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Journal of Virology, November 1999, p. 9080-9088, Vol. 73, No. 11
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Identification and Characterization of the
Functional Elements within the Tobacco Etch Virus 5' Leader Required
for Cap-Independent Translation
Mario
Niepel and
Daniel R.
Gallie*
Department of Biochemistry, University of
California, Riverside, California 92521-0129
Received 12 May 1999/Accepted 20 July 1999
 |
ABSTRACT |
Translation in plants is highly cap dependent, and the only plant
mRNAs known to naturally lack a cap structure (m7GpppN) are
viral in origin. The genomic RNA of tobacco etch virus (TEV), a
potyvirus that belongs to the picornavirus superfamily, is a
polyadenylated mRNA that is naturally uncapped and yet is a highly
competitive mRNA during translation. The 143-nucleotide 5' leader
is responsible for conferring cap-independent translation even on
reporter mRNAs. We have carried out a deletion analysis of the TEV
5' leader to identify the elements responsible for its regulatory
function and have identified two centrally located cap-independent
regulatory elements (CIREs) that promote cap-independent translation.
The introduction of a stable stem-loop structure upstream of each
element demonstrated that CIRE-1 is less 5' end dependent in function
than CIRE-2. In a dicistronic mRNA, the presence of the TEV 5'
leader sequence in the intercistronic region increased expression of
the second cistron, suggesting that the viral sequence can function in
a 5'-distal position. Interestingly, the introduction of a stable
stem-loop upstream of the TEV leader sequence or upstream of either
CIRE in dicistronic constructs markedly increased their regulatory
function. These data suggest that the TEV 5' leader contains two
elements that together promote internal initiation but that the
function of one element, in particular, is facilitated by proximity to
the 5' end.
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INTRODUCTION |
Virtually all eukaryotic cellular
mRNAs contain a 5' cap structure [m7G(5')ppp(5')N]
that is required for maintaining mRNA integrity and promoting
efficient translation. In an early step during translation initiation,
the cap is bound by the eukaryotic initiation factor 4F (eIF4F), which
is composed of eIF4E, the cap-binding subunit, and eIF4G, a
considerably larger subunit. eIF4G serves as a multiadapter protein
that, in addition to eIF4E, binds eIF4A, eIF3, the poly(A)-binding protein, and RNA (9, 15, 22, 23, 34, 38). The binding of a
40S ribosomal subunit to an mRNA is mediated by eIF3. As a result,
the binding of eIF4E to the cap structure and the interaction between
eIF4E, eIF4G, and eIF3 direct the binding of 40S subunits preferentially to the 5' ends of capped mRNAs.
The only known mRNAs that naturally lack a cap are viral in origin.
The picornaviral superfamily includes viruses that infect animals,
e.g., poliovirus and encephalomyocarditis virus, and those that use
plants as their host, e.g., tobacco etch virus (TEV). Regardless of the
difference in host species, the genomic architectures of these
viruses are highly similar. In each case, the single-stranded,
positive-sense RNA genome functions as a monocistronic mRNA for a
single polyprotein which, once produced, is processed by virus-encoded
proteases into capsid and noncapsid proteins that are required to carry
out the viral life cycle. Moreover, the viral RNA, which is
polyadenylated but lacks a 5' cap structure, contains a virus protein
genome (VPg) linked to the 5' terminus (5). However, the VPg
is removed prior to recruitment of the viral RNA into polysomes, at
least for poliovirus (13, 25, 26, 33). Consequently, it is
the 5' leader sequences of these viral mRNAs that confer on them
the ability to be translated in a cap-independent manner (3, 11,
17, 30). For poliovirus and encephalomyocarditis virus, the 5'
leader varies in length from 650 to 1,300 nucleotides (nt), is highly
structured, and contains multiple AUGs upstream of the initiation codon
of the polyprotein-coding region (reviewed in reference
27). A region within these leaders serves as an
internal ribosome entry site (IRES) that allows 40S ribosomal subunits
to bind at or upstream of the true initiation codon (reviewed in
reference 6). 40S subunit binding to the IRES can be
mediated by a proteolytic fragment of eIF4G that contains the
RNA-binding and eIF3 interaction domains (31, 32).
Consequently, the 5' leaders of picornaviral mRNAs promote
cap-independent translation by recruiting 40S subunits via an internal
initiation mechanism.
In plants, it follows that those viral mRNAs that naturally lack a
5' cap structure must be translated through a cap-independent mechanism. The 5' leaders of several plant viral mRNAs, including members of the tobamoviral, potyviral, comoviral, and luteoviral families, are responsible for conferring cap-independent
translation (3, 11, 16, 37, 39). However, whether the
translation of any plant viral mRNA occurs through internal
initiation has been controversial (2, 39). A 351-nt region
upstream of an AUG distal to the first initiation codon within the
cowpea mosaic virus middle component RNA was reported to allow internal
initiation at the distal AUG (39), although this has been
disputed (2). Because both of these studies used animal
cells or lysate for their analyses, neither could conclude whether
internal initiation occurs in plants. The 5' leader of turnip mosaic
potyvirus RNA or the sequence upstream of the 3'-proximal coat protein
subgenomic mRNA of a crucifer-infecting tobamovirus was
reported to allow internal initiation (1, 16); however, the
use of capped mRNAs in plant cells in the former example or
uncapped mRNAs in in vitro translation lysates failed to
demonstrate internal initiation of uncapped mRNAs in vivo.
Previous studies have demonstrated that the TEV 5' leader mediates
cap-independent translation (3) and is functionally analogous to a cap in that it interacts with the poly(A) tail to
promote efficient translation (11) similar to that observed between a cap and a poly(A) tail (10). Precisely how the TEV 5' leader substitutes for the cap to confer cap-independent translation has not been investigated. In this study, we have identified the elements within the TEV 5' leader that are required to direct cap-independent translation. Two distinct cap-independent regulatory elements (CIREs) are present within the central region of the 143-base
leader. The 5'-proximal element (CIRE-1) is more 5' end independent
than is the 5'-distal element (CIRE-2), and their combinatorial effects
are approximately multiplicative, suggesting that the two elements are
not functionally redundant in promoting cap-independent translation.
