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Vol. 294, Issue 2, 605-612, August 2000
Departments of Pharmacology (B.M.M., E.G.E.) and Anesthesiology (E.G.E.), University of Illinois College of Medicine at Chicago, Chicago, Illinois
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Abstract |
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 Top
 Abstract
 Introduction
Experimental Procedures
Results
Discussion
References
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Angiotensin I-converting enzyme (kininase II) inhibitors (ACEis) are very widely used to treat cardiac conditions and nephropathies, but some of their beneficial activities cannot be attributed to enzyme inhibition alone. We investigated the effects of ACEis on the human bradykinin (BK) B2 receptor expressed in Chinese hamster ovary cells transfected with the cDNA of human receptor and ACE, and on human pulmonary endothelial cells that constitutively express both proteins. BK and its ACE-resistant peptide analog activated the B2 receptor to release arachidonic acid and elevate [Ca2+]i and subsequently desensitized it. The release of arachidonic by BK was independent of extracellular Ca2+. BK enhanced phosphorylation of the immunoprecipitated B2 receptor but enalaprilat significantly reduced it. ACEi resensitized the receptor by initiating a cross talk between the receptor and ACE. Protein kinase C and phosphatase inhibitors distinguished the signaling by the receptor when activated first by BK from BK acting on the resensitized receptor. Treatment of cells with 1 µM calphostin, 100 nM staurosporine, 100 nM calyculin, or 500 nM okadaic acid did not affect either one of the primary actions of BK on the receptor. Protein kinase C or phosphatase inhibitors, however, blocked the effects of BK on the receptor resensitized by enalaprilat or ramiprilat. The experiments clearly differentiate the primary activation of the receptor by BK from activation of the resensitized receptor after ACEi treatment. The existence of an intermediate component involved in the action of ACEis to enhance release of vasoactive mediators by BK is suggested.
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Introduction |
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Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
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Inhibitors
of angiotensin I-converting enzyme (ACE or kininase II) are
administered to millions of patients with strikingly beneficial effects
in a variety of cardiovascular and other conditions, including
hypertension, congestive heart failure, myocardial infarction, diabetic
nephropathy (Pfeffer et al., 1992
; Gavras, 1994; Ambrosioni et al.,
1995; Lewis, 1996; Mancini et al., 1996; HOPE Study Investigators, 2000). Recently, it was reported after extensive clinical studies that
an ACE inhibitor (ACEi) even reduced the occurrence of diabetes (HOPE
Study Investigators, 2000). ACEis block both the release of angiotensin
II and the inactivation of bradykinin (BK; Yang et al., 1971; Linz et
al., 1995). The inhibitors significantly enhance the activity of BK and
the release of mediators such as nitric oxide (NO) and prostaglandins
by the peptide (Bhoola et al., 1992; Carretero and Scicli, 1995;
Margolius, 1995). The interaction of the inhibitors with BK, however,
cannot be attributed only to blocking the breakdown of the peptide
(Skidgel and Erdös, 1998); for example, the potentiation of the
effect of BK and its ACE resistant analogs on the
B2 receptor (Auch-Schwelk et al., 1993; Hecker et
al., 1994) and the immediate resensitization of the receptor
desensitized by the agonist BK (Minshall et al., 1997a,b; Marcic et
al., 1999, 2000) have been documented. ACE and the
B2 receptor have to be sterically close to each
other on the cell membrane to induce these effects, possibly by forming a heterodimer (Marcic et al., 2000).
The very favorable results obtained while treating a large number of
patients with ACEi in a variety of clinical conditions (HOPE Study
Investigators, 2000) made it even more interesting to study further the
activities of ACEis at the cellular level on the phenomena induced by
them, independent of inhibition of BK inactivation (Minshall et al.,
1997b; Deddish et al., 1998; Erdös et al., 1999; Benzing et al.,
1999; Marcic et al., 1999, 2000). The use of protein kinase C (PKC) or
phosphatase inhibitors clearly distinguished the primary action of the
ligand BK on the receptor from the reactivation of the desensitized
B2 receptor by BK, after it was resensitized by
an ACEi. This tenet, based on determining arachidonic acid (AA) release
and [Ca2+]i equally
applies to cultured cells that were either transfected to express human
B2 receptor and ACE [Chinese hamster ovary
(CHO)/AB] or expressed both proteins constitutively, such as human
pulmonary artery endothelial (HPAE) cells.
