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J Biol Chem, Vol. 275, Issue 2, 1485-1494, January 14, 2000
From the Department of Molecular Genetics and Microbiology,
University of Florida, Gainesville, Florida 32610-0266
Prior phenotypic analysis of a vaccinia virus
gene A18R mutant, Cts23, showed the synthesis of longer
than wild type (Wt) length viral transcripts during the intermediate
stage of infection, indicating that the A18R protein may act as a
negative transcription elongation factor. The purpose of the work
described here was to determine a biochemical activity for the A18R
protein. Pulse-labeled transcription complexes established from
intermediate virus promoters on bead-bound DNA templates were assayed
for transcript release during an elongation step that contained
nucleotides and various proteins. Pulse-labeled transcription complexes
elongated in the presence of only nucleotides were unable to release
nascent RNA. The addition of Wt extract during the elongation phase
resulted in release of the nascent transcript, indicating that
additional factors present in the Wt extract are capable of inducing
transcript release. Extract from Cts23 or mock-infected cells was
unable to induce release. The lack of release upon addition of Cts23 extract suggests that A18R is involved in release of nascent RNA. By
itself, purified polyhistidine-tagged A18R protein (His-A18R) was
unable to induce release; however, release did occur in the presence of
purified His-A18R protein plus extract from either Cts23 or
mock-infected cells. These data taken together indicate that A18R is
necessary but not sufficient for release of nascent transcripts. We
have also demonstrated that the combination of A18R protein and mock
extract induces transcript release in an ATP-dependent
manner, consistent with the fact that the A18R protein is an
ATP-dependent helicase. Further analysis revealed that the release activity is not restricted to a vaccinia intermediate promoter
but is observed using pulse-labeled transcription complexes initiated
from all three viral gene class promoters. Therefore, we conclude that
A18R and an as yet unidentified cellular factor(s) are required for the
in vitro release of nascent RNA from a vaccinia virus
transcription elongation complex.
Elongation and termination are key control points in both
prokaryotic and eukaryotic transcription (1). Transcriptional events
such as pausing, arrest, and termination are regulated by cis- and
trans-acting factors that decide the fate of a given transcript, either
elongation or termination. A paused complex, in which the 3' end of the
nascent RNA is retained in the polymerase catalytic site, can be
induced by a DNA sequence-specific element, such as a T-rich sequence,
or blockage of the RNA polymerase by so-called negative elongation
factors. Elongation of a paused complex may resume either spontaneously
or in response to positive elongation factors. An arrested complex, in
which the catalytic site of the polymerase has slipped backwards and
out of context with the 3' end of the nascent transcript, must cleave
the nascent RNA to return the 3' end to the catalytic site in order to
relieve arrest. Cleavage is an endogenous activity of the RNA
polymerase but is activated in response to trans-acting factors. A
transcription complex that releases its nascent transcript and
dissociates from the DNA template is considered terminated. Termination
may or may not require both cis-acting nucleic acid sequence elements and trans-acting factors. For example, the murine factor TTF-I binds to
a specific DNA sequence and blocks elongating RNA polymerase I allowing
another factor, PTRF (polymerase I transcript
release factor), to induce transcription
termination (2). In contrast, Drosophila factor 2 induces
transcription termination in a sequence-independent manner (3, 4).
Vaccinia virus has historically served as a superb model for
transcription (5). The prototypic Orthopoxvirus has a linear double-stranded DNA genome of 192,000 base pairs, which it replicates in the cytoplasm of the infected host cell. Due to the cytoplasmic site
of infection, the virus encodes the majority of the enzymatic machinery
necessary for both viral RNA and DNA metabolism. During infection,
viral genes are expressed in a transcriptional cascade encompassing
three stages as follows: early, intermediate, and late. Each stage
requires trans-acting factors for transcription initiation that are
synthesized in the previous stage thus providing the basis for
sequential regulation. Biochemical and biological experiments during
the past few years have shown elongation and termination of all three
transcriptional stages are also regulated events.
The general features of vaccinia early gene transcription elongation
and termination are fairly well understood. Early gene mRNA 3' ends
are formed by termination and not endonucleolytic cleavage (6, 7).
Termination depends on extrusion of a UUUUUNU RNA signal from the
ternary complex, as well as ATP hydrolysis (8). The model for early
termination proposes that vaccinia termination factor (identical to the
vaccinia virus capping enzyme) is poised to scan the RNA for the
termination signal. Recognition of the signal by vaccinia termination
factor activates the ATPase activity of NPH-I, a virus-coded
DNA-dependent ATPase, resulting in release of the nascent
transcript from the elongation complex (9, 10). Termination occurs
20-50 nt downstream of the termination signal (11, 12).
Less is understood concerning intermediate and late vaccinia
transcription elongation and termination, although these processes differ from early transcription and are clearly regulated. Genetic experiments imply the existence of both positive and negative virus-coded intermediate and late transcription elongation factors; however, these factors have not been characterized biochemically (13-16). The elongation complexes from intermediate and late gene promoters do not recognize early termination signals, indicating that
the factors necessary for intermediate and late termination may be
different from those utilized during early transcription termination.
Intermediate and late transcripts are also 3' heterogeneous for any
given gene, which may indicate that there is no sequence-specific termination signal as found in early gene termination.
Based on the phenotypic analysis of Cts23, a temperature-sensitive
mutant in the vaccinia gene A18R, we propose that the A18R protein functions as a negative transcription elongation factor or a
termination factor. Analysis of several vaccinia genes using Northern
blots, RNase protection, and reverse
transcriptase-PCR1 analysis
determined that mutations in the gene A18R result in readthrough transcription from intermediate promoters into downstream genes (16). These transcripts are longer than those synthesized during
a Wt infection. Previous analysis of the A18R gene
determined that it encodes a 56-kDa protein that is expressed
throughout infection and packaged in virions (17). The A18R protein is both a DNA helicase and a DNA-dependent ATPase, not
inconsistent with a role as a termination factor (18, 19).
To test the hypothesis that A18R is a transcription termination factor,
intermediate promoter-specific, pulse-labeled transcription complexes
established on bead-bound DNA templates were assayed for transcript
release during an elongation step that contained nucleotides and
various proteins. Release was analyzed by comparing transcripts present
in the supernatant to transcripts in the bead-bound fraction. Extract
from Wt-infected cells, but not mock- or Cts23-infected cells,
stimulated transcript release. We were also able to demonstrate transcript release using a combination of extract from mock-infected cells plus purified A18R protein. The release activity is dependent upon ATP hydrolysis, arrest of the transcription elongation complex, presence of the proteins prior to arrest of the complex, and is active
on all three classes of promoters.
