Transmembrane Domains 4 and 7 of the M1Muscarinic Acetylcholine Receptor Are Critical for Ligand Binding and the Receptor Activation Switch

Lu, Zhi-Liang; Saldanha, José W.; Hulme, Edward C.

doi:10.1074/jbc.m104217200

Cited by 87 publications

(128 citation statements)

References 36 publications

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“…Based on a better overall structural preservation of the model and a more reasonable hydrogenbond pattern evolving between residues T3.37, Y4.57 and E5.46, the placement of Y4.57 into the binding site was favoured. Such a placement is also in accordance with the observation that for residue 4.57 an involvement in ligand binding or receptor activation has been reported for other GPCRs [40][41][42]. For the clash involving Y2.61, W3.28, W7.40, and W7.43 too many placements and corresponding start conformations for MD-simulations would have resulted when following this strategy.…”

Section: Resultssupporting

confidence: 88%

“…As can be seen from Fig. 10, the mean docking score for the hH 3 R actives lay in the cluster of [40,50] and was thus significantly shifted by a value of 20 to higher docking scores, when compared to the mean value of the distribution of WDI and MDB compounds ( [20,30]), thereby indicating that by docking into the hH 3 R binding site, significant higher scores were in average obtained for validated hH 3 R ligands. At the arbitrary chosen GoldScore cut-off of 40, at which 66.5% of the validated hH 3 R antagonists would have been retrieved, 87% of the WDI and MDB compounds were filtered out, resulting in 1720 structures, which were further analysed by visual inspection.…”

Section: Resultsmentioning

confidence: 92%

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Generation of a homology model of the human histamine H3 receptor for ligand docking and pharmacophore-based screening

Schlegel

Laggner

Meier

et al. 2007

J Comput Aided Mol Des

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The human histamine H 3 receptor (hH 3 R) is a G-protein coupled receptor (GPCR), which modulates the release of various neurotransmitters in the central and peripheral nervous system and therefore is a potential target in the therapy of numerous diseases. Although ligands addressing this receptor are already known, the discovery of alternative lead structures represents an important goal in drug design. The goal of this work was to study the hH 3 R and its antagonists by means of molecular modelling tools. For this purpose, a strategy was pursued in which a homology model of the hH 3 R based on the crystal structure of bovine rhodopsin was generated and refined by molecular dynamics simulations in a dipalmitoylphosphatidylcholine (DPