From the Division of Cardiovascular Research, Research Institute, Hospital for Sick Children, and Departments of Biochemistry and Laboratory Medicine and Pathobiology, University of Toronto, Toronto, Ontario M5G 1X8, Canada
![]() |
ABSTRACT |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Synthesis of aortic elastin peaks in the
perinatal period and then is strongly down-regulated with postnatal
vascular development. Our laboratory has previously shown that changes
in elastin mRNA stability contribute to this developmental decrease
in elastin production. Here we identify a large region of stable
secondary structure in the 3'-untranslated region (3'-UTR) of chicken
elastin mRNA. Reverse transcriptase polymerase chain reaction or
polymerase chain reaction amplification of the 3'-UTR consistently
resulted in products with an ~328-bp deletion from the central region
of the 3'-UTR, suggesting the presence of secondary structure. The presence of this structure was confirmed by probing the 3'-UTR with
RNases with selectivity for single- or double-stranded RNA. Gel
migration shift assays using cytosolic extracts from 2-day old chicken
aorta demonstrate specific binding of a cytosolic protein to riboprobes
containing the 3'-UTR of elastin but not to riboprobes either
corresponding to other areas of the message or containing the 3'-UTR
but lacking the region of secondary structure. Binding of cytosolic
protein was particularly prominent in aortic extracts from 2-day old
chickens, a time when elastin message is stable, as compared with 8- and 15-week old chickens, when the elastin message is relatively
unstable, suggesting that this region of secondary structure may play a
role in developmental regulation of stability of elastin mRNA.
Elastin is the major matrix protein of elastic ligaments and large
blood vessels, such as the aorta, and also occurs in significant amounts in lung parenchyma, skin, and elastic cartilages. The presence
of elastin in these tissues gives them the physical properties of
extensibility and elastic recoil which are essential for their physiological function. An unusual characteristic of elastin is that,
once firmly incorporated into the extracellular matrix, this protein
does not turn over at any appreciable rate (1, 2). Consistent with this
lack of turnover, production of elastin in tissues such as the large
arteries normally takes place only during vascular development and
growth, after which synthesis and accumulation of the protein
essentially ceases. For example, in the chicken thoracic aorta, elastin
production is very rapid around the time of hatching but has decreased
markedly by 4 weeks and can no longer be detected after 10-12 weeks of
age (3).
Decreased synthesis of elastin after vascular development and growth is
completed is also reflected in marked declines in steady state levels
of mRNA for elastin (see Fig. 1) (3). We have previously reported
that the developmental decrease in steady state levels of mRNA for
elastin was due, at least in part, to decreased stability of elastin
mRNA (4). That is, the half-life of aortic elastin mRNA in the
2-day old chicken, a time at which synthesis is rapid, is approximately
25 h. However, by 8 weeks after hatching, when elastin synthesis
and steady state mRNA levels for elastin have fallen to low levels,
the half-life of this message has decreased to approximately 7 h
(4). Decreased stability of mRNA has also been reported to be
important for developmental regulation of elastin synthesis in rat lung
(5). Furthermore, stability of elastin mRNA has also been reported
to be affected by transforming growth factor- Although several mechanisms for regulating stability of mRNAs have
been described, only a few have been well characterized (10). In
general, removal of 5'-cap structures or 3'-polyadenosine tails are
considered to lead to rapid degradation of messages (11, 12). Sequence
elements in the 3'-untranslated region (3'-UTR)1 have also been
implicated in regulation of the stability of many mRNAs (13-16).
For example, AU-rich elements have been shown to regulate turnover of
several messages, particularly those with a relatively short half-life
(17, 18). Stability of other messages appears to involve C-rich
sequences (19-21). In some cases, rates of turnover and rates of
cleavage have been related to the formation of secondary structures
such as stem-loops or hairpins, with regulatory proteins binding to
these structures to alter susceptibility to RNases (22, 23).
