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Previous Article | Next Article 
Journal of Virology, November 1998, p. 8710-8717, Vol. 72, No. 11
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Infection of Ducklings with Virus Particles
Containing Linear Double-Stranded Duck Hepatitis B Virus DNA:
Illegitimate Replication and Reversion
Wengang
Yang and
Jesse
Summers*
Department of Molecular Genetics and
Microbiology, The University of New Mexico School of Medicine,
Albuquerque, New Mexico 87131
Received 13 May 1998/Accepted 14 August 1998
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ABSTRACT |
Double-stranded linear DNA is synthesized as a minor viral DNA
species by all hepadnaviruses. In a previous study (W. Yang and J. Summers, J. Virol. 69:4029-4036, 1995) we showed that virus particles containing linear DNA of the duck hepatitis B virus (DHBV)
could initiate an infection of primary duck hepatocytes. In cells
infected by linear DNA containing viruses the transcriptional template,
covalently closed circular DNA, was formed by circularization of linear
DNA by nonhomologous recombination between the two ends. This process
was shown to result in viral DNA replication through multiple
generations of linear DNA intermediates, a process we called
illegitimate replication. In this study we showed that viruses
containing linear DHBV DNA produced by engineered insertions in the r
sequence, which encodes the 5' end of the pregenome, could infect
hepatocytes in vivo, and these hepatocytes proceeded to carry out
illegitimate replication. Nonhomologous recombination quickly produced
revertants and partial revertants in which all or part of the insertion
was deleted. One such partial revertant that replicated primarily
through circular DNA intermediates, but which synthesized elevated
levels of linear DNA, could be sustained for several days as the
predominant genotype in vivo, but this mutant was eventually displaced
by variants showing full reversion to legitimate replication and that
synthesized normal low levels of linear DNA. Full revertants did not
necessarily contain the wild-type r sequence. The results suggest that
the linear DNA produced during DHBV infection initiates cycles of illegitimate replication by generating mutants with altered r sequences. Some r sequence mutants carry out a mixture of legitimate and illegitimate replication that can contribute to elevated production of linear DNA in individual cells.
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INTRODUCTION |
Hepadnaviruses are a family of small
DNA-containing viruses that replicate their genomes through reverse
transcription of RNA intermediates called pregenomes (5, 6, 17,
21, 23). The template for the transcription of pregenomic RNA is
nuclear covalently closed circular DNA (cccDNA) (17, 26, 28,
30). Pregenomic RNA is encapsidated in the cytoplasm and is used
as a template for the synthesis of a double-stranded circular form of
the genome, produced through a reverse transcription step. Capsids
containing double-stranded DNA, called relaxed circular DNA (rcDNA),
can be assembled into an envelope and secreted from the infected cell
as infectious virus or they can be transported to the nucleus, where
rcDNA is released and converted to additional cccDNA molecules
(10, 11, 25, 28, 30). An important feature of this
conversion is that all genomic information stored in the rcDNA is
precisely conserved in the resulting cccDNA molecule so that pregenomic
RNA transcribed from this cccDNA can direct the synthesis of progeny
rcDNAs that are genetically identical to their parental rcDNA molecule.
We have called this process, which occurs in every cycle of
hepadnavirus infection, legitimate replication (31) (Fig.
1A).
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FIG. 1.
Legitimate and illegitimate pathways of DHBV DNA
replication. (A) Legitimate replication occurs through transcription of
viral cccDNA to produce the RNA pregenome (RNA). Transcription
initiates at the 5' boundary (left boundary) of the 9-bp r sequence
(box), at nucleotide 2529, and after one circuit of the genome,
terminates around nucleotide 2800, so that the pregenome contains a 5'
copy and a 3' copy of r. Reverse transcription initiates at the 3'
boundary (right boundary) of the 3' r and proceeds to the 5' end of the
pregenome, producing a cDNA, ( )DNA, with terminal duplications of r.
Plus-strand DNA synthesis initiates at position 2491 on the ()DNA,
and elongation proceeds through r, causing circularization of the
genome through a template switch (rcDNA). rcDNA is converted to a
progeny copy of cccDNA that is identical to the parental copy. (B)
Illegitimate replication occurs through the same pathway, except rcDNA
is not formed. Instead, plus-strand synthesis is initiated near the 3'
end of ()DNA, producing a linear double-stranded DNA (linDNA). linDNA
is converted to cccDNA by nonhomologous recombination. The progeny
cccDNA is not identical to the parental molecule, as indicated by the
partially filled box. Please see reference 31 for
details.
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However, rcDNA is not the only double-stranded viral DNA synthesized in
the cytoplasm of an infected cell. The production of genome-sized
double-stranded viral linear DNA is observed in all natural
hepadnavirus infections (24, 27, 29). The mechanism underlying the linear DNA synthesis has been elucidated and is due to
the failure of a specific step in plus-strand synthesis, i.e., RNA
primer translocation from DR1 to DR2 (12, 13), a step
required for genome circularization. As a result of this failure,
plus-strand DNA synthesis is initiated in situ 19 nucleotides from the
3' end of the minus-strand DNA (15, 22). In situ priming
produces a double-stranded linear copy of the viral DNA, with nine
nucleotides of information repeated at each end (13). In
situ priming of plus-strand DNA occurs during DNA replication of
wild-type hepadnaviruses at a frequency of 5 to 10% of all plus
strands synthesized (22, 29, 31).
