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Journal of Virology, July 2000, p. 5788-5795, Vol. 74, No. 13
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Association of RNA Polymerase Complexes of the
Parasitic Protozoan Cryptosporidium parvum with Virus-Like
Particles: Heterogeneous System
Nikolai V.
Khramtsov* and
Steve J.
Upton
Division of Biology, Kansas State University,
Manhattan, Kansas 66506-4901
Received 16 February 2000/Accepted 13 April 2000
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ABSTRACT |
RNA polymerase complexes were purified from Cryptosporidium
parvum, a parasitic protozoan known to infect many species of mammals including humans. Western blot analysis revealed the
association of the complexes with two different proteins, encoded by
large and small segments of viral double-stranded RNAs. Each complex was found to contain only double-stranded RNA, both double- and single-stranded RNA, or only single-stranded RNA. Maximum RNA-dependent RNA polymerase activity was observed within the complexes containing both double- and single-stranded RNAs. These complexes possessed both
transcriptase and replicase polymerase activities. Virus-like particles
with a diameter of 31 nm were copurified with RNA polymerase complexes,
and buoyant density and polymerase studies suggest that C. parvum harbors a putative double-stranded RNA virus which separately encapsidates the large and small RNA segments. The mechanism
of replication and other characteristics of this virus are similar to
those of the viruses of the family Partitiviridae, previously identified only in fungi and plants.
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INTRODUCTION |
Cryptosporidium parvum is
an intestinal intracellular parasitic protozoan of the phylum
Apicomplexa which infects a wide variety of mammalian species.
Infection results in diarrhea that is self-limiting in most cases but
may be life threatening in immunocompromised individuals. C. parvum is one of the opportunistic infections in AIDS patients,
and thus far, there is no effective treatment for cryptosporidiosis
(8). Because of the lack of adequate treatment, other types
of therapeutic targets are being sought, and extrachromosomal genetic
elements are considered potential targets. For example, the
extranuclear plastid genomes of Plasmodium and
Toxoplasma spp., both parasites distantly related to
C. parvum, are essential for parasite survival, and
inhibition of plastid replication blocks the multiplication of
parasites (9).
All isolates of C. parvum tested thus far are known to
harbor both large (L) and small (S) extrachromosomal viral
double-stranded RNA (dsRNA) segments (17, 19). The cDNAs of
both dsRNAs have been cloned and sequenced, and only a single long open
reading frame (ORF) has been identified in each dsRNA. The deduced
protein sequence of the L-dsRNA (1,786 nucleotides [nt]) has
similarity with viral RNA-dependent RNA polymerases (RDRP). The
sequence of the putative protein encoded by the S-dsRNA (1,374 nt) has no significant similarity with polypeptide sequences in databases (17). The presence of RDRP activity in crude lysates of
C. parvum oocysts, as well as replicative intermediates (RI)
and full-size plus strands, which may represent mRNAs of the dsRNAs,
suggests that these molecules are transcribed in the parasite
(18). Additional indirect evidence of protein coding
capacity of the dsRNAs exists as a result of a comparative analysis of
the sequences of dsRNAs from a number of isolates of C. parvum with two distinct genotypes. The majority of nucleotide
substitutions occur in the third positions of the codons in putative
ORFs and fail to change the protein sequences (19). However,
to date, there is no direct evidence for the presence of proteins
encoded by the dsRNAs, nor have virus particles been identified in the
previous studies (17-19).
Extrachromosomal dsRNAs are very common in protozoa (24, 28,
29), fungi (2, 7, 11, 30), and plants (21). Although many of these genomes have no "visible" effect on the host, some dsRNAs do appear to influence host biology (20). For example, yeasts from several genera contain dsRNA viruses encoding
toxins that kill other strains not synthesizing the protein (26,
30). Infection of the chestnut blight fungus, Cryphonectria parasitica, with dsRNA associated with membranous vesicles causes reduction of virulence (hypovirulence) of the fungus (20,
23). However, the effect of extrachromosomal dsRNAs on the
biology of C. parvum and the routes of transmission are as
yet unknown. The purpose of the present study was to further examine
dsRNAs, in respect to protein coding capacity, complex formation, and replication mechanism, with the aim of helping determine the
relationship of the segments with other known dsRNA genetic elements
and to help understand the role of these dsRNAs within the parasite.
