Department of Pharmacology, College of Medicine, University of
California, Irvine, Irvine, California
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Introduction |
M2
and M3 muscarinic receptor subtypes are
abundantly expressed in smooth muscle throughout the gastrointestinal
tract (Eglen et al., 1996
; Ehlert et al., 1997). Radioligand binding
(Giraldo et al., 1988; Michel and Whiting, 1990), mRNA hybridization
(Maeda et al., 1988), and immunoprecipitation studies (Wall et al.,
1991) have shown that the M2 receptor is the more
abundant of the two receptors in the intestine (Ehlert et al., 1997).
Interestingly, a large body of pharmacological evidence shows that the
less abundant M3 receptor mediates contraction of
gastrointestinal smooth muscle under standard conditions (i.e., no
other contractile or relaxant agents present). The
M3 receptor is known to stimulate phospholipase C
in a variety of cell types, including smooth muscle. Presumably, this mechanism mobilizes calcium and initiates contraction in smooth muscle.
The M2 receptor is known to mediate a pertussis
toxin-sensitive inhibition of adenylyl cyclase activity in the guinea
pig ileum and colon (Candell et al., 1990; Zhang and Buxton, 1991; Thomas and Ehlert, 1994). Muscarinic agonists have been shown in both
ileum and colon to oppose the increase in cAMP elicited by forskolin,
isoproterenol, and a variety of other compounds that stimulate cAMP
accumulation (Griffin and Ehlert, 1992; Ostrom and Ehlert, 1997; Sawyer
and Ehlert, 1998). The M2 receptor also elicits
an indirect contraction in both the guinea pig ileum and colon by
preventing the relaxant effects of forskolin and isoproterenol on
histamine-induced contraction (Thomas et al., 1993; Thomas and Ehlert,
1994; Ostrom and Ehlert, 1997; Sawyer and Ehlert, 1998). The
M2-mediated indirect contraction is pertussis
toxin sensitive (Sawyer and Ehlert, 1998), unlike the standard
M3-mediated contraction.
Extensive alkylation of M3 receptors by the
selective irreversible antagonist
N-(2-chloroethyl)-4-piperidinyl diphenylacetate (4-DAMP
mustard) (Thomas et al., 1993) renders the contractile response of the
guinea pig colon sensitive to pertussis toxin treatment (Sawyer and
Ehlert, 1998). This sensitivity suggests that the
M2 receptor may directly participate in the
contractile response of the colon after most of the
M3 receptors have been inactivated with 4-DAMP
mustard. When expressed in high abundance, M2
receptors have been shown to mediate a weak, pertussis toxin-sensitive, phosphoinositide response by coupling to Gi
(Ashkenazi et al., 1987; Lai et al., 1991; Dell'Acqua et al., 1993).
Such a mechanism would be difficult to detect in the face of a large
M3 phosphoinositide response via
Gq. Thus, it is important to consider whether
M2 receptors in the colon are capable of
eliciting contraction through the phosphoinositide pathway after most
of the M3 phosphoinositide response has been inactivated.
In the present report, we investigated this hypothesis and have shown
that although the muscarinic contractile response is extremely
sensitive to pertussis toxin after 4-DAMP mustard treatment, the
phosphoinositide response is not. Thus, our results provide no evidence
for the direct coupling of M2 receptors to
phosphoinositide hydrolysis. Instead, our results are consistent with a
mathematical model in which the M2 receptor is
capable of eliciting contraction when there is a low level of
M3 receptor activation. This model accounts for
the finding that the muscarinic contractile response after 4-DAMP
mustard treatment is sensitive to pertussis toxin yet nevertheless
relatively insensitive to the M2-selective
antagonist AF-DX 116.
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Experimental Procedures |
Contractile Measurements.
Male Hartley guinea pigs (300-400
g) were asphyxiated with CO2 followed immediately
by exsanguination, and segments of colon (1-2 cm) were harvested 1 cm
from the cecum. Each segment was rapidly cleaned with
Krebs-Ringer-bicarbonate (KRB; 124 mM NaCl, 5 mM KCl, 1.3 mM
MgCl2, 26 mM NaHCO3, 1.2 mM
KH2PO4, 1.8 mM
CaCl2, 10 mM glucose) buffer to remove its
contents. The segments were connected to a force transducer and mounted
longitudinally in an organ bath containing 50 ml of KRB buffer at
37°C gassed with O2/CO2
(19:1). The colonic segments were allowed to equilibrate for 40 min at
a resting tension equivalent to a load of 1.5g (optimal pretension was determined after constructing a pretension versus force
of contraction curve) before measurement of isometric contractions with
a force transducer and polygraph. A test dose of the highly efficacious
muscarinic agonist oxotremorine-M was then added to each bath. Once
each tissue reached a sustained contraction, each bath was washed with
KRB buffer and allowed to incubate for 5 min before the addition of two
more test doses. These three test doses were used to ensure
reproducibility of the preparations. Segments of colon that did not
contract to at least 60% of that elicited by 100 mM KCl were
discarded. After the last 5-min incubation, the KRB buffer was replaced
with 50 ml of Ca2+-free KRB buffer (124 mM NaCl,
5 mM KCl, 1.3 mM MgCl2, 26 mM
NaHCO3, 1.2 mM
KH2PO4, 1 mM EGTA, 10 mM
glucose). The colon was incubated in Ca2+-free
medium for 10 min to inhibit myogenic contraction and cause full
relaxation. During this period, a resting tension of 1.5g was maintained. Subsequently, the Ca2+-free KRB
buffer was replaced with 50 ml of K+-deficient
KRB buffer (124 mM NaCl, 1.3 mM MgCl2, 26 mM
NaHCO3, 1.2 mM
KH2PO4, 1.8 mM
CaCl2, 10 mM glucose) to inhibit spontaneous contractions. After the addition of the
K+-deficient KRB buffer, a large contraction was
observed that declined to resting tension within 7 to 10 min.
Cumulative agonist concentration-response curves were measured by
adding 9 to 18 geometrically spaced (0.33 log unit) concentrations of
oxotremorine-M to each of the organ baths. The
EC50 value was determined from this curve as
described below. The K+-deficient KRB buffer was
washed from the bath, and 50 ml of KRB buffer was added. Colonic
segments were allowed to incubate for 30 min before any further
measurements were made. The above procedure (excluding three test
doses) was repeated before each EC50 measurement made with the same tissue.
