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Vol. 283, Issue 2, 735-741, 1997
Torrey Pines Institute for Molecular Studies, San Diego, California (C.T.D., C.G.S., R.A.H) and SRI International, Menlo Park, California (I.P.B-G., K.C., I.D.A., S.R.B., L.T.).
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Abstract |
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 Top
Abstract
Introduction
Methods
Results
Discussion
References
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Fifteen hexapeptides having high affinity for the opioid-like receptor
ORL1 were identified from a combinatorial library containing more than
52 million different hexapeptides. The five compounds with the highest
affinity were characterized further by use of a variety of in
vitro models. Binding studies indicated that these five
peptides have affinity for ORL1 in the nanomolar range, similar to the
recently discovered endogenous ligand called nociceptin and orphanin FQ
(N/OFQ). The activity of these compounds was investigated in three
different assays: stimulation of [35S]GTP
S binding and
inhibition of forskolin-stimulated cAMP accumulation in Chinese hamster
ovary cells transfected with ORL1, and inhibition of electrically
induced contractions in the mouse vas deferens. In each assay, the five
hexapeptides acted as partial agonists. The EC50 values for
stimulation of [35S]GTPS binding and inhibition of
cAMP accumulation were in the range of that for N/OFQ, but maximal
effects ranged from 70 to 90% of N/OFQ in the cAMP assay, and 30 to
60% of N/OFQ in the GTPS assay. The positive hexapeptides
identified were found to have minimal structural similarity to N/OFQ.
The peptides are positively charged, which could enable them to bind to
the negatively charged second extracellular loop thought to be a likely
binding site for N/OFQ.
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Introduction |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The
cloning of the opioid receptors led to the discovery by several groups
of an additional receptor from this family (Bunzow et al.,
1994
; Lachowicz et al., 1995; Mollereau et al.,
1994; Wang et al., 1994). Although this receptor, referred
to here as ORL1 after Mollereau et al. (1994), has very high
homology with the opioid receptors, the receptor transfected into
mammalian cells did not bind opiates with the expected high affinity.
This suggested the presence of an unknown endogenous neurotransmitter as its natural ligand. This endogenous ligand was subsequently identified by two groups independently (Meunier et al.,
1995; Reinscheid et al., 1995) and was found to be a
heptadecapeptide, with a sequence most closely resembling the opioid
peptide dynorphin. The peptide was named orphanin FQ by Reinscheid
et al. to designate the fact that it was an endogenous
ligand for an orphan receptor and that its first and last amino acids
were phenylalanine and glutamine. Meunier and colleagues named it
nociceptin as an indication of its in vivo activity, because
it was discovered that intracerebroventricular injection into mice led
to a decrease in the hot-plate escape jumping latency (Meunier et
al., 1995) and tail-flick latency (Reinscheid et
al., 1995).
The in vitro activity of N/OFQ, as determined in cells
transfected with ORL1, was as expected for an opioid-like receptor. N/OFQ, at low concentrations, inhibits forskolin-stimulated cAMP accumulation and stimulates [35S]GTPS
binding in brain membranes and transfected cells (Sim et
al., 1996; Adapa and Toll, in press). Radioreceptor assays have
been developed by use of both iodinated
Tyr14-N/OFQ (Reinscheid et al., 1995)
and the tritiated version of the Tyr14 analog
(Adapa and Toll, in press), and the native peptide (Dooley and
Houghten, 1996). Both peptides have been shown to bind with high
affinity to transfected cells and brain membranes, and the binding
properties seem to be very similar.
Unlike its close relatives the opioid receptors, very little is known
of the pharmacology of ORL1. Meunier et al. (1995)
demonstrated that the Tyr1 analog behaves very
much like the native peptide, as does the Tyr14
analog (Reinscheid et al., 1995). The first
structure-activity studies with truncated versions of N/OFQ have
demonstrated that the amino-terminal portion of the peptide is
essential for high binding affinity and that the four C-terminal amino
acids are not necessary for binding (Dooley and Houghten, 1996;
Reinscheid et al., 1996). Although the sequence of N/OFQ has
striking similarity to opioid peptides, and in particular dynorphin,
the dynorphin gene products have only moderate affinity for ORL1,
ranging from 100- to 1000-fold lower affinities than for the
kappa opioid receptor (Adapa and Toll, in press). The
development of new agonists and antagonists is of high priority if the
in vivo functions of ORL1 and N/OFQ are to be better
understood.
