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Molecular and Cellular Biology, January 1999, p. 657-670, Vol. 19, No. 1
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Direct Regulation of Mitochondrial RNA
Synthesis by Thyroid Hormone
José A.
Enríquez,*
Patricio
Fernández-Silva,
Nuria
Garrido-Pérez,
Manuel J.
López-Pérez,
Acisclo
Pérez-Martos, and
Julio
Montoya*
Departamento de Bioquímica y
Biología Molecular y Celular, Universidad de Zaragoza,
E-50013 Zaragoza, Spain
Received 18 June 1998/Returned for modification 27 July
1998/Accepted 15 September 1998
 |
ABSTRACT |
We have analyzed the influence of in vivo treatment and in vitro
addition of thyroid hormone on in organello mitochondrial DNA (mtDNA)
transcription and, in parallel, on the in organello footprinting
patterns at the mtDNA regions involved in the regulation of
transcription. We found that thyroid hormone modulates mitochondrial RNA levels and the mRNA/rRNA ratio by influencing the transcriptional rate. In addition, we found conspicuous differences between the mtDNA
dimethyl sulfate footprinting patterns of mitochondria derived from
euthyroid and hypothyroid rats at the transcription initiation sites
but not at the mitochondrial transcription termination factor (mTERF)
binding region. Furthermore, direct addition of thyroid hormone to the
incubation medium of mitochondria isolated from hypothyroid rats
restored the mRNA/rRNA ratio found in euthyroid rats as well as the
mtDNA footprinting patterns at the transcription initiation area.
Therefore, we conclude that the regulatory effect of thyroid hormone on
mitochondrial transcription is partially exerted by a direct influence
of the hormone on the mitochondrial transcription machinery.
Particularly, the influence on the mRNA/rRNA ratio is achieved by
selective modulation of the alternative H-strand transcription
initiation sites and does not require the previous activation of
nuclear genes. These results provide the first functional demonstration
that regulatory signals, such as thyroid hormone, that modify the
expression of nuclear genes can also act as primary signals for the
transcriptional apparatus of mitochondria.
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INTRODUCTION |
Thyroid hormone regulates the
expression of key nucleus encoded mitochondrial genes (23, 37, 38,
47) and the steady-state concentration of all mitochondrial DNA
(mtDNA)-encoded mRNAs (mt-mRNAs) (15-17, 32, 44). In rat
liver, changes in mt-mRNA levels in response to in vivo treatment with
thyroid hormones were well correlated with amounts of the corresponding
polypeptides, while mtDNA copy number remained unmodified (33,
47). Based on these observations, transcriptional control has
been tentatively proposed as the main mechanism to explain the thyroid
hormone effect on mt-mRNA steady-state levels and protein synthesis
(33-36).
Two alternative potential mechanisms for the regulation of mtDNA
transcription by thyroid hormone have been suggested: through activation of mitochondrial transcription factor A (mtTFA)
expression (18, 45), or by a direct action of the
hormone through mitochondrial receptors (48). The second
alternative is supported by earlier (42, 43) and recent
(1, 48) reports that have proposed the existence of
T3 (3,3,5-triiodo-L-thyronine) binding proteins in mitochondria, which could interact with cis elements of
mtDNA (7, 48). However, the lack of experimental evidence
showing thyroid hormone-mediated transcription regulation in the
absence of nuclear gene expression prevents any definitive conclusion about whether direct regulation of mtDNA transcription by this hormone
occurs (38). Presently it is more generally believed that
this transcriptional regulation, if it exists, could be
exclusively exerted through the activation of nucleus encoded
transcription factors (22, 33, 36, 41, 47).
The influence of thyroid hormone on the steady-state level of mtRNAs,
however, represents a more complex situation. Reports from several
groups showed a decrease in the in vivo steady-state mRNA/rRNA
ratio in hypothyroid versus euthyroid mitochondria (referred to
hereafter in this work as hypothyroid and euthyroid mitochondria, respectively). This effect was mainly due to a decrease in the mRNA
levels, since rRNA levels were not (17, 32) or were only slightly (44) affected. Therefore, the proposed
transcriptional control should be able to discriminate between mRNA
and rRNA genes, although different effects of T3 on the
stability of mRNAs and rRNAs could also account for this phenomenon.
Several mechanisms could potentially be responsible for the
discrimination between mRNA and rRNA synthesis. The mammalian mtDNA H strand encodes the two rRNAs and all but one of the
mt-mRNAs, and it is transcribed as two polycistronic
molecules (31). The smaller polycistron, responsible
for synthesis of the rRNAs, completely overlaps the larger one,
responsible for synthesis of the mRNAs. Two models have been
proposed to explain the independent regulation of mRNA and
rRNA syntheses in mammalian mitochondria. One model is based on the
identification of the 5' end of the transcripts synthesized on a
partially reconstructed in vitro transcription system (6,
13), and it proposes that the synthesis of both polycistrons starts at a single initiation site, upstream of
the tRNAPhe gene. The polymerase transcribes the rRNA genes
more frequently stopping at the 3' end of 16S rRNA due to the binding
to mtDNA of a mitochondrial transcription termination factor (mTERF)
(6, 12, 21, 25). Occasionally, the polymerase is able to
pass through this termination point and then also synthesize the
mRNAs. A second model, based on the identification of the 5' end of
the in vivo synthesized primary transcripts, proposes the existence of
two sites for H-strand transcription initiation. Thus, synthesis of the
small polycistron starts at the IH1 initiation
site, upstream of the tRNAPhe gene (31), which
corresponds to the unique initiation site in the previous model.
Synthesis of the larger polycistron starts at the
IH2 initiation site, at the border between the 12S rRNA and
tRNAPhe genes (3, 30, 31). According to this
model, when transcription initiates at the IH1 site, it
normally stops at the 3' end of 16S rRNA due to the action of mTERF. In
this model, when the polymerase initiates at the IH2 site,
it is able to read through the mTERF-dependent termination,
transcribing almost the whole mtDNA H strand, including both rRNAs and
most of the mRNAs. Thus, in the first model, regulation of the
mRNA/rRNA ratio could be achieved only by modulation of the
transcription termination at the mTERF binding site. The second model
suggests that this ratio could be preferentially modulated by changing
transcription initiation between IH1 and IH2.