We previously found that double-stranded linear DNA-containing duck
hepatitis B virus (DHBV) (18) could infect primary duck hepatocyte cultures and deliver linear DNA molecules to the nucleus of
the infected hepatocytes, where cccDNA was formed as efficiently as
from rcDNA-containing virus (31). We found that cccDNA had been converted from the double-stranded linear DNA by means of nonhomologous recombination occurring preferentially around the two
ends of the linear DNA (Fig. 1B). Most cccDNAs formed by this mechanism
had lost one or more cis- or trans-acting
elements required for DNA replication; however, more than 10% could
participate in further DNA synthesis. In most of the molecules that
retained sufficient genetic information to produce progeny DNA,
alterations in the length or in the sequence of the r region of the
pregenomes that were transcribed resulted in the synthesis of a
higher-than-wild-type ratio of linear DNAs to rcDNAs. Thus, the
formation of cccDNA from linear DNA initiated a process in which linear
viral DNA production was favored, resulting in second and higher
generations of cccDNAs with complex multiple recombination joints
within the r region. We argued that, in theory, this process of DNA
replication was capable of producing unlimited generations of DNA
molecules, a subset of which contained r sequences that were able to
revert to the wild-type r sequence through subsequent generations of nonhomologous recombination. Since the precise sequence in a parental cccDNA was not conserved in its progeny cccDNA due to the step of
nonhomologous recombination, we called this mechanism for propagating DNA molecules "illegitimate replication." Because the rate of illegitimate replication is very low, the presence of illegitimate replication is obscured by the relatively higher levels of legitimate replication in natural infections. We speculated that the low levels of
replication inherent in illegitimate replication, however, might be
favored in some in vivo situations, e.g., in evading antigen-specific
cellular cytotoxicity.
In the livers of woodchucks chronically infected with the mammalian
hepadnavirus woodchuck hepatitis virus and undergoing a chronic
inflammatory reaction we found evidence that nonhomologous recombination of double-stranded linear DNA was responsible for the
formation of a significant fraction of cccDNA. In one infected liver at
least 10% of total cccDNA was apparently formed from linear
precursors. Sequence analysis predicted that some of these cccDNAs
would be functional for progeny linear DNA synthesis (32). Evidence for the occurrence of illegitimate replication through multiple generations of linear DNA, however, was not obtained. To date,
the fate of hepatocytes infected in vivo with linear DNA-containing
viruses has not been described due to the overwhelming level of
legitimate replication that occurs in the liver.
In this study we have examined the fate of hepatocytes infected in vivo
with linear DNA-containing viruses that mimicked the types of virus
that can arise during a natural infection, i.e., viruses that could
revert to wild type through nonhomologous recombination between the
ends of the linear DNA. Our results directly demonstrated that linear
DNA-containing viruses initiated an infection in vivo through the
production of cccDNA by nonhomologous recombination. Some of these
first-generation cccDNAs were used for subsequent generations of
illegitimate replication. Illegitimate replication also produced a
spectrum of cccDNAs that acquired the ability to carry out various
levels of legitimate replication, through rcDNA, yet at the same time
produced higher-than-wild-type levels of linear DNA in infected cells.
Variants showing complete reversion for legitimate replication also
occurred but these did not necessarily acquire the original wild-type r
sequence.
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MATERIALS AND METHODS |
Ducks.
One-day-old Pekin common hybrid ducks were purchased
from Metzer Farms (Redlands, Calif.). All ducks used for experimental infection were screened by dot blot hybridization of duck sera, and
DHBV DNA-negative ducks at an age of 3 to 5 days posthatch were
inoculated intravenously with virus particles containing DHBV wild-type
or mutant genomes.
Plasmid and mutations.
A plasmid expression vector,
pSPDHBV5.1(2X), containing EcoRI-linearized DHBV16 DNA
(16) cloned into the plasmid vector pSP65 as a head-to-tail
dimer was previously described (20). This plasmid was used
as the template in the site-directed mutagenesis described below. To
introduce an insertion in the r sequence, a procedure involving PCR and
a biotin-labeled primer was designed. The first PCR amplification
included a 5' end biotin-labeled plus-orientation (+) primer (DHBV
nucleotides 2217 to 2240) and a mutagenic minus-orientation () primer
(nucleotides 2544 to 2511) containing one of three specific insertions
in the nine-nucleotide r sequence. A high-fidelity DNA polymerase
Pwo (Boehringer Mannheim) was chosen for the amplification, in which about one error in a total of 5 kb of DNA could be detected by
sequencing of individual clones (data not shown). The resulting biotinylated (+) PCR product then was used as a megaprimer and annealed
with cloned DHBV DNA template cleaved with BamHI at DHBV nucleotide 1658. One cycle of elongation was carried out by
Pwo DNA polymerase, and the 5' end biotin-labeled
single-stranded DNA containing the engineered mutation was isolated by
absorbing the biotinylated DNA strand to streptavidin-coated M 280 Dynabeads (Dynal Corp.) and eluting nonbiotinylated DNA with alkali.
The remaining DNA was then used as a template for a final amplification (DHBV 2217 to 2240 and DHBV 70 to 45). The resulting PCR products were
cut with the restriction enzymes NcoI and NsiI,
and the 500-bp fragment was gel purified and exchanged into both copies
of the DHBV monomer in pSPDHBV5.1(2X). The region between
NcoI and NsiI in the plasmid was sequenced to
exclude possible secondary mutations. The plasmids containing the r
sequence mutations are shown in Fig. 2A.
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FIG. 2.
Insertion mutants of DHBV and the effects of the
insertions on rcDNA synthesis. (A) Top: map of the DHBV dimer in
pSPDHBV5.1(2×) showing two copies of the mutated r region. Bottom: the
mutations I1, I2, and I8 within the r sequence (underlined). The site
of initiation of pregenome transcription in cccDNA (top arrow) and the
site of minus-strand initiation at the 3' boundary of the downstream
copy of r (bottom arrow) in the wild-type pregenome are indicated. (B)
DHBV DNA extracted from enveloped virus particles in the culture medium
of LMH cells transfected with DHBV dimer plasmids containing the
indicated mutations. The migration positions of molecular size markers
are shown on the left (arrows). The two bands are indicated by RC
(rcDNA) and L (linear DNA).