Eukaryotic Cells, Viruses, and Bacterial Hosts--
A549 cells,
wild type vaccinia strain WR, the A18R temperature-sensitive mutant
Cts23, and the conditions for their growth, infection, and plaque assay
have been described previously (20-22). Escherichia coli
DE3 pLysS contains an isopropyl-1-thio- Plasmids--
All plasmids used for transcription are based on
pC2AT19 (24) containing a 375-nt G-less cassette cloned
into pUC13 with the total size approximately 3 kilobase pairs. pG8G,
pVGFG, and pCFW10 contain upstream of the 375-nt G-less cassette
promoters from the intermediate vaccinia virus gene G8R, the
early vaccinia gene C11R, and the late vaccinia gene
F17R (20, 25), respectively. pSB24 contains a synthetic
early promoter upstream from the 375-nt G-less cassette (26).
pG8GX is a derivative of pG8G that contains the vaccinia gene
G8R intermediate promoter upstream of a 3'-truncated, 94-nt G-less cassette derived from pC2AT19. The G8R
promoter and the 5' 92 nt of the pC2AT19 G-less
cassette were PCR-amplified from pG8G using the M13-40 universal
sequencing primer as the upstream primer and a downstream primer that
contained nucleotides 73-92 of the G-less cassette flanked with a
SmaI site, a ScaI site, and a BamHI
site. The PCR-amplified fragment was cleaved with EcoRI
(upstream) and BamHI (downstream) and cloned into the vector portion of pC2AT19, which had also been cleaved with
EcoRI and BamHI. The SmaI site at the
3' end of the resulting truncated G-less cassette serves to arrest
efficiently transcription of the G-less cassette, and the downstream
ScaI site was used for identification of the desired clone.
Accurate transcription of the pG8GX G-less cassette should yield an RNA
of approximately 94 nt in length.
p16A18 (19) contains the vaccinia virus gene A18R coding
sequence inserted in frame downstream from an amino-terminal
polyhistidine tag in the vector pET16b (Novagen).
Infected Cell Extracts for Transcription--
Confluent 100-mm
dishes of A549 cells were either mock-infected or infected with
vaccinia virus with a multiplicity of infection of 15 and incubated at
40 °C for 16 h in the presence of 10 mM hydroxyurea
or in the absence of drug. Extracts were prepared as described (20).
Briefly, vaccinia-infected cell monolayers were permeabilized with
lysolecithin, harvested, treated with micrococcal nuclease, clarified
by centrifugation, and stored at Immobilized DNA Templates--
All templates used for
transcription were immobilized by binding linearized plasmid DNA to
paramagnetic beads. One set of immobilized templates, including NpG8G,
NpSB24, and NpCFW10, were generated by linearization with
NdeI, which cleaves the DNA template 220 nt upstream from
the promoter. The resulting templates contain a 375-nt G-less cassette
and approximately 2400-nt DNA downstream from the G-less cassette. Two
additional shorter templates, N/VpG8G and N/VpG8GX, were constructed by
restriction digest with NdeI and VspI. The
resulting templates contain 220 base pairs DNA upstream from the G8R
intermediate promoter and either 540 or 260 base pairs downstream for
transcription (Fig. 1B). In all cases the cleaved DNA
fragments were end-filled with Klenow, dCTP, dGTP, dATP, and
biotin-16-dUTP (Roche Molecular Biochemicals). The biotinylated DNA was
separated from the free nucleotides using the High Pure PCR Product
Purification Kit (Roche Molecular Biochemicals). The DNA was eluted
from the column in 100 µl of TE (10 mM Tris-HCl, pH 8.0, 1 mM EDTA) and adjusted to 1 M NaCl. DNA
samples were then incubated with streptavidin-conjugated Dynabeads M280
(Dynal) in 1 M NaCl/TE for 30 min at 42 °C to generate
bead-bound templates. Beads with bound DNA were concentrated using a
magnet and washed twice in 1 M NaCl/TE, followed by two
washes in TE. The bead-bound DNA was stored in TE at 4 °C.
In Vitro Transcript Release Assay--
Transcription reactions
were done in three phases, initiation, pulse, and chase. Reactions (25 µl) contained a final concentration of 25 mM HEPES, pH
7.4, 4.5% glycerol, 80 mM KOAc, 5 mM
MgCl2, 1.6 mM DTT, 1 mM ATP, 5 µl
of bead-bound DNA template, and 15 µl of extract from
hydroxyurea-treated wild type vaccinia-infected cells. Reactions were
incubated at 30 °C for 10 min to form initiation complexes. The
pulse phase was initiated by adding 3 µl of a solution containing 11 mM ATP, 11 mM GTP, 6 mM UTP, and 6 µCi of [ Chromatography and Fractionation--
Extract from Wt or
Cts23-infected A549 cells was chromatographed on 2-ml columns of
phosphocellulose (Whatman) or Q-Sepharose (Amersham Pharmacia Biotech)
equilibrated in Buffer A (25 mM Tris-HCl, pH 7.5, 1 mM EDTA, 0.01% Nonidet P-40, 1 mM DTT, 10%
glycerol, 0.1 mM phenylmethylsulfonyl fluoride, 0.5 µg/µl leupeptin, and 0.7 µg/µl pepstatin A). All steps were
performed at 4 °C. Extract was loaded on the column, and the column
was washed in 4 ml of Buffer A, and 0.5 ml of flow-through fractions
were collected. Bound proteins were eluted stepwise with 4 ml each of
Buffer A containing 0.25, 0.5, and 1 M NaCl, and 0.5-ml
fractions were collected. Peak fractions were identified using the
Bradford protein assay, pooled, and dialyzed overnight against Buffer A
containing 50 mM NaCl. The fractions were stored at
Induction and Preparation of Extract from E. coli--
An
overnight culture of pLysS cells harboring the p16A18 plasmid was used
to inoculate 1 liter of L-broth, containing 50 µg/ml ampicillin and
34 µg/ml chloramphenicol. The culture was incubated at 37 °C to an
A600 of 0.5. Isopropyl-1-thio- His-Bind Column and Phosphocellulose Column--
The supernatant
was mixed for 1 h with 2 ml of nickel-nitrilotriacetic
acid-agarose resin (Qiagen) that had been equilibrated with lysis
buffer. The slurries were poured into a column and washed sequentially
with 20 ml of lysis buffer, 20 ml of binding buffer (5 mM
imidazole, 0.5 M NaCl, 20 mM Tris-HCl, pH 7.9, 5% glycerol), and 20 ml of wash buffer 1 (60 mM imidazole,
0.5 M NaCl, 20 mM Tris-HCl, pH 7.9, 5%
glycerol). Bound proteins were eluted with 20 ml of wash buffer 2 (200 mM imidazole, 0.5 M NaCl, 20 mM
Tris-HCl, pH 7.9, 5% glycerol) collecting 1-ml fractions. Peak
fractions were identified using the Bradford protein assay (Bio-Rad),
pooled, and dialyzed overnight against 1 liter of Buffer A. The
dialysate was applied to a 2-ml column of phosphocellulose that had
been equilibrated with Buffer A. The column was washed with 5 ml of
Buffer A containing 250 mM NaCl. Bound proteins were eluted
with 10 ml of Buffer A containing 500 mM NaCl collecting 0.5-ml fractions. Peak fractions were identified using the Bradford protein assay, pooled and dialyzed overnight against 4 changes, 1 liter
each, of a solution containing 40 mM Tris-HCl, pH 8, 20 mM KCl, and 40% glycerol. The enzyme was stored at
Polyhistidine-tagged vaccinia virus J3R protein, prepared in a fashion
similar to His-A18R, was a gift from Dr. Ying Xiang (University of Florida).
