From the Department of Pathology and Laboratory Medicine, University of Texas Medical School, Houston, Texas 77030
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ABSTRACT |
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Activation of cytochrome c (cyt c) transcription in electrically stimulated neonatal rat cardiac myocytes is preceded by transient expression of the activating protein-1 family of transcription factors, c-Fos, c-Jun, and JunB, as well as nuclear respiratory factor-1 (NRF-1). Mutations in either the NRF-1 or in the two cyclic AMP response elements on the cyt c promoter significantly reduce cyt c promoter activation produced either by electrical stimulation (Xia, Y., Buja, L. M., Scarpulla, R. C., and McMillin, J. B. (1997) Proc. Natl. Acad. Sci. U. S. A. 94, 11399-11404) or by transfection of c-jun into nonpaced cardiac myocytes. Electrical stimulation of cardiac myocytes activates the c-Jun N-terminal kinase (McDonough, P. M., Hanford, D. S., Sprenkle, A. B., Mellon, N. R., and Glembotski, C. C. (1997) J. Biol. Chem. 272, 24046-24053) so that the fold-activation of the cyt c promoter is increased by pacing when either c-jun or c-fos/c-jun were cotransfected. Physical association of NRF-1 protein with the NRF-1 enhancer element and of c-Jun with the cyclic AMP response element binding sites on the cyt c promoter was demonstrated by gel shift competition assays and by antibody super shifts. This is the first demonstration that induction of NRF-1 and c-Jun by pacing of cardiac myocytes directly mediates cyt c gene expression and mitochondrial proliferation in response to hypertrophic stimuli in the heart.
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INTRODUCTION |
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Hypertrophic growth is a basic mechanism for increasing cell size
in post-mitotic cardiac muscle. Hearts that have been subjected to
hemodynamic stress increase intermediate early gene and contractile protein expression as part of the hypertrophic response. Likewise, in
cardiac myocytes in culture, application of mechanical stimuli produces
increases in the intermediate early genes c-fos,
c-jun and junB (1-4), and re-expression of
-myosin heavy chain, all characteristic of hypertrophic growth (for
review, see Ref. 5). When neonatal rat cardiac myocytes in culture are
paced, both the content and organization of cellular contractile
proteins increase (6). The increased energy demand resulting from
electrical stimulation of cardiac myocytes is associated with increased
mitochondrial number and cytochrome oxidase activity (7). The
proliferation of mitochondria observed with electrical stimulation is
coincidental with increased mRNA content for cytochrome oxidase
subunit Va and cytochrome c (1, 7). Pacing also increases
c-fos,
-myosin heavy chain, and cytochrome c
promoter activities which coincide with the rise in their respective
gene transcripts. These results are consistent with the interpretation
that electrical stimulation of cardiac myocytes produces
transcriptional activation of nuclear-encoded mitochondrial proteins.
Therefore, electrical stimulation provides a model whereby
physiologically meaningful expression of transcription factors specific
to nuclear-encoded mitochondrial target genes in cardiac myocytes can
be identified.
Pacing of cardiac myocytes induces a rise in cytoplasmic calcium, an event which has been demonstrated to activate multiple signaling pathways (8, 9). Atrial natriuretic factor (anf) gene induction by electrical stimulation in neonatal cardiac myocytes is dependent on Ca2+ influx and calmodulin activity (6). Whereas the cAMP response element binding protein (CREB)1 functions as a Ca2+-regulated transcription factor and as a substrate for depolarization-activated Ca2+-calmodulin dependent protein kinases I and II in neuronal cell lines (10), McDonough and Glembotski (6) observed no change in cAMP formation after electrical stimulation of neonatal cardiac myocyte cultures. Ramirez et al. (11) demonstrated that activation of c-Jun N-terminal kinase (JNK) in neonatal rat ventricular myocytes and in adult myosin light chain-2v-Val-12 Ras mice is associated with cardiac hypertrophy. These authors concluded that maintenance of elevated JNK activity is important for development of the hypertrophic state. The latter data, together with observations that JNK is activated by Ca2+ (12, 13) and that transcriptional activation of the cardiac-specific anf promoter occurs by collaborative interactions between JNK, c-Jun, serum response factor and Sp-1 (2), suggest that there is participation of c-Jun in pathways involving Ca2+-activated gene expression and the hypertrophic response.
