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Vol. 284, Issue 2, 500-507, February 1998
Departments of Pharmacology (I.K., H.I.Y., E.V.V., W.R.R.), Biochemistry (H.I.Y.), Psychiatry (H.I.Y.), Program for Neurosciences (H.I.Y., W.R.R.) and Medicine (S.L.W., W.R.R.), The University of Arizona, Health Sciences Center, Tucson, Arizona
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Abstract |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The coding sequence of the human m2 receptor gene was amplified
by polymerase chain reaction and stably transfected into a murine
fibroblast cell line (B82). We have compared the human M2 clonal cell
line (HM2-B10) with the previously established B82 cell line
(M2LKB2-2) expressing the rat M2 receptor to assess drug specificity,
drug selectivity and effector coupling. Both transfected cell lines
showed a high level of specific, saturable [3H](
)-N-methyl-3-quinuclidinyl benzilate binding with
Kd values of 243 pM (155-352 pM)
and 345 pM (234-539 pM) and Bmax values of
97 ± 4 and 338 ± 16 fmol/106 cells,
respectively. Inhibition of
[3H]()-N-methyl-3-quinuclidinyl benzilate binding to
HM2-B10 cells and M2LKB2-2 cells showed the same rank order of potency
for the antagonists: atropine > dexetimide > 4-diphenylacetoxy-N-methylpiperidine methiodide > himbacine > methoctramine > 11-[[2-[(diethylamino) methyl]-1-piperidinyl]acetyl]-5,11-dihidro-6H-pyrido-[2,3-b](1,4)-benzodiazepine-6-one > hexahydro-sila-difenidol hydro-chloride > pirenzepine. Correlation analysis of the
pKi values indicate that the
expressed human and rat M2 receptors have nearly identical
ligand-binding characteristics. Carbachol inhibited
forskolin-stimulated cAMP formation with similar potency in both cell
lines [EC50 = 2.4 µM (0.2-2.8) and 1.1 µM (0.2-5.3)
for the human and rat M2 receptor, respectively]. In the M2LKB2-2
cells, carbachol slightly stimulated the [3H]inositol
monophosphate formation but had no significant effect in HM2-B10 cells.
In conclusion, the human and rat M2 receptors expressed in the B82 cell
line have very similar binding properties but exhibit slight
differences in effector coupling mechanisms.
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Introduction |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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mAChRs
have been classified pharmacologically into three subtypes (M1, M2 and
M3) according to their affinities for different antagonists (Hammer
et al., 1980
). Conventional pharmacological studies on
muscarinic receptors have been difficult because of the lack of
subtype-specific ligands and the fact that different tissues express a
mixture of different subtypes. The muscarinic receptors of the heart
belong predominantly to the M2 subtype, although a small population of
M1 sites also are present (Sharma et al., 1997; Watson
et al., 1983). The M2 receptor has very important regulatory
control over heart rate (negative chronotropic) and myocardial
contractility (negative inotropic). Many cardiac and noncardiac drugs
bind to these receptors, causing serious side effects. A number of
models have been used to study the cardiac muscarinic receptors.
Primary cultures of myocytes from adult or fetal rat heart are hard to
maintain and are contaminated with other cell types. Furthermore,
myocyte cultures are obtained from animal (mostly rat) tissues,
although ultimately, pharmacological data must be obtained for drugs
used in humans.
Molecular biological techniques have made possible the separate
characterization of a single receptor population in transfected mammalian cells expressing a high density of a particular receptor subtype. Five muscarinic receptor genes (m1-m5) (Bonner et
al., 1987, 1988; Kubo et al., 1986a, 1986b; Peralta
et al., 1987a, 1987b) encoding highly related receptor
proteins have been cloned from different species. The human (Peralta
et al., 1987a) and the rat (Lai et al., 1990) m2
receptor show 100% amino acid homology in the putative transmembrane
and extracellular loop regions. Site-directed mutagenesis and affinity
labeling experiments implicate these regions in the ligand binding;
therefore, the binding characteristics of the rat and human M2
receptors are expected to be very similar. However, the results
available in the literature for the cloned M2 receptors indicate
species differences for the affinity of AF-DX 116 (11-[[2-[(diethylamino)methyl]-1-piperidinyl]acetyl]-5,11-dihidro-6H-pyrido-[2,3-b](1,4)-benzodiazepine-6-one) and PZ (Akiba et al., 1988; Buckley et al., 1989;
Lai et al., 1990).
