporated into virions despite detectable levelof the protein in transfected cell lysate (upper panel). UNG2was incorporated in a Vpr-dependent manner, since it was detectedin virions when 293T cells were transfected with pCMV $Delta$ R8.2 butnot when cells were transfected with pCMV $Delta$ R8.9 lacking the vprgene (Fig. 4C). These results indicate that nuclear UNG2 is thepreferential form incorporated into HIV-1 particles.

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FIG. 4. Preferential incorporation of nuclear UNG2 into HIV-1 virions. (A) Cellular distribution and Vpr binding of UNG1, UNG2, and UNG57/66. UNG1 and UNG2 have 35 and 44 unique N-terminal aa, respectively, while the C-terminal 269 aa are identical. Cellular distribution was analyzed by indirect immunofluorescence assay of 293T cells transfected with plasmid pAS1B-UNG1, -UNG2, or -UNG57/66. Vpr binding was determined in a two-hybrid assay of L40 yeast cells expressing the LexABD-Vprwt hybrid and either UNG1, UNG2, or the UNG57/66 Gal4AD hybrid. mitochon., mitochondria; nucl., nucleus; cytos., cytoplasm. (B) Virion incorporation analysis of the two UNG forms. 293T cells were cotransfected with pCMV $Delta$ R8.2, pMD.G, and either plasmid pAS1B-UNG1, -UNG2, or -UNG57/66. (C) Vpr-dependent incorporation of UNG2 into virions. 293T cells were cotransfected with pMD.G, pAS1B-UNG2, and either plasmid pCMV $Delta$ R8.2 or pCMV $Delta$ R8.9. In panels B and C, proteins from cell and virion lysates were separated by SDS-PAGE and analyzed by Western blotting with anti-HA (cells and virions, upper panels) or anti-CAp24 (cells and virions, lower panels) antibody.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This work focused on the functional characterization of the interaction of HIV-1 Vpr with UNG, a cellular protein that isimplicated in the DNA repair process. The results indicate thecontribution of the binding of Vpr to UNG to the in vivo mutationrate of HIV-1. Further data are presented which show that theVpr recruitment of the nuclear form of UNG into HIV-1 particlesis required for Vpr to influence the in vivo mutation rate. Thecorrelation between the capacity of Vpr to interact with UNG andits ability to both influence the HIV-1 mutation rate and mediatevirion packaging of UNG supports this conclusion. In contrast,Vpr binding to HHR23A, the other Vpr-interacting DNA repair protein,does not correlate with the influence of Vpr on the mutation rate(L.M.M. and S.B., unpublishedresults).

Two Vpr variants were tested for their influence on the in vivo mutation rate of HIV-1 in order to assess whether the interactionof Vpr with the DNA repair protein UNG could be correlated withthe influence of Vpr on the mutation rate. The Vpr*W54R variantdoes not bind UNG, does interact with the Gag precursor, is efficientlyincorporated into virus particles, and causes cell cycle arrest.This indicates that Vpr*W54R displays a wt phenotype, with theexception of its inability to bind UNG. When Vpr*W54R was usedfor trans complementation of vpr null mutant HIV-1 in a singlecycle of replication, it was found that the rate of mutation wascomparable to that of noncomplemented vpr null mutant HIV-1 alone.In addition, vpr null mutant HIV-1 complemented with Vpr*W54Rhad a spectrum of mutations similar to that of noncomplementedvpr null mutant HIV-1. This provides genetic evidence in supportof the conclusion that the inability of Vpr*W54R to interact withUNG influences the in vivo mutation rate of HIV-1. In contrast,Vpr*R90K influences the in vivo mutation rate in a manner comparableto that of wt Vpr but completely fails to induce a G₂ arrest (34).Therefore, the Vpr effects on the cell cycle are genetically separablefrom those on the HIV-1 mutation rate since they are related todistinct regions of Vpr. Alpha-helical region II of the proteincontributes to reverse transcription accuracy, while the C-terminalbasic domain is crucial for the G₂ arrest activity (8, 52).

The absence of UNG in HIV-1 particles that have efficiently incorporated Vpr*W54R indicates that the failure of Vpr*W54R tointeract with UNG not only prevents virion incorporation of UNGbut also affects the influence of Vpr on the HIV-1 mutation rate.The Vpr dose dependence for incorporation of UNG into HIV-1 particlesalso provides evidence for a Vpr-specific mechanism of UNG incorporation.These observations indicate that for Vpr to influence the in vivomutation rate of HIV-1, both Vpr and UNG must be efficiently incorporatedinto HIV-1 particles. Nuclear UNG2 is the predominant form ofUNG that is incorporated into virions, whereas the mitochondrialUNG1 form is not efficiently incorporated. Like UNG2 (28), HIV-1Vpr displays evident karyophilic properties (15, 31, 46),suggesting that the Vpr-UNG2 complex takes place in the nucleiof infected cells, migrates to the cytoplasm, and then is incorporatedinto virions through the interaction of Vpr with the Gag precursorprotein. The inability of Vpr*W54R to mediate UNG incorporationis not related to a defect of nuclear import of this Vpr variant,since it localizes to the nucleus as efficiently as the wt protein(not shown). Alternatively, the Vpr-UNG2 complex could be formedin the cytoplasm and targeted to the plasma membrane before nuclearimport of both Vpr and UNG2. Since the Trp54 residue located inC-terminal alpha-helical region II of Vpr is crucial for the maintenanceof UNG binding (34), it appears that Vpr may also simultaneouslyinteract with the Gag precursor through N-terminal alpha-helicalregion I (8, 23, 35, 50). In contrast, the UNG1 formsequestered into mitochondria fails to access the core of HIV-1virions although it displays the ability to physically interactwith Vpr. It was recently reported that UNG was detected in HIV-1virions in the absence of Vpr, requiring the presence of the viralintegrase protein when Vpr is absent for UNG incorporation (48).Determination of UNG incorporation with a Vpr mutant that wasdeficient in UNG binding but was efficiently incorporated intoHIV-1 particles was not analyzed in this study. Our data indicatethat when Vpr is not present in HIV-1 particles, there is no detectableUNG incorporation. While we cannot formally exclude the possibilitythat integrase also contributes to UNG incorporation in the virionpackaging assay used in the present study, our results suggestthat the interaction of UNG with Vpr is the major pathway forUNG incorporation into HIV-1particles.

