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Journal of Virology, January 2001, p. 45-51, Vol. 75, No. 1
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.1.45-51.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Pseudopackaging of Adenovirus Type 5 Genomes into
Capsids Containing the Hexon Proteins of Adenovirus Serotypes B, D,
or E
Philomena
Ostapchuk and
Patrick
Hearing*
Department of Molecular Genetics and
Microbiology, School of Medicine, State University of New York at
Stony Brook, Stony Brook, New York 11794-5222
Received 19 July 2000/Accepted 25 September 2000
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ABSTRACT |
Adenoviruses (Ad) show promise as a vector system for gene delivery
in vivo. However, a major challenge in the development of Ad vectors is
the circumvention of the host immune responses to Ad infection,
including both the host cytotoxic T-cell response and the humoral
response resulting in neutralizing antibodies. One method to circumvent
the effect of neutralizing antibodies against an Ad vector is to use
different Ad serotypes to deliver the transgene of interest. This
approach has been demonstrated with Ad genomes of highly related
members of subgroup C. However, it is not known whether an Ad5-based
vector DNA molecule can be packaged into capsids of evolutionarily more
divergent adenoviruses. The aim of these studies was to determine if
capsids containing hexon proteins from other Ad subgroups could package
the Ad5 genome. A genetic approach utilizing an Ad5
temperature-sensitive (ts) mutant with a mutation in the
hexon protein was used. When grown at the nonpermissive temperature,
Ad5 ts147 replicates normally, providing a source of Ad5
DNA for virus assembly, but does not produce virus particles due to the
hexon protein mutation. Coinfection of Ad5 ts147 with a
wild-type virus of other Ad serotypes (Ad3, Ad4, or Ad9), which supply
functional hexon proteins, resulted in the pseudopackaging of the Ad5
DNA genome. Furthermore, the pseudopackaged Ad5 DNA virions obtained in
the coinfections were infectious. Therefore, switching hexons did not
impair the infectivity or uncoating process of the pseudopackaged
virion. Since hexon protein is a major antigenic determinant of the Ad
capsid, this approach may prove useful to reduce the antigenicity of
therapeutic Ad vectors and allow repeated vector administration.
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INTRODUCTION |
Considerable progress has been made
toward the development of viral vectors for the short- and long-term
treatment of disease by gene therapy. Adenoviruses (Ad) show promise as
a vector system for gene delivery in vivo for a number of reasons
(3, 5, 26). Ad has a wide host cell range and infects both
dividing and nondividing cells in vitro and in vivo. Thus, it is
possible to transduce quiescent and differentiated cells with Ad to
direct the expression of a therapeutic gene. The Ad life cycle has been well characterized, its genome may be readily manipulated in the laboratory, and it is easily grown to high titers in cultured cells.
Finally, Ad is a relatively benign human virus that is associated with
mild disease and, importantly, is not associated with the development
of any human malignancy.
A major challenge in the development of Ad vectors for gene therapy,
however, is the circumvention of the host immune responses to viral
infection. The host cytotoxic T-cell response to antigens presented by
virus infection leads to clearance of Ad-infected cells and thus
significantly reduces the efficacy of the therapy. Experiments using
animal model systems including nonhuman primates have demonstrated that
both antigen-specific and nonspecific immune responses to Ad infection
extinguish the expression of a transgene included in the viral vector
(22, 43-45, 47). Furthermore, the humoral response of the
host to the initial virus inoculum is a significant barrier to
readministration of an Ad vector, which largely limits the utility of
the therapy to a single administration (6, 17, 22, 44,
48). Similarly, the results of analyses with human subjects
receiving Ad therapeutic vectors suggest that a critical factor which
determines the extent of the humoral response of the recipient to Ad
inoculation reflects the initial humoral immune state of the host
(8, 17). Neutralizing antibodies that prevent the Ad
vector from competently infecting its target cell pose a major problem
in obtaining a therapeutic effect of vector delivery.