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Experimental Procedures |
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Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
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Materials.
BK, hippuryl-His-Leu (Hip-His-Leu), tissue
culture medium, buffers, and reagents were from Sigma Chemical Co. (St.
Louis, MO).
[Phe8(CH2NH)Arg9]BK,
ACE-resistant BK analog (Drapeau et al., 1988; Marcic et al., 2000) was
obtained from Novabiochem (San Diego, CA). Fetal bovine serum was from
Atlanta Biologicals (Norcross, GA) and Z-Phe-His-Leu was from Bachem
(Philadelphia, PA). Enalaprilat was provided by Merck, Sharpe & Dohme
Research Division (Whitehouse, NJ), ramiprilat by Upjohn Laboratories
(Kalamazoo, MI), and HOE 140 by Hoechst Co. (Frankfurt, Germany).
[3H]BK (97 Ci/mmol) was from Amersham Pharmacia
Biotech, Inc. (Piscataway, NJ).
[5,6,8,9,11,12,14,15-3H(N)]AA
([3H]AA; 100 Ci/mmol) was purchased from
American Radiolabeled Chemicals (St. Louis, MO). The original cDNA of
wild-type ACE was kindly donated by Professor P. Corvol of College de
France, Paris. B2 receptor cDNA was provided by
Dr. K. Jarnigan (Syntex, Palo Alto, CA). CHO cells were from the
American Type Culture Collection (Rockville, MD). HPAE cells were
purchased from Clonetics (San Diego, CA). Mammalian expression vectors
pcDNA3 and pCEP4 were from Invitrogen (Carlsbad, CA).
Anti-B2 receptor antibodies were kindly provided
by Professor W. Müller-Esterl of Gutenberg University, Mainz,
Germany. Transfection reagent (Superfect) and geneticin (G418) were
from Life Technologies (Grand Island, NY). Hygromycin B, staurosporine,
calphostin C, calyculin A, and okadaic acid were purchased from
Calbiochem (San Diego, CA)
Cell Culture.
CHO cells were grown as described (Minshall et
al., 1997b; Marcic et al., 1999). HPAE cells were cultured in
Dulbecco's modified Eagle's medium with the same supplements. Cells
were routinely subcultured with trypsin-EDTA to mobilize them (Minshall
et al., 1997b). For transfection, CHO cells were plated at density
1 × 105 cells/60-mm dish 1 day before transfection.
Transfection and Cloning.
To establish cell lines with
stable expression, CHO cells were transfected with human wild-type ACE
cDNA in pCDNA3 expression vector, carrying neomycin resistance gene
with Superfect method with serum-free Ham's F-12 medium without
antibiotic. The Superfect-DNA complex was added into the dish over the
entire surface and incubated with the cells for 3 h at 37°C. The
cells were subcultured into medium containing 500 µg/ml geneticin
G418. In 10 to 20 days, clones of transfected cells were formed (Marcic
et al., 1999).
Screening of Clones for ACE Activity.
Individual clones were
evaluated both for cell-associated and -released ACE activity. Cells
were incubated in serum-free medium for 24 h, medium was
collected, the cells were washed and lysed in 3 ml of 8 mM
3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonic acid in PBS,
pH 7.4. Both the supernatants and the lysates were centrifuged (for 15 min at 900g) and their aliquots were mixed with 1 mM
Hip-His-Leu or Z-Phe-His-Leu of substrate and incubated 4 h at
37°C. After the reaction was terminated, His-Leu released was
determined by coupling with o-phthaldialdehyde at 365 nm
excitation and 500 nm emission wavelengths (Deddish et al., 1998).
Clones with highest levels of ACE expression were transfected with
B2 receptor cDNA (Marcic et al., 1999).
Transfection with Human B2 Receptor cDNA.
The
selected clones were transfected with pCEP4 vector containing human
B2 BK receptor cDNA with the Superfect
transfection method (Marcic et al., 1999). After transfection, cells
were selected in Ham's F-12 medium containing 0.5 mg/ml Hygromycin B
(pCEP4 vector with Hygromycin B resistant gene).
Radioligand Binding on Selected Clones.