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MATERIALS AND METHODS |
Parasite and oocyst purification.
The KSU-1 isolate of
C. parvum was used in this study. Oocysts were purified from
feces of infected 5-day-old calves by CsCl gradient centrifugation as
described previously (27).
RNA polymerase assay.
The assay was carried out in 50-µl
reaction volumes containing 50 mM Tris-HCl, pH 7.4; 100 mM NaCl; 10 mM
MgCl2; 10 mM dithiothreitol; 1 mM (each) GTP, CTP, and ATP;
10 µCi of [
-32P]UTP (3,000 Ci/mmol); 0.5 mg of
actinomycin D per ml; and aliquots of crude lysate of C. parvum oocysts or fractions from sucrose or CsCl gradients. After
incubation at 37°C for 1 h, reactions were terminated by
addition of 50 µl of stop solution (0.2% sodium dodecyl sulfate
[SDS], 50 mM EDTA, 0.5 mg of proteinase K, 3 µg of total yeast RNA)
and incubated at 37°C for 10 min. In pulse-chase experiments, and
before termination of the reaction with stop solution, cold UTP was
added to a final concentration of 1 mM and the mixture was incubated
for an additional 30 min at 37°C. Nucleic acids from one-half of
these reaction mixtures were twice precipitated with 2 M
NH4OAc and 3 volumes of ethanol. Pellets were washed with
70% ethanol, dried in a vacuum, dissolved in 20 µl of TE buffer (10 mM Tris-HCl [pH 7.5], 1 mM EDTA), and then resolved on 0.8% agarose
gels. After electrophoresis, gels containing 32P-labeled
products of the RNA polymerase assays were incubated for 20 min in 10%
trichloroacetic acid and then dried for 3 h between filter paper
prior to exposure to X-ray film at 
70°C with an intensifying
screen. Quantitation of incorporation of 32P into nucleic
acids was estimated by counting the radioactivity of the second aliquot
of the reaction mixture after trichloroacetic acid precipitation as
described previously (18).
Northern blot hybridization.
Agarose gel electrophoresis on
1.2% nondenaturing gels and Northern blot hybridization at high
stringency with 32P-labeled RNAs were performed as
described previously (10).
Expression of ORFs of dsRNA in Escherichia coli and
preparation of antiserum to recombinant proteins.
All standard DNA
manipulations were performed as previously described (25).
The numbering is based on the published sequences of the L- and
S-dsRNAs (17). DNA fragments, containing entire coding
sequences including start and terminator codons (nt 134 to 1708 and 248 to 1207 for L- and S-dsRNAs, respectively), were generated on total
nucleic acids purified from oocysts by reverse transcription-PCR using
avian myeloblastosis virus reverse transcriptase (Promega) and High
Fidelity Taq DNA polymerase (Boehringer Mannheim). The set
of primers for L-dsRNA was as follows: sense, LVN-1,
5'-ctggatccATGAAGTTTGTCAATATCTATG, and
antisense, LVC-1,
5'-gggtcgacTTATCCATAAATTTTGTGACTC;
the set for S-dsRNA was as follows: sense, SVN-1,
5'-ctggatccATGATTACAAGTTTTGAATCAA, and
antisense, SVC-1,
5'-aagtcgacCTAATGGGAGCGATCTGCGCTA.
Lowercase letters represent nucleotides used for cloning
purposes. The sites for restriction endonuclease BamHI are
underlined, and the sites for SalI are double underlined.
Start codons in sense primers and stop codons in antisense primers are
italicized. The amplified products were digested with the restriction
endonucleases BamHI and SalI and ligated into the
bacterial expression vector pET-28(a+) (Novagen) previously digested
with the same enzymes. This bacterial expression vector was chosen
because it has previously been shown to allow for high expression of
C. parvum genes (16). The recombinant plasmids
were introduced into the E. coli strain BL21(DE3) (Novagen). The fusion proteins, containing N-terminal peptides (34 amino acids)
with six histidine residues (His tag) encoded by vector DNA and
polypeptides encoded by the ORF of the dsRNA, were synthesized in
E. coli after induction with 1 mM
isopropyl-1-thio-
-D-galactopyranoside (IPTG).