The cloned M2 receptor is known to be inversely coupled to cAMP
formation (Peralta et al., 1988) and has some stimulatory effect on IP1 formation. The differences between
the rat and the human M2 receptors are found almost exclusively in the
putative third intracellular loop region (fig.
1). The third intracellular loop is
thought to have an important role in determining the specificity of the
G protein coupling. This suggests that there can be some differences in
the second-messenger coupling between the human and rat M2 receptors.
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The rat m2 gene expressed in vitro in mammalian cells showed
the characteristics of the pharmacologically defined M2 receptors (Lai
et al., 1990). In our study, we report the cloning and
expression of the human M2 receptor in the B82 fibroblast cell line. To
examine the possible species differences, we compared the binding
properties and effector coupling of the human M2 receptor with those of
the rat M2 receptor, both expressed in the same B82 cell line using whole-cell preparations and physiological conditions. In addition, we
performed radioligand binding assays on the human clone with several
nonmuscarinic compounds (including nicotinic, cardiac and neuroleptic
drugs) to examine possible drug interactions.
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Methods |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Amplification of the coding sequence of the human muscarinic m2
receptor gene by PCR.
The open reading frame of the human m2
receptor gene was amplified from human placental genomic DNA (Clontech,
Palo Alto, CA) by PCR (Saiki et al., 1985). Two specific
primers based on the human cardiac m2 receptor gene sequence (Peralta
et al., 1987a) were synthesized using a Cyclone Plus DNA
synthesizer (Milligen Bio-Research, Wovajo, CA). The primers were
purified by anion exchange chromatography, using OLIGO-PACK columns
(Milligen/Biosearch, Burlington, MA).
primer (5-ACGTCGACATGAATAACTCAACAAACTCC-3) carried
a SalI restriction site (underlined) as a linker. The 3
primer included a HindIII restriction site linker sequence
(underlined): 5-CGAAGCTTTTACCTTGTAGCGCC-TATGTT-3). The
PCR amplification was carried out in a Programmable Cyclic Reactor
(Ericomp, San Diego, CA). In the reaction, we used Taq DNA
polymerase and Gene Amp DNA amplification kit (Perkin-Elmer Cetus,
Norwalk, CT). The reaction mixture contained 200 µM concentration of
each dNTP, 1 µg of each primer and 1 µg of the human genomic DNA.
The conditions were the following: initial denaturation at 94°C for 2 min, annealing at 55°C for 20 sec, chain extension at 72°C for 1 min, denaturation at 94°C for 20 sec (25 cycles) and a final
extension step of 10 min at 72°C. The PCR product was analyzed on
0.8% agarose gel and isolated from the gel by electroelution.
Subcloning and sequencing.
The purified PCR product was
subcloned into pGEM3Zf() vector (Promega, Madison, WI) with the
homopolymer tailing method (Boehringer-Mannheim Biochemica, Mannheim,
Germany) using poly(G)-tail on the PCR product and poly(C)-tail on the
vector. The sequence of the subcloned DNA was determined by the
dideoxy-chain termination method (Sanger et al., 1977) using
Sequenase Version 2.0 sequencing kit (United States Biochemical,
Cleveland, OH) on 5% polyacrylamide gel prior to autoradiography. The
sequence data were analyzed with the Genepro DNA analysis program
(Hoeffer Scientific, San Francisco, CA) and the comparison with the
published hm2 sequence showed 100% homology.