Although stability of the elastin mRNA appears to be an important
factor in the regulation of expression of this protein with development, details of the mechanism of this regulation are still not
understood. The 3'-UTR of elastin is relatively large and contains
regions of substantial sequence similarity among species, suggesting
that these sequences may have some role to play in regulation. In
addition, the 3'-UTR of elastin is unusually rich in G and C
nucleotides (68% in the chicken). High GC content has been related to
the ability to form stable secondary structures in RNA, and such
GC-rich secondary structures have been postulated to be implicated in
regulating stability of other messages (24). Here we report the
presence of a large, stable domain of secondary structure in the 3'-UTR
of chicken mRNA and provide evidence that this structure may play a
role in the regulation of stability of the elastin message with development.
RNA Isolation and Northern Analyses--
Thoracic aortas were
dissected from chickens of different ages. Total RNA was isolated from
these tissues by extraction with guanidine thiocyanate and
centrifugation through CsCl, as described previously (25).
For Northern analyses, 10 µg of total RNA was separated by 1%
agarose gel electrophoresis and transferred to Hybond-N membranes (Amersham Pharmacia Biotech). RNA was cross-linked to the membranes using a UV Stratalinker (Stratagene) and baked at 80 °C for 2 h. Blots were prehybridized for 4 h at 42 °C with 50%
formamide, 5× Denhardt's, 5× saline/sodium phosphate/EDTA, 0.1%
SDS, and 100 µg/ml salmon sperm DNA and then hybridized for 16-18 h
at 42 °C using cDNA probes radiolabeled with
[32P]dCTP by random priming. This was followed by washes
in 2× SSC, 0.1% SDS for 40 min at 55 °C, followed by 0.1× SSC,
0.1% SDS for 30-40 min at 55 °C. The blots were exposed to x-ray
film (Eastman Kodak Co.) at Reverse Transcription of Total RNA--
Total RNA was
reversed transcribed by Superscript II reverse transcriptase (RT) using
the protocol recommended by the supplier (Life Technologies). 1 µg of
total RNA was mixed with 0.5 µg of oligo(dT) primers in 11 µl of
DEPC-treated water. This mixture was incubated for 10 min at 70 °C
and quickly chilled on ice. 7 µl of master mix containing DTT, first
strand buffer, and dNTPs was added. After 2 min of incubation at
42 °C, 200 units of reverse transcriptase was added, and the 20-µl
mixture was incubated at 42 °C for an additional 50 min. The first
strand cDNA product was incubated for 15 min at 70 °C and then
diluted to 50 µl with TE buffer (pH 8.0) and stored at PCR Amplification of cDNA--
The PCR protocol used was
adapted from that recommended for Taq Polymerase (Life
Technologies). The PCR reaction mixture included 1× PCR buffer, 5%
Me2SO, 0.2 mM each of dNTPs, 1.0 or 1.5 mM MgCl2, 0.5 µM of both upper
and lower primers, 2.5 units of Taq DNA polymerase, and 2 µl of first strand cDNA. This solution was kept on ice in a
500-µl Eppendorf tube and overlaid with mineral oil. Each PCR reaction mixture was denatured for 4 min at 95 °C, followed by PCR
amplification using a Robocycle 480 (Stratagene) (denaturation, 1 min
at 95 °C; annealing, 1 min between 51 °C and 65 °C; extension, 1 min at 72 °C). After 30-35 cycles, samples were denatured and annealed as above, except that the incubation at 72 °C was extended to 7 min for 1 cycle. After PCR amplification, 10 µl of each PCR product (total 50 or 100 µl) was analyzed on a 1.5% agarose gel. This PCR product was sequenced using a Pharmacia ALF automated sequencing system.