Interestingly, the regulation of the mRNA/rRNA ratio by thyroid
hormone represents an occasion to address both models.
To discriminate between the alternative mechanisms proposed for the in
vivo-induced changes in the steady-state level of mtRNAs by thyroid
hormone, as well as for its selective influence on mRNA versus rRNA
synthesis, we took advantage of a highly efficient in organello
transcription system (9, 10), using liver mitochondria isolated from rats differing in thyroid status. Thus, we have analyzed
the influence of the in vivo treatment and the in vitro addition of
thyroid hormone on in organello mtRNA synthesis and stability. In
parallel, using transcriptionally active organelles, we have
investigated the influence of the hormone on the in organello footprinting patterns at the mtDNA regions involved in the regulation of transcription. The results presented in this report confirm that
transcriptional control is the main mechanism underlying the thyroid
hormone effect on mtRNA steady-state concentration. In addition, they
strongly support a model in which this regulation is achieved by acting
at multiple levels and involving both genomes. Here, we show that the
action of T3 on control of the mRNA/rRNA ratio is
exclusively due to changes in transcriptional rate and is exerted
directly on mitochondria, without prior activation of nuclear genes.
Our results also suggest that this effect is achieved by selective
modulation of the activity of the alternative H-strand transcription
initiation sites.
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MATERIALS AND METHODS |
Animals.
Hypothyroidism was induced in male Wistar rats
weighing 200 to 250 g by administration of 0.05% (wt/vol)
propylthiouracyl (PTU) in drinking water for 4 to 8 weeks. A subgroup
of hypothyroid rats (treated group) were injected intraperitoneally
once daily with 20 µg and 3 µg of T4
(3,3',5,5'-tetraiodo-L-thyronine) and T3,
respectively, per 100 g of body weight for 2 days, and the animals
were killed 15 h after the second treatment. Hyperthyroidism was
induced in euthyroid rats by daily intraperitoneal injections of the
same amount of T4 and T3 as before for 5 days,
and the rats were used for experimentation on day 6 after initiation of treatment. Control hypothyroid and euthyroid rats were injected for the
same time period with the same volume of vehicle (0.9% NaCl-propylene glycol).
In organello RNA synthesis and pulse-chase experiments.
Mitochondria were isolated from rat liver as previously described
(9, 10) and incubated at a final mitochondrial protein concentration of 2 mg/ml in 0.5 ml of incubation buffer containing 25 mM sucrose, 75 mM sorbitol, 100 mM KCl, 10 mM
K2HPO4, 0.05 mM EDTA, 5 mM MgCl2, 1 mM ADP, 10 mM glutamate, 2.5 mM malate, 10 mM Tris-HCl (pH 7.4), and 1 mg of bovine serum albumin per ml in 1.5-ml Eppendorf tubes (9,
10). For in organello transcription analysis, 20 µCi of
[
-32P]UTP (400 to 600 Ci/mmol) was added to the
medium, and incubation was maintained at 37°C for 60 min in a rotary
shaker (12 rpm). For pulse-chase experiments, isolated mitochondria
were prelabeled with [-32P]UTP for 2 h; then the
mitochondrial samples were pelleted at 13,000 × g for
1 min, and the supernatant with the nonincorporated [-32P]UTP was removed. Then, the mitochondria were
resuspended in incubation medium in the presence of a 200-fold excess
of unlabeled UTP and incubated for various periods of time before
harvesting (9). Mitochondrial nucleic acids were extracted
and analyzed by methylmercury hydroxide-agarose gels as previously
described (11). Subsequently, the gels were first stained
with ethidium bromide and photographed under UV light and then dried
and exposed for autoradiography either at 
70°C with a DuPont screen
intensifier or at room temperature. Amounts of RNA on the
autoradiograms were quantified, after selection of the appropriate
exposures, with an LKB Ultroscan XL laser densitometer and Gel Scan XL software.
In organello and in vitro footprinting.
For methylation
interference assays, mitochondria were incubated for 30 min as
described above, then dimethyl sulfate (DMS) was added to a final
concentration of 0.1% and allowed to react for 2 min at 37°C, and
the mixture was quickly cooled on ice. Then 1 ml of ice cooled
incubation buffer was added, and the organelles were spun down for 1 min at 13,000 rpm. This wash was repeated twice, and mtDNA was isolated
as described below. For each set of in organello footprinting
experiments, a sample of the mitochondrial fraction was treated
identically except for the omission of DMS, and mtDNA was extracted.
For in vitro DMS treatment of naked mtDNA, 15 to 25 µg of
mitochondrial nucleic acids derived from non-DMS-treated organelles was
resuspended in 200 µl of Tris-EDTA, DMS was added to a final
concentration of 0.1% and allowed to react for 2 min at 37°C, and
the mixture was quickly cooled on ice. Then the reaction was stopped by
adding 50 µl of DMS stop buffer (1.5 M sodium acetate [pH 7.0], 1 M
2-mercaptoethanol). Finally, mtDNA was recovered by ethanol
precipitation (28).
Piperidine cleavage of DNA was performed on pellets containing mtDNA
from in organello DMS-treated mitochondrial fraction and on equivalent
samples of in vitro DMS-treated total mitochondrial nucleic acids as
described previously (28).
Primer extension of the DMS-treated mtDNA.
The following
oligodeoxynucleotides, designated according to the numbering system of
Gadaleta et al. (14), were used for primer extension:
H30-5'-GAATCCATCTAAGCATTTTCAG-3' (designated P-REV1 in
reference 5),
H175-5'-TATATTATGTGCTTGATGCCCT-3', L16108-5'CCCCAAAAACATTAAAGCAAGA-3' (D-Rat-viv-2 in
reference 5), and
L16228-5'-GACACAAAATCTTTCCTCCTAA-3' for footprinting of the
transcription initiation areas; H16107-5'TTTGGCATTGAAGTTTCAGGTG-3' (D-REV2 in reference 5) and
L15747-5'-ACTGAAACTTTACAGGCATCTG-3' for footprinting of the
region containing the putative thyroid-responsive element (TRE); and
H2761-5'-GATTAGGAGTGTTAGGATATTA-3' (ND1 in reference
5) and L2542-5'-CCCAGTTACGAAAGGACAAGAG-3' (16S
in reference 5) for footprinting of the rDNA
transcription termination region. These oligodeoxynucleotides were
5'-end labeled with [
-32P]ATP as detailed previously
(28).