Several different approaches have been tested to escape the limitations
set by the host immune response to Ad vectors. The host may be
targeted, for example, by oral tolerization (19) or
suppression of the immune response by blocking CD4+ T-cell
activation (20, 25, 46). The viral vector may be targeted,
for example, by physically masking the capsid from neutralizing antibodies by encapsidation in polyacid copolymers (2) or
covalently attaching a polymer of polyethylene glycol
(34). Alternatively, the effect of neutralizing antibodies
against an Ad gene therapy vector may be circumvented through transient
immunosuppression (4, 9-11, 21, 27) or by utilizing
different Ad serotypes to deliver the transgene of interest (23,
28, 29, 32). The latter approach may be accomplished through the
development of the genomes of many different Ad serotypes to carry a
transgene of interest or through the use of a single viral transgene
with encapsidation into the capsids of different Ad serotypes. This has
been demonstrated with an Ad5 genome packaged into an Ad2 capsid
(15, 35) and offers the facility of having a single vector
DNA backbone whose capsid immunogenicity may be changed by packaging
into alternative capsid structures. At present, this approach is
limited to the Ad5 and Ad2 serotypes, two very closely related viruses
of Ad subgroup C. It is not known whether an Ad5-based vector DNA
molecule could be packaged into a more divergent Ad capsid. The
necessity of having a wider distribution of Ad vectors from different
serotypes is further exemplified by epidemiological studies. One study
of a 10-year period from 1967 to 1976 showed that the absolute
distribution of antibodies in the worldwide population to the more than
49 serotypes of adenovirus in decreasing order was Ad2, Ad1, Ad7, Ad3,
Ad5, Ad6, Ad4, and Ad8, with antibodies against the other serotypes
being found on a much less frequent basis (40). Taken
together, these results demonstrate that a therapeutic Ad vector system
that permitted the exchange of the exterior capsid, and hence the
immunogenicity of the virus, with a single viral genome carrying a
transgene of interest would be very useful.
Most current Ad vectors are based on serotypes Ad5 and Ad2 because of
the extensive research with these viruses, including their genomic
sequences. Earlier attempts to exchange the hexon protein of an
Ad5-based vector with that of a more distantly related serotype, Ad7,
were unsuccessful (15). The authors suggested that
incompatibilities of the Ad7 hexon protein with other proteins of Ad5,
for example the 100-kDa protein (100K protein) which is involved in
hexon assembly and transport to the nucleus or other Ad capsid proteins
that interact with hexon in the virus particle, may explain these
results. We have tested if the Ad5 genome may be packaged into virus
particles that contain hexon proteins of another Ad serotype. Using
viruses that represent subtypes B (Ad3), D (Ad9), and E (Ad4), we
demonstrate that Ad5 DNA can be packaged in the capsids that contain
the hexons of more divergent subtypes. Since hexon is the major
antigenic component of the Ad capsid (14, 33), this
approach may prove useful to reduce the antigenicity of therapeutic Ad
vectors and allow repeated vector administration.
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MATERIALS AND METHODS |
Viruses and cells.
293 cells (16) and A549
cells (American Type Culture Collection) were maintained as monolayer
cultures in Dulbecco's modified Eagle's medium containing 10% bovine
calf serum and the antibiotics penicillin and streptomycin. Virus
stocks of Ad3, Ad5, Ad2, Ad4, and Ad9 (American Type Culture
Collection) were generated by infection of either 293 or A549 cells at
a multiplicity of infection of 200 particles/cell for 1 h at
37°C. Fresh medium was added, and the infected cells were maintained
at 37°C until the appearance of a cytopathic effect, usually ~72 h
postinfection. A stock of Ad5 ts147 (24) was
generated following infection of A549 cells by maintenance of the
infected cells at 32°C until the appearance of a cytopathic effect.
For the preparation of virions, infected cell lysates were prepared by
suspension of cells in Tris-buffered saline solution followed by three
freeze-thaw cycles and centrifugation at 3,000 × g at
4°C for 15 min. Purified virus particles were prepared by
centrifugation over a CsCl2 step gradient (1.4 to 1.25 g of CsCl2 per cc) and final purification on a
CsCl2 equilibrium gradient (1.33 of CsCl2 per
cc). Virus particles were quantified by measurement of absorbance at
260 nm, taking 1 optical density unit at 260 nm to be equivalent to
1012 particles.