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Transfections.
Transfection of the chicken hepatoma cell
line LMH (2, 8), isolation and assay of replicative
intermediates by Southern blot hybridization, and concentration and
assay of enveloped virus by the pronase-DNase I method were performed
as previously described (10, 11).
Analysis of viral DNA in sera.
Duck serum (50 µl) was
mixed with 150 µl of digestion solution containing a final
concentration of 10 mM EDTA, 1% sodium dodecyl sulfate (SDS), 0.1 M
NaCl, and 0.5 mg of Pronase/ml and incubated at 45°C for 2 h.
After phenol extraction, viral DNA was precipitated with ethanol and
analyzed by Southern blot hybridization.
Analysis of DHBV DNA replicative intermediates and cccDNAs in the
infected livers.
For viral DNA purification, 60 mg of liver tissue
was homogenized with 2 ml of ice-cold TE buffer (50 mM Tris-HCl [pH
8.0], 1 mM EDTA [pH 8.0]) with a loose-fitting plunger in a 7-ml
Dounce homogenizer. The homogenate then was equally divided into two parts. For purification of viral replicative intermediates, one part of
the homogenate was mixed with 50 µl of 10% Nonidet P-40 and
incubated on ice for 30 min and the nuclei and other debris were
removed by microcentrifugation. The supernatant was adjusted to a final
concentration of 10 mM EDTA-1% SDS-0.1 M NaCl-0.5 mg of Pronase/ml
and incubated at 37°C for 1 to 2 h. After phenol extraction, DNA
was recovered by ethanol precipitation and dissolved in TE (10 mM
Tris-HCl [pH 8.0], 1 mM EDTA [pH 8.0]), and the nucleic acid
concentrations were normalized by absorbance at 260 µm.
For viral cccDNA purification, the second portion of homogenate was
mixed with an equal volume of 4% SDS by vortexing. Cellular DNA,
proteins, and viral protein-bound DNAs were precipitated by the
addition of 0.5 ml of 2.5 M KCl. After centrifugation at 4°C for 10 min, the supernatant was removed and extracted with phenol. Viral DNA
was collected by ethanol precipitation and dissolved in TE (10 mM
Tris-HCl [pH 8.0], 1 mM EDTA [pH 8.0]). The total nucleic acid
concentration of each sample was normalized by absorbance at 260 µm.
Viral replicative intermediates and cccDNA from equal amounts of total
nucleic acids (usually 20 µg) were analyzed by 1.7% agarose gel
electrophoresis and Southern blot hybridization.
PCR amplification and sequencing.
A pair of primers
corresponding to DHBV16 DNA sequence 70 to 45 [() primer] and 2217 to 2240 [(+) primer] was used in all PCR amplification experiments
described in this study unless otherwise indicated (see Fig. 5C). Hot
start (2 min at 80°C before adding Mg2+-containing
buffer) was used in all PCR amplifications to decrease nonspecific
template binding. Amplification reactions consisted of a denaturation
step at 94°C for 1 min, annealing at 55°C for 2 min, and elongation
at 72°C for 3 min for 30 cycles with Taq DNA polymerase.
To construct a library, PCR products were diluted 100-fold in fresh
reaction buffer and subjected to two additional cycles of amplification
to eliminate heteroduplex molecules before being cloned. The
reamplified PCR products were cloned in the TA cloning vector pCRII and
transformed into Escherichia coli INV
F'. Colony screening
and sequencing were performed as previously described (32).
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RESULTS |
We previously showed that linear DNA-containing viruses could
initiate a cycle of replication through linear DNA intermediates in
primary duck hepatocytes. Because this process, which we called illegitimate replication, has potential consequences for infected cells
that differ from the consequences of legitimate replication, we wanted
to know if illegitimate replication also occurs in vivo and what the
fate of cells carrying out illegitimate replication in vivo would be.
In vivo, illegitimate replication would be difficult to detect because
it would contribute only a small fraction of the replicative
intermediates in the DNA extracted from a piece of liver tissue. To
circumvent this technical difficulty, we infected ducklings with high
titers of virus particles that contained mutant DNAs that mimicked the
type of DNAs that could be formed from linear DNA in a natural
infection. To produce these mutant genomes we inserted 1, 2, or 8 nucleotides into the r regions of a standard wild-type DHBV plasmid
expression vector to produce the mutants 1I, 2I, and 8I, respectively.
These insertion mutants resembled those that would occur in natural
infections in that they could be reverted to produce the wild-type
sequence by deleting the inserted nucleotides during nonhomologous
recombination. The structure of these mutant genomes is shown in Fig.
2A. As assayed by transfection of the plasmid expression vectors into
LMH cells, the various insertions were found to produce corresponding
defects in the production of rcDNA in favor of linear DNA in the
enveloped virus particles released from the transfected cells (Fig.
2B). The virus produced by transfection of these insertion mutant
plasmids was used for the infection of ducklings.
Infection initiated by linear DNA.
In order to determine if an
infection could be initiated in vivo by linear DNA-containing virus
particles, we assayed for the appearance of cccDNA in the livers of
ducklings after inoculation with the I8 mutant virus. As a negative
control for infection we tested whether the appearance of cccDNA was
dependent on the presence of the preS envelope protein. Finally, by
sequencing, we tested whether the structure of the cccDNA was
consistent with its having been formed by nonhomologous recombination
of the input linear DNA. To carry out this experiment, we modified the
I8 genome by introducing a second mutation (1165A) that destroyed the
ability of the expression vector to produce the large envelope protein, preS (26). The expression vector containing the
double-mutant genome, I8/1165A, was transfected into LMH cells in the
presence or absence of a preS expression vector, 
DR1 (4).
Particles were concentrated from the supernatants and inoculated into
six ducklings at 4 days posthatch. After 2 days, cccDNA was selectively extracted from the livers and assayed by PCR (Fig.
3A, left). Only those three ducklings
inoculated with enveloped virus particles contained cccDNA by this
assay. To determine if the cccDNA detected was derived from linear DNA
provided by the inoculated virus, direct sequencing through the r
region was performed on two of the samples (Fig. 3A, right). Only the
product from the duckling infected with enveloped virus particles
produced a sequence ladder, as expected. More importantly, the sequence
ladder showed a high degree of degeneracy beginning approximately at
the boundary of the r region, consistent with a population of cccDNA
molecules formed by nonhomologous recombinations at different sites.
This result indicated that linear DNA-containing virus particles had initiated an infection through the production of cccDNA by
nonhomologous recombination.
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FIG. 3.
Infection of ducklings with the I8 mutant virus. (A)
Specificity of the assay for infected hepatocytes. Supernatants from
LMH cells transfected with the DHBV I8/1165A plasmid, defective in preS
envelope protein, with and without an envelope expression vector
(DR1), were used to infect 4-day-old ducklings (1.3 × 109 and <106 enveloped viral genomes per bird,
respectively). The ducklings were sacrificed at day 2 postinfection,
and cccDNA was extracted from the livers and amplified by PCR (left
panel). Two samples were subjected to direct sequencing. (B) In a
parallel experiment, ducklings were infected with DHBV/I8 virus
containing a wild-type preS gene. Two ducklings were sacrificed at the
indicated times up to day 23 postinfection, and replicative
intermediates and cccDNA were extracted from their livers. Fractions
containing replicative intermediates (equivalent to 5 mg of liver
tissue from ducklings sacrificed up to day 8 postinfection) were
analyzed for viral DNA by agarose gel electrophoresis and blot
hybridization with a 32P-labeled riboprobe specific for
detection of the minus strand. (C) cccDNAs from the samples used for
panel B were subjected to PCR and direct sequencing across the r
region. Degeneracy in the sequence ladder indicates the presence of
different sequences in the template population. wt, wild type.
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Emergence of revertants following infection with linear DNA.
We next followed the progress of virus infection initiated by linear
DNA. Twelve ducklings were infected with virus particles containing the
linear I8 genome produced in LMH cells, and the livers were removed at
various times postinfection. Viral replicative intermediates were
extracted from the livers harvested through 8 days postinfection to
determine the extent of replication and spread of infection. Southern
blot analysis of these replicative intermediates (Fig. 3B) showed
detectable viral DNA signals beginning at day 2 postinfection,
increasing through day 8. All virus replication detectable by Southern
blot hybridization was apparently due to infection with spontaneously
occurring viral variants that carry out legitimate replication, since
rcDNA was present in normal proportions (overexposure of the film makes
this difficult to see). The data are consistent with a rapid emergence
and spread of such phenotypically revertant viruses within and from
cells originally infected with linear DNAs.
This interpretation was confirmed by analysis of the
cccDNAs that were present in the livers of the ducklings
infected with the I8 genome. cccDNAs extracted from these livers were
subjected to PCR amplification, and the sequences around the r regions
were determined by direct sequencing of the products. As shown in Fig. 3C, only a very weak sequence ladder was visible in these assays in the
sample harvested at 1 h postinfection, but in samples taken at 1 day and beyond, strong sequence ladders were produced. A high degree of
degeneracy of the sequence ladder at 1 and 2 days postinfection was
seen in this experiment as in the previous experiment (Fig. 3A), and
this degeneracy was substantially reduced at 4, 8, and 23 days, when
high levels of virus replication were detectable by Southern blot
analysis (Fig. 3B). As early as 4 days, the major species were resolved
into two r sequence lengths, of eight and nine nucleotides (as
indicated by doublet bands throughout the regions in the sequencing gel
above the r region), apparently consisting of more than one sequence
for each species (see below). This result is consistent with the
conclusion that the genomes responsible for legitimate replication were
derived from the input linear DNA rather than from contamination with
wild-type virus.
Illegitimate replication following infection with linear DNA.
Evidence for illegitimate replication occurring in the livers of ducks
infected with linear DNA-containing viruses was obtained by amplifying,
cloning, and sequencing individual r regions from the cccDNA of a duck
infected with the I8 mutant and harvested at day 2 postinfection. As
indicated by the direct sequencing experiments shown in Fig. 3A and C,
the cccDNA molecules present at day 2 were highly diverse with respect
to the sequences around the r region. Of 67 individual clones sequenced
in this experiment, no clone was found to contain a wild-type r
sequence, which could only be derived by a single type of nonhomologous
recombination. Sixty-four of 67 r sequences were apparently formed
by nonhomologous recombination, since they differed from both the
wild-type and the I8 sequences. The three r sequence clones that
matched the I8 sequence could have been derived either by homologous
recombination or by amplification of trace amounts of contaminating
plasmid DNA from the I8 expression vector.
Of 64 clones with apparent nonhomologous recombination joints, 46 clones had sequences that could have been generated by a single
recombination event between the ends of the linear I8 DNA. The
sequences of three such clones are shown in Fig.
4. Clone 18 exemplifies one class of
recombinants in which the loss of a cis-acting sequence (DR1
in this case) would render pregenomes produced by this cccDNA largely
inactive for further DNA synthesis. Twelve of the 46 single-site
recombinants were presumed to be inactive in further DNA synthesis
because of deletions extending into DR1 or the pol open
reading frame. Clone 31 is an example of a partial revertant clone,
identical to the I1 mutant, which would be capable of supporting
further DNA synthesis, with the production of excess levels of linear
DNA and a second generation of cccDNAs by both legitimate and
illegitimate replication. In clone 42 a nonhomologous
recombination generated an additional insertion of 5 bp in the r
region. In this clone, DNA synthesis would be expected to occur, but
only linear DNA would be produced because of the excessive length of
the r sequence. This type of recombinant would be likely to produce a
second generation of cccDNAs through illegitimate replication.