Recent studies from our laboratory also support a potential regulatory role for activating protein-1 (AP-1) as well as nuclear respiratory factor-1 (NRF-1) in the initiation of mitochondrial proliferation in response to electrical stimulation. The promoters of many nuclear genes encoding respiratory subunits are at least partially dependent on the nuclear respiratory factors, NRF-1 and NRF-2 (reviewed in Ref. 14). These nuclear transcription factors also act on genes that encode key components of mitochondrial transcription and replication suggesting that they may act to coordinate nuclear-mitochondrial interactions (15). Consistent with an important role of NRF-1 in mitochondrial gene activation, mutations in the NRF-1 site of the cyt c promoter inhibited the induction by electrical stimulation by 5-fold (1). Likewise, mutations in the CRE (ATF) sites of the cyt c promoter also significantly reduced the induction of this gene by electrical stimulation (1). Recent findings suggest that the Fos/Jun and ATF/CREB families of transcription factors interact and should be grouped into a superfamily of transcription factors (16). Since both NRF-1 and Fos/Jun mRNAs appear in time just prior to activation of cyt c gene expression, and since AP-1 factors play a central role in mitogenesis (17), we asked whether AP-1 is involved in cyt c gene expression, and whether this involvement is a direct interaction. The results herein describe the transcriptional response of the cyt c promoter to a hypertrophic stimulus in the neonatal cardiac myocyte.
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EXPERIMENTAL PROCEDURES |
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Cell Culture and Electrical Stimulation--
Neonatal (1-3 day
old) cardiac myocytes were isolated and plated in 12-well dishes in
Dulbecco's modified Eagle's medium supplemented with 10% Hyclone
calf serum at a plating density of 4 × 105 cell/21 cm
as described previously by this laboratory (7). After 24 h, the
serum-containing medium was removed, and the cells were washed and
subsequently maintained for 72 h in Dulbecco's modified Eagle's
medium, in the absence of serum, containing 1% bovine serum albumin
(fraction V). The medium was exchanged for fresh serum-free medium at 2 days. After 4 days in culture (24 h + serum, 72 h serum), three
wells containing myocytes were stimulated for 72 h using the
method of Brevet et al. (18) as modified by McDonough and
Glembotski (6). Three additional wells in the dish were maintained in
the same medium as the stimulated cells, but in the absence of
contractile stimulation. During the experimental period, the medium
bathing the control and stimulated cells was changed after 48 h to
fresh Dulbecco's modified Eagle's medium + 1% bovine serum
albumin.
RNA Isolation and Northern Blot Analysis--
RNA was isolated
(Ultraspec RNA isolation system, Biotex Laboratories, Houston, TX)
either at a single time or during sequential experiments (0, 3, 6, 12, and 24 h) from control or electrically stimulated neonatal rat
cardiac myocytes. For Northern blot analysis, 20 µg of total cellular
RNA was electrophoresed in 1% agarose containing 0.6% formaldehyde at
45 V for 3 h. Fractionated RNA was transferred to a Duralon-UV
nylon membrane (Stratagene, La Jolla, CA) by capillary action for
24 h. After blotting, the RNA was cross-linked to the filter by UV
irradiation. Following prehybridization overnight at 42 °C, the blot
was hybridized in the same prehybridization solution containing 1%
dextran sulfate and the labeled cDNA fragment of cyt c
(1). After washing, the blots were visualized by autoradiography following storage at 70 °C for 24 h.
Preparation of NRF-1 Riboprobe and RNase Protection
Assay--
The MNRFIRP plasmid containing the 487-base pair
ClaI-SphI fragment includes coding exon 2 of the
mouse nrf-1 gene in pGEM7Zf. Radiolabeled RNA transcripts
were synthesized from template DNA linearized with Eco0109
as described by the Promega technical manual using Sp-6 RNA polymerase,
ATP, GTP, UTP and [-32P]CTP (0.5 mM each)
in the presence of RNasin and spermidine. After DNase digestion, the
cRNA probes were hybridized to 20 µg of total RNA and then digested
with RNase A (Boehringer Mannheim), and the RNA/RNA hybrid was analyzed
using 3.5% PAGE in the presence of 8 M urea.
