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From the
Received for publication, May 23, 2001, and in revised form, November 9, 2001
The signal transduction pathway linking
physiological concentrations of [Arg8]vasopressin
(AVP) to an increase in frequency of Ca2+ spiking was
examined in confluent cultures of A7r5 vascular smooth muscle cells.
Immunoprecipitation/Western blot studies revealed a robust increase in
tyrosine phosphorylation of the non-receptor tyrosine kinase, PYK2, in
A7r5 cells treated with 4 Periodic or oscillatory increases in cytosolic free
[Ca2+]
([Ca2+]i)1
in vascular smooth muscle cells are believed to underlie arterial vasomotion. These rhythmic contractions of resistance arteries and
arterioles are important for local perfusion of tissues (1) as well as
a determinant of blood pressure and peripheral resistance (2).
Vasomotion correlates with action potentials in the smooth muscle cells
of the artery wall (3-7). This activity depends on activation of
L-type voltage-sensitive Ca2+ channels (5, 7) and may be
triggered or enhanced by vasoconstrictor hormones (3, 8-12). The
mechanisms whereby vasoconstrictor hormones stimulate
Ca2+-dependent action potentials in vascular
smooth muscle cells have not been elucidated.
AVP is a potent vasoconstrictor peptide. It binds to heptahelical
V1a vasopressin receptors on vascular smooth muscle cells, leading to G protein-dependent activation of phospholipase
C (PLC) and the consequent release of Ca2+ from
intracellular stores. This signal transduction pathway is activated
independently of L-type voltage-sensitive Ca2+ channels
(13) and requires nanomolar concentrations of AVP for half-maximal
activation (14, 15). We have identified previously a novel signal
transduction pathway in A7r5 vascular smooth muscle cells that is
activated by physiological concentrations of AVP (between 10 and 100 pM) and leads to oscillations of
[Ca2+]i (Ca2+ spiking) that increase
in frequency with [AVP] (15, 16). This effect of low [AVP] is
dependent on L-type voltage-sensitive Ca2+ channels (15)
and correlates with action potential generation (16), suggesting that
it may represent an effect equivalent to stimulation of arterial
vasomotion in vivo. We have recently shown that
AVP-stimulated Ca2+ spiking in A7r5 cells involves
phospholipase D (17) and activation of one or more protein kinase C
(PKC) isoforms (18).
It remains to be elucidated how activation of PKC ultimately produces
Ca2+ spiking. One possibility is that PKC activation leads
to membrane depolarization and consequently to activation of L-type
voltage-sensitive Ca2+ channels. We have preliminary data
that suggest that inhibition of delayed rectifier K+
channels (Kv channels) may provide the trigger for
L-type Ca2+ channel activation (16). The present study
examines the possibility that one or more tyrosine kinases may serve as
intermediary links in this signaling cascade. In particular, we focus
on the non-receptor tyrosine kinase PYK2 (proline-rich tyrosine kinase
2, also known as RAFTK or CADTK), a member of the focal adhesion kinase
(p125FAK) family, which is activated by stimuli that
increase [Ca2+]i or activate PKC in cultured rat
aortic smooth muscle cells (19-21). PYK2 has also been linked with
inhibition of delayed rectifier K+ channels in non-muscle
cells (22, 23).
Src family kinases (SFKs) and epidermal growth factor receptors (EGFR)
are tyrosine kinases that have been implicated as activators and/or
downstream mediators of PYK2 in other systems (19, 21, 24-26).
Activation of PYK2 is associated with its autophosphorylation on
tyrosine 402. This phosphotyrosine moiety may then serve as a docking
site for the SH2 domain of Src (22, 26). Another tyrosine residue in
PYK2 (Tyr-881) may also be phosphorylated and serve as a docking
site for Grb2, leading to activation of ERK1/2, members of the family
of mitogen-activated protein kinases (MAPKs) (22, 26). The roles of
SFKs and transactivation of EGFR or MAPKs in AVP-stimulated
Ca2+ spiking have not been examined previously. The results
of the present study are consistent with roles for SFKs and PYK2
activation leading to tyrosine phosphorylation of delayed rectifier
K+ channels in this novel signal transduction pathway.
However, activation of EGFR or ERK1/2 does not appear to be either
necessary or sufficient to induce Ca2+ spiking in A7r5 cells.
Materials--
Cell culture media were from Invitrogen or
MediaTech (Herndon, VA). Fura-2-AM, fura-2 pentapotassium salt,
fluo3-AM, and Pluronic F127 were from Molecular Probes, Inc. (Eugene,
OR). Monoclonal anti-PKC and anti-PYK2 antibodies and polyclonal
anti-phosphotyrosine antibodies were from Transduction Laboratories
(San Diego, CA). Monoclonal anti-Kv1.2 and
anti-phosphotyrosine (clone 4G10) and polyclonal anti-PYK2 were from
Upstate Biotechnology, Inc. (Lake Placid, NY). Polyclonal anti-Kv1.2
channel antibodies were from Chemicon (Temecula, CA). Monoclonal
anti-Src antibodies were from Oncogene Research Products (San Diego,
CA). Anti-phospho-ERK antibodies were from Promega (Madison, WI). AVP,
epidermal growth factor, salicylate, and ionomycin were from Sigma.
4 Cell Culture--
A7r5 cells were cultured as described
previously (13). Cells were subcultured onto rectangular (9 × 22-mm, number 11/2) glass coverslips or plastic tissue culture
dishes (Corning Glass). Confluent cell monolayers were used 2-5 days
after plating.
[Ca2+]i Measurements--
Essentially as
described previously (15, 18), coverslips were washed twice with
control medium (135 mM NaCl, 5.9 mM KCl, 1.5 mM CaCl2, 1.2 mM MgCl2,
11.5 mM glucose, 11.6 mM HEPES, pH 7.3) and
then incubated in the same medium with 2 µM fura-2-AM, 0.1% bovine serum albumin, and 0.02% Pluronic F127 detergent (27) for
90-120 min at room temperature (20-23 °C) in the dark. The cells
were then washed twice and incubated in the dark in control medium (or
pretreated with drugs) for 1-5 h prior to the start of the experiment.
Fura-2 fluorescence (at 510 nm) was measured in cell populations with a
PerkinElmer Life Sciences LS50B fluorescence spectrophotometer.
Background fluorescence was determined at the end of the experiment by
quenching the fura-2 fluorescence for 10-15 min in the presence of 5 µM ionomycin and 6 mM MnCl2 in Ca2+-free medium. After background fluorescence was
subtracted, the ratio of fluorescence at 340 nm excitation to that at
380 nm was calculated and calibrated in terms of
[Ca2+]i.
We found that salicylate interfered with the measurement of fura-2
fluorescence, so fluo3 was used to measure
[Ca2+]i responses in the presence of salicylate.
A7r5 cells were incubated for 1 h in the presence of 10 µM fluo3-AM, 0.1% bovine serum albumin, and 0.02%
Pluronic F127 detergent, then washed, and incubated in control medium
in the absence of fluo3-AM for at least 30 min. For these experiments,
a single excitation wavelength (505 nm) was used, and emitted
fluorescence (at 535 nm) was collected at 0.5-s intervals.
Calibration of fura-2 fluorescence in terms of
[Ca2+]i was carried out as described previously
(28) using solutions of known Ca2+ concentration to
construct a standard curve. The Ca2+ concentration of the
standard solutions was calculated using software (MaxChelator, version
6.60) that accounts for binding of Ca2+ to each constituent
of the solution. For analysis of fluorescence ratios recorded from
cells, the equation [Ca2+]i = KD· Immunoprecipitation and Western Blotting--
A7r5 cells were
grown to confluence on 100-mm tissue culture dishes (Corning Glass).
Cells were washed and incubated in control medium (see above) for
3 h at room temperature, followed by treatment for the indicated
time in control medium ± agonist. The medium was aspirated, and
0.8 ml of ice-cold lysis buffer (1% sodium deoxycholate, 0.1% SDS,
1% Triton X-100, 100 mM NaF, 10 mM sodium pyrophosphate, 1 mM EGTA, 1.5 mM
MgCl2, 10% glycerol, 150 mM NaCl, 10 µg/ml
leupeptin, 10 µg/ml aprotinin, 1 mM
Na3VO4, 50 mM HEPES, pH 7.4) was
added to the dish on ice for 10 min. Cell lysates were collected,
sonicated for 15 s, and centrifuged at 16,000 × g
for 20 min at 4 °C. The protein concentration in the supernatant was
determined using a bicinchoninic acid protein assay (Pierce), and 600 µg of protein from each sample was incubated with 3 µg of
polyclonal anti-phosphotyrosine antibody overnight at 4 °C with
rocking. 40 µl of packed protein A-Sepharose beads (Sigma) were then
added to each sample and incubated with rocking for 60 min at 4 °C.
The beads were then pelleted by centrifugation at 14,000 × g and washed three times in 500 µl of lysis buffer.
The procedure for the Kv1.2 or PYK2 immunoprecipitation was similar
except that a milder lysis buffer was used to preserve protein-protein
interactions (100 mM NaCl, 1% Nonidet P-40 (IGEPAL CA-630), 0.25% sodium deoxycholate, 30 mM sodium
pyrophosphate, 5 mM
For Western blotting, the immunoprecipitates were subjected to
SDS-PAGE, electrophoretically transferred to a nitrocellulose membrane,
and immunoblotted with the indicated antibody. After blotting, the
membrane was washed and treated with horseradish peroxidase-conjugated
secondary antibody (goat anti-mouse or anti-rabbit IgG). The
immunoreactive bands were visualized using enhanced chemiluminescence
reagents (Amersham Biosciences) exposed to Hyperfilm (Amersham
Biosciences) in the linear range of the film density. The films were
scanned, and densitometric analysis was performed with NIH image software.
A variation of these methods was used to measure phosphorylation of
ERK1/2. A7r5 cells grown on 100-mm plastic tissue culture dishes were
equilibrated for 2 h in control medium at room temperature. The
cells were then pretreated for 1 h with 2.5 µM
U-0126 or vehicle or 30 min with 20 mM salicylate or
vehicle, followed by treatment for up to 30 min with 100 pM
AVP in the presence or absence of U-0126 or 20 mM
salicylate. The cells were then lysed in 50 mM sodium
pyrophosphate, 50 mM NaF, 50 mM NaCl, 5 mM EDTA, 5 mM EGTA, 0.1 mM
NaVO4, 0.01% Triton X-100, 10 µg ml Data Analysis--
Data are expressed as mean ± S.E. for
at least n = 3 experiments and were analyzed using
InStat (Graphpad) or SigmaStat (SPSS Scientific) statistical software.
One-way repeated measures analysis of variance (ANOVA) followed by
Bonferroni's test or a Dunnett's test was used for comparisons among
multiple groups. Paired Student's t test was used to
evaluate the effects of PP2 on AVP-stimulated Ca2+ spiking.
PYK2 in A7r5 Cells--
Stimuli that activate PKC or elevate
[Ca2+]i have been found to activate the tyrosine
kinase, PYK2, leading to its autophosphorylation on a tyrosine residue.
The presence of PYK2 in A7r5 cells was confirmed by Western blot
analysis that identified a band at ~112 kDa (Fig.
1) that did not cross-react with
p125FAK antibodies (not shown). Immunoprecipitation using
anti-phosphotyrosine antibodies revealed an increase in
tyrosine-phosphorylated PYK2 in response to both PMA (1 nM)
and ionomycin (1 µM), indicating that it can be activated
by either PKC or increased [Ca2+]i in A7r5 cells
(Fig. 2).
Time-dependent Activation of PYK2 by AVP--
100
pM AVP was also found to stimulate PYK2 phosphorylation.
The time course for stimulation of tyrosine phosphorylation of PYK2 by
100 pM AVP is shown in Fig.
3, A and B. A
significant increase in tyrosine phosphorylation was detected after 2 min, followed by a further increase, which plateaued between 5 and 20 min and then declined at 30 min. The Ca2+-spiking response
to 100 pM AVP was typically delayed by several minutes (on
average 4.2 ± 0.6 min, as reported previously (18)) but is
sustained for as long as AVP is present, at least up to 1 h (18).