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FIG. 4.
Sequences of individual clones of r regions formed by
nonhomologous recombination in I8-infected ducklings at 2 days
postinfection. Nucleotides derived from the I8 insertion are shown in
bold and are not included in the numbering system. A reference I8
sequence between nucleotides 2518 and 2580 is shown at the top, and the
positions of the two ends of in situ-primed linear DNA, defined by the
5' and 3' ends of the minus strand, are indicated. Nucleotides 2549 to
2572 are omitted for brevity. The sequences show evidence of single
(18, 32, and 42) or multiple (40, 81, and 30) nonhomologous
recombinations. See the text for further explanation. The site of
reverse transcription of the minus-strand primer in the 3'  is
underlined.
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More direct evidence for illegitimate replication was obtained from the
sequences of 18 other clones, whose sequences around the r region
showed evidence of more than one nonhomologous recombination event,
consistent with more than one generation of cccDNA formed from linear
DNA. Two such sequences, clones 40 and 81, are shown in Fig. 4.
Fourteen of these 18 sequences required two (clone 40) or more
recombination events to generate the observed sequence, while 4 sequences required up to 4 generations of cccDNA synthesis to be
produced by nonhomologous recombination events, as seen in clone 81. These results support the conclusion that illegitimate replication
through several generations of linear DNA occurred within an initial
period of less than 2 days following infection of cells with linear
DNA.
A third group of recombination joints, previously not seen by us, was
observed in five different clones in this library, exemplified by clone
29. The sequence of each of the five clones required two nonhomologous
recombination events, one of which occurred between sites near the ends
of conventional in situ primed linear DNA. The second recombination
event occurred between a site located near the conventional 3' end of
the minus strand and a site at or just upstream of nucleotide 2576 at
the 5' end of the minus strand in linear DNA. The structures of these
joints indicated that a double-stranded linear DNA with a long direct
repeat on each end might have been the precursor of these cccDNA
molecules and that the 5' end of the minus strand in this linear
precursor mapped to the UUAC in the 3' 
of pregenomic RNA. This
model is consistent with previous reports (3) that a minor
fraction of the minus-strand 5' end maps to nucleotide 2576. The exact mechanism for generation of such minus strand ends is not known.
Partial revertants of illegitimate replication.
By day 4 postinfection with the I8 mutant, the infection was dominated by
genomes carrying out legitimate replication, as judged by the
preponderance of rcDNA in the liver. However, among the genomes
produced by nonhomologous recombination, some genomes suffering short
deletions or insertions would be predicted to carry out a mixture of
legitimate and illegitimate DNA synthesis in individual cells. To
investigate the course of an infection initiated by such partial
revertants, we generated a massive infection with a mutant DHBV genome
containing a 2-bp insertion in the r sequence (mutant I2). Virus
prepared from this mutant was used to inoculate two 4-day-old ducklings
at 5 × 109 viral genomes per duckling. For
comparison, two ducklings were inoculated with a similar dose of
wild-type virus particles. The ducklings were bled at days 1, 4, 5, and
6 postinfection, and they were sacrificed at day 6 and DNA was
extracted from their livers. Results from this experiment are shown in
Fig. 5. All ducklings were viremic at day
4 postinfection, after which titers of virus in the blood of both
groups decreased (Fig. 5A). The decrease in circulating wild-type virus
seen in this experiment is commonly observed in experimentally infected
ducklings and occurs in conjunction with sustained levels of
replicative intermediates in the liver, as shown in this experiment. We
do not know the cause of this reduction in the titer of circulating
virus.
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FIG. 5.
Infection of ducklings with the I2 mutant. Virus
particles containing the mutant I2 or wild-type genome were prepared by
transfection of LMH cells and used to infect four 4-day-old ducklings
at a dose of 5 × 109 viral genomes per bird. (A)
Virus present at the indicated times in 25 µl of serum was extracted
and analyzed by agarose gel electrophoresis and blot hybridization. The
top panel was exposed approximately four times as long as the bottom
panel (compare hybridization marker signals). (B) Liver samples
(equivalent to 5 mg) were analyzed for viral replicative intermediates
present at day 6 postinfection by gel electrophoresis and blot
hybridization. Each lane contained the DNA extracted from an equivalent
of 5 mg of liver tissue. (C) rcDNA extracted from enveloped virus in
the blood and cccDNA from the liver at day 6 postinfection was
subjected to PCR amplification and direct sequencing of the PCR
products through the r region. Primers corresponding to nucleotides
2492 to 2516 and 70 to 45 were used for amplification of the rcDNA. The
sequencing gel shows the presence of the I2 mutation in the day 6 postinfection samples in comparison with the wild-type sequence.
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The patterns of viral DNA observed in the I2-infected ducklings showed
a substantial enrichment in linear double-stranded DNA compared with
that of the wild type, suggesting that the I2 virus was propagated in
vivo. This mutant phenotype was also seen in the replicative
intermediates extracted from liver tissue at day 6 postinfection (Fig.
5B), demonstrating that the production of high levels of linear DNA in
the liver, compared with levels seen in wild-type infection, could be
obtained in fully infected livers. The presence of the original I2
mutation, detected by direct PCR sequencing of the cccDNA as well as
the viral DNA (Fig. 5C), explains the enhanced production of linear DNA
and indicates that the replication of partial revertants of insertion
mutants such as I8, as represented by the mutant I2, could be sustained in the infected cells for at least 6 days. However, passage of the
virus in the sera of these infected ducks through a second group of
ducklings at an inoculation dose of 108 viral genomes
resulted in a complete reversion to legitimate replication (data not
shown). As in the I8 infection, however, the phenotypically revertant
viruses were a mixture of different viruses containing r sequences of 8 or 9 bp (see below).