DMS-treated and piperidine-cleaved mtDNA (0.5 µg) was used as a
template for primer extension analysis with the appropriate
labeled
oligodeoxynucleotide. PCR amplification and electrophoresis
of the
products through 6% polyacrylamide (19:1 acrylamide/bisacrylamide)-7
M urea sequencing gels in Tris-borate-EDTA buffer were carried
out as
previously described (
28).
DMS is known to methylate mainly guanine and, with lower frequency,
adenine residues (
27). Cytosine and thymine can also
be
methylated when in single-stranded DNA, with the alkylation
of the
latter being favored in alkaline solution (
27). In the
present work, the majority of methylation reactivity changes were
observed at purine sites, although some pyrimidines also showed
an
altered methylation pattern as reported by others (
5,
20,
29). The methylation of cytosine residues in organello was
explained
by the occurrence of single-stranded DNA segments at those
sites
as a result of helical distortions caused by protein binding or
by RNA polymerase pauses (
29). In the case of thymine, it
was
suggested that the alkaline environment of the mitochondrial matrix
would favor its methylation (
29).
| |
RESULTS |
The transcriptional ability of isolated mitochondria is
predetermined in vivo by thyroid hormone.
To investigate the
mechanism responsible for the in vivo-induced changes in the
steady-state level of mitochondrial mRNAs by thyroid hormones, we
performed in organello transcription experiments with isolated rat
liver mitochondria purified from rats of four different thyroid states:
a control group (euthyroid animals), a group treated for a minimum of 1 month with drinking water containing PTU (17) (hypothyroid
animals), a group injected for 5 consecutive days with constant doses
of hormone (hyperthyroid animals), and a group consisting of
hypothyroid animals injected for 2 days with the same hormone doses
(treated animals). The body weight of the animals, monitored to follow
the influence of the PTU treatment, reached an average difference of
1.4-fold in favor of the euthyroid animals compared with the
hypothyroid ones. Blood samples of all the animals were collected at
the moment of sacrifice, and the levels of hormones were analyzed by
radioimmunoassay to check their thyroid status (Table
1).
As shown in Fig.
1A, transcription was
more active in the organelles isolated from animals with higher plasma
concentrations
of thyroid hormones. Thus, hypothyroid mitochondria
showed a 50%
reduction of the radioactivity incorporated into RNA
compared
with euthyroid organelles. Furthermore, this decrease was
partially
restored by in vivo treatment of the hypothyroid animals with
thyroid hormone. In agreement with this general trend, isolated
organelles from hyperthyroid rats were able to accumulate labeled
RNA
at a higher rate than controls.
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FIG. 1.
In organello RNA synthesis in rat liver mitochondria
isolated from animals of different thyroid status. (A) Diagram showing
the overall transcriptional rate of mitochondria isolated from
euthyroid (E), hypothyroid [1-month PTU treatment; H
(1M)], treated [hypothyroid treated with hormone; T (1M)], and
hyperthyroid (H+) animals. Data were normalized to the
content of mtDNA in each lane, taking the euthyroid value as 100%, and
are given as mean ± standard error of the mean (n = 5). (B) Electrophoretic patterns of the in organello-synthesized
RNAs by mitochondria from the indicated thyroid status (lanes 1 to 4)
and from hypothyroid rats obtained by 2-month PTU treatment
[H (2M)] and 2-month hypothyroid treatment with hormone
[T (2M)] (lanes 5 and 6). Similar amounts of total radioactivity
incorporated into RNA were loaded on lanes 1 to 4, and amounts of mtRNA
synthesized by equivalent fractions of mitochondria were loaded on
lanes 5 and 6. (C) Relative mRNA/rRNA ratio for different
representative mRNAs synthesized by mitochondria isolated from rats
of the indicated thyroid status. The values (mean ± standard
error of the mean n = 5) correspond to the ratio
mRNA to all transcribed 16S rRNA genes (see text) and are given as
relative to the euthyroid ratio (100%). The differences in
mRNA/rRNA ratio between the euthyroid group and the hypothyroid and
hyperthyroid groups were significant (P < 0.005) by
Student's t test. COI, COII, and COIII, mRNAs for
subunits I, II, and III of cytochrome c oxidase; ND1, ND2,
ND3, ND4/4L, and ND5, mRNAs for subunits 1, 2, 3, 4, 4L, and 5 of
the NADH dehydrogenase; A6/8, mRNA for subunits 6 and 8 of
H+-ATPase; Cyt b, mRNA for apocytochrome b;
p-rRNAs, precursors of rRNAs; p-CoI, precursor of COI mRNA.
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|
Besides this general effect of thyroid hormone on mtRNA transcription
rate, a fine analysis of the synthesis of discrete RNA
species
revealed that T
3 also promoted a remarkable change in
the
relative synthesis of mRNAs with respect to rRNAs (Fig.
1B
and C).
Thus, when the relative labeling of several mRNAs was
compared with
the labeling of the RNAs (calculated as the radioactivity
incorporated into mature 16S rRNA plus the radioactivity incorporated
into the rRNA precursor that includes 16S rRNA), an average
~1.6-fold
reduction in the mRNA/rRNA ratio in hypothyroid
mitochondria was
observed (Fig.
1B, lane 2; Fig.
1C). This
reduction was reversed
almost completely by in vivo treatment of the
hypothyroid rats
with the hormone (Fig.
1B, lane 3; Fig.
1C). Moreover,
hyperthyroid
organelles showed a ~1.9-fold increase in the
mRNA/rRNA ratio
relative to the control. Interestingly, the
decrease in the mRNA/rRNA
ratio was even higher when mitochondria
from rats treated for
2 months with PTU were assayed (Fig.
1B, lane 5),
and the modification
of the mRNA/rRNA ratio was again partially
recovered by 2 days
of in vivo treatment of the animals with
thyroid hormones (Fig.
1B, lane 6; Fig.
1C). It should be
mentioned that fractionation
of in vivo- and in organello-synthesized
mtRNAs by oligo(dT)-cellulose
columns allowed us to determine that the
ratio of 12S to 16S rRNA
was not affected by the thyroid status of the
animals (not
shown).