Treatment of A7r5 cells with PLD (2.5 units/ml, 15 min), which has been
shown previously to stimulate Ca2+ spiking in A7r5 cells
(17), also stimulated PYK2 tyrosine phosphorylation (not shown).
PKC Dependence of PYK2 Activation--
The stimulation of PYK2
tyrosine phosphorylation by 100 pM AVP was inhibited in a
concentration-dependent manner by the selective PKC
inhibitor Ro-31-8220 (Fig. 4). This drug
was shown previously to block AVP-stimulated Ca2+ spiking
(18). Similar results were obtained using another structurally unrelated PKC inhibitor, chelerythrine chloride (0.1-20
µM, not shown).
Inhibition of PYK2 Phosphorylation by Salicylate and PP2 but Not
Tyrphostin--
Salicylate has been reported recently (30) to inhibit
selectively PYK2 tyrosine phosphorylation in angiotensin II-stimulated cardiac fibroblasts. Salicylate (20 mM) inhibited
AVP-stimulated PYK2 tyrosine phosphorylation by 82% (p < 0.01, n = 3; Fig.
5A) and completely abolished
AVP-stimulated Ca2+ spiking (Fig. 5B) in A7r5
cells. In three independent paired experiments, the mean frequency of
Ca2+ spiking in cells treated with 100 pM AVP
alone was 7.8 ± 1.1 min
PP2 is a relatively selective inhibitor of SFKs (31). 10 µM PP2 completely inhibited AVP-stimulated
Ca2+ spiking, whereas its inactive analog, PP3, had no
effect (Fig. 5C). PP2 also abolished PMA-stimulated
Ca2+ spiking (not shown). AVP-stimulated tyrosine
phosphorylation of PYK2 was significantly inhibited (by 65 ± 3%,
n = 3, p < 0.05) by PP2 (Fig.
5D). SFKs have been found to associate with active PYK2 by
binding to its phosphorylated tyrosine (Tyr-402; see Refs. 22 and 26).
We examined the possibility that Src and PYK2 might become associated
following AVP treatment. Co-immunoprecipitation results are shown in
Fig. 6. A7r5 cells were treated for
varying times with 100 pM AVP followed by
immunoprecipitation of PYK2. Although PYK2 was readily detected in the
immunoprecipitates (and depleted from the supernatants), Src was not
detectable in the immunoprecipitates at any time point (but was readily
detected in the supernatants). Similar results were obtained by
immunoprecipitating Src and probing for PYK2 (not shown).
Tyrphostin Inhibition of Ca2+ Spiking--
The effects
of another tyrosine kinase inhibitor, tyrphostin A47 (TyrA47), on the
Ca2+-spiking responses to 100 pM AVP or 1 nM PMA are shown in Fig. 7
(A-F). TyrA47 (50 µM) completely abolished
the Ca2+-spiking response to both agents, whereas the
inactive analog, TyrA63 (50 µM), did not affect the
responses. However, in contrast to salicylate or PP2, neither TyrA47
nor TyrA63 prevented AVP- or PMA-stimulated tyrosine phosphorylation of
PYK2 (Fig. 7G).
Potential Downstream Effectors of PYK2--
Transactivation of EGF
receptors (EGFR) and activation of ERK1 and ERK2 MAPKs have been
implicated as downstream effectors in other PYK2-mediated cell
responses (9-22, 24, 25, 32). Activation of ERK1/2 requires dual
threonine and tyrosine phosphorylation, both catalyzed by another
highly specific kinase, MEK. EGF at concentrations ranging from 1 pM to 100 nM failed to stimulate Ca2+ spiking in A7r5 cells, whereas 50 pM AVP
elicited a robust Ca2+-spiking response in the same cells
(not shown). Despite its inability to stimulate Ca2+
spiking, EGF (10 nM) robustly activated ERK1/2 (Fig.
8A). Salicylate (20 mM) did not prevent EGF-stimulated ERK1/2 phosphorylation (Fig. 8A), whereas U-0126 (2.5 µM, a selective
MEK inhibitor) completely abolished this effect (Fig. 8B).
Phosphorylation of ERK1/2 in response to 100 pM AVP was
undetectable in 6 of 9 experiments (Fig. 8A) and U-0126 did
not inhibit AVP-stimulated Ca2+ spiking (Fig.
8C; frequency of Ca2+ spiking in response to 100 pM AVP was 3.8 ± 0.5 min
We next determined whether Kv1.2-delayed rectifier K+
channels might be a potential effector for PYK2 in the stimulation of Ca2+ spiking. Kv1.2 channels have been shown to be
tyrosine-phosphorylated by PYK2, leading to an inhibition of outward
K+ currents in Xenopus oocytes (22). We found
that, in A7r5 cells, treatment of the cells with 100 pM AVP
significantly increased tyrosine phosphorylation of the Kv1.2 channel
protein (Fig. 9A) and that
Kv1.2 channel protein co-immunoprecipitated with PYK2 (Fig.
9B). The amounts of Kv1.2 detected in the PYK2
immunoprecipitates from untreated cells were similar to those from
cells treated with 100 pM AVP in five independent
experiments (Fig. 9B and results not shown). AVP-stimulated
tyrosine phosphorylation of Kv1.2 was significantly inhibited by PP2,
Ro-31-8220, and salicylate, but not by tyrphostin A47 (% inhibition = 100, 36.9, 31.3, and 18.1, respectively; Fig.
9C).
We have identified previously (15) a novel signal transduction
pathway activated by physiological concentrations of AVP that lead to
stimulation of Ca2+ spiking in vascular smooth muscle
cells. The Ca2+ spikes are due to action potentials and are
dependent on L-type voltage-sensitive Ca2+ channels (15,
16, 33, 34). The frequency of action potential firing/Ca2+
spiking increases with increasing AVP concentration (15, 16). This
frequency-modulated response provides a potential mechanism for
fine-tuning of arterial constriction that may be important for
determining regional tissue blood supply as well as peripheral vascular resistance.
We have recently postulated (18) an essential role for one or more
PKC isoforms in the AVP-stimulated Ca2+-spiking response.