For virus coinfection experiments, A549 cells were infected with Ad5
ts147 and the different wild-type Ad serotypes at 200 particle of each virus per cell for 1 h at 37°C, and the
cultures were then maintained at the nonpermissive temperature for Ad5 ts147 of 39.5°C for 60 to 72 h. Virus particles were
purified from coinfected cells as described above. Secondary infection of A549 cells with mixed populations of virus particles obtained from
primary coinfections of Ad5 ts147 with the different
wild-type Ad serotypes was performed at 1,000 particles per cell to
facilitate the detection of both the Ad5 ts147 and wild-type
genomes in the replication assay.
Determination of packaging efficiencies.
A Southern filter
hybridization assay was used to quantify the relative amounts of the
Ad5 ts147 and wild-type DNAs in the coinfection experiments.
Ad5 ts147 was distinguished from the wild-type viruses by
restriction enzyme digestion of the DNAs: SphI for Ad2 and
Ad9 or MluI for Ad3 and Ad4. The products were separated on
a 0.8% agarose gel with 1× TBE (90 mM Tris borate, 2 mM EDTA) and 0.5 µg of ethidium bromide per ml. The probe for hybridization was a
160-nucleotide (nt) PCR product extending from Ad5 nt 19839 to 19999 within a relatively conserved region of the hexon gene among the
different serotypes. The DNA probe was labeled using the AlkPhos Direct
labeling system from Amersham Life Sciences; this resulted in the
covalent attachment of alkaline phosphatase molecules to the DNA.
Filters from the hybridizations were incubated with a fluorescent
substrate for alkaline phosphatase, ATTOPHOS (JBL Scientific
Inc./Promega). The substrate yields a fluorescent product upon cleavage
by alkaline phosphatase, and the signals were imaged on a Storm 860 instrument (Molecular Dynamics) and quantified using Imagequant
software version 1.2 (Molecular Dynamics). A titer determination of Ad5
DNA was included in each experiment to ensure that the fluorescent
signals obtained were in the linear range of the assay. Since the DNAs
of different Ad serotypes have several nucleotide mismatches with the
Ad5 probe sequences, a correction factor for quantification of each
serotype was determined empirically by averaging the fluorescent
signals in several experiments from hybridization of the Ad5 probe to several concentrations of DNA from the other serotypes. The relative correction factor multiplied by the signal (minus background) equals
the corrected value for hybridization of the Ad5 probe to a different
serotype. The correction factors used in the calculations were as
follows: Ad5, 1; Ad2, 2.4; Ad3, 5.5; Ad4, 5.3; and Ad9, 4.7.
The packaging efficiencies of Ad5
ts147 in coinfections with
different wild-type Ad serotypes were determined by quantifying
the
relative amounts of packaged DNA isolated from purified virus
particles
in comparison to the relative amounts of total viral
nuclear DNA, as
described previously (
39). The replication ratio
is
expressed as the signal from the Ad5
ts147 DNA divided by
the
sum of the signals of viral DNAs of Ad5
ts147 and the
different
wild-type viruses in coinfections of A549 cells. Similarly,
the
packaged ratio is expressed as the signal from the Ad5
ts147 viral
DNA divided by the sum of the signals from viral
DNAs of Ad5
ts147
and the different wild-type viruses in
co-infections. The percent
packaging efficiency reflects the relative
level of Ad5
ts147
viral genomes packaged in a coinfection
relative to the amount
of Ad5
ts147 viral genomes
replicated. These results are expressed
as follows: percent packaging
efficiency = [(
ts147 packaged viral
DNA/total packaged
viral DNA)/(ts replicated DNA/total replicated
viral DNA)] × 100%.
Protein analyses.
Hexon protein monomers in virus particles
from single infections and coinfections were visualized by sodium
dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and
silver staining of proteins. Viral proteins from approximately 1 × 109 to 4 × 109 particles from the
coinfections and from 0.4 × 1010 to 2 × 1010 particles from single infections were solubilized in a
final concentration of 1× sample buffer (30 mM Tris [pH 6.8], 3%
SDS, 5% glycerol, 0.002% bromophenol blue, 5% 
-mercaptoethanol).
The proteins were separated by electrophoresis on an SDS-7.5%
polyacrylamide gel as described previously (37) and
stained with silver using an abbreviated version of the method of
Merril et al. (31). Briefly, proteins were fixed in the
polyacrylamide gel by incubation in 50% methanol-10% acetic acid
followed by successive incubation of the gel in 10% methanol-5%
acetic acid, 0.0326 mM dithiothreitol, and 12 mM silver nitrate. The
signal was developed by incubation in 2% potassium carbonate
containing 0.044% formaldehyde, and development of the staining was
stopped by incubation in 1% acetic acid.