Recombinant proteins were found in inclusion bodies and purified on His
Bind columns under denaturing conditions according to the
manufacturer's recommendations (Novagen). Purified recombinant proteins were dialyzed overnight against phosphate-buffered saline (PBS) and used to produce polyclonal antibodies in rats as described previously (15). Antibodies against some E. coli
proteins were removed by adsorption of antiserum with concentrated
lysates of E. coli strain BL21(DE3) containing only the
cloning vector as described previously (25).
Western blot analysis.
Proteins were resolved by
electrophoresis on SDS-10% polyacrylamide gels and then
electrotransferred to NitroPure membrane (Micron Separations Inc.).
Blots were blocked for 2 h in PBS containing 5% nonfat dry milk
and 0.05% Tween 20 (blocking solution). Blots were then incubated for
2 h with the rat antiserum (diluted 1:100 in blocking solution) to
recombinant proteins. The blots were then washed six times for 5 min
each in PBS and incubated for 1 h with a horseradish
peroxidase-coupled goat anti-rat secondary antibody (Sigma). Blots were
developed with 4-chloro-1-naphthol as substrate.
Isolation of VLPs.
Ten billion purified CsCl oocysts were
excysted by incubation at 37°C for 90 min in 5 ml of PBS. Mixtures of
sporozoites and nonexcysted oocysts were harvested by low-speed
centrifugation (2,000 × g, 3 min), resuspended in 15 ml of buffer A (50 mM Tris-HCl, pH 7.4; 100 mM NaCl; 10 mM
MgCl2; 10 mM dithiothreitol), and frozen at 70°C. All
other steps of virus-like particle (VLP) isolation were performed at
4°C. After thawing of sporozoites-oocysts on ice, the cellular debris
and nuclei were removed by centrifugation at 2,000 × g
for 5 min and then twice at 10,000 × g for 10 min. Five milliliters of clarified supernatant (crude lysate) was layered on
top of a 10 to 40% (wt/wt) linear sucrose gradient in buffer A (35 ml)
and centrifuged at 100,000 × g for 3 h; fractions
of 2 ml were collected. In other experiments, crude lysates were extracted twice with an equal volume of chloroform. The aqueous phase
was collected and centrifuged at 10,000 × g for 10 min. A portion of the 4.5-ml clarified supernatant was pelleted through a cushion of 1 ml of 15% sucrose by centrifugation at
100,000 × g for 2 h. The pellet was resuspended
by sonication in 1.2 ml of buffer A and loaded atop a preformed
gradient of CsCl (1 ml with 1.5 g/ml, 1 ml with 1.4 g/ml, 1.5 ml with
1.3 g/ml, and 1 ml with 1.2 g/ml) and centrifuged at 100,000 × g for 16 h. Thirty fractions of 180 µl each were
collected and dialyzed against buffer A overnight. Each fraction of the
gradient was tested for the presence of (i) RNA polymerase activity;
(ii) dsRNAs and single-stranded RNAs (ssRNAs), by Northern blot
hybridization; and (iii) proteins encoded by ORFs of both segments of
dsRNAs, by Western blot analysis.
Electron microscopy.
Aliquots of the CsCl gradient fractions
were deposited onto carbon-coated 200-mesh copper grids, negatively
stained with 2% uranyl acetate, and visualized with a Philips 201 transmission electron microscope for the presence of VLPs.
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RESULTS |
Stability of RNA polymerase activity.
Incubation of crude
oocyst lysates with proteinase K (up to 2 mg/ml) (Fig.
1A) did not have a significant effect on
RNA polymerase activity, which suggests that the polymerase might be
protected from digestion. When RNase A was eliminated by digestion with proteinase K before the RNA polymerase assay, treatment of lysate with
RNase (up to 2 mg/ml) (Fig. 1B) did not change incorporation of
32P into nucleic acids. This suggests that templates for
RNA polymerase are protected. When reactions were performed in the
presence of 10 µg of RNase A per ml, 32P-labeled products
of the polymerase assay were visible on autoradiograms (Fig. 1B). This
suggests that the newly synthesized products of polymerase assay are
also protected, as the purified dsRNAs and ssRNAs have been shown to be
completely degraded at this RNase A concentration (17).
