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Plant Physiol, July 2001, Vol. 126, pp. 930-938
Silencing on the Spot. Induction and Suppression of RNA Silencing
in the Agrobacterium-Mediated Transient Expression
System1
Lisa K.
Johansen and
James C.
Carrington*
Institute of Biological Chemistry, Washington State University,
Pullman, Washington 99164-6340
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ABSTRACT |
The Agrobacterium-mediated transient expression
assay in intact tissues has emerged as a rapid and useful method to
analyze genes and gene products in plants. In many cases, high levels of active protein can be produced without the need to produce transgenic plants. In this study, a series of tools were developed to
enable strong or weak induction of RNA silencing and to suppress RNA
silencing in the absence of stable transgenes. Transient delivery of a
gene directing production of a double-stranded green fluorescent protein (GFP) transcript rapidly induced RNA silencing of a codelivered GFP reporter gene, effectively preventing accumulation of GFP protein
and mRNA. RNA silencing triggered by the strong dsGFP inducer was
partially inhibited by the tobacco etch virus silencing suppressor,
P1/HC-Pro. In the absence of the strong double-stranded GFP inducer,
the functional GFP gene served as a weak RNA silencing inducer in the
transient assay, severely limiting accumulation of the GFP mRNA over
time. The weak silencing induced by the GFP gene was suppressed by
P1/HC-Pro. These results indicate RNA silencing can be triggered by a
variety of inducers and analyzed entirely using transient gene delivery
systems. They also indicate that RNA silencing may be a significant
limitation to expression of genes in the
Agrobacterium-mediated transient assay but that this limitation can be overcome by using RNA silencing suppressors.
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INTRODUCTION |
RNA silencing in plants (also known
as post-transcriptional gene silencing) is the remarkable process,
whereby foreign RNA molecules are recognized and degraded in a
sequence-specific manner (Meins, 2000 ; Sijen and Kooter, 2000). The
foreign RNAs can derive from a highly expressed or aberrant transgene
or from an infectious virus. In fact, RNA silencing is an adaptive
defense response that can limit virus infection and the severity of
symptoms (Marathe et al., 2000). RNA silencing in plants is closely
related to the process of RNA interference in animals, which has been
studied most intensively in Caenorhabditis elegans and
Drosophila (Hunter, 2000). In many organisms, RNA silencing
has proven to be a highly effective tool for producing epigenetic
knockout phenotypes in whole organisms (Baulcombe, 1999; Bosher and
Labouesse, 2000).
Through genetic and biochemical analyses in a variety of systems, the
molecular basis for RNA silencing is partially understood (Bass, 2000;
Carrington, 2000). A key early step in RNA silencing is formation of
double-stranded (ds) RNA. In the case of most plant viruses, dsRNA is
formed during the intermediate steps of genome replication, and this
may explain why viruses are often potent inducers of RNA silencing
(Baulcombe, 1999). RNA silencing triggered by transgenes, but not some
viruses, requires an RNA-dependent RNA polymerase (RdRp)-like protein
that is hypothesized to catalyze synthesis of RNA complementary to the
target species (Dalmay et al., 2000; Mourrain et al., 2000).
Double-stranded RNA is then recognized by a dsRNA-specific nuclease and
cleaved to produce small (21-23 nucleotides) RNA species (Hamilton and
Baulcombe, 1999; Hammond et al., 2000; Zamore et al., 2000). The small
RNAs are proposed to associate with one or more nuclease-like proteins and serve as guides for sequence-specific cleavage of silencing target
RNAs (Bass, 2000). This explains how a given inducer molecule can
trigger RNA degradation directed against itself and against any RNA
with high levels of sequence identity.
The differential requirements for RNA silencing triggered by transgenes
and by RNA viruses in plants, and the effects of various virus-encoded
silencing suppressors support a model in which there are two induction
pathways leading to RNA silencing in plants (Carrington, 2000; Dalmay
et al., 2000; Voinnet et al., 2000). Silencing triggered by a transgene
mRNA, or an RNA with limited amounts of ds secondary structure, depend
on the "weak" inducer pathway that involves the RdRp. It is
interesting that this pathway also leads to systemic RNA silencing in
which tissues distal to the initial sites of silencing induction also
acquire the silenced state (Voinnet et al., 2000). Systemic silencing
involves a graft-transmissible signal that moves through the phloem
(Fagard and Vaucheret, 2000). Silencing triggered by some replicating
RNA viruses, and possibly by inducers with very long segments of dsRNA,
may occur through a "strong" inducer pathway in which the
requirement for the RdRp is bypassed. The strong inducers may be
recognized directly by the dsRNase required for synthesis of the small
RNAs (Zamore et al., 2000).