Western Blot Analysis--
Samples were separated by
electrophoresis on 10% SDS-PAGE. The proteins were transferred to
nitrocellulose in 25 mM Tris-HCl, 192 mM
glycine, 20% methanol at 4 °C overnight. Nitrocellulose filters
were incubated with monoclonal anti-A18 primary antibody (1:10,000)
(15), and the bound antibody was detected using polyclonal anti-mouse
horseradish peroxidase-conjugated antibody (1:5000; Amersham Pharmacia
Biotech) and enhanced chemiluminescence. Western blotting reagents
(Amersham Pharmacia Biotech) were used as described by the manufacturer.
To measure the activity of the vaccinia virus A18R protein
in vitro, we developed a transcription elongation assay
based on a previously described crude system for study of vaccinia
early, intermediate, and late gene transcription initiation (20).
Previous experiments showed that crude extracts prepared from cells
infected under normal conditions are competent for transcription of
early, intermediate, and late gene promoters. Since intermediate and late viral gene expressions are coupled to viral DNA replication, treatment of infected cells with a DNA replication inhibitor such as
hydroxyurea permits synthesis of only early gene products, including
intermediate transcription factors. Thus extracts prepared from cells
infected in the presence of hydroxyurea are competent for transcription
of intermediate promoters only (20). For most experiments, we chose to
use hydroxyurea-treated, intermediate promoter-specific extract for two
reasons. First, the best evidence that the A18R protein has elongation
factor activity is based on in vivo studies of intermediate
genes (16). Second, we wished to prepare extracts from A18R mutant
infections under non-permissive conditions while at the same time
circumventing undesirable pleiotropic effects of the A18R mutation.
Readthrough transcription from convergent intermediate promoters during
A18R mutant infections causes double-stranded RNA accumulation,
induction of the cellular 2-5A pathway, and ultimately activation of
RNase L (27, 28). Hydroxyurea treatment prevents 2-5A pathway
activation by preventing intermediate transcription. Cells infected
with A18R mutant virus at the non-permissive temperature produce less
than 10% of the normal amount of A18R protein due to instability of
the mutant protein (17). Thus preparation of extracts from A18R
mutant-infected cells at the non-permissive temperature provides an
A18R protein-deficient extract that is otherwise comparable to extract
from cells infected with Wt virus under identical conditions.
Extract from hydroxyurea-treated vaccinia-infected cells was used to
assay elongation and transcript release from linear bead-bound DNA
templates containing a vaccinia intermediate promoter as follows. First, transcription complexes were assembled during a preincubation reaction containing Wt extract, bead-bound template, and ATP. Transcription was then initiated, and the nascent transcript was radiolabeled by the addition of [ Transcription Is Specific for the Viral Promoter--
As an
initial test of the fidelity of the system, we sought to prove that the
intermediate promoter was accurately recognized. Two bead-bound
templates were designed such that transcription from the G8R
promoter to the downstream end of the template would generate
either 260 or 540 nt of RNA (Fig.
1B). Pulse-labeled elongation
complexes were established and analyzed on a denaturing polyacrylamide
gel (Fig. 1A, lanes 1 and 10). The transcripts were approximately 100 nt in length and were cut off on the
autoradiograph shown. Elongation was continued upon addition of
ribonucleotides during the chase phase and the transcripts synthesized
from each template were of the appropriate length, either 260 or 540 nt (Fig. 1A, lanes 2 and 11). At the end of the
chase phase, the bead-bound template was separated from the supernatant
using a magnet. Comparison of Fig. 1A, lanes 2 and
3 and lanes 11 and 12, indicates that
transcripts synthesized during a nucleotides-only chase reaction are
not released into the supernatant but remain associated with the
bead-bound template. Our protocol for generating elongation complexes
required extensive washing with 1 M salt, and we questioned
whether additional proteins could act on the isolated elongation
complexes to induce release of the nascent transcript from the
bead-bound template. Chase reactions were therefore performed in the
presence of nucleotides plus extract from mock-, Wt-, or the A18R
mutant Ts23-infected cells. The addition of extract from Wt-infected
cells resulted in the release of transcripts during a 20-min chase from
either template (Fig. 1A, compare lanes 6 and
7, and lanes 15 and 16). The percent
transcript release was analyzed by phosphorimagery, Fig. 1C.
Extract from neither mock-infected nor Ts23-infected cells was capable
of generating a significant amount of released transcripts (Fig.
1A, lanes 4 and 5, 8 and 9, 13 and
14, and 17 and 18, and Fig. 1C). In
summary, these experiments show that initiation in vitro
occurs specifically at the viral intermediate promoter. These data also
suggest that transcript release in Wt extract is due to the presence of
A18R protein, which is absent in Ts23 extract.
Release Does Not Require the Presence of A18R during
Initiation--
In the previous experiment, Wt extract was used to
generate the transcription complexes formed during the preincubation
step. To determine whether factors specific to a Wt extract and present in the washed elongation complex contributed to release, we compared transcription complexes formed using either Wt or Ts23 extract during
the preincubation and pulse steps (Fig.
2A, Wt or
Ts23 PIC). Transcription complexes were formed on linearized
bead-bound NpG8G, a template that contains approximately 3 kilobase
pairs of sequence downstream from the G8R promoter. These complexes were chased in the presence of unlabeled ribonucleotides or nucleotides plus mock, Wt, or Ts23 extract (Fig. 2A). Both complexes
show similar levels of transcript release in response to the addition of Wt extract (Fig. 2A, compare lanes 5 and
6, 13 and 14, and Fig. 2B). Therefore,
Wt or Ts23 extracts are equally competent for transcription complex
assembly and initiation. Therefore, Wt extract was used to generate
transcription complexes for all release assays.