Primer Sequences--
Gene-specific oligonucleotide PCR primers
were designed based on published chick elastin cDNA sequences
(26-28). The following primers were used for PCR amplification
and analysis of chick elastin 3'-UTR cDNA: A,
5'-ATAGGATCCACCCCACGGCAGCGTCAG-3'; B, 5'-CATGAATTCGCCACCGGGGACCCTTCT-3'; C,
5'-CGGAAGCTTCGGGATCAAGGCGAAAGG-3'; D,
5'-GCCTCTAGACAACCCCAGGCACAGCAC-3'; E,
5'-AATGGATCCTGCTGGGGTTGGAGTTCC-3'; F, 5'-TCCGAATTCCATTAAAAACTTGTCCT-3';
G, 5'-AAGGGATCCAAGACCTACGGAGGAG-3'; H,
5'-CGGAAGCTTCCGCCCACCATCACCGAT-3'; and I,
5'-GCCTCTAGACCATTAAAAACTTGTCCT-3'.
Preparation of pTE2--
pTE2 was a gift of Dr. Shingo
Tajima, National Defense Medical College, Japan. 1 ng/µl pTE2 plasmid
was used to transform DH5 Preparation of cDNA Corresponding to the Region Containing
Secondary Structure--
The cDNA probe was synthesized by PCR,
using the pTE2 as a template and primers A and B as described above.
The upper primer (A) annealed to a sequence approximately 30 nucleotides downstream from the 5'-end of the region of secondary
structure. The lower primer (B) annealed to a sequence approximately 30 nucleotides upstream from the 3'-end of the region of secondary
structure. PCR amplification was as described above, using 1.0 mM MgCl2 and an annealing temperature of
65 °C. PCR products were resolved on a 1.5% agarose gel, and the
280-base band was isolated using a QiaEx II gel extraction kit (Qiagen
Inc.).
Preparation of cDNA Corresponding to a Protein-coding
Sequence from Chick Elastin mRNA--
Total RNA prepared from
3-day old chicken aortic tissue was reverse transcribed using an
oligo(dT) primer and Superscript II reverse transcriptase, as described
above. The resulting first strand cDNA was amplified using primers
C and D, described previously. The upper primer (C) annealed to a
sequence 586 bp downstream from the 5'-end of the chick elastin
cDNA sequence published by Bressan et al. (26). The
lower primer (D) annealed to a sequence 1341 bp downstream from the
5'-end of this sequence. After digestion with HindIII and
XbaI, the 780-bp cDNA product was subcloned into pGEM-4Z.
Preparation of cDNAs Corresponding to the 3'-UTR of Elastin
mRNA--
A cDNA containing the 3'-UTR of elastin, but lacking
the region of secondary structure, was produced by PCR synthesis using pTE2 as a template and primers E and F, described above, in the presence of 1.5 mM MgCl2. The upper primer (E)
annealed to the 5'-end of exon 33 of chick elastin cDNA. The lower
primer (F) annealed to the 3'-end of 3'-UTR, just upstream of the
poly(A) site. After digestion with BamHI and
EcoRI, this resulting 380-bp cDNA product was subcloned
into pGEM-4Z.
A cDNA containing the complete 3'-UTR of elastin with some
additional protein coding sequence was produced by PCR synthesis using
pTE2 as a template and primers G and F, described above, in the
presence of 1.0 mM MgCl2. The upper primer (G)
annealed to the 5'-end of exon 35 of chick elastin cDNA. After
digestion with BamHI and EcoRI, the 600-bp
cDNA product was subcloned into pGEM-4Z.
A cDNA containing the complete 3'-UTR of elastin without protein
coding sequence was produced by PCR synthesis using pTE2 as a template
and primers H and I, described above, in the presence of 1.0 mM MgCl2. The upper primer (H) annealed to the
5'-end of the 3'-UTR. The lower primer (I) annealed to 3'-end of the
3'-UTR. After digestion with HindIII and XbaI,
the 500-bp cDNA product was subcloned into pGEM-4Z. These PCR
products were sequenced using a Amersham Pharmacia Biotech ALF
automated sequencing system.