Products of RNA polymerase activity are more likely to form complexes
with the protein(s), as they do not migrate into the polyacrylamide
gels if loaded directly from the polymerase mixture (Fig. 1C). However,
32P-labeled L- and S-dsRNAs were resolved by
electrophoresis when complexes were destroyed before loading onto gels
by incubating the polymerase mixture with 0.1% SDS, or SDS and 0.5 mg
of proteinase K per ml, or extraction with phenol-chloroform (Fig. 1C).
The extraction of crude lysate three times with organic solvents
(butanol or chloroform) prior to the RDRP assay did not have any effect on RNA polymerase activity (data not shown). This may be explained by
RNA polymerase activity not being associated with membranous structures.
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FIG. 1.
Resistance of RNA polymerase activity in crude oocyst
lysates. 32P-labeled products of RNA polymerase assays were
resolved by electrophoresis on 0.8% agarose gels (A and B) or on a 6%
polyacrylamide gel (C) under nondenaturing conditions and were then
exposed to X-ray film. (A) Assays were performed in the presence of
different concentrations of proteinase K. (B) Aliquots were incubated
for 30 min at 37°C with different concentrations of RNase A, then
RNase was destroyed by treatment with proteinase K (0.5 mg/ml, 30 min
at 37°C), and finally [-32P]UTP was added and the
mixture was incubated for 1 h at 37°C. (C) RNA polymerase
mixtures were untreated, incubated with 0.1% SDS or 0.1% SDS-0.5 mg
of proteinase K per ml, or extracted once with phenol-chloroform and
then loaded on the gel.
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Some viral RNAs are associated with RNA polymerase activity, and
others are not.
Results presented above suggest that viral RNA
might be associated with RNA polymerase. Attempts were made to obtain
evidence of copurification of viral RNAs and RNA polymerase. Crude
oocyst lysates were fractionated by sucrose gradient centrifugation. The fractions were collected and analyzed for the presence of viral
RNAs by staining with ethidium bromide (Fig.
2A), Northern blot hybridization (Fig.
2B), and also RNA polymerase activity (Fig. 2C). dsRNA and ssRNA (plus
strands) were identified in fractions 2 to 16 (Fig. 2B);
single-stranded minus strands were not found (data not shown). Free
minus strands were not identified previously in crude oocyst extracts
(17). RI and RNA polymerase activity were found only in
fractions 2 to 12 and not in fractions 14 to 16 (Fig. 2B and C). These
data suggest that at least two types of viral RNAs might be found in
oocysts. Only one type was associated with polymerase activity. More
likely, RNAs from fractions 14 to 16 are free, i.e., not bound to the
protein(s), as they were localized in low-density fractions from the
bulk of rRNAs derived from ribosomes (fractions 6 to 12) (Fig. 2A).
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FIG. 2.
Presence of two distinct types of viral RNAs, with one
of these associated with RNA polymerase activity. Crude lysates of
oocysts were fractionated by sucrose gradient centrifugation, and the
fractions were analyzed for the presence of viral RNA and RNA
polymerase activity. (A) Ethidium bromide-stained 0.8% agarose gel
with nucleic acids purified from even fractions of gradient. (B)
Northern blot analysis, where nucleic acids were extracted from
fractions and separated on agarose gels under nondenaturing conditions,
then denatured in situ, and transferred to the filter. Hybridization
was performed with 32P-labeled riboprobes complementary to
the plus strand of the L-dsRNA. A similar pattern of hybridization was
observed with riboprobes complementary to the plus strand of the
S-dsRNA (data not shown). In experiments with 32P-labeled
riboprobes complementary to the minus strands of the L- and S-dsRNAs,
hybridization occurred only with RI and dsRNA (data not shown). (C)
Autoradiogram of 32P-labeled products of RNA polymerase
assay resolved by electrophoresis on an 0.8% agarose gel.