Clones with the
highest expression of B2 receptors were selected
by [3H]BK saturation binding on whole-cell
monolayers expressing both ACE and B2 receptors.
Equilibrium binding of 0.05 to 20 nM [3H]BK
with or without 10 µM unlabeled BK was done in Ham's F-12 cell
culture medium for 1 h at 37°C (Minshall et al., 1997). Bound radioactivity was separated from excess [3H]BK
by washing and counted in liquid scintillation vials. Clones with the
high expression of B2 receptors on the cell
surface were chosen and used further. Cells expressing both human
B2 receptor and wild-type ACE were designated as
CHO/AB cells.
Measurement of Changes in [Ca2+]i and
[3H]AA.
Free cytosolic calcium
[Ca2+]i was measured with
a microspectrofluorometer (PTI Deltascan, Princeton, NJ), or Attofluor
Ratiovision with fura-2/AM reagent. Cells were grown to confluence on
glass coverslips, then incubated with 2 to 5 µM fura-2/AM for 1 h at 37°C, washed with buffer, and mounted in a Sykes-Moore chamber (Bellco, Vineland, NJ) at room temperature. Cellular fluorescence at
510 nm was measured after excitation at wavelengths of 340 and 380 nm
(Erdös et al., 1999; Marcic et al., 2000).
[3H]AA release was measured as described in
Minshall et al. (1997b).
De- and Resensitization of B2 Receptor.
After
desensitization of the receptor by initial exposure of cells to a kinin
(Minshall et al., 1997b), the restoration of sensitivity to the agonist
(resensitization) was measured either by [3H]AA release
or by mobilization of [Ca2+]i. For example,
monolayers of transfected CHO cells loaded with [3H]AA
were stimulated with 1 µM BK or its ACE-resistant analog for 30 min.
Then, without removal of BK, cells were exposed to either enalaprilat
(5 nM or 1 µM) or ramiprilat (5 nM or 1 µM) without adding more
kinin or, as control, to a second dose of only kinin for an additional
5 min. (Minshall et al., 1997b). The amount of [3H]AA
released was determined by taking AA released during the first 30 min
as baseline, and normalizing to the amount released by buffer alone
during the 5-min reactivation.
B2 Receptor Phosphorylation. The phosphorylation of B2 receptors by BK was measured in confluent monolayers of CHO/AB cells loaded with [32P]orthophosphate (100 µCi/ml medium) for 4 h. Subsequently, the cells were either treated with buffer alone, or 1 µM BK, or 1 µM BK and 1 µM enalaprilat for 30 min. As control, 1 µM phorbol-12-myristate-13-acetate (PMA) was used for 30 min at 37°C. The cells in monolayers were solubilized with 1% Triton X-100, centrifuged at 100,000g for 15 min, and the supernatants were saved. Anti-B2 receptor polyclonal antibodies were added at 1:1000 v/v dilution and samples were incubated overnight with shaking at 4°C. When insoluble protein A was added to each sample to 10%, incubation continued for 2 h at 4°C. Beads with immune complexes were sedimented by centrifugation at 1000g for 15 min. The presence of B2 receptors was verified by [3H]BK binding and the receptors were subjected to 10% SDS-polyacrylamide gel electrophoresis. The bands labeled with 32P were visualized by autoradiography and the densities of B2 receptor bands were quantitated by scanning densitometry.
Kinase and Phosphatase Inhibition.
Inhibitors of the PKC and
phosphatases 1 and 2A were used. Cultured HPAE or CHO/AB cells were
pretreated with 100 nM staurosporine, an inhibitor of all PKC
isoenzymes except the atypical one (Tamaoki et al., 1986; Hofmann,
1997), for 15 min. Alternatively, the same cells were pretreated with 1 µM calphostin C, an inhibitor of all PKC isoenzymes (Hofmann, 1997),
for 15 min.
) for 30 min before
experiments. Another, more specific inhibitor of phosphatases 1 and 2A,
okadaic acid (Gjertsen et al., 1994), was used at 500 nM for 30 min.
Statistics. The data in the figures and text are expressed as mean ± S.E. when n = 3 or more. When some previously reported experiments were repeated with the same results, they were done once or twice in duplicate and not pursued further. [Ca2+]i levels are represented as the percentage of mean fluorescence intensity increase relative to control levels, calculated as nanomolar concentrations. Statistical evaluation was performed by one-way ANOVA for matched values. Values of P less than .05 were considered statistically significant.