Preparation of in Vitro Transcripts--
A riboprobe in
vitro transcription system (Promega Corp.) was used to produce RNA
transcripts from 1 µg of linearized plasmid DNA. RNAs were
transcribed using T7 RNA polymerase at 37 °C for 1 h in the
presence of [ Preparation of Cytoplasmic Extracts--
Thoracic aortas
dissected from 2-day old and 15-week old chickens were rinsed with
phosphate-buffered saline, cut into small pieces, and transferred to a
7-ml Dounce homogenizer containing 2 ml of ice-cold hypotonic buffer
(25 mM Tris-HCl (pH 8), 0.5 mM EDTA). The
tissues were then homogenized using 20 strokes with a tight-fitting
pestle. Homogenates were centrifuged at 10,000 × g for
20 min at 4 °C, and the resulting supernatants were removed and
quickly frozen at RNA Mobility Shift Assays--
Cytoplasmic extracts containing
8-10 µg of protein were incubated at 20 °C for 30 min with
2-4 × 104 cpm of 32P-labeled transcripts
in 5 mM Hepes buffer (pH 7.9), containing 0.5 mM MgCl2, 7.5 mM KCl, 0.5 mM DTT, 0.12 mM EDTA, and 200 ng/µl yeast
tRNA (Sigma-Aldrich), in a total volume of 20 µl. For competition experiments, proteins were pre-incubated with a 150-fold excess of
unlabeled competitor RNA for 30 min at 20 °C, followed by incubation with the labeled RNA for another 30 min at 20 °C. Reaction mixtures were then incubated with 1:100-1:150 dilution of RNase Plus
(0.83-1.25 units/ml RNase T1, 0.005-0.007 units/ml RNase
A, 5 Prime RNase Digestion--
Radiolabeled in vitro
transcribed riboprobes (4 × 104-8 × 104 cpm) were heated to 100 °C and cooled slowly to room
temperature. Enzymatic digestions of the riboprobes were carried out in
Hepes buffer (10 mM Hepes (pH 7.9) containing 40 mM KCl, 3 mM MgCl2, 1 mM DTT, and 0.5 µg/ml yeast tRNA) with either 0.625 units/µl RNase T1 (5 Prime
RNA molecular size standards were produced by in vitro
transcription of a mixture of RNA templates (Century Marker Plus,
Ambion Inc.) in the presence [ RNA Folding Software--
RNA secondary structure predictions
were performed using Zuker's MFOLD program as implemented in the GCG
molecular biology software package (Wisconsin Package Version 9.0, Genetics Computer Group (GCG), Madison, WS).
Initially an RT-PCR approach was used to obtain a full-length
3'-UTR from chicken mRNA. For this purpose, RNA was isolated from
18-day embryo chickens, a time when elastin synthesis is rapid and
elastin mRNA is abundant (Fig. 1).
However, for several pairs of primers spanning the 3'-UTR region of the
mRNA, RT-PCR products were always smaller than expected. Moreover,
if one or both primers were situated in the central region of the
3'-UTR, no product was seen. The size discrepancy between products
expected and found was consistently approximately 300 bases. However,
RT-PCR products using primers located within the coding region of the mRNA were always of the expected size.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
(TGF-
) (6, 7),
phorbol esters (8), and vitamin D (9).
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
70 °C. Equal loading of lanes for
Northern blotting was confirmed by ribosomal RNA bands visualized by
ethidium bromide staining. cDNA probes for chicken elastin included
pCEL, a gift of Dr J. A. Foster, Department of Biochemistry,
Boston Medical School, Boston, MA.
20 °C
until further use. A similar reaction without the addition of RT was
always performed in parallel as a negative control.
competent cells. After transformation,
cells were plated on an LB-ampicillin culture plate to select for
ampicillin-resistant pTE2-containing colonies. pTE2 DNA was isolated
from bacterial culture by a standard alkaline lysis method followed by
two extractions with phenol/chloroform/isoamyl alcohol (24:24:1). The
protocol used for PCR amplification from pTE2 DNA templates was as
described above.