Contractile Experiments Using 4-DAMP Mustard-Treated Colonic
Segments.
Some colonic segments were incubated with 40 nM
concentration of the aziridinium ion of 4-DAMP mustard for 1 h
in the presence of 1.0 µM
[[2-[(diethylamino)methyl]-1-piperidinyl]acetyl]-5,11-dihydro-6H-pyrido[2,3b][1,4]benzodiazepine-6-one (AF-DX 116) to selectively alkylate M3 muscarinic
receptors (Thomas et al., 1993). The colon segments were washed
thoroughly to remove AF-DX 116 and any unreacted 4-DAMP mustard before
measurement of concentration-response curves as described above. Some
tissues were washed with KRB buffer, and the aziridinium ion of 4-DAMP mustard (40 nM) and AF-DX 116 (1.0 µM) were added again for an additional hour (i.e., total incubation time of 2 h) before
measurement of concentration-response curves. In other experiments,
colonic segments were exposed to 4-DAMP mustard for a total of 3 or
4 h using the same washing procedure described above at the end of
each hour of exposure. In all experiments, 4-DAMP mustard was first
converted to its aziridinium ion by incubation for 30 min at 37°C in
10 mM NaKPO4, pH 7.4, as previously described
(Thomas et al., 1992).
Phosphoinositide Hydrolysis Assay.
Male guinea pigs
(300-400 g) were sacrificed as described above, and an approximately
16-cm segment of colon was rapidly harvested 1 cm distal the cecum. The
colon was placed in ice-cold KRB gassed with
O2/CO2 (19:1) and cleaned
to remove the contents. The colonic segment was cut longitudinally, and
the mucosa was removed using a microscope slide. The segment was
cross-chopped at 350 µM using a McIlwain tissue chopper. The
resulting colonic slices were immediately suspended in 37°C KRB
gassed with O2/CO2 (19:1)
and then washed with KRB (37°C) three times. The slices were allowed
to incubate in KRB at 37°C gassed with
O2/CO2 (19:1) for 30 min.
In some experiments, segments of whole colon were first incubated with
AF-DX 116 and 4-DAMP mustard for 2 h before slicing of the tissue.
For these incubations, approximately 10 cm of colon was incubated in a
final volume of 330 ml of KRB buffer containing AF-DX 116 (1 µM) and 4-DAMP mustard (40 nM). The tissue was washed extensively to remove AF-DX 116 and any unreacted 4-DAMP mustard, and the tissue was sliced
as described above. To 10 ml of packed colonic slices, 8 ml of KRB
buffer containing 100 µCi of
myo-[3H]inositol was added, and the
mixture was incubated for 90 min. The slices were gassed with
O2/CO2 (19:1) every 30 min.
After this incubation, the slices were washed with KRB (37°C) three times. The slices were allowed to settle before pipetting 100-µl aliquots of slices into tubes with 0.35 ml of KRB (37°C) gassed with
O2/CO2 (19:1) containing 5 mM LiCl and various concentrations of oxotremorine-M without or with
antagonists in concentrations identified in Results. The
slices were incubated for 30 min in these tubes at 37°C. The
incubation was stopped by adding 1.13 ml of chloroform/methanol (1:2,
v/v). The accumulated inositol phosphates were extracted and separated
according to the method of Berridge et al. (1982), as described
briefly. Chloroform (0.37 ml) and water (0.37 ml) were added to the
tubes to separate the organic and aqueous phases. After centrifugation,
1 ml of the aqueous phase was pipetted into tubes to which 2 ml of
water was added. These tubes were centrifuged to sediment any
chloroform, and 2.9 ml of the aqueous phase was applied to a Dowex AG
1-X8 (100-200 mesh, 1 ml) anion exchange column. The column was washed three times with 5 ml of water each to remove
[3H]inositol and discarded.
[3H]Inositol phosphates were eluted from the
column with 2.5 ml of 1 M ammonium formate/0.1 M formic acid solution.
The elutant was then counted to determine the amount of radioactivity
using a scintillation counter. In some experiments and in all
experiments in which pertussis toxin-treated colonic slices were used,
200 µl of the organic phase was removed, dried, and then counted to determine the amount of [3H]inositol
incorporated into phospholipids. In these experiments, the amount of
[3H]inositol phosphates formed is calculated as
a percentage of the total amount of radioactivity in the organic phase
plus the inositol phosphate fraction. This was done to determine
whether there were differences in the uptake of
[3H]inositol in tissues treated with pertussis
toxin compared with tissues that were not treated with pertussis toxin.
In Vivo Pertussis Toxin Treatment.
Male Hartley guinea pigs
(300-400 g) were injected i.p. with pertussis toxin (50-100 µg/kg
b.wt.) 3 days before being euthanized for the in vitro experiments. For
the contractile assays, a dose of 100 µg/kg b.wt. pertussis toxin was
used, whereas in the phosphoinositide assays, a dose of 50 µg/kg
b.wt. pertussis toxin was used. Initial experiments showed that these
two doses yielded similar results in the phosphoinositide assay.
Data Analysis.
The concentration of oxotremorine-M eliciting
half-maximal contraction (EC50) was estimated by
nonlinear regression analysis according to an increasing logistic
equation as described previously (Candell et al., 1990).
The dissociation constant (KB) of the
antagonists AF-DX 116, pirenzepine, and
para-fluoro-hexahydro-sila-difenidol (p-F-HHSiD) were estimated from the shift that the antagonists caused in the oxotremorine-M concentration-response curve:
KB = [B]/(CR 
1). In this equation,
[B] represents the concentration of the antagonist, and
CR corresponds to the concentration ratio (the ratio of the EC50 value of oxotremorine-M measured in the
presence of the antagonist divided by that measured in the absence of
the antagonist).