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Results |
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Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
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CHO/AB and HPAE Cells
Transfected CHO/AB cells express 2 × 105 B2 receptors/cell as
determined by [3H]BK saturation binding, in
agreement with our previous results (Marcic et al., 1999;
n = 5). Binding experiments were performed regularly
during culture and the B2 receptor expression did
not change with passage. The very high expression of transfected ACE (106 ACE molecules/cell) in CHO/AB cells and the
inhibition of the enzyme by enalaprilat (72% at 5 nM) were previously
described (Marcic et al., 1999). HPAE cells constitutively expressed
14,000 B2 receptors/cell (n = 4).
Expression of ACE in HPAE cells decreased with the number of passages
(Johnson, 1980); after eight passages (the highest used), it was 7000 to 9000 molecules/cell (n = 3).
B2 Receptor Phosphorylation
The effects of ACE inhibitors on the phosphorylation of the
B2 receptors were tested in transfected CHO/AB
cells, expressing wild-type human ACE and human
B2 receptors, after treating them with
32P. The results, calculated as changes in
relative optical densities, were the following: no treatment = 1.0, enalaprilat = 1.1 ± 0.1, BK = 1.9 ± 0.3, and
BK and enalaprilat = 1.3 ± 0.1 (P < .05). As control, PMA was added, which increased phosphorylation to 2.4 ± 0.3 (n = 5; P < .05). Thus, in
these experiments, 1 µM enalaprilat significantly decreased the
phosphorylation of the B2 receptor induced by 1 µM BK (Fig. 1). Enalaprilat added alone
without BK had no effect.
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Effects of PKC and Phosphatase Inhibition on [Ca2+]i Increase
ACE inhibitors can resensitize the B2
receptor to the agonist both in transfected cultured cells and in cells
that constitutively express both ACE and B2
receptors (Minshall et al., 1997b, Marcic et al., 1999). We wished to
determine whether the first response to activation of the receptor by
the agonist that immediately desensitizes it, and the one after
reactivation of the B2 receptor, resensitized by
ACEi to the agonist present in the medium, may proceed through
different signal transduction pathways. For this purpose, we tested
inhibitors of PKC and phosphatases 1 and 2A on both transfected CHO/AB
cells and on HPAE cells, which constitutively express the proteins.
CHO/AB Cells.
ACE inhibitors resensitize the
B2 receptor to BK in the medium that previously
desensitized the receptor in CHO/AB cells. The response was measured by
the increase in [Ca2+]i
level to BK analog in the medium after adding an ACEi
(n = 6; Fig. 2A).
Pretreatment of cultured CHO/AB cells with PKC inhibitor 1 µM
calphostin C (Hofmann, 1997) for 15 min did not affect the elevation of
[Ca2+]i by BK because 10 nM BK analog still transiently increased
[Ca2+]i. However, after
calphostin C 1 µM ramiprilat did not resensitize the
B2 receptor to BK analog (n = 4;
Fig. 2B). Pretreatment of CHO/AB cells with another PKC inhibitor, 100 nM staurosporine, also blocked the resensitization by ACEi (data not
shown).
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HPAE Cells.
Experiments with HPAE cells that constitutively
express ACE and B2 receptor yielded the same
results as with the transfected cells. Enalaprilat (1 µM)
resensitized the B2 receptor to
[Ca2+]i mobilization
induced by BK (n = 3; Fig.
3A). Exposing HPAE cells to 1 µM
calphostin C for 15 min did not affect the primary action of BK, but
blocked the effect of enalaprilat. It did not resensitize the receptor
to the BK (10 nM) in the medium (n = 3; Fig.
3B). The results with staurosporine (100 nM) were identical (data not shown).
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Okadaic Acid.
Another inhibitor of the phosphatases 1 and 2A,
okadaic acid (Gjertsen et al., 1994), also was tested in both cell
types. When both HPAE or CHO/AB cells were pretreated with 500 nM
okadaic acid for 30 min, the mobilization of
[Ca2+]i by BK (10 nM) was
not affected (Fig. 4). However, just as
with calcyculin, okadaic acid abolished resensitization of the receptor to BK by 1 µM enalaprilat both in HPAE cells (n = 5;
Fig. 4A) and in CHO/AB cells (n = 4; Fig. 4B).