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RESULTS |
A genetic approach was used to address whether an Ad5 DNA genome
could be packaged into the capsids of other, more divergent serotypes
of Ad. Specifically, we chose to examine whether the hexon protein, one
of the major serotype-specific antigenic determinants of Ad (14,
33), could be switched from Ad5 subtype C to other Ad subtypes
(B, D, or E). Ad5 packaging is of particular interest since this is the
major serotype of Ad used for the generation of Ad vectors for gene
therapy (3, 5, 26). We took advantage of Ad5 ts
mutants with mutations in the hexon protein. When grown at the
nonpermissive temperature, ts hexon mutants replicate
normally to provide a source of Ad5 DNA for virus assembly but do not
produce virus particles due to the hexon protein mutation
(24). We surmised that assembly of the Ad5 DNA genome into
infectious virus particles could occur by pseudopackaging, that is, the
packaging of Ad5 DNA into virus particles provided by coinfection with
a wild-type virus of another Ad serotype that would supply a functional
hexon protein. The hexon mutant used was Ad5 ts147
(24). At the permissive temperature of 32°C, this virus
grows to wild-type levels; at the nonpermissive temperature of
39.5°C, the infectious-virus yield of Ad5 ts147 is reduced
by 5 log units (24) and the virus does not make detectable
virus particles (data not shown) because the hexon protein synthesized
cannot be transported to the nucleus (24).
An assay was developed to distinguish the Ad5 ts147 DNA
genome from that of a coinfecting wild-type virus of another Ad
serotype in order to measure packaging efficiencies in coinfection
experiments. A quantifiable Southern blot assay was used. A series of
restriction endonucleases were tested empirically for their ability to
generate DNA fragments that distinguish the genomes of different Ad
serotypes. Viral DNA fragments were hybridized with a probe derived
from Ad5 that corresponds to a relatively conserved region of the hexon protein and cross-hybridizes with the genomes of different Ad serotypes. The mobilities of these diagnostic fragments on an agarose
gel are shown in Fig. 1. The genome of
Ad5 ts147 could be separated from that of wild-type Ad3 and
Ad4 by digestion of the DNAs with the restriction endonuclease
MluI. Similarly, Ad2 and Ad9 were separated from Ad5
ts147 by digestion with SphI. The relative
intensities of the hybridization signals from each Ad serotype in this
assay were used to normalize the efficiency of cross-reactivity of the
Ad5 DNA probe with the DNAs of the other Ad serotypes. These correction
values (see Materials and Methods) were used in subsequent experiments
to measure viral DNA replication and packaging efficiencies in
coinfections of cells with Ad5 ts147 and different wild-type
Ad serotypes.
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FIG. 1.
Diagnostic restriction endonuclease fragments of viral
DNAs from different Ad serotypes. Southern blot analysis was used to
distinguish viral DNAs of different Ad serotypes. Purified viral DNAs
were digested with MluI (lane 1, Ad3; lane 2, Ad4; lane 3, Ad5 ts147) or SphI (lane 4, Ad2; lane 5, Adts147;
lane 6, Ad9). The blot was hybridized with a 160-nt Ad5 probe
corresponding to coding sequences for hexon protein.
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A549 cells, a lung epithelial cell line permissive for infection by
different Ad serotypes, were coinfected with an equal number of
particles of Ad5 ts147 and either Ad3 (subgroup B), Ad4
(subgroup E), or Ad9 (subgroup D). Additionally, Ad5 ts147 was coinfected with Ad2, which is a member of the same subgroup, C. A549 cells were chosen for these analyses since the different Ad
serotypes under study all productively infect this cell line and
produce comparable levels of infectious virus particles on a per cell
basis. Infected cells were maintained at the nonpermissive temperature
(39.5°C) for the Ad5 ts147 mutant (24). At
this temperature, the wild-type viruses of different Ad serotypes were only moderately reduced (ca. two- to threefold) in yield when grown
individually, in comparison to the virus yields obtained at 37°C
(data not shown). After 3 days of infection, the entire cell population
was infected as judged by the complete cytopathic effect of the cell
monolayer cultures. Infected cells were collected, and a fraction of
the cells were used to isolate total nuclear DNA to examine the
replication levels of the coinfected viruses. Virus particles were
isolated from the remaining cells by CsCl2 equilibrium
centrifugation, and the relative packaging efficiencies of Ad5
ts147 in comparison to the different wild-type Ad serotypes were determined. The results of the Southern blot analysis of a
representative coinfection are shown in Fig.