The amount of receptor inactivation and the
pKA value were estimated using a
modification of the method of Furchgott (1966) as described previously
(Ehlert, 1987). Briefly, equieffective doses of oxotremorine-M were
obtained from the concentration-response curves before and after
treatment with 4-DAMP mustard. These estimates were fitted to the
following equation by nonlinear regression analysis:
![<UP>Log A</UP>=<UP>Log</UP>([<UP>A′</UP>K<SUB><UP>A</UP></SUB>q]/[K<SUB><UP>A</UP></SUB>+(1−q)A′])](/content/vol289/issue1/fulltext/464/img001.gif)
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(1)
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In this equation, A and A' correspond to
the concentration of oxotremorine-M eliciting equivalent contraction
before and after treatment with 4-DAMP mustard, q denotes
the proportion of inactivated receptors, and
KA denotes the affinity of the agonist for the receptor.
Significance values (p values) were calculated by using the
paired t test and are reported where appropriate.
Mathematical Modeling.
In this investigation, we examined
two mathematical models (model I and model II) for an interaction
between two receptor subtypes (M2 and
M3). In model I, activation of the
M3 receptor by itself causes contraction. The
M2 receptor has no effect by itself but can
greatly potentiate the contraction elicited by the
M3 receptor when activated. In model II,
occupation of the M3 receptor initiates the
activation of two parallel signaling pathways. One pathway causes a
direct contraction and is referred to as component A. The other pathway
has no effect by itself, but when activated in the presence of occupied
M2 receptor, a contraction ensues (component B).
The M2 receptor is incapable of eliciting
contractions by itself. Component B of model II is similar to model I
in that it represents an
M2/M3 interaction. However,
the contraction elicited by component B is conditional, occurring only
when both M2 and M3
receptors are activated. The mathematical derivation of these models is
described in Appendix and illustrated in Fig.
1.
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Fig. 1.
Schematic representation of two models for
interaction between M2 and M3 receptors. Solid
lines indicate contractile signals. Dashed lines indicate silent
signals that interact with another signal to elicit contraction.
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Materials.
Islet-activating protein (pertussis toxin) was
obtained from LIST Biological Laboratories (Campbell, CA).
myo-[3H]Inositol was from NEN
(Boston, MA). AF-DX 116 was from Boehringer Ingelheim Pharmaceuticals
(Ridgefield, CT). Pirenzepine, p-F-HHSiD, and oxotremorine-M
were from Research Biochemicals Inc. (Natick, MA). 4-DAMP mustard was
synthesized as described previously (Thomas et al., 1992). All
remaining drugs and chemicals were from Sigma Chemical Co. (St. Louis, MO).
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Results |
Effect of 4-DAMP Mustard Treatment on Contraction Elicited by
Oxotremorine-M Under Standard Conditions.
To investigate the
possible contribution of the M2 receptor to the
contractile response of the guinea pig colon, we treated colonic
segments with 4-DAMP mustard to inactivate M3
receptors. The isolated colon was incubated with the aziridinium ion of
4-DAMP mustard (40 nM) in the presence of AF-DX 116 (1 µM) for 1, 2, 3, or 4 h and then washed extensively. AF-DX 116 is used to
protect M2 receptors from alkylation by 4-DAMP
mustard. In the presence of AF-DX 116, the aziridinium ion of 4-DAMP
mustard has been shown to be an irreversible, muscarinic antagonist
that alkylates M3 receptors selectively over
M2 receptors (Thomas et al., 1993). Incubation of
the isolated colon with 4-DAMP mustard for 1, 2, 3, and 4 h caused
a progressive shift to the right and decrease in the maximum of the
concentration-response curve to oxotremorine-M (Fig.
2 and Table
1).
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Fig. 2.
Effects of 4-DAMP mustard treatment on contractile
response to increasing concentrations of oxotremorine-M under standard
conditions. Contractile measurements were made in tissues before ( )
and following 4-DAMP mustard treatment (40 nM) for 1 h ( ),
2 h ( ), 3 h ( ), and 4 h ( ). Each data point
represents mean ± S.E.M. of four to eight experiments.
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The effect of 4-DAMP mustard at 1, 2, 3, and 4 h corresponded to
receptor inactivation values of 93.7%, 97.6%, 98.8%, and 98.7%
(Table 1), respectively, as estimated according to the method of
Furchgott (see Experimental Procedures) assuming that a
single receptor type mediates the contractile response (Table 1). This
large inhibitory effect of 4-DAMP mustard is consistent with the
postulate that the M3 receptor mediates the
contractile response under standard conditions. It also appears that
the effect of 4-DAMP mustard reaches a limit of approximately 98%
receptor inactivation after 2 h of treatment, with little
additional alkylation at 4 h of treatment. These results suggest
that some of the M3 receptors are inaccessible to
4-DAMP mustard or that a 4-DAMP mustard-insensitive receptor (i.e.,
M2) contributes to the contractile response after
lengthy treatment with 4-DAMP mustard.
Effect of Pertussis Toxin on Contractile Response to
Oxotremorine-M.
We examined the effect of pertussis toxin on the
residual contractile response that persisted after 1- and 4-h treatment
with 4-DAMP mustard to determine whether the M2
receptor is contributing to the remaining contractile response.
Pertussis toxin treatment had no inhibitory effect on the contractile
response to oxotremorine-M when measured under standard conditions
(Fig. 3). In fact, a small potentiation
in contraction was observed at high concentrations of oxotremorine-M.
After 1- and 4-h 4-DAMP mustard treatment, however, pertussis toxin
caused a significant 25.4-fold (p = 3.1 × 10
4) and 72.5-fold (p = 8.5 × 106) increase in the
EC50 value of oxotremorine-M, respectively (Fig. 3, A and B). The sensitivity of the residual contraction to pertussis toxin suggests that the M2 receptor participates
in the contractile response, when a substantial portion of
M3 receptors are alkylated by 4-DAMP mustard.
This participation by the M2 receptor can explain why the effects of 4-DAMP mustard appear to reach a limit (see prior
discussion of Fig. 2).
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Fig. 3.
Effects of pertussis toxin treatment (, ) on
contractile response to oxotremorine-M in control ( , ) and 4-DAMP
mustard-treated tissues ( , ). Contractile responses were measured
in 1-h (A) and 4-h (B) 4-DAMP mustard-treated tissue. Each data point
represents mean ± S.E.M. of five to six experiments.