The Agrobacterium tumefaciens-mediated transient expression
system is a versatile tool to rapidly introduce genes into plant tissue. This system enables gene expression within a short period of
time and without the requirement for regenerating transgenic plants. A
useful feature of this system is the ability to introduce multiple
genes simultaneously into a patch of leaf tissue. This system will
likely increase in utility, particularly for high-throughput functional
genomic and proteomic analyses. The Agrobacterium-mediated expression system has also been used effectively as a means to deliver
RNA silencing inducers and suppressors into transgenic plants that
express a silencing reporter gene (for example, Brigneti et al., 1998;
Voinnet et al., 1998, 2000; Llave et al., 2000).
In this study, we developed tools and procedures to enable analysis of
RNA silencing using the Agrobacterium-mediated transient expression system in the absence of a stable transgene reporter. The
response of a reporter gene in the presence of weak and strong RNA
silencing inducers was analyzed as was the effect of co-introduction of
a virus-encoded silencing suppressor. The results indicate that highly
effective RNA silencing can be triggered rapidly with strong inducers.
The results also indicate that RNA silencing may be an inevitable
consequence of Agrobacterium-mediated transient delivery of
functional genes under the control of a strong promoter but that this
can be countered through use of silencing suppressors.
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RESULTS |
Transient Delivery of RNA Silencing Inducers and
Targets
Most studies to analyze RNA silencing in plants have depended on
transgenic plants that express an active or silenced reporter gene. To
enable analysis of RNA silencing that is independent of transgenes, an
Agrobacterium-mediated transient system was devised to
simultaneously introduce both silencing inducer and target RNAs in
Nicotiana benthamiana. Two key constructs were used in most
experiments. A 35S-green fluorescent protein (GFP) gene (referred to as
the GFP construct) encoded the soluble-modified form of green
fluorescent protein. A 35S-GFP/antisense GFP gene contained the
full-length GFP coding sequence, an intron, and a full-length GFP
sequence in the inverted orientation (Fig.
1A). Transcription of this gene and RNA
processing was predicted to yield an intron spliced hairpin RNA that
was referred to as the dsGFP RNA. Constructs directing synthesis of
dsRNAs in transgenic plants were shown to be potent inducers of RNA
silencing (Waterhouse et al., 1998; Chuang and
Meyerowitz, 2000; Schweizer et al., 2000; Smith et al., 2000). An empty
vector construct was also used in all experiments as a negative
control.
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Figure 1.
Agrobacterium-mediated transient
expression in N. benthamiana leaves. A, Constructs used
contained the 35S promoter (arrow) and terminator sequences (black
circle). The GFP construct contained a functional copy of the
soluble-modified GFP coding sequence, whereas the dsGFP
construct contained both sense and antisense smGFP sequences separated
by an intron. B and C, Agrobacterium-infiltrated
non-transgenic (B) and GFP-transgenic (C) leaves were viewed at 6-d
p.i. under long wavelength UV illumination. Spots in half leaves were
infiltrated with Agrobacterium containing the indicated
constructs.
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Leaves of N. benthamiana plants were infiltrated
with cultures of Agrobacterium containing vector, GFP, or
dsGFP constructs, and GFP fluorescence was monitored using a handheld
long wavelength UV light source. Noninfiltrated zones and zones
infiltrated with cells containing the vector alone appeared red due to
autofluorescence. Tissue infiltrated with bacteria containing the GFP
gene appeared bright green (Fig. 1B). In contrast, tissue infiltrated
with Agrobacterium containing the dsGFP construct appeared
red and was indistinguishable from the vector-only infiltration sites.
Similar results were obtained when Agrobacterium cultures
containing the vector, GFP and dsGFP constructs were injected into
leaves of GFP-expressing transgenic N. benthamiana plants.
In these plants, GFP expressed from the injected construct was detected
against a background of light green fluorescence from the
transgene-expressed protein (Fig. 1C).
RNA Silencing by a Strong Inducer in the Transient
System
A time-course analysis of GFP- and dsGFP-expressing tissue was
done to examine the initiation of RNA silencing in the infiltrated tissues. High Mr and small RNAs were
extracted from Agrobacterium-injected tissue and analyzed by
blot hybridization with a radiolabeled probe specific for the GFP
sequence. The small RNA fraction was prepared to analyze RNA
silencing-associated 21- to 23-nucleotide RNA species. In cells
undergoing RNA silencing, these small RNAs correspond to both sense and
antisense fragments of the silencing target (Hamilton and Baulcombe,
1999). In non-transgenic tissue, the 35S-GFP mRNA was detected at 2-d
postinfiltration (p.i.). After peaking at 3-d p.i., however, the level
of GFP mRNA declined dramatically through 6-d p.i. (Fig.