Phenotypically revertant r sequences that carry out legitimate
replication.
To determine what r sequences supporting legitimate
replication were selected in vivo, viral cccDNA was extracted from the liver of an I8-infected duckling at 23 days postinfection. The r region
from the cccDNA was amplified and cloned to produce a library of
plasmids, and individual clones were sequenced through the r region.
The sequences and frequency of their occurrence among 38 clones
analyzed are shown in Table 1. Only one
example of a genotypically wild-type revertant was seen among the 38 clones. One r sequence of 10 bp, 26 r sequences of 9 bp, and
11 r sequences of 8 bp were found. All but 2 of 38 examples could
have been generated by a single nonhomologous recombination event
between the predicted ends of I8 linear DNA. The basis for the
selection of this particular collection of non-wild-type r sequences is
not understood. While r sequences containing 9 bp were more frequent
than any other length, some 8-bp lengths were stable through a
subsequent passage in ducklings. To test the stability of these variant
r sequences during a second passage, serum (2 × 108
viral genomes) from a duckling infected with the I8 mutant, collected at day 8 postinfection (see Fig. 3B and C), was used to infect a second
bird. At day 7 postinfection, viral DNA from the serum and replicative
intermediates and cccDNA from the liver were all purified and amplified
by PCR for direct sequencing (Fig. 6). The mixed sequence ladder characteristic of the inoculum was still present in virus particles, replicative intermediates, and cccDNA at
day 7 postinfection. Because the wild-type sequence was shown to be
present in the inoculum, we concluded that this sequence (shown in the
ladder on the right) did not have a replication advantage over the
mixed sequences under these outgrowth conditions.
View this table:
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[in a new window]
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TABLE 1.
Different r sequences and their frequencies in a library
of PCR products of cccDNAs at day 23 postinfection with the
I8 mutant
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View larger version (113K):
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FIG. 6.
Stability of non-wild-type r sequences in a second
passage. Virus (2 × 108 viral genomes) from an
I8-infected duck from the experiment described in the legend for Fig.
3B and C was used as the inoculum for a 4-day-old duckling, and viral
DNA was extracted from serum and the liver at day 7 postinfection. DNA
was subjected to PCR amplification, and direct sequencing of the PCR
product was performed. The sequence of the virus particles used as the
inoculum and that of the wild-type virus are shown. In all five
samples, the primers used for amplification were outside the cohesive
end region, as described in Materials and Methods. As has been
previously reported (9), the amplification efficiency of an
rcDNA template was greatly reduced but not eliminated with these
primers.
|
|
| |
DISCUSSION |
Illegitimate replication was previously shown to occur in primary
hepatocyte cultures (31). These cultures were infected with
mutants of DHBV that were defective in rcDNA synthesis as a result of
nucleotide substitutions in and around DR1. Illegitimate replication,
which occurs at very low levels, could be detected in the experiments
because of the suppression of legitimate replication by a stable defect
in rcDNA synthesis. In natural infections, illegitimate replication is
likely to be initiated by a different process, i.e., by infection of
cells with viruses that contain naturally occurring linear
double-stranded DNAs of wild-type sequence, produced by in situ
priming. Linear DNAs were shown to be converted efficiently to cccDNA
by nonhomologous recombination, and those cccDNAs suffered deletions or
insertions of nucleotides within the r region, changing the length of
the r region. Alterations in the length of the r sequence have been
shown to increase in situ priming of plus-strand DNA synthesis,
independent of any DR1-associated mutation (15).
As a result of changes in the r sequence, cccDNA synthesized during the
infection of a hepatocyte by naturally occurring linear DNA-containing
virus would frequently carry out only linear DNA synthesis and
illegitimate replication. These types of mutations are easily reverted,
however, in a subsequent generation of nonhomologous recombination by
insertion or deletion of the exact number of nucleotides that were
originally deleted or inserted, respectively, in the r region during
the initial nonhomologous recombination event. Because of the high
level of linear DNA synthesis (5 to 10%) in a wild-type infection, it
is possible that cycles of illegitimate replication are repeatedly
initiated. We speculated that in an infected liver, a small proportion
of infected cells may be carrying out illegitimate replication at any
one time, and that these cells might have a survival advantage under
some circumstances, for example, in the presence of antigen-specific
cytotoxic T cells. Such cells carrying out illegitimate replication in
the liver would be very difficult to detect by biochemical means since
illegitimate replication levels are so low in comparison with those of
legitimate replication (31). In addition, microscopic
methods might not distinguish between such cells and uninfected cells.
Even though evidence for the existence of such a population of cells in
natural infections is not available, we set out to characterize the
fate of DHBV illegitimate replication in such cells.
By these experiments we demonstrated that hepatocytes infected with
linear DNAs in vivo were able to carry out illegitimate replication and
to give rise to variant viruses that replicate by legitimate
replication. Illegitimate replication was readily detected by day 2 postinfection, as judged by the appearance of cccDNAs containing more
than one nonhomologous recombination joint per r sequence. Assuming
that each joint corresponded to at least one generation of illegitimate
replication, we could detect up to four generations occurring within
the 2-day postinfection period. As we expected, replication quickly was
dominated by variants carrying out legitimate replication by day 4 postinfection. Since the outgrowth of phenotypic revertants resulted in
an approximately 50-fold increase in viral replicative intermediates in
the liver between days 2 and 4 postinfection it was not possible to
follow the fate of illegitimate replication past day 2. We concluded that revertants arose from nonhomologous recombination since most revertants did not contain the wild-type r sequence.