2. The results of three independent
coinfection experiments were quantified and are presented in Table
1.
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FIG. 2.
Ad5 ts147 DNA is packaged into virions
containing hexon proteins of other Ad serotypes. Southern blot analysis
was used to quantify replicated and packaged viral DNAs from
coinfections of A549 cells with Ad5 ts147 and different
wild-type Ad serotypes. Lanes 1 to 5, dilution of Ad5 DNA (lane 1, 495 ng; lane 2, 158 ng; lane 3, 59 ng; lane 4, 20 ng; lane 5, 10 ng); lanes
6 and 11, Ad5 ts147 DNA digested with SphI or
MluI, respectively; lanes 7, 8, 12, and 13, replicated viral
DNAs present in total nuclear DNA isolated from cells coinfected with
Ad5 ts147 plus Ad2 (lane 7), Ad9 (lane 8), Ad3 (lane 12),
and Ad4 (lane 13); lanes 9, 10, 14, and 15, packaged viral DNAs present
in purified virus particles isolated from cells coinfected with Ad5
ts147 plus Ad2 (lane 9), Ad9 (lane 10), Ad3 (lane 14), and
Ad4 (lane 15). The asterisks indicate the Ad5 ts147 fragment
in each coinfection. replic., replicated; pack., packaged.
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As expected, replication of Ad5 ts147 at the restrictive
temperature of 39.5°C was readily detected (Fig. 2, lanes 6 and 11) in a single infection while no virus assembly was observed (data not
shown). In coinfection experiments, Ad5 ts147 and the
different wild-type Ad serotypes all replicated, although to somewhat
variable levels depending on the coinfecting viruses (lanes 7, 8, 12, and 13). Most importantly, the Ad5 ts147 genome was rescued
for packaging by coinfection with wild-type viruses of different Ad
serotypes (Fig. 2, lanes 9, 10, 14, and 15). The results of quantifying the relative levels of Ad5 ts147 genomes packaged with the
different wild-type viruses are shown in Table 1 (percent packaging
efficiency). Coinfection of Ad5 ts147 with the closely
related virus Ad2 resulted in efficient packaging of the Ad5 genome
(37% of Ad2 levels). Significant but less efficient packaging of Ad5
ts147 DNA was evident with the other Ad serotypes tested,
where a four- to ninefold reduction in packaged Ad5 ts147
DNA was observed with Ad3, Ad4, and Ad9 in comparison to coinfection
with Ad2. Thus, we conclude that the hexon proteins of Ad2, Ad3, Ad4,
and Ad9 provide the necessary functional properties to allow the
encapsidation of an Ad5 genome into virus particles.
The hexon proteins present in the virus particles obtained from
coinfection experiments were examined. The hexon composition of virus
particles obtained from two different coinfection experiments is shown
in Fig. 3. Hexon monomers of Ad5
ts147 may be separated from hexon monomers of Ad2, Ad3, Ad4,
and Ad9 by virtue of their different electrophoretic mobilities in
SDS-PAGE (Fig. 3, lane 4, Ad5 ts147, versus lanes 5 to 8, Ad2, Ad3, Ad4, and Ad9, respectively). In coinfections of Ad5
ts147 with Ad4 and Ad9, the hexon proteins found in virus
particles correspond to the hexon produced by the wild-type virus.
Lanes 1 to 4 show a dilution of Ad5 ts147 particles and the
resulting hexon protein signal detected by silver staining. In a
coinfection with Ad4 (Ad5 ts147 at 10% packaging
efficiency), we would anticipate an Ad5 ts147 hexon signal
similar to the intensity observed for 1.4 × 108
particles in the Ad5 dilution if the Ad5 ts147 hexon was
present in the purified virus particles. Similarly, in a coinfection
with Ad9 (Ad5 ts147 at 4.4% packaging efficiency), we would
anticipate an Ad5 ts147 hexon signal similar to the
intensity observed for 6 × 107 particles if the Ad5
ts147 hexon was present in the purified virus particles.