One method that has been very successful in the identification of novel
peptidic and nonpeptidic structures that bind to opioid and other
receptors has been the use of SCL (Houghten et al., 1991).
SCLs are composed of mixtures of large numbers of compounds (e.g., 50 million, representing all possible combinations of
the building blocks used) which are tested as mixtures. One of the major advantages of the SCLs is that the compounds are not
support-bound and thus can be used directly in solution for binding or
functional assays (Houghten et al., 1992). Houghten and
colleagues (1991) originally demonstrated the use of an SCL to identify
peptides which corresponded to the antigenic determinant of an
antibody. The use of an SCL to identify peptides closely related to the natural enkephalins was demonstrated in an opioid receptor assay (Houghten et al., 1992; Houghten and Dooley, 1993). Novel
peptide antagonists to the mu receptor, the Acetalins
(Dooley et al., 1993) and an all D-amino acid
agonist (Dooley et al., 1994) were also identified through
the use of combinatorial libraries. Deconvolution, or identification of
individual compounds from the complex mixtures in the libraries, can be
achieved through an iterative process (described in the papers
mentioned above) or by using a positional scanning library (Pinilla
et al., 1992; Dooley and Houghten 1993). A PS-SCL enables
the determination of the most active amino acids or building block at
each position of a peptide or nonpeptide directly from the initial
screening data. With the use of peptides as an example, PS-SCLs are
composed of individual positional SCLs in which one or two positions
are defined with a single amino acid, whereas the remaining positions
are composed of mixtures of amino acids. The defined position(s) is
"walked" through the entire sequence of the PS-SCL. It should be
noted that each positional SCL, although addressing a single position
of the sequence, represents the same collection of individual peptides.
When used in concert, the data derived from each positional SCL yield
information about the most important amino acids for every position.
This library can be screened, and data obtained, in as little as a
single assay. This information can then be used to synthesize highly
active individual compounds. The work presented here describes the
identification and properties of five hexapeptides having high affinity
for ORL1, identified from a PS-SCL composed of more than 52 million
hexapeptides.
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Methods |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Cell Culture
ORL1-containing CHO cells came from two sources. The rat receptor in CHO cells were obtained from Dr. Ping Law (University of Minnesota). The cDNA for the mouse receptor was obtained from Dr. Brigitte Kieffer (University of Strasbourg). The mouse ORL1 was subcloned into pcDNA3.1/His (Invitrogen, San Diego, CA) and this vector was transfected into CHO cells. pcDNA3.1/His produces a fusion protein containing a poly-His region and an antigenic epitope for commercial antibodies on the amino terminus of the protein. We have discovered no apparent effect of the amino-terminal tag on receptor binding or function, and the entire fusion protein has been used for the experiments described herein.
The cells were grown in Dulbecco's modified Eagle's medium with 10% fetal bovine serum, in the presence of 0.4 mg/ml G418 and 0.1% penicillin/streptomycin, in 100-mm plastic culture dishes. For binding assays, the cells are scraped off the plate at confluence. For determination of inhibition of cAMP accumulation, cells were subcultured onto 24-well plates and used at confluence.
Receptor Binding
Binding to brain membranes.
Binding to brain membranes was
conducted as described previously (Dooley and Houghten, 1996). Rat
brains, (Harlan, Indianapolis, IN) minus cerebella, were homogenized in
40 ml of Tris buffer (50 mM Tris, 2 mM ethylenediaminetetraacetic acid,
100 µM phenylmethylsulfonyl fluoride, pH 7.4). Homogenates were spun
for 10 min at 38,000 × g (Beckmann H2-JC, Fullerton,
CA). Pellets were resuspended and incubated at 37°C for 30 min, and
centrifuged for 10 min. Pellets were resuspended in 100 volumes of
buffer, and bovine serum albumin (2 mg/ml) was added. Competition
experiments were carried out in the presence of 3 nM
[3H]N/OFQ (33 Ci/mmol) in a final volume of
0.65 ml. The reaction was terminated by filtration by a Tomtec 96 harvester (Orange, CT) through GF-B filters, previously soaked in 0.1%
polyethyleneimine. Bound radioactivity was counted on a Pharmacia
Biotech beta-plate liquid scintillation counter (Piscataway, NJ) and
expressed in counts per minute. IC50 values were
determined with six concentrations of each peptide analog, and
calculated by use of Graphpad/Prism (ISI, San Diego, CA).