Autoradiography was performed as described above for Northern
blots.
Preparation of Plasmids for Transfection--
The plasmid
pRC4Luc/326 containing 1.1 kilobase pairs of the first intron and the
5'-flanking region of rat cyt c was constructed by cloning
the BglII and XhoI fragment from RC4RAT/
326
(Dr. Richard C. Scarpulla, Northwestern University) into the pGL3-Basic
vector. Cloning the BglII and XhoI fragments of
the respective mutant promoters into pGL3-Basic vector generated
plasmids containing the mutated cyt c promoter constructs
(mSp-1, dmCRE, and mNRF-1). The mSp-1-Luc mutation was generated in the
first intron by a +83/+100 deletion and point mutations of +103 and
+104 from CC to ag; the dmCRE was generated by a double mutation in two
CRE sites, respectively:
119/
96, from CTACGTCAC to CTAatTaAt, and
281/
256, from TGACGTCA to TGAatTaA; mNRF-1 was generated by BamHI linker insertion at SphI between
172 and
147. The plasmid pc-Fos (pF100) was constructed by cloning the full
human c-fos cDNA (Dr. Ann-Bin Shyu, the University of
Texas Medical School at Houston) into a pGM-2 vector between
EcoRI and HindIII restriction sites. The plasmid
pc-Jun was constructed by cloning a 2.6-kilobase pair fragment of
c-jun cDNA into the pGM-2 vector between
EcoRI sites. The plasmid pJunB was constructed by cloning
1.2-kilobase pair fragment of JunB cDNA into pGM-2 vector between
EcoRI and SmaI sites. The canonical AP-1 response
element, TRE-Luc, and the neutral core promoter,
56 Fos-Luc, were
generous gifts of Dr. Michael Schneider (Baylor College of
Medicine).
DNA Transfection--
Cardiac myocytes were grown in
serum-containing medium for 24 h; the myocytes were transfected by
the (Ca)3(PO4)2 precipitation method (19). To detect the interrelationship of the early gene products
with subsequent expression of later genes, e.g. cyt
c, 0.1 µg of pc-Fos, 1 µg of pc-Jun, and 1 µg of pJunB
were cotransfected singly or in combination with 2 µg of wild type or
the mutated cyt c promoters. In each case, 2 µg of Rous
sarcoma virus -galactosidase (
-gal) expression plasmid was
cotransfected to monitor transfection efficiency. Six hours after
transfection, the cells were washed twice and maintained in serum-free
medium for another 12 h. Electrical stimulation was initiated and
cell extracts were isolated either at the point when electrical
stimulation began (zero time) or after 6, 12, 24, 48, and 72 h.
The control cells were maintained under the same conditions as the
stimulated cells, only in the absence of electrical stimulation.
Luciferase and
-gal assays were performed (20) and normalized to
protein content (21).
Preparation of cDNA Probes for Electrophoretic Mobility Shift
Assays--
DNA sequences of oligonucleotides used to generate the
cDNA probes and mutated competitors for electrophoretic
mobility shift assays were as follows. CRE-1-cyt c
(281/
256): P1, 5'-GATCCGGAGGGTGACGTCATCCA-3'; P2,
3'-GGCCTCCCACTGCAGTAGGTTCG-5'; CRE-2-cyt c (
119/
96): P1, 5'-GATCCGACATGCGGCTACGTCACGGCGCA-3'; P2,
3'-GCTGTACGCCGATGCAGTGCCGCGTTCG-5'; NRF-1-cyt c
(
172/
147): P1, 5'-GATCCTGCTAGCCCGCATGCGCGCGCACCTTA-3'; P2,
3'-GACGATCGGGCGTACGCGCGCGTGGAATTCG-5'; mCRE-I-cyt c
(
281/
256): P1, 5'-GATCCGGAGGGTGAatAaATCCA-3'; P2,
3'-CCTCCCACTtaTtTAGGTTCG-5'; mCRE-2-cyt c
(
119/
96): P1, 5'-GATCCGACATGCGGCTAatTaACGGCGCA-3'; P2,
3'-GCTGTACGCCGATtaAtTGCCGCGTTCG-5'; mNRF-1-cyt c
(
172/
147): P1,
5'-GATCCTGCTAGCCCGCggatccGCGCGCGCACCTTA-3'; P2,
3-'GACGATCGGGCGcctaggCGCGCGCGTGGAATTCG-5'; Ap1: P1,
5'-GTCGACGTCACTCAGCGCGATCGTGACTCAGCGCGC-3', P2,
3'-TGCAGTGAGTCGCGCTAGCACTGAGTCGCGCGTCG-5'.