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Effect of AF-DX 116 on Contractile Response After 4-DAMP Mustard
Treatment.
If the M2 receptor is
contributing to the contractile response after 4-DAMP mustard
treatment, the remaining response may be antagonized by AF-DX 116 (M2- and M4-selective
antagonist) in a manner consistent with an
M2-mediated response. Isolated colonic segments
were treated with 4-DAMP mustard (40 nM) in the presence of AF-DX 116 (1 µM) for 4 h and then washed extensively as described in
Experimental Procedures. Treatment with 4-DAMP mustard
caused a 16.3-fold increase in the EC50 value of
oxotremorine-M (control EC50 = 94 nM) and a 60%
reduction in the maximal contractile response (control
Emax = 9.5g). This
suppression in maximal response was not as great as that observed in
similar experiments shown in Figs. 2 and 3, which we attribute to
experimental variation. The contractile response to oxotremorine-M was
determined in the absence and presence of 1 µM AF-DX 116 after 4-h
4-DAMP mustard treatment (Fig. 4). AF-DX
116 caused a significant 1.8-fold increase (p = 3.9 × 103) in the
EC50 value of the contractile response elicited
to oxotremorine-M. The pKB value for
AF-DX 116 estimated from this rightward shift (see Experimental
Procedures) was 5.9 ± 0.11, which is in close agreement with
the binding affinity (pKD = 6.10 ± 0.06) of AF-DX 116 at the human M3 receptor
transfected into Chinese hamster ovary cells (Esqueda et al., 1996).
Thus, the contractile response after 4-h 4-DAMP mustard treatment is
enigmatic; it is M2-like in its sensitivity to
pertussis toxin, yet it is M3-like in its weak
antagonism by AF-DX 116. AF-DX 116 (1.0 µM) also weakly antagonized the contractile response to oxotremorine-M measured before 4-DAMP mustard treatment (pKB = 6.07; see
Table 4).
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Fig. 4.
Effects of AF-DX 116 (1 µM) on contractile response
to oxotremorine-M in 4-h 4-DAMP mustard-treated tissues. Contractile
measurements were made in 4-DAMP mustard-treated colon in the absence
() and presence () of AF-DX 116 (1.0 µM). Each data point
represents mean ± S.E.M. of three experiments.
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Mathematical Modeling.
To explain the behavior of the
muscarinic contractile response in the guinea pig colon after 4-DAMP
mustard treatment, we investigated mathematical models for an
interaction between two receptor subtypes (M2 and
M3). We used a strategy based on the operational
model of Black and Leff (1983) to calculate the theoretical concentration-response curves. We also calculated the effects of AF-DX
116 and pertussis toxin treatment on the theoretical responses. Our
methods are described in Appendix.
The first model (model I) is based on the assumption that
oxotremorine-M elicits a contractile response through an interaction between M2 and M3
receptors. Activation of the M3 receptor causes smooth muscle contraction, whereas activation of the
M2 receptor has no effect by itself but greatly
potentiates the contraction elicited by the M3
receptor. Figure 5 shows the results of
these calculations. In this model, the affinity of the agonist is the same for both the M2 and M3
receptor; however, the sensitivities of the signals elicited by the two
receptors are varied, allowing us to modulate the contribution of
either receptor to the response (see Appendix). We therefore
describe three cases within model I: in case 1, the
M2 signal is less sensitive than the
M3 signal (Fig. 5A); in case 2, the sensitivities
of both the M2 and M3 receptor are the same (Fig. 5B); and in case 3, the
M3 signal is less sensitive than the
M2 signal (Fig. 5C). The effects of progressive
M3 receptor inactivation on this model are shown
in Fig. 5. The closed symbols show a response mediated by the
M2/M3 interaction, whereas
the open symbols show the response mediated solely by the
M3 receptor.
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Fig. 5.
Simulation of a response mediated through interaction
of an agonist with two receptors (i.e., M2 and
M3 receptors; model I). Response mediated by
M2/M3 interaction (filled symbols) was compared
with a response mediated solely by M3 receptor (open
symbols). Curves are shown before (, ) and after 90% (,  ),
99% (, ), and 99.8% (,  ) M3 receptor
inactivation. A, response of M2 receptor was less sensitive
than that of M3 receptor (KM2 = 0.1; KM3 = 0.01). B, response of
M2 and M3 receptors were equisensitive
(KM2 = 0.01; KM3 = 0.01). C, response of M3 receptor was less sensitive than
that of M2 receptor (KM2 = 0.001; KM3 = 0.01). Theoretical points for
M3 response and M2/M3 interaction
were calculated using eqs. 7 and 8, respectively, as described in the
Appendix.
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When the M2 signal is less sensitive to agonist
than the M3 signal (Fig. 5A), the
M2 receptor exhibits no potentiating effect on
the M3 response before receptor inactivation.
However, with progressive inactivation of M3
receptors, the potentiating effect of the M2
receptor becomes apparent (Fig. 5A and Table
2). Because pertussis toxin eliminates
signaling through the M2 receptor, the responses
mediated solely by the M3 receptor can be likened to the consequence of pertussis toxin treatment on the
M2/M3 interaction. Thus,
pertussis toxin treatment has no effect before receptor inactivation
but greatly inhibits the response measured after M3 receptor inactivation (Fig. 5A and Table 2).
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TABLE 2
Effects of M3 receptor inactivation, AF-DX 116 (1 µM), and
pertussis toxin on the response predicted by model I
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Cases 2 (Fig. 5B) and 3 (Fig. 5C) yield calculated responses that are
inhibited by pertussis toxin treatment before and after M3 receptor inactivation. These calculated
responses were inconsistent with the contractile response observed in
the guinea pig colon. The results are summarized in Table 2.
Figure 6 shows the effects of AF-DX 116 (1.0 µM) on the M2/M3
interaction calculated in case 1 before and after varying degrees of
M3 receptor inactivation. It can be seen that the
dextral shift in the concentration-response curve caused by AF-DX 116 is only 2.3-fold before M3 receptor inactivation.