-32P]CTP (3000Ci/mmol), nucleotides,
RNase inhibitor, and buffer mixture as recommended by the manufacturer.
One unit of RNase-free DNase was added to the reaction mixture for 15 min at 37 °C to remove template DNA. After phenol/chloroform
extraction, the transcripts were precipitated using 2.4 M ammonium acetate and ice-cold 100% ethanol for 1.5 h at
70 °C. The RNA pellets were resuspended in 30 µl of
RNase-free TE (pH 8.0), and purified on a RNase-free G-25 RNA
purification column (Boehringer-Mannheim). Determination of percent
incorporation of radiolabeled nucleotides into transcripts was done by
TCA precipitation. The integrity of the RNA was confirmed by 6% native
polyacrylamide gel electrophoresis. Unlabeled RNA transcripts were
generated in a similar manner but in the absence of
[
-32P]CTP.
20 °C. Protein concentrations were determined using the BCA protein assay reagent (Pierce) using bovine serum albumin
as a standard. Total protein extracted from aortas of chickens at
different ages was similar (2.3 mg/100 mg tissue wet weight from 2-day
old as compared with 1.8 mg/100 mg tissue wet weight from 15-week old).
Equal loadings of extracts from aortas of different ages on
SDS-polyacrylamide gel electrophoresis also showed similar protein
profiles after staining with Coomassie Blue (data not shown).
Furthermore, Western blotting of these gels with antibodies to
-tubulin and
-actin showed similar quantities of these cytosolic
proteins in aortic extracts from 2-day and 15-week old chickens (data
not shown).
3 Prime Inc.) for a further 15 min at 37 °C.
Electrophoresis of RNA-protein complexes was carried out on a 6%
native polyacrylamide gel (acrylamide/bisacrylamide ratio = 60/1)
with 0.3 × TBE (Tris borate-EDTA) running buffer (pH 8.4). The
gels were subsequently dried under vacuum at 80 °C for 1 h and
exposed to x-ray film at
70 °C.
Prime, Inc.) or 9 × 10
3 units/µl of RNase V1 (Amersham
Pharmacia Biotech), or a combination of both enzymes for 8 min at
37 °C. After phenol/chloroform extraction, the digested RNA products
were precipitated using 2.4 M ammonium acetate and ice-cold
100% ethanol for 1-2 h at
70 °C. The RNA pellets were
resuspended in sample solution (10 M urea, 1.2 mM EDTA, 6% glycerol, 0.06% bromphenol blue, and 0.06%
xylene cyanole tracking dye), heated to 70 °C for 10 min, and then
cooled on ice. Electrophoresis was carried out on an 8.3 M
urea, 8% polyacrylamide gel with 1× TBE running buffer. The gels were
subsequently dried under vacuum at 80 °C for 3 h and exposed to
a PhosphorImager screen (Molecular Dynamics).
-32P]CTP (3000 Ci/mmol).
The radiolabeled RNA markers were then purified in a manner similar to
that of the radiolabeled RNA transcripts used in RNA gel shift assays.
Typically, 1 × 104 to 1.5 × 104 cpm
of RNA markers were used per experiment.
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
View larger version (69K):
[in a new window]
Fig. 1.
Decrease in steady state elastin mRNA
levels with development. Total RNA was isolated from aortic tissue
of chickens at the 18 day embryo (18d emb) stage and at 3 days and 4, 8, and 15 weeks after hatching. For Northern blotting, 10 µg of total RNA was separated by 1% agarose gel electrophoresis,
transferred to Hybond-N membranes, and probed with a chicken elastin
cDNA (pCEL). Loading of RNA in gel lanes is indicated by ethidium
bromide staining of the gel (bottom).