Electrophoretic Mobility Shift Assays--
Nuclear extracts were
isolated from control and stimulated cardiac myocytes. Cells were
washed twice with cold phosphate-buffered saline, scraped in 100 µl
of phosphate-buffered saline, put on ice, and centrifuged at 3000 rpm
for 5 min at 4 °C. The pellet was dissolved in buffer containing 10 mM HEPES (pH 7.9), 10 mM KCl, 0.1 mM EDTA, 1.5 mM MgCl2, 0.2% (v/v)
Nonidet P-40, 1 mM dithiothreitol, 0.5 mM
phenylmethylsulfonyl fluoride, put on ice for 5 min, gently vortexed,
and centrifuged at 3000 rpm for 10 min at 4 °C. The pellet was
dissolved in buffer containing 20 mM HEPES (pH 7.9), 420 mM NaCl, 0.1 mM EDTA, 1.5 mM
MgCl2, 25% (v/v) glycerol, 1 mM
dithiothreitol, 0.5 mM phenylmethylsulfonyl fluoride,
gently vortexed while on ice, and centrifuged at 14,000 rpm for 10 min.
The supernatant was stored at 70 °C. Gel mobility shift assays
were performed as follows. 10-20 µg of nuclear extracts were
incubated with 2-5 × 105 cpm of
32P-end-labeled DNA probe in 20 µl of 20 mM
HEPES, pH 7.9, 25 mM KCl, 0.1 mM EDTA, 10%
glycerol, 10 mM MgCl2, 0.2 mM
dithiothreitol, 0.025% Nonidet P-40, 50 µg/ml poly(dI-dC) or poly
(dG-dC), and 50 µg/ml bovine serum albumin. Poly(dI-dC) was used for
assays involving both cyt c CRE and Sp-1 probes; poly(dG-dC)
was used for assays involving the cyt c NRF-1 probe.
DNA-protein complexes were incubated at room temperature for 20 min.
For supershifts with antibodies anti-c-Jun, anti-CREB-1 (Santa Cruz
Biotechology) and anti-NRF-1 (gift of Dr. Richard Scarpulla,
Northwestern University School of Medicine), the complexes were further
incubated under the same conditions for an additional 20 min. The
reaction mixtures were loaded on a 5% low ionic strength
polyacrylamide gel (acrylamide:bisacrylamide, 80:1) containing 45 mM Tris borate, and 1 mM EDTA, and
electrophoresed in 45 mM Tris borate, 1 mM EDTA
at room temperature and 250 V for 2 h. After drying, the gel was
visualized by autoradiography following storage at
70 °C for 6-12
h.
Statistics-- The significance of the changes reported was determined using Student's t test for paired and nonpaired variates. Data are presented as the mean ± S.E.
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RESULTS |
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Overexpression of c-Jun Protein in the Cardiac Myocytes Induces the
mRNA Level of NRF-1 and Cyt c--
Activation of c-fos,
c-jun, and junB in cultured myocytes and in
intact animals precedes the hypertrophic response with up-regulation of
"fetal" cardiac isoforms (1-4, 11). Electrical stimulation of
neonatal cardiac myocytes induces sequential expression of c-Jun,
NRF-1, and cyt c mRNA (1). To answer the question
whether increased levels of c-Jun expression, independent of electrical stimulation, can increase mRNA for either NRF-1 and/or cyt
c, we overexpressed c-Jun by cotransfecting the
c-jun expression vector with -galactosidase in neonatal
cardiac myocytes. The mRNA for NRF-1 began to rise after 3 h
of transfection of c-jun, peaked at 12 h, and declined
to control levels at 24 h. Subsequent to the rise in NRF-1, a
small (67%) but significant induction of cyt c mRNA in
the transfected, unstimulated myocytes was observed at 12 and 24 h
(Fig. 1). These results suggest that
induction of c-jun early gene expression, either by
transfection or by electrical stimulation (1), is important for
subsequent expression of nrf-1. These experiments also raise
the possibility that, in addition to NRF-1, intermediate early genes
may also play a direct role in cyt c gene transcription in
the heart.