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Effects of Kinase and Phosphatase Inhibition on [3H]AA Release
ACE inhibitors also can resensitize the B2
receptor to BK to release AA from cells expressing both
B2 receptors and ACE (Minshall et al., 1997b;
Marcic et al., 1999). Because
[Ca2+]i elevation and AA
leading to the synthesis of different mediators, prostaglandins and NO,
involve the coupling of different G-proteins to the receptor (deWeerd
and Leeb- Lundberg, 1997; Erdös et al., 1999), we tested the
effects of kinase and phosphatase inhibitors on AA release from CHO/AB cells.
Kinase Inhibition.
Enalaprilat (1 µM) resensitized the
B2 receptor, desensitized by the ligand (Marcic
et al., 1999) in CHO/AB cells, and enhanced [3H]AA release 3.4 ± 0.6-fold
compared with the addition of buffer alone (n = 4, P < .05). Calphostin C (1 µM; 15 min) pretreatment abolished 98 ± 7% (n = 4; P < .05) of this resensitization by enalaprilat (Fig.
5).
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Phosphatase Inhibition.
Effect of the phosphatase inhibitor
calyculin A on the resensitization of B2 receptor
by enalaprilat was tested similarly by measuring
[3H]AA release. Enalaprilat (1 µM)
resensitized BK-induced [3H]AA release from
CHO/AB cells 4.9 ± 0.7-fold compared with the addition of buffer
alone (n = 3; P < .05). Calyculin A
(100 nM; 30 min) pretreatment abolished 87 ± 16%
(n = 3; P < .05) of the resensitization (Fig. 6).
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Calcium-Free Medium
We studied a potential involvement of extracellular calcium influx
in the resensitization of the receptor to release
[3H]AA. This was done to establish whether
blocking of the phosphorylation or dephosphorylation might block a
putative opening of calcium channels by ACE inhibitors and thereby
inhibit the resensitization of B2 receptor. We
measured the liberation of AA by BK in calcium-free medium. Even in the
absence of extracellular calcium, ramiprilat both in high (1 µM) and
low (5 nM) concentrations resensitized [3H]AA
release induced by the ACE-resistant BK analog (n = 3;
P < .05; Fig. 7),
negating the possibility that a blockade of extracellular Ca2+ uptake would be responsible for the lack of
ACEi effect in the above-mentioned experiments.
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Discussion |
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Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
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BK as an agonist induces the phosphorylation of the
B2 receptor at serine residues, which leads to
the desensitization of the receptor (Leeb-Lundberg et al., 1987;
Roberts and Gullick, 1990; Blaukat et al., 1996; Pitcher et al., 1998).
In the above-experiments, enalaprilat decreased the phosphorylation of
the receptor stimulated by BK (Fig. 1), in good accord with the
potentiation of BK actions by ACEis. Enalaprilat, also in agreement
with previous experiments describing no direct effects of ACEis on the
receptor (Minshall et al., 1997a,b; Marcic et al., 1999, 2000), did not
induce phosphorylation in the absence of BK.
After using PKC and phosphatase inhibitors, we concluded that the activation of the receptor by BK and its reactivation by BK after resensitization by ACEi initiate different signal transduction pathways.
