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Department of Biochemistry and Molecular Biology, St. Louis University Health Sciences Center, St. Louis, Missouri 63104
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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In isolated, perfused adult rat hearts, global ischemia increased the phosphorylation of cAMP response element-binding protein (CREB) relative to control levels, and this phosphorylation was reversed with reperfusion. CREB phosphorylation elicited by 5 min of global ischemia was sensitive to treatments with the calcium-independent phospholipase A2 (iPLA2) inhibitor bromoenol lactone (BEL) and occurred in the absence of increases in myocardial cAMP content. In contrast, CREB phosphorylation elicited by 15 min of global ischemia was likely mediated by elevated cAMP levels. The expression of c-fos, in response to brief myocardial ischemia, was also sensitive to BEL treatment. The induction of iPLA2-mediated CREB phosphorylation was further substantiated by the observations that lysoplasmenylcholine increased both the phosphorylation of CREB and the induction of c-fos expression in the absence and presence of BEL. CREB phosphorylation in both ischemic hearts and lysoplasmenylcholine-perfused hearts was inhibited by pretreatment of hearts with the specific cAMP-dependent protein kinase (PKA) inhibitor H-89. Taken together, these data demonstrate that iPLA2 mediates CREB phosphorylation through a PKA-dependent pathway during brief periods of myocardial ischemia, possibly through the formation of lysophospholipids.
signal transduction; cAMP response element-binding protein; protein kinase A
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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THE CALCIUM-INDEPENDENT PHOSPHOLIPASE A2 (iPLA2) is a predominant phospholipase A2 activity present in myocardium and is selective for arachidonylated plasmalogen substrates (5, 12). Furthermore, iPLA2 is rapidly activated after global ischemia (5). We (21) recently demonstrated the activation of cAMP-dependent protein kinase (PKA) by lysoplasmenylcholine, an enzymic product of iPLA2-mediated hydrolysis of plasmenylcholine. This activation was found to be specific for lysophospholipids containing a choline polar head group. Thus the activation of PKA by iPLA2 catabolites may represent a key signal transduction mechanism for the phosphorylation of cAMP response element-binding protein (CREB) and the induction of nuclear gene expression in response to myocardial ischemia.
Elevation of intracellular cAMP levels can result in either stimulation or repression of specific gene expression, and most of these genes contain one or more cAMP response elements (CREs) (14). The signal transduction of cAMP is through PKA. The regulatory subunit of PKA binds cAMP and releases the active catalytic subunit (4). This subunit phosphorylates the transactivation domain of CREB at serine-133 as well as CRE modulator and several activating transcription factors, which induces the expression of genes containing CREs (19). The CREB proteins are basic leucine zipper transcription factors and are active as either homo- or heterodimers, which bind to the specific consensus sequence TGACGTCA CRE (10).
In cardiac myocytes, CREB has been shown to be expressed and
phosphorylated in response to elevated levels of cAMP (6, 7). Primary embryonic chick heart cultures stimulated with forskolin or isoproterenol resulted in the increased phosphorylation of
CREB protein along with a corresponding increase in CREB mRNA (6). More specifically, the CREB protein is present, but
not phosphorylated, within the nuclei of myocytes isolated from
neonatal rat hearts (7). Nuclear CREB protein was found to
be phosphorylated after stimulation of neonatal myocytes with
isoproterenol or forskolin (7). Furthermore, skeletal
-actin and -myosin gene expression were increased after treatment
with isoproterenol, suggesting that increased CREB phosphorylation
induces nuclear gene expression (7, 8). Finally, CREB
phosphorylation and CREB mRNA expression were identified in end-stage
failing human hearts and in rat hearts subjected to prolonged
-adrenergic treatment (7, 15).
CREB phosphorylation during myocardial ischemia has not been extensively examined. Several protooncogenes (e.g., c-fos and c-jun) containing CREs have been highly expressed during reperfusion of ischemic myocardium (3). Because PKA is activated by lysoplasmenylcholine (21) and iPLA2 is rapidly activated during myocardial ischemia (5, 12), the hypothesis to be tested in the studies herein is that CREB is phosphorylated during myocardial ischemia through an iPLA2-dependent pathway. Accordingly, the present study demonstrates for the first time that CREB is phosphorylated in response to myocardial ischemia and that iPLA2 regulates CREB phosphorylation during brief intervals of ischemia, whereas prolonged ischemia leads to cAMP accumulation, which also regulates CREB phosphorylation.