2A). Relatively little small RNA with
homology to the GFP sequence was detected during the time course. In
contrast, neither a full-length dsGFP transcript nor a unit length GFP
RNA was detected in non-transgenic tissue expressing the dsGFP gene
(Fig. 2A). However, GFP-specific small RNA was detected at 2-d p.i. and
accumulated over the 6-d time course in non-transgenic plants. In the
GFP-expressing transgenic plants, the dsGFP gene also induced formation
of GFP-related small RNAs as well as a moderate decline in the level of
GFP transgene mRNA between 2- and 6-d p.i. (Fig. 2B). Transient
expression of the dsGFP gene, therefore, was sufficient to induce RNA
silencing in the injection zone of both non-transgenic and
GFP-transgenic plants.
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Figure 2.
Analysis of GFP-related RNAs from tissue
infiltrated with Agrobacterium containing the GFP and dsGFP
genes. HMW RNA (5 µg) and small RNA (50 µg) samples were prepared
at various times p.i. and subjected to RNA-blot analysis using a
radiolabeled GFP sequence probe. A, Time course analysis of GFP-related
RNAs in Agrobacterium-infiltrated non-transgenic leaf tissue
expressing GFP or dsGFP genes. B, Limited time-course analysis of
GFP-related RNAs in GFP-transgenic plants that were infiltrated with
Agrobacterium containing empty vector or the dsGFP gene. The
electrophoretic positions of GFP mRNA and oligonucleotide standards (20 and 24 nucleotides) are shown at the left.
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To determine if transient dsGFP expression was sufficient to silence
the Agrobacterium-injected GFP gene, coinfiltration
experiments with both GFP and dsGFP constructs were done. In these and
subsequent experiments, three Agrobacterium cultures were
mixed in equal parts prior to all injections. One culture contained the
GFP reporter gene. Depending on the experiment, the other two cultures
contained empty vector, the dsGFP construct, or another test construct
(see below). In all cases, however, the amount of injected
Agrobacterium containing the GFP reporter was constant,
regardless of whether or not additional cultures containing test
constructs were added to the injection mix. In non-transgenic plants,
infiltration of an Agrobacterium mixture containing the GFP
gene and empty vector resulted in bright green fluorescence within
2 d of p.i. (Fig. 3, A and C). GFP
fluorescence required a Vir+
Agrobacterium strain, as tissue injected with a
Vir strain containing the GFP construct failed
to fluoresce (Fig. 3G). Infiltration of a mixture containing the GFP
gene, dsGFP gene, and empty vector resulted in no GFP fluorescence
(Fig. 3A). The same results were obtained when the mixtures were
injected into GFP-expressing transgenic plants (Fig. 3, D and F). The
suppression of GFP activity in tissue injected with the GFP plus dsGFP
mixture required that the dsGFP construct be in a
Vir+ Agrobacterium strain (Fig. 3H).
Furthermore, the GFP-inhibitory effect of the dsGFP construct was
sequence-specific, as co-injection of Agrobacterium
containing the GFP construct and a dsGUS construct resulted in strong
GFP fluorescence (Fig. 3I).
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Figure 3.
Agrobacterium-mediated transient
expression of combinations of GFP, dsGFP, and P1/HC-Pro constructs.
Non-transgenic (A-C and G-I) or GFP-transgenic
(D-F) N. benthamiana leaves were
infiltrated and analyzed as described in Figure 1. The vir strain of
Agrobacterium lacked DNA transfer properties and was used in
a series of controls (G and H). All infiltrations with a mixture of
three Agrobacterium cultures (A-F) were done using
equivalent amounts of the individual components. In half leaves shown
in A, C, D, and F, two equivalents of the empty vector (V) culture were
used.
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The effect of co-introduction of GFP and dsGFP genes was investigated
by analysis of GFP protein in the infiltrated tissue of transgenic and
non-transgenic plants. As controls, tissues were infiltrated with
Agrobacterium containing empty vector, GFP plus empty
vector, and dsGFP plus empty vector. The GFP protein was detected in
transgenic plants but not non-transgenic plants injected with
Agrobacterium containing empty vector (Fig.
4, A and B, lanes 1-3). In
non-transgenic tissue injected with the GFP gene plus empty vector, GFP
protein accumulated to increasing levels over the 6-d time course (Fig.
4A, lanes 4-6), whereas in transgenic tissue GFP accumulated to levels
higher than the endogenous (transgene-encoded) levels (Fig. 4B, compare
lanes 4-6 with 1-3). However, in non-transgenic tissue infiltrated
with the Agrobacterium mixture containing GFP and dsGFP
genes, no GFP protein was detected at any time point (Fig. 4A, lanes
10-12). These data indicate that the dsGFP construct was inhibitory to accumulation of protein encoded by the injected GFP gene. Similarly, the levels of endogenous GFP in the transgenic plants decreased 5-fold,
relative to tissue expressing the empty vector, over the time-course in
tissue infiltrated with the Agrobacterium mixtures containing the dsGFP gene alone or the dsGFP plus GFP genes (Fig. 4B,
lanes 7-12).