The differences in accumulation of RNA by isolated organelles
could be due either to modifications of the transcriptional
activity or
to alterations of the RNA stability. To distinguish
between these
two alternatives, we performed pulse-chase experiments
and
estimated the overall decay and half-lives of RNA synthesized
by
isolated organelles from euthyroid and hypothyroid rats. Thus,
overall
half-lives of 64.23 ± 7.23 and 136.9 ± 14.27 min (mean
± standard deviation) found for the RNA synthesized by euthyroid
and
hypothyroid organelles, respectively (Fig.
2). Therefore,
since the stability of the
RNA is increased in hypothyroid organelles,
the reduced accumulation of
labeled RNA in hypothyroid mitochondria
must be a consequence of
differences in the rate of RNA synthesis.
Pulse-chase experiments also
allowed estimation of stability for
the different species of RNA.
Figure
2 shows that after short
periods of chase, the radioactivity
incorporated in several of
the discrete RNA bands increases due to the
transformation of
previously labeled nascent chains into mature RNAs
(
9). This
is more evident with euthyroid (Fig.
2A, left)
than with hypothyroid
(Fig.
2A, right) organelles, possibly because of
the lower transcription
activity in hypothyroid mitochondria. In
contrast, after longer
periods of chase, the labeling of all RNA
species synthesized
during the pulse by both types of mitochondria
decreases progressively,
allowing determination of their stability
(Fig.
2B). Interestingly,
we found that the half-lives of the mRNAs
and rRNAs were increased
(1.65- and 2.48-fold, respectively) in
hypothyroid mitochondria.
Therefore, the alteration in the
mRNA/rRNA ratio promoted by thyroid
hormone is due to differences
in their relative transcriptional
rates rather than a consequence of
posttranscriptional regulation
phenomena. In summary, these results
confirm that thyroid hormone
promotes differences both in the overall
transcriptional rate
of mtDNA and in the relative transcriptional rate
of the rRNA
and mRNA genes.
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FIG. 2.
Influence of thyroid status on the stability of the RNAs
synthesized by isolated mitochondria. (A) Pulse-chase experiment of in
organello RNA synthesis with mitochondria isolated from euthyroid and
hypothyroid animals. Pulse (P) was 2 h of incubation in the
presence of [-32P]UTP, after which the mitochondria
were pelleted, washed and resuspended in fresh medium with excess of
unlabeled UTP, and incubated for the indicated chase periods. Bands are
labeled as in Fig. 1. (B) Half-lives (mean ± standard deviation),
in minutes, for total RNA (overall) or different mtRNA species
calculated from the pulse-chase experiments. Ratio is
hypothyroid/euthyroid value.
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In vitro addition of thyroid hormone to isolated hypothyroid
mitochondria restores the normal mRNA/rRNA proportion.
To
investigate if the influence of thyroid hormones on mtDNA transcription
could be exerted directly on mitochondria, in organello RNA synthesis
was carried out with rat liver mitochondria isolated from 1-month
hypothyroid rats incubated in the presence of different concentrations
of added hormone. As shown in Fig. 3A, addition of increasing
concentrations of T3 to the incubation medium did not
significantly influence the overall transcriptional rate of mitochondria. However, the hormone strikingly modified the ratio of
mRNA/rRNA synthesized by isolated organelles. In agreement with the
in vivo hormone effect described above, T3 addition
preferentially favored mRNA labeling, increasing the mRNA/rRNA
ratio (Fig. 3A and C). This effect was
revealed at a very low concentration of T3 (10 pg/ml),
reaching a plateau at 50 pg/ml, where the increase of the mRNA/rRNA
ratio was 1.8- to 2.0-fold (Fig. 3A and C). Similar results were
obtained in three independent experiments (Fig. 3C). Furthermore, when
2-month hypothyroid mitochondria were assayed, a similar increase in
the mRNA/rRNA ratio induced by a very low concentration of
T3 (10 pg/ml) was again observed (Fig. 3B, lanes 5 and 6).
Very interestingly, reverse-T3 (rT3), a much
less active analog of T3, was unable to induce any effect
on the mRNA/rRNA ratio in the same organelles, even at a 10-fold
higher concentration (100 pg/ml). Only when rT3 was added
at 500 pg/ml was it able to mimic the effect on the mRNA/rRNA ratio
produced by T3 (Fig. 3B, lane 4). It should be noted that
the in vitro addition of T3 to hypothyroid mitochondria
produced an increase in the mRNA/rRNA ratio quantitatively
identical to that observed in hypothyroid animals treated with thyroid
hormones (Fig. 3C).
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FIG. 3.
Effect of thyroid hormone addition to the incubation
medium on in organello mtRNA synthesis. (A and B) Electrophoretic
patterns of the in organello-synthesized RNA by isolated mitochondria
from hypothyroid rat liver (1-month treatment) incubated in the
presence of the indicated T3 concentrations (A) and from
hypothyroid rat liver (2-month treatment) incubated in the presence of
the indicated concentration of rT3 (lanes 1 to 4) or
T3 (lanes 5 and 6) (B). Amounts of RNA synthesized by an
equal fraction of mitochondria were loaded per lane in each gel. (C)
Comparison of the in vivo effect of T3 and in vitro
addition effect of T3 or rT3 on the in
organello mRNA/rRNA synthesis ratio. Left, average change in the
mRNA/rRNA ratio after addition of T3 in three
independent experiments ( ,  ,  ) or rT3 ( ) to the
incubation medium. The differences in the mRNA/rRNA ratio at any
concentration of T3 added to the incubation medium compared
with no T3 were significant (P < 0.001) by
Student's t test. The difference in mRNA/rRNA ratio at
500 pg of rT3 per ml compared with no addition was
significant (P < 0.01) by Student's t
test. Right, effect of the in vivo treatment of hypothyroid animals
with T3 on the mRNA/rRNA ratio. The difference was
significant (P < 0.01) by Student's t
test. Data are expressed as the mean ± standard error of the mean
of the proportion of radioactivity incorporated in the bands for the
mRNAs ND5, COI plus ND4/L, Cyt b, and COIII plus A6/8 (see the
legend to Fig. 1 for definitions) with respect to the radioactivity
incorporated into the band corresponding to the mature 16S rRNA plus
the corresponding fraction of 16S rRNA contained in the p-rRNAs band.
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|
The footprinting pattern of the transcription regulatory region of
mtDNA is predetermined in vivo by thyroid hormone.