Binding to cell membranes. Binding to cell membranes was conducted in a 96-well format. Cells were removed from the plates by scraping with a rubber policeman, homogenized in Tris buffer with a Polytron homogenizer, then centrifuged once and washed by an additional centrifugation at 27,000 × g for 15 min. The pellet was resuspended in 50 mM Tris, pH 7.5, and the suspension incubated with [3H]N/OFQ (120 Ci/mmol) in a total volume of 0.2 ml for 120 min at 25°C. Samples were filtered and counted as described above.
Inhibition of forskolin-stimulated cAMP accumulation.
The
potency for the inhibition of forskolin-stimulated cAMP accumulation
was conducted basically as described previously by Meunier et
al. (1995) in intact CHO cells plated on 24-well plastic plates.
To the cells was added [3H]adenine (1.0 µCi)
in 0.4 ml of culture medium. The cells remained at 37°C for 2 h
to allow the adenine to incorporate into the intracellular ATP pool.
After 2 h, the cells were washed once with incubation buffer
containing: 130 mM NaCl, 4.8 mM KCl, 1.2 mM
KH2PO4, 1.3 mM
CaCl2, 1.2 mM MgSO4, 10 mM
glucose, 1 mg/ml bovine serum albumin and 25 mM HEPES, pH 7.4, and
replaced with buffer containing forskolin (10 µM) and
isobutylmethylxanthine (50 µM). After 10 min, the medium was
aspirated and replaced with 0.5 ml, 0.2 M HCl. Approximately 1000 cpm
of [14C]cAMP was added to each well and used as
an internal standard. The contents of the wells were then transferred
to columns of 0.65 g dry alumina powder. The columns were eluted
with 4 ml of 5 mM HCl, 0.5 ml of 0.1 M ammonium acetate, then two
additional milliliters of ammonium acetate. The final eluate was
collected into scintillation vials and counted for
14C and tritium. Amounts collected were corrected
for recovery of [14C]cAMP.
[35S]GTPS binding.
[35S]GTPS binding was conducted basically as
described by Traynor and Nahorski (1995). Cells were scraped from
tissue culture dishes into 20 mM HEPES, 1 mM ethylenediaminetetraacetic
acid, then centrifuged at 500 × g for 10 min. Cells
were resuspended in this buffer and homogenized with a
Polytron Homogenizer. The homogenate was centrifuged at
27,000 × g for 15 min, and the pellet resuspended in
buffer A, containing: 20 mM HEPES, 10 mM MgCl2, 100 mM NaCl, pH 7.4. The suspension was recentrifuged at 20,000 × g and suspended once more in buffer A. The pellet was
sometimes frozen at 
70°C before use. For the binding assay,
membranes (8-15 µg protein) were incubated with
[35S]GTPS (50 pM), GDP (10 µM) and N/OFQ,
in a total volume of 1.0 ml, for 60 min at 25°C. Samples were
filtered over glass fiber filters and counted as described for the
binding assays. Statistical analysis was conducted with the program
Prism.
).
[3H]N/OFQ (120 and 33 Ci/mmol respectively)
were synthesized and generously donated by New England Nuclear/Dupont
(Boston, MA), or synthesized as described previously (Dooley and
Houghten, 1996). N/OFQ was from Phoenix Pharmaceuticals (Belmont, CA);
Tyr14-N/OFQ was synthesized by Research Genetics
(Huntsville, AL); and other reagents were obtained from Sigma Chemical
Co. (St. Louis, MO).
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Results |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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A hexapeptide PS-SCL containing two defined positions was screened
in the assay for N/OFQ. This PS-SCL can be represented by the formula
(Ac-O1O2X3X4X5X6-NH2,
Ac-X1X2O3O4X5X6-NH2,
Ac-X1X2X3X4O5O6-NH2), in which the positions labeled (O) are individually defined by the 20 natural L-amino acids (i.e., AA, AC, AD, ... , YV, YW, YY). The positions labeled (X) consist of equimolar mixtures
of 19 of the natural L-amino acids (omitting cysteine).