Although sequences of the protein coding region of chicken elastin had been reported previously by several investigators (26-28), only one clone reported included the sequence of the entire 3'-UTR of chicken elastin (27). This clone, designated pTE2, was obtained from Dr. Shingo Tajima, National Defense Medical College, Japan, and used in a PCR approach as an alternative method to obtain the complete 3'-UTR of chicken elastin. However, as observed using the RT-PCR procedures, while primers to the coding region of the clone yielded the expected products, primers spanning the 3'-UTR again resulted in products approximately 300 bases shorter than expected. Restriction digests of the pTE2 clone confirmed that these results were not because of a truncated 3'-UTR in the pTE2 cDNA template. Furthermore, lowering of the concentration of magnesium chloride from 1.5 to 1.0 mM in the PCR reaction resulted in the shift of the major PCR product to the expected size.
Sequencing of RT-PCR products from isolated RNA and PCR products
from the pTE2 clone revealed that the size discrepancies of the
products were, in fact, because of the absence of a central region of
the 3'-UTR consisting of 328 bases (Fig.
2). Otherwise, the sequence corresponded
to that reported for the 3'-UTR of elastin mRNA (27). The location
of the missing region was consistent between RT-PCR and PCR products.
Furthermore, sequencing of additional RT-PCR and PCR products using
other primer pairs demonstrated a deletion at the same site (data not
shown). Moreover, sequencing of the larger PCR product produced under
low magnesium conditions showed that this product had the expected
sequence corresponding to the full-length 3'-UTR of chicken elastin
(Fig. 2).
|
Although restriction digests of pTE2, and PCR of pTE2 under
conditions of lower magnesium concentration, confirmed that this clone
contained the full-length elastin 3'-UTR, attempts to alter RT-PCR
conditions to produce a similar full-length product from isolated RNA
were consistently unsuccessful. To confirm that the missing region was,
in fact, present in the mRNA, a cDNA probe corresponding to the
deleted region was prepared by PCR from pTE2 at 1.0 mM
MgCl2. Northern blots using this probe confirmed that the
deleted region was indeed present in the isolated RNA used for RT-PCR
(Fig. 3).
|
Whereas the entire 3'-UTR of chick elastin is relatively GC rich (68%), the GC content is particularly high in the deleted domain (79%). Consistent with its high GC content, RNA folding software (MFOLD) predicted that this region could form extensive, stable secondary structures through internal base pairing. Predicted structures of this region consistently indicated that ~70% of the bases were paired. This region of secondary structure included more than 50% of the 3'-UTR of elastin message.
The presence of a large region of stable double-stranded RNA in the
3'-UTR of chicken elastin was further confirmed by treatment of
riboprobes corresponding to various regions of the elastin mRNA
(Fig. 4A) with RNases with selectivity
for single-stranded or double-stranded RNA. Incubation of radiolabeled
riboprobes containing the 3'-UTR of elastin (RP2) with RNase
T1, an RNase with selectivity for G nucleotides in
single-stranded RNA, resulted in incomplete digestion, leaving a
discrete band corresponding to regions of the riboprobe resistant to
digestion. However, incubation with both RNase V1 and RNase
T1 resulted in complete digestion of the riboprobe.
Digestion with RNase V1 alone also resulted in complete
digestion of the riboprobe, except for a faint band corresponding in
size to the undigested riboprobe. Similar results were seen with RP1, a
second riboprobe containing the 3'-UTR of elastin (data not shown). In
contrast, a riboprobe corresponding to the protein coding region of
elastin mRNA (RP3) was completely digested by RNase T1
(Fig. 4C). Effects on RP3 of RNase V1 alone or a
combination of RNase T1 and RNase V1 were
essentially identical (data not shown). These results were consistent
with the presence of large regions of double-stranded RNA in the 3'-UTR
of the elastin message.