As the degree of receptor inactivation increases to 99%, the dextral
shift increases to 5.5-fold. However, with further
M3 receptor inactivation (99.8%), the shift
declines to 3.6-fold. These results are summarized in Table 2 along
with the results from cases 2 and 3.
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Fig. 6.
Simulation of effects of AF-DX 116 and M3
receptor inactivation on response to an agonist mediated through
interaction of an agonist with two receptors (i.e., M2 and
M3 receptors; model I). Curves are shown before (, )
and after 90% (, ), 99% (, ), and 99.8% (, )
M3 receptor inactivation in the absence (filled symbols)
and presence (open symbols) of AF-DX 116 1 µM. Response of
M2 receptor was less sensitive than that of M3
receptor (KM2 = 0.1;
KM3 = 0.01). Each point was calculated using
eq. 8 as described in the Appendix.
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The results shown in Figs. 5A and 6 are similar to the behavior of the
guinea pig colon in that the contractile response is sensitive only to
pertussis toxin after 4-DAMP mustard treatment, not before. In
addition, the response is relatively insensitive to AF-DX 116 both
before and after extensive M3 receptor inactivation.
We also considered an alternative model (model II) for
M2/M3 receptor interactions
consisting of two components (A and B). Stimulation of
M3 receptors leads to the activation of two
parallel signaling pathways. One pathway causes a direct contraction of smooth muscle (component A). The other pathway has no effect by itself,
but it is required for M2 receptor-mediated
contractions (component B). By itself, the M2
receptor is incapable of eliciting contractions. Thus, component B
represents an M2/M3
interaction, with the response being conditional on stimulation of both
receptors. We show the behavior of component B in Fig. 8. In Figs. 9
and 10, we show the behavior of the complete model obtained by
combining both components (A plus B).
Figure 7 illustrates the effects of AF-DX
116 (1 µM) and M3 receptor inactivation on the
response of component A of model II. This response is highly sensitive,
so progressive receptor inactivation (90%, 99%, and 99.8%) causes a
sizable shift to the right in the concentration-response curve,
followed by a depression in its maximum (Table
3). With greater than 99.8% receptor
inactivation, the response is essentially eliminated. Assuming a
pKD value of 6.1 for the AF-DX
116-M3 receptor complex, it can be shown that AF-DX 116 should cause a 2.3-fold shift to the right in the
concentration-response curve before and after receptor inactivation.
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Fig. 7.
Simulation of effects of AF-DX 116 and M3
receptor inactivation on response to an agonist mediated through a
single receptor site (model II, component A). Curves are shown before
(, ) and after 90% (, ), 99% (, ), and 99.8% (,
) receptor inactivation in the absence (filled symbols) and presence
(open symbols) of AF-DX 116 (1 µM). Each point was calculated using
eq. 7 as described in the Appendix.
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TABLE 3
Effects of M3 receptor inactivation and AF-DX 116 (1 µM) on
the responses predicted by model II
The effects on components A and B and their combination are shown.
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Component B of model II is illustrated in Fig.
8. In component B, the affinity of the
agonist is the same for both the M2 and
M3 receptor; however, the sensitivities of the
signals elicited by the two receptors are varied, allowing us to
modulate the contribution of either receptor to the response (see
Appendix). We therefore describe three cases within
component B: in case B1, the M2 signal is less
sensitive than the M3 signal (Fig. 8A); in case
B2, the M3 signal is less sensitive than the
M2 signal (Fig. 8B); and in case B3, the
sensitivities of both the M2 and
M3 receptor are the same (Fig. 8C). Figure 8
shows the effects of AF-DX 116 (1 µM) on the contractile-response
curves of the model before and after selective inactivation of
M3 receptors.
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Fig. 8.
Simulation of effects of AF-DX 116 and M3
receptor inactivation on response mediated through interaction of an
agonist with two receptors (i.e., M2 and M3;
component B, model II). Curves are shown before (, ) and after
90% (, ), 99% (, ), and 99.8% (, ) M3
receptor inactivation in the absence (filled symbols) and presence
(open symbols) of AF-DX 116 (1 µM). A, response of M2
receptor was less sensitive than that of M3 receptor
(KM2 = 0.03; KM3 = 0.01). B, response of M3 receptor was less sensitive than
that of M2 receptor (KM2 = 0.003; KM3 = 0.01). C, response of
M2 and M3 receptors were equisensitive
(KM2 = 0.01; KM3 = 0.01). Each point was calculated using eq. 10 as described in the
Appendix.
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When the signal elicited by the M2 receptor is
less sensitive to the agonist than that elicited by the
M3 receptor (Fig. 8A), 90%
M3 receptor inactivation has little effect on the
concentration-response curve of component B1. Moreover, AF-DX 116 (1 µM) caused a large 20-fold dextral shift in the
concentration-response curve both before and after 90%
M3 receptor inactivation. However, as the degree
of M3 receptor inactivation increased to 99% and
99.8%, the concentration-response curve shifts to the right and shows a decrease in maximum (Table 3). Under these conditions, the dextral
shift caused by AF-DX 116 declined to 6.1- and 2.3-fold at 99% and
99.8% receptor inactivation, respectively. Thus, when the
M2 signal is less sensitive to the agonist than
the M3 signal, component B1 initially behaves
like an M2 response with high sensitivity to
AF-DX 116. However, as the degree of M3 receptor
inactivation increases, component B1 behaves more like an
M3 response with low sensitivity to AF-DX 116.
Figure 8B illustrates the response of component B2 when the
M2 signal is more sensitive to agonist than the
M3 signal. Under these conditions, the response
is highly sensitive to M3 receptor inactivation.
There was a progressive shift to the right followed by a decrease in
maximal response as the degree of M3 receptor inactivation increased (Table 3). AF-DX 116 (1 µM) caused a 6.3-fold increase in the EC50 value before
M3 receptor inactivation and 2.3-fold increases
after 90%, 99%, and 99.8% M3 receptor
inactivation (Table 3). Thus, when the M2 signal
is more sensitive to agonist then the M3 signal,
component B2 behaves more like an M3 response (i.e., compared with Fig. 8A) both before and after
M3 receptor inactivation.