This library contains 1200 mixtures (three sets of 400 mixtures each);
each mixture contains 130,321 peptides (52,128,400 hexapeptides in total). Each set of 400 contains the same peptides, the difference being which positions are specifically defined. Upon screening the
first sublibrary at 0.4 mg/ml (fig. 1A),
which defined the first and second
positions, only three mixtures inhibited 100% of
[3H]N/OFQ binding,
Ac-RFXXXX-NH2,
Ac-RWXXXX-NH2 and
Ac-RYXXXX-NH2. IC50 values
calculated for Ac-RFXXXX-NH2
(IC50 = 21 µM),
Ac-RWXXXX-NH2 (IC50 = 21 µM) and Ac-RYXXXX-NH2
(IC50 = 8.5 µM) indicated that the third
mixture was more active than the first two. All other mixtures had
IC50 values greater than 40 µM.
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In the second sublibrary (fig. 1B), which defined the third and fourth
positions, four mixtures inhibited more than 90% of [3H]N/OFQ binding (1/% Bound > 0.1):
Ac-XXFRXX-NH2,
Ac-XXWRXX-NH2, Ac-XXYKXX-NH2 and
Ac-XXYRXX-NH2. The most active mixture was
Ac-XXYRXX-NH2, with an IC50
of 24 µM. In the third sublibrary (fig. 1C), which defined the fifth
and sixth positions, two mixtures inhibited more than 90% of
[3H]N/OFQ binding:
Ac-XXXXWK-NH2 (92%) and
Ac-XXXXWR-NH2 (93%), with a third mixture
Ac-XXXXIK-NH2 inhibiting 75% of
[3H]N/OFQ binding. Mixtures from the third
sublibrary were less active; the most active mixture was
Ac-XXXXWR-NH2, which had an IC50 of 91 µM, indicating that appropriate
amino acids around the amino terminus are important for receptor
binding. This is consistent with our previous findings with truncated
N/OFQ peptides (Dooley and Houghten, 1996). Because the iterative
mixture set Ac-RYOXXX-NH2 had been synthesized
earlier for an unrelated study, the IC50 values
for each of the 20 mixtures were calculated. Three mixtures were found
to be more active than Ac-RYXXXX-NH2. The most
active iterative mixture found was Ac-RYYXXX-NH2
with an IC50 of 0.7 µM, which indicates that
tyrosine is the preferred amino acid in the third position. With the
knowledge that the most effective amino acids in the first three
positions were arginine, tyrosine and tyrosine, a series of 20 individual compounds were synthesized. These peptides contained
arginine in the first position and tyrosine in the second and third
positions, and combinations of the amino acids found in active mixtures
for positions 4 to 6 (i.e., R, K,F, L in the fourth
position, W and I in the fifth position and K, R, W in the sixth
position). Preliminary binding experiments indicated that
IC50 values of these compounds ranged from
approximately the affinity of N/OFQ to more than 2000 nM. Of these 20 compounds, five with high binding affinity were further characterized.
The five peptides were tested in three functional assays; inhibition of
cAMP accumulation and stimulation of GTPS binding in CHO cells
transfected ORL1, and in the mouse vas deferens assay, and for binding
affinity in transfected cells.
Table 1 shows
Ki values for each compound plus N/OFQ
determined at the mouse ORL1 in CHO cells. In addition, table 1 lists the EC50 value for stimulation of
[35S]GTPS binding plus the percent maximal
stimulation, as compared with N/OFQ, in these cells. Each novel peptide
stimulated [35S]GTPS binding at low
concentrations, but none of the compounds stimulated to the extent of
N/OFQ. Figure 2 shows this graphically and indicates the absolute amount of stimulated
[35S]GTPS binding. No binding of
[3H]N/OFQ, nor stimulation of
[35S]GTPS binding was found in
nontransfected CHO cells.
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This partial agonist activity was also demonstrated in the other assays used. N/OFQ inhibited cAMP accumulation by an average of 84% in five experiments, with an IC50 of approximately 1.5 nM (table 2). Each of the peptides also inhibited cAMP accumulation, with approximately the same potency as N/OFQ. Once again none inhibited to the same maximal extent as N/OFQ, four of the peptides being significantly different in percent maximal inhibition.
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The compounds were also tested in the MVD assay. We have previously
shown that N/OFQ is able to block the electrically induced contractions
of the MVD (Berzetei-Gurske et al., 1996). In the MVD assay,
the compounds showed reasonably potent partial agonist activity.