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Association of RNA polymerase complexes with the VLPs.
To
further characterize the RNA polymerase complex, crude lysates of
oocysts were twice extracted with chloroform, pelleted through a
sucrose cushion, and fractionated by isopycnic centrifugation on CsCl
density gradients. Northern blot analysis (Fig.
3) revealed that the lighter fractions
(14 for L-probe and 14 and 15 for S-probe) contained mainly ssRNAs
(plus strands) whereas the heaviest (7 for L-probe and 8 for
S-probe) contained only dsRNA. Different types of RNA (dsRNA,
ssRNA, and RI) were found together in fractions 9 to 11 for L-probe and
10 to 12 for S-probe. RI appeared to be growing in size, reaching
maximum lengths in the heaviest fractions (9 for L-probe and 10 for
S-probe). In these fractions, the highest amounts of ssRNA were
detected (Fig. 3A, compare fraction 9 with fractions 10 and 11 for
L-probe; Fig. 3B, compare fraction 10 with fractions 11 and 12 for
S-probe). This suggests that, once synthesis of new strand is
completed, one of the plus strands is released from the RI. More
likely, the released strand still stays as a complex with the
protein(s), as free ssRNA and dsRNA were removed (by centrifugation
through a cushion of sucrose) prior to loading on CsCl gradients. RNA
polymerase assays were performed on each fraction, and activity was
found in fractions 8 to 14 with maximum activity in fractions 9 to 12 (see below). This suggests cosedimentation of viral RNAs with
polymerase activity. All three kinds of viral RNA (dsRNA, ssRNA, and
RI) were identified in the heaviest fractions when hybridization was
performed with probes to L-dsRNA and then with probe to S-dsRNA
(compare Fig. 3A and B). This indicates that large and small segments
are associated with different polymerase complexes and that the
complexes can be separated based on their densities on CsCl gradients.
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FIG. 3.
Distribution of viral RNAs in CsCl fractions. Nucleic
acids were purified from fractions from CsCl gradients, resolved on an
0.8% agarose gel under nondenaturing conditions, transferred to
nitrocellulose filters, and hybridized with 32P-labeled
riboprobe complementary to plus strands of L-dsRNAs (A) or S-dsRNAs
(B). Only fractions 5 to 18 out of 30 total are shown.
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Because it was unknown whether the ORFs of the dsRNAs really encoded
proteins, both ORFs were expressed in
E. coli (Fig.
4A)
and antiserum raised to the
recombinant proteins was used to probe
Western blots containing
proteins from CsCl fractions. Antibodies
to the protein encoded by the
ORF of the L-dsRNA (putative RDRP)
(
17) recognized a band
with a molecular size of 65 kDa in fractions
8 to 13 (Fig.
4B).
Antisera to protein from the S-dsRNA (protein
with unknown function)
(
17) identified a band with a molecular
size of 37 kDa in
fractions 6 to 17 (Fig.
4C). The sizes of both
bands were similar to
those predicted from amino acid sequences.
This suggests that extensive
modifications to the proteins are
probably lacking. Coomassie blue
staining of the SDS-polyacrylamide
gel (Fig.
4D) showed that fractions
8 to 12 contained few proteins;
one of them (37 kDa) was identified by
Western blot analysis and
the other proteins more likely had a host
origin. The putative
RDRP (65-kDa protein) was not visible, perhaps
because this protein
may be less abundant than the 37-kDa protein.
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FIG. 4.
Distribution of proteins encoded by ORFs of the L- and
S-dsRNAs in CsCl gradient fractions. (A) Expression of the ORFs of the
L- and S-dsRNAs in E. coli. Shown is a Coomassie
blue-stained SDS-10% polyacrylamide gel with total proteins from
uninduced (IPTG) and induced (+IPTG) E. coli cells and
affinity-purified recombinant proteins. Arrows show positions of
recombinant proteins. Molecular size standards are shown in kilodaltons
in the right margin. (B and C) Immunoblot analysis of the proteins from
the CsCl fraction using antibodies raised against recombinant proteins
of L-dsRNA (B) and S-dsRNA (C). (D) Coomassie blue-stained SDS-10%
polyacrylamide gel with the proteins from CsCl fractions. Molecular
size standards are shown in kilodaltons in the right margin. Only
fractions 5 to 18 out of 30 total are shown.