When the sensitivities of the M2 and
M3 receptors are identical (Fig. 8C), the effects
of M3 receptor inactivation were similar to those
observed in Fig. 8B (Table 3). AF-DX 116 (1 µM) caused a large
12.6-fold dextral shift in the concentration-response curve before
M3 receptor inactivation. After
M3 receptor inactivation, AF-DX 116 caused 2.3- to 3.3-fold increases in the EC50 value (Table
3).
Having described the individual components of model II (A and B), we
calculated the complete model by combining the two components. Figure
9 shows the results of these
calculations. Figure 9A shows the composite response resulting from the
summation of components A and B1. It can be seen that increasing the
degree of M3 receptor inactivation causes a
progressive shift to the right and a decrease in the maximal response.
However, the effects of M3 receptor inactivation are not as great as those observed with a homogeneous
M3 receptor-mediated response, like component A
shown in Fig. 7. Thus, the summation of component A with component B1
yields a composite response that exhibits a refractoriness to
M3 receptor inactivation, like that observed in
the guinea pig colon (see Fig. 2). Moreover, this composite response is
relatively insensitive to AF-DX 116. At 1 µM, AF-DX 116 caused only
2.3- to 3.7-fold shifts in the concentration response curves both
before and after varying degrees of M3 receptor inactivation. These results are similar to those observed in the guinea
pig colon.
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Fig. 9.
Simulation of effects of AF-DX 116 and M3
receptor inactivation on combined response of model II (i.e.,
combination of components A and B). Curves are shown before (, )
and after 90% (, ), 99% (, ), and 99.8% (, )
M3 receptor inactivation in the absence (filled symbols)
and presence (open symbols) of AF-DX 116 (1 µM). A, response of
M2 receptor was less sensitive than that of M3
receptor (KM2 = 0.03;
KM3 = 0.01). B, response of M3
receptor was less sensitive than that of M2 receptor
(KM2 = 0.003; KM3 = 0.01). C, response of M2 and M3 receptors
were equisensitive (KM2 = 0.01;
KM3 = 0.01). Each point was calculated using
eq. 13 as described in the Appendix.
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Figure 9B shows the composite response derived from a combination of
components A and B2. Increasing amounts of M3
receptor inactivation caused a progressive dextral shift of the
concentration-response curve and a decrease in the maximum (Table 3).
After 99.8% M3 receptor inactivation, the
response was essentially eliminated. AF-DX 116 (1 µM) caused
2.3- to 2.6-fold increases in the EC50 value
before and after varying degrees of M3 receptor
inactivation (Table 3). Similar results were obtained for the composite
response derived from a combination of components A and B3 (Fig. 9C).
Compared with the model shown in Fig. 9A, the models of Figs. 9B and C were more sensitive to M3 receptor inactivation.
Figure 10A show the effects of
pertussis toxin on the composite response resulting from a combination
of components A and B1. It can be seen that the response is initially
insensitive to pertussis toxin; however, after progressive
M3 inactivation, the response becomes pertussis
toxin sensitive. These results are similar to those observed in the
guinea pig colon (see Fig. 3). The effects of pertussis toxin were
modeled by assuming that the toxin prevented M2
receptor signaling (see Appendix). The effects of pertussis
toxin on the composite responses derived by a combination of components A and B2 and a combination of components A and B3 are shown in Fig. 10,
B and C. It can be seen that these composite responses remained fairly
insensitive to pertussis toxin both before and after
M3 receptor inactivation.
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Fig. 10.
Simulation of effects of pertussis toxin treatment
and M3 receptor inactivation on combined response of model
II (i.e., combination of components A and B). Curves are shown before
(, ) and after 90% (, ), 99% (, ), and 99.8% (,
) M3 receptor inactivation before (filled symbols) and
after (open symbols) pertussis toxin treatment. A, response of M2
receptor was less sensitive than that of M3 receptor
(KM2 = 0.03; KM3 = 0.01). B, response of M3 receptor was less sensitive than
that of M2 receptor (KM2 = 0.003; KM3 = 0.01). C, response of
M2 and M3 receptors were equisensitive
(KM2 = 0.01; KM3 = 0.01). Theoretical points before and after pertussis toxin treatment
were calculated using eqs. 13 and 7 as described in the Appendix.
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Phosphoinositide Hydrolysis.
When transfected into cells in
high abundance, M2 receptors have been shown to
mediate a weak phosphoinositide response through a pertussis
toxin-sensitive G protein. Consequently, we investigated whether a
pertussis toxin-sensitive phosphoinositide response could be detected
in the guinea pig colon after inactivation of most of the
M3 receptors. Such a mechanism could account for
a direct, pertussis toxin-sensitive contractile response mediated by
the M2 receptor after inactivation of most of the
M3 receptors with 4-DAMP mustard. However, such a
response should be potently antagonized by AF-DX 116, which was not
observed in the guinea pig colon (see Fig. 4). Nevertheless, we wished
to explore the possible coupling of M2 receptors
to phospholipase C via a pertussis toxin-sensitive G protein. First,
we characterized the phosphoinositide response by measuring the ability
of the subtype-selective antagonists AF-DX 116, p-F-HHSiD,
and pirenzepine to shift the concentration-response curve for
oxotremorine-M-induced phosphoinositide hydrolysis to the right (Fig.
11). We estimated the
KB values of the antagonists from
these rightward shifts as described in Experimental
Procedures. These KB values are
listed in Table 4 together with the
binding affinities (KD values) of the
same antagonists measured in Chinese hamster ovary cells transfected
with the M2 and M3 subtypes
of the muscarinic receptor (Esqueda et al., 1996; Ehlert et al., 1997).
Also listed in Table 4 are the pKB for
the antagonists determined in contractile studies in the guinea pig
colon (Sawyer and Ehlert, 1998). The binding assays for these
KD estimates were conducted in a
HEPES-buffered KRB solution similar to that used in our contractile and
phosphoinositide hydrolysis assays. It can be seen that the
KB values of AF-DX 116, p-F-HHSiD, and pirenzepine are in agreement with their
respective KD values for the
M3 receptor but not with those of the
M2 receptor (Table 4). These values also were in
close agreement with the values obtained previously from contractile
studies conducted in the guinea pig colon (Table 4). There also was a
lack of agreement between the antagonist KB values of AF-DX 116, p-F-HHSiD, and pirenzepine and their respective KD values for the
M1 (6.24, 7.08, 7.77), M4
(6.96, 7.08, 7.23), and M5 (5.29, 6.26, 6.55)
subtypes, as reported by Esqueda et al. (1996) and Ehlert et al.