However, in this assay, the activity was difficult to determine because
each of the peptides produced very strong tachyphylaxis. In other
words, after each addition of the peptide, the vas deferens was
unresponsive to an additional administration of the compound, or to the
administration of N/OFQ (see fig. 3). We
attempted to obtain IC50 values by extensive
washing after each addition, but consistent data could not be
generated. It was clear, however, that significant inhibition of the
twitch response could be achieved at low concentrations, but high
concentrations never produced the maximal inhibition level achieved by
N/OFQ. One could tell that these actions were not through the opioid
receptors because the agonist activity was not blocked by naloxone, and
the tachyphylaxis induced by the peptides was selective for ORL1. After
treatment with one of the ORL1 peptides, N/OFQ was no longer functional as an agonist, but the ability of the delta opioid agonist
DPDPE to inhibit twitch was undiminished.
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Discussion |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The identification of novel ligands for receptors has
traditionally been by standard medicinal or peptide chemistry, with new
compounds based on the structure of known compounds. Particularly important for physiological studies would be the identification of
high-affinity and stable analogs that could be used in vivo. This process may be difficult for larger peptides such as N/OFQ (FGGFTGARKSARKLANQ), because there are numerous potential sites not
only for modification, but more importantly for degradation. N/OFQ also
poses a particular problem because the truncation on the
carboxy-terminal side produces inactive peptides when shorter than
N/OFQ 1-14 (Dooley and Houghten, 1996). Furthermore, removal of the
amino-terminal Phe (N/OFQ 2-17) produces an inactive compound (Matthes
et al., 1996). It is the removal of
Phe1 that is the initial and primary degradative
step in processing N/OFQ (Yu et al., 1996).
Another, more novel method for the identification of new ORL1 ligands is the use of combinatorial libraries. In the present study, a peptide PS-SCL containing more than 150 million individual hexapeptides was used to identify compounds with affinities for ORL1 similar to that of N/OFQ. Because of the positional scanning nature of the libraries, this identification required the individual synthesis of only 20 peptides. Of these 20 peptides, five compounds with high affinity were studied further in three functional assays.
Each of the five peptides tested had high affinity for ORL1, and was a
potent agonist in the inhibition of forskolin-stimulated cAMP
accumulation and the stimulation of GTPS binding in CHO cells
transfected with ORL1. Although the concentrations in which the
peptides produced their agonist activities in each of the systems were
similar to that of N/OFQ, the maximal activity of each peptide was less
than that of N/OFQ in each assay. For the rat receptor transfected into
CHO cells, N/OFQ could induce a maximal 84% inhibition of
forskolin-induced cAMP accumulation. The maximal inhibition of cAMP
accumulation induced by the five peptides ranged from approximately 60 to 75%. This makes the peptides approximately 70 to 90% as
efficacious as N/OFQ in this system. The reason for the partial agonist
activity of these peptides is unknown. Although the activity of many
peptide hormones can be mimicked by shorter peptides, or even
nonpeptides, it is possible that in this case, a peptide of greater
than six amino acids would be required for full agonist activity.
Although initial experiments were carried out on cells transfected with
the rat receptor, receptor binding was difficult with these cells, as
were the GTPS binding studies (unpublished observation), probably
because of a low receptor number. For this reason, we transfected CHO
cells with the mouse receptor and obtained a clone for which the
receptor number was quite high (1.2 pmol/mg) (Adapa and Toll, in
press). Stimulation of GTPS binding was conducted on these cells. In
this system, each of the peptides also stimulated GTPS binding at
low concentrations, but once again, maximal activity was found to be
significantly less than that found for N/OFQ. In this case the peptides
ranged from 30% (peptide 3) to 60% (peptide 4) of the maximal
[35S]GTPS binding induced by N/OFQ.
The increased facility in demonstrating partial agonist activity in the
GTPS binding assay as opposed to the inhibition of cAMP accumulation
is probably a function of the assay rather than the difference in
species or potential differences in receptor number. First of all, the
rat and mouse receptors are very similar, differing by one amino acid
in the amino terminus and one in the carboxy terminus (Wick et
al., 1994; Matthes et al., 1996), so it is unlikely
that the primary sequence would affect the relative agonist activities.
Second, the receptor number is higher in the CHO cells transfected with
the mouse receptor. Finally, in the opioid system, the GTPS assay is
particularly adept at identifying partial agonist activity, which
demonstrates partial agonist activity for morphine at the mu
receptor (Traynor and Nahorski, 1995), although morphine is a
prototypical full agonist in most in vivo and in
vitro paradigms.