Clearly, no Ad5 ts147 hexon monomers were observed in the
particles isolated from the cells coinfected with Ad5 ts147 and either Ad4 or Ad9. Unexpectedly, the hexons from the viral particles obtained from coinfection with Ad5 ts147 and Ad2
were mixtures of Ad2 and Ad5 ts147 hexon proteins (lanes 9 and 13). Hexon protein bands of almost equivalent intensity for Ad2 and Ad5 ts147 were observed, suggesting that the defect in the
nuclear transport of the Ad5 ts147 hexon was rescued by
coinfection with Ad2. In coinfections of Ad5 ts147 with Ad3,
a band at the apparent mobility of Ad5 ts147 hexon was
apparent in purified virus particles (lanes 10 and 14); however, a band
of identical mobility was present in Ad3 particles isolated from a
single-virus infection as well (lane 6). In addition, there was no
apparent increase in the relative intensity of the faster-migrating
band seen in the particles from the coinfection with Ad3 compared to
the single infection (lane 6 versus lanes 10 and 14). In fact, the
relative intensity of this band appeared lower in the particles from
the coinfection with Ad3. Thus, we believe the presence of the Ad5
ts147 hexon in particles from coinfections with wild-type
Ad3 to be minimal or nonexistant. We conclude that Ad5 ts147
DNA is packaged into virus particles utilizing solely the hexon protein
of Ad3, Ad4, and Ad9.
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FIG. 3.
Analysis of hexon proteins in mixed virus particles
obtained from coinfection of A549 cells with Ad5 ts147 and
different wild-type Ad serotypes. Hexon protein present in purified
virus particles was analyzed by silver staining of viral proteins
separated by SDS-PAGE. Lanes 1 to 4, hexon protein from a dilution of
Ad5 ts147 particles (lane 1, 6 × 107
particles; lane 2, 2 × 108 particles; lane 3, 6 × 108 particles; lane 4, 2 × 109
particles); ts147 particles were produced in cells infected
at the permissive temperature of 32°C; lanes 5 to 8, hexon proteins
of different wild-type Ad serotypes; lanes 9 to 16, the results from
two experiments (Expt. 1 and Expt. 2) examining the hexon content of
mixed virus particles obtained from coinfection of A549 cells with Ad5
ts147 and Ad2 (lanes 9 and 13), Ad3 (lanes 10 and 14), Ad4
(lanes 11 and 15), or Ad9 (lanes 12 and 16).
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To determine if the Ad5 ts147 DNA-containing particles that
were pseudopackaged with the hexons of other Ad serotypes were infectious, A549 cells were infected with equal numbers of the mixed
particles obtained from each of the coinfection experiments. The
infectivity of the Ad5 ts147 pseudopackaged virions was
measured by Southern blot analysis of total nuclear DNA isolated at 6 and 48 h after infection (Fig. 4). A
6-h time point was used to attempt to detect input viral DNAs before
the onset of replication, but the signals were below the level of
detection (Fig. 4, lanes 1 to 4). In contrast, replicated viral DNA was
readily detected at the 48-h time point, indicative of virus infection
and genome amplification (lanes 5 to 8). The significant increase in
viral DNAs observed at the 48-h time point in comparison to the 6-h time point clearly demonstrates that the coinfecting viruses were infectious and replicated. Quantification of these results is shown in
Table 2. In each case, the relative
replication ratio of Ad5 ts147 in comparison to the
coinfecting wild-type viruses was very similar to those found in the
initial coinfection experiments (Table 1). These results demonstrate
that the pseudopackaged Ad5 ts147 viruses were infectious.
In summary, we conclude that Ad5 DNA can be packaged into virus
particles that contain the hexon proteins of other Ad serotypes and
that these particles are infectious.
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FIG. 4.
Pseudopackaged particles of Ad5 ts147 DNA are
infectious. Southern blot analysis was used to quantify the replication
of viruses recovered in the coinfections of A549 cells. Lanes 1 to 4, DNAs isolated 6 h postinfection from cells infected with mixed
particles from the Ad5 ts147 plus Ad2 (lane 1), Ad4 (lane
2), Ad3 (lane 3), or Ad9 (lane 4); lanes 5 to 8, DNAs isolated 48 h postinfection from cells infected with mixed particles from Ad5
ts147 plus Ad2 (lane 5), Ad4 (lane 6), Ad3 (lane 7), or Ad9
(lane 8). The asterisks indicate the Ad5 ts147 DNA
fragments.