In vitro expression of the human m2 muscarinic
receptor gene in murine fibroblast (B82) cell line.
The cloned and
sequenced DNA was excised from the recombinant pGEM3Zf() with
SalI and HindIII restriction enzymes. The
fragment was ligated into the expression vector pH
APr-1-neo (a gift
from Dr. L. Kedes, Stanford University, Stanford, CA), which has a SalI/HindIII cloning site downstream from the
human -actin promoter (Gunning et al., 1987).
). The transfected cells were selected for
the expression of neomycin resistance with 500 µg/ml geneticin (G418;
GIBCO BRL, Grand Island, NY). Clones with stable, high-affinity
[3H]()-MQNB binding were maintained in a
nonselecting medium (5% fetal calf serum, 5% newborn calf serum, 45%
Ham's F-12, 45% Dulbecco's modified Eagle's medium, 100 U/ml
penicillin and 100 µg/ml streptomycin) in a humidified atmosphere
with 95% air/5% CO2.
All assays were carried out on intact cells; 50 000 cells/well were
plated out onto 24-well titer plates (Costar, Cambridge, MA) 48 hr
before each assay. The cells were counted on the day of the assay. G418
was omitted throughout these experiments.
Radioligand binding assays.
[3H]()-MQNB (87.4 Ci/mmol; New England
Nuclear, Boston, MA) binding assay on the intact transfected B82 cells
was carried out as described previously (Mei et al., 1989b).
The saturation assays were performed using 32.5 to 951 pM
[3H]()-MQNB.
Ligand/[3H]()-MQNB competition assays were
carried out using 10 concentrations of the competing ligands and an
average concentration of 341 pM [3H]()-MQNB.
The ligands used include atropine sulfate, carbachol, quinidine (all
from Sigma Chemical, St. Louis, MO); AF-DX 116, PZ (both were gifts
from Dr. K. Thomae, Biberach, Germany); 4-DAMP, methoctramine,
d-tubocurarine, hemicholinium-3, gallamine, HHSiD, dexetimide, levetimide (from RBI, Natick MA); himbacine (gift from Dr.
W. Taylor); and procainamide (gift from Squibb Institute) Both
saturation and competition assays were conducted in 1 ml of IMDM at
37°C for 3 hr. Specific binding was determined as the amount of
binding inhibited by 1 µM atropine sulfate. Radioactivity was
measured by liquid scintillation counting (Searle Analytic 81; 45%
efficiency.)
cAMP formation assay.
The cAMP formation studies were
performed according to a modified method of Gilman (1970). The cAMP
formation was stimulated with l00 µM forskolin
[(7-deacetyl-7-
-N-methylpiperazino)-butyryl dihydrochloride]
(Cal-Biochem, La Jolla, CA) in the presence of 5 mM IBMX (Sigma, St.
Louis, MO) in IMDM for 3 min at 37°C, with or without 10 pM to 10 mM
carbachol or 1 µM atropine. The preparation of the cell extracts and
the measurement of the cAMP content were carried out as described
previously (Mei et al., 1989a).
Inositol lipid hydrolysis studies.
A method modified from
that described by Berridge et al. (1982) was used to measure
the accumulation of
[3H]IP1 after the
stimulation by 100 pM to 10 mM carbachol with or without 1 µM
atropine in the presence of 10 mM lithium chloride. The experimental
procedure was essentially described previously (Mei et al.,
1989b) with 5 mM sodium tetraborate/60 mM sodium formate instead of
myoinositol during ion exchange chromatography before eluting the
[3H]IP1 with 2 ml of 0.2 M ammonium formate/0.1 M formic acid. The radioactivity in the eluate
was determined by liquid scintillation spectrophotometry.
Data analysis.
The ligand binding data were analyzed by
logistic nonlinear least-squares analysis using a computerized
iterative procedure developed by S. Yamamura for the Apple computer. In
the inhibition experiments, the IC50 values were
corrected to Ki values using the
Cheng-Prusoff equation (1973), results are presented as the geometric
mean (range).