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Figure 4.
Immunoblot analysis of GFP and HC-Pro
in Agrobacterium-infiltrated tissue. Time course analysis of
GFP and HC-Pro protein in non-transgenic (A) or GFP transgenic (B)
N. benthamiana plants infiltrated with
Agrobacterium containing empty vector (lanes 1-3) or
combinations of Agrobacterium containing empty vector (V),
GFP, dsGFP, or P1/HC-Pro constructs (lanes 4-15). Normalized extracts
(20 µg) were prepared at 2-, 4-, and 6-d p.i. and subjected to
immunoblot analysis with anti-GFP or anti-HC-Pro sera.
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Co-introduction of GFP and dsGFP genes was further investigated by
analysis of GFP mRNA and small RNAs from the infiltrated tissues of
non-transgenic plants. As in the previous experiment (Fig. 2A),
infiltrated tissue expressing the GFP gene contained the GFP mRNA,
which declined significantly between the 4- and 6-d-p.i. time points
(Fig. 5, lanes 2-4). This decrease in
GFP mRNA steady-state level over time contrasted with the increasing accumulation of GFP protein (Fig. 4A, lanes 4-6). The high
steady-state level of protein likely resulted from the high stability
of GFP. Little or no GFP-related small RNA was detected using these
experimental conditions, even at 6-d p.i. (Fig. 5, lanes 2-4).
However, these small RNAs were detected using higher specific activity
probes and increasing exposure times (data not shown). No GFP mRNA was detected after co-introduction of the GFP and dsGFP genes, whereas small RNA accumulated to increasing levels throughout the time course
(Fig. 5, lanes 8-10). The cumulative data from in situ visualization
of fluorescence, and from analysis of GFP protein, GFP mRNA and GFP
small RNA indicate that the dsGFP construct induced silencing rapidly
and efficiently in the transient system, regardless of whether or not a
homologous nuclear transgene was present.
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Figure 5.
RNA-blot analysis of GFP-specific RNAs in
Agrobacterium-infiltrated non-transgenic N. benthamiana tissue. HMW RNA (5 µg) and small RNA (50 µg)
samples were prepared at various times p.i. and subjected to RNA-blot
analysis using a radiolabeled GFP sequence probe. Samples were
extracted from tissue that was infiltrated with
Agrobacterium containing empty vector (V, lane 1) or
combinations of Agrobacterium containing empty vector (v),
GFP, dsGFP, or P1/HC-Pro constructs (lanes 2-13). The electrophoretic
positions of oligonucleotide standards (20 and 24 nucleotides) are
shown at the left.
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Suppression of RNA Silencing by Tobacco Etch Virus (TEV) P1/HC-Pro
in the Transient System
The TEV-encoded RNA silencing suppressor, P1/HC-Pro (Anandalakshmi
et al., 1998; Brigneti et al., 1998; Kasschau and Carrington, 1998),
was introduced into the GFP-based transient silencing system to address
two issues. First, the ability of P1/HC-Pro to suppress RNA silencing
from the "strong" inducer derived from the dsGFP gene was tested.
In previous studies, P1/HC-Pro was shown to reverse RNA silencing
triggered by a "weak" transgene inducer in transgenic plants (Llave
et al., 2000). Second, the ability of P1/HC-Pro to inhibit
decline of the GFP mRNA in tissues expressing the functional GFP gene
was tested. If the decline was due to slow or weak induction of RNA
silencing, then P1/HC-Pro was predicted to inhibit the decline.
P1/HC-Pro is actually a polyprotein that undergoes autoproteolytic processing catalyzed by proteinase domains within the P1 and HC-Pro proteins (Carrington et al., 1990).
In contrast to the lack of GFP fluorescence in tissues injected with
mixtures of Agrobacterium containing GFP plus dsGFP genes, tissues infiltrated with the triple mixture containing GFP, dsGFP, and
P1/HC-Pro genes exhibited bright green fluorescence, regardless of
whether the plants were non-transgenic or GFP-transgenic (Fig. 3, B, C,
E, and F). In non-transgenic plants, the appearance of green
fluorescence in leaves injected with the triple mixture corresponded with accumulation of GFP protein in time-course
experiments (Fig. 4A, lanes 13-15). HC-Pro was also detected in the
immunoblot assay at 4- and 6-d p.i., although accumulation of HC-Pro
was delayed relative to accumulation of GFP (Fig. 4A, lanes 13-15). In
transgenic plants, the level of GFP protein that accumulated in tissues
receiving the triple mixture was enhanced relative to tissues injected
with the GFP plus dsGFP mixture (Fig. 4B, lanes 10-15). The
enhancement (11.3-fold) was particularly evident at 6-d p.i. (Fig. 4B,
compare lanes 12 and 15). In addition, the presence of P1/HC-Pro in
non-transgenic tissues injected with the triple mixture resulted in
accumulation of GFP mRNA (Fig. 5, lanes 11-13). However, as seen in
tissues expressing GFP alone (Fig. 5, lanes 2-4), the GFP mRNA
declined between 4- and 6-d p.i. Furthermore, the presence of P1/HC-Pro
did not prevent accumulation of silencing-specific small RNAs (Fig. 5,
lanes 11-13). At the 6-d p.i. time-point, in six independent
experiments, the level of accumulation of GFP-related small RNAs in
tissue injected with the triple mixture was equal to or greater than
that detected in tissue expressing GFP plus dsGFP alone. These data
suggest that P1/HC-Pro partially suppresses RNA silencing initiated by the strong inducer in the transient GFP expression system, although suppression likely occurs only at the early time points examined.