Considering the ultimate involvement of voltage-sensitive Ca2+ channels, a link between PKC and membrane potential
may be proposed. Our preliminary studies have suggested that inhibition
of voltage-gated K+ (Kv) channels may
provide the membrane depolarization necessary to trigger
Ca2+ spiking in response to AVP (16). PKC-mediated
inhibition of delayed rectifier K+ channels has been
proposed to explain angiotensin II-induced constrictor responses in
rabbit portal vein smooth muscle cells (35, 36). Salter et
al. (37) have reported that endothelin-1 causes vasoconstriction
and inhibition of delayed rectifier K+ currents in rat
pulmonary artery myocytes.
It is not clear whether these vasoconstrictor actions involve direct
serine or threonine phosphorylation of Kv channels by PKC or an indirect effect involving other signaling intermediates. An indirect effect of PKC on Kv channels has been
suggested by Huang et al. (38) who found that, in
Xenopus oocytes, activation of Gq-coupled
receptors or treatment with PMA inhibited Kv currents by a mechanism that was dependent on tyrosine phosphorylation of the channels. PYK2, a tyrosine kinase that may be activated by PKC,
was subsequently proposed to mediate the tyrosine phosphorylation and
inhibition of delayed rectifier Kv channels (22, 23)
in Xenopus or mammalian expression systems.
We have found that PYK2 is expressed in vascular smooth muscle cells
and is tyrosine-phosphorylated by stimuli that activate PKC or increase
[Ca2+]i, including AVP, which both activates PKC
and increases [Ca2+]i. AVP-stimulated PKC
activation is apparently required for PYK2 tyrosine phosphorylation
since PKC inhibitors abolish this effect. The possibility that
AVP-stimulated PYK2 tyrosine phosphorylation occurs secondarily due to
the Ca2+-spiking response can be ruled out based on the
observation that tyrphostin A47 pretreatment blocks AVP-stimulated
Ca2+ spiking (Fig. 6B) but does not prevent
tyrosine phosphorylation of PYK2 (Fig. 6G).
The initiation of Ca2+ spiking correlates temporally with
AVP-stimulated tyrosine phosphorylation of PYK2, but the
Ca2+-spiking effect is sustained for an hour or more,
whereas the tyrosine phosphorylation of PYK2 persists for only 20-30
min. AVP-stimulated translocation of PKC- Inhibition of AVP-stimulated Ca2+ spiking by three
different tyrosine kinase inhibitors (PP2, salicylate, and tyrphostin
A47) suggests that tyrosine phosphorylation is essential for this
effect. Salicylate prevents AVP-stimulated PYK2 phosphorylation and
Ca2+ spiking but not EGF-stimulated ERK1/2 activation. A
similarly selective effect of salicylate was reported recently by Wang
and Brecher (30), who found that 20 mM salicylate abolished
angiotensin II- or platelet-derived growth factor-stimulated tyrosine
phosphorylation of PYK2 without inhibiting platelet-derived growth
factor-stimulated phosphorylation of PLC- SFKs have been implicated in PYK2 signaling (21, 24-26, 32, 39) as
well as in direct tyrosine phosphorylation of Kv channels (40). A role of SFKs in AVP signal transduction is indicated
by the inhibition of Ca2+ spiking by PP2 (Fig.
5C). PP2 also inhibited PMA-stimulated Ca2+
spiking, suggesting that Src is downstream of PKC in the signal transduction cascade. Our findings are consistent with studies in other
cell systems, which have suggested that activation of Src or one of its
family members is necessary for PYK2 activation (26, 32, 39, 41, 42).
Once activated, PYK2 is believed to autophosphorylate on tyrosine 402, which then acts as a scaffold for binding of Src via its SH2 domain
(22, 26). Src may then phosphorylate other tyrosines on PYK2 such as
Tyr-881 to allow Grb2 binding and propagation of the signal to MAPKs
(22, 26). At least two recent studies (32, 41) have indicated that Src itself does not associate with PYK2, but rather another member of the
family, Yes, binds to PYK2 and is necessary for PYK2 signaling. Our
results indicate that in A7r5 cells Src and PYK2 do not
co-immunoprecipitate (Fig. 6). Additional studies will be required to
determine whether another SFK is responsible for activation of PYK2 and
perhaps also for phosphorylation of Kv1.2 channels. SFKs have been
found to act directly on L-type Ca2+ channels in other cell
systems (43), but we do not find any effect of 100 pM AVP
on L-type Ca2+ currents under voltage clamp conditions in
A7r5 cells,2 suggesting that
L-type channels are not a direct target of Src family kinases at
concentrations of AVP that stimulate Ca2+ spiking.
We found that tyrphostin A47 inhibits AVP-stimulated Ca2+
spiking but not tyrosine phosphorylation of PYK2 or of Kv1.2. This finding leads us to speculate that the target of TyrA47 may be another
signaling event that is not dependent on PYK2 activation but is
nonetheless required for stimulation of Ca2+ spiking. One
possibility may be activation of non-selective cation channels by AVP,
for which we have previous evidence (44, 45). Such channels may also
contribute to membrane depolarization in vascular smooth muscle (46)
and may be regulated by tyrosine kinases (43). Additional studies will
be required to determine whether AVP stimulates Ca2+
spiking by a combination of K+ channel inhibition (mediated
by PYK2) and activation of an additional tyrphostin A47-sensitive
pathways, perhaps leading to activation of non-selective cation channels.
Transactivation of EGFR has been implicated as a downstream mediator of
PYK2 activation in angiotensin II-stimulated vascular smooth muscle
cell hypertrophy (21, 24, 25, 32). However, we found that direct
activation of EGFR by binding of EGF did not stimulate Ca2+
spiking despite activation of ERK1/2. We also found that salicylate did
not affect EGF-stimulated ERK activation (Fig. 8A).
100 pM AVP did not detectably increase ERK1/2
phosphorylation, and the MEK inhibitor, U-0126, which completely
abolished EGF-stimulated ERK1/2 phosphorylation, did not inhibit
AVP-stimulated Ca2+ spiking. Although it did activate
ERK1/2, EGF did not stimulate Ca2+ spiking. These findings
lead us to conclude that ERK1/2 activation is neither necessary nor
sufficient for the stimulation of Ca2+ spiking by AVP.
Potassium channels play an essential role in vascular smooth muscle
cells in determining membrane potential and thereby regulating cell
excitability. Numerous studies (47-50) have found that inhibition of
delayed rectifier Kv channels leads to
vasoconstriction and/or arterial vasomotion. Tyrosine phosphorylation
of Kv channels has been linked to inhibition of
Kv currents (22, 23, 38, 40). We have found for the
first time that Kv1.2 channels in vascular smooth muscle cells exist in
a complex with PYK2 and are tyrosine-phosphorylated in response to
physiological vasoconstrictor concentrations of AVP. Kv1.2 channels
were recently found to be highly expressed in vascular smooth muscle of
resistance arteries and to have increased expression levels in tissues
from spontaneously hypertensive rats (51).
Arterial vasomotion is believed to originate within the smooth muscle
cell layer of the artery wall because it can occur independently of
endothelium (6, 8) or innervation (1, 3, 6, 52). Although AVP has been
reported to stimulate vasomotion in several arterial preparations (3,
9, 10), the biochemical mechanisms underlying this effect have not been
elucidated. What is known is that vasomotion is dependent on L-type
voltage-sensitive Ca2+ channels and that it correlates with
action potential firing in the vascular smooth muscle cells (6, 7). In
addition, drugs that inhibit delayed rectifier K+ channels
have been shown to stimulate arterial vasomotion and/or action
potential generation (8, 47-50). These observations along with the
results of our present and previous studies (15-18) lead us to
speculate that the signaling mechanisms coupling V1a
vasopressin receptors to firing of action potentials in arterial
myocytes may proceed via a novel signal transduction pathway involving phospholipase D, protein kinase C, an Src family kinase, and PYK2 (Fig.
10). According to our hypothesis, PYK2
activation triggers tyrosine phosphorylation of Kv1.2 channels, leading
to inhibition of Kv currents, membrane
depolarization, and activation of L-type voltage-sensitive
Ca2+ channels. This ultimately produces repetitive
Ca2+ spiking and arterial vasomotion.
Repetitive Ca2+ spiking might arise due to an oscillatory
signal transduction pathway that turns on and off with each spike. However, oscillations in second messenger generation or channel phosphorylation may not be necessary. Even a steady-state channel phosphorylation might produce rhythmic spiking if Kv currents oppose a pacemaker depolarization of the membrane. In this
case, inhibition of Kv currents may result in a positive pacemaker slope that allows the membrane potential to reach a
threshold potential for firing of action potentials. Once triggered to
fire, the voltage dependence of activation and time- and
voltage-dependent inactivation characteristics of the
channels involved would drive the action potential through its cycle of depolarization and repolarization. According to this simple model, following repolarization the pacemaker will kick in again and trigger
the next action potential. Increasing or decreasing the proportion of
phosphorylated Kv channels would increase or
decrease the slope of the pacemaker depolarization and thereby determine the frequency of action potential firing. The
concentration-dependent effect of AVP on Ca2+
spike frequency in A7r5 cells (15) may therefore be due to a
concentration-dependent increase in the proportion of
phosphorylated Kv channels.
We also observed that a maximal increase in spike frequency occurs at
less than nanomolar concentrations of AVP (15), when only a fraction of
the V1a vasopressin receptors are occupied. A potential
explanation for this classic "spare receptor" phenomenon is that
channel phosphorylation is limiting, i.e. the channels are
fully phosphorylated at fractional receptor occupancy. Increasing the
proportion of occupied V1a vasopressin receptors would have no further effect on this pathway, although it may still lead to
increased PLC activation and release of intracellular Ca2+ stores.
Many of the therapeutic agents currently used to treat cardiovascular
diseases such as hypertension, coronary artery disease, and angina act
directly as inhibitors of L-type voltage-sensitive Ca2+
channels or indirectly via activation of K+ channels. The
resultant vasodilatory effects and hence the therapeutic benefit of
these agents may arise in part because of opposition to the effects of
vasoconstrictor hormones such as AVP, which stimulate arterial
vasomotion by inhibition of Kv channels and
activation of L-type Ca2+ channels. Understanding the
biochemical mechanisms that regulate arterial constriction may help to
develop more effective therapies for cardiovascular diseases.
We gratefully acknowledge the technical
assistance of Ryan Reed and John Barakat.
*
This work was supported by the Eugene J. and Elsie E. Weyler
Endowment for Clinical Cardiology Research, the John and Marian Falk
Trust for Medical Research, and NHLBI Grants R01HL60164 (to K. L. B.)
and R29HL56046 (to P. A. L.) from the National Institutes of Health.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: Loyola University
Medical Center, Cardiovascular Institute, 2160 South First Ave., Maywood, IL 60153. Tel.: 708-327-2819; Fax.: 708-327-2849; E-mail: kbyron@lumc.edu.
Published, JBC Papers in Press, December 5, 2001, DOI 10.1074/jbc.M104726200
2
L. I. Brueggemann and K. L. Byron,
unpublished observations.