ACEis do not act directly on the B2 receptor
because they are inactive on cells where ACE is not expressed (Minshall
et al., 1997a,b; Marcic et al., 1999). They can enhance the primary
effects of BK and its ACE-resistant peptide analogs on the receptor,
and, as also shown in Fig. 2, they resensitize the receptor
desensitized by BK. This response to the peptides present in the medium
is immediate without adding more BK. All of these experiments exclude the blocking of BK breakdown as the sole reason for the effects of
ACEis in this system. ACEis enhance the effect of BK on the B2 receptor indirectly, first by reacting with an
active center of ACE (Marcic et al., 1999), resulting in an allosteric
modification in the enzyme receptor complex. This, in turn, would lead
to resensitization of the receptor desensitized to its ligand. In this
study, we used PKC and phosphatase inhibitors that caused no harm to
the primary effect of BK on the receptor or any good to the
reactivation of the B2 receptor. Or, in other
words, they did not affect primary activation of the receptor, which is
followed by desensitization (tachyphylaxis) to the agonist peptide. The
elevation of [Ca2+]i or
the release of [3H]AA by BK was not blocked by
PKC inhibitors, in line with the observations of others (Blaukat et
al., 1996; Pizard et al., 1998), or, in our experiments, by two
membrane phosphatase inhibitors. However, the application of either one
of the two PKC or phosphatase inhibitors abolished the very well
documented resensitization of the B2 receptor by
the ACEi to BK present in the medium (Minshall et al., 1997a,b; Benzing
et al., 1999; Erdös et al., 1999; Marcic et al., 1999, 2000). We
tested two different ACEis, enalaprilat and ramiprilat, to distinguish
between specific and group-related structural effects of the compounds,
and the results were identical with both inhibitors. Besides BK, an
ACE-resistant peptide analog, a ligand to B2
receptor not cleaved by ACE was used (Drapeau et al., 1988; Marcic et
al., 2000). The activation of the B2 receptor was
assessed by measuring AA release and
[Ca2+]i elevation as
parameters of the important indirect cardiovascular actions of BK,
namely, the liberation of prostaglandins and NO (Cachofeiro and
Nasjletti, 1991; Bhoola et al., 1992; Carretero and Scicli, 1995). In
addition, in some tissues, AA is metabolized to endothelium-derived
hyperpolarizing factors (Campbell and Harder, 1999).
The lack of effect of PKC inhibitors on the primary activation of the
B2 receptor by the ligand is understandable if
the receptor is phosphorylated by another kinase. The 
-adrenergic
receptor kinase can phosphorylate BK B2 receptor
in vitro followed by a secondary action of PKC (Blaukat et al., 1996).
If -adrenergic receptor kinase is involved in BK-induced
phosphorylation of B2 receptors, ACEis can still
lower phosphorylation directly or indirectly. Reducing
B2 receptor phosphorylation, thus,
desensitization, renders it more reactive to BK already present in the medium.
Speculative explanations of roles of PKC and phosphatase inhibitors in
blocking the resensitization of B2 receptors by
ACEi include the following. Dephosphorylation is the final step of receptor recycling. Inhibition of phosphatases that act on cell membranes may block removal of phosphate groups from
B2 receptors, which are recycled back to the
surface and prevent signaling of receptors. In this model, rapid
recycling would be promoted by ACE inhibitors. However, we found
previously that B2 receptor endocytosis in
transfected CHO cells is a slow process (Minshall et al., 1997b).
Inhibition of PKC also could affect phosphorylation of an intermediate
protein that is mediating the interaction between
B2 receptors and ACE induced by ACEi. This
putative switch protein, which may be a regulator of
B2 receptor signaling, is phosphorylated by PKC
and dephosphorylated on the membrane. Inhibiting either process blocks
the rapid resensitization of the receptor. For example, PKC can affect
a G-protein-coupled receptor kinase (Pitcher et al., 1998) that may be
responsible for B2 receptor desensitization, thus
inhibiting PKC may block this secondary event. Such an enzyme may be
the primary factor in receptor desensitization, thus PKC may
destabilize it. Phosphatase inhibition may block the recycling of this
intermediary protein kinase.
The cytosolic portion of ACE is unlikely to be phosphorylated because
deletion of three of five potentially phosphorylated residues from the
C-terminal end of recombinant ACE did not affect the actions of ACEis
(Marcic et al., 2000).
The above-mentioned experiments showed that the transduction pathway
mediating the action on the resensitized B2
receptor differs from the initial pathway involved in primary response to BK. Dalemar et al. (1996) described that PKC and PKA can modulate expression of B2 receptor affinity forms.
Consequently, there is a possible conformational change in the receptor
involved in the signaling, and after the application of ACEi, the
reactivated receptor signals through alternate pathways. We reported
that a physical proximity between B2 receptors
and ACE is required for the resensitization phenomenon to occur (Marcic
et al., 2000), possibly the formation of an
ACE-B2 receptor heterodimer. It follows that in
the absence of ACE expression, ACEis are ineffective (Minshall et al.,
1997b; Marcic et al., 1999).
