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The Journal of Neuroscience, August 15, 1998, 18(16):6081-6092
The cAMP Transduction Cascade Mediates the Prostaglandin
E2 Enhancement of the Capsaicin-Elicited Current in Rat
Sensory Neurons: Whole-Cell and Single-Channel Studies
John C.
Lopshire1 and
Grant D.
Nicol2
1 Medical Neurobiology Program and
2 Department of Pharmacology and Toxicology, Indiana
University School of Medicine, Indianapolis, Indiana 46202
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ABSTRACT |
Treatment with proinflammatory prostaglandin E2
(PGE2) produced a transient sensitization of
whole-cell currents elicited by the vanilloid capsaicin. The
intracellular signaling pathways that mediate the initiation of this
PGE2-induced sensitization of the capsaicin-elicited
current in rat sensory neurons are not well established. Treatment with
either forskolin (100 nM to 10 µM) or
membrane-permeant analogs of cAMP, 8-bromo-cAMP (8-Br-cAMP) and
chlorphenylthio-cAMP (10 µM to 1 mM),
transiently sensitized neuronal responses elicited by capsaicin in a
manner analogous to that produced by PGE2. The duration of
sensitization was lengthened with increasing concentrations of
forskolin; however, higher concentrations of 8-Br-cAMP or
chlorphenylthio-cAMP led to a shortening of sensitization. The inactive
analog of forskolin, dideoxy-forskolin, had no effect on capsaicin
responses. Inclusion of the inhibitor of protein kinase A in the
recording pipette completely suppressed the sensitization produced by
PGE2 or forskolin. In recordings from membrane patches in
the cell-attached configuration, the bath application of capsaicin evoked single-channel currents in which the level of channel activity was concentration-dependent and had an EC50 of 1.4 µM. These single-channel currents evoked by capsaicin
exhibited an apparent reversal potential of +4 mV and were blocked by
the capsaicin antagonist capsazepine. Exposure of the sensory neuron to
either PGE2 or forskolin produced a large and transient
increase in the mean channel activity (NPo) elicited
by capsaicin, although the unitary conductance remained unaltered.
Taken together, these observations suggest that modulation of the
capsaicin-gated channel by the cAMP-protein kinase A signaling pathway
enhanced the gating of these channels and consequently resulted in the
sensitization of the whole-cell currents.
Key words:
prostaglandin E2; cAMP; protein kinase
A; capsaicin; sensitization; neuronal excitability
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INTRODUCTION |
A specific population of mammalian
sensory neurons can be distinguished by their excitatory response to
the vanilloid capsaicin. These capsaicin-sensitive A- and C fibers
are believed to be involved in the perception and signaling of
nociceptive information (for review, see Holzer, 1991 ; Szallasi and
Blumberg, 1996). Indeed, the intradermal injection of capsaicin in
human subjects provokes intense pain (LaMotte et al., 1991, 1992). In
responsive sensory neurons, capsaicin generates an inward current that
results in the depolarization of the neuron (Heyman and Rang, 1985;
Marsh et al., 1987; Bevan and Forbes, 1988; Bevan and Szolcsanyi,
1990). This inward current results from the opening of a nonselective cationic channel that is largely permeable to Na+
and Ca2+ (Marsh et al., 1987; Wood et al., 1988;
Bevan and Szolcsanyi, 1990; Oh et al., 1996a). Recently, the capsaicin
receptor has been cloned, and the expressed protein has
electrophysiological properties that are quite similar to the currents
conducted by the native receptor (Caterina et al., 1997). Although
there is considerable information concerning the excitatory properties of capsaicin, the exact role of this receptor in nociception remains to
be elucidated. Similarly, little is known about the capacities of
intracellular signaling pathways to modulate either the
capsaicin-elicited whole-cell current or the activity of the
capsaicin-gated ion channel.
The sensitivity or excitability of mammalian sensory neurons in
response to various forms of noxious stimulation, such as mechanical
pressure or chemical agents, can be facilitated by exposure to
proinflammatory prostaglandins (Higgs et al., 1984; Foreman, 1987;
Salmon and Higgs, 1987). In behavioral studies, sensitization is
manifested as a heightened perception of pain (for review, see
Handwerker and Kobal 1993; Kress and Reeh, 1996). Furthermore, in
electrophysiological recordings obtained from isolated sensory neurons
grown in culture, treatment with prostaglandin E2
(PGE2) enhances the number of action potentials
generated by exposure to either elevated levels of potassium
(Baccaglini and Hogan, 1983) or focally applied bradykinin (Nicol and
Cui, 1994). The increased excitability results, in part, from the
modulation of specific membrane currents. Treatment with
PGE2 results in the facilitation of a
tetrodotoxin-resistant sodium current (Gold et al., 1996; England et
al., 1996) and the suppression of a potassium current (Nicol et al.,
1997).
Recent studies indicate that this PGE2-induced
sensitization results from activation of the cAMP transduction
cascade. Experimental findings that support this notion are threefold.
First, PGE2 increases intracellular levels of cAMP in
sensory neurons (Hingtgen et al., 1995). Second, the exogenous
application of membrane-permeant analogs of cAMP mimics the sensitizing
effects of PGE2 in studies examining either the excitatory
response elicited by bradykinin (Cui and Nicol, 1995) or the
release of neuropeptides from sensory neurons (Hingtgen et al., 1995).
Last, inhibition of the cAMP-dependent protein kinase A (PKA) blocks
sensitization by PGE2 (Cui and Nicol, 1995). These studies
indicate that the cAMP transduction cascade plays a critical role in
the PGE2-induced sensitization; however, the role of the
cAMP transduction pathway in mediating the onset of sensitization and
its capacity to modulate the excitatory response to capsaicin remain to
be defined. Therefore, in this study we examined the capacity of both
the proinflammatory prostaglandin PGE2 and activators of
the cAMP transduction cascade to sensitize the response to capsaicin
recorded from rat sensory neurons grown in culture. Our findings
demonstrate that PGE2, through activation of the
cAMP-PKA signaling pathway, increases the whole-cell currents elicited
by capsaicin and that this enhancement results from the increased
activity of the capsaicin-gated ion channel.
Portions of this work have been published previously (Lopshire and
Nicol, 1997a).
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MATERIALS AND METHODS |
Isolation and culture of embryonic rat sensory
neurons. The procedures used for the isolation and maintenance of
embryonic rat sensory neurons have been described previously (Vasko et
al., 1994). Briefly, pregnant Harlan Sprague Dawley (Indianapolis, IN)
rats were rendered unconscious by exposure to CO2 and
killed by cervical dislocation. The dorsal root ganglia (DRG) were
removed from the embryos (days 15-17 of gestation) and placed in a
dish containing sterile calcium-free, magnesium-free HBSS at 4°C. The DRG were incubated in HBSS containing 0.025% trypsin for 30 min at
37°C. The digestion was terminated with the addition of 0.25% trypsin inhibitor. The ganglia were washed once with HBSS, centrifuged, and resuspended in growth medium (DMEM; Life Technologies, Grand Island, NY) supplemented with 2 mM glutamine, 50 µg/ml
penicillin and streptomycin, 10% (v/v) heat-inactivated fetal bovine
serum, 50 µM 5-fluoro-2'-deoxyuridine, 150 µM uridine, and 250 ng/ml 7S nerve growth factor (Harlan
Bioproducts, Indianapolis, IN). Individual cells were obtained by
dissociation with a fire-polished pipette. Approximately 300,000 cells
were plated on a collagen-coated culture dish (35 mm) containing small
plastic coverslips. Cells were maintained at 37°C in a 5%
CO2 atmosphere, and the media were changed every 2 d.