The abbreviations used are:
[Ca2+]i, cytosolic free Ca2+
concentration;
AVP, [Arg8]vasopressin;
fura-2-AM, fura-2
acetoxymethyl ester;
EGF, epidermal growth factor;
EGFR, epidermal
growth factor receptor;
MAPKs, mitogen-activated protein kinases;
PKC, protein kinase C;
PLC, phospholipase C;
PLD, phospholipase D;
PMA, 4
Signal Transduction of Physiological Concentrations of
Vasopressin in A7r5 Vascular Smooth Muscle Cells
A ROLE FOR PYK2 AND TYROSINE PHOSPHORYLATION OF K+
CHANNELS IN THE STIMULATION OF Ca2+ SPIKING*
§ and Loyola University Chicago, Department of
Medicine, Cardiovascular Institute, Maywood, Illinois 60153 and
¶ Department of Physiology and Biophysics, University of Alabama
at Birmingham, Birmingham, Alabama 35294
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-phorbol 12-myristate 13-acetate or
ionomycin. 100 pM AVP also induced PYK2 tyrosine phosphorylation, and this effect was inhibited by protein kinase C
inhibitors Ro-31-8220 (1-10 µM) or chelerythrine
chloride (1-20 µM). In fura-2-loaded A7r5 cells, the
stimulation of Ca2+ spiking by 100 pM AVP or 1 nM 4-phorbol 12-myristate 13-acetate was completely
blocked by PP2 (10 µM, a Src family kinase inhibitor). Salicylate (20 mM, recently identified as a PYK2 inhibitor)
and the tyrosine kinase inhibitor, tyrphostin A47 (50 µM), but not its inactive analog, tyrphostin A63, also
blocked AVP-stimulated Ca2+ spiking. PYK2 phosphorylation
was inhibited by both PP2 and salicylate, whereas tyrphostin A47 failed
to inhibit PYK2 tyrosine phosphorylation. ERK1/2 kinases did not appear
to be involved because 1) 100 pM AVP did not appreciably
increase ERK1/2 phosphorylation and U-0126 (2.5 µM) did
not inhibit AVP-stimulated Ca2+ spiking; and 2) epidermal
growth factor (10 nM) robustly stimulated ERK1/2
phosphorylation but did not induce Ca2+ spiking. Delayed
rectifier K+ channels may mediate the PYK2 activity because
Kv1.2 channel protein co-immunoprecipitated with PYK2 and tyrosine
phosphorylation of Kv1.2 was stimulated by AVP and inhibited by
Ro-31-8220, PP2, and salicylate but not tyrphostin A47. Our findings
are consistent with a role for PYK2 and phosphorylation of
K+ channels in the stimulation of Ca2+ spiking
by physiological concentrations of AVP.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-Phorbol 12-myristate 13-acetate, chelerythrine chloride,
tyrphostins A47 and A63, and Ro-31-8220 were from Calbiochem. U-0126
was from Biomol (Plymouth Meeting, PA). Pefabloc SC" was
from Roche Molecular Biochemicals.
·((r 
Rmin)/(Rmax r)) (29) was fit to the standard curve (using SigmaPlot®
software, SPSS Inc., Chicago, IL) and used to convert ratios
(r) into [Ca2+]i. In situ
calibration of fura-2 fluorescence by direct determination of minimum
and maximum ratios (Rmin and
Rmax, respectively (29)) from within cells
yields similar calibrated values. Traces shown are representative of at
least three similar experiments.
-glycerophosphate, 10 µg/ml
leupeptin, 0.5 mM Pefabloc, 10 µg/ml aprotinin, 500 µM Na3VO4, 20 mM
HEPES, pH 7.4). 700 µg of cell lysates were incubated with 4 µg of
monoclonal Kv1.2 antibodies or 5 µg of polyclonal anti-PYK2
antibodies overnight at 4 °C, and immune complexes were collected by
incubation with 40 µl of packed protein G-agarose beads.
1
aprotinin, 10 µg ml1 leupeptin, 0.5 mM
Pefabloc, 10 mM HEPES, pH 7.4, scraped off the dish, and
centrifuged at 12,000 × g at 4 °C for 10 min. The supernatant (a volume containing 40 µg of protein) was subjected to
SDS-PAGE, electrophoretically transferred to a nitrocellulose membrane,
and immunoblotted with polyclonal antibodies against phospho-ERK
proteins (Promega, Madison, WI; 1:10,000 dilution). The membranes were
re-probed for total ERK protein using polyclonal anti-ERK antibodies
(Upstate Biotechnology, Inc.).
RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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Fig. 1.
PYK2 expression in A7r5 cells. Western
blot analysis reveals the presence of a single PYK2 immunoreactive band
at ~112 kDa in A7r5 vascular smooth muscle cells (VSMC).
PC12 cells (22) and rat aortic smooth muscle cells (RASM
(19)) were used as positive controls.
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Fig. 2.
PYK2 activation by PMA or ionomycin.
Tyrosine phosphorylation of PYK2 was assessed by immunoprecipitation
(IP) with anti-phosphotyrosine (pTyr) antibodies
followed by immunoblotting with anti-PYK2. Left panel shows
a representative immunoblot from cells treated with PMA (1 nM, 10 min) or ionomycin (Iono, 1 µM, 10 min); right panel shows a quantitative
densitometric analysis from five experiments (mean ± S.E.).
Results are presented as a fold increase above control, which was set
at 1. A one-way repeated measures ANOVA was performed. * indicates
significant difference from control, p < 0.01.
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Fig. 3.
Time-dependent stimulation of
PYK2 by AVP. A, A7r5 cells were treated with 100 pM AVP for 0-30 min. Tyrosine phosphorylation of PYK2 was
assessed by immunoprecipitation (IP) with
anti-phosphotyrosine (pTyr) and immunoblotting with
anti-PYK2 antibodies. A representative Western blot is shown in the
top panel and cumulative results (mean ± S.E.) from
densitometric analysis of six blots are shown in the lower
panel. Data are presented as fold increase above control
(time = 0), which was set to 1. * denotes significant difference
from control (p < 0.01). B, a
similar increase in PYK2 activity following 20 min of exposure to 100 pM AVP was detected by immunoprecipitation with PYK2
antibodies followed by immunoblotting with anti-phosphotyrosine
antibodies.
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Fig. 4.
Concentration-dependent
inhibition of tyrosine phosphorylation of PYK2 by the PKC inhibitor
Ro-31-8220. A7r5 cells were pretreated for 1 h with varying
concentrations of Ro-31-8220 followed by treatment for 10 min with 100 pM AVP. Cell lysates were immunoprecipitated
(IP) with anti-phosphotyrosine (pTyr) antibodies
and then immunoblotted with anti-PYK2. A representative Western blot is
shown in the top panel, and cumulative results (mean ± S.E.) from densitometric analysis of six blots are shown in the
lower panel. Data are presented as fold increase above
control, which was set to 1. * denotes significant difference from
control (p < 0.05). ** denotes significant difference
from cells treated with AVP alone (p < 0.05). # denotes significant difference from cells treated with AVP alone
(p < 0.001).
1, whereas no spiking was
observed in cells treated with 100 pM AVP in the presence
of 20 mM salicylate. This concentration of salicylate did
not prevent 100 nM AVP-stimulated release of
Ca2+ from intracellular stores, the
[Ca2+]i response to a high external
[K+] solution (not shown), or EGF-stimulated ERK1/2
phosphorylation (see below).
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Fig. 5.