Regulation of
the mRNA/rRNA ratio by thyroid hormone could be exerted by
selective modulation of the H-strand transcription initiation at
IH1 or IH2 (3, 30, 31). Therefore,
we first investigated if thyroid hormone modifies the protein-DNA
interactions in the transcription initiation area in a way that could
be detected by methylation interference analysis. Figures
4 and 5
show the methylation patterns of the L and H strands in the area where the transcription promoters for both strands are located. By comparing the in organello mtDNA methylation patterns of euthyroid (Fig. 4, lanes
E) and hypothyroid (lanes H) animals with those generated
by DMS treatment of deproteinized (naked) mtDNA (lanes C), one can
identify several regions of altered methylation reactivity. In
particular, the nucleotides located around the transcription start
sites for the L strand (for IL, nucleotide [nt] 16178)
and the H strand (for IH1, nt 16283; for IH2,
nt 66) show clear protections and hypermethylations (Fig. 4 and 5A).
Additional alterations are concentrated in the regions spanning nt
16197 to 16215 and nt 16252 to 16271 (Fig. 4 and 5A), which correspond
to the binding sites of the mitochondrial transcription activator mtTFA
(5, 13). Finally, it was possible to observe some
methylation alterations in the regions spanning nt 16211 to 16252, between the IL and IH1 promoters, and in the
region spanning nt 22 to 41, between the IH1 and
IH2 transcription initiation sites (Fig. 4 and 5A).
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FIG. 4.
Effect of the in vivo thyroid status on the footprinting
pattern at the mtDNA transcription initiation region. Comparison
between euthyroid and hypothyroid mitochondria of the in
organello footprinting patterns of mtDNA H strand (A) and L strand (B)
in the region containing the transcription initiation sites. C, naked
mtDNA treated in vitro with DMS; E, in organello DMS-treated mtDNA from
euthyroid animals; H, in organello DMS-treated mtDNA from
hypothyroid animals. Hypermethylated bands are represented by open
squares for euthyroid and open circles for hypothyroid samples;
protected bands are represented by closed squares for euthyroid and
closed circles for hypothyroid samples. Gray boxes indicate the
proposed mtTFA binding sites. IL, IH1,
IH2, transcription initiation sites at the L and the H
strands (IL and IH1 according to reference
5; IH2 by analogy with human DNA
[29]).
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FIG. 5.
Summary and details of the methylation interference
sites from hypothyroid (circles) and euthyroid (squares) mitochondria
in the mtDNA transcription initiation region. (A) Sequence of the
DMS-sensitive positions within the D-loop region containing the
transcription initiation sites. The mtTFA binding areas and the
transcription initiation sites (IL, IH1, and
IH2) are shown. (B and C) Comparison of densitometric
tracings from footprinting analysis, between hypothyroid (bottom) and
euthyroid (middle) mitochondria, at the template strand of the H-strand
initiation sites IH1 (B) and IH2 (C). A summary
of the changes is shown above each panel on the sequence containing
each initiation site. IO, in organello DMS-treated mtDNA; other symbols
are as described in the legend to Fig. 4.
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In summary, most of the protection or hypermethylation phenomena
described above appear to occur at positions of known protein-DNA
interactions (mtTFA) or at potential sites of similar interactions
(RNA
polymerase or transcription factor[s]) at or near the positions
of RNA synthesis initiation. There is a reasonable correspondence
between the mtDNA regions exhibiting methylation alterations shown
in
Fig.
4 and
5 with those found previously in rat liver (
5),
bovine brain (
19), and human mtDNA (
20,
29).
Comparison of the footprinting patterns of euthyroid and hypothyroid
mitochondria revealed clear differences (Fig.
4 and
5A).
In particular,
the areas surrounding the I
L, I
H1, and
I
H2 transcription
start sites showed the most conspicuous
differences between hypothyroid
and euthyroid mtDNA. Remarkably, they
mostly affected the template
strand for each start site, the L strand
for I
L (Fig.
4A, left
panel) and the H strand for
I
H1 (Fig.
4B, central panel; Fig.
5B) and I
H2
(Fig.
4B, right panel; Fig.
5C). In addition, some
differences were
also evident on both strands in the binding regions
of the
transcription factor mtTFA. Those mainly consisted in the
weakening or
loss of the footprinting signal for the mtTFA binding
site close to
I
L in the hypothyroid sample (Fig.
4, left panels).
The
changes in the mtTFA binding site near the H-strand rRNA initiation
site (I
H1) were more complex, showing new nucleotides with
methylation
interference (i.e., nt 16255, 16259, and 16265 [Fig.
4B,
central
panel]) and reversion of the methylation status in other
positions
(i.e., nt 16256 and 16264 [Fig.
4B, central panel])
in the hypothyroid
sample. These differences suggest either an
alteration of the
DNA-protein interactions or a structural change in
mtDNA at the
transcription promoter area determined by the in vivo
thyroid
state that could be responsible for the changes in the
transcription
activity described
above.
In vitro addition of thyroid hormone to isolated hypothyroid
mitochondria restores the euthyroid footprinting patterns of the
transcription regulatory region of mtDNA.
Since the in vitro
addition of the hormone was able to modify the transcription activity
of the organelles, we next analyzed whether this addition would also
affect the footprinting patterns of hypothyroid mitochondria in a way
that could be correlated with the transcription changes. For this, we
performed methylation interference experiments with hypothyroid
mitochondria in the presence of different concentrations of thyroid
hormone. We observed that the addition of increasing amounts of
T3 modified the footprinting pattern of the transcription
initiation areas such that it becomes progressively more similar to
that obtained from euthyroid organelles (Fig.
6, lanes 10 and 50). This is clearly
indicated by the intensification of the footprinting signal on both
strands at the mtTFA binding site close to IL (Fig. 6, left
panels). Furthermore, the euthyroid-like methylation status of the
mtTFA binding site near IH1 is also recovered with the
addition of increasing concentrations of the hormone (e.g., nt 16255, 16256, 16263, and 16264; Fig. 6B, central panel). Remarkably, the DMS
sensitivity at the L-strand and the two H-strand transcription
initiation sites was strongly modified by T3 addition to
the incubation medium, and again the euthyroid-like methylation pattern
was reached at 50 pg of T3 per ml (Fig. 6, lanes 50).