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Preparation of crude nuclear fractions from Langendorff-perfused rat hearts. Male Sprague-Dawley rats were utilized for preparation of Langendorff-perfused hearts as described previously (2, 5), and the protocol was in accordance with the National Institutes of Health (NIH) Guide for the Care and Use of Laboratory Animals. After the hearts were equilibrated, hearts were subjected to control perfusions, ischemia, or ischemia-reperfusion. In selected experiments, inhibitors such as bromoenol lactose (BEL), H-89, Rp-8-bromo-adenosine 3',5'-cyclic monophosphate (Rp-8-Br-cAMP), or the cAMP analog 8-Br-cAMP (Sigma) were included in perfusion buffers after equilibration before ischemia or perfusions with lipids. In other experiments, selected concentrations of lysoplasmenylcholine (11), lysophosphatidylcholine (Avanti Polar Lipids), or lysoplasmenylethanolamine (11) were included in the perfusion buffer after the initial equilibration period.
After the ventricles were perfused, the ventricles were either freeze-clamped and pulverized or were homogenized in 5 volumes (wt/vol) of homogenization buffer (20 mM HEPES, 2.5 mM MgCl2, 100 µM EDTA, 20 mM-glycerophosphate, 0.05% Triton X-100, 500 µM
dithiothreitol, 100 µM Na3VO4, 4 µg/ml
leupeptin, 1 mM phenylmethylsulfonyl fluoride, and 75 mM NaCl; pH 7.7)
by Polytron. Samples were centrifuged at 10,000 g for 5 min,
the supernatant was decanted, and the pellet was homogenized in 5 volumes (wt/vol) of homogenization buffer supplemented with 1% Triton
X-100 by Teflon homogenizer followed by centrifugation at 15,000 g for 30 min. The resulting supernatant contained the
soluble crude nuclear fraction.
Western blotting. Crude nuclear proteins were quantitated (13) and normalized before Western blot analysis. Anti-CREB (1 µl/ml, rabbit; New England Biolabs), anti-phosphorylated CREB (Serine-133) (1 µl/ml, rabbit; New England Biolabs), and anti-iPLA2 (10 µg/ml, rabbit; Cayman Chemical) were utilized as primary antibodies along with the horseradish peroxidase-conjugated secondary antibody (1:7,000 dilution, goat anti-rabbit horseradish peroxidase; Sigma). Commercially available, positive controls (New England Biolabs) for either CREB or phosphorylated CREB were prepared from cell extracts of human neuroblastoma cells (SK-N-MC cells) that were either untreated or treated, respectively, with fibroblast growth factor, 1-methyl-3-isobutylxanthine, and forskolin. Immunoreactive bands were visualized by chemiluminescence detection (Amersham) on X-ray film (X-OMAT AR). The intensity of each band from multiple analyses was quantitated with the use of NIH Image software and expressed as a percentage of the intensity of the control sample.
cAMP and PKA assays. Myocardial cAMP content was measured using an enzyme-linked immunosorbent assay (ELISA) kit (Calbiochem). Results were expressed as picomoles of cAMP per milligram of ventricular protein. PKA activity was measured from reconstituted catalytic and regulatory subunits as previously described (21).
RNA extraction and Northern blot analysis of c-fos expression.
Total RNA was isolated from 500 mg of powdered tissue from isolated,
perfused rat hearts with the use of the RNAzol B reagent (Tel-Test).
RNA (10 µg) was subjected to size fractionation on a 1% agarose gel
containing formaldehyde and was transferred to a Duralon (Stratagene)
membrane. RNA was fixed to the membrane by ultraviolet cross-linking
with the use of a Stratalinker (Stratagene), and the membranes were
prehybridized at 42°C for 6 h in 5× standard sodium citrate
(SSC), 0.2% SDS, 2× Denhardt's solution, 50% formamide, 50 mM
KPO4, and 100 µg/ml denatured salmon sperm DNA, and
hybridized for 18-36 h with 1 × 106 cpm/ml of
-32P-labeled probe, i.e., c-fos (Oncogene) or
dlyceraldehyde-3-phosphate dehydrogenase (Clontech). Unbound
probe was removed by washing in 0.1× SSC and 0.1% sodium dodecyl
sulfate, and hybridized probe was visualized by detection on X-ray film
(X-OMAT AR). Hybridized probe was quantitated with the use of NIH Image
software and expressed as the degree of induction of c-fos mRNA.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Elevated CREB phosphorylation during ischemia.