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Results |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The PCR using the two gene-specific primers for the human M2
muscarinic receptor yielded the selective amplification of a 1.4-kb DNA
fragment from human genomic DNA. The fragment was subcloned into
pGEM3Zf() vector and sequenced. The sequence analysis showed 100%
homology with the published sequence.
In vitro expression and characterization of the
amplified human m2 muscarinic receptor gene in the murine fibroblast
(B82) cell line.
The untransfected B82 cells did not exhibit any
specific [3H]()-MQNB binding. After the
transfection, 26 clones selected by G418 resistance showed high-level
specific binding for [3H]()-MQNB. One of the
clones, HM2-B10, which had the highest specific binding for
[3H]()-MQNB, was chosen for the
pharmacological characterization. In parallel with each experiment on
the human HM2-B10 cell line, we did the pharmacological
characterization on the rat M2LKB2-2 cells (Lai et al.,
1990).
Pharmacological characterization.
The G418-resistant clonal
cell line HM2-B10 showed a high level of specific, saturable
[3H]()-MQNB binding (fig.
2A) with a
Kd value 243 pM (155-352 pM) and
Bmax value of 96.8 ± 3.8 fmol/106 cells. The parallel experiment with the
rat M2LKB2-2 showed a Kd value of
345 pM (234-539 pM) and a Bmax value
338 ± 16 fmol/106 cells (fig. 2B). During
the 6-month experiment period, the density of
[3H]()-MQNB binding sites remained stable.
Inhibition of [3H]()-MQNB binding to HM2-B10
cells and to M2LKB2-2 cells by several antagonists and the agonist
carbachol is shown in figure 3.
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)-MQNB binding was atropine > himbacine > methoctramine > AF-DX 116 > PZ. Carbachol
inhibited [3H]()-MQNB binding on the HM2-B10
cells with a Ki value of 1.8 µM
(1.7-1.9 µM) and a pseudo-Hill coefficient of 1.1 ± 0.33. These results are characteristic of the pharmacologically defined M2 type receptor that predominates in cardiac tissue (Watson et
al., 1986). We performed competition assays with 13 muscarinic
drugs. The inhibition constants (Ki
values) for these muscarinic drugs and the pseudo-Hill coefficients of
the respective ligand/[3H]()-MQNB competition
isotherms for the human and rat M2 cells are summarized in table
1.
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). In the present study, we tested the
ability of the same 52 nonmuscarinic drugs to compete for
[3H]()-MQNB binding sites on the human
HM2-B10 cells under physiological buffer conditions. The
Ki values and pseudo-Hill
coefficients for the most potent drugs are shown in table
2. The nicotinic drugs decamethonium and
d-tubocurarine as well as the choline reuptake inhibitor
hemicholinium-3 had potency in inhibiting
[3H]()-MQNB binding with
Ki values in micromolar
concentrations. The commonly used antiarrhythmic agents quinidine and
procainamide also had a Ki value in
the low micromolar range. The tricyclic antidepressant imipramine had a
Ki value of 0.13 µM, which may account for its cardiotoxicity. Other compounds that were able to
inhibit [3H]()-MQNB by 40% to 50%
concentrations of 100 µM include the beta adrenergic
blockers labetalol and metoprolol, the beta adrenergic agonist dobutamine, the K+-sparing diuretics
spironolactone and amiloride, the cholesterol synthesis inhibitor
lovastatin and the phosphodiesterase inhibitor papaverin. The ability
of glycerin to inhibit [3H]()-MQNB binding by
68% even at 10 µM is probably due to nonspecific membrane
perturbations.
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Functional coupling of the expressed mAChRs to cAMP formation.