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Transactivation of the Cyt c Promoter by Jun Requires both CRE and
NRF-1 Sites--
Mutational analysis has revealed the essential role
of CRE and NRF-1 sites in the cyt c promoter in the response
of cardiac myocytes to electrical stimulation (1). To test the
hypothesis that AP-1 proteins might map to one or both electrical
stimulation response elements of the cyt c promoter
(i.e. CRE and NRF-1), unstimulated cardiac myocytes were
cotransfected with the c-jun expression vector and a
luciferase reporter gene driven by the wild-type or by series mutants
of the cyt c promoter. Negative control experiments were
carried out by transfection of empty vector/-gal alone or with
c-jun, as well as transfection of the neutral core promoter,
56 Fos-Luc/
-gal alone or with c-jun. There was no
inductive response of the reporter gene in either of the negative
control transfections (Fig. 2). The
TRE-Luc/
-gal transfection served as a positive control. The
unstimulated cardiac myocytes demonstrated a slight inductive response
(p < 0.05) with the TRE expression construct alone,
and this response was significantly (p < 0.01)
augmented by cotransfection with c-jun (Fig. 2). Similarly, transfection of cyt c/
-gal alone produced a small but
significant (p < 0.05) augmentation of reporter gene
expression, and this increase was significantly (p < 0.01) enhanced by cotransfection with c-jun (Fig. 2).
Mutation of Sp-1 sites in the cyt c promoter did not alter
transactivation by c-Jun. In contrast, mutation of both CRE sites
reduced c-Jun-dependent promoter transcription by 80%
(p < 0.05, Fig. 2). Mutation of the NRF-1 site in the
cyt c promoter resulted in 57% decrease from reporter gene
activity when myocytes were transfected with c-jun
(p < 0.05, Fig. 2). The dependence of the cyt
c promoter on intact NRF-1 sites in the absence of
electrical stimulation is consistent with up-regulation of NRF-1
mRNA observed with transfection of c-jun (Fig. 1).
Together, these mutations suggest that both CRE and NRF-1, but not
Sp-1, are necessary for full transactivation of the cyt c
promoter by c-Jun.
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AP-1 Proteins Activate the Cyt c Promoter in Cardiac Myocytes in
the Absence of Electrical Stimulation--
Electrical stimulation of
neonatal rat cardiac myocytes produces an early (15 min to 3 h)
increase in c-Fos, c-Jun, and JunB mRNA, with subsequent induction
of cyt c beginning at 12 h (1). To determine whether
the cyt c promoter is a physiological target for c-Fos,
c-Jun and JunB activities in heart, cardiac myocytes were cotransfected
with the cyt c Luc/-gal reporter genes with c-fos, c-jun, and junB expression
vectors (singly or in combination) in the absence of
electrical stimulation (open bars, Fig.
3). Although expressed at low levels, the
cyt c promoter was significantly (p < 0.05) activated
by c-Fos, c-Jun, or JunB alone (5.35-, 5.89-, and 7.05-fold,
respectively; Fig. 3, open bars). The effect of c-fos alone appears to be an amplification of the response
of the cyt c promoter to endogenous levels of c-Jun present
in these cells (1). This interpretation is supported by activation of the TRE promoter construct when it is transfected alone in unstimulated cells (see Fig. 2). When the combinations c-fos + junB and c-jun + junB, were
cotransfected with cyt c/
-gal, cyt c promoter
gene activities were not different when compared with the single
transfection of junB (Fig. 3, open bars).
However, the combination of c-fos/c-jun slightly
(1.5-fold) increased cyt c promoter expression compared with
cotransfection with either c-fos or c-jun alone
(Fig. 3, open bars). This small response may be rate limited
by c-Jun phosphorylation by the low levels of JNK activity present in
unstimulated neonatal cardiac myocytes (2).