All procedures were approved by the Animal Care and Use Committee at
Indiana University School of Medicine.
Electrophysiology. The procedures for whole-cell patch-clamp
recording from rat sensory neurons have been described previously (Lopshire and Nicol, 1997b). Briefly, a coverslip of sensory neurons (typically after 4-5 d in culture) was placed in a recording chamber where the neurons were superfused with normal Ringer's solution of the
following composition (in mM): 140 NaCl, 5 KCl, 2 CaCl2, 1 MgCl2, 10 HEPES, and 10 glucose, pH 7.4, with NaOH. Small-diameter sensory neurons were
selected for these recordings. Membrane currents or voltages were
recorded with a List EP-7 patch-clamp amplifier (List Electronic,
Darmstadt, Germany) using the whole-cell patch-clamp technique (Hamill
et al., 1981). Recording pipettes were pulled from borosilicate glass
and typically had resistances of 2-4 M when filled with the
following solution (in mM): 140 KCl, 5 MgCl2, 4 Na2 ATP, 0.3 Na3
GTP, 2.5 CaCl2, 5 EGTA (calculated free calcium concentration of ~150 nM), and 10 HEPES, pH 7.2, with
KOH. After establishing the whole-cell configuration and allowing a
5-10 min equilibration period, the cell capacitance was compensated by
the nulling circuitry of the amplifier. The series resistance was
compensated (average value, 38.2 ± 1.5%), which yielded
uncompensated series resistances that ranged from 2.2 to 7.9 M
(average value, 3.7 ± 0.4 M). The membrane was voltage-clamped
at  60 mV, which is close to the normal resting potential of this
neuronal population (Nicol and Cui, 1994). The whole-cell currents
evoked by capsaicin were filtered at 3 kHz and sampled at 500 Hz using
the Fetchex program of pClamp 6.0.3 (Axon Instruments, Foster City,
CA). In those experiments examining inhibition of PKA, the recording
pipettes were backfilled with the normal internal solution containing
20 µM PKI14-24. Before any recording was
initiated, a period of 10 min was used to permit the equilibration of
PKI between the pipette and the cytoplasm of the neuron.
For the experiments examining single-channel activities, recording
pipettes were coated with Sylgard (Dow Corning, Midland, MI) and
heat-polished with a custom-built microforge. The pipette resistance
was typically 3-5 M after filling with a low-calcium external
solution of the following composition (in mM): 140 NaCl, 5 KCl, 10 HEPES, 10 glucose, 2 MgCl2, 2 CaCl2, and 3.5 EGTA (calculated free calcium
concentration of ~150 nM), pH 7.4, with NaOH. The low-calcium external solution was used to superfuse the neurons. Single-channel currents were recorded using the cell-attached patch-clamp technique (Hamill et al., 1981). Currents evoked by capsaicin were filtered at 1 kHz using an eight-pole Bessel filter (Frequency Devices, Haverhill, MA), digitized at 5 kHz using the Fetchex program of pClamp, and stored in a personal computer. The
traces of single-channel activity shown in the figures were filtered
digitally at 500 Hz.
Capsaicin was administered to the neuron by either bath application or
focal application via a large-bore pipette (5-10 µm tip
diameter and positioned within 20-40 µm of the cell body) containing
the desired external solution, the appropriate concentration of
capsaicin, and 1 mM trypan blue dye. During continuous
superfusion of the bath, positive pressure (1-2 sec duration for the
whole-cell experiments and continuous for the single-channel
experiments) was applied to the focal pipette, resulting in the
delivery of capsaicin to the cell body. The trypan blue allowed for
visual confirmation of drug delivery. The focal application of trypan blue alone had no effect on these neurons (Nicol and Cui, 1994; Lopshire and Nicol, 1997b). Two control responses to capsaicin, separated by ~2 min, were obtained before the application of
sensitizing agents. The response to capsaicin then was tested at the
subsequent times indicated in each figure. To avoid desensitization,
responses to capsaicin were obtained from only a single neuron on each
coverslip.
Unless otherwise noted, all voltages are expressed as the membrane
voltage, i.e., inside the cell relative to the outside for the
whole-cell recordings or the negative of the pipette potential for the
single-channel recordings. To determine the contribution of the resting
membrane potential to the total membrane voltage of the cell-attached
patch, the effects of a continuous exposure to capsaicin on the
membrane potential were examined. Using the whole-cell configuration in
current-clamp mode, the bath application of 1 µM
capsaicin in a low-calcium Ringer's solution depolarized the membrane
from 54 ± 1 to 5 ± 1 mV (n = 5) with an
average onset latency of 19 ± 2 sec (expressed as the time
elapsed from initiation of capsaicin exposure to steady-state
depolarization; see Fig. 7B, inset, for a
representative trace). This depolarization was maintained; after 4 and
20 min of continuous exposure to capsaicin the potentials were 4 ± 1 and 5 ± 1 mV, respectively. Because the voltage recorded
under these conditions remained near a value of 0 mV, the small
contribution of the resting membrane potential was neglected. The
voltages indicated in the single-channel measurements are reported as
the negative of the applied pipette voltage.
For the whole-cell experiments, all neurons were required to maintain a
zero-current potential more hyperpolarized than 45 mV for 4-5 min
after establishing the whole-cell configuration, and the peak
amplitudes of the two control currents elicited by capsaicin had to be
within 10% of their mean value. If a neuron failed to satisfy these
criteria, the recording was terminated. Depolarizing currents are shown
as downward. All experiments were performed at room temperature
(~21°C).
Analysis. All values are reported as the mean ± SEM.
In the whole-cell experiments, the time course of sensitization for
each neuron was characterized by two parameters, the time to peak
sensitization and the time for sensitization to return to half-maximal
values (t1/2MAX). The values from
individual neurons were then averaged to obtain the mean ± SEM
for each experimental treatment. The time to peak sensitization is
defined as the time elapsed from the delivery of sensitizing agent to
the maximal sensitization, and the
t1/2MAX is defined as the time elapsed
from the maximally sensitized response to the point at which
sensitization has returned to halfway between the peak and control
values.
For the analysis of single-channel recordings, all-points
amplitude histograms and events lists were constructed using the Fetchan program of pClamp. The all-points amplitude histograms were fit
by Gaussian functions using the pStat program of pClamp. Channel
openings were detected using the half-amplitude detection algorithm. A
minimum estimate of the number of channels was obtained from the
maximum number of overlapping events observed in each patch.
NPo was calculated as follows:
|
(1)
|
where i is the level of the open channel,
N is the maximum number of overlapping events observed in
that recording (assumed to be the maximum number of open channels), and
Poi is the probability of i channels
being open as reported by Fetchan. The total time of the recording was
obtained from the events list and was typically ~40 sec.