Transcript Release Is Time- and
Concentration-dependent--
To determine the kinetics of
release, we performed a chase time course. Pulse-labeled elongation
complexes were formed, and samples were taken at various time points
during elongation. Similar kinetics of elongation were observed with
the addition of ribonucleotides alone or in combination with Wt or Ts23
extract (Fig. 3A). Release is
detected with the addition of Wt extract (Fig. 3A, lanes
13-24), and the level of release increases linearly as a function
of time (Fig. 3B). Longer incubation times do not result in
more than 60% release. Ts23 extract also resulted in a linear increase
in release activity with time that was measurably above the
nucleotides-only control but significantly less than Wt (Fig. 3A,
lanes 25-36, and Fig. 3B). The lower level of release
observed with addition of Ts23 extract could represent nonspecific
release or result from the lower level of A18R protein in Ts23 extract.
In summary, release activity is significantly diminished in a Ts23
extract throughout a time course substantiating our hypothesis that
release is specific to A18R protein.
We next performed an extract titration to determine the optimal
quantity of extract for efficient release. Transcription complexes were
formed from Wt extract, washed, and increasing concentrations of mock,
Wt, or Ts23 extract were tested in combination with ribonucleotides for
release during a 20-min chase reaction. Increased transcript release
occurred as the quantity of Wt extract was increased (Fig. 4A, lanes 11-18, and Fig.
4B); however, no effect on release was observed with
increasing quantities of either mock or Ts23 extract (Fig. 4A,
lanes 3-10 and lanes 21-28, and Fig. 4B).
These results further support the hypothesis that A18R is important for
transcript release.
Transcript Release Is Complemented by Crude Fractions from Wt
Extract--
In an attempt to correlate the release activity achieved
by the addition of Wt extract with the presence of A18R protein, a
crude fractionation protocol was employed. Extracts were prepared from
either Wt- or Ts23-infected cells and fractionated on phosphocellulose and Q-Sepharose columns separately. Columns were eluted stepwise with
0.25, 0.5, and 1 M NaCl. Each Wt extract fraction was
analyzed by PAGE (data not shown) and by Western blot analysis using an anti-A18 monoclonal antibody (Fig. 5,
B and C). As demonstrated by Western blot, A18R
protein fractionated into the 0.5 M phosphocellulose fraction and the 0.25 M Q-Sepharose fraction (Fig.
5B, 0.5 M and Fig. 5C, 0.25 M). Each fraction was assayed for release during a chase
reaction from pulse-labeled elongation complexes (Fig. 5A).
As controls, chase reactions containing ribonucleotides alone or
ribonucleotides plus mock, Wt, or Ts23 extract were performed (Fig.
5A, lanes 1-8 and lanes 13 and
14). As previously shown, only the addition of Wt extract is
capable of inducing transcript release (Fig. 5A, lanes 5 and
6 and lanes 13 and 14, and Fig. 5D). Two of the column fractions were capable of inducing
release, the 0.5 M phosphocellulose fraction and the 0.25 M Q-Sepharose fraction (Fig. 5A, lanes 23 and
24 and lanes 31 and 32). These same
fractions contain A18R protein as judged by Western blot analysis (Fig.
5B, 0.5 M, and Fig.
6C, 0.25 M). The
phosphocellulose wash fraction, Fig. 5A, lanes 19 and
20, also showed release in this experiment. This result was
not reproducible in subsequent release experiments done with the same
material. For comparison, Ts23 extract was also fractionated by the
same protocol (data not shown). A18R protein was not detected by
Western blot in extract from Ts23-infected cells (Fig. 5B,
E122297) nor any Ts23 extract fractions from the
phosphocellulose or Q-Sepharose columns (data not shown). In addition,
no significant release was detected with the addition of fractions from
Ts23 extract. The fractionation protocol described here provides
circumstantial evidence for the role of A18R protein in transcript
release. However, these are crude fractions that contain many more
proteins than just A18R. Conclusive evidence for the role of A18R must
be obtained with a purified fraction or purified protein.
Release Occurs from a Stalled Elongation Complex and Can Be
Complemented by His-A18R and a Cellular Factor--
In all experiments
described above release occurs predominantly at the downstream end of
the template where the template is joined to a paramagnetic bead. In
order to eliminate the possibility that the observed release is an
artifact due to the presence of the bead, we conducted experiments
designed to promote release in the middle of a DNA template. We refer
to this protocol as a "mid-template" assay. This assay is designed
to reflect the situation in vivo where a transcription
complex will terminate despite the presence of additional template
downstream. We accomplished this by arresting transcription at the end
of a 375-nt G-less cassette downstream from the intermediate G8R
promoter present within the 3-kilobase pair template NpG8G.
Pulse-labeled elongation complexes formed on NpG8G were washed and
elongated either in the absence of GTP (with all other nucleotides
present) (data not shown) or in the presence of 3'-OMeGTP and all other
ribonucleotides (Fig. 6A) with additional proteins provided
as indicated. The addition of 3'-OMeGTP arrests the elongation complex
at the end of the G-less cassette where the first GTP would be
incorporated (Fig. 6A, lane 1) resulting in the synthesis of
an approximately 400-nt transcript. Addition of Wt extract during the
chase reaction resulted in release of the transcript at the end of the
G-less cassette (Fig. 6A, lanes 5 and 6). Release
did not occur with mock or Ts23 extract (Fig. 6A, lanes 3 and 4 and lanes 7 and 8). Similar
results were obtained when the complex was elongated in the absence of
GTP (data not shown). In other experiments not shown, we attempted to
induce release by first elongating to the end of the G-less cassette in
the absence of added extract and then adding extract to the arrested
complex. We also tried to induce mid-template release by slowing
elongation using reduced concentrations of UTP. In neither protocol did
we observe significant mid-template release. These results show
definitively that release can be induced in the middle of the template
but strongly suggest that release can only be accomplished on a complex
that is stalled. Furthermore, the results indicate that in order to
observe release, release factors need to be present during elongation,
before the polymerase stalls.
In order to determine definitively whether A18R is required for
transcript release, we attempted to complement the defect in release
activity observed in Ts23 extracts by addition of purified A18R
protein. Pulse-labeled elongation complexes were formed and assayed
during the chase phase with His-A18R protein. His-A18R was expressed in
E. coli and purified over nickel and phosphocellulose columns as described under "Experimental Procedures." The addition of ribonucleotides, Ts23 extract, or purified His-A18R protein alone to
the chase was not sufficient for transcript release (Fig. 6A,
lanes 11 and 12, and Fig. 6B). Addition of
increasing amounts of His-A18R protein to the Ts23 extract resulted in
increasing release equivalent to the levels of His-A18R protein (Fig.
6A, lanes 15-24, and Fig. 6C). As a control, a
similar titration of purified His-J3R protein (J3R is a vaccinia
2'-O-methyltransferase and poly(A) polymerase processivity
factor) expressed in E. coli was tested in combination with
Ts23 extract (data not shown). The transcription complexes did not
release the nascent RNA in the presence of His-J3R protein. These
results demonstrate that the release defect observed in Ts23 extract
can be complemented by purified A18R protein.
The results described above show that purified A18R protein is
necessary but not sufficient for transcript release. To determine whether the additional factors required for release are viral or
cellular in nature, extract from mock-infected cells was tested in the
release assay. Mock extract alone does not produce a significant level
of released transcripts (Fig. 6A, lanes 3 and 4).
A titration of His-A18R in combination with mock extract induced more
efficient release than His-A18R plus Ts23 extract (Fig. 6A,
compare lanes 27-36 and lanes 15-24, and Fig.
6C). The simplest explanation for these observations is that
a cellular factor(s) is needed in addition to A18R for transcript release.
Release Requires ATP Hydrolysis--
It has been shown previously
that A18R possesses a DNA-dependent ATPase activity and
that the enzyme can readily use dATP as a substrate rather than ATP
(19). We therefore hypothesize that any stage of transcription that
requires A18R would also be ATP-dependent. Assessing the
role of ATP hydrolysis in transcription is complicated by the
requirement for ATP as a substrate for the polymerase during
elongation. Therefore, we examined the ATP dependence of the release
activity by replacing the ATP in the chase reaction of the mid-template
assay with the non-hydrolyzable ATP analog, AMPPNP. AMPPNP can be used
as a substrate for the vaccinia RNA polymerase, and substitution
results in efficient synthesis of long transcripts (Fig.
7A, compare lanes 1 and 3). Substitution of ATP with dATP, a hydrolyzable ATP
analog that cannot be efficiently used for synthesis, yielded
transcripts that are much shorter in length (Fig. 7A,
compare lanes 1 and 5). Transcription elongation in the presence of dATP can be rescued with the provision of AMPPNP (Fig. 7A, lane 7). The combination of dATP and AMPPNP
satisfies the energy requirement and provides a nucleotide capable of
being incorporated into the nascent RNA chain. We then assayed the
effect of AMPPNP substitution on release in combination with mock
extract (Fig. 7A, Mock), Wt extract (Fig.
7A, Wt), or mock extract plus His-A18R protein
(Fig. 7A, Mock+A18). As controls, the level of release in response to a given extract was assayed using ATP or dATP
alone or the combination of AMPPNP and dATP and quantitated as
described previously (Fig. 7A, lanes 9 and 10, 15 and 16, 17 and 18, 23 and 24, 25 and
26, and 31 and 32, and Fig.
7B). Since the extracts added during the chase reactions
contain some endogenous ATP, substitution of ATP with dATP in these
controls did not restrict elongation as much as in chase reactions done
in the presence of nucleotides alone. Substitution of ATP with AMPPNP
did not have an effect on the low level of release detected in the
presence of mock extract (Fig. 7A, compare lanes
9 and 10 and lanes 11 and 12, and
Fig. 7B). On the other hand, replacing ATP with AMPPNP severely inhibits transcript release when assayed with Wt extract (Fig.
7A, compare lanes 17 and 18 and lanes 19 and 20, and Fig. 7B) or mock extract plus His-A18R protein (Fig.
7A, compare lanes 25 and 26 and
lanes 27 and 28, and Fig. 7B).
Therefore, we conclude that A18R-catalyzed transcript release is an
ATP-dependent event.
A18R-dependent Transcript Release Occurs from All
Vaccinia Promoters--
The previous experiments were all carried out
using a template that contained a vaccinia intermediate promoter.
However, further characterization of the mechanism by which A18R
functions in transcription termination requires analysis of the
specificity of the release activity for the different stages of
transcription. We therefore performed A18R-dependent
transcript release assays using templates that contain a promoter from
each of the three stages of transcription. Each template is precisely
analogous to the intermediate promoter containing template described
above and contains a 375-nt G-less cassette downstream from an early,
intermediate, or late gene promoter. In order to assay transcription
from early and late promoter-driven initiation complexes, we used
extract from Wt-infected cells that were not treated with hydroxyurea
as a source of activity for forming pulse-labeled elongation complexes.
Intermediate promoter-driven complexes can be formed using extract from
either hydroxyurea-treated or non-hydroxyurea-treated Wt-infected
cells. The mid-template assay was performed using complexes initiated
from each promoter and elongated in the presence of ATP, CTP, UTP, and
3'-OMeGTP, as well as additional proteins. The ability of each complex
to release the nascent RNA was determined using mock extract plus His-A18R protein. In the case of each promoter, release occurred only
in the presence of both mock extract and His-A18R protein (Fig.
8A, lanes 9 and 10, 19 and 20, 29 and 30, 39 and 40, 49 and 50, and Fig. 8B). Although the
absolute level of transcription in non-hydroxyurea extract is less than
the hydroxyurea extract, the amounts of released RNA observed from the
intermediate promoter template are equivalent (Fig. 8, A and
B, NpG8G(+) and NpG8G( Previous research has implicated the vaccinia virus
A18R gene product in 3' end formation of vaccinia virus
intermediate stage transcripts. Specifically, mutations in the
A18R gene result in synthesis of readthrough transcripts at
intermediate times during infection implying that the A18R protein acts
as a negative elongation or termination factor (16). We developed an
immobilized template assay to study the effects of the A18R protein on
elongation and release of nascent RNA from vaccinia virus transcription
complexes. The results of this study allow us to draw several major
conclusions. First, nascent transcript release requires A18R protein
and an additional activity that can be provided by either mock extract or extract from A18R mutant (Cts23)-infected cells. Second, the A18R
protein and/or the cellular factor must be present during elongation in
order for release to occur. Third, release requires a stalled
transcription elongation complex. Fourth, transcript release requires
ATP hydrolysis. Finally, the transcript release activity provided by
mock extract and A18R protein, or Cts23 extract and A18R protein,
can catalyze release of transcripts synthesized from promoters
representing all stages of vaccinia transcription.
A18R protein alone cannot induce transcript release but requires an
additional factor that can be provided by extract from either mock or
A18R mutant-infected cells. The activity is heat-labile as demonstrated
by the abolishment of transcript release activity after heating the
extract for 10 min at
65 °C.2 The simplest
explanation for these observations is that a cellular factor(s) is
needed in addition to A18R for transcript release. Another possible
explanation is that the factor(s) from Cts23-infected cells and the
factor(s) from mock-infected cells are different. Extract from
mock-infected cells could be providing an analogous activity or an
activity that abolishes the need for the viral factor. The proof of
either hypothesis requires that this factor be purified and identified
from uninfected cell extract and potentially Cts23-infected cell
extract. Participation of cellular factors in vaccinia virus
transcription is not without precedence. Two groups have reported
evidence for the requirement of cellular factors, VLTF-X and LPBP, for
late transcription initiation (29-31). Whether these are the same
factor or two different factors is not known. An additional factor,
VITF-2, is provided by the nucleus of uninfected cells and is required
for intermediate transcription initiation in vitro (32).