Forskolin elevated the cellular cAMP level in a dose-dependent manner
in both the transfected and nontransfected B82 cells. Forskolin (100 µM) elicited a maximal stimulation of cAMP formation that was 10-fold
over the basal level. In the nontransfected B82 cells, carbachol had no
effect on forskolin-stimulated cAMP formation (Mei et al.,
1989a).
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Effect of carbachol on the hydrolysis of inositol lipids in the
transfected cells.
In the nontransfected B82 cells, 100 µM
carbachol has no effect on the basal
[3H]IP1 accumulation (Mei
et al., 1989b). The basal
[3H]IP1 accumulation was
the same in the HM2-B10 and M2LKB2-2 cells. Carbachol at 100 pM to 10 mM had no significant stimulatory effect in the human M2 cells
(F = .6, P = NS, fig.
6A). In the rat M2 cells, the agonist
carbachol significantly (t = 2.5, P < .05) stimulated the [3H]IP1
accumulation at 10 µM concentration with an
Emax value of 1.8 ± 0.24-fold over the
basal level. With the increase of the carbachol concentration, the
level of the [3H]IP1
accumulation declined. This response to the agonist was totally
abolished by the addition of 1 µM atropine.
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| |
Discussion |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The human m2 receptor gene was amplified by PCR and expressed in
the murine fibroblast B82 cell line, which previously lacked mAChRs.
Binding and functional comparisons in parallel experiments were carried
out with the previously cloned rat m2 receptor gene expressed in the
B82 cells. The results of these studies are (1) the human m2 gene was
successfully expressed in the B82 cells, (2) the human and rat m2
receptors bound [3H]()-MQNB with similar
Kd values, (3) the
pKi comparison showed high similarity
between the rat and human clones for 13 muscarinic drugs, (4) the human
M2 clone showed significantly lower inhibition of the forskolin
stimulated cAMP formation, and (5) the human clone had no significant
effect on the [3H]IP1
hydrolysis.
Recombinant cell lines expressing a single population of receptors are valuable tools for the primary, high-throughput screening of compounds with potential use in human pharmacotherapy. They also provide inexpensive and rapid means to test the cross reactions of drugs with a wide variety of cell lines expressing different nontarget receptors to determine the possible side effects. On the other hand, in the final stage of drug testing before the human clinical trials, in vivo animal experiments (most frequently rat) are still indispensable. It is important, therefore, to examine the validity of data obtained from rat tissues for a potential human drug.
In addition to this simple utilitarian point of view, recombinant cell lines further our knowledge about the mechanisms of the drug action. Accumulating results from using different cell lines for the expression of the same receptor called our attention to the tissue specificity of the drug response. It is becoming increasingly clear that the cellular environment (G protein and effector pool) and the density of the expressed receptors can modify the response to the same drug even when it acts through the same receptor. To understand the complexity of the action of a drug in a living organism and to be able to select a valid model for drug screening, more pharmacological data are needed from recombinant cell lines.
By cloning the human muscarinic m2 receptor gene, we were able to
compare the human and rat muscarinic M2 receptors expressed in the same
B82 cell line. The deduced amino acid sequence comparison between the
human and the rat m2 receptor genes showed 96% homology. This is
higher than expected because the rat m2 gene cloned in our laboratory
(Lai et al., 1990) is slightly different from that previously published (Gocayne et al., 1987). Based on the
amino acid sequence identity between the two genes in the transmembrane domains, we expected very similar binding properties. The differences between the two receptor proteins are located almost exclusively in the
third intracellular loop. The regions of the third intracellular loop
adjacent to the transmembrane domains are known to have a role in the
coupling of the receptors to G proteins (Lechleiter et al.,
1990; Wess et al., 1990, 1997). These regions are completely homologous between the human and rat receptors, whereas the middle section of the loop contains a number of substitutions. It is not known
what effect these substitutions have on the secondary structure of the
loop and, therefore, on the G protein-coupling specificity. On the
other hand, ligand binding and G protein coupling are allosteric
processes, so it is conceivable that the differences in the
conformation of the intracellular loop might have an allosteric effect
on the ligand binding.