Judging from experiments based on AA release and
[Ca2+]i elevation, both
G
i- and Gq-coupled
B2 receptors are involved in the reactivation
process (Burch and Axelrod, 1987; de Weerd and Leeb-Lundberg, 1997;
Marcic et al., 1999). The Gq-mediated
activation of phospholipase C by BK is followed by inositol
phosphate3 release that mobilizes [Ca2+]i from internal
sources. Reactivation of the receptor to the BK in the medium elevates
[Ca2+]i level in CHO
cells by promoting the entry of calcium from extracellular sources
(Marcic et al., 1999). However, as shown above, resensitization by
ACEis to a Gi-mediated, BK-induced
[3H]AA release is possible even in the absence
of extracellular calcium, suggesting an involvement of a
calcium-insensitive phospholipase A2 (Balsinde
and Dennis, 1997). These findings also indicate that mechanisms of AA
release and increase in
[Ca2+]i level induced by
BK on the resensitized receptor are different.
In conclusion, the use of PKC and phosphatase inhibitors clearly distinguishes the primary activation of the B2 receptor by agonist and subsequent action on the receptor reactivated by an ACEi. These observations point to possible additional beneficial consequences of ACEi application by amplification of BK effects.
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Acknowledgments |
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We are grateful to Drs. Peter A. Deddish, Randal A. Skidgel, and Richard D. Minshall for helpful discussion and to Sara Bahnmaier for editorial assistance.
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Footnotes |
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Accepted for publication April 4, 2000.
Received for publication March 9, 2000.
1 This study was supported in part by National Institutes of Health National Heart, Lung and Blood Institute Grants HL36473 and HL58118.
Send reprint requests to: Ervin G. Erdös, M.D., University of Illinois College of Medicine at Chicago, Department of Pharmacology (M/C 868), 835 S. Wolcott Ave., Rm. E403, Chicago, IL 60612-7344. E-mail: egerdos{at}uic.edu
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Abbreviations |
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ACE, angiotensin I-converting enzyme; ACEi, ACE inhibitor; BK, bradykinin; NO, nitric oxide; PKC, protein kinase C; AA, arachidonic acid; CHO, Chinese hamster ovary; HPAE, human pulmonary artery endothelial; PMA, phorbol-12-myristate-13-acetate.
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References |
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Top
Abstract
Introduction
Experimental Procedures
Results
Discussion
References
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-nitro-L-arginine.
Hypertension
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683-688 subunits Gq and Gi in caveolae in DDT1 MF-2 smooth muscle cells.
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(CH2-NH)Arg9]bradykinin, a B2 receptor selective agonist which is not broken down by either kininase I or kininase II.
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Some unanswered questions about system characteristics and roles in human disease.
Hypertension
26:
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 C. Hecquet, D. Biyashev, F. Tan, and E. G. Erdos Positive cooperativity between the thrombin and bradykinin B2 receptors enhances arachidonic acid release Am J Physiol Heart Circ Physiol, March 1, 2006; 290(3): H948 - H958. [Abstract] [Full Text] [PDF]
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D. Biyashev, F. Tan, Z. Chen, K. Zhang, P. A. Deddish, E. G. Erdos, and C. Hecquet Kallikrein activates bradykinin B2 receptors in absence of kininogen Am J Physiol Heart Circ Physiol, March 1, 2006; 290(3): H1244 - H1250. [Abstract] [Full Text] [PDF]
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 D. J. Campbell, H. Krum, and M. D. Esler Losartan Increases Bradykinin Levels in Hypertensive Humans Circulation, January 25, 2005; 111(3): 315 - 320. [Abstract] [Full Text] [PDF]
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 E. G Erdos Kinins, the long march--A personal view Cardiovasc Res, June 1, 2002; 54(3): 485 - 491. [Full Text] [PDF]
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 H. L. Jackman, M. G. Massad, M. Sekosan, F. Tan, V. Brovkovych, B. M. Marcic, and E. G. Erdos Angiotensin 1-9 and 1-7 Release in Human Heart: Role of Cathepsin A Hypertension, May 1, 2002; 39(5): 976 - 981. [Abstract] [Full Text] [PDF]
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P. A. Deddish, B. M. Marcic, F. Tan, H. L. Jackman, Z. Chen, and E. G. Erdos Neprilysin Inhibitors Potentiate Effects of Bradykinin on B2 Receptor Hypertension, February 1, 2002; 39(2): 619 - 623. [Abstract] [Full Text] [PDF]
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