|
Gel migration shift assays using riboprobes corresponding to the 3'-UTR
of elastin (RP1, RP2, Fig. 4A) demonstrated the presence of
a protein or proteins in cytosolic extracts of 2-day old chicken aorta,
which bound to these riboprobes (Fig. 5,
B and C). Such binding was much less prominent
using cytosolic extracts from aortas of 15-week old chickens, a
developmental time when the mRNA of elastin is considerably
destabilized (4). Cytosolic extracts from aortas of 8-week old chickens
showed intermediate binding (Fig. 5B). No binding was seen
either with a riboprobe corresponding to the coding region of elastin
mRNA (RP3), or with a riboprobe of the 3'-UTR lacking the region of
secondary structure (RP4), suggesting that the region of secondary
structure in the 3'-UTR was required for binding of this cytosolic
factor. Binding to the radiolabeled riboprobe could be competed away
using unlabeled riboprobe RP1, corresponding to the 3'-UTR, but not by
riboprobe RP3, corresponding to the coding sequence (Fig.
5C). Binding to the 3'-UTR riboprobes was also abolished by
pre-treatment of the cytosolic extracts with proteinase K (data not
shown).
|
![]() |
DISCUSSION |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
The abundance of elastin mRNA in aortic tissues of perinatal animals is consistent with the rapid synthesis and accumulation of elastin in these tissues at this stage of development (3). Similarly, the rapid decrease in steady state mRNA levels of elastin with post-natal development and growth corresponds to decreases in synthesis over this developmental period. We had previously shown that decreased stability of elastin mRNA over this developmental period contributed to the decline in steady state mRNA (4). Evidence from others also indicated that stability of elastin mRNA is likely to be an important site for regulation of synthesis of this protein (6-9).
The unusually high GC content of the 3'-UTR of chicken elastin mRNA had raised the possibility of the presence of secondary structures in this region of the elastin message. Our data, using primers spanning the 3'-UTR of elastin, demonstrated that RT-PCR or PCR products were consistently shorter than expected by approximately 300 bases. Sequencing clearly demonstrated that this shortening was because of the consistent deletion of a central region of the 3'-UTR of the elastin message. This deleted region contained 328 bases, was particularly GC-rich (79%), and was capable of forming stable secondary structures with ~70% of the bases paired. Deletion of this region from PCR products of the elastin 3'-UTR was not because of the absence of this sequence from the pTE2 clone, as demonstrated both by restriction digests and by the fact that full-length products with the expected sequence could be obtained by PCR of this clone under conditions of lower magnesium chloride concentration. Furthermore, Northern blotting with probes specific to the missing region of the 3'-UTR showed that the inability to obtain a full-length product by RT-PCR was not because of the absence of this region from the RNA used in the reaction. Mechanisms accounting for the ability of a polymerase copying a template to skip a large region and then resume faithful transcription of the remainder of the sequence have been proposed by others to explain internal deletions occurring during DNA synthesis by DNA polymerase (29-32). In all cases, these models require that the deleted sequence contains a region of stable secondary structure. Our observations were therefore consistent with the presence of a large region of secondary structure in the 3'-UTR of elastin mRNA across which the polymerase or reverse transcriptase could skip in the PCR or RT-PCR reactions, continuing the replication of the sequence beyond the site of secondary structure. The role of secondary structure in this deletion event is supported by the fact that shortened PCR products were promoted by higher magnesium concentrations, since magnesium has been reported to promote base pairing into higher order structures (33-36).
Similar deletions in RT-PCR or PCR products using primers spanning the 3'-UTR of elastin from other species have not been described. This may be related to the fact that the 3'-UTR of chicken elastin mRNA is both the shortest and the most GC-rich of those reported. Indeed it is interesting to note that, of the three chicken elastin clones for which sequence is available (26-28), only one contained a complete 3'-UTR (27). Thus, chicken elastin message may have been a fortuitous choice to demonstrate the presence of this secondary structure. Although these structures are perhaps particularly stable and thus most easily demonstrated in chicken elastin, they may nevertheless also be present in, and important for the stability of, elastin message in other species.