Taking into account the fact that A18R and the cellular factor act on
polymerase complexes initiated from all three stages of transcription,
either or both of the previously mentioned cellular factors could be
the activity we have discovered. Transcript release was also
complemented with partially purified fractions from Wt-infected cells.
Additional mock extract was not required for release to occur,
providing evidence that the factor was present in the fractions.
Therefore, the factor either cofractionated with A18R due to intrinsic
properties or it was bound to A18R.
We have observed that the A18R protein and/or the cellular factor must
be present during elongation in order for transcript release to occur.
The factors need not be present during initiation, because washed
elongation complexes that are incapable of transcript release can be
induced to release RNA by subsequent addition of A18R protein and the
cellular factor. Whether both A18R and the cellular factor must be
present during elongation remains to be determined. These results
suggest that at least one of the two factors may become associated with
the elongation complex after initiation and "ride" the complex,
poised for arrest and termination. This phenomenon is not without
precedent. For example, the eukaryotic elongation factors TFIIF (33),
Elongin (34), and ELL (35) and the prokaryotic elongation factors GreA
(36), Q (37), and N (38) must all form an association with their
cognate elongation complex as a prerequisite to activity (1).
We have observed that the elongation complex must be stalled in order
for transcript release to occur. Specifically, detection of transcript
release in vitro requires arrest of the polymerase induced
by transcribing to a bead attached to the downstream end of a DNA
template or by transcribing to the end of a G-less cassette in the
absence of GTP or in the presence of 3'-OMeGTP. We have tested
elongation through both bacterial plasmid sequences and authentic viral
sequences, and we have observed no effect of specific nucleic acid
sequence on transcript release in vitro. In vivo, transcripts synthesized from either intermediate or late genes are
heterogeneous in length, consistent with a sequence-independent termination event. The possibility exists that other factors in vivo may act to either pause or arrest the transcription complex prior to termination. Thus termination of post-replicative
transcription in vaccinia may resemble murine RNA polymerase I
termination, where transcription is blocked by TTF-I prior to
transcript release catalyzed by PTRF (2, 39).
A18R shares a requirement for ATP hydrolysis with several transcription
termination factors from both prokaryotic and eukaryotic systems (1,
19). These factors include Rho (40), La (41), factor 2 (42), and NPH-I
(43). Each protein requires a different nucleic acid cofactor for its
activity. The A18R ATPase activity is stimulated by single-stranded
DNA, double-stranded DNA, and DNA-RNA hybrids, similar to NPH-I, factor
2, and La, respectively. Of these termination factors only Rho and A18R
have identified helicase activity. The other proteins contain helicase
motifs; however, no helicase activity has been described. The weak
helicase activity of A18R is capable of unwinding a DNA duplex that is 20 nt or less (18). The protein is also capable of binding
single-stranded DNA in the absence of ATP. Whereas our results
demonstrate that transcript release is dependent upon ATP hydrolysis,
this could be the activity of A18R or the unidentified cellular factor.
To determine the ATP-dependent factor, we attempted to
purify A18R mutant protein (D206N) for analysis in the transcript
release assay. This mutation results in a single amino acid change
within the Walker B box sequence proposed to be associated with ATP
binding and should have the effect of reducing the ATPase activity of A18R. This mutation destabilized the protein preventing its
purification for use in the transcript release assay. Based on these
findings we propose that during elongation the A18R protein binds to
the single-stranded non-template DNA strand in the region of the
transcription bubble (44) and awaits activation of both ATPase and
helicase activities to induce transcript release. This activity would
be similar to that proposed for NPH-I, the energy coupling factor required for vaccinia early gene transcription termination. NPH-I is
postulated to bind to the non-template DNA strand within the transcription bubble. Recognition of the early termination signal by
vaccinia termination factor would activate the ATPase activity of NPH-I
resulting in the release of the nascent RNA (9, 10).
The observation that the A18R protein catalyzes transcript release from
early as well as late transcription complexes suggests that A18R acts
on all three classes of transcription in vivo. Early
transcription elongation complexes are significantly different than
intermediate and late transcription complexes both in structure and
function (5). Early transcription is catalyzed entirely by enzymes
packaged in the virion and presumably occurs within uncoated viral core
particles in vivo. By contrast, intermediate and late
transcription occurs in viral DNA-containing cytoplasmic centers of
replication called virosomes. Early complexes contain RAP94, a viral
factor that is required for early transcription initiation and that
remains strongly associated with the early elongation complex, while
intermediate and late transcription complexes probably lack this
factor. Early transcripts are homogeneous in length, resulting from
recognition of a cis-acting RNA sequence by the vaccinia virus capping
enzyme and NPH-I, whereas intermediate and late transcripts are
heterogeneous in length. Nevertheless, the fact that the A18R protein
is synthesized throughout infection and packaged within virions
supports a role for A18R during early transcription. A18R mutants do
not affect early viral transcription in vivo (28), but this
is not atypical for mutations in vaccinia virion enzymes. For example,
temperature-sensitive mutants in the virion early transcription
initiation factor VETF (45), the RNA helicase NPH-2 (46), the mRNA
capping enzyme (47), and the RNA polymerase (48, 49) have shown no
pronounced effect on early transcription in vivo. Although
the mechanism of early transcription termination is reasonably well
understood, a role for A18R as an early transcript release factor has
not been ruled out.
Genetic and biochemical evidence suggests that both vaccinia
intermediate and late gene transcription elongation are regulated by
several viral genes in addition to A18R. The fact that both intermediate and late transcripts possess heterogeneous 3' ends implies
a similar mechanism of transcription termination for both gene classes.
Mutation of either gene G2R (14) or
J3R3 results in
synthesis of 3'-truncated intermediate and late viral mRNAs,
implying that each of these gene products exerts positive transcription
elongation factor activity on both intermediate and late viral genes.
Mutations in either G2R (13) or
J3R4 suppress
A18R mutations, strongly suggesting that all three genes function in the same pathway. Interestingly, the J3R gene
product has previously been shown to encode a protein with both
2'-O-methyltransferase and poly(A) polymerase processivity
activities (50); no distinct biochemical activity has yet been
identified for the G2R protein. One additional protein, the viral
H5R gene product, has been shown to associate directly with
the G2R protein (15). The H5R protein is an abundant phosphoprotein
found associated with virosomes (51), and it has been shown to
stimulate late viral transcription in vitro (52). Finally,
evidence exists that the A18R, G2R, and H5R proteins are all associated
either directly or indirectly as a complex in vivo (15). In
summary, the evidence to date suggests that intermediate and late gene
transcription elongation in vaccinia is controlled by a complex of
viral and cellular factors possessing both positive and negative
elongation factor activities. The powerful combination of genetics and
the in vitro system described here provide us with an
opportunity to investigate the activities of the individual components
of this transcription elongation complex. Vaccinia has often served as
a valuable model system for transcription in higher eukaryotes, and
thus these studies of vaccinia transcription elongation and termination
may provide insight into the same processes in mammalian cells.