To determine the dependence of the relative NPo of the
capsaicin-gated channel on membrane potential, these results were
fitted by the Boltzmann relation:
![<UP>Relative</UP> NP<SUB><UP>o</UP></SUB>=1/[1+<UP>exp</UP>(<UP>V<SUB>m</SUB></UP>−<UP>V</UP><SUB>0.5</SUB>)/k]](/content/vol18/issue16/fulltext/6081/img002.gif)
|
(2)
|
where Vm is the membrane potential, V0.5
is the voltage at half-maximal activation, and k is a
steepness factor.
The concentration-response relation was fitted with a ligand-binding
isotherm of the following form:
![<UP>CAP<SUB>RESP</SUB></UP>=<UP>CAP<SUB>MAX</SUB></UP>/(1+([<UP>CAP</UP>]<SUB>0.5</SUB>/[<UP>CAP</UP>])<SUP><UP>n</UP></SUP>)](/content/vol18/issue16/fulltext/6081/img003.gif)
|
(3)
|
where CAPRESP is NPo at the test
concentration, CAPMAX is the maximum NPo
elicited by capsaicin, CAP0.5 is the concentration of
capsaicin that produces a half-maximal response, CAP is the test
concentration of capsaicin, and n is a steepness factor. Statistical
differences were determined using a one-way ANOVA with a Student
Newman-Keuls post hoc test. Values of
p < 0.05 were judged to be statistically
significant.
Chemicals. Prostaglandins were obtained from Cayman Chemical
Co. (Ann Arbor, MI). Protein kinase A inhibitor 14-24 amide
(PKI14-24) was obtained from Peninsula Laboratories, Inc.
(Belmont, CA). All other chemicals were obtained from Sigma (St. Louis,
MO). Prostaglandins, capsaicin, forskolin, and dideoxyforskolin were first dissolved in methyl-2-pyrolidinone (HPLC grade; Aldrich, Milwaukee, WI) and subsequently diluted in the appropriate solution to
the desired concentration. The concentrations of free
Ca2+ were calculated from the binding constants
described by Caldwell (1970).
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RESULTS |
Prostaglandin E2 and forskolin transiently sensitize
sensory neurons to capsaicin excitation
The focal application of capsaicin evoked an inward current when
applied to small-diameter sensory neurons voltage-clamped at 60 mV in
the whole-cell configuration. The peak amplitude of the
capsaicin-elicited current (ICAP) was
increased transiently after treatment with PGE2. Control
and experimental responses after PGE2 treatment obtained
from a representative neuron are shown in Figure
1A. The left
trace illustrates the current response to a 2 sec
application of 100 nM capsaicin. This concentration of
capsaicin was used in all whole-cell experiments because it is slightly
less than the EC50 (156 nM) established for the
whole-cell current evoked by capsaicin in these cultured sensory
neurons (Lopshire and Nicol, 1997b). In this neuron, the peak amplitude of the control response was 240 pA. After a 10 min exposure to 1 µM PGE2, the amplitude of
ICAP was increased to 822 pA, a 3.4-fold increase. After a 25 min exposure to PGE2, the
transient nature of the PGE2-induced sensitization was
evident. In the continued presence of PGE2,
ICAP was reduced to 246 pA and was similar to the control response. Another series of experiments examined the notion
that the PGE2-induced increase in the amplitude of
ICAP might result from an acceleration of the
response kinetics to these brief applications of capsaicin. Capsaicin
(100 nM) was applied focally to the neuron to obtain a
response that reached a stable plateau; the application was then
continued for an additional 2 sec. In six neurons, the average times to
peak for the two control responses were 6.6 ± 0.9 and 6.2 ± 0.4 sec (peak amplitudes of 109 ± 31 and 112 ± 29 pA,
respectively) in which the average times of capsaicin exposure were
8.7 ± 0.9 and 8.8 ± 0.5 sec, respectively. Using this
stimulus protocol, treatment with 1 µM PGE2
significantly enhanced ICAP by 2.2 ± 0.3-fold (range, 1.5 to 3.1-fold; data not shown). The time course of
sensitization was similar to that shown in Figure 1A
for the shorter exposures to capsaicin in which the maximal
sensitization occurred after a 10 min treatment with PGE2.
These results corroborate our previous observations in which treatment
of sensory neurons with PGE2 produced a transient increase in the amplitude of ICAP. Although
ICAP was enhanced, PGE2 had no
significant effect on the holding current. In those experiments using
both short and long capsaicin exposures, the average holding current
under control conditions was 55 ± 11 pA (n = 15) compared with 71 ± 17 pA (n = 15) after a
10 min exposure to 1 µM PGE2 (the time of
peak sensitization). In the absence of PGE2, the repeated application of 100 nM capsaicin at 2 min intervals
did not alter the response, indicating that these brief exposures to a
low concentration of capsaicin produced neither sensitization nor
desensitization of ICAP (Lopshire and Nicol,
1997b).
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Figure 1.
PGE2 and forskolin treatment enhance
the amplitude of the whole-cell current elicited by capsaicin.
A, Voltage-clamp recording (holding potential 60 mV)
obtained from a representative neuron in which PGE2
treatment increased the amplitude of the current elicited by a 2 sec
focal application of capsaicin. B, Sensitizing effects
of 100 nM and 1 µM forskolin treatment
(top and bottom traces, respectively) on
capsaicin responses in two other neurons. The times indicate when these
recordings were obtained after the onset of prostaglandin or forskolin
treatment. The extent and time courses of sensitization induced by
different concentrations of forskolin are summarized in
C. The amplitude of the capsaicin response after
forskolin treatment was normalized to the average of the two control
responses and represented as the fold increase relative to the control
value. The bar beginning at 3 min represents the change
to forskolin-containing Ringer's solution. D, Effects
of dideoxyforskolin on the capsaicin response. The
hatched and open bars indicate the
applications of dideoxyforskolin and PGE2,
respectively. Asterisks indicate significant differences
at p < 0.05 compared with control.
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The response of sensory neurons to bradykinin undergoes a
PGE2-induced sensitization in which this enhancement was
mediated by the cAMP transduction cascade (Cui and Nicol, 1995). To
investigate whether sensitization of capsaicin responses by
PGE2 involved similar cellular mechanisms, we determined
the ability of forskolin, a diterpene that directly activates adenylyl
cyclase (Seamon et al., 1981), to produce an analogous sensitization of
capsaicin responses. The forskolin concentrations (100 nM
to 10 µM) used in these experiments elevated the
intracellular cAMP content by 2- and 10-fold, respectively, in cultured
sensory neurons (Fig. 1, Hingtgen et al., 1995). Figure
1B (top panel) shows that 100 nM forskolin sensitized capsaicin responses. The control
response in this representative neuron was 510 pA. After a 10 min
exposure to 100 nM forskolin, the amplitude of
ICAP was increased to 1356 pA, a 2.7-fold
enhancement. Analogous to the PGE2-induced increase in
ICAP, the sensitization produced by
forskolin was transient; after a 35 min exposure to forskolin,
ICAP (530 pA) returned to control levels.