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Electron microscopy analysis of CsCl gradient fractions revealed the
presence of isometric VLPs with a diameter of about 31
nm in fractions
7 to 18. The concentration and purity of these
particles were the
highest in fractions 8 to 12 (density, 1.439
to 1.391 g/ml). Figure
5 shows particles from fraction 10. Observations
of viral RNAs, RNA polymerase activity, proteins encoded
by both
dsRNAs, and the particles themselves in these same fractions of
CsCl gradient strongly indicate their association and suggest
that
C. parvum harbors a potential dsRNA virus.
Presence of transcriptase and replicase activities in identical
fractions of CsCl gradient.
When RNA polymerase mixtures of the
pulse experiment were resolved on nondenaturing agarose gels, several
bands were visualized on autoradiograms (Fig.
6A). The heaviest fractions, from 8 to 12, synthesized products migrating as RI, dsRNA, and low-molecular-size material. Fraction 8 incorporated 32P predominantly into
the band migrating as the L-dsRNA, and fraction 12 incorporated
32P mainly into the band migrating as the S-dsRNA. These
data provide additional evidence that L- and S-dsRNAs form different
complexes with polymerase and can be separated according to their
buoyant density. Fractions 10 and 11 synthesized approximately similar amounts of L- and S-dsRNA. The lightest, fraction 14, incorporated 32P mainly in the bands migrating as ssRNA. In the
pulse-chase experiment (Fig. 6B), most of the radioactivity was
incorporated into dsRNA in all fractions. So far, it is difficult to
find an explanation of why fraction 14 synthesizes ssRNA in pulse and
double-stranded molecules in pulse-chase experiments. The amount of RI
and the smaller-size products was decreased in fractions 8 to 12, compared to the amounts in the pulse experiment. The
smaller-molecular-size molecules in fractions 8 to 12 most likely
represent incomplete products synthesized at a limiting concentration
of one of the nucleotides, as these small-size products were converted
to full-size molecules at a higher concentration (1 mM) of all four
nucleotides (pulse-chase experiment) (compare Fig. 6A and B). To
confirm the chemical structure of the polymerase products, the
32P-labeled RNAs from fractions 10 and 14 were purified
from the pulse experiment by phenol-chloroform extraction and subjected to RNase A digestion in low- and high-salt buffer. Figure 6C shows that
the products of fraction 10 were mostly dsRNA, as they were not
degraded in the presence of RNase A and 0.6 M NaCl, and that the
products of fraction 14 were mostly ssRNA. To verify the polarity of
the synthesized products, the 32P-labeled RNAs from
fractions 10 and 14 were used as probes in hybridization experiments
with unlabeled plus and minus transcripts obtained from cDNAs of the L-
and S-dsRNAs (Fig. 6D). These experiments revealed that
32P-labeled plus and minus strands were present in fraction
10 and indicate that two polymerase activities exist in this fraction, transcriptase and replicase. The intensity of the hybridization signals
suggests that fraction 10 synthesizes more plus strands than minus
strands. Only replicase activity was observed in fraction 14, as the
32P-labeled products hybridized mostly with unlabeled
transcripts, corresponding to plus strands of the L- and S-dsRNAs. The
synthesis of minus strands most likely occurs on single-stranded plus
strands, as only these kinds of molecules were identified in this
fraction by Northern blot analysis (Fig. 3).
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FIG. 6.
Association of transcriptase and replicase activities
with fractions of CsCl gradients. (A and B) 32P-labeled
products from pulse (A) and pulse-chase (B) RNA polymerase assays
resolved by electrophoresis on 0.8% agarose and exposed to X-ray film.