In addition to examination of the effect of P1/HC-Pro on dsGFP-induced
RNA silencing, the effect of P1/HC-Pro on expression and accumulation
of the GFP mRNA in the absence of dsGFP was tested. As in previous
experiments (Figs. 2A and 5), tissue injected with Agrobacterium containing the GFP gene accumulated GFP mRNA
to relatively high levels within 2-d p.i., but GFP mRNA levels declined at later time points (Fig. 6, lanes
1-3). In contrast, tissue injected with an Agrobacterium
mixture containing GFP and P1/HC-Pro genes accumulated GFP mRNA to
relatively high levels that did not decrease between 2- and 6-d p.i.
(Fig. 6, lanes 10-12). These data indicate that the slow decline in
GFP mRNA after Agrobacterium-mediated introduction of the
GFP gene into leaf tissue is likely due to RNA silencing and that this
is efficiently suppressed by P1/HC-Pro. This differs from the effect of
P1/HC-Pro on dsGFP-mediated silencing of the GFP mRNA where the
suppressor promotes accumulation of the GFP mRNA early (2-d p.i.) but
not late (6-d p.i.) in the time course (Fig. 6, lanes 7-9).
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Figure 6.
RNA-blot analysis of GFP-specific RNAs in
Agrobacterium-infiltrated non-transgenic N. benthamiana tissue. HMW RNA samples (5 µg) were prepared at
various times p.i. and subjected to RNA-blot analysis using a
radiolabeled GFP sequence probe. Samples were extracted from tissue
that was infiltrated with combinations of Agrobacterium
containing empty vector (V), GFP, dsGFP, or P1/HC-Pro constructs. The
blot was stripped and reprobed using radiolabeled DNA corresponding to
ribosomal RNA.
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DISCUSSION |
RNA Silencing in the Transient Assay
The Agrobacterium-mediated transient expression system
was used to deliver RNA silencing inducer, reporter, and suppressor constructs to intact tissues of N. benthamiana. This system
enabled analysis of RNA silencing of a GFP construct based entirely on genes delivered in the transient assay. RNA silencing triggered by a
strong inducer derived from the dsGFP construct occurred rapidly,
regardless of whether or not the plant contained a GFP transgene. A key
feature of this system is the ability to simultaneously introduce
additional genes along with silencing reporter genes. For
example, the effects of silencing suppressors can be tested by
adding Agrobacterium cultures containing test
constructs to the injection mix. The codelivery of multiple constructs
is enabled by the extremely high efficiency of
Agrobacterium-mediated gene transfer in N. benthamiana leaves. Microscopic examination of tissue injected
with Agrobacterium containing the GFP construct suggests
that virtually all cells express the gene (unpublished observations).
The finding that transient delivery of dsGFP triggered RNA silencing
efficiently is fully consistent with several other studies using
transgenic plants (Waterhouse et al., 1998; Chuang and Meyerowitz, 2000; Smith et al., 2000). The basis for this strong inducer activity relates to the probable role of dsRNA as the substrate for a nuclease that catalyzes cleavage to 21 to 23 nucleotide RNAs (Zamore et al.,
2000). The small RNAs are proposed to guide a nucleolytic ribonucleprotein complex to target RNAs. Thus, increasing amounts of
dsRNA would lead to increasing amounts of small RNAs, which would lead
to increasing amounts of a component of the sequence-specific nuclease.
In clear support of this model, small RNAs were produced in relatively
high quantities after introduction of the dsGFP construct. This was in
stark contrast to the relatively low levels of small RNA in tissues
expressing the functional GFP gene, at least during the time course examined.