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|
FIG. 6.
Effect of in vitro thyroid hormone addition to
organelles isolated from hypothyroid animals on the footprinting
patterns of mtDNA at the transcription initiation region. Shown is
comparison of the mtDNA DMS reactivity, at the L strand (A) and H
strand (B), between euthyroid (E) and hypothyroid mitochondria
incubated without (H) or with the indicated
T3 concentration (10 or 50 pg/ml). For the naked DNA
methylation pattern, see Fig. 4. Symbols are as described in the legend
to Fig. 4.
|
|
The more interesting changes induced by T
3 were observed at
the two putative H-strand transcription initiation sites
(I
H1 and I
H2), because of their proposed role
in the regulation of
mRNA and rRNA synthesis (
31). Those
changes affected only nucleotides
on the template strand (Fig.
6B,
central and right panels; Fig.
7). A
similar phenomenon can be observed at the L-strand promoter
(Fig.
6A,
left panel). In particular, at the I
H1 site, nt
T16287,
G16288,
T16291,
G16292,
T16293, and
G16294 recovered
the
euthyroid methylation status when hypothyroid organelles were
incubated
in the presence of 50 pg of T
3 per ml (Fig.
7A and C).
Similarly, at the I
H2 site, nt A57, G58, T65, G66, and T67
recovered
the euthyroid methylation status after incubation with
thyroid
hormone (Fig.
7B and D). However, recovery of the euthyroid
footprinting
pattern at the I
H1 and I
H2 sites
was not complete. Thus, at the
I
H1 site, nt
A16284 and
G16285 were hypermethylated in the
presence of 50 pg of T
3
per ml and unmodified in the euthyroid
patterns, and nt
A16290 was
unmodified in the presence of 50
pg of T
3 per ml and
protected in the euthyroid patterns (Fig.
7A and C). On the other hand,
at the I
H2 site, nt T55, T56, and
T64 were protected in the
euthyroid patterns and unmodified after
incubation of hypothyroid
mitochondria with the hormone (Fig.
7B and D). It should be mentioned
that only at the I
H2 site were
methylation patterns of the
H-strand naked euthyroid and hypothyroid
mtDNAs not identical. Thus, nt
G68 showed a clear methylation
in the hypothyroid naked mtDNA patterns
but only a faint methylation
in its euthyroid naked mtDNA counterpart
(Fig.
4B, right panel).
This observation was consistent between
different independent
experiments, but its significance is unclear.
Nevertheless, the
changes in the methylation sensitivity of each
nucleotide with
respect to the naked control DNA can still be clearly
detected.
In summary, the addition of T
3 to the incubation
medium of hypothyroid
mitochondria modifies the footprinting patterns
of the transcription
regulatory regions of mtDNA, substantially
restoring the patterns
observed in euthyroid mitochondria.
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|
FIG. 7.
Summary of the influence of in vitro T3
addition on the methylation reactivity at the two H-strand
transcription initiation sites. Shown are densitometric tracings of the
mtDNA footprinting patterns from Fig. 6 at the template strand of the
IH1 (A and C) and IH2 (B and D) transcription
initiation sites. (A and B) Changes in the methylation reactivity of
mtDNA from hypothyroid organelles incubated without (IO [in organello
DMS-treated] H mtDNA) or with the indicated
concentrations of T3 (10 and 50 pg/ml). (C and D)
Densitometric tracings showing the methylation reactivity of
hypothyroid mtDNA incubated in the presence of T3 (50 pg/ml) at the IH1 (C) and IH2 (D) areas.
Comparison with the methylation reactivity of euthyroid mtDNA (open and
closed squares) is shown above each panel on the sequence containing
each initiation site.
|
|
The footprinting pattern of the transcription termination region of
mtDNA is not influenced by the in vivo thyroid status or by the in
vitro addition of thyroid hormone to hypothyroid mitochondria.
Another potential mechanism to regulate the mRNA/rRNA ratio could
be by influencing mTERF-dependent transcription termination. The
function of mTERF requires its specific binding to an mtDNA motif at
the boundary between the rRNA and mRNA genes (6, 12, 21,
25). Therefore, we also analyzed the footprinting pattern of the
mtDNA area containing the mTERF binding site in organelles isolated
from euthyroid and hypothyroid animals, in the latter case with and
without the addition of T3 to the incubation medium (Fig.
8). We observed a strong modification in
methylation reactivity with respect to naked DNA (Fig. 8, lanes C) in
the in organello DMS-treated samples, regardless of their in vivo
thyroid status (lanes E and H). Nucleotides on both
strands were clearly affected in a way very similar to that described
previously (5). However, no significant differences between
hypothyroid and euthyroid samples were observed (Fig. 8). Moreover,
when thyroid hormone was added to the incubation medium of hypothyroid
mitochondria, no changes in the methylation reactivity at the mTERF
binding site could be detected (lanes 10 and 50). Therefore, we
conclude that thyroid hormone does not affect the binding of mTERF to
mtDNA.
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FIG. 8.
Effect of in vivo thyroid status and in vitro
T3 addition on the footprinting pattern of mtDNA at the
transcription termination region. Shown are in organello footprinting
patterns of rat mtDNA transcription termination areas at the L and H
strands. In the sequence summary at the bottom, the gray box indicates
the tridecamer sequence where mTERF binds. Symbols are as described in
the legend to Fig. 6.
|
|
The footprinting pattern of a putative TRE in the mtDNA D-loop
region reveals no detectable protein-DNA interactions.
Wrutniack
and coworkers (48) have described a mitochondrial matrix
43-kDa protein able to bind T3 and canonical TREs as well
as a specific sequence in the rat mtDNA D-loop area near the
transcription promoters; this observation was obtained by gel mobility
retardation assays. To verify its potential role as a cis
element that might mediate the action of thyroid hormone on
mitochondrial transcription, we investigated the existence of
protein-DNA interactions at this location. We performed
footprinting analysis on a 300-bp area (from nt 15768 to 16086),
which includes the full oligonucleotide used by Wrutniack et al.