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Effects of Electrical Stimulation on Cyt c Promoter Expression-- Pacing specifically activates c-Jun N-terminal kinase so that the combination of pacing and c-jun transfection of cardiac myocytes synergistically stimulates expression of the anf promoter (2). Based on these observations, electrical stimulation should further increase the c-jun enhancement of cyt c promoter expression (Fig. 2) by activation of the c-Jun N-terminal kinase. Effects due to pacing were assessed by taking the ratio of the levels of cyt c promoter expression in the paced, transfected myocytes to the levels in control (nonpaced), transfected cardiac myocytes (Fig. 3). Pacing stimulated cyt c transcription 5.7-fold (Fig. 3, compare filled bars to open bars). The stimulatory effect of pacing on cyt c promoter activation was not further enhanced by cotransfection of junB (ratio = 6.0) or by the combinations of c-fos + junB (ratio = 6.3) and of c-jun + junB (ratio = 5.7) (Fig. 3). Significant increases (p < 0.05) in cyt c promoter activation by electrical stimulation were seen in cardiac myocytes which were cotransfected with c-jun alone (ratio = 8.5) or with c-jun + c-fos (ratio = 8.38) (Fig. 3). These results implicate the AP-1 proteins, c-Fos and c-Jun, in the activation of cyt c transcription as mitochondria proliferate in response to electrical stimulation (7).
Electrical Stimulation Increases the Content of Transcription Factors That Bind to CRE and NRF-1 Sites in the Cyt c Promoter-- Since both CRE and NRF-1 elements are essential for the response of cardiac myocytes to electrical stimulation, transcription factors that bind to these sites should be increased in cells subjected to pacing. Densitometric analysis of gel mobility shift assays were used to estimate the extent to which 32P-end-labeled CRE and NRF-1 elements were shifted in the presence of nuclear extracts from control and paced cardiac myocytes (Fig. 4A). CRE-1 label density increased by 3-fold, CRE-2 increased by 2-fold, and NRF-1 increased by 1.5-fold (Fig. 4A). Confirming that the shifts were a result of a specific interaction between protein factors and the specific enhancer DNA, competition assays were carried out using unlabeled CRE-1, CRE-2, mCRE-1, mCRE-2, and NRF-1, as well as authentic AP-1 oligonucleotide (Fig. 4B). Unlabeled probes specific for each element were effective competitors, whereas the mutated probes were not (Fig. 4B). Unlabeled AP-1 was tested for its ability to compete for extract protein binding to labeled CRE-1 and CRE-2. In each case, the observed shifts of both labeled enhancer oligonucleotides were abolished (Fig. 4B). These results demonstrate that protein factors binding to the CRE sites also bind the AP-1 probe with high affinity, consistent with the suggestion that there is a Jun-dependent transactivation of cyt c.
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Electrical Stimulation Activates Cyt c Transcription by c-Jun Binding to the CRE Sites-- The ability of the AP-1 oligonucleotide to compete with protein associated with the CRE sites on the cyt c promoter suggests that c-Jun might activate CRE by physical association with these sites. To identify the protein associated with CRE, supershifts were performed by using anti-c-Jun (Fig. 5). Anti-c-Jun completely blocked both CRE shifts (Fig. 5, CRE-1 and -2, lanes 3), suggesting that the protein associated with the CRE sites is c-Jun. Conversely, anti-NRF-1 did not interact with CRE-bound protein (Fig. 5, CRE-1 and -2, lanes 4). Parallel experiments were carried out using AP-1 as the consensus probe. Anti-c-Jun, but not anti-NRF-1, produced a supershift with protein bound to the AP-1 oligonucleotide (Fig. 5, AP-1, lanes 3 and 4), confirming that c-Jun was present in the nuclear extracts from the electrically stimulated myocytes. Other control experiments were carried out to confirm the specificity of the anti-c-Jun results. Anti-NRF-1 resulted in a supershift of protein bound to the NRF-1 site but not to the CRE sites (Fig. 5, NRF-1, lanes 3 and 4). In the negative control experiment, neither anti-c-Jun (Fig. 5, Sp-1, lane 3) nor anti-NRF-1 (Fig. 5, Sp-1, lane 4) was able to produce supershifts of protein bound to the Sp-1 probe.