To compare the ligand binding and second-messenger coupling characteristics of the rat and human M2 receptors, the open reading frame of each gene was cloned from genomic DNA by PCR (the muscarinic receptor genes have no introns) and transfected by the same method into the same cell line using the same expression vector. It is well known that the binding affinity of a ligand to the receptor is modified by both intracellular and extracellular conditions. The relationship between the high- and low-affinity states in the signal transduction process is not established; however, it is reasonable to assume that the initial encounter between the ligand and the receptor in living tissue happens under physiological ion and nucleotide concentrations, and therefore affinity values measured under these conditions will determine the occupancy of the receptors. For this reason in the binding experiments, we used whole-cell preparations, and the assays were conducted in IMDM medium (1.5 mM Ca++, 4.8 mM K+, 0.8 mM Mg++ and 115 mM Na+) at 37°C.
The transfected cells exhibited stable, specific, high-affinity
[3H]()-MQNB binding. The
Kd values were approximately the same in the human and rat clonal cell line. The
Bmax value of the human HM2-B10 cells was
3.5 times lower than the Bmax value of the
rat M2LKB2-2 cells (96.9 ± 3.8 and 338 ± 16 fmol/106 cells, respectively). These values
correspond to 510 fmol/mg protein for the HM2-B10 cells and 1778 fmol/mg protein for the M2LKB2-2 cells. The density of muscarinic
receptors in heart tissue homogenates shows a 3-4-fold difference for
different species (Fields et al., 1978). The maximal number
of [3H]()-QNB binding sites is 57 fmol/mg
tissue in rabbit heart, 144 fmol/mg tissue in rat heart and 178 fmol/mg
tissue in guinea pig heart. We also determined previously the regional
distribution of [3H] ()-QNB binding sites in
rat (Yamada et al., 1980), rabbit (Fields et al.,
1978) and human (Roeske and Yamamura, 1980) heart. The atrial tissue
generally contains six to nine times more muscarinic receptors (300 fmol/mg protein in rabbit left atrium) than ventricular tissue (53 fmol/mg protein in rabbit right ventricle).
The inhibition of the [3H]()-MQNB binding by
the muscarinic antagonists showed a rank order of potency typical for
the cardiac muscarinic M2 receptors of atropine > himbacine > methoctramine > AF-DX 116 > PZ > carbachol.
Himbacine (Wang et al., 1988), AF-DX 116 (Watson et
al., 1986) and methoctramine (Melchiorre et al., 1987)
have been shown to be selective for the M2 receptor. These ligands had
much higher affinity for the rat and human M2 receptors than PZ, which
has been shown to have low affinity for the M2-type receptor.
Methoctramine showed a high pseudo-Hill coefficient in both cell lines,
as has been found in neuronal and cardiac membranes (Giraldo at al.,
1988i; Melchiorre et al., 1987). This effect is probably due
to an allosteric interaction of methoctramine with the receptors.
Carbachol inhibits [3H]()-MQNB binding in the
human and rat M2 cells with similar Ki values (1.8 and 2 µM,
respectively). The pseudo-Hill coefficient indicates a single-affinity
state for this agonist in both cell lines. In rat cardiac tissue, there
are two agonist affinity states of the M2 receptors resulting from
interaction with G proteins (Watson et al., 1986). In CHO
cells transfected with the porcine m2 receptor gene (Ashkenazi et
al., 1987) and in the human kidney cells transfected with the
human m2 receptor gene (Peralta et al., 1987a),
multiple-affinity states were also observed for carbachol. This
difference may be due to the different assay conditions. The
pKi values for 10 muscarinic
antagonist and 3 agonist drugs were highly similar between the human
and rat clones with similar pseudo-Hill coefficient values.