Despite the relatively low levels of small RNA in the functional
GFP-expressing tissue, RNA silencing was eventually detected in the
absence of the dsGFP inducer. Similarly, Voinnet et al. (2000) found
that infiltration of a GFP-expressing construct in GFP transgenic
plants resulted intitally in strong fluorecence at the site of
infiltration, followed by systemic silencing of the GFP transgene and
small RNA accumulation. The results of experiments using P1/HC-Pro
support the hypothesis that the decline in GFP steady-state level was
due to RNA silencing. Co-introduction of GFP and P1/HC-Pro constructs
resulted in maintenance of relatively high steady-state levels of GFP
mRNA. As P1/HC-Pro has little or no effect on transcription (Kasschau
and Carrington, 2001), maintenance of high GFP mRNA levels by P1/HC-Pro
likely resulted from RNA silencing suppression.
These studies underscore the idea that there are two types of RNA
silencing inducers (Dalmay et al., 2000; Voinnet et al., 2000). Strong
inducers are those that contain extensive amounts of dsRNA, either
because a gene directs synthesis of a transcript that adopts
considerable double stranded structure or because a replicating virus
produces dsRNA during the course of genome replication. Weak inducers
are those that contain relatively little double stranded structure but
that are eventually recognized by the silencing apparatus and targeted.
An important step in targeting a weak inducer may be recognition by the
cellular RdRp, which is proposed to catalyze synthesis of complementary
RNA and which would lead to accumulation of dsRNA intermediates (Dalmay
et al., 2000; Mourrain et al., 2000). How a weak inducer is initially recognized remains to be determined.
The effects of TEV P1/HC-Pro on RNA silencing induced by a
 -glucuronidase (GUS) transgene was analyzed previously (Kasschau and
Carrington, 1998; Llave et al., 2000). The GUS transgene in those
studies likely resulted in formation of a weak inducer RNA in
transgenic plants. Co-expression of P1/HC-Pro effectively suppressed both RNA silencing and formation of small RNAs (Kasschau and
Carrington, 1998; Llave et al., 2000). In the dsGFP-induced system
described here, P1/HC-Pro transiently suppressed RNA silencing induced
by the dsGFP construct. However, RNA silencing triggered by the dsGFP construct in the presence of P1/HC-Pro eventually occurred in the 6-d
time course experiments, resulting in declining GFP mRNA levels and
accumulation of small RNAs. It is proposed that in the presence of low
levels of dsRNA inducer, P1/HC-Pro effectively suppresses RNA
silencing. However, as dsRNA inducer accumulates, the suppressing
activity of P1/HC-Pro is overcome, and RNA silencing occurs. These data
suggest that P1/HC-Pro inhibits a dsRNA-dependent step in the RNA
silencing pathway.
Applications
There are three types of applications that arise from this
work. First, the transient RNA silencing assay using various types of
inducers and GFP as a reporter provides a rapid method to screen candidate genes, or random genes from a library, for effects of RNA
silencing. Screens could be designed for positive or enhancing effects
in the case of genes encoding RNA silencing activators or effectors.
Alternatively, screens can be done for silencing suppressors that have
a negative effect. Such a strategy for identification of positive and
negative factors involved in RNA silencing will complement mutant screens.
Second, the transient delivery of dsRNA constructs provides a rapid
method to potentially silence any gene in the Agrobacterium infiltration zone. Of course, the use of dsRNA-mediated transient silencing depends on the availability of an assay to monitor effects, and the range of processes that might be investigated using this approach in leaf tissue is limited. The transient RNA silencing system
is further limited by potential residual effects of gene products that
accumulate prior to induction of silencing. This point is illustrated
by examination of the effects of dsGFP on endogenous GFP protein and
mRNA levels in GFP-transgenic tissue (Figs. 2B and 4B). Although the
dsGFP inducer triggered RNA silencing, residual GFP protein and GFP
mRNA were still detected at 6-d p.i. In addition, the applicability of
the transient system is limited to those species that are amenable to
delivery and expression of T-DNA constucts by
Agrobacterium.
Third, the effect of P1/HC-Pro on RNA silencing triggered by functional
(weak silencing inducer) genes has broad use. The use of the
Agrobacterium delivery system to introduce foreign genes
into leaf tissue continues to grow. Further, we see tremendous potential for this system in functional genomics and proteomics programs, in which expression of wild-type or tagged proteins is
followed by analysis of effects on global gene expression, metabolic
pathways, or protein complex formation. Under the control of the 35S
promoter, it is clear that the GFP gene is subject to RNA silencing
after an initial burst of gene expression. It is reasonable to expect
that many genes, expressed in a similar manner, will follow the same
pattern. Co-introduction of P1/HC-Pro with the GFP gene suppressed the
RNA silencing response. It follows, therefore, that P1/HC-Pro will
suppress RNA silencing triggered by other constructs and result in
maintenance of high expression levels for extended periods.
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MATERIALS AND METHODS |
Plasmid Construction
The base vector for all constructs, pRTL2 (Restrepo et al.,
1990), contained an enhanced 35S promoter from cauliflower mosaic virus, the TEV 5'-non-translated sequence, and the 35S terminator.