Because CREB is expressed and phosphorylated in cardiac myocytes and
has been shown to be expressed and phosphorylated in failing human
hearts (6, 15), the phosphorylation of CREB was determined
in the Langendorff-perfused rat heart. Western blot analysis of nuclear
fractions from perfused hearts indicated that CREB is rapidly
phosphorylated (e.g., CREB is phosphorylated after 2 min of global
ischemia) (Fig. 1, A
and C). Only minimal levels of phosphorylated CREB were
detected in control-perfused hearts. CREB phosphorylation steadily
increased through 15 min of global ischemia. The increase in
phosphorylated CREB is due to an increase in phosphorylation and not
due to an increase in CREB protein because basal levels of CREB, as
determined by Western blot analysis by using an antibody specific for
CREB, did not change during global ischemia (Fig.
1B). The specificity of the phosphorylated CREB antibody was
determined using nonphosphorylated and phosphorylated CREB control cell
extracts. Phosphorylated CREB was detected exclusively in the
phosphorylated CREB control lane by anti-phosphorylated CREB (Fig.
1A), whereas basal levels of CREB protein were detected in
both phosphorylated and nonphosphorylated CREB lanes by anti-CREB (Fig.
1B).
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iPLA2-mediated CREB phosphorylation during myocardial
ischemia.
Because we have recently shown that PKA can be activated by
lysoplasmenylcholine (21), and because iPLA2
activity increases rapidly after myocardial ischemia (5,
12), the iPLA2-specific inhibitor BEL
(12) was used to determine if CREB phosphorylation during
myocardial ischemia was mediated by iPLA2. BEL (10 µM) inhibited CREB phosphorylation elicited by either 5 or 15 min of global ischemia by 90% and 50%, respectively (Fig.
2, A and B, respectively).
BEL-sensitive, ischemia-elicited CREB phosphorylation was also
observed in cytosolic fractions (100,000 g supernatant) prepared from these hearts with a similar temporal course to that observed in the crude nuclear fraction (data not shown).
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iPLA2 translocation during myocardial ischemia.
Because pretreatment of ischemic rat hearts with the
iPLA2-specific inhibitor BEL results in a reduction in CREB
phosphorylation, and because iPLA2 has been shown to be
activated during myocardial ischemia (5, 12), the
presence of iPLA2 in membrane preparations containing
nuclei from control and globally ischemic hearts was determined. Western blot analyses demonstrated minimal amounts of
iPLA2 present in the membrane preparations isolated from
control-perfused hearts. In contrast, iPLA2 was
translocated to the membrane fraction within 5 min of global
ischemia (Fig. 3). Further
increases in iPLA2 in this membrane fraction were observed
with prolonged global ischemia (Fig. 3).
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Induction of CREB phosphorylation by lysoplasmenylcholine.
Because our present studies utilizing BEL have suggested that
iPLA2 may mediate, in part, CREB phosphorylation during
myocardial ischemia through a PKA-dependent mechanism, the
ability of the product of iPLA2, lysoplasmenylcholine, to
elicit CREB phosphorylation was assessed. Western blot analysis of
crude nuclear proteins indicated that CREB phosphorylation is elevated
after only 2 min of heart perfusion with 500 nmol/l
lysoplasmenylcholine (Fig. 4A). The phosphorylation of
CREB increased with increasing time intervals of perfusion with
lysoplasmenylcholine. Perfusion of hearts with lysoplasmenylcholine for
15 min, followed by perfusion with lysoplasmenylcholine-free buffer
resulted in a time-dependent reduction in CREB phosphorylation (Fig.
4B). Additionally, H-89 pretreatment of
lysoplasmenylcholine-treated hearts resulted in a significant decrease
in phosphorylated CREB compared with the CREB phosphorylation obtained
by lysoplasmenylcholine perfusion alone (Fig. 4B). In
contrast, BEL pretreatment of lysoplasmenylcholine-treated hearts did
not reduce phosphorylated CREB (Fig. 4B). Additionally, neither lysoplasmenylcholine nor BEL treatments of isolated adult rat
hearts resulted in changes in measured cAMP compared with control-perfused hearts (Fig. 4C).
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CREB phosphorylation induced by 8-Br-cAMP treatment and
lysoplasmenylcholine.