Moreover, the TEV leader sequence or each CIRE promoted the translation
of a second cistron when the viral leader sequence was present in the
intercistronic region of a dicistronic mRNA. These observations
suggest that specific CIREs are present within the TEV 5' leader and
that these CIREs function optimally in a 5'-proximal position but can
also promote translation when positioned internally within a
dicistronic mRNA.
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MATERIALS AND METHODS |
Plasmid and mRNA constructs.
The full-length TEV 5'
leader and subsequences were synthesized by PCR, and each DNA fragment
was flanked by a HindIII and SalI restriction
site. Each PCR product was introduced into the HindIII
and SalI restriction sites upstream of the luciferase (luc) gene in the pT7-luc-A50
construct, a construct that has been described previously
(10) to result in either
TEV1-143-luc-A50 (i.e., the
full-length TEV leader upstream of the luc coding region) or
the following TEV 5' leader deletion constructs:
TEV1-118-luc-A50, TEV1-65-luc-A50,
TEV28-143-luc-A50,
TEV28-118-luc-A50, TEV28-65-luc-A50,
TEV66-143-luc-A50, and
TEV66-118-luc-A50.
Control leader constructs were designed to contain one or two copies
(both in a forward orientation) of a 60% AT-rich, 72-nt sequence
(AATATCTTATTG CCGGGAAAAGTGTACGTATCACCGTTTGTGTGAACAACGAACTGAA CTGGCAGACTATAA)
introduced into the HindIII and SalI
sites of pT7-luc-A50, resulting in
Con72-luc-A50 or
Con144-luc-A50 mRNAs. The free
energy (
G) calculated by the fold algorithm for these mRNA
leaders is 
11.5 kcal/mol, which is approximately equal to the free
energy of the 5' leader of the
TEV1-143-luc-A50 mRNA construct
(G = 10.7 kcal/mol) (41). A third
control mRNA, Con17-luc-A50, was
constructed with the 17-nt 5' leader sequence GCCTAAGCTTGTCGACC,
representing a free energy of 0.9 kcal/mol.
The above control 72-nt sequence was used to replace the 5'-terminal 65 nt of the TEV 5' leader to result in
Con
72-TEV
66-143-
luc-A
50 mRNA or was used to replace the 3'-terminal 78 nt of the TEV 5'
leader to result in
TEV
1-65-Con
72-
luc-A
50 mRNA.
Introduction of a stable secondary structure was carried out by
inserting a palindromic sequence
(AAGCTTGGGCCCAGATCTACGCGTACGTACGCGTAGATCTGGGCCCAAGCTT)
into
the
HindIII site 4 nt downstream of the T7
promoter transcriptional
start site, producing a stem-loop (SL)
composed of a 24-bp stem
close to the 5' terminus of the TEV-leader
mRNA constructs
SL-TEV
1-143-
luc-A
50,
SL-TEV
1-65-
luc-A
50,
SL-TEV
66-143-
luc-A
50, and
SL-TEV
66-118-
luc-A
50 and the
control mRNA constructs
SL-Con
7-
luc-A
50,
SL-Con
62-
luc-A
50,
and
SL-Con
134-
luc-A
50. The calculated
free energy of this SL structure
is
42.9 kcal/mol.
Dicistronic constructs were generated by inserting the
uidA
gene (composed of the coding region for
-glucuronidase [GUS]
and 73 nt of sequence 3' to the
uidA termination codon)
upstream
of the TEV-
luc and control-
luc
constructs, resulting in the following
mRNA constructs:
GUS-TEV
1-143-
luc-A
50,
GUS-SL-TEV
1-143-
luc-A
50,
GUS-TEV
1-65-
luc-A
50,
GUS-SL-TEV
1-65-
luc-A
50,
GUS-TEV
66-143-
luc-A
50,
GUS-SL-TEV
66-143-
luc-A
50,
GUS-Con
17-
luc-A
50,
GUS-SL-Con
7-
luc-A
50,
GUS-Con
72-
luc-A
50,
GUS-SL-Con
62-
luc-A
50,
GUS-Con
144-
luc-A
50, and
GUS-SL-Con
134-
luc-A
50.
In vitro transcription.
RNAs were synthesized with template
plasmids linearized immediately downstream of the poly(A)50
sequence by NdeI to produce polyadenylated mRNAs or
template plasmids linearized upstream of the poly(A)50
sequence by BamHI to produce poly(A)
mRNAs. Uncapped mRNAs were synthesized in vitro as described previously (40) with 10 µg of template DNA in a solution
consisting of 40 mM Tris-HCl (pH 7.9), 6 mM MgCl2, 2 mM
spermidine, 100 µg of bovine serum albumin/ml, 500 µM (each) ATP,
CTP, UTP, and GTP, 10 mM dithiothreitol, 0.5 U of RNase inhibitor
RNasin (Promega), and 0.5 U of T7 RNA polymerase (New England Biolabs)
per ml. Capped RNAs were synthesized with 8 µg of template in the
same reaction mixture as that described above except that GTP was used
at 160 µM and 1 mM m7GpppG was included in the reaction
mixture. Under these conditions more than 95% of the mRNA is capped.
mRNA delivery to plant protoplasts.
Protoplasts were
isolated from a carrot (RCWC) cell suspension (used previously in the
analysis of the translational regulatory function of the TEV 5' leader
as well as for other viral translation studies [11,
12]) by digestion with 0.25% CELF cellulase, 1% cytolase,
0.05% pectolyase Y23, 0.5% bovine serum albumin, and 7 mM
-mercaptoethanol in protoplast isolation buffer (12 mM sodium
acetate [pH 5.8], 50 mM CaCl2, 0.25 M mannitol) for 90 to
120 min. Protoplasts were washed with protoplast isolation buffer
followed by electroporation buffer (10 mM HEPES [pH 7.2], 130 mM KCl,
10 mM NaCl, 4 mM CaCl2, 0.2 M mannitol) and resuspended in
electroporation buffer to approximately 106 cells/ml. Equal
amounts of mRNAs (approximately 2.5 µg) were added to 400 µl of
cell suspension immediately before electroporation (250 µF, 300 V,
0.2-mm electrode) with an IBI GeneZapper. The electroporated cells were
incubated in protoplast growth medium (MS salts [pH 5.8] and 30 g of sucrose, 100 mg of myo-inositol, 0.1 mg of
2,4-dichlorophenoxyacetic acid, 1.3 mg of niacin, 0.25 mg of thiamine,
0.25 mg of pyridoxine, and 0.25 mg of calcium pentothenate per liter)
supplemented with 20% cultured medium (protoplast growth medium
conditioned with carrot cells for 3 days) overnight prior to the assay
for reporter gene activity. For each experiment, an mRNA was
delivered to triplicate samples of protoplasts and each sample was
assayed in duplicate. Each experiment was repeated a minimum of three
times. The average value and standard deviation for the constructs of a
typical experiment are reported. For the monocistronic luc
mRNA constructs, capped GUS-A50 mRNA was
codelivered to serve as an internal control. For dicistronic mRNAs,
GUS served as the 5'-proximal cistron. Luciferase in vivo activity
normalized to GUS specific activity is reported.
In vitro translation.
Equal amounts of mRNA were
translated with wheat germ extract as described by the manufacturer
(Promega) except that all amino acids were unlabeled. The reaction
mixtures were incubated for 2 h at 22°C, and aliquots of 3 µl
were assayed. Each mRNA construct was translated in triplicate, and
each in vitro translation was assayed in duplicate for luciferase
activity. The average value and standard deviation for each construct
are reported.
Luciferase and GUS assays.
Carrot protoplast extracts in
luciferase assay buffer (25 mM Tricine [pH 8], 5 mM
MgCl2, 0.1 mM EDTA supplemented with 33.3 mM
dithiothreitol, 270 µM coenzyme A, and 500 µM ATP) were assayed for
luciferase activity following injection of 0.5 mM luciferin with a
Monolight 2010 luminometer (Analytical Luminescence Laboratory).
GUS activity in a 100-µl reaction mixture was assayed as described
previously (
7) with 1 mM
4-methylumbelliferyl-
-
D-glucuronide
as the substrate.
The assay was performed for 30 min at 37°C,
whereupon the reaction
was terminated by addition of 900 µl of
0.2 M NaCO
2. The
amount of the fluorescent product produced in
each assay was measured
in a TKO 100 fluorometer (Hoefer Scientific,
Inc.), with excitation at
365 nm and emission at 455
nm.
| |
RESULTS |
Identification of the CIREs within the TEV 5' leader.
Previous
work demonstrated that the TEV 5' leader enhances the in vivo
translation of reporter mRNAs in a cap-independent manner (3,
11). Enhancement was observed in tobacco (3), a host
for TEV, and carrot (11), which, as a nonhost, permits the
analysis of the translational regulatory function of the TEV 5' leader
independent of any potential host factor influence. To identify the
region within the leader that is responsible for conferring
cap-independent translation, a series of deletions was introduced
throughout the TEV leader sequence and the resulting mutant leaders
were tested for their ability to enhance the translation of luciferase
(luc) mRNA in vivo following mRNA delivery to carrot protoplasts or in vitro by translating each mRNA in wheat germ lysate. The context of the luc initiation codon
(GUCGACCAUGG, where the underlined AUG indicates
the luc start codon) for all constructs used in this study
was identical. The degree of cap-independent translation conferred by
the full-length construct or each truncated TEV leader construct was
measured relative to a control luc mRNA that contained a
5' leader of similar length and degree of secondary structure (as
described in Materials and Methods) but was unrelated in sequence. As
previous work demonstrated that in vivo translation increases
moderately as the length of the 5' leader increases (12), it
was necessary to employ control mRNAs that approximate the
length of the TEV leader in order to establish that the enhancement conferred by the TEV 5' leader was the result of specific regulation associated with this viral leader and not a consequence of its length.
The presence of the TEV 5' leader upstream of the
luc coding
region (i.e., TEV
1-143-
luc-A
50)
resulted in a 189-fold
increase in translation of the uncapped mRNA
relative to the uncapped
control
luc mRNA containing a
5' leader of similar length (i.e.,
Con
144-
luc-A
50) (Fig.
1), demonstrating that the increased
translation
conferred by the TEV leader was not merely a
consequence of its
length. Deletion of the 5'-terminal 27 nt
(i.e., TEV
28-143-
luc-A
50)
or
3'-terminal 25 nt (i.e.,
TEV
1-118-
luc-A
50) had little
effect on the ability of the TEV 5' leader to confer cap-independent
translation (Fig.
1). The TEV leader in which both terminal regions
were deleted (i.e.,
TEV
28-118-
luc-A
50) exhibited only a
small decrease in its regulatory function, suggesting that neither
terminal region was essential for the TEV leader-mediated
cap-independent
translation. However, deletion of the 3'-terminal 78 nt
(i.e.,
TEV
1-65-
luc-A
50) did
result in a reduction in cap-independent
translation, i.e.,
TEV
1-65-
luc-A
50 mRNA was
translated to
an 18-fold-greater degree than the control mRNA,
compared to the
189-fold enhancement associated with the full-length
TEV leader
construct, i.e.,
TEV
1-143-
luc-A
50 (Fig.
1).
Similarly, the
deletion of the 5'-terminal 65 nt (i.e.,
TEV
66-143-
luc-A
50)
resulted in a
reduction in the degree of cap-independent translation
to 19-fold
(relative to the control mRNA). It should be noted
that
although the separation of the 5' and 3' halves of the TEV
5' leader
resulted in a 10-fold reduction in cap-independent translation,
the TEV
1-65 and TEV
66-143 subsequences still
retain
substantial regulatory function (18- and 19-fold increases,
respectively,
in cap-independent translation relative to the control
mRNA) (Fig.
1).
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FIG. 1.