(48) in their band shift assays and also includes the
conserved sequence block I, a region known to interact with proteins
(5). In agreement with previous descriptions (5),
we found conspicuous alteration of DMS reactivity at and downstream of
the conserved sequence block I region (nt 16001 to 16057) that was not
affected by the in vivo thyroid status or by the in vitro addition of
the hormone to the incubation medium of hypothyroid mitochondria (data
not shown). In contrast, no differences in DMS reactivity between naked
mtDNA (Fig. 9, lanes C) and in organello
mtDNA (lanes E and H) were observed within the area
containing the proposed TRE (nt 15923 to 15949). We could find only one
hypermethylated band, at position 15960 on the H strand, downstream of
the proposed TRE-containing region. Moreover, the in vivo thyroid
status as well as the in vitro addition of the hormone to the isolated
organelles did not affect the mtDNA DMS reactivity properties in this
area (Fig. 9).
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FIG. 9.
In organello footprinting pattern (top) and sequence
summary (bottom) of rat mtDNA in the D-loop area proposed to contain
the TRE. The gray box indicates the location of the putative TRE (DR2).
Symbols are as described in the legend to Fig. 6.
|
|
| |
DISCUSSION |
Our results have allowed a deeper understanding of the influence
of thyroid hormone on the expression of mtDNA. (i) We have confirmed
that T3 exerts in vivo a double effect on mitochondrial transcription: an increase in the overall transcriptional rate, and a
differential modulation of the relative mRNA/rRNA transcriptional rate. (ii) Part of this influence, i.e., the change in ratio of mRNA to rRNA synthesis, is exerted directly on mitochondria,
without previous modulation of nuclear gene expression, and it is
probably achieved by selection of transcription initiation at
alternative sites on the H strand.
The observation of a double effect of T3 on mtDNA
transcription is fully in agreement with previous reports from
different groups that showed a 1.4-fold (2) or 3- to 7-fold
(32) increase in transcription activity between rat liver
mitochondria isolated from hypothyroid rats and hypothyroid animals
treated in vivo with T3. Likewise, a ~2-fold decrease in
the in vitro activity of RNA polymerase partially purified from
hypothyroid rat liver mitochondria compared with control mitochondria
was also reported (17). Furthermore, our results are also in
agreement with previous reports showing a decrease in the mRNA/rRNA
ratio of the in vivo steady-state levels of rat liver mtRNAs in
hypothyroid versus euthyroid mitochondria. This effect was mainly due
to a decrease in the mRNA levels since rRNA levels were not
(17, 32) or were only slightly (44) affected.
Thus, variations of ~1.75-fold (17), 2- to 7-fold
(32), or 1.5- to 2-fold (44) in the mRNA/rRNA ratio were observed. Although these observations strongly suggested a
regulatory action of thyroid hormone on mtDNA transcription, the lack
of experimental data on direct measurement of the transcriptional rate
and on stability of the different mitochondrial transcripts prevented a
definitive conclusion. The reproduction in our in organello
transcription system of the effects observed in vivo confirms the
suitability of this experimental approach to investigate the action of
thyroid hormone on mtDNA transcription. Moreover, the maintenance of in
vivo-like conditions for mtDNA transcription, the analysis of the RNA
synthesized de novo under controlled conditions, and, in parallel, the
possibility of footprinting specific mtDNA areas while transcription is
in progress allowed us to obtain an integrated picture of the action of
thyroid hormone on mitochondrial transcription.
Thus, we have demonstrated that the thyroid status affects the
stability of all mtRNAs, being on average twofold more stable in
hypothyroid than in control organelles. The increase in mtRNA stability
probably reflects a general mechanism operating in mitochondria when
transcription is depressed, rather than a specific regulatory action of
thyroid hormone. In fact, an increase in the stability of mtRNAs
induced after inhibiting mitochondrial transcription has been described
previously for cultured cells (8). If the stability of the
RNAs is taken into consideration, the decrease in the rate of RNA
synthesis observed in hypothyroid mitochondria is greater than that
indicated by the incorporation of [-32P]UTP into RNA
(2.34-fold versus 1.85-fold). In addition, the reduction in the
mRNA/rRNA ratio observed in hypothyroid mitochondria must be a
consequence of the alteration in the relative rate of synthesis
of both types of RNA, since the increase in stability of the
mRNAs is slightly (1.5-fold) higher than that of the rRNAs.
Besides the effects on transcription, we have also found that the
footprinting patterns at the regions of mtDNA that contain the
transcription start sites of both strands are predetermined in vivo by
thyroid hormone. This observation strongly suggests that the
interaction of the proteins involved in the initiation of transcription
with mtDNA is influenced by the hormone levels. In contrast, the in
vivo thyroid status does not affect the interaction of mTERF with
mtDNA. It should be remarked that thyroid hormone particularly affects
the footprinting patterns at the template strand on the L-strand and
the two H-strand transcription initiation sites. Therefore, in light of
these results, the observed changes in the relative synthesis of
mRNA and rRNA are more likely due to the influence of
T3 on the selection of the H-strand initiation sites than
to transcription termination at the mTERF binding site.
In summary, our results confirm that transcriptional control is the
main mechanism underlying the thyroid hormone effect on mtRNA
steady-state levels. However, the in vivo experiments discussed above
do not allow discrimination between nucleus-dependent or direct
regulation of mtDNA transcription by the hormone.
In the nucleus, thyroid hormone stimulates transcription through its
interaction with receptors that recognize TREs located in the
regulatory region of target genes. In mitochondria, two alternative
models of action of thyroid hormone have been proposed. On one side,
T3 could activate mitochondrial transcription by an
indirect mechanism, the previous activation of mtTFA synthesis (46). In support of this, it has been reported that in
hyperthyroid rats the level of the mtTFA mRNA in liver increases in
parallel with mtDNA-encoded transcripts (18), and a putative
TRE has been found in the promoter region of the mtTFA gene
(18). However, the recent development of mtTFA knockout mice
shows that there is not a direct correlation between the amount of
mtTFA and the steady-state levels of mtRNA (26). On the
other hand, a direct action of the hormone through mitochondrial
receptors that would be able to interact with TREs present at the
regulatory region of mtDNA has been proposed (1, 7, 48).
This model is supported by recent reports describing c-Erb-related
proteins in rat liver mitochondria (1, 48). Particularly, a
43-kDa protein, immunologically related to c-ErbA1, which is able to
bind specifically and with high affinity to T3 and
canonical TREs, has been found in the mitochondrial matrix. Very
interestingly, this protein is able to show specific binding, in gel
mobility shift assays, to sequences contained in the regulatory region
of rat mtDNA (48).