In testing the human cell line with nonmuscarinic compounds, we found
that the classic nicotinic cholinergic drugs d-tubocurarine and decamethonium showed potency in inhibiting
[3H]()-MQNB binding. These compounds at high
concentrations appear to interact with both muscarinic and nicotinic
receptors, as was demonstrated in rabbit heart tissue (Fields et
al., 1978). Hemicholinium-3, a choline uptake inhibitor, has been
shown to effect the muscarinic receptors in rabbit heart (Fields
et al., 1978), and we could also see an effect in the
HM2-B10 cells. Imipramine, a tricyclic antidepressant with severe
cardiotoxicity (Spiker et al., 1976), had affinity for the
human M2 receptors at concentrations below the clinically used level.
The action on the muscarinic receptors may play a role in this serious
side effect. The antiarrhythmic, cardioactive drugs quinidine and
procainamide were also tested on the HM2-B10 cells. Quinidine had
higher potency in inhibiting the [3H]()-MQNB
binding than procainamide, but both exhibited interactions with the
muscarinic receptors. Among the neuroleptic drugs, the very potent and
widely used chlorpromazine showed high affinity (215 nM) to the HM2-B10
cells, similar to the hm2-transfected CHO cells (Bolden et
al., 1992). The marked anticholinergic side effects of this drug
can be explained with its interactions with M2 muscarinic receptors.
To determine the interaction of the expressed M2 receptors with G
proteins, we measured the effects of carbachol on two second-messenger systems: adenylyl cyclase and phospholipase C. In the human M2 cell
line, 100 µM forskolin stimulated the cAMP formation 10 times over
the basal level. We could see the same effect on the rat M2 clone, but
interestingly there was a difference in both the basal and
forskolin-stimulated cAMP levels between the two cell lines. The human
clone showed significantly higher basal and stimulated cAMP levels.
Carbachol inhibited the cAMP formation in both cell lines, but there
was a greater level of inhibition in the cells expressing the rat m2
cDNA. Carbachol (10 µM) inhibited forskolin-stimulated cAMP formation
by 54% in the HM2-B10 (human M2) and 70% in the M2LKB2-2 (rat M2)
cells. It was shown with other m2-transfected cells (Peralta et
al., 1987a) that the increase in the
Bmax has only a weak effect on the
inhibition of cAMP formation. One possibility in our case is that in
the transfected cells, the cAMP homeostasis was slightly altered
because we saw differences in both the basal and maximal
forskolin-stimulated cAMP level before carbachol application. It was
shown (Jakubik et al., 1995) that the mAChRs exhibit
constitutive activity at high expression levels. This
agonist-independent constitutive inhibition of adenylyl cyclase at high
receptor densities may explain the lower basal and forskolin-stimulated
cAMP formation in the M2LKB2-2 (rat M2) cells.
The effect on the [3H]IP1
accumulation in the two cell lines also was different. In the human M2
cell line, carbachol had no significant effect on the
[3H]IP1 accumulation,
whereas in the cells expressing the rat M2 receptor, we could see a
mild but significant stimulation of the inositol lipid level. This
difference can be explained by the different
Bmax value because it was shown with
porcine M2 receptor (Ashkenazi et al., 1987) that the PI
response is dependent on a higher level of receptor expression than the
cAMP response. The physiological significance of this coupling is not
clear. It is interesting to note that in the B82 cell system, the
EC50 values of carbachol in inhibiting the
forskolin-stimulated cAMP formation and in stimulation of PI hydrolysis
are approximately the same. Evidence now shows (Camps et
al., 1992) that the pertussis toxin-sensitive stimulation of PI
hydrolysis found for many Gi-coupled receptors is
mediated by G protein beta gamma subunits through direct
interaction with phospholipase C2 or C3. This response requires
both high receptor expression level and high agonist concentrations.