Identification of the two elements required for
cap-independent translation. The full-length TEV 5' leader or various
subsequences were introduced upstream of the luc coding
region in a T7 promoter-based construct that permitted the in vitro
synthesis of mRNA terminating in a poly(A)50 tail. The
region of the TEV 5' leader present in each construct is indicated by a
thick line, and the portion of the TEV leader sequence included in each
construct is indicated as a subscript. The control sequence is
indicated by a thin line, and the length of control sequence (Con)
included in each construct is indicated as a subscript. Expression from
an mRNA following delivery to carrot protoplasts by electroporation
or following translation in wheat germ lysate is shown to the right of
each construct. Each uncapped mRNA construct was delivered to
triplicate samples of protoplasts or translated in triplicate in vitro,
and each sample was assayed in duplicate. The experiment was repeated a
minimum of three times, and the average value and standard deviation
for the constructs of a typical experiment are reported.
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|
One possible explanation for the reduction of cap-independent
translation of the TEV
1-65-
luc-A
50
and TEV
66-143-
luc-A
50 mRNAs
could be the change in position with respect to either the
initiation
codon or the 5' terminus, respectively. To test this
possibility, a
72-nt control sequence (one of two copies present
in the leader of the
Con
144-
luc-A
50 mRNA) was
substituted for
the 3'-terminal 78 nt of the TEV leader sequence,
resulting in
the construct
TEV
1-65-Con
72-
luc-A
50.
Introduction of this
control sequence positioned the
TEV
1-65 subsequence relative
to the
luc
initiation codon with approximately the same spacing
as that in
the TEV
1-143-
luc-A
50 mRNA
construct. The degree
of cap-independent regulatory function from the
TEV
1-65-Con
72-
luc-A
50 mRNA was not significantly different (23-fold enhancement relative
to the control construct,
Con
144-
luc-A
50) (Fig.
1) from
that observed
for the
TEV
1-65-
luc-A
50 mRNA
(18-fold enhancement relative
to the control construct); these data
suggest that the change
in spacing had little effect on the
regulatory function of the
TEV
1-65 subsequence.
Replacing the 5'-terminal 65 nt with
the 72-nt control sequence (i.e.,
Con
72-TEV
66-143-
luc-A
50)
positioned the TEV
66-143 subsequence relative to
the 5'
terminus with approximately the same spacing as that in
the TEV
1-143-
luc-A
50 mRNA
construct. The regulatory function from
Con
72-TEV
66-143-
luc-A
50 did not increase relative to that observed for
TEV
66-143-
luc-A
50 (12-fold versus
19-fold, respectively, relative to the
Con
144-
luc-A
50 control mRNA)
(Fig.
1), suggesting that maintaining the spacing
of the 5' terminus
relative to the TEV
66-143 subsequence
is not required for
the regulatory function of this
subsequence.
The regulatory elements present within the TEV
1-65 and
TEV
66-143 subsequences were further delineated
following
the deletion of the 5'-terminal 27 nt from the
TEV
1-65-
luc-A
50 construct
(resulting in TEV
28-65-
luc-A
50) or
3'-terminal
25 nt from the
TEV
66-143-
luc-A
50 construct
(resulting in
TEV
66-118-
luc-A
50).
Translation from TEV
28-65-
luc-A
50 mRNA was 10-fold higher than that from the control mRNA, and
translation
from
TEV
66-118-
luc-A
50 mRNA was
11-fold higher than that
from the control. Consequently, deletion
of the terminal sequences
reduced cap-independent translation by only a
small extent relative
to that observed from the
TEV
1-65-
luc-A
50 and
TEV
66-143-
luc-A
50 constructs. These
data suggest that a CIRE resides within the
TEV
28-65
subsequence (referred to as CIRE-1) and that a
second element is
present within the TEV
66-118 subsequence
(referred
to as CIRE-2). The multiplicative effect of the individual
contributions of CIRE-1 and CIRE-2 (i.e., 10-fold × 11-fold =
110-fold relative to the control mRNA)
produced a degree of cap-independent
translation that was similar
to the actual degree of translation
conferred when both elements were
present together in the
TEV
28-118-
luc-A
50 construct (123-fold relative to the control mRNA), suggesting
independence of function. The failure of the full-length TEV 5'
leader
or any TEV deletion construct to enhance translation in
vitro (Fig.
1)
suggested that CIRE-1 and CIRE-2 do not function
in vitro. The in vitro
results are in good agreement with previous
observations with the
full-length TEV 5' leader (
11).
CIRE-1 and CIRE-2 promote optimal cap-independent translation
largely through a 5'-end-dependent mechanism.
eIF4F, when
bound to a 5' cap structure, directs 40S subunit binding to the 5' end
of a capped mRNA. The absence of a cap or a reduction in functional
eIF4F reduces 5'-end-dependent binding of 40S subunits and increases
internal binding in Saccharomyces cerevisiae
(35). The presence of secondary structure or RNA-protein complexes positioned close to the 5' cap structure can function as an effective barrier to 5'-end-dependent translation by
blocking 40S subunit binding to the mRNA (19, 20, 24, 28,
29). Secondary structure is less effective in impeding the
translation of uncapped mRNA in yeast because 40S subunit binding
is not directed to the 5' terminus (35, 36). However, in
rabbit reticulocyte lysate, translation of an uncapped mRNA remains
5' end dependent (4), suggesting that a difference between
yeast and mammalian translation may exist.
To examine whether the cap-independent translation conferred by the TEV
5' leader requires an unstructured 5' terminus, a
stable SL structure
(with a calculated free energy of
42.9 kcal/mol)
was introduced 4 nt
downstream of the 5' terminus of the control
and TEV-containing
mRNA constructs used in the previous experiment.
Translation
of uncapped mRNAs with or without the SL structure
was
assayed following their delivery to carrot protoplasts or
in wheat germ
lysate. In the absence of an SL, expression from
the constructs
containing the control sequence as the 5' leader
increased moderately
with the length of the leader in protoplasts
(Fig.
2). Translation of the
SL-Con
7-
luc-A
50 construct (in which
the SL was introduced into the control construct
Con
17-
luc-A
50)
was reduced to just
13% of that observed for
Con
17-
luc-A
50 (Fig.
2). In contrast,
the introduction of the SL 62 nt upstream of
the
luc
cistron, i.e., SL-Con
62-
luc-A
50,
resulted in a level of
translation that was 40% of that for the
corresponding control
mRNA (i.e.,
Con
72-
luc-A
50) in protoplasts (Fig.