We thank Jackie Lewis for expert technical
assistance; William McDonald for protein fractionation protocols; and
Mingyi Liu, David Price, Richard Moyer, and Penni Black for helpful
discussions while this work was in progress.
*
This work was supported by National Institutes of Health
Grant AI18094 (to R. C. C.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
2
C. A. Lackner and R. C. Condit,
unpublished observations.
3
Y. Xiang, D. Latner, and R. C. Condit,
manuscript in preparation.
4
D. Latner, Y. Xiang, J. P. Condit, J. I. Lewis, and R. C. Condit, manuscript in preparation.
The abbreviations used are:
PCR, polymerase
chain reaction;
nt, nucleotide;
DTT, dithiothreitol;
PAGE, polyacrylamide gel electrophoresis;
Wt, wild type;
AMPPNP, adenosine 5'-(
Vaccinia Virus Gene A18R DNA Helicase Is a Transcript
Release Factor*
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-D-inducible chromosomal copy of the bacteriophage T7 RNA polymerase gene (23).
70 °C. Total protein
concentration was determined by the Bradford protein assay
(Bio-Rad).
-P32]CTP (~3000 Ci/mmol stock) such that
the final concentration is 2.1 mM ATP, 1.1 mM
GTP, 0.6 mM UTP, 22.3 mM HEPES, pH 7.4, 4% glycerol, 71.4 mM KOAc, 4.5 mM
MgCl2, and 1.4 mM DTT in a total of 28 µl.
These reactions were then incubated at 30 °C for 30 s. The
reactions were stopped by placing the tube on a magnet on ice. The
pellets were washed with 1-1.5 pulse reaction volumes of high salt
transcription buffer (5 mM MgCl2, 25 mM HEPES, pH 7.4, 1.6 mM DTT, 1 M
KOAc, and 7.5% glycerol), followed by three washes in 1-1.5 pulse
reaction volumes of low salt transcription buffer (5 mM
MgCl2, 25 mM HEPES, pH 7.4, 1.6 mM
DTT, 80 mM KOAc, 200 µg/ml bovine serum albumin, and
7.5% glycerol). The chase phase was done by adding to the resuspended
complexes a mixture of NTPs, extract, and proteins in a final volume of
25 µl containing 25 mM HEPES, pH 7.4, 4.5% glycerol, 80 mM KOAc, 5 mM MgCl2, 1.6 mM DTT, 600 µM ATP, 600 µM GTP
or 10 µM 3'-OMeGTP, 600 µM UTP, 1.2 mM CTP, 20 units RNasin, and purified protein or extract as indicated. Chase reactions were performed at 30 °C for various times. The beads were concentrated using a magnet, and the 25-µl supernatant was removed to a separate tube. One hundred seventy five
microliters of "PK mix" (114 mM Tris-HCl, pH 7.5, 14 mM EDTA, 150 mM NaCl, 1.14% SDS, 40 µg of
glycogen, 230 µg/ml proteinase K) was added, and reactions were
incubated at 37 °C for 30 min. Reactions were extracted once with
175 µl of phenol/chloroform. Nucleic acids were precipitated by
addition of 50 µl 10 M ammonium acetate and 150 µl
isopropyl alcohol, incubation at room temperature for 30 min, and
centrifugation for 20 min. Pellets were washed once with 70% ethanol,
dried, and resuspended in 10 µl of formamide loading buffer. Samples
were denatured at 90 °C for 3 min and loaded on a 6% 8 M urea-PAGE. Gels were fixed, dried, and analyzed by
autoradiography and phosphorimagery. Released transcripts were expressed as a percentage derived by dividing the quantity of transcripts in the supernatant by the total quantity of transcripts in
both the supernatant and associated with the beads.
20 °C.
-D-GALACTOPYRANOSIDE was added to a
final concentration of 1 mM, and the culture was incubated
at 37 °C for 4 h. The cells were pelleted and stored at
70 °C overnight. All subsequent procedures were performed at
4 °C. The thawed bacterial pellet was resuspended in 50 ml of lysis
buffer (50 mM Tris, pH 7.5, 0.15 M NaCl, 10%
sucrose) plus a final concentration of 50 µg/ml lysozyme and 0.1%
Triton X-100. The cells were sonicated at 4 °C for eight sequences
consisting of 15 s on and 45 s off. Insoluble material was
removed by centrifugation for 30 min at 18,000 rpm in a Sorvall SS34
rotor at 4 °C. For purification of the soluble A18R protein, the
supernatant was then chromatographed on a His-Bind (Novagen) column and
phosphocellulose column as described below.
20 °C. The His-A18R protein preparation was greater than 90% pure
as judged by PAGE and displayed DNA-dependent ATPase
activity of 10,000 nmol of ATP hydrolyzed per min per µg of protein,
equivalent to previously reported preparations (19).
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-32P]CTP, ATP, GTP,
and UTP during a short, 30-s pulse reaction. The ternary complexes,
consisting of the DNA template, the transcription apparatus, and the
radiolabeled nascent RNA, were stripped of nonspecific proteins and
unincorporated nucleotides during three washes in high salt
transcription buffer followed by three washes in low salt transcription
buffer. An elongation reaction was then done by adding to the
resuspended complexes a chase mixture containing NTPs, extract, and
proteins. Following the elongation reaction the beads were concentrated
using a magnet; the supernatant was removed to a separate tube, and the
labeled RNA in each fraction was analyzed on a denaturing
polyacrylamide gel. Released transcripts were expressed as a percentage
derived by dividing the quantity of transcripts in the supernatant by
the total quantity of transcripts in both the supernatant and
associated with the beads.
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Fig. 1.
Transcription is promoter-specific.
A, autoradiogram of in vitro transcript release
assay. Transcription complexes were formed from Wt extract on
immobilized N/V pG8GX or N/V pG8G DNA that contain the vaccinia
G8R intermediate promoter. Following a 30-s pulse reaction
(Pulse), labeled complexes were washed in transcription
buffer, and elongation was continued in the presence of 0.6 mM ATP, 0.6 mM GTP, 0.6 mM UTP, and
1.2 mM CTP alone (NTP) or with additional 7.5 µg mock extract (Mock), Wt extract (Wt), or
Ts23 extract (Ts23) for 20 min. The bead-bound RNA
(B) was separated from released RNA (S) using a
magnet. These transcripts were analyzed by 6% 8 M
urea-PAGE. Sizes, in nt, are shown on the left.