Higher concentrations of forskolin produced a similar level of
sensitization; however, the duration of this sensitization was
increased. The bottom panel in Figure 1B illustrates
the effect of 1 µM forskolin on
ICAP in another neuron. After a 10 min exposure to forskolin, ICAP was 836 pA, a threefold
increase over the control response (280 pA). Although
ICAP was enhanced, the holding current was
unaltered by forskolin; after a 10 min application, the holding current
was 79 ± 45 pA compared with the control value of 68 ± 23 pA (n = 7). This higher concentration of forskolin
produced a sensitization of greater duration. After exposure to
forskolin for 50 min, ICAP remained almost
twofold larger than the control response. This concentration-dependent
effect of forskolin on the duration of the enhanced capsaicin response
was obtained in all neurons and is summarized in Figure 1C.
The responses obtained after forskolin treatment were normalized to the
mean of the two control responses. Exposure to 100 nM
forskolin caused a significant and transient 2.7 ± 0.2-fold
increase in the amplitude of ICAP with a time to
peak of 11.3 ± 1.0 min and a
t1/2MAX of 5.3 ± 0.6 min
(n = 3). In neurons exposed to either 1 or 10 µM forskolin, ICAP exhibited a
3.7 ± 0.4-fold (n = 7) or 3.1 ± 0.4-fold
(n = 6) increase, respectively. The times to peak of
14.7 ± 3.3 min and 20.5 ± 3.3 min were similar for either 1 or 10 µM forskolin, respectively. However, compared with
the results obtained with 100 nM forskolin, the
sensitization remained significantly elevated for longer times. For 1 and 10 µM forskolin,
t1/2MAX was increased to 19.2 ± 4.0 and 19.8 ± 5.0 min, respectively. Therefore, 100 nM
forskolin appears to elicit maximal sensitization of
ICAP, whereas higher concentrations
prolong the period of sensitization.
To determine whether the sensitizing effects of forskolin were
attributable to a specific action on adenylyl cyclase or reflected some
other nonspecific action, we tested the effects of dideoxyforskolin, a
forskolin analog that does not stimulate adenylyl cyclase (Seamon et
al., 1983). As shown in Figure 1D, treatment with 1 µM dideoxyforskolin had no effect on
ICAP (n = 3). To determine
whether dideoxyforskolin somehow influenced the capacity of neurons to
be sensitized, another series of experiments was conducted in which
neurons were first exposed to dideoxyforskolin and then to
PGE2. As before, dideoxyforskolin had no effect on
ICAP; however, in the continued presence
of dideoxyforskolin, treatment with 1 µM PGE2
produced a significant and transient 2.0 ± 0.1-fold increase in
ICAP (n = 4). In all four
neurons examined, the time to peak was at 6 min with a
t1/2MAX of 3.9 ± 0.2 min. Taken
together, these experiments indicate that forskolin treatment, in a
manner analogous to the sensitization evoked by PGE2, produced a transient increase in the magnitude
of ICAP. This sensitization resulted from
stimulation of adenylyl cyclase because of the lack of effect of
dideoxyforskolin. Additionally, the duration of sensitization produced
by forskolin was concentration-dependent, suggesting that increased
concentrations of intracellular cAMP lead to greater durations of
sensitization of ICAP.
Analogs of cAMP also sensitize the capsaicin-elicited current
To explore the notion that the sensitization produced by
PGE2 and forskolin was mediated by the cAMP pathway, the
capacity of a membrane-permeable analog of cAMP, 8-bromo-cAMP
(8-Br-cAMP), to enhance ICAP was examined. The
concentrations of 8-Br-cAMP used in these experiments facilitated the
release of neuropeptides evoked by excitatory chemical agents in
cultured rat sensory neurons (Hingtgen et al., 1995). In a
representative neuron, the control response to capsaicin was 220 pA
(Fig. 2A, top
panel). After a 10 min exposure to 10 µM 8-Br-cAMP, ICAP was increased
by twofold (434 pA). Unlike the results obtained with 100 nM forskolin, the duration of sensitization was prolonged
in this neuron and remained elevated by 1.4-fold (314 pA) compared with
the control responses, even after a 35 min exposure to 8-Br-cAMP. To
determine whether the duration of the 8-Br-cAMP-induced sensitization
was also concentration-dependent, 1 mM 8-Br-cAMP was used
in an attempt to produce longer periods of sensitization. The results
from a representative neuron are shown in the bottom panel of Figure
2A. After a 6 min exposure to 1 mM
8-Br-cAMP, the amplitude of ICAP was increased
to 449 pA, a 2.3-fold increase from control response of 199 pA.
Surprisingly, the duration of the sensitization produced by this
concentration of 8-Br-cAMP was shortened, wherein the response had
returned to control levels after only 20 min (response amplitude of 229 pA).
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Figure 2.
Treatment with membrane-permeant analogs of cAMP
enhance the whole-cell responses to capsaicin. A,
Sensitizing effect of 10 µM and 1 mM
8-Br-cAMP treatment (top and bottom
traces, respectively) on capsaicin responses in two different
neurons. B, Extent and time course of the sensitization
produced by these concentrations of 8-Br-cAMP. C,
Sensitization induced by 10 and 100 µM
chlorphenylthio-cAMP. In B and C, the
bar beginning at 3 min represents the change to
Ringer's solution containing the indicated concentrations of cAMP
analogs. Asterisks indicate significant differences at
p < 0.05 compared with control.
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The apparent inverse concentration effect (lower concentrations of
8-Br-cAMP producing a longer duration of sensitization) was obtained in
all neurons exposed to 8-Br-cAMP. These experimental results are
summarized in Figure 2B. Exposure to 10 µM 8-Br-cAMP produced a significant 2.8 ± 0.3-fold
increase in the amplitude of ICAP with a time to
peak of 11.6 ± 0.1 min and a
t1/2MAX of 22.3 ± 2.1 min
(n = 5). In neurons exposed to 100 µM
8-Br-cAMP, ICAP was increased significantly by
2.4 ± 0.4-fold above the control responses with a time to peak of
9.3 ± 1.5 min (n = 6). However, the duration of
sensitization was decreased significantly where t1/2MAX was reduced to 3.8 ± 0.4 min. Increasing the concentration of 8-Br-cAMP to 1 mM
significantly enhanced ICAP by 2.0 ± 0.1-fold and had a time to peak of 6.0 ± 0.1 min
(n = 3). This concentration of 8-Br-cAMP produced a
further decrease in t1/2MAX to 2.3 ± 0.1 min. Although the exact mechanism(s) for the
inverse-concentration effect obtained with 8-Br-cAMP remains unclear
(but see below), treatment with 8-Br-cAMP sensitized the capsaicin
response in a manner analogous to that produced by PGE2 and
forskolin. These results then suggest that increased levels of
intracellular cAMP likely mediate the sensitization produced by
PGE2.
The shortened duration of sensitization obtained with higher
concentrations of the cAMP analog 8-Br-cAMP suggests that this agent
may have other cellular actions. Therefore, to explore this possibility, the capacity of another membrane-permeant cAMP analog, chlorphenylthio-cAMP (cpt-cAMP) to sensitize sensory neurons was determined. As presented in Figure 2C, the results obtained
with cpt-cAMP were similar to those obtained with 8-Br-cAMP. Exposure to 10 µM cpt-cAMP produced a 2.2 ± 0.1-fold
increase in the amplitude of ICAP with a time to
peak of 16.0 ± 2.1 min (n = 4). The sensitization produced by 10 µM cpt-cAMP remained significantly
elevated for a sustained period, as evidenced by the
t1/2MAX of 26.7 ± 5.0 min.