Salicylate and PP2 inhibit AVP-stimulated
PYK2 activation and Ca2+ spiking. A, A7r5
cells were pretreated for 30 min with 20 mM salicylate or
vehicle followed by treatment for 10 min with 100 pM AVP. A
representative immunoblot (top) and cumulative data from
three experiments (bottom) are presented. * denotes
significant difference from control (p < 0.01, one-way
repeated measures ANOVA). 
denotes significant difference from 100 pM AVP alone (p < 0.01, one-way repeated
measures ANOVA). B, [Ca2+]i responses
in fluo3-loaded A7r5 cells are represented as fluorescence
(F) relative to starting fluorescence
(F0); top panel shows a control
response to 100 pM AVP; bottom panel shows a
response to AVP in the presence of 20 mM salicylate
(following a 30-min pretreatment with salicylate alone). C,
A7r5 cells were treated with 75 or 100 pM AVP in the
presence or absence of 10 µM PP2 or 10 µM
PP3 (PP2 or PP3 was present in all solutions beginning 30 min before
recording of fura-2 fluorescence). The frequency of Ca2+
spiking was measured during the final 5 min of a 20-min treatment with
AVP. Results from four experiments are summarized showing that PP2
significantly inhibited AVP-stimulated Ca2+ spiking
(p < 0.05, paired Student's t test)
compared with cells treated with AVP alone (Control). PP3
had no effect. D, immunoblot analysis of phosphotyrosine
immunoprecipitates (IP) blotted for PYK2. A7r5 cells were
treated for 20 min with 100 pM AVP in the presence or
absence of 10 µM PP2. PP2 significantly inhibited
AVP-stimulated tyrosine phosphorylation of PYK2 (*, significantly
different from control, p < 0.01; , significantly
different from AVP alone, p < 0.05, 65 ± 3%
inhibition, n = 3).
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Fig. 6.
Src does not co-immunoprecipitate with
PYK2. A7r5 cells were treated with 100 pM AVP for
varying times. Cell lysates were immunoprecipitated with polyclonal
anti-PYK2 antibodies. Both the immunoprecipitates and the supernatants
from each sample were separated by SDS-PAGE, transferred to
nitrocellulose, and blotted for PYK2 (upper half of
membrane) or Src (lower half of membranes). A representative
immunoblot is shown, indicating that for each of the samples (control
and AVP-treated) PYK2 is depleted from the supernatants, whereas Src
remains in the supernatants and is undetectable in the
immunoprecipitates. Rat brain lysates (5 µg of protein) were run in
lane 1 for both supernatants and immunoprecipitates as a
positive control for PYK2 and Src. Results are representative of five
experiments.
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Fig. 7.
Tyrphostin A47 inhibits AVP- or
PMA-stimulated Ca2+ spiking in A7r5 cells but does not
inhibit PYK2 activation. Fura-2-loaded A7r5 cell monolayers were
treated with 100 pM AVP (shaded box,
A-C) or 1 nM PMA (shaded box,
D-F). A and D, control
responses; B and E, responses after
pretreatment for 1 h with 50 µM TyrA47;
C and F, responses after pretreatment for 1 h with TyrA63. G, A7r5 cells were pretreated for 1 h with 50 µM TyrA47, 50 µM TyrA63, or
vehicle followed by treatment for 10 min in the presence or absence of
1 nM PMA or 100 pM AVP. A representative
immunoblot (top) and cumulative data from at least four
experiments (bottom) are presented. * denotes significant
difference from control (p < 0.01, one-way repeated
measures ANOVA). IP, immunoprecipitation.
1 in the
absence of U-0126 and 5.3 ± 0.9 min1 in the
presence of U-0126, p > 0.1, n = 4).
These results suggest that activation of EGF receptors or ERK1/2 MAPKs
is neither necessary nor sufficient to elicit the
Ca2+-spiking effect.
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Fig. 8.
ERK activation by EGF but not AVP.
A, representative Western blot showing phosphorylation of
ERK1 and ERK2 in A7r5 cells treated with 10 nM EGF or 100 pM AVP for 30 min in the presence or absence of 20 mM salicylate (following a 30-min pretreatment with
salicylate alone). ERK1/2 phosphorylation was detected by Western blot
analysis using phospho-ERK antibodies (see "Experimental
Procedures"). The same blots were re-probed for total ERK
(lower panels) to verify uniform loading. B,
representative Western blot showing phosphorylation of ERK1 and ERK2 in
A7r5 cells pretreated for 1 h with vehicle or 2.5 µM
U-0126 followed by treatment for 30 min with 10 nM EGF.
ERK1/2 phosphorylation was detected by Western blot analysis using
phospho-ERK antibodies. C, fura-2-loaded A7r5 cells were
pretreated with vehicle followed by treatment with 100 pM
AVP (top panel) or pretreated for 1 h with 2.5 µM U-0126 followed by treatment with 100 pM
AVP (lower panel). All results shown are representative of
at least 3-6 similar experiments.
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Fig. 9.
Tyrosine phosphorylation of Kv1.2-delayed
rectifier K+ channel and co-immunoprecipitation of Kv1.2
with PYK2. A, A7r5 cells were treated with 100 pM AVP for 10-20 min. Tyrosine phosphorylation of Kv1.2
was assessed by immunoprecipitation (IP) with monoclonal
anti-Kv1.2 antibodies and immunoblotting with monoclonal
anti-phosphotyrosine (pTyr) antibodies. A representative
Western blot is shown in the top left panel and cumulative
results (mean ± S.E.) from densitometric analysis of 6-8 blots are shown in
the lower panel. Data are presented as fold increase above
control (time = 0), which was set to 1. * denotes significant
difference from control (p < 0.05). B,
association between PYK2 and Kv1.2 was assessed by immunoprecipitation
with monoclonal anti-PYK2 antibodies followed by immunoblotting with
polyclonal Kv1.2 antibodies. A representative Western blot is shown;
similar results were obtained in five independent experiments.