Each high-affinity peptide is very highly charged, containing three
basic residues (Arg or Lys). In fact, in each sublibrary tested
(Ac-OOXXXX-NH2,
Ac-XXOOXX-NH2, and
Ac-XXXXOO-NH2), Arg was found to be a preferred
amino acid in one of the defined positions. In this respect they are
similar to N/OFQ, which has 4 positively charged amino acids among its
17 amino acids. These highly charged peptides would be expected to bind
tightly to a potential N/OFQ binding site on the acidic amino acid-rich
second extracellular loop of ORL1 (Meunier et al., 1995). It
is also noteworthy that these sequences bear modest resemblance to the
Acetalins, Ac-RFMWMK-NH2, however the Acetalins
were found to bind poorly (>15,000 nM) to ORL1 and the five peptides
described here bound poorly (>4000 nM) in mu,
delta and kappa opioid receptor assays.
In conclusion, these studies demonstrate the utility of combinatorial chemistry for the identification of novel ligands for a G protein-coupled receptor. The five high-affinity hexapeptides represent the first small peptides with high affinity for ORL1 and identify not only potentially useful ligands for the investigation into the function of ORL1, but also an improved starting place for the discovery of new ligands. The investigation of the in vivo activity of these hexapeptides is currently underway.
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Acknowledgments |
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The authors would like to thank Dr. Y.-P. Wan of Dupont/New England Nuclear for the synthesis and gift of the [3H]N/OFQ, and Eileen Weiler for editorial assistance.
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Footnotes |
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Accepted for publication July 14, 1997.
Received for publication March 20, 1997.
1 This work was supported by National Institute on Drug Abuse grants DA06682 (LT) and DA09410 (RAH), and Houghten Pharmaceuticals Inc., San Diego, CA.
2 To whom correspondence concerning the combinatorial chemistry should be addressed: Torrey Pines Institute for Molecular Studies, 3550 General Atomics Court, San Diego, CA 92121.
3 To whom correspondence concerning the pharmacological evaluation should be addressed: SRI International, 333 Ravenswood Avenue, Menlo Park, CA 94025.
Send reprint requests to: Dr. Lawrence Toll, SRI International, 333 Ravenswood Avenue, Menlo Park, CA 94025.
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Abbreviations |
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N/OFQ, Nociceptin, Orphanin FQ;
SCL, synthetic
combinatorial libraries;
PS-SCL, Positional Scanning SCL;
CHO, Chinese
hamster ovary;
MVD, mouse vas deferens;
DPDPE, [D-Pen2-D-Pen5]enkephalin;
HEPES, N-2-hydroxyethylpiperazine-N
-ethanesulfonic acid.
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References |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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, or 
opioid receptor type.
FEBS Lett.
347: 284-288, 1994.S binding in rat brain.
NeuroReport
7: 729-733, 1996.-O-(3-[35S]thio)triphosphate binding to membranes from human neuroblastoma SH-SY5Y cells.
Mol. Pharmacol.
47: 848-854, 1995., and opioid receptors.
Mol. Brain Res.
27: 37-44, 1994.This article has been cited by other articles:
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  N. Akuzawa, S. Takeda, and M. Ishiguro Structural Modelling and Mutation Analysis of a Nociceptin Receptor and its Ligand Complexes J. Biochem., June 1, 2007; 141(6): 907 - 916. [Abstract] [Full Text] [PDF]
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 T. V. Khroyan, N. T. Zaveri, W. E. Polgar, J. Orduna, C. Olsen, F. Jiang, and L. Toll SR 16435 [1-(1-(Bicyclo[3.3.1]nonan-9-yl)piperidin-4-yl)indolin-2-one], a Novel Mixed Nociceptin/Orphanin FQ/{micro}-Opioid Receptor Partial Agonist: Analgesic and Rewarding Properties in Mice J. Pharmacol. Exp. Ther., February 1, 2007; 320(2): 934 - 943. [Abstract] [Full Text] [PDF]