(1997). Therefore, we conclude that the M3
receptor mediates phosphoinositide turnover in the guinea pig colon
under standard conditions.
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Fig. 11.
Competitive antagonism of phosphoinositide response
to oxotremorine-M in guinea pig colon. Phosphoinositide response to
oxotremorine-M in the absence () and presence () of p-F-HHSiD
(0.1 µM) (A), AF-DX 116 (1 µM) (B), and pirenzepine (1 µM) (C).
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View this table:
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TABLE 4
pKB values for antagonism of oxotremorine-M-induced
phosphoinositide hydrolysis in guinea pig colon by AF-DX 116, pirenzepine, and p-F-HHSiD compared with
pKB obtained from contractile studies in the guinea
pig colon and binding affinities (pKD) at the human
M2 and M3 receptors transfected into Chinese hamster
ovary cells
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Effect of 4-DAMP Mustard Treatment and Pertussis Toxin on
Phosphoinositide Hydrolysis Elicited by Oxotremorine-M.
We
measured the pertussis toxin sensitivity of the phosphoinositide
response both before and after 4-DAMP mustard treatment to investigate
the possible contribution of the M2 receptor to the response. Colonic slices were incubated with 4-DAMP mustard (40 nM)
in the presence of AF-DX 116 (1 µM) for 2 h and washed extensively. Incubation for 2 h with 4-DAMP mustard caused a
significant 9.34-fold (p = 1.5 × 105) increase in the EC50
value and a 60% reduction in the maximal response to oxotremorine-M
(Fig. 12). As in the functional assays, pertussis toxin did not affect the response to oxotremorine-M; in fact,
there was a slight increase in the hydrolysis of phosphoinositides (Fig. 12). Unlike the contractile experiments, however, pertussis toxin
had no inhibitory effect on phosphoinositide hydrolysis after 2-h
4-DAMP mustard treatment (Fig. 12). In fact, there was a slight
potentiation of the response as well. Consequently, the M2 receptor does not appear to couple with a
phosphoinositide signaling pathway to rescue the contractile response
after 4-DAMP mustard treatment.
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Fig. 12.
Effects of pertussis toxin treatment on
phosphoinositide response to oxotremorine-M in control and 2-h 4-DAMP
mustard-treated colon. Phosphoinositide hydrolysis was measured in 2-h
4-DAMP mustard-treated (, ) and untreated (, ) colon from
pertussis toxin-treated (, ) and untreated (, ) guinea
pigs. Each data point represents mean ± S.E.M. of four
experiments.
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Discussion |
There is an abundance of data on smooth muscle demonstrating that
it is primarily the M3 receptor that mediates
contraction to muscarinic agonists in the absence of other contractile
and relaxant agents (Eglen, 1996; Ehlert et al., 1997). This condition occurs in variety of smooth muscle types, including the circular and
longitudinal muscles of the colon (Zhang and Buxton, 1991; Sawyer and
Ehlert, 1998). The data of the present report are also consistent with
this hypothesis; the contractile response was sensitive to 4-DAMP
mustard and insensitive to pertussis toxin and the
M2-selective antagonist AF-DX 116.
However, a different picture emerges when we consider the residual
contractile response that persisted after selective inactivation of
most of the M3 receptors with 4-DAMP mustard.
This response was highly sensitive to pertussis toxin and relatively
insensitive to 4-DAMP mustard. Both of these characteristics suggest an
M2 receptor mechanism; but the contractile
response was relatively insensitive to the
M2-selective antagonist AF-DX 116. To explain this enigma, we suggest that the response may represent an interaction between M2 and M3
receptors. Accordingly, the M2 receptor may mediate contractions through some mechanism that depends on a low level
of signaling through the M3 receptor. By itself,
this low level of M3 signaling is insufficient to
generate a sizable contraction, yet it enables activated
M2 receptors to elicit contraction. The results
of our mathematical analysis are not inconsistent with this hypothesis.
We considered two models for the interaction between
M2 and M3 receptors. In
both models, it was assumed that activation of M2
receptors has no effect by itself, but M2
receptors can interact with M3 receptors to
trigger a contraction. In the first model (model I), it was assumed
that the M2 receptor simply potentiated the
contractile response of the M3 receptor. This
model yielded results similar to the behavior of the colon when it was
assumed that oxotremorine-M elicits contraction through the
M3 receptor with greater potency than that with
which it activates the potentiating M2 signal
(case 1). Under this condition, oxotremorine-M can elicit a maximal
contraction through the M3 receptor at
concentrations that are insufficient to activate the
M2 pathway. Thus, the M2 receptor does not contribute to the contraction in untreated tissue, and consequently, the response is pertussis toxin insensitive. However,
after inactivation of most of the M3 receptors,
the M2 receptor contributes to the contraction,
rendering it sensitive to pertussis toxin. Model I, case 1, also
predicts that AF-DX 116 should cause only a 2.3- to 3.6-fold shift to
the right in the concentration-response curve both before and after
extensive M3 receptor inactivation. Such results
were observed in the colon. After a moderate degree of
M3 receptor inactivation, model I, case 1, predicts that AF-DX 116 (1.0 µM) should cause a 4.2- to 5.5-fold
dextral shift in the concentration-response curve. The largest shift
that we observed for AF-DX 116 after a moderate degree of receptor
inactivation was 4.3-fold (Sawyer and Ehlert, 1998).
We also investigated an additional model (model II) that provided a
somewhat better approximation of our data in the colon. Model II is
based on the assumption that the M3 receptor
signals through two parallel pathways. The first pathway gives rise to a simple M3 receptor-mediated contraction
(component A), and the second pathway is silent by itself but interacts
with a silent M2 receptor to generate a
contraction (component B) (see Fig. 8). Component A is more sensitive,
so when contractile responses to oxotremorine-M are measured in
untreated tissue, the contractions are due to activation of
M3 receptors. However, after selective inactivation of M3 receptors, the sensitivity of
component A is greatly reduced so component B becomes the more
sensitive component.