C, tyrosine phosphorylation of Kv1.2 was evaluated as in
A in A7r5 cells treated for 10 min with 100 pM
AVP in the presence or absence of 20 mM salicylate (30 min
pretreatment), 10 µM Ro-31-8220 (30 min pretreatment), 50 µM tyrphostin A47 (3 h pretreatment), or 10 µM PP2 (30 min pretreatment). A representative immunoblot
(top) and cumulative data from 3 to 5 experiments
(bottom) are presented. *, p < 0.01, versus control. , p < 0.05 versus AVP. , p < 0.01 versus
AVP.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
, -
, and -
isoforms
from cytosolic to membrane compartments are also initiated over a time frame of 1-5 min, but this redistribution is transient for
PKC- and - isoforms, whereas PKC- translocation
persists for up to 30 min (18). The pattern of PKC- translocation is
most temporally similar to PYK2 tyrosine phosphorylation, allowing for
some discrepancy due to differences in assay conditions and sensitivity
of detection. The explanation for sustained Ca2+ spiking
despite only transient tyrosine phosphorylation of PYK2 may be that a
signal generated as a result of PYK2 activation persists after PYK2
becomes dephosphorylated.
or angiotensin
II-stimulated phosphorylation of EGFR in cardiac fibroblasts.
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Fig. 10.
Hypothetical signal transduction
pathway for AVP-stimulated Ca2+ spiking in vascular smooth
muscle cells. A schematic diagram is shown illustrating a
hypothetical pathway whereby binding of physiological concentrations of
AVP (10-100 pM) to V1a vasopressin receptors
activates a cascade of events including activation of PLD, PKC, an Src
family kinase, and PYK2. PYK2 activation leads to tyrosine
phosphorylation and the consequent inhibition of current through
delayed rectifier K+ channels (Kv). This
results in membrane depolarization and firing of action potentials
involving Ca2+ influx via L-type voltage-sensitive
Ca2+ channels (CaL). Such action potentials
would be expected to produce rhythmic vasomotion in resistance
arteries, leading to an increase in peripheral vascular resistance.
Nanomolar concentrations of AVP activate PLC and the release of
Ca2+ from the sarcoplasmic reticulum (SR). The
abbreviations used are: DAG, diacylglycerol;
IP3, inositol 1,4,5-trisphosphate;
PA, phosphatidic acid; PC, phosphatidylcholine;
PIP2, phosphatidylinositol 4,5-bisphosphate;
V1a, V1a vasopressin receptors.
ACKNOWLEDGEMENTS
FOOTNOTES
ABBREVIATIONS
-phorbol 12-myristate 13-acetate;
PYK2, proline-rich tyrosine
kinase 2;
SFKs, Src family kinases;
TyrA47, tyrphostin A47;
TyrA63, tyrphostin A63;
ERK, extracellular signal-regulated kinase;
ANOVA, analysis of variance.
REFERENCES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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L. I. Brueggemann, C. J. Moran, J. A. Barakat, J. Z. Yeh, L. L. Cribbs, and K. L. Byron Vasopressin stimulates action potential firing by protein kinase C-dependent inhibition of KCNQ5 in A7r5 rat aortic smooth muscle cells Am J Physiol Heart Circ Physiol, March 1, 2007; 292(3): H1352 - H1363. [Abstract] [Full Text] [PDF]
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 O. Levy and Y. Granot Arginine-Vasopressin Activates the JAK-STAT Pathway in Vascular Smooth Muscle Cells J. Biol. Chem., June 9, 2006; 281(23): 15597 - 15604. [Abstract] [Full Text] [PDF]
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 L. I. Brueggemann, D. R. Markun, K. K. Henderson, L. L. Cribbs, and K. L. Byron Pharmacological and Electrophysiological Characterization of Store-Operated Currents and Capacitative Ca2+ Entry in Vascular Smooth Muscle Cells J. Pharmacol. Exp. Ther., May 1, 2006; 317(2): 488 - 499. [Abstract] [Full Text] [PDF]
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 T. Florio, S. Casagrande, F. Diana, A. Bajetto, C. Porcile, G. Zona, S. Thellung, S. Arena, A. Pattarozzi, A. Corsaro, et al. Chemokine Stromal Cell-Derived Factor 1{alpha} Induces Proliferation and Growth Hormone Release in GH4C1 Rat Pituitary Adenoma Cell Line through Multiple Intracellular Signals Mol. Pharmacol., February 1, 2006; 69(2): 539 - 546. [Abstract] [Full Text] [PDF]
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 D. I. Palen, S. Belmadani, P. A. Lucchesi, and K. Matrougui Role of SHP-1, Kv.1.2, and cGMP in nitric oxide-induced ERK1/2 MAP kinase dephosphorylation in rat vascular smooth muscle cells Cardiovasc Res, November 1, 2005; 68(2): 268 - 277. [Abstract] [Full Text] [PDF]
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R. Zhou, L. Liu, and D. Hu Involvement of BKCa {alpha} subunit tyrosine phosphorylation in vascular hyporesponsiveness of superior mesenteric artery following hemorrhagic shock in rats Cardiovasc Res, November 1, 2005; 68(2): 327 - 335. [Abstract] [Full Text] [PDF]
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 H. Sekimoto, J. Eipper-Mains, S. Pond-Tor, and C. M. Boney {alpha}v{beta}3 Integrins and Pyk2 Mediate Insulin-Like Growth Factor I Activation of Src and Mitogen-Activated Protein Kinase in 3T3-L1 Cells Mol. Endocrinol., July 1, 2005; 19(7): 1859 - 1867. [Abstract] [Full Text] [PDF]
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J. L. Dyer, Y. Liu, I. P. de la Huerga, and C. W. Taylor Long Lasting Inhibition of Adenylyl Cyclase Selectively Mediated by Inositol 1,4,5-Trisphosphate-evoked Calcium Release J. Biol. Chem., March 11, 2005; 280(10): 8936 - 8944. [Abstract] [Full Text] [PDF]
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L. I. Brueggemann, B. L. Martin, J. Barakat, K. L. Byron, and L. L. Cribbs Low voltage-activated calcium channels in vascular smooth muscle: T-type channels and AVP-stimulated calcium spiking Am J Physiol Heart Circ Physiol, February 1, 2005; 288(2): H923 - H935. [Abstract] [Full Text] [PDF]
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G. Vazquez, B. J. Wedel, B. T. Kawasaki, G. St. J. Bird, and J. W. Putney Jr. Obligatory Role of Src Kinase in the Signaling Mechanism for TRPC3 Cation Channels J. Biol. Chem., September 24, 2004; 279(39): 40521 - 40528. [Abstract] [Full Text] [PDF]
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