(C) Effect of RNase on products of RNA polymerase reactions from
fractions 10 and 14. Purified products were treated with RNase A (10 µg/ml, for 30 min at 37°C) in the absence () or presence (+) of
0.6 M NaCl. After treatment, RNA was separated on an 0.8% agarose gel
and detected by autoradiography. (D) Identification of the polarity of
the RNA polymerase products from fractions 10 and 14. Unlabeled
transcripts corresponding to minus and plus strands of the L-dsRNA (L)
and S-dsRNA (S) were synthesized on cDNA clones using T7 and T3 RNA
polymerases. Usually, two bands were identified by ethidium bromide
staining of the products of the reaction, as was observed previously
(18). Then unlabeled products were electrophoresed on 1.2%
agarose, transferred to filters, and probed with
32P-labeled products of polymerase reactions synthesized by
fractions 10 and 14.
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RNA polymerase assays were performed on fractions 10 and 14 in the
presence of different concentrations of proteinase K (Fig.
7A) and RNase A (Fig.
7B). RNA polymerase
activity in fraction
10 was more resistant to both treatments than was
activity in
fraction 14. The products of polymerase activity were still
observed
in fraction 14 after treatment with 1 µg of RNase A
per ml. These
results indicate that newly synthesized ssRNAs are
protected in
this fraction, as this concentration of RNase A is known
to completely
degrade purified ssRNA (
17). The protection
assays provide evidence
of encapsidation of viral RNAs and RNA
polymerase into the particles.
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FIG. 7.
Resistance of viral RNA polymerase activity in fractions
10 and 14 of the CsCl gradient. 32P-labeled products of RNA
polymerase assays were resolved by electrophoresis on an 0.8% agarose
gel and exposed to X-ray film. Assays were performed in the presence of
different concentrations of proteinase K (A) or RNase A (B).
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DISCUSSION |
This study demonstrates association of enzymatically active RNA
polymerase complexes with VLPs. The population of complexes can be
divided into two groups. The first type, with a higher density,
contains a large segment, and the second, with the lower density,
contains a small segment of viral RNA. Each type represents a
heterogeneous system and can be separated into three classes according
to the type of copurified nucleic acids: complexes with only
dsRNA, complexes with only ssRNA, and complexes with both dsRNA
and ssRNA. The proteins encoded by the ORFs for both dsRNAs were
identified and found to be associated with RNA polymerase complexes.
This is direct evidence for the expression of dsRNA genes in the
oocysts of C. parvum. The study of RNA polymerase activity
suggests encapsidation of viral RNAs and RNA polymerase into the
particles. If the RNAs are encapsidated into VLPs, then the functions
of both proteins can be explained. The protein product of the L-dsRNA
is most likely a polymerase and has significant similarity with RDRP
from viruses of the family Partitiviridae (17).
The product of the S-dsRNA, which is more abundant than polymerase,
most likely represents the capsid protein. It is in agreement with the
hypothesis that all dsRNA viruses share a common capsid architecture
and have a 120-capsid subunit and one or fewer molecules of polymerases
(5, 14).
Using a taxonomic key for the placement of viruses in taxa
(22), it is possible to unambiguously classify the virus of
C. parvum as a new member of the family
Partitiviridae. Table 1 shows
a comparison of the main features of viruses from this family with
those of the C. parvum virus (CPV). The partitiviruses
include four genera, Partitivirus, Chrysovirus,
Alphacryptovirus, and Betacryptovirus. Up until
this time, all members of the Partitiviridae have been found
in only fungi and plants. It appears that CPV is the first member of
the family in a protozoan host. The other dsRNA viruses of protozoa
belong to the family Totiviridae (13).