Similarly, ICAP was enhanced significantly by
2.0 ± 0.2-fold after treatment with 100 µM
cpt-cAMP; the sensitization had a time to peak of 10.0 ± 0.1 min
(n = 4). However, with this higher concentration of
cpt-cAMP, t1/2MAX was reduced to 3.1 ± 0.3 min. This series of experiments suggests that, like forskolin, elevations in intracellular cAMP enhanced the sensitivity of the neuron
to capsaicin. However, unlike forskolin, higher concentrations of the
cAMP analogs somehow led to a decreased duration of sensitization.
The above studies raise the possibility that the more transient
sensitization observed with higher concentrations of the cAMP analogs
may reflect the activity of these agents at an effector that normally
is not activated by physiological increases in the concentration of
cAMP. Previous studies observed that cAMP analogs and high
concentrations of cAMP were capable of activating cyclic GMP-dependent
protein kinase (PKG); this pattern of stimulation was termed
cross-activation (Jiang et al., 1992). In support of this notion, our
previous results demonstrated that recovery of PGE2-induced
sensitization of ICAP was mediated by activation of PKG (Lopshire and Nicol, 1997b). To investigate the possibility that
these cAMP analogs reverse the sensitization through the cross-activation of PKG, we examined the action of 1 mM
8-Br-cAMP on ICAP in neurons that were
sensitized fully by consecutive treatments with 1 and 10 µM forskolin. These results are shown in Figure 3. After exposure to 1 µM
forskolin, ICAP was enhanced by 2.1-fold compared with the control responses and had a time to peak of 7.3 ± 1.1 min (n = 3). The enhanced response to capsaicin
stabilized at this level. If the reversal or inactivation of
sensitization was produced by an additional large increase in cAMP,
then treatment of these neurons with 10 µM forskolin
should cause the sensitization to recover to control levels. However,
10 µM forskolin produced no further change in the level
of sensitization. After ~21 min in 10 µM forskolin,
ICAP was maintained at a twofold increase over
the control levels, suggesting that maximal sensitization had been
attained. At this time, exposure to 1 mM 8-Br-cAMP
caused the enhanced ICAP to return rapidly to
control levels with a t1/2MAX of 2.7 ± 0.3 min (relative to the time of the last capsaicin response before
8-Br-cAMP addition). These results suggest that higher concentrations
of cAMP analogs may act at site(s) distinct from those usually
stimulated by normal physiological changes in the levels of cAMP.
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Figure 3.
Treatment with 8-Br-cAMP reverses the
forskolin-induced sensitization. The consecutive application of 1 and
10 µM forskolin is indicated by the
hatched and solid bars, respectively. In
the presence of 10 µM forskolin, the addition of 1 mM 8-Br-cAMP (open bar) rapidly reversed the
forskolin-induced sensitization. The inset traces
illustrate the capsaicin responses from a representative neuron at the
indicated times. Asterisks indicate significant
differences at p < 0.05 compared with
control.
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Inhibition of protein kinase A prevents PGE2- and
forskolin-induced sensitization
Both forskolin and cAMP analogs gave rise to a sensitization of
ICAP that was similar to that produced by
PGE2. To establish whether this increased sensitivity to
capsaicin was attributable to a direct action of cAMP or was dependent
on cAMP activation of PKA, a series of experiments was conducted in
which sensory neurons were perfused intracellularly with the peptide
inhibitor of PKA, PKI14-24 (Cheng et al., 1986). In the
presence of 20 µM PKI14-24, the peak
amplitudes of the control responses to 100 nM capsaicin
were not different significantly from control responses obtained in
earlier experiments (PKI + PGE2 series: 325 ± 111 pA;
n = 8; PKI + forskolin series: 284 ± 44 pA;
n = 4; and no PKI series: 255 ± 18 pA;
n = 50). As shown in Figure 4, intracellular perfusion of
PKI14-24 completely blocked the capacity of either 1 µM PGE2 or 1 µM forskolin (Fig.
4A,B, respectively) to enhance
ICAP. The insets illustrate representative responses obtained at the indicated times during both experiments. These findings demonstrate that activation of PKA was necessary and
sufficient for the sensitization of ICAP
produced by either PGE2 or forskolin.
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Figure 4.
PKI14-24 treatment blocks both the
PGE2- and forskolin-induced sensitization.
A, Results from experiments with PKI14-24
and PGE2 treatment. The hatched and
open bars indicate the addition of PKI14-24
and PGE2, respectively. B, Results
from experiments with PKI14-24 and forskolin treatments.
The hatched and open bars indicate the
presence of PKI14-24 and forskolin, respectively. The
inset traces illustrate representative responses to
capsaicin from two different neurons for each experimental condition at
the times indicated. Asterisks indicate significant differences at
p < 0.05 compared with control.
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Capsaicin elicits single-channel activity in cell-attached
membrane patches that is antagonized by capsazepine
The cAMP-mediated sensitization of ICAP
likely is manifested by a change in one or more of the single-channel
properties of the capsaicin-gated channel. Oh et al. (1996a,b) reported
recently that, in cell-attached recordings, extracellularly applied
capsaicin elicited single-channel currents in the membrane patch. Thus, these investigators proposed that capsaicin crosses the plasma membrane
and binds to the channel at the intracellular surface of the membrane.
Based on these observations, the cell-attached configuration was used
to explore the modulation of the capsaicin-gated ion channel by
PGE2 and the cAMP pathway. An additional advantage of this
approach is that normal intracellular signaling pathways of the neuron
remain intact.
Initially, the properties of the capsaicin-gated channel in these
cultured sensory neurons were characterized. In a representative recording in which the membrane potential was maintained at 60 mV
(Fig.
5A,B),
changing the superfusate to low-calcium external solution containing 1 µM capsaicin evoked the appearance of inward currents,
which was indicative of the activation of capsaicin-gated ion channels.
Figure 5B illustrates selected portions of the compressed traces shown in Figure 5A on an expanded time scale. Each
trace is taken from that particular segment of the recording indicated by its respective number. The unitary nature of the multiple channel openings is evident in traces 2 and 4. After washout of capsaicin, the
inward currents were no longer present. Inclusion of 10 µM capsazepine, the competitive antagonist of capsaicin
(Bevan et al., 1992), with the 1 µM capsaicin low-calcium
external solution, produced a nearly complete suppression of the
currents elicited by capsaicin. With the removal of capsazepine, the
introduction of capsaicin again elicited the channel currents. The
decreased channel activity observed during this second capsaicin
application may reflect the presence of residual capsazepine or
desensitization of the capsaicin response. Desensitization seems less
likely, because this process should be diminished at the reduced
calcium concentrations (~150 nM) used in these
experiments. This notion was based on previous observations in which
desensitization of the capsaicin response was attenuated greatly as the
external calcium was lowered (Cholewinski et al., 1993; Liu and Simon, 1996; Koplas et al., 1997).
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Figure 5.
Capsaicin elicits single-channel activity that is
blocked by capsazepine. A, Representative recording from
a cell-attached patch held at 60 mV. Changing the superfusate from
the low-calcium external solution (trace 1) to one
containing 1 µM capsaicin (CAP) promoted
single-channel activity that was blocked reversibly by 10 µM capsazepine (CAP + CZP).