2). Introduction
of the SL 134 nt upstream of the
luc
cistron had an even smaller
effect on in vivo expression: translation
from SL-Con
134-
luc-A
50 was 52% that
of Con
144-
luc-A
50. Translation of
the same mRNAs
in vitro yielded a similar trend: the presence of
the SL 7 nt
upstream of the
luc initiation codon reduced
translation to 3%
of the control, whereas translation was 41% of the
corresponding
control when the SL was positioned 134 nt upstream of the
initiation
codon (Fig.
2). One exception to the trend observed in vitro
was
with the SL-Con
62-
luc-A
50
mRNA construct, which was translated
to just 5% of the
corresponding control in vitro but was translated
to 40% of the
control in vivo. These results suggest that the
spacing between the
secondary structure and the initiation codon
determines the extent of
translational repression at the appropriate
start codon of uncapped
mRNAs. Moreover, these data demonstrate
that although the
repressive effect of an SL on the translation
of an uncapped mRNA
can be reduced by increasing the distance
between it and the initiation
codon, a difference in the distance
required is observed for
translation in vivo versus in vitro.
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FIG. 2.
Analysis of the translational efficiency of uncapped
mRNAs with a free or inaccessible 5' terminus. The effect of
increasing the length of the 5' leader on the translational efficiency
of an uncapped mRNA with or without an SL present at the 5'
terminus was examined in carrot protoplasts and in wheat germ lysate.
Control 5' leaders 17, 72, or 144 nt in length were introduced upstream
of the luc coding region, and each mRNA was synthesized
in vitro to terminate in a poly(A)50 tail. The 144-nt
leader contains two copies of the 72-nt sequence present in the 72-nt
leader construct. The length of the control sequence (Con) included in
each construct is indicated as a subscript. The 24-bp SL introduced
into each construct is indicated diagrammatically. Expression from each
mRNA following delivery to carrot protoplasts by electroporation or
following translation in wheat germ lysate is shown to the right of
each construct. Each uncapped mRNA construct was delivered to
triplicate samples of protoplasts or translated in triplicate in vitro,
and each sample was assayed in duplicate. The experiment was repeated a
minimum of three times, and the average value and standard deviation
for the constructs of a typical experiment are reported.
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The same SL was then introduced upstream of the TEV 5' leader in order
to examine whether the cap-independent translation
mediated by this
leader is 5' end dependent or 5' end independent.
Translation of
SL-TEV
1-143-
luc-A
50 in protoplasts
(in which
the SL was introduced into the control construct
TEV
1-143-
luc-A
50)
was reduced to
just 12% of that observed for
TEV
1-143-
luc-A
50 (Fig.
3). As seen above, translation from
SL-Con
134-
luc-A
50 was
52% of that
observed for the Con
144-
luc-A
50
control construct.
Consequently, the repressive effect of the SL when
present upstream
of the TEV 5' leader was disproportionately greater
than what
would have been expected from its position with respect to
the
luc cistron, suggesting that the TEV 5' leader requires
an accessible
5' terminus for optimal regulatory function. However,
even with
the SL positioned upstream of the TEV 5' leader, translation
was
still more than 60-fold greater than that from the
Con
144-
luc-A
50 construct (Fig.
3),
suggesting that the TEV 5' leader retained
substantial function even in
the absence of a free 5' terminus.
View larger version (15K):
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FIG. 3.
Analysis of the 5'-end dependence of the TEV 5' leader
and CIRE-1 and CIRE-2. The 5'-end dependence of the full-length TEV
leader and of each CIRE individually was examined by introducing each
sequence upstream of the luc coding region. Each uncapped
mRNA, with or without an SL present at the 5' terminus, was
synthesized in vitro to terminate in a poly(A)50 tail. The
region of the TEV 5' leader present in each construct is indicated by a
thick line, and the portion of the TEV leader sequence included in each
construct is indicated as a subscript. The 24-bp SL introduced into
each construct is indicated diagrammatically. The control sequence is
indicated by a thin line, and the length of the control sequence (Con)
included in the control construct is indicated as a subscript.
Expression from each mRNA following delivery to carrot protoplasts
by electroporation is shown to the right of each construct.
|
|
To examine the effect of the SL on cap-independent translation
conferred by each of the two CIREs within the TEV 5' leader,
the SL was
introduced upstream of each CIRE individually. Translation
from
SL-TEV
1-65-
luc-A
50 (in which the SL
was introduced
into the construct
TEV
1-65-
luc-A
50, which contains
CIRE-1)
in protoplasts was 52% of that observed for
TEV
1-65-
luc-A
50 (Fig.
3). The
effect of the SL was similar to its effect on the
control leader of
similar length (compare the degree of repression
from
SL-Con
62-
luc-A
50 relative to that
from Con
72-
luc-A
50 [Fig.
2]). In
contrast, the introduction of the SL upstream of CIRE-2,
i.e.,
SL-TEV
66-143-
luc-A
50, had a
disproportionately repressive
effect in that it reduced translation to
22% of that observed
for
TEV
66-143-
luc-A
50 (Fig.
3).
Consequently, the cap-independent
translation conferred by the region
of the TEV 5' leader containing
CIRE-2 is more 5' end dependent than
that conferred by the region
containing CIRE-1. It should be noted that
the effect of the SL
was reproducibly greater for the full-length TEV
5' leader than
it was for either CIRE individually, indicating that the
two elements
exhibit greater 5' end dependence when together than when
separate.
Additionally, it should be noted that the introduction of the
SL upstream of either CIRE failed to abolish entirely the
cap-independent
translation conferred by either element, suggesting
that although
CIRE-2 may be more 5' dependent than CIRE-1, both retain
substantial
regulatory function in the absence of a free 5'
end.
The poly(A) tail promotes cooperativity between CIRE-1 and
CIRE-2.