Resistance of riboprobes corresponding to the 3'-UTR of elastin mRNA to digestion with RNase with specificity for single-stranded RNA offered further evidence for the presence of this region of stable secondary structure. Digestion of RP2, a riboprobe containing the entire 3'-UTR of elastin message, with RNase T1 resulted in a residual product corresponding to ~200 nucleotides. Although this is somewhat smaller than the 328 nucleotides predicted to be involved in the region of secondary structure, this can be accounted for by the fact that loops or bulges in this structure containing unpaired G nucleotides would also be susceptible to the enzyme. These data, together with the ability of a combination of RNase V1 and RNase T1 to digest RP2 completely, were consistent with the presence of a large region of secondary structure. Furthermore, the ability of RNase T1 to digest completely a riboprobe corresponding to the coding sequence of elastin mRNA (RP3) confirmed that this resistance of the 3'-UTR to digestion was not a general characteristic of all regions of the elastin message.
The presence of secondary structure in the 3'-UTR of elastin
mRNA does not necessarily implicate such structures in
developmental regulation of the stability of the elastin message.
However, evidence from gel mobility shift assays clearly demonstrates
specific binding of a cytosolic protein or complex of proteins to
riboprobes containing the 3'-UTR of elastin. Such binding is not seen
to riboprobes corresponding to other areas of the elastin mRNA and
appears to require the presence of the region of secondary structure
because a riboprobe containing the 3'-UTR sequence but lacking the
deleted region showed no binding. Moreover, binding of the cytosolic
protein to the 3'-UTR of elastin mRNA is particularly prominent for
extracts of aortic tissue from 2-day old chickens, a period when
elastin mRNA is known to be stable (4), as compared with binding of cytosolic extracts from 8- and 15-week old chickens, when the elastin
message is relatively unstable. It is unlikely that this difference in
binding pattern between cytosolic extracts of 2-day and 15-week old
aortic tissue could be accounted for by differential protein extraction
because total soluble protein recovered from these tissues was similar,
patterns of proteins in the extracts were similar on Coomassie Blue
staining after SDS-polyacrylamide gel electrophoresis, Western blotting
demonstrated similar quantities of -actin and
-tubulin in these
cytosolic extracts, and similar amounts of total soluble protein were
used in each of the gel mobility shift assays.
In summary, we have demonstrated the presence of a large region of
stable secondary structure in the 3'-UTR of chicken elastin. Gel
mobility shift assays indicate that binding of cytosolic proteins to
this region of secondary structure is correlated with developmental periods of stability of the elastin mRNA, suggesting that such structure may play a role in developmental regulation of stability of
elastin mRNA. Investigations to characterize specific binding sequences and their trans-acting proteins, and to confirm the potential
role and mechanisms of these factors in determining elastin message
stability, are now underway.
![]() |
FOOTNOTES |
---|
* This work was supported by grants from the Medical Research Council of Canada and the Heart and Stroke Foundation of Ontario.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.
Recipient of Studentship award from the Medical Research Council
of Canada.
§ To whom correspondence should be addressed: Division of Cardiovascular Research, Hospital for Sick Children, 555 University Ave., Toronto, ON M5G 1X8, Canada. Tel.: 416-813-6704; Fax: 416-813-7480; E-mail: fwk{at}sickkids.on.ca.
![]() |
ABBREVIATIONS |
---|
The abbreviations used are: 3'-UTR, 3'-untranslated region; DEPC, diethyl pyrocarbonate; dNTPs, deoxynucleotide triphosphates; TE, Tris-EDTA; PCR, polymerase chain reaction; DTT, dithiothreitol; RT-PCR, reverse transcription-polymerase chain reaction; TBE, Tris borate-EDTA; bp, base pair(s); RP, riboprobe.
![]() |
REFERENCES |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|