Infection with viruses containing linear DNA also resulted in the
production of partial phenotypic revertants containing less extensive
changes in the r region. As judged by infection experiments with one
such partial revertant, I2, partial revertants possessed the potential
to establish an infection in individual hepatocytes and to produce
elevated levels of linear DNA in infected cells. Such partial
revertants also gave rise to full phenotypic revertants by
nonhomologous recombination. Full revertants were able to displace partial revertants in multiple cycles of replication, presumably due to
their replication advantage in the synthesis of functional cccDNA. Full
revertants did not necessarily contain the wild-type r
sequence, and these non-wild-type revertants did not appear to be at a
disadvantage compared with wild-type virus in these short-term
experiments. This result extends the previous finding of Loeb et al.
(14) that some variations of the wild-type r sequence do not
result in defects in genome circularization. In addition, this
interpretation seems to predict that r sequence variation would be
observed among and within the various DHBV strains; however, no such
variation has been reported to our knowledge.
The experiments suggest that in natural infections linear DNA may be
generated in three different populations of infected hepatocytes. In
cells infected with virus particles that contain wild-type rcDNA,
linear DNA production is only 5 to 10% that of rcDNA. Since the
average cccDNA content of infected cells has been estimated to be
between 3 and 20 copies per cell (7, 26), many of the cells
in this population would contain cccDNA that was derived only from
rcDNA, while others would contain only one or two copies of cccDNA
derived from linear DNA. In cells infected with viruses that contained
rcDNA with small insertions or deletions in the r region, such as the
I2 mutant, the amount of linear DNA synthesized from the original
cccDNA can exceed the amount of rcDNA produced. Thus, a large fraction
of cccDNA produced by amplification in such cells may be formed from
linear DNA, as previously reported (31), and may, therefore,
preferentially produce linear DNA. In cells infected with virus
particles containing linear DNA, as in the I8 mutant, the original
cccDNA molecule formed by nonhomologous recombination would, in most
cases, be unable to generate rcDNA, so that the entire pool of
amplified cccDNA might be derived from linear DNAs. Such cells would be
expected to carry out predominantly illegitimate replication. The three
populations of cells that produce linear viral DNA would be predicted
to show differences in their levels of virus replication according to
the amount of their cccDNA that was derived from rcDNA. These
differences could contribute to the ability of a chronic virus
infection to survive antigen-specific cell-mediated cytotoxicity or
other selective pressures that might be based on the levels of virus
replication. In addition, the three populations of cells would be
expected to differ, according to the level of linear DNA production, in their susceptibility to insertional mutagenesis by nonhomologous recombination of linear viral DNA with cellular DNA ends generated by
DNA damaging agents (19). In the mammalian hepadnavirus
woodchuck hepatitis virus, insertional mutagenesis is thought to be an
important step in the malignant transformation of hepatocytes (reviewed in reference 1).
| |
ACKNOWLEDGMENT |
This work was supported by Public Health Service grant CA-42542
from the National Cancer Institute.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Molecular Genetics and Microbiology, The University of New Mexico
School of Medicine, Albuquerque, NM 87131. Phone: (505) 272-8896. Fax: (505) 272-8896. E-mail: jsummer{at}unm.edu.
| |
REFERENCES |
| 1.
|
Beundia, M. A.
1992.
Hepatitis B viruses and hepatocellular carcinoma.
Adv. Cancer Res.
59:167-226[Medline].
|
| 2.
|
Condreay, L.,
C. Aldrich,
L. Coates,
W. Mason, and T.-T. Wu.
1990.
Efficient duck hepatitis B virus production by an avian tumor cell line.
J. Virol.
64:3249-3258[Abstract/Free Full Text].
|
| 3.
|
Condreay, L. D.,
T. T. Wu,
C. E. Aldrich,
M. A. Delaney,
J. Summers,
C. Seeger, and W. S. Mason.
1992.
Replication of DHBV genomes with mutations at the sites of initiation of minus and plus strand synthesis.
Virology
188:208-216[Medline].
|
| 4.
|
Horwich, A. L.,
K. Furtak,
J. C. Pugh, and J. Summers.
1990.
Synthesis of hepadnavirus particles containing replication-defective duck hepatitis B virus genomes in cultured Huh-7 cells.
J. Virol.
64:642-650[Abstract/Free Full Text].
|
| 5.
|
Huang, M., and J. Summers.
1991.
Infection initiated by the RNA pregenome of a DNA virus.
J. Virol.
65:5435-5439[Abstract/Free Full Text].
|
| 6.
|
Huang, M., and J. Summers.
1994.
pet, a small sequence distal to the pregenome cap site, is required for transcription of the duck hepatitis B virus pregenome.
J. Virol.
68:1564-1572[Abstract/Free Full Text].
|
| 7.
|
Jilbert, A. R.,
T.-T. Wu,
J. M. England,
P. D. L. M. Hall,
N. Z. Carp,
A. P. O'Connell, and W. S. Mason.
1992.
Rapid resolution of duck hepatitis B virus infection occurs after massive hepatocellular involvement.
J. Virol.
66:1377-1388[Abstract/Free Full Text].
|
| 8.
|
Kawaguchi, T.,
K. Nomura,
Y. Hirayama, and T. Kitagawa.
1987.
Establishment and characterization of a chicken hepatocellular carcinoma cell line LMH.
Cancer Res.
47:4460-4464[Abstract/Free Full Text].
|
| 9.
|
Koeck, J., and H.-J. Schlicht.
1993.
Analysis of the earliest steps of hepadnaviral replication: genome repair after infectious entry into hepatocytes does not depend on viral polymerase activity.
J. Virol.
67:4867-4874[Abstract/Free Full Text].
|
| 10.
|
Lenhoff, R., and J. Summers.
1994.
Coordinate regulation of replication and virus assembly by the large envelope protein of an avian hepadnavirus.
J. Virol.
68:4565-4571[Abstract/Free Full Text].
|
| 11.
|
Lenhoff, R., and J. Summers.
1994.
Construction of avian hepadnavirus variants with enhanced replication and cytopathicity in primary hepatocytes.