Because CREB is phosphorylated through a PKA-dependent mechanism, and
because PKA can be activated by both cAMP and products of
iPLA2 (i.e., lysophospholipids) (21), we
examined the effects of the exogenously added cAMP analog on CREB
phosphorylation. Although 0.1 µM 8-Br-cAMP did not result in a
significant increase in phosphorylated CREB compared with control
perfused hearts (Fig. 6A), 1 µM of this cAMP analog elicited CREB phosphorylation (Fig. 6A). Simultaneous perfusion of hearts with both 50 nM
lysoplasmenylcholine and 1 µM 8-Br-cAMP resulted in levels of
phosphorylated CREB that were approximately the sum of CREB
phosphorylation from perfusion with 50 nM of lysoplasmenylcholine and 1 µM 8-Br-cAMP independently (Fig. 6B). These data suggest
that cAMP and lysoplasmenylcholine activate PKA through a common site
on the PKA regulatory subunit. Further support for this common
mechanism of PKA activation is provided by the findings that both cAMP
and lysoplasmenylcholine activation of PKA, in an in vitro assay
system, are attenuated by treatment with the PKA regulatory site
inhibitor Rp-8-Br-cAMP (Fig. 6C). Additionally, Rp-8-Br-cAMP
inhibited CREB phosphorylation after both 5 and 15 min of global
ischemia (Fig. 2, A and B).
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Inhibition of ischemia-induced c-fos expression by BEL.
Because c-fos expression has been demonstrated to be highly
induced during ischemia in porcine myocardium (3),
and because c-fos expression in myocardium is regulated, in
part, by the cAMP pathway (16), we determined if BEL
treatment could attenuate c-fos expression during myocardial
ischemia. The levels of c-fos mRNA expression were
determined by Northern blot analysis (Fig. 7A). Global ischemia,
as well as perfusion of hearts with lysoplasmenylcholine, significantly
induced c-fos expression compared with the levels of
c-fos mRNA present in control perfused hearts (Fig.
7B). Furthermore, treatment of hearts with BEL followed by
global ischemia significantly reduced the levels of
c-fos mRNA detected (Fig. 7B).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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The phosphorylation of CREB has been implicated in the transcriptional activation of many genes (e.g., c-fos, c-jun) induced by various stimuli (1, 18). Phosphorylated CREB binds to the distinct consensus sequences (CRE) in the promoter regions of genes regulated by the cAMP-signaling pathway (14). In the heart, it has been shown that CREB is phosphorylated in response to agents that increase intracellular camp, including forskolin and isoproterenol (6-8, 15). Although CREB phosphorylation has also been observed in end-stage heart failure, CREB phosphorylation has not been demonstrated in response to myocardial ischemia. The present study demonstrates for the first time that CREB is rapidly phosphorylated in response to brief intervals of myocardial ischemia.
Because PKA has been recently shown to be activated by
lysoplasmenylcholine (21) and because iPLA2 is
activated by myocardial ischemia (5, 12), CREB
phosphorylation mediated by iPLA2 during myocardial
ischemia was explored. The data presented herein support Fig.
8, which shows a likely mechanism through
which PKA is modulated during myocardial ischemia ultimately
leading to the phosphorylation of CREB and the expression of
c-fos. PKA is initially activated during myocardial
ischemia through the actions of iPLA2-mediated
production of lysophospholipids possessing a choline polar head group
(see Fig. 8). Furthermore, the prolonged activation of PKA in response
to extended intervals of myocardial ischemia is mediated by
elevations in cAMP (see Fig. 8). Through either signal, PKA
phosphorylates CREB which then leads to c-fos production.
The early phase of activation shown in Fig. 8 (i.e., iPLA2-mediated CREB phosphorylation via activation of PKA
by lysophospholipids) is supported by the following four results from
hearts rendered globally ischemic for 5 min. First, the
iPLA2 inhibitor BEL almost completely ablates CREB
phosphorylation after 5 min of global myocardial ischemia.
Second, the PKA inhibitor H-89 inhibits CREB phosphorylation after 5 min of global myocardial ischemia. Third, cAMP levels do not
increase in the first 5 min of global ischemia. Fourth, the
product of iPLA2, lysoplasmenylcholine, elicits CREB phosphorylation in isolated, perfused hearts that are not subjected to
ischemia. The second prolonged (or delayed) phase of activation is shown in Fig. 8 (i.e., CREB phosphorylation via activation of PKA by
cAMP) and is supported by the following three results from hearts
rendered globally ischemic for 15 min. First, the iPLA2 inhibitor BEL only partially inhibited CREB
phosphorylation after 15 min of global myocardial ischemia.
Second, the PKA inhibitor H-89 inhibits CREB phosphorylation after 15 min of global myocardial ischemia. Third, cAMP levels increased
twofold after 15 min of global ischemia. The downstream
targeting of CREB phosphorylation mediating c-fos expression
was also supported by the findings that c-fos is induced in
ischemic myocardium, as well as myocardium treated with
lysoplasmenylcholine, and that BEL partially inhibits c-fos
expression in ischemic myocardium. Thus the results herein strongly suggest that both lysophospholipid production mediated by
iPLA2 activity and cAMP production share an integral role
in signal transduction during ischemia resulting in the
phosphorylation of CREB and subsequent induction of immediate, early
gene expression.