Previous work demonstrated that the TEV 5' leader
functionally interacts with the poly(A) tail to promote cap-independent translation (11). This interaction is analogous to that
observed between a cap and a poly(A) tail (10), suggesting
that one or more elements within the TEV 5' leader are responsible for
the functional interaction with the poly(A) tail. To examine the
poly(A) tail dependence of each CIRE and the degree of 5'-end
dependence of each CIRE in the absence of a poly(A) tail, those
constructs used in Fig. 3 were introduced as poly(A)
mRNAs into carrot protoplasts and their relative levels of
translation were determined (Fig. 4). The
presence of the SL upstream of the full-length TEV 5' leader construct
(i.e., SL-TEV1-143-luc) reduced translation to
33% of that observed for TEV1-143-luc (Fig.
4). However, as noted above, the introduction of the SL upstream of the
full-length TEV 5' leader had a greater repressive effect when the
mRNA was polyadenylated (i.e.,
SL-TEV1-143-luc translated at 12% of the level
observed for TEV1-143-luc [Fig. 3]),
suggesting that one functional consequence of the interaction between
the TEV 5' leader and the poly(A) tail is to increase the 5'-end
dependence of the full-length TEV 5' leader.
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|
FIG. 4.
The poly(A) tail is required for CIRE-1 and CIRE-2
regulatory function. The regulatory function and 5'-end dependence of
the full-length TEV 5' leader and each CIRE individually were examined
by introducing each sequence upstream of the luc coding
region. Each uncapped mRNA, with or without an SL present at the 5'
terminus, was synthesized in vitro without a poly(A) tail. The region
of the TEV 5' leader present in each construct is indicated by a thick
line, and the portion of the TEV leader sequence included in each
construct is indicated as a subscript. The 24-bp SL introduced into
each construct is indicated diagrammatically. Control sequence is
indicated by a thin line, and the length of the control sequence (Con)
included in the control construct is indicated as a subscript.
Expression from each mRNA following delivery to carrot protoplasts
by electroporation is shown to the right of each construct.
|
|
Each CIRE, when tested individually in poly(A)
mRNAs,
i.e., as either TEV
1-65-
luc (containing CIRE-1)
or TEV
66-143-
luc (containing CIRE-2), retained
the ability to confer cap-independent
translation (Fig.
4),
demonstrating that neither element is wholly
dependent on the poly(A)
tail for its function. As observed for
the full-length TEV 5' leader,
introduction of the SL affected
the function of each CIRE to a lesser
extent in poly(A)
mRNAs (Fig.
4) than in
polyadenylated mRNAs (Fig.
3).
The absence of a poly(A) tail also affected the combinatorial
effect of CIRE-1 and CIRE-2 on cap-independent translation.
When
mRNA lacked a poly(A) tail, translation from
TEV
1-65-
luc (containing CIRE-1)
and TEV
66-143-
luc (containing CIRE-2)
was 3.8- and 3.2-fold, respectively, less than that from
TEV
1-143-
luc (containing both CIRE-1 and
CIRE-2), as calculated from the data
in Fig.
4, but was 14.4- and
8.9-fold, respectively, less than
that from
TEV
1-143-
luc-A
50 when the mRNAs
were polyadenylated
(calculated from the data in Fig.
3). Because
separation of the
CIREs resulted in a greater loss of translational
efficiency when
the mRNA was polyadenylated, these data suggest
that another consequence
of the interaction between the TEV 5' leader
and the poly(A) tail
is to increase the combinatorial effect of CIRE-1
and CIRE-2 on
cap-independent
translation.
The TEV 5' leader sequence can increase translation when positioned
internally in a dicistronic construct.
To examine whether the TEV
5' leader sequence can promote the translation of the second cistron of
a dicistronic mRNA when present in an intercistronic position, a
series of dicistronic constructs in which TEV leader or control
sequences were introduced between the region encoding GUS as the
5'-proximal cistron and the luc coding region as the distal
cistron were made (see Fig. 5 and 6 for construct design). In the first
series of constructs to be examined, the control 5'-leader sequences
used in Fig. 2 were tested as intercistronic sequences. These included
the control sequence of 17 (i.e.,
GUS-Con17-luc-A50), 72 (i.e.,
GUS-Con72-luc-A50), and 144 nt
(i.e., GUS-Con144-luc-A50). An
additional 73 nt from the GUS 3'-untranslated region contributed to the
intercistronic region of each construct. Each construct was introduced
as a capped mRNA into carrot protoplasts, and the degree of
translation from the 5'-distal luc cistron was normalized to
the amount of GUS produced from the 5'-proximal cistron. Levels of
translation from these three control mRNAs in carrot protoplasts
and in wheat germ lysate were not significantly different (Fig.
5), suggesting that the difference in the
length of the intercistronic region in the range represented by these
constructs did not influence initiation at the distal cistron. This is
in contrast to the moderate increase in translation observed when the
length of the 5' leader was increased for a monocistronic mRNA
(Fig. 2).
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|
FIG. 5.
The effect of intercistronic length on the translation
of the 5'-distal cistron in a dicistronic mRNA. Dicistronic
mRNAs with GUS as the 5'-proximal cistron and luc as the
5'-distal cistron were constructed with intercistronic regions
containing control sequence 17, 72, or 144 nt in length. Each capped
mRNA construct was synthesized in vitro to terminate in a
poly(A)50 tail. The 144-nt intercistronic region contains
two copies of the 72-nt sequence present in the 72-nt intercistronic
construct. The length of the control sequence (Con) included in each
construct is indicated as a subscript. The 24-bp SL introduced into
each construct is indicated diagrammatically. Expression from each
mRNA following delivery to carrot protoplasts by electroporation or
following translation in wheat germ lysate is shown to the right of
each construct. Each mRNA construct was delivered to triplicate
samples of protoplasts or translated in triplicate in vitro, and each
sample was assayed in duplicate. The experiment was repeated a minimum
of three times. The average value and standard deviation for the
constructs of a typical experiment are reported.
|
|
The translational regulation of
GCN4 in yeast involves
several short upstream open reading frames (uORFs) present in the 5'
leader of the mRNA (reviewed in reference
14).
Translation initiation
at the main cistron occurs by those 40S
ribosomal subunits that
have resumed scanning following
translational termination of the
short uORFs (
14). Whether
40S subunits can resume scanning following
translational
termination of a coding region of typical length
has not been
established in plants. However, in order to prevent
the possibility of
any 40S subunits reaching the intercistronic
region through the
resumption of scanning following translational
termination of the
upstream GUS coding region, the SL used in
Fig.