Analysis of viral RNAs by Northern blot analysis and products of RNA
polymerase assays in the CsCl gradient fractions allow us to identify
intermediates of the multiplication cycle and propose an in vitro model
of virus replication. For simplicity, only replication of the L-dsRNA
will be discussed below. The RNA polymerase from the particles with
lighter density (1.348 g/ml), containing mainly single-stranded plus
strands (fraction 14, Fig. 3A), synthesizes a minus strand using plus
strand as template (replication). Newly synthesized minus strand
anneals with plus strand and forms dsRNA, as was observed in
pulse-chase experiments (Fig. 6B). One molecule of dsRNA per particle
would be a result of this first step, and these particles should have
higher density. Only dsRNA was found in fraction 12 with a density of
1.391 g/ml (Fig. 3A). These dsRNAs more likely appeared from the
particles with only one molecule of dsRNA. The majority (70%) of
polymerase activity was found in fractions 9 to 11 (Fig. 6A and B)
containing dsRNA, ssRNA, and RI (Fig. 3). Transcriptase and replicase
activities were observed in these same fractions. The polymerase
synthesizes a new plus strand (transcription) by a semiconservative
mechanism, as was shown previously (18). Thus, the synthesis
of a new strand occurs through RI in fractions 9 to 11 (Fig. 3A) using
the dsRNA as template. When synthesis is completed (fraction 9),
parental plus strand is released from the RI but still stays inside the
particle. This ssRNA most likely serves as a template for synthesis of
the complementary minus strand (replication), forming a new dsRNA
molecule. As a result of transcriptase and replicase activities, one
particle could have two identical molecules of dsRNA. These particles
should have the highest buoyant density in the CsCl gradient. Indeed, only dsRNAs were detected in fraction 7 (density, 1.460 g/ml) by
Northern blot hybridization (Fig. 3A). These dsRNAs could be derived
from particles with two molecules of dsRNA.
Two identical molecules of dsRNA in the same particle have been found
previously in viruses of the family Partitiviridae, for
example, from Penicillium stoloniferum (1) and
Aspergillus foetidus (3). It was proposed
previously that these particles could be uncoated in vivo, followed by
RNA polymerase activity to produce copies of the mRNA using uncoated
dsRNA as a template (4). The presence of free viral dsRNA
and ssRNA in crude lysates of oocysts of C. parvum may offer
some support for this model, but RNA polymerase activity was not found
to be associated with these RNAs in vitro. An alternative possibility
is that particles with two molecules of dsRNA synthesize and release
mRNA, as was shown previously for VLPs from yeast with M1
dsRNA encoding a killer toxin (6). These authors proposed a
head-full type of replication mechanism. The M1 virus is a
satellite of L-A virus from the family Totiviridae, and the
M1 dsRNA is packaged and replicates in L-A particles. L-A
particles have a structure primarily adapted to encapsidate only one
molecule of L-A dsRNA (10); however, because the
M1 dsRNA (1.8 kbp) is less than half the size of L-A dsRNA
(4.6 kbp), the L-A particles can comfortably encapsidate one or two
molecules of M1 dsRNA as well (6).
The dsRNA virus of C. parvum has features most similar to
viruses of the family Partitiviridae (Table 1). However, the
head-full replication mechanism of satellite viruses of the family
Totiviridae seems to be the most likely mechanism for the
replication of both the C. parvum dsRNA virus and other
partitiviruses. Since partitiviruses are thought have evolved from the
totiviruses by dividing their genome between two separately
encapsidated dsRNA segments (11), then the head-full
mechanism of replication is plausible. The capsids of the
partitiviruses might have an architecture and size similar to those of
the ancestral totiviruses, which may allow them to encapsidate one or
two identical molecules of dsRNA, as the C. parvum dsRNAs
are around one-half the size of the putative ancestral RNA.
Several important issues about the CPV still remain unknown. Both the
route of transmission and the relative importance of this virus for
parasite survival or pathogenicity are areas of research yet to be
explored. However, based on our data and what is known for other
related viruses, it is likely that extracellular, horizontal
transmission of the virus does not occur and the virus are passed only
during cell division and gamete fusion. Thus, it is likely that the
virus will be shown to have little or no negative effect on the host,
as in the case for partitiviruses in general.
| |
ACKNOWLEDGMENTS |
We acknowledge A. Q. Pauson for help with electron
microscopy. We also thank R. A. Consigli for critically reading
the manuscript and for helpful advice during experiments.
This work was supported by NIH grant 1RO1AI/DK42545-01A1 to S.J.U. and
N.V.K. and by EPA grant R825148-01-0 to S.J.U.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Ackert Hall,
Division of Biology, Kansas State University, Manhattan, KS 66506-4901. Phone: (785) 532-6639. Fax: (785) 532-6653. E-mail:
podolsk{at}ksu.edu.
Kansas Agricultural Experiment Station contribution no. 00-301-J.
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