However, there also is evidence for a pertussis toxin-insensitive
mechanism, which can act synergistically with the beta gamma
stimulation (Zhu and Birnbaumer, 1996). On the other hand, the maximal
stimulation of the PI hydrolysis was only 1.8- fold. This is much lower
than was seen in the CHO cells expressing the porcine M2 receptors
(Ashkenazi et al., 1987) and with human kidney cells
expressing the human M2 receptor (Peralta et al., 1988) at
similar receptor densities. It is possible that in B82 cells, one or
more components of the above signaling mechanisms are not present.
Recombinant cell lines are very useful in the primary screening of candidate drugs and in the study of the signal transduction mechanisms initiated by a single receptor subtype without the interference of other subtypes. These systems generally have higher expression levels of the transfected receptor population and can amplify some weak responses. These responses may not be noticed in tissue preparations in which an average response is measured but may be physiologically important for small subpopulations of cells with high receptor expression levels. The choice of the host cell line is very important because the second-messenger interaction with the expressed receptors depends on the coupling system of the host cells. To obtain reliable comparisons between subtypes or species, the same host cell lines with similar receptor densities should be used. To select an adequate model system, further work is needed to characterize the signal transduction machinery (G protein subunits, adenylyl cyclase types, and so on) present in the host cells.
In conclusion, our results demonstrate that the human and rat M2 receptors are very similar to each other in binding characteristics and that the binding results correlate with the functional physiological data from heart tissue. However, there is a slight difference in the coupling characteristics of the two clones. Further experiments are necessary to determine whether the stimulation of PI hydrolysis found in the cells expressing the rat M2 receptors have physiological consequences in heart areas (e.g., left atria) with high M2 receptor densities.
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Acknowledgments |
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The authors would like to thank Dr. Robert Horvath for the data analysis, Ms. Carol A. Haussler for tissue culture and Ms. Pam Abrams for preparation of the manuscript.
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Footnotes |
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Accepted for publication October 22, 1997.
Received for publication July 7, 1997.
1 This work was supported by Grant HL20984 from the National Institutes of Health.
Send reprint requests to: William R. Roeske, M.D., Department of Medicine, The University of Arizona, Health Sciences Center, Tucson, AZ 85724.
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Abbreviations |
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MQNB, N-methyl-3-quinuclidinyl benzilate; EC50, half-effective concentration; Emax, maximal effective concentration; IC50, half-inhibitory concentration; Kd, dissociation constant; Bmax, maximal binding; Ki, inhibition constant; pKi, negative logarithm of Ki; nH, Hill coefficient; IBMX, 3-isobutyl-methylxanthine; PI, phosphoinositide; IP1, inositol monophosphate; CHO, Chinese hamster ovary; IMDM, Iscove's modified Dulbecco's medium; PZ, pirenzepine; 4-DAMP, 4-diphenylacetoxy-N-methylpiperidine methiodide; mAChR, muscarinic acetylcholine receptor; HHSiD, hexahydro-sila-difenidol hydrochloride; PCR, polymerase chain reaction; dNTP, deoxynucleotidetriphosphate; ANOVA, analysis of variance.
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References |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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,5-cyclic monophosphate.
Proc Natl Acad Sci USA
67:
305-312-adrenergic and muscarinic cholinergic receptors obtained by automated DNA sequence analysis: Further evidence for a multigene family.
Proc Natl Acad Sci USA
84:
8296-8300-actin expression vector system directs high-level accumulation of antisense transcripts.
Proc Natl Acad Sci USA
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4831-4835)-[3H]quinuclidinyl benzilate binding to rat cerebral cortical and cardiac muscarinic cholinergic sites. I: Characterization and regulation of agonist binding to putative muscarinic subtypes.
J Pharmacol Exp Ther
237:
411-418
16 and evidence for synergic interaction between G
and subunit of a receptor-activated G-protein.
Proc Natl Acad Sci USA
93:
2827-2831
0022-3565/98/2842-0500$03.00/0
THE JOURNAL OF PHARMACOLOGY AND EXPERIMENTAL THERAPEUTICS
Copyright © 1998 by The American Society for Pharmacology and Experimental Therapeutics
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