The GFP construct (pRTL2-smGFP) contained the coding region of
the soluble-modified green fluorescent protein from Aequorea victoria (nucleotides 21-737) (Davis and Vierstra, 1998). An
additional codon (GCA) was inserted immediately after the start codon
to form a NcoI restriction site at the 5' end of the
open reading frame. The 3' end of the GFP coding sequence contained the
authentic stop codon followed by a KpnI site. The GFP
coding sequence was inserted between the NcoI and
KpnI sites of pRTL2.
The dsGFP construct (pRTL2-dsGFP) contained the entire GFP open reading
frame, including the stop codon, a 120-nucleotide intron from the
RTM1 gene of Arabidopsis Col-0 (Chisholm et al., 2000),
and the entire GFP coding region in the antisense orientation. The
dsGFP construct was made by joining the RTM1 intron to
the 3' end of the GFP coding sequence using PCR. This fragment was cloned into pRTL2-smGFP using KpnI and
XbaI restriction sites.
The dsGUS construct (pRTL2-dsGUS) contained the entire GUS coding
region, followed by the RTM1 intron, and then an
antisense copy of the 3'-proximal 558 nucleotides of the GUS coding
sequence. The intron-antisense GUS fragment was inserted into pRTL2-GUS (Restrepo et al., 1990) between the BglII and
BamHI sites.
Construction of the P1/HC-Pro construct (pRTL2-0027) was described
previously (Carrington et al., 1990). This construct contained the
sequence corresponding to nucleotides 12 to 2,681 of the TEV genome,
which encodes the P1 and HC-Pro proteins and the N-terminal 82 amino
acid residues of the P3 protein.
The expression cassette from each pRTL2-based construct was excised
using PstI and inserted into the plant transformation vector, pSLJ755I5 (Jones et al., 1992). Each of these plasmids was
introduced into Agrobacterium tumefaciens strain GV2260
or the avirulent strain C58C1D by triparental mating.
Plant Material and Agrobacterium Infiltration
Transgenic Nicotiana benthamiana plants
expressing GFP protein were provided by Dr. David C. Baulcombe
(Sainsbury Laboratory) and were described previously (Schaad et al.,
1997; Brigneti et al., 1998). Agrobacterium infiltration
of leaves was done as described (Llave et al., 2000) except that the
cultures were incubated overnight in infiltration medium at room
temperature. Agrobacterium cultures were mixed prior to
infiltration by combining equal volumes of individual cultures. A 3-cc
syringe was used to infiltrate tissue from the underside of leaves.
GFP Imaging
Visual detection of GFP fluorescence was done using a
long-wave UV lamp (Black Ray model B 100 AP). Plants were photographed with a 950 digital camera (Nikon, Tokyo) mounted with both UV and
yellow filters. The images were processed electronically using Adobe Photoshop.
RNA Isolation and Blot Analysis
Total RNA from infiltrated spots was extracted by grinding
leaf tissue in liquid nitrogen and resuspending the frozen powder in
Trizol reagent (10 [v/w]) (Life Technologies/Gibco-BRL, Cleveland). After 5 min at room temperature, chloroform was added (0.2 [v/v]) and
the solution was mixed thoroughly. The RNA was separated from the DNA
and protein by centrifugation at 12,000g for 15 min at 4°C. The RNA phase was removed, and RNA was precipitated by the addition of isopropanol (0.5 [v/v]). The RNA pellet was dissolved in
1 mL of Qiagen buffer QRL1 (Qia RNA/DNA Midi Kit). Nine milliliters of
QRV2 buffer was added to the solution. The RNA was applied to a Qiagen
RNA/DNA column according to the manufacturer's directions. Low
Mr (LMW) RNA was eluted with buffer QRW2,
and high Mr (HMW) RNA was subsequently
eluted with buffer QRU. The RNA was precipitated with ice-cold
isopropanol (1 [v/v]) and recovered by centrifugation at
15,000g for 30 min at 4°C. The RNA pellets were
resuspended in diethyl pyrocarbonate-treated water, and total RNA
concentration was determined using a UV-1601 spectrophotometer
(Shimadzu, Columbia, MD).
The LMW RNA (50 µg) was resolved by electrophoresis in a 15% (w/v)
polyacrylamide-7 M urea gel in TBE buffer (45 mM Tris-borate, pH 8.0, 1 mM EDTA). The HMW RNA
(5 µg) was resolved by electrophoresis in a 1.5% (w/v)
agarose-formaldehyde gel using a buffer consisting of 20 mM
HEPES, pH 7.8, 1 mM EDTA. The RNA in gels was transferred to HyBond-N membrane and subjected to UV crosslinking (1,200 µJ, Stratalinker, Stratagene, La Jolla, CA). The LMW and HMW RNA blots were
prehybridized in solution (50% formamide [v/v], 10× Denhardt's solution, 0.5 mg/mL sheared salmon sperm DNA, 1% [w/v] SDS, 3× SSC,
and 50 mM phosphate buffer) at 35°C and 42°C,
respectively, for at least 3 h. GFP specific radioactive DNA
probes were generated by a random priming technique. Hybridization of
the LMW (35°C) and HMW (42°C) blots was done overnight in a
rotating incubator and was followed by four washes (20 min each) in 2×
SSC buffer and 0.2% (w/v) SDS at 50°C and 65°C, respectively.