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D. R. Kapusta, C. Thorkildsen, V. A. Kenigs, E. Meier, M. M. Vinge, C. Quist, and J. S. Petersen Pharmacodynamic Characterization of ZP120 (Ac-RYYRWKKKKKKK-NH2), a Novel, Functionally Selective Nociceptin/Orphanin FQ Peptide Receptor Partial Agonist with Sodium-Potassium-Sparing Aquaretic Activity J. Pharmacol. Exp. Ther., August 1, 2005; 314(2): 652 - 660. [Abstract] [Full Text] [PDF]
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D. R. Kapusta, M. A. Burmeister, G. Calo', R. Guerrini, H. B. Gottlieb, and V. A. Kenigs Functional Selectivity of Nociceptin/Orphanin FQ Peptide Receptor Partial Agonists on Cardiovascular and Renal Function J. Pharmacol. Exp. Ther., August 1, 2005; 314(2): 643 - 651. [Abstract] [Full Text] [PDF]
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G. Carra, A. Rizzi, R. Guerrini, T. A. Barnes, J. McDonald, C. P. Hebbes, F. Mela, V. A. Kenigs, G. Marzola, D. Rizzi, et al. [(pF)Phe4,Arg14,Lys15]N/OFQ-NH2 (UFP-102), a Highly Potent and Selective Agonist of the Nociceptin/Orphanin FQ Receptor J. Pharmacol. Exp. Ther., March 1, 2005; 312(3): 1114 - 1123. [Abstract] [Full Text] [PDF]
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 M. Corbani, C. Gonindard, and J.-C. Meunier Ligand-Regulated Internalization of the Opioid Receptor-Like 1: A Confocal Study Endocrinology, June 1, 2004; 145(6): 2876 - 2885. [Abstract] [Full Text] [PDF]
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P. F. Zaratin, G. Petrone, M. Sbacchi, M. Garnier, C. Fossati, P. Petrillo, S. Ronzoni, G. A. M. Giardina, and M. A. Scheideler J. Pharmacol. Exp. Ther., February 1, 2004; 308(2): 454 - 461. [Abstract] [Full Text] [PDF]
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D. Rizzi, A. Rizzi, R. Bigoni, V. Camarda, G. Marzola, R. Guerrini, C. De Risi, D. Regoli, and G. Calo' [Arg14,Lys15]Nociceptin, a Highly Potent Agonist of the Nociceptin/Orphanin FQ Receptor: in Vitro and in Vivo Studies J. Pharmacol. Exp. Ther., January 1, 2002; 300(1): 57 - 63. [Abstract] [Full Text] [PDF]
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 J. S. Mogil and G. W. Pasternak The Molecular and Behavioral Pharmacology of the Orphanin FQ/Nociceptin Peptide and Receptor Family Pharmacol. Rev., September 1, 2001; 53(3): 381 - 415. [Abstract] [Full Text] [PDF]
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H. Berger, G. Calo', E. Albrecht, R. Guerrini, and M. Bienert [Nphe1]NC(1-13)NH2 Selectively Antagonizes Nociceptin/Orphanin FQ-Stimulated G-Protein Activation in Rat Brain J. Pharmacol. Exp. Ther., August 1, 2000; 294(2): 428 - 433. [Abstract] [Full Text]
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 L. Mouledous, C. M. Topham, C. Moisand, C. Mollereau, and J.-C. Meunier Functional Inactivation of the Nociceptin Receptor by Alanine Substitution of Glutamine 286 at the C Terminus of Transmembrane Segment VI: Evidence from a Site-Directed Mutagenesis Study of the ORL1 Receptor Transmembrane-Binding Domain Mol. Pharmacol., March 1, 2000; 57(3): 495 - 502. [Abstract] [Full Text]
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 J. A. J. Becker, A. Wallace, A. Garzon, P. Ingallinella, E. Bianchi, R. Cortese, F. Simonin, B. L. Kieffer, and A. Pessi Ligands for kappa -Opioid and ORL1 Receptors Identified from a Conformationally Constrained Peptide Combinatorial Library J. Biol. Chem., September 24, 1999; 274(39): 27513 - 27522. [Abstract] [Full Text] [PDF]
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C. Mollereau, L. Mouledous, S. Lapalu, G. Cambois, C. Moisand, J.-L. Butour, and J.-C. Meunier Distinct Mechanisms for Activation of the Opioid Receptor-Like 1 and kappa -Opioid Receptors by Nociceptin and Dynorphin A Mol. Pharmacol., February 1, 1999; 55(2): 324 - 331. [Abstract] [Full Text]
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L. Mouledous, C. M. Topham, H. Mazarguil, and J.-C. Meunier Direct Identification of a Peptide Binding Region in the Opioid Receptor-like 1 Receptor by Photoaffinity Labeling with [Bpa10,Tyr14]Nociceptin J. Biol. Chem., September 15, 2000; 275(38): 29268 - 29274. [Abstract] [Full Text] [PDF]
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