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CREB Is Not a Major Component of the CRE Site-- Depolarization-induced calcium entry in pheochromocytoma cells leads to phosphorylation of CREB, contributing to Ca2+ activated gene transcription (22). Association of c-Jun protein with the CRE site on the cyt c promoter may involve formation of a tertiary complex with CREB, where activation of CREB is mediated through a calcium-dependent pathway (22). Gel shifts were carried out using anti-CREB to detect possible CREB association with the CRE sites on the cyt c promoter (Fig. 6A). While anti-Jun reduced the shift observed with labeled CRE probe, anti-CREB had no effect on the interaction between CRE and nuclear proteins extracted from paced myocytes (Fig. 6, lane 3 versus 4). Anti-NRF-1 had no effect on the shift with labeled CRE (Fig. 6, lane 5). To ensure that the absence of both supershifts and blocking by anti-CREB-1 was not due to an inadequate amount of antibody, larger amounts of anti-CREB (1.5, 2.0, and 3.0 µg) were used to interact with DNA-protein complex. The increased amounts of anti-CRE had no effect on the shifts (Fig. 6B, lanes 2-5).
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DISCUSSION |
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Electrical stimulation of neonatal cardiac myocytes in culture is associated with expression of the immediate early genes, c-fos and c-jun, followed by the appearance of mRNA for the transcription factor, NRF-1. Up-regulation of these transcription factors precedes the transcriptional activation of cyt c in these cells (1). NRF-1 plays a pivotal role in activation of nuclear-encoded mitochondrial gene expression as well as in the coordination of this process with increased mitochondrial DNA synthesis (14, 15). In electrically stimulated cardiac myocytes, both NRF-1 and CRE elements in the cyt c promoter are required for enhanced transcription of the cyt c gene (1). There is ample evidence that AP-1 components, and in particular c-Jun, are essential for hypertrophy and expression of fetal cardiac genes, as well as being involved in the proliferative and differentiation responses of many cell types (5, 23). Mitochondrial proliferation is a necessary component of cell growth, suggesting a potential role for c-Jun in the activation of cyt c transcription. The temporal relationship between c-Jun, JunB, and NRF-1 expression relative to transcriptional activation of cyt c was the first indication that there is a physiologically relevant role for these transcription factors in cyt c expression in heart (1).
The present results provide evidence that there is physical association of NRF-1 with the cyt c promoter. Our data also provide the first demonstration that the protoncogene product, c-Jun, mediates the transcriptional response of cyt c to pacing in neonatal cardiac myocytes. The initial piece of evidence supporting this contention is the dependence of the c-Jun-dependent up-regulation of the cyt c promoter on the presence of intact CRE enhancer elements. The second observation consistent with a role for c-Jun in transcriptional activation of cyt c is the augmentation of the c-Jun response by electrical stimulation. Pacing has been shown to activate the c-Jun N-terminal kinase so that participation of JNK (2) and its substrate, c-Jun, in calcium-activated expression of the anf gene in cardiac myocytes has been proposed. Increased activity of JNK in this setting is consistent with the present finding of a significantly enhanced response of the cyt c promoter when c-jun and c-jun/c-fos are cotransfected concomitant with electrical stimulation. Whereas JunB can act as a "surrogate" of c-Jun in unpaced cardiac myocytes to enhance cyt c promoter activation, cotransfection of junB alone or in combination with either c-fos or c-jun produced no pacing-dependent enhancement of cyt c promoter expression. Phosphorylation of c-Jun by c-Jun kinase is known to increase its transcriptional activity. However, JunB is not phosphorylated by c-Jun N-terminal kinase (24) so that activation of this kinase by electrical stimulation does not enhance the JunB effect on cyt c. The combination of c-jun/junB transfection was also unaltered by electrical stimulation, reflecting the antagonist or neutral effects of JunB under conditions where the formation of c-Jun/JunB dimers is favored (25-27). Finally, evidence of a physical association of c-Jun with the CRE elements of the cyt c promoter was the first direct demonstration that induction of this transcription factor by pacing plays an essential role, along with NRF-1, in the proliferative response of mitochondria to cardiac myocyte hypertrophy. The induction of NRF-1 mRNA by transfection of cells with c-jun has not been previously reported. The time course of this induction relative to activation of c-jun transcription (1) suggests that transcription of nrf-1 may be activated by c-Jun in electrically stimulated cardiac myocytes.