J. Virol.
68:5706-5713[Abstract/Free Full Text].
|
| 12.
|
Lien, J. M.,
C. Aldrich, and W. S. Mason.
1986.
Evidence that a capped oligonucleotide is the primer for duck hepatitis B virus plus-strand DNA synthesis.
J. Virol.
57:229-236[Abstract/Free Full Text].
|
| 13.
|
Lien, J. M.,
D. Petcu,
C. Aldrich, and W. S. Mason.
1987.
Initiation and termination of duck hepatitis B virus DNA synthesis during virus maturation.
J. Virol.
61:2286-2296[Abstract/Free Full Text].
|
| 14.
|
Loeb, D.,
K. J. Gulya, and R. Tian.
1997.
Sequence identity of the terminal redundancies on the minus-strand DNA template is necessary but not sufficient for the template switch during hepadnavirus plus-strand DNA synthesis.
J. Virol.
71:152-160[Abstract].
|
| 15.
|
Loeb, D.,
R. Hirsch, and D. Ganem.
1991.
Sequence-independent RNA cleavages generate the primers for plus strand DNA synthesis in hepatitis B viruses: implications for other reverse transcribing elements.
EMBO J.
10:3533-3540[Medline].
|
| 16.
|
Mandart, E.,
A. Kay, and F. Galibert.
1984.
Nucleotide sequence of a cloned duck hepatitis B virus genome: comparison with woodchuck and human hepatitis B virus sequences.
J. Virol.
49:782-792[Abstract/Free Full Text].
|
| 17.
|
Mason, W. S.,
C. Aldrich,
J. Summers, and J. M. Taylor.
1982.
Asymmetric replication of duck hepatitis B virus DNA in liver cells (free minus strand DNA).
Proc. Natl. Acad. Sci. USA
79:3997-4001[Abstract/Free Full Text].
|
| 18.
|
Mason, W. S.,
G. Seal, and J. Summers.
1980.
A virus of Pekin ducks with structural and biological relatedness to human hepatitis B virus.
J. Virol.
36:829-836[Abstract/Free Full Text].
|
| 19.
|
Petersen, J.,
M. Dandri,
A. Burkle,
L. Zhang, and C. E. Rogler.
1997.
Increase in the frequency of hepadnavirus DNA integrations by oxidative DNA damage and inhibition of DNA repair.
J. Virol.
71:5455-5463[Abstract].
|
| 20.
|
Pugh, J. C.,
K. Yaginuma,
K. Koike, and J. Summers.
1988.
Duck hepatitis B virus (DHBV) particles produced by transient expression of DHBV DNA in a human hepatoma cell line are infectious in vitro.
J. Virol.
62:3513-3516[Abstract/Free Full Text].
|
| 21.
|
Seeger, C.,
D. Ganem, and H. E. Varmus.
1986.
Biochemical and genetic evidence for the hepatitis B virus replication strategy.
Science
232:477-484[Abstract/Free Full Text].
|
| 22.
|
Staprans, S.,
D. Loeb, and D. Ganem.
1991.
Mutations affecting hepadnavirus plus-strand synthesis dissociate primer cleavage from translocation and reveal the origin of linear viral DNA.
J. Virol.
65:1255-1262[Abstract/Free Full Text].
|
| 23.
|
Summers, J., and W. S. Mason.
1982.
Replication of the genome of hepatitis B-like virus by reverse transcription of an RNA intermediate.
Cell
29:403-415[Medline].
|
| 24.
|
Summers, J.,
A. O'Connell, and I. Millman.
1975.
Genome of hepatitis B virus: restriction enzyme cleavage and structure of the DNA extracted from Dane particles.
Proc. Natl. Acad. Sci. USA
72:4597-4601[Abstract/Free Full Text].
|
| 25.
|
Summers, J.,
P. Smith, and A. L. Horwich.
1990.
Hepadnaviral envelope proteins regulate amplification of covalently closed circular DNA.
J. Virol.
64:2819-2824[Abstract/Free Full Text].
|
| 26.
|
Summers, J.,
P. Smith,
M. Huang, and M. Yu.
1991.
Morphogenetic and regulatory effects of mutations in the envelope proteins of an avian hepadnavirus.
J. Virol.
65:1310-1317[Abstract/Free Full Text].
|
| 27.
|
Summers, J.,
J. M. Smolec, and R. Snyder.
1978.
A virus similar to hepatitis B virus associated with hepatitis and hepatoma in woodchucks.
Proc. Natl. Acad. Sci. USA
75:4533-4537[Abstract/Free Full Text].
|
| 28.
|
Tuttleman, J.,
C. Pourcel, and J. Summers.
1986.
Formation of the pool of covalently closed circular viral DNA in hepadnavirus-infected cells.
Cell
47:451-460[Medline].
|
| 29.
|
Wei, Y.,
J. E. Tavis, and D. Ganem.
1996.
Relationship between viral DNA synthesis and virion envelopment in hepatitis B viruses.
J. Virol.
70:6455-6458[Abstract].
|
| 30.
|
Wu, T.-T.,
L. Coates,
C. E. Aldrich,
J. Summers, and W. S. Mason.
1990.
In hepatocytes infected with duck hepatitis B virus, the template for viral RNA synthesis is amplified by an intracellular pathway.
Virology
175:255-261[Medline].
|
| 31.
|
Yang, W., and J. Summers.
1995.
Illegitimate replication of linear hepadnaviral DNA through nonhomologous recombination.
J. Virol.
69:4029-4036[Abstract].
|
| 32.
|
Yang, W.,
W. S. Mason, and J. Summers.
1996.
Covalently closed circular viral DNA formed from two types of linear DNA in woodchuck hepatitis virus-infected liver.
J. Virol.
70:4567-4575[Abstract].
|
Journal of Virology, November 1998, p. 8710-8717, Vol. 72, No. 11
0022-538X/98/$04.00+0
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Top
Abstract
Introduction