B, diagram of the DNA templates used for transcription. The
DNA template (line) contains a biotinylated ATP incorporated
at both the 5' and 3' end, which anchors the DNA to a
streptavidin-coated magnetic bead (circles). The bead is
anchored 220 nt from the promoter at the 5' end of the template. The
transcription unit consists of the G8R intermediate promoter
(arrow) fused to either 260 or 540 nt of downstream DNA.
C, graphic representation of the percent transcript release
for each reaction in A. Bound and released transcripts were
quantitated using a PhosphorImager; the quantity of transcripts in the
supernatant was divided by the quantity of transcripts on both the
beads and in the supernatant and expressed as a percentage.
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Fig. 2.
A18 is not required for initiation in
vitro. A, transcription complexes were
formed on immobilized NpG8G DNA containing the vaccinia G8R
intermediate promoter and extracts from either Wt- (Wt
PIC) or Ts23 (Ts23 PIC)-infected cells. Transcription
was performed as described in Fig. 1 and released transcripts
(S) were separated from bound transcripts (B) and
analyzed by 6% 8 M urea-PAGE. Sizes in nt are shown at the
right. B, graphic representation of the percent
transcript release for each reaction in A.
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Fig. 3.
Time course of elongation in a chase
reaction. A, pulse-labeled transcription elongation
complexes were formed on NpG8G bead-bound template using extract from
Wt-infected cells. Complexes were washed in 1 M
transcription buffer, and transcription was continued in the presence
of 0.6 mM ATP, 0.6 mM GTP, 0.6 mM
UTP, and 1.2 mM CTP alone (NTPs) or in addition
to 30 µg of Wt extract (Wt) or Ts23 extract
(Ts23) for 1, 2.5, 5, 10, 15, and 20 min. Released
transcripts in the supernatant (S) and bound transcripts
associated with the bead-bound template (B) were separated
and analyzed by denaturing 6% PAGE. B, graphic
representation of the percent transcript release for each reaction in
A.
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Fig. 4.
Add-back extract titration.
A, elongation complexes were generated as detailed in Fig. 3
(Pulse) and washed in 1 M transcription buffer,
and transcription was continued for 20 min in the presence of 0.6 mM ATP, 0.6 mM GTP, 0.6 mM UTP, and
1.2 mM CTP alone (NTPs). Other reactions were
supplemented with increasing concentrations of mock extract
(Mock), Wt extract (Wt), or Ts23 extract
(Ts23), as follows: 0.5 µg (lanes 4 and
5, 12 and 13, and 23 and
24), 3 µg (lanes 6 and 7, 14 and
15, and 25 and 26), 15 µg
(lanes 8 and 9, 16 and 17, and
27 and 28), 30 µg (lanes 10 and
11, 18 and 19, and 29 and
30). B, bound; S, supernatant.
B, percent transcript release plotted against the quantity
of mock, Wt, or Ts23 extract.
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Fig. 5.
Wt extract fractionation. A,
pulse-labeled elongation complexes were generated as detailed in Fig.
3. Transcript release was assayed with the addition of 0.6 mM ATP, GTP, UTP, and 1.2 mM CTP
(NTPs) or NTPs and 30 µg of mock (Mock), Wt
(Wt and E080798), or Ts23 (Ts23)
extract, 1.32 µg of vaccinia virus (vv) His-A18 protein
(A18), or 5 µg of each fraction from the phosphocellulose
and Q-Sepharose columns during a 20-min chase reaction. E080798 was the
extract fractionated on the phosphocellulose and Q-Sepharose columns.
B, bound; S, supernatant. B and
C, Western blot analysis. Monoclonal -A18R antibody was
used to probe a 10% SDS-PAGE containing 3.125 µg of each sample from
the phosphocellulose and Q-Sepharose columns, 7.5 µg either Wt
extract (E080798) or Ts23 extract (E122297), and
0.3 µg of purified vvHis-A18 protein. D,
graphic representation of the percent transcript release for each
sample in A.
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Fig. 6.
Release occurs from a stalled elongation
complex and can be complemented by His-A18 and a cellular factor.
A, pulse-labeled transcription elongation complexes were
formed on NpG8G bead-bound template using extract from Wt-infected
cells. Complexes were washed in 1 M transcription buffer,
and transcription elongation was continued to the end of the G-less
cassette using 0.6 mM ATP, UTP, 1.2 mM CTP, and
0.01 mM 3'-OMeGTP alone (NTPs), or in addition
to 30 µg of mock-infected extract (Mock), Wt extract
(Wt), or Ts23 extract (Ts23). Transcripts
synthesized in the presence of 3'-OMeGTP are approximately 400 nt in
length. Purified recombinant His-A18 protein was used at 300 ng either
alone (A18) or in combination with Ts23 or mock extract.
DB, A18 storage buffer; B, bound; S,
supernatant. B and C, graphic representation of
the percent transcript release for each sample in A.
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Fig. 7.
Transcript release requires ATP
hydrolysis. A, ternary complexes were formed and
elongated as described in Fig. 6. The standard elongation reaction
included 0.6 mM ATP, UTP, 0.01 mM 3'-OMeGTP,
and 1.2 mM CTP (A, C, G, U). In other
reactions, adenosine analogs AMPPNP (AMPPNP) and dATP
(dA) replaced ATP as indicated, each at 0.6 mM
concentration. Released transcripts (S) were separated from
bound transcripts (B) and analyzed as described previously.
B, released and bound transcripts are expressed as percent
transcript release.
)). Additionally, the absolute level of transcription using the various promoters is different, but release does occur and is specific for the
presence of mock extract plus His-A18R protein. These results indicate
that the activity provided by mock extract and His-A18R protein acts on
complexes initiated from all three promoters, early, intermediate, and
late, implying that A18R could serve as a release factor at each stage
in vivo.
View larger version (52K):
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Fig. 8.
A18-dependent transcript release
occurs from all vaccinia promoters. A, transcription
elongation complexes were formed as described in Fig. 6 using templates
containing an early promoter (NpSB24 and NpVGFG),
an intermediate promoter (NpG8G), or a late promoter
(NpCFW10). The (+) indicates that the transcription
complexes were generated using extract from hydroxyurea-treated
Wt-infected cells. The ( ) indicates that the transcription complexes
were generated using extract from non-hydroxyurea-treated Wt-infected
cells. B, bound; S, released. B,
released and bound transcripts are expressed as percent transcript
release.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
ACKNOWLEDGEMENTS
FOOTNOTES
To whom correspondence should be addressed. Tel.: 352-392-3128;
Fax: 352-392-3133; E-mail: condit@mgm.ufl.edu.
ABBREVIATIONS
,
-imino)triphosphate.
REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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