2 to
4 was introduced
into the 17-, 72-, and 144-nt control
intercistronic sequences. The
73-nt GUS 3'-untranslated region
upstream of the SL provided sufficient
distance between the termination
codon of the GUS coding region and the
SL so that translational
termination from the 5'-proximal cistron would
not be negatively
affected (
24a). Introduction of the SL 7 nt upstream of the distal
cistron (i.e.,
GUS-SL-Con
7-
luc-A
50) resulted in a
level of translation
that was just 17% of that observed for the
corresponding control
(i.e.,
GUS-Con
17-
luc-A
50) in protoplasts
(Fig.
5). Introduction
of the SL into the 72- or 144-nt intercistronic
region (i.e.,
GUS-SL-Con
62-
luc-A
50
or GUS-SL-Con
134-
luc-A
50,
respectively) had
no effect on translation from the distal cistron in
vivo, and
introduction of the SL into the 144-nt
intercistronic region had
no effect in vitro (Fig.
5). The presence of
the SL 62 nt upstream
of the
luc cistron in the dicistronic
construct (i.e.,
GUS-SL-Con
62-
luc-A
50)
reduced
luc expression in vitro (relative to that for the
control
GUS-Con
62-
luc-A
50 construct
[Fig.
5]) just as it had when the
SL was positioned the same distance
upstream of
luc in the analogous
monocistronic construct
(i.e., SL-Con
62-
luc-A
50) during in
vitro
translation (Fig.
2), confirming that 62 nt between an SL and
an
initiation codon is not a sufficiently long distance to permit
optimal
expression of the dicistronic construct in vitro. These
data indicate
that any ribosomal subunits that may resume scanning
from the upstream
GUS coding region do not contribute significantly
to the translation of
the 5'-distal
luc cistron and suggest that
the in vivo
translation of the distal cistron in the 72- or 144-nt
intercistronic
region constructs results from internal
initiation.
The presence of the TEV sequence in the intercistronic region increased
translation from the distal
luc cistron 13.4-fold
relative
to that from the construct containing the 144-nt control
sequence
in the intercistronic region (i.e.,
GUS-Con
144-
luc-A
50)
in
protoplasts (Fig.
6), demonstrating that
the TEV leader sequence
can function to promote translation when in an
intercistronic
position. As above, an SL was introduced immediately
upstream
of the TEV sequence to exclude the possibility of any
ribosomal
subunits reaching the TEV leader sequence. Surprisingly,
instead
of a negative or neutral effect on
luc expression,
as observed
when the control sequence constituted the intercistronic
region,
the presence of the SL upstream of the TEV leader sequence in
a
dicistronic mRNA resulted in an additional 6.1-fold increase
in the
translation of the distal
luc cistron (Fig.
6). This
increase
was specific to expression from the downstream
luc
cistron because
expression from the upstream GUS cistron was not
significantly
affected by the introduction of the SL (data not shown).
Consequently,
the TEV leader sequence positioned downstream of the SL
resulted
in an 82-fold increase in expression from the
luc
cistron relative
to that from the
GUS-Con
144-
luc-A
50 control construct
(Fig.
6).
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|
FIG. 6.
The TEV 5' leader can promote translation from an
intercistronic position. Dicistronic mRNAs with GUS as the
5'-proximal cistron and luc as the 5'-distal cistron were
constructed with intercistronic regions containing the full-length TEV
leader sequence or each CIRE individually. The region of the TEV leader
present in each construct is indicated by a thick line, and the region
of the TEV leader sequence included in each construct is indicated as a
subscript. The 24-bp SL introduced into each construct is indicated
diagrammatically. The control sequence is indicated by a thin line, and
the length of the control sequence (Con) included in the control
construct is indicated as a subscript. Each capped mRNA construct
was synthesized in vitro to terminate in a poly(A)50 tail.
Expression from each mRNA following delivery to carrot protoplasts
by electroporation or following translation in wheat germ lysate is
shown to the right of each construct. Each mRNA construct was
delivered to triplicate samples of protoplasts or translated in
triplicate in vitro, and each sample was assayed in duplicate. The
experiment was repeated a minimum of three times, and the average value
and standard deviation for the constructs of a typical experiment are
reported.
|
|
Similar results were observed when the region of the TEV leader
sequence containing either CIRE-1 or CIRE-2 was introduced
as the
intercistronic region (i.e.,
GUS-TEV
1-65-
luc-A
50 or
GUS-TEV
66-143-
luc-A
50,
respectively). The presence of
either CIRE-1 or CIRE-2 in the
intercistronic region increased
translation from the 5'-distal
luc cistron by 3.6- and 11.7-fold,
respectively, relative to
that from the GUS-Con
144-
luc-A
50
control
construct (Fig.
6). Similar to the results obtained with the
full-length
TEV leader, the introduction of the SL upstream of either
CIRE-1
or CIRE-2 (i.e.,
GUS-SL-TEV
1-65-
luc-A
50 or
GUS-SL-TEV
66-143-
luc-A
50,
respectively) resulted in a further 9.7- or 4.0-fold increase,
respectively, in the translation of the distal
luc cistron
(Fig.
6). Consequently, CIRE-1 or CIRE-2 positioned downstream of the
SL resulted in a 35- or 46-fold increase, respectively, in the
expression from the
luc cistron relative to that from the
GUS-Con
144-
luc-A
50 control
construct. No SL-associated increase was observed when
these same
constructs were translated in vitro, data consistent
with the lack of a
TEV leader-mediated enhancement in translation
lysate as observed in
Fig.