Radioactivity on the blots was quantitated using a phosphoimager. Blots
were then exposed to x-ray film.
Immunoblot Analysis
Leaf tissue from infiltration zones was ground in liquid
nitrogen and resuspended (5 [v/w]) in dissociation buffer (40 mM sodium phosphate, pH 7.0, 10 mM EDTA, 0.1%
[v/v] Triton X-100, 0.1% [w/v] N-lauryl sarcosine,
10 mM -mercaptoethanol, 0.5 mM phenylmethylsulfonyl fluoride, 1 µg/mL aprotinin, and 1 µg/mL leupeptin). Total protein concentration was determined by the method of
Bradford using the Protein Assay dye reagent (Bio-Rad Laboratories,
Hercules, CA). Protein samples (20 µg) were subjected to SDS-PAGE and
immunoblot analysis using anti-GFP (Promega, Madison, WI) or
anti-HC-Pro-specific sera. Immunoreactions were detected using an
alkaline phosphataselinked second antibody and a chemiluminescence procedure. Blots were exposed to x-ray film for different periods of
time. Densitometry of bands was done using an Eagle Eye II system (Stratagene).
| |
ACKNOWLEDGMENTS |
We thank Christa Weathers for help in the initial
Agrobacterium infiltration experiments and assistance in
taking photographs of leaf tissue. We also thank Kristin Kasschau and
Cesar Llave for helpful comments and advice during the course of this work.
| |
FOOTNOTES |
Received December 19, 2000; returned for revision February 27, 2001; accepted March 16, 2001.
1
This work was supported by the National
Institutes of Health (grant nos. AI43288 and AI27832) and by the U.S.
Department of Agriculture (grant no. 98-35303-6485).
*
Corresponding author; e-mail carrington{at}wsu.edu; fax
509-335-2482.
| |
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Negative-Strand Tospoviruses and Tenuiviruses Carry a Gene for a Suppressor of Gene Silencing at Analogous Genomic Positions
J. Virol.,
December 20, 2002;
77(2):
1329 - 1336.
[Abstract]
[Full Text]
[PDF]
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F. Qu, T. Ren, and T. J. Morris
The Coat Protein of Turnip Crinkle Virus Suppresses Posttranscriptional Gene Silencing at an Early Initiation Step
J. Virol.,
December 6, 2002;
77(1):
511 - 522.
[Abstract]
[Full Text]
[PDF]
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N. E. Yelina, E. I. Savenkov, A. G. Solovyev, S. Y. Morozov, and J. P. T. Valkonen
Long-Distance Movement, Virulence, and RNA Silencing Suppression Controlled by a Single Protein in Hordei- and Potyviruses: Complementary Functions between Virus Families
J. Virol.,
November 13, 2002;
76(24):
12981 - 12991.
[Abstract]
[Full Text]
[PDF]
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A. C. Mallory, B. J. Reinhart, D. Bartel, V. B. Vance, and L. H. Bowman
From the Cover: A viral suppressor of RNA silencing differentially regulates the accumulation of short interfering RNAs and micro-RNAs in tobacco
PNAS,
November 12, 2002;
99(23):
15228 - 15233.
[Abstract]
[Full Text]
[PDF]
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A. I. Prokhnevsky, V. V. Peremyslov, A. J. Napuli, and V. V. Dolja
Interaction between Long-Distance Transport Factor and Hsp70-Related Movement Protein of Beet Yellows Virus
J. Virol.,
October 2, 2002;
76(21):
11003 - 11011.
[Abstract]
[Full Text]
[PDF]
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C. Llave, K. D. Kasschau, M. A. Rector, and J. C. Carrington
Endogenous and Silencing-Associated Small RNAs in Plants
PLANT CELL,
July 1, 2002;
14(7):
1605 - 1619.
[Abstract]
[Full Text]
[PDF]
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S. Pfeffer, P. Dunoyer, F. Heim, K. E. Richards, G. Jonard, and V. Ziegler-Graff
P0 of Beet Western Yellows Virus Is a Suppressor of Posttranscriptional Gene Silencing
J. Virol.,
June 5, 2002;
76(13):
6815 - 6824.
[Abstract]
[Full Text]
[PDF]
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TOP
ABSTRACT
INTRODUCTION