B, Selected portions of the compressed traces shown in
A at greater time resolution. The numbered
traces in B represent the channel activity
observed for those specific portions indicated by their respective
numbers under the traces of A. The arrows
indicate the closed level for each trace. C, All-points
histogram generated from a 40 sec recording during the first
application of capsaicin to this neuron. D, Effect of
capsaicin and capsaicin-capsazepine treatment on the mean
NPo in three cell-attached patches.
Asterisks indicate significant differences at
p < 0.05 compared with control.
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An all-points amplitude histogram was constructed from the initial
capsaicin exposure in this neuron and is shown in Figure 5C.
The peaks in this histogram were fitted with a Gaussian distribution in
which the values corresponded to one closed level and four open levels.
This suggested that there were at least four active capsaicin channels
in this patch. The amplitude of the unitary current obtained for the
open levels was 2.1 ± 0.1 pA and yielded a single-channel
conductance of 35.1 ± 1.5 pS. The mean values for NPo
obtained under these different experimental conditions in three
different neurons are summarized in Figure 5D. These results
demonstrate that the addition of 1 µM capsaicin produced a large increase in NPo that was blocked by the addition of
capsazepine. Taken together, our observations support the previous
results of Oh et al. (1996 a,b) that capsaicin is capable of
diffusing through the plasma membrane to elicit single-channel activity in these cell-attached patches.
Capsaicin-elicited channel activity is concentration-dependent
To ascertain the appropriate concentration of capsaicin with which
to probe the activity of single channels in cell-attached patches, we
determined the concentration-response relationship for capsaicin
applied extracellularly. The patch was held at 60 mV and exposed to
increasing bath concentrations of capsaicin that ranged from 30 nM to 10 µM. Between capsaicin applications the cell was washed extensively with low-calcium external solution. NPo at each concentration of capsaicin was determined, and
the results from nine neurons were pooled to obtain the mean
NPo for a given concentration (Fig.
6). The results were fitted by a
ligand-binding isotherm (described in Materials and Methods) that
yielded an EC50 of 1.4 µM and a steepness
factor of 2.5.
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Figure 6.
NPo depends on the concentration of
capsaicin. These results summarize the effect of increasing
concentrations of bath-applied capsaicin on mean NPo in
eight cell-attached patches. The line through the data
points represents the fit obtained for the ligand-binding isotherm as
described in Materials and Methods.
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The capsaicin-gated channel exhibits outward rectification and
increased activity at positive potentials
Figure 7A illustrates
representative single-channel currents elicited by 1 µM
capsaicin at several membrane voltages. At 60 mV, the currents were
inward; the currents remained inward at 30 and 10 mV but were
reduced in amplitude. At positive membrane potentials, the currents
became outward and increased in amplitude with depolarizing potentials.
NPo increased from 0.11 to 1.27 as the potential changed
from 60 to +60 mV values, respectively. The current-voltage relation
obtained for the single-channel currents is summarized in Figure
7B. The current-voltage relationship appeared linear
between 60 and +20 mV with an average conductance of 33 ± 1 pS
at 60 mV. At more positive potentials, the current began to rectify
with the single-channel conductance increasing to 46 ± 3 pS at
+60 mV. The apparent reversal potential (uncorrected for membrane
potential) obtained from this relation was +4 ± 1 mV, which was
similar to values reported previously for capsaicin-elicited currents
(Oh et al., 1996a; Caterina et al., 1997).
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Figure 7.
The capsaicin-gated channel exhibits outward
rectification and increased NPo at positive membrane
potentials. A, Effect of membrane potential on the
single-channel activity elicited by bath exposure to 1 µM
capsaicin in a representative patch. The arrows indicate
the closed level for each trace. The membrane potential for each trace
is provided at the right. B,
Current-voltage relation obtained from recordings in which the number
of sensory neurons ranged between three and nine. The
inset shows a representative current-clamp recording for
the depolarization (to 3 mV) elicited by treatment with 1 µM capsaicin. C, Dependence of the
relative NPo elicited by 1 µM capsaicin
(normalized to that obtained at +60 mV) on membrane potential
(n = 3). The line through the
bars represents the fit described by the Boltzmann
relation.
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In cell-attached patches from embryonic sensory neurons,
NPo of the capsaicin-gated channel increased as the
membrane potential was depolarized. Because NPo was maximal
at +60 mV, values for NPo obtained at other membrane
voltages were normalized to this maximum for each neuron. Figure
6C shows that the relative NPo increased from
0.04 ± 0.02 to 1 (n = 3) as the membrane
potential was changed from 60 to +60 mV. The dependence of the
relative NPo on membrane potential was described by the
Boltzmann relation where V0.5 was 9 and k was
20 mV. Previous results demonstrated similar findings for the
capsaicin-gated channel in sensory neurons of the neonatal rat (Oh et
al., 1996a).
PGE2 and forskolin treatment transiently increase
capsaicin-gated channel activity
To investigate the capacity of PGE2 and forskolin to
sensitize the capsaicin-gated channel, we used a concentration of 300 nM capsaicin to evoke recordings of only single-level
openings of the channel. This choice was based on two observations.
First, 300 nM was well below the EC50 for the
concentration-response relation (Fig. 6). Second, in preliminary
studies, recordings obtained with 100 nM capsaicin failed
to exhibit reliable levels of activity under control conditions (data
not shown). The results obtained from a cell-attached patch exposed to
300 nM capsaicin are shown in Figure
8A. However, in this
trace, two overlapping open events were detected, indicating that at
least two active channels were present. The mean unitary current was
1.9 pA, which corresponds to a single-channel conductance of 31 pS;
NPo in this trace was 0.13. After exposure to 1 µM PGE2 for 12 min, there were clearly three
overlapping open levels observed, and NPo was increased to
0.53. There was no change in the unitary current after PGE2
treatment; it remained at 2.0 pA (Fig. 8B). In this neuron, the PGE2-induced increase in NPo was
transient when, after a 20 min exposure to PGE2,
NPo was reduced to 0.03. The unitary current remained
unchanged at 2.0 pA (Fig. 8C). Interestingly, the
application of 10 µM capsaicin (Fig.
8D) after a 25 min exposure to PGE2
produced a large increase in NPo to 0.85 with three
detectable open levels. The unitary current was still unchanged at
2.0 pA.
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Figure 8.
PGE2 treatment enhances the channel
activity elicited by capsaicin. A, Representative
recording of the single-channel activity elicited by 300 nM
capsaicin under control conditions. In B, the
single-channel activity elicited by capsaicin is increased after
treatment with 1 µM PGE2 in the same neuron.
The inset trace shows, at greater time resolution, the
capsaicin response during the period indicated by the
bar. The transient nature of the
PGE2-induced increase in channel activity is shown in
C. The trace illustrates the recording
obtained after 20 min of continuous exposure to PGE2.
D, Effect of 10 µM capsaicin treatment in
this same neuron after a 25 min exposure to PGE2. The
inset illustrates the response to capsaicin obtained
during the time indicated by the bar. In all traces, the
arrows indicate the closed level. The all-points
histogram generated for each trace is provided at the
right.