1. These results suggest that the TEV
leader sequence or the
individual CIRE elements can promote translation
when positioned in the
intercistronic region and that the presence
of an SL upstream of these
elements in a dicistronic construct
assists in maintaining their
function as translational
regulators.
| |
DISCUSSION |
In the present study, we identified the regulatory elements within
the TEV 5' leader responsible for promoting cap-independent translation
and determined the extent to which their function was dependent on
proximity to the 5' end. We observed that the TEV 5' leader contained
two elements (i.e., CIRE-1 and CIRE-2) that were required for
cap-independent translation. The 5'-proximal CIRE-1 (present
within a 39-nt region) was less 5' end dependent than the distal
CIRE-2 (present within a 53-nt region), suggesting that the
two elements are functionally distinct. Moreover, as the combinatorial
effect of CIRE-1 and CIRE-2 was approximately multiplicative, both
elements appear to be required to confer full cap-independent
translation and may be considered as components of a single regulatory locus.
The TEV 5' leader confers cap-independent translation, in part,
through a functional interaction with the poly(A) tail (11). Analysis of the function of CIRE-1 and CIRE-2 in
poly(A)+ and poly(A) mRNAs suggests that
the combinatorial effect of CIRE-1 and CIRE-2 is regulated by the
presence of the poly(A) tail. Separation of CIRE-1 and CIRE-2 in
polyadenylated mRNAs resulted in a 9- to 14-fold decrease in
cap-independent translation. In contrast, the separation of CIRE-1 and
CIRE-2 resulted in only a 3- to 4-fold decrease in the cap-independent
translation of nonpolyadenylated mRNAs. These data suggest that one
function of the poly(A) tail on the expression from TEV mRNA
is to increase the combined effect of CIRE-1 and CIRE-2 in order to
promote cap-independent translation.
The TEV leader sequence (or either CIRE) also promoted translation of
the second cistron of a dicistronic mRNA when present in the
intercistronic region. Interestingly, the introduction of an SL
downstream of the first cistron but immediately upstream of the TEV
leader or either CIRE substantially increased the regulatory ability of the TEV leader sequence (Fig. 6). As no similar increase was
observed when the SL was introduced upstream of a control sequence of
equivalent length, these observations suggest that the SL promoted
the TEV regulatory function. Because the presence of the SL
decreased the regulatory function of the TEV sequence when the
latter was present as the 5' leader of monocistronic mRNAs,
the stimulatory effect of the SL on TEV regulatory function is specific
to the dicistronic constructs. We postulate that the SL prevented
interference with the TEV regulatory function by ribosomal subunits
that may have remained associated with the mRNA following
translational termination of the first cistron. Translation of
GCN4 mRNA in yeast requires that 40S subunits resume scanning following translational termination of the short uORFs in the
5' leader. Such 40S subunits are initially incompetent following
translation termination and cannot participate in a subsequent round of
initiation until a new ternary complex, composed of eIF2,
Met-tRNAi, and GTP, has bound (14, 21). As a
minimum distance between a short uORF and the main ORF is necessary,
this has been interpreted to mean that the restoration of translational competence of a 40S subunit by means of binding a new ternary complex
is time dependent. Evidence that ribosomal subunits remain associated
following the translation of a cistron of normal length has been
obtained with electron micrographs of polysomes (8, 18), but
the extent to which these subunits regain competency for translational
initiation while associated with an mRNA is not known. If,
following translational termination of a full-sized 5'-proximal
cistron, a 40S subunit is at least as incompetent for reinitiation as
it is following termination from a minicistron, its scanning through
the TEV leader sequence (as the intercistronic region) may inhibit its
ability to recruit translationally competent 40S subunits and thereby
reduce the extent to which the TEV leader can enhance translation of
the second cistron. Consequently, the introduction of an SL immediately
upstream of the TEV leader sequence might stall incompetent 40S
subunits from scanning into the TEV leader sequence and thereby allow
the TEV leader sequence to function unimpeded to recruit
translationally competent 40S subunits. Thus, the introduction of an SL
upstream of the TEV leader sequence when present in the intercistronic
region of a dicistronic mRNA would act to increase its function.
The inhibitory effect of the SL on the TEV sequence when present as the
5' leader is consistent with this conclusion: the SL would be expected
to reduce but not abolish the regulatory function of the TEV leader
sequence because (i) there is no upstream cistron from which
incompetent 40S subunits may scan and (ii) the TEV leader exhibits a
functional preference for proximity to a free 5' terminus.
As mentioned above, CIRE-1 is functionally less 5' end
dependent than CIRE-2, suggesting that the two elements are
functionally distinct. The multiplicative increase in cap-independent
translation when both elements are present suggests a concerted
mechanism to recruit 40S subunits or to stabilize the association of
40S subunits recruited by one CIRE through interaction with the other CIRE. 40S subunit recruitment may involve direct interaction with a
CIRE or, alternatively, each CIRE may serve as a binding site for
trans-acting factors that mediate 40S subunit recruitment. The latter possibility is supported by the observation that the TEV 5'
leader forms specific complexes with proteins in a gel retardation
assay (37a). Such a trans-acting factor(s) may
preferentially associate with a CIRE when positioned proximal to an
accessible 5' end and may be prevented from binding efficiently to an
intercistronic CIRE if translationally incompetent ribosomal subunits
are transiting between cistrons in a dicistronic mRNA. The
increased function of an intercistronic CIRE positioned downstream of
an SL could be explained if the SL excluded incompetent ribosomal
subunits and thus permitted more-efficient trans-acting
factor binding. These data suggest that significant differences between
the translational regulatory mechanism of those members of the
picornaviral superfamily that infect plants and that of those that
infect animals exist. Those that infect animals contain a highly
structured 5' leader, which can be several hundred nucleotides in
length, whereas the TEV 5' leader is not long or highly structured. And
yet both types of viral leaders direct 40S subunit binding in the
absence of a 5' cap structure. How these different members of the same
viral superfamily achieve the efficient recruitment of the
translational machinery in their respective host species will provide
insight into the similarities and differences in translation in plants and animals.
| |
ACKNOWLEDGMENT |
This work was supported by U.S. Department of Agriculture grant
NRICGP 96-35301-3144 (to D.R.G.).
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Biochemistry, University of California, Riverside, CA 92521-0129. Phone: (909) 787-7298. Fax: (909) 787-3590. E-mail:
drgallie{at}citrus.ucr.edu.
| |
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Journal of Virology, November 1999, p. 9080-9088, Vol. 73, No. 11
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Abstract
Introduction