Recent findings suggest that the Fos/Jun and ATF/CREB families of transcription factors interact and should be grouped into a "superfamily" of transcription factors (16). The CRE (ATF) elements (TGACGTA) present in the cyt c promoter are defined as the activating transcription factor binding site or the site for binding of the cAMP response element binding protein (CREB). In neuronal cell lines, activation of L-type voltage-sensitive Ca2+ channels stimulates phosphorylation of CREB contributing to calcium-activated gene transcription through a Ca2+ calmodulin-dependent protein kinase pathway (22). However, neither phosphoinositide hydrolysis or cAMP formation are contributors to gene expression in electrically stimulated neonatal cardiac myocytes (6). The latter observation is consistent with our findings using the cardiac myocyte model developed by McDonough and Glembotski (6), i.e. there is no detectable contribution of CREB to the protein complex associated with the CRE sites in the cyt c promoter. The strong blockade of the CRE shift by anti-Jun suggests that the binding affinity of c-Jun to the CRE binding sites is low compared with binding of the cardiac nuclear protein extracts to authentic AP-1. In the latter case, supershifts are observed with anti-c-Jun. This supershift pattern was also characteristic of anti-NRF-1 when the antibody was used against cardiac nuclear proteins associated with the NRF-1 binding element. This differential effect of antibodies on the binding patterns reflects the finding that Fos/Jun proteins bind to the ATF/CRE sites with a lower affinity than to the AP-1/TRE site (16).
Our data represent the first physiological evidence that the activity of AP-1 proteins, particularly, c-Jun, is essential for cyt c gene expression, contributing to the proliferation of mitochondria during cardiac myocyte cell growth and differentiation (1, 7). Cyt c represents a target gene which plays an important role not only in assuring adequate energy supplies to an actively contracting cardiac myocyte, but is also important to the initiation of apoptosis (28). This situation is particular relevant in heart where compensatory hypertrophy progresses to failure, the latter characterized by programmed cell death (29). It is intriguing that c-Jun and c-Jun N-terminal kinase have been implicated in induction of programmed cell death (30). Although AP-1 is not an integral part of the basic elements involved in cell death, it may be required to initiate expression of limiting components that are required for apoptosis to occur. One of these components which is essential to programmed cell death is cyt c, which activates the cysteine protease, CPP32 (28). The cellular pathway that leads directly to cyt c accumulation in the cytosol has been the subject of recent interest with release of cyt c from the mitochondrial inner membrane proposed as an initiating event (31). Other investigators have measured no change in the difference spectra for cyt c of mitochondria isolated from control and apoptotic cells (32). The latter results suggest that cyt c remains on the mitochondrial inner membrane but is instead inactivated during programmed cell death (32). One could also speculate that, under certain conditions, activation of cyt c gene transcription could enhance myocyte concentrations of cyt c for initiation of apoptosis. Finally, a function for c-Jun N-terminal kinase activation in the apoptotic effect of ceramides has been demonstrated (30). Furthermore, Fas- or ceramide-mediated cell death is inhibited by transfection of Jurkat cells with an inhibitory Jun construct (30). AP-1 may play a role in directing the dual functions of the c-Fos, c-Jun family members to mediate cell proliferation or cell death by activating target genes, e.g. cyt c, which respond to the intracellular milieu by amplification of the appropriate signaling pathways.
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FOOTNOTES |
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* This work was supported in part by National Institutes of Health RO1-HL38863 (to J. B. M.), and by funds from a bridging grant from the University of Texas Medical School at Houston.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.
To whom correspondence should be addressed: Dept. of Pathology and
Laboratory Medicine, The University of Texas Medical School at Houston,
6431 Fannin, Houston, TX 77030. Tel.: 713-500-5335; Fax:
713-500-0730.
1
CRE, cAMP response element; CREB, CRE binding
protein; mCRE, murine CRE; JNK, c-Jun N-terminal kinase; AP-1,
activating protein-1; NRF-1, nuclear respiratory factor-1; mNRF-1,
murine NRF-1; cyt, cytochrome; Luc, luciferase; -gal,
-galactosidase; Sp-1, GC-rich binding protein; TRE, phorbol
12-O-tetradecanoate 13-acetate-responsive element.
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