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DISCUSSION |
A limitation of using Ad as a therapeutic vector for gene therapy
is the host immunological responses to the virus. One way of
circumventing a preexisting humoral immunity to a particular serotype
of Ad is to deliver the therapeutic viral genome in the capsid of a
different serotype that would not be neutralized by the antibodies
present. It has been shown previously that the genome of Ad5 can be
packaged in the capsid of Ad2 (15, 35). Ad5 and Ad2 are
evolutionarily very closely related viruses (1); both are
members of subgroup C. The aim of the experiments presented here was to
determine whether virus particles containing the hexons of Ads from
other subgroups are capable of packaging the Ad5 genome. Utilizing
representatives of subgenera B (Ad3) D (Ad9), and E (Ad4), our results
showed that, indeed, the Ad5 genome could be pseudopackaged into
capsids containing the hexons derived from viruses that are not members
of subgroup C, albeit at a lower efficiency. These results demonstrated
that there is no subgroup specificity for packaging of the Ad5 genome,
at least with regard to hexons from subgroups B, D, and E. That the
hexons can be switched may not be surprising, given the conservation of
the amino acid sequence across subtypes
79% (for hexon from a
subgroup D virus, Ad48) to 88% (for the subgroup C virus Ad5) of the
amino acids are identical to those of the Ad2 hexon. More than 99% of
the variability between the hexons of different Ad serotypes is
accounted for in seven hypervariable regions (12) that map
to the exterior of the protein and include the serotype-specific
epitopes (36).
There are at least 12 other proteins that contribute to the capsid
structure of the virion and several additional proteins that
participate temporarily in the assembly process (41). In the coinfections, all of these proteins were synthesized by both the
Ad5 ts147 and wild-type viruses of different serotypes,
except for hexon and possibly pVI. In addition to the mutation in the hexon gene of Ad5 ts147, growth of this virus at the
nonpermissive temperature results in reduced levels of pVI compared to
the levels seen with wild-type Ad (24). We do not know if
this reduction occurred in the coinfections as well, but if so, pVI,
which interacts with hexons, would be replaced by the pVI of the
coinfected wild-type virus in these experiments. It has been shown
previously that pVI from different subtypes of Ad, including nonprimate
Ads, can bind the hexon trimers of Ad2 (30). It would be
interesting to know if any of the other structural and nonstructural
proteins segregate in a subtype-specific fashion or if the subtype
source for the proteins in the capsids from these mixed infections is random. We examined the population of pentons from viruses obtained in
the coinfections; Ad3, Ad4, and Ad9 penton monomers can be distinguished from that of Ad5 penton by their different mobilities using SDS-PAGE. We observed pentons from both wild-type viruses of
different serotypes and Ad5 with the viruses obtained in the coinfection experiments (data not shown), demonstrating that the pentons of Ad5 can interact with the hexons of subgroups other than
subgroup C. Interestingly, Gall et al. (15) were unable to
generate an Ad5/Ad7 virus chimera that had the Ad5 hexon gene replaced
by the Ad7 hexon gene, although they could generate an Ad5 virus with
an Ad2 hexon replacement. Ad7 is a member of subgenus B. They surmised
that there may be an incompatibility of the Ad7 hexon in its
interaction with other Ad5 proteins, for example, the 100K protein. The
100K protein binds hexon and is involved in the trimerization and
nuclear translocation of hexons (7). The fact that the Ad5
genome was packaged into virus particles containing subtype B (Ad3)
hexons, when all other proteins of the subtype B were present, supports
their interpretation.
The subtypes used to provide the helper function in these experiments
are closer evolutionary relatives to subtype C than to subtypes A and F
(1). B and E are more closely related to each other than
to C, and D probably diverged in its evolution between the C and B
viruses (1). Not only are these viruses related by their
DNA sequences, but also viruses of subtypes B, C, D, and E all cause
ocular and respiratory infections (18). We were also
interested in determining if Ad5 genomes could be packaged in capsids
with the hexons from Ad subtypes less closely related to subtype C,
that is, from subgroups A and F. Consistent with the evolutionary
distance from Ad5, these viruses also have a different tropism, since
they infect cells of the gastrointestinal tract (18). We
attempted to use Ad12, a member of subgroup A, in pseudopackaging
experiments. Results from these experiments, however, were inconclusive
because Ad12 did not grow reproducibly in mixed infections of A549
cells with Ad5 ts147. We could not use Ad40 and Ad41 of
subgroup F in coinfection experiments in A549 cells since these viruses
do not grow well in established cell culture lines (42).