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In tissues other than myocardium, the phosphorylation of CREB occurs after the translocation of the catalytic subunit of PKA to the nucleus (19). Nuclear phosphorylation of CREB by PKA occurs at a single site (serine-133), which then activates transcription (10). We have recently shown that lysoplasmenylcholine, a product of iPLA2 enzymatic action on plasmenylcholine, as well as other lysophospholipids containing a choline polar head group (e.g., lysophosphatidylcholine and lyso platelet activating factor), activate PKA in vitro through a cAMP-independent mechanism that likely involves dissociation of the catalytic subunit from the regulatory subunit (21). These previous studies, in conjunction with the present results, suggest that myocardial ischemia-induced activation of iPLA2 may result in the formation of lysophospholipid second messengers that activate PKA, allowing the catalytic subunit of PKA to translocate to the nucleus and mediate the phosphorylation of CREB and the subsequent induction of immediate early gene transcription. Alternatively, iPLA2 that is activated during myocardial ischemia may reside in the nucleus, resulting in production of the PKA activator, lysophospholipid, that would activate PKA locally at the nucleus.
It should also be appreciated that cAMP-independent CREB phosphorylation during early stages of ischemia potentially may be mediated by calmodulin-dependent kinase (17, 20). A role for iPLA2 in this pathway could be mediated through alterations in intracellular calcium during myocardial ischemia mediated by the production of arachidonic acid and lysoplasmenylcholine (or lysophosphatidylcholine) (9). Although the present studies do not rule out this potential mechanism for ischemia-elicited CREB phosphorylation through the activation of calmodulin-dependent kinase, the present findings suggest that the majority of CREB phosphorylation during the ischemic intervals studied is mediated through PKA because PKA-specific inhibitors blocked CREB phosphorylation elicited by either ischemia or perfusions with lysoplasmenylcholine. Additionally, lysoplasmenylcholine directly activates PKA in kinase assays with purified PKA (21).
It has previously been shown that c-fos is rapidly expressed after myocardial ischemia (3). Immediate early genes, such as c-fos, are regulators of transcription, and it is hypothesized that the induction of immediate early genes (i.e., c-fos) in response to myocardial ischemia may lead to the activation of genes involved in the repair of reversible damage to the myocardium (3). The expression of c-fos during myocardial ischemia likely occurs through the activation of PKA and subsequent CREB phosphorylation because c-fos contains a CRE and is regulated by PKA in the adult rat heart (16). Furthermore, the present results suggest that c-fos is induced through biochemical mechanisms involving the bimodal regulation of PKA by lysoplasmenylcholine and cAMP during myocardial ischemia (Fig. 8).
In summary, the results herein support a signaling role of iPLA2 activation during myocardial ischemia that includes the sequential downstream activation of PKA, CREB phosphorylation, and early gene induction. Additionally, a bimodal regulatory mechanism is proposed for this signal transduction pathway that is mediated by iPLA2 during the early stages of ischemia, whereas cAMP levels activate this pathway during prolonged ischemia. Thus the present results demonstrate a novel signaling pathway mediated by iPLA2, which represents the first time a signaling pathway has been shown to be mediated by iPLA2. Furthermore, these studies demonstrate that iPLA2 activated during myocardial ischemia likely plays an important role in myocardial ischemia through this pathway that results in the production of early gene products.
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ACKNOWLEDGEMENTS |
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This research was supported jointly by National Heart, Lung, and Blood Institute Grant HL-42665 (to D. A. Ford) and Research Career Development Award HL-03316 (to D. A. Ford). This work was performed during the tenure of a predoctoral fellowship award (to S. D. Williams) from the American Heart Association, Heartland Affiliate.
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FOOTNOTES |
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Address for reprint requests and other correspondence: D. A. Ford, Dept. of Biochemistry and Molecular Biology, St. Louis Univ. Health Sciences Center, 1402 S. Grand Blvd., St. Louis, MO 63104 (E-mail: fordda{at}slu.edu).
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.
Received 18 January 2001; accepted in final form 14 March 2001.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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P < 0.01 for comparisons between phosphorylated CREB
from hearts rendered globally ischemic for 5 or 15 min and
phosphorylated CREB from ischemic hearts treated with the
selected inhibitors. n.d., Not detectable. C: cAMP content
of hearts subjected to the indicated experimental conditions was
determined using an enzyme-linked immunosorben assay (ELISA) as
described in MATERIALS AND METHODS. *P < 0.01 for comparison between cAMP levels in control-perfused hearts and
hearts rendered globally ischemic for 15 min.