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As summarized in Figure 9,
PGE2 significantly enhanced NPo in all seven
neurons examined. After a 12 min exposure, PGE2 increased NPo to 0.79 ± 0.1 from the control level of 0.07 ± 0.03. Furthermore, this increase was transient wherein
NPo returned to control levels after only 20 min in the
continuous exposure to PGE2. The unitary conductance of the
capsaicin-gated channel remained unaltered throughout the exposure to
PGE2, having values of 33 ± 0.7, 33 ± 0.4, and 33 ± 0.6 pS for the control condition and for 12 and 20 min exposures to PGE2, respectively. In all of these
recordings, multiple channel openings were noted after PGE2
exposure, thereby complicating a kinetic analysis of channel activity.
Similarly, treatment with 1 µM forskolin resulted in a
significant and transient increase in NPo evoked by 300 nM capsaicin (Fig. 9), whereas the unitary conductance was
unaltered (33 ± 0.8 and 34 ± 0.4 pS for the control and
after a 12 min exposure to forskolin, respectively). In the absence of
PGE2 or forskolin, neither the unitary conductance nor
NPo elicited by 300 nM capsaicin was changed
over the 23 min time course (Fig. 9). Thus, these findings suggest that
the PGE2- or forskolin-induced enhancement of
NPo without a concomitant change in unitary conductance
results from an increase in the number of active channels and/or an
increased open probability of the channel.
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Figure 9.
PGE2 or forskolin treatment
transiently increases NPo of the capsaicin-gated channel.
The hatched bar indicates the time and duration for the
application of each agent. Asterisks indicate
significant differences at p < 0.05 compared with
control.
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DISCUSSION |
Capsaicin-elicited currents in sensory neurons
In this report we demonstrated that the application of the
vanilloid capsaicin to embryonic sensory neurons elicits whole-cell currents that are similar to those observed in previous studies (Marsh
et al., 1987; Bevan and Szolcsanyi, 1990; Koplas et al., 1997; Lopshire
and Nicol, 1997b). Likewise, the properties of the capsaicin-gated ion
channel described in embryonic sensory neurons are comparable to
characterizations of this channel in sensory neurons of the neonatal
rat (Oh et al., 1996a) as well as the cloned vanilloid receptor
expressed in mammalian HEK293 cells (Caterina et al., 1997). For
example, the EC50 (1.4 µM) and the steepness
factor n (2.5) determined for the single-channel recordings in Figure 6
are similar to those values (1.1 µM and 1.8) reported by
Oh et al. (1996a) for neonatal rat sensory neurons. Our observation
that n > 2 indicates that two or more molecules of capsaicin bind
to the channel to promote opening. In addition, our estimation of the
single-channel conductance at 60 mV is similar to previously
described values that ranged from 30 to 45 pS (Bevan and Szolcsanyi,
1990; Oh et al., 1996a; Caterina et al., 1997). The conductance
exhibits rectification wherein the value increased by nearly twofold
(ranging from 70 to 80 pS) at +60 mV (Bevan and Szolcsanyi, 1990; Oh et
al., 1996a; Caterina et al., 1997). However, the increase in
conductance at +60 mV determined in our studies was smaller than that
described in these previous studies. This may result from the higher
concentration of extracellular calcium used in our study (~150
nM) compared with other studies in which no added calcium
was used (Oh et al., 1996a; Caterina et al., 1997). Indeed, both Forbes
and Bevan (1988) and Oh et al. (1996a) reported that the conductance of
the capsaicin-gated channel can be reduced by increased levels of
extracellular calcium.
The relative NPo increased with depolarizing potentials
(Fig. 7C); these results were described by the Boltzmann
relationship in which the values of V0.5 and k
were 9 and 20 mV, respectively. These values corroborate a previous
report by Oh et al. (1996a) in which V0.5 was 9 and
k was 29 mV. Thus, the channel properties determined in
embryonic rat sensory neurons are similar to those published by other
investigators using different preparations. This then suggests that the
electrophysiological properties of the capsaicin receptor are not
regulated or modified differentially during development.
Sensitization of the response to capsaicin
Treatment with the proinflammatory prostaglandin PGE2
enhanced by twofold to threefold the amplitude of whole-cell currents elicited by capsaicin (Lopshire and Nicol, 1997b). This sensitization was transient wherein the capsaicin response returned to control levels
after ~20-25 min in the continued presence of PGE2 (Fig. 1A,D). This reversal of
sensitization does not involve desensitization of the capsaicin
response because the recovery was blocked by inhibitors of nitric oxide
synthase (Lopshire and Nicol, 1997b), whereas desensitization was
insensitive to inhibitors of nitric oxide synthase but was suppressed
by calcineurin inhibitors (Docherty et al., 1996). In addition, this
eicosanoid significantly increased the value of NPo for the
capsaicin-gated channel; however, the conductance was unaltered. Thus,
the enhanced whole-cell currents appear to be a direct result of the
PGE2-induced modification of the capsaicin receptor that
leads to increased levels of activity without modulation of the
conductance.
Previously, we demonstrated that the duration of
PGE2-induced sensitization of the capsaicin response
depended on the concentration of extracellular calcium wherein lowered
levels lengthened the period of sensitization (Lopshire and Nicol,
1997b). We observed that the duration of the transient sensitization
(Fig. 9) of single-channel activity (performed at ~150 nM
extracellular calcium) was similar to the transient sensitization of
whole-cell currents (performed at 2 mM external calcium).
This correspondence may result from the different procedures used to
deliver capsaicin. In the whole-cell studies, capsaicin was applied
focally in puffs of 1-2 sec, whereas in the single-channel studies,
capsaicin was administered continuously during the recording. Despite
the lowered calcium concentration, this persistent depolarization
occurring with the continuous delivery (Fig. 7B,
inset) might permit a sufficient calcium influx to activate pathways that reverse sensitization.
Signaling pathways that mediate sensitization
Previous studies demonstrated that activation of the cAMP
transduction pathway played a necessary and sufficient role in the PGE2-induced sensitization of the bradykinin response in
sensory neurons (Cui and Nicol, 1995; Hingtgen et al., 1995). In our
studies described above, forskolin, an activator of adenylyl cyclase, or membrane-permeant analogs of cAMP enhanced the amplitude of the
whole-cell current elicited by capsaicin in a manner comparable to
PGE2. In support of our findings, Pitchford and Levine
(1991) reported that exposure to PGE2 or analogs of cAMP
increased the amplitude of the capsaicin-evoked current in adult rat
sensory neurons. However, given the high concentrations of
PGE2 (1 mM) or 8-Br-cAMP (20 mM)
used in that study, it is difficult to assess directly the
physiological significance of such findings. We also observed that
treatment with either PGE2 or forskolin increased NPo of the channel in response to activation by capsaicin.
After treatment with either PGE2 or forskolin, the
amplitude histograms revealed openings to additional levels (Fig.
8B) that were not observed in the control recording
(Fig. 8A). These results raise the possibility that
PGE2 or forskolin increased the sensitivity of the channel
to activation by capsaicin. In support of this notion is the
observation that after treatment with PGE2, the histogram obtained for 300 nM capsaicin (well below the
EC50) was very similar to that obtained with a
maximal concentration of 10 µM capsaicin (Fig. 8, compare
B,D).