The observation that Vpr binding to UNG correlates with the in vivo mutation rate of HIV-1 implies a role for UNG in the accuracyof the reverse transcription process. UNG functions in cells asa DNA repair enzyme that specifically removes from DNA the RNAbase uracil, which appears by misincorporation during DNA synthesiswhen the dUTP pool is high or by cytosine deamination of dCMP.When cytosine deamination occurs, the result is a C-to-T transitionmutation in that DNA strand and a G-to-A transition in the oppositestrand in the next round of replication. The data presented inFig. 2 indicate that the predominant types of mutations detectedin vpr null mutant HIV-1 both alone and trans complemented withVpr*W54R were G-to-A and C-to-T transition mutations. Based uponwhat is known of UNG function, a G-to-A transition mutation inthe HIV-1 plus-strand DNA, in the absence of functional UNG activity,could be an indication of cytosine deamination in the minus strandDNA made during reverse transcription. In the presence of UNGactivity, the uracil created by cytosine deamination would bein the DNA strand of a DNA-RNA hybrid, assuming that the cytosinedeamination occurred during the minus strand DNA synthesis stepof reverse transcription. Little is known regarding the functionof UNG in removing uracil from DNA that is in a DNA-RNA hybrid.The presence in HIV-1 particles of other repair enzymes whichparticipate in the uracil excision repair pathway could help tosupport the specific role in virion packaging of UNG and the HIV-1mutation rate. However, we failed to detect in HIV-1 virions theapurinic/apyrimidinic (AP) endonuclease (known as HAP, APEX, orRef-1), the second enzyme involved in this pathway (19), suggestingthat the other enzymes are recruited after viral entry into thetarget cells. Although the data presented here indicate that UNGenzymatic activity directly influences the HIV-1 mutation rate,UNG may also influence the mutation rate by other mechanisms,such as modulation of the access of deoxynucleoside triphosphatesto reverse transcriptase or interaction of the Vpr-UNG complexwith the reverse transcriptase to influence its enzymaticfidelity.

Most nonprimate lentiviruses are known to encode and package into virus particles a dUTPase, an enzyme that regulates thelevels of dUTP in cells and therefore influences the potentialmisincorporation of uracil into viral DNA (9, 20, 21, 38,43-45). Replication of nonprimate lentiviruses that lack functionaldUTPase activity leads to misincorporation of uracil into viralDNA, a reduced level of replication in macrophages (i.e., nondividingcells), and an increased level of G-to-A transition mutations.The inhibition of dUTPase activity leading to an increased levelof G-to-A transitions appears to have a phenotype similar to thatof vpr null mutant HIV-1 or vpr null mutant HIV-1 trans complementedwith Vpr*W54R in the mutation rate assay. Both primate and nonprimatelentiviruses have the ability to replicate in nondividing cells,which are presumed to have low levels of S-phase cellular enzymesinvolved in DNA synthesis and repair, such as dUTPase and UNG(19, 29, 37). The encoding of dUTPase by nonprimate lentivirusesand the incorporation of UNG by primate lentiviruses such as HIV-1by its interaction with Vpr support the hypothesis that thesedifferent mechanisms evolved in order for these viruses to removeuracil from their DNA when replicating in nondividingcells.

	ACKNOWLEDGMENTS

We thank L. Bernard and R. Casseron for outstanding technical assistance and D. Trono and the National Institutes of HealthAIDS Reagent Program for the kind gift of various reagents. Wealso thank M. Emerman for stimulating conversations and M. Williamsfor comments on themanuscript.

This work was supported by grant GM 56615 from the Public Health Service (to L.M.M.), by the French National Agency for AIDSResearch (R.B.), and by SIDACTION (S.B.).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Virology, Immunology, and Medical Genetics, 2078 Graves Hall,333 West 10th Ave., Columbus, OH 43210. Phone: (614) 292-5525.Fax: (614) 292-9805. E-mail: mansky.3{at}osu.edu.

Present address: Hybrigenics, Inc., Paris,France.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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Hu, W.-S., Pathak, V. K. (2000). Design of Retroviral Vectors and Helper Cells for Gene Therapy. Pharmacol. Rev. 52: 493-512 [Abstract] [Full Text]
Mansky, L. M. (2000). In Vivo Analysis of Human T-Cell Leukemia Virus Type 1 Reverse Transcription Accuracy. J. Virol. 74: 9525-9531 [Abstract] [Full Text]
Mansky, L. M., Bernard, L. C. (2000). 3'-Azido-3'-Deoxythymidine (AZT) and AZT-Resistant Reverse Transcriptase Can Increase the In Vivo Mutation Rate of Human Immunodeficiency Virus Type 1. J. Virol. 74: 9532-9539 [Abstract] [Full Text]

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