Two lines of evidence indicate that T3 directly influences
mtDNA transcription. First, our analysis shows that the modification of
the mRNA/rRNA ratio induced in vivo by T3 can be fully
reproduced by the direct addition of the hormone to isolated
hypothyroid mitochondria. In agreement with this, we also found that
the normal DMS interference methylation patterns in the regulatory
region of initiation of mtDNA transcription, predetermined in vivo by thyroid hormone, can be substantially reestablished by in vitro addition of the hormone to isolated hypothyroid mitochondria.
The very low amount of hormone that is needed to promote the change in
the mRNA/rRNA ratio (10 pg/ml), plus the fact that it is a
saturable effect, strongly suggests that this phenomenon can be
mediated by a high-affinity T3 receptor present in limited amount in the mitochondria. The specificity of the in vitro action of
T3 was tested by monitoring the ability of rT3
to promote the same effect in the relative synthesis of mRNA versus
rRNA. It is known that rT3 is able to bind nuclear
c-ErbA-type T3 receptors but with a ~100-fold-lower
affinity than T3 (39). However, while the
affinity of the receptor for different T3 analogues may
vary, the occupancy of the ligand-binding domain by iodothyronine or similar ligands will mimic the T3 effect (4). If
a c-ErbA-like receptor is somehow involved in the observed effect of
T3 on in organello transcription, then this effect would be
mimicked by rT3 but only at a clearly higher
concentration. In agreement with this, a change of the
mRNA/rRNA ratio qualitatively similar to that produced by 10 pg
of T3 per ml was observed only when rT3 was
added at 500 pg/ml. This observation could support the existence of
c-ErbA-related proteins in rat liver mitochondria as proposed elsewhere
(1, 48).
Wrutniak et al. (48) have also found a direct repeat
sequence (DR2) within the regulatory region of mtDNA (nt 15923 to
15949) that was proposed as a potential TRE. They have shown that an oligonucleotide containing this sequence is specifically bound by the
mitochondrial c-ErbA-related protein (48). We could not verify by DMS methylation interference experiments if the proposed mtDNA TRE was in fact interacting with proteins in functional isolated
mitochondria. However, while T3 was able to induce
detectable alterations at the binding site of other transcription
factors, the absence of DMS reactivity changes at well-characterized
TREs on the regulatory region of nuclear genes seems to be a common phenomenon (24). Therefore, on the grounds of the absence of DMS methylation reactivity, we cannot rule out the role of the proposed
region of the mtDNA as a true TRE.
Concerning the mechanism by which the relative synthesis of mRNA
and rRNA could be affected in mitochondria, differential regulation of
the two H-strand initiation sites by T3 seems to us the
more plausible explanation. Footprinting analysis reveals that the
protein-DNA interactions at the mtTFA binding sites as well as at the
transcription start sites are remarkably different in hypothyroid and
euthyroid mtDNAs. In parallel, the mRNA/rRNA ratio as well the
overall transcriptional rate are modified. The in vitro presence of the
hormone is sufficient to recover the way in which transcription
factor(s) interact with the mtDNA in euthyroid organelles. The changes
in the DMS reactivity induced in vitro by T3 were not
accompanied by alterations of the transcriptional activity as a whole
but correlated with a reduction in the synthesis of rRNAs in favor of
the mRNAs. Thus, the differential accessibility of transcription
initiation factor(s) and likely the RNA polymerase to mtDNA, induced by
T3, would enhance the election of IH2 as the
transcription initiation site for the H strand. Interestingly, this
behavior substantially resembles what has been described for the
influence of T3 on the regulatory region of the nucleus encoded growth hormone gene. There, the presence of T3 does
not seem to be required for, but facilitates, the binding of other transcription factors, such as Sp-1 or Pit-1, to the DNA
(24). The alternative explanation for the modulation of the
mRNA/rRNA ratio, that is, regulation of the transcription
termination of the smaller H-strand-derived polycistron, seems
unlikely, because the binding activity of the factor responsible for
the termination of transcription (mTERF) remains unaltered between
different thyroid statuses and after the in vitro addition of the hormone.
Finally, the fact that the in vitro addition of T3 to the
incubation medium was unable to increase the overall transcriptional rate in isolated mitochondria suggests that this effect, promoted in
vivo by the hormone, is probably mediated by an indirect mechanism that
can involve modulation of nuclear gene expression. As a consequence, the mt-mRNA/rRNA ratio is increased in organello, to the detriment of the synthesis of rRNAs (Fig. 3A and B). Interestingly, when the
effect on the mRNA/rRNA ratio is combined with the stimulation in
the overall transcription observed after in vivo treatment with the
hormones, a net accumulation of mt-mRNAs should be expected (1.6- to 2.3-fold), while the steady-state level of the rRNAs should remain
constant or increase only slightly. This is, in fact, what has been
described by several groups (17, 32, 44).
In conclusion, the results presented in this report are the first
functional demonstration of a direct influence of hormones, particularly thyroid hormone, on the expression of mtDNA. This evidence
is fundamental not only for a better understanding of the genetic
regulation of the energetic metabolism by thyroid hormone but also to
prove the existence of non-nucleus-mediated regulators of mammalian
mtDNA transcription (9) and understand the signaling
pathways that coordinate gene expression between the mitochondrial and
nuclear compartments (40).
| |
ACKNOWLEDGMENTS |
We are very grateful to F. Martínez-Azorín for
valuable comments and discussion and to Santiago Morales for excellent
technical assistance.
This work was supported by grants from the Spanish Dirección
General de Investigación Científica y Técnica
(PB94-0567 and PB97-1019) and from the Zaragoza City Council.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Departamento de
Bioquímica y Biología Molecular y Celular, Universidad
de Zaragoza, Miguel Servet 177, E-50013 Zaragoza, Spain. Phone for
José A. Enríquez: 34-976761646. Phone for Julio Montoya:
34-976761640. Fax: 34-976761612. E-mail for José A. Enríquez: enriquez{at}posta.unizar.es. E-mail for
Julio Montoya: jmontoya{at}posta.unizar.es.
| |
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Molecular and Cellular Biology, January 1999, p. 657-670, Vol. 19, No. 1
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Copyright © 1999, American Society for Microbiology. All rights reserved.
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Abstract
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