Packaging of the Ad genome occurs by recognition of packaging sequences
at the left end of the viral genome (38) and, presumably, by the incorporation of the DNA into a preformed viral capsid. At
present, no specific viral protein(s) has been conclusively identified
that directs the packaging event. However, many DNA viruses do require
a viral protein for initiating packaging (13), and it
seems likely that Ad is no exception. Furthermore, there may be a
cellular protein(s) involved in packaging, referred to as P complex
(39). This complex binds the packaging sequences of Ad5 in
a manner consistent with playing a role in the packaging process. It is
likely that the complex would bind the packaging sequences of Ad2,
which are virtually identical to those of Ad5 (Fig.
5). However, it is not known whether this
complex binds the equivalent packaging regions of Ad3, Ad4, and Ad9.
The fact that the Ad5 genome was pseudopackaged into capsids containing hexons from viruses of subgenera B, D, and E demonstrates that the
communication, whether direct or indirect, between the packaging factor(s) of Ad5 and the hexons from the different Ad serotypes was not
impaired. An alignment of the nucleotide sequences of the packaging
regions of the Ad genomes used in these experiments is shown in Fig. 5.
The A repeat elements identified in the genome of Ad5 that are crucial
for packaging include a conserved TTTG followed by 8 nt and a CG, as
indicated in the figure (38). There is strong conservation
of these sequences, particularly within the equivalent A5 and A6
repeats among the different subtypes, suggesting that these viruses may
use the same packaging factors.
View larger version (52K):
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|
FIG. 5.
Comparison of the nucleotide sequences of the packaging
regions of the different Ad serotypes. Shown are the nucleotides of the
packaging region of Ad5 (nt 242 to 386) and the equivalent regions of
Ad2, Ad3, Ad4, and Ad9. A1, A2, A5, and A6 refer to the A repeats
identified in Ad5 that are required for efficient packaging of the
viral DNA, with the conserved TTTGN8CG consensus indicated
in the dark boxes (where N is any nucleotide). Similarly conserved
sequences are also indicated in the nucleotide sequences of the other
serotypes.
|
|
The pseudopackaged Ad5 virions that were obtained in the coinfections
were infectious. These pseudopackaged Ad5 virions were infectious at a
level similar to the Ad5 ts147 genome packaged in virus
particles containing its own hexons. Therefore, switching hexons, and
possibly other structural proteins, does not impair the infectivity or
uncoating process of the pseudopackaged virion. These results
demonstrate that the Ad5 genome can be packaged not only within the
hexon coat of a virus from the same subgenera but also in a broad range
of viruses containing hexons from other subgenera as well. This expands
the possibilities for methods of evading the preexisting immunity of
the host when using Ad as a therapeutic vector. For this approach to be
feasible for the production of gene therapy vectors, inhibition of the
packaging of viral genomes of the wild-type viruses of different Ad
serotypes will be required. The Cre-Lox system (reviewed in reference
26) could be utilized to inhibit the packaging of
the genomes of different Ad serotypes while allowing the packaging of
an Ad5-based vector. This approach could be used to scale up the
production of pseudopackaged Ad vectors.
| |
ACKNOWLEDGMENTS |
We thank Ece Erturk, Jared Evans, Amy Ostrom, and Ziv Sandalon
for many helpful discussions and critical reviews of the manuscript. We
thank Gia Feeney for excellent technical assistance and Hamish Young
for generously providing Ad5 ts147.
This research was supported by Public Health Service grant AI41636.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Molecular Genetics and Microbiology, SUNY at Stony Brook, Stony Brook, NY 11794-5222. Phone: (631) 632-8813. Fax: (631) 632-8891. E-mail: phearing{at}ms.cc.sunysb.edu.
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Journal of Virology, January 2001, p. 45-51, Vol. 75, No. 1
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.1.45-51.2001
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Abstract
Introduction