Our analysis of component B provides an understanding of the
competitive antagonism of a response to an agonist that is mediated through an interaction between two receptors. We have shown that there
is a tendency for the antagonism to resemble that predicted for the
less sensitive receptor mechanism. Consider an example where receptor X
interacts with receptor Y to trigger a response. If the signal elicited
by receptor X is less sensitive than that elicited by receptor Y, then
the nature of the competitive antagonism of the interaction will tend
to resemble that predicted for receptor X. If a highly Y-selective
competitive antagonist is used, its calculated
pKB value will be less than that of
the Y receptor and may approach that of the X receptor. On the other
hand, if an X-selective antagonist is used, its calculated
pKB value will be equivalent to that
of the X receptor.
Model II agreed best with the contractile data when it was assumed that
the M3 signal of component B was more sensitive
than the M2 signal (i.e., the conditions of model
II, B1). Under these conditions, the model predicts that the
competitive antagonism of component B1 by AF-DX 116 (1.0 µM) should
resemble that expected for the less sensitive receptor signaling
pathway: M2. This antagonism was manifest as a
relatively large AF-DX 116-induced shift (19.6-fold) in the
concentration-response curve of component B1 (see Fig. 8A).
Nevertheless, the complete response obtained by combining components A
and B1 exhibited relatively low sensitivity to AF-DX 116 (1 µM) (see
Fig. 9A). This behavior can be explained by the greater sensitivity of
component A, which is capable of mediating a maximum contraction at
agonist concentrations that are insufficient to elicit a response
through component B1. It is only after M3 receptors are inactivated that component B1 dominates the contractile response. However, under these conditions, the M3
signal of component B1 is less sensitive than the
M2 signal, and consequently, the competitive
antagonism of component B1 resembles that expected for an
M3 response, with low sensitivity to AF-DX 116. As a result, the complete response (i.e., the combination of components
A and B1) exhibited relatively low sensitivity to AF-DX 116 both before and after varying degrees of M3 receptor
inactivation. However, careful inspection of the theoretical curves
shows that the shift in the concentration-response curved caused by
AF-DX 116 (1.0 µM) increased from 2.3-fold before receptor
inactivation to 3.7-fold after 90% inactivation of
M3 receptors. With further receptor inactivation,
the AF-DX 116-induced shift declined to 2.3-fold. Interestingly, we
observed a similar phenomenon in the guinea pig colon. We found that
the shift in the concentration response curve caused by AF-DX 116 increased from 2.2-fold in untreated tissue to 4.3-fold after 2-h
4-DAMP mustard treatment (Sawyer and Ehlert, 1998). After 4-h
treatment, the AF-DX 116-induced shift returned to a low value of
1.8-fold (see Fig. 4).
So far, we have no direct evidence on the possible signaling mechanisms
involved in the interaction between M2 and
M3 receptors. Nevertheless, it is interesting to
note that muscarinic agonists trigger a nonselective cation conductance
in smooth muscle (Benham et al., 1985; Inoue and Insenberg, 1990a).
This conductance is pertussis toxin sensitive, and it is enhanced by
calcium, particularly in the colon, where the response is completely
dependent on calcium (Inoue and Insenberg, 1990b; Lee et al., 1993).
The pertussis toxin sensitivity and the calcium requirement suggest a
mechanism involving both M2 and
M3 receptors. Bolton and Zholos (1997) have shown
that the competitive antagonism of the muscarinic-induced cation
conductance is consistent with a response mediated by both the
M2 and M3 receptors.
Perhaps this conductance is involved in the interaction between
M2 and M3 receptors.
The low sensitivity of the postulated interaction between
M2 and M3 receptors raises
the question of its physiological significance. What function could the
interaction have if muscarinic agonists are capable of eliciting
contraction through a more potent M3 mechanism?
This question is particularly relevant if the nature of the interaction
simply involves an M2 receptor-mediated
potentiation of M3 receptor-mediated contractions
(model I). However, if the interaction involves an
M2 potentiation of an alternate
M3 signal that is incapable of eliciting
contraction by itself (model II), then this mechanism could function in
isolation of the standard M3 receptor-mediated
contraction. Moreover, it could have a pattern of distribution distinct
from that of the standard M3 receptor mechanism,
making it the dominant mechanism at some neuroeffector junctions.
This appendix describes our calculations for generating the
theoretical concentration-response curves for the two models of M2 and M3 receptor
interactions. Some general calculations that apply to both models are
described first. Later, we describe the specific details of each model
in Model I and Model II.
In our analysis, we assumed that occupancy obeys the law of mass-action
and that the concentration-response curve of the agonist obeys a
logistic equation. These assumptions are valid because 1) the intact
cell contains high concentrations of GTP and the binding of agonists to
M2 and M3 muscarinic
receptors obeys mass-action behavior when measured in the presence of
guanine nucleotides (Ehlert and Yamamura, 1995) and 2) the
concentration-response curves of muscarinic agonists in the guinea pig
colon and ileum typically obey a logistic equation with Hill
coefficients of approximately 2. Black and Leff (1983) have shown that
if occupancy obeys mass-action behavior and the concentration-response
curve obeys logistic behavior, then the relationship between occupancy
and response must also be logistic. Consequently, we calculated the
response (R) using the following logistic
equation:
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Abstract
Introduction
![<UP>Occupancy</UP>=q[A]/([A]+K<SUB><UP>D</UP></SUB>(1+[I]/K<SUB><UP>I</UP></SUB>))](/content/vol289/issue1/fulltext/464/img004.gif)
![S<SUB><UP>M2</UP></SUB>=q[A]/[[A]+10<SUP><UP>−</UP>5</SUP>(1+[I]/5.4×10<SUP><UP>−</UP>8</SUP>)]](/content/vol289/issue1/fulltext/464/img005.gif)
![S<SUB><UP>M3</UP></SUB>=q[A]/[[A]+10<SUP><UP>−</UP>5</SUP>(1+[I]/7.9×10<SUP><UP>−</UP>7</SUP>)]](/content/vol289/issue1/fulltext/464/img006.gif)