Sensitization of the capsaicin response results from activation of
adenylyl cyclase and the consequent activation of PKA. This idea is
corroborated by two additional observations. First, dideoxyforskolin,
which retains all of the properties of forskolin except the capacity to
activate adenylyl cyclase, did not sensitize capsaicin-elicited
currents, and it failed to alter the PGE2-induced sensitization of capsaicin responses (Fig. 1D).
Second, intracellular perfusion of the neuron with the inhibitor of
PKA, PKI14-24, blocked both the PGE2- and
forskolin-induced sensitization, suggesting that a cAMP-dependent
phosphorylation played a key role in the sensitization of the capsaicin
response. The notion that the activity of the capsaicin-gated ion
channel can be modulated by a phosphorylation reaction mediated by PKA
is supported by the amino acid sequence determined for the cloned
vanilloid receptor. The receptor cDNA predicted three putative sites
for phosphorylation by PKA on the cytoplasmic side of the protein
(Caterina et al., 1997). The role of PKA in modulating the sensitivity
of sensory neurons to noxious stimulation was defined further in
studies examining mice with a targeted mutation of the type I
regulatory subunit (RI ) of PKA. The heightened thermal sensitivity
after injection of PGE2 into the hindpaw of the targeted
mice was reduced in comparison to the wild-type mice (Malmberg et al.,
1997). Taken together, these findings suggest that elevated levels of
intracellular cAMP lead to the activation of PKA. It is this activated
PKA that subsequently modifies the capsaicin receptor-ion channel
complex resulting in an altered sensitivity to capsaicin and/or
increasing the open probability of the channel.
It is interesting that increasing concentrations of forskolin
lengthened the duration of sensitization, whereas higher concentrations of either 8-Br-cAMP or cpt-cAMP decreased the duration (compare Figs.
1C, 2B,C). In a previous
study (Lopshire and Nicol, 1997b), we demonstrated that the
PGE2-induced sensitization of the capsaicin-elicited current was inactivated or reversed by stimulation of PKG. Based on
these findings, we speculate that the rapid inactivation of sensitization observed with higher concentrations of 8-Br-cAMP or
cpt-cAMP results from the cross-activation of PKG. As suggested by
Figures 1-3, we assume that the onset and amplitude of sensitization are correlated directly with the intracellular levels of cAMP. Both 1 and 10 µM forskolin produced maximal levels of
sensitization (Fig. 1C), and, in fact, there was no further
change in the level of sensitization when treatment with 1 µM forskolin was followed subsequently by 10 µM forskolin (Fig. 3). This implies that the physiological effects of the elevated cAMP were maximized and that any
additional increases in cAMP did not produce greater levels of
sensitization. Also shown in Figure 3, addition of 1 mM
8-Br-cAMP rapidly reversed the sensitization, suggesting that this
recovery was mediated by a pathway independent of the activation of PKA
by cAMP. The rapid reversal of sensitization was similar to that
previously observed after treatment with either nitric oxide donors or
8-Br-cGMP (Lopshire and Nicol, 1997b). In that study, inhibition of PKG
prevented the cGMP-induced inactivation of sensitization. Taken
together, these findings suggest that the reversal of sensitization by
high concentrations of cAMP analogs may result from their
cross-activation of PKG.
Biochemical studies examining the activity of purified PKG isolated
from bovine lung (PKG type I ) demonstrated that cAMP was capable of
activating PKG, although 50-100 times greater concentrations of cAMP
were required to produce activation levels equivalent to cGMP (Lincoln
et al., 1977). In a later study, Francis et al. (1988) found that
8-Br-cGMP activated purified PKG with a Ka of 0.025 µM and had an EC50 of 47 µM for the relaxation of coronary artery. However, both
cpt-cAMP and 8-Br-cAMP activated PKG and produced relaxation with
cpt-cAMP being more effective (Ka, 0.2 µM; EC50, 30 µM) than
8-Br-cAMP (Ka, 5.8 µM;
EC50, 1670 µM). Activation of PKG by
cAMP itself was much less effective compared with cpt-cAMP in which the
Ka was 16 µM (Wolfe et al.,
1989).
These values for the effectiveness of cAMP, cpt-cAMP, and 8-Br-cAMP to
activate PKG could account for our observations regarding the recovery
times shown in Figures 1C and 2, B and
C. Increasing forskolin concentrations, which elevate
intracellular cAMP (a poor activator of PKG), produced a sensitization
of longer durations. Increasing concentrations of cAMP analogs, which
are better activators of PKG, cause the duration of sensitization to be
shortened. Furthermore, 100 µM cpt-cAMP inactivated
sensitization on a time course that was similar to 1 mM
8-Br-cAMP; this may result from the greater ability of cpt-cAMP
relative to 8-Br-cAMP to activate PKG.
In conclusion, PGE2 sensitizes the capsaicin response
through activation of the cAMP transduction cascade. Increased levels of intracellular cAMP lead to the activation of PKA. This kinase enhances the activity of the capsaicin-gated ion channel by increasing the sensitivity of the receptor to capsaicin and/or the open
probability. A direct consequence of the facilitation is the increased
whole-cell current that may give rise to a larger and/or longer
depolarization, thereby enhancing the excitability of the sensory
neuron. This cAMP-mediated sensitization ultimately augments the
capacity of the sensory neuron to signal the reception of nociceptive
stimulation to the spinal cord.
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FOOTNOTES |
Received Feb. 3, 1998; revised May 26, 1998; accepted May 27, 1998.
This work was supported by National Institute of Neurological Disorders
and Stroke Grant NS-30527 to G.D.N. J.C.L. was supported by grants
from the Indiana University-Purdue University, Indianapolis Research Investment Fund and the American Heart Association, Indiana Affiliate. We are grateful to Dr. Jim Kenyon for his advice regarding the analysis of single-channel activity.
Correspondence should be addressed to Dr. Grant Nicol, Department of
Pharmacology and Toxicology, Indiana University School of Medicine,
Indianapolis, IN 46202.
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H.-J. Hu, G. Bhave, and R. W. Gereau IV
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D. Yang and R. W. Gereau IV
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P. M. Zygmunt, D. A. Andersson, and E. D. Hogestatt
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S. L Borgland, M. Connor, R. M Ryan, H. J Ball, and M. J Christie
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D Levy and A M Strassman
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X. Shu and L. M. Mendell
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L. S. Premkumar
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P. Chaudhary, M.E. Martenson, and T.K. Baumann
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M. Tominaga, M. Wada, and M. Masu
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M. Kress and S. Guenther
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T. K. Baumann and M. E. Martenson
Extracellular Protons Both Increase the Activity and Reduce the Conductance of Capsaicin- Gated Channels
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D Levy and A M Strassman
Distinct sensitizing effects of the cAMP-PKA second messenger cascade on rat dural mechanonociceptors
J. Physiol.,
January 15, 2002;
538(2):
483 - 493.
[Abstract]
[Full Text]
[PDF]
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S. L Borgland, M. Connor, R. M Ryan, H. J Ball, and M. J Christie
Prostaglandin E2 inhibits calcium current in two sub-populations of acutely isolated mouse trigeminal sensory neurons
J. Physiol.,
March 1, 2002;
539(2):
433 - 444.
[Abstract]
[Full Text]
[PDF]
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Top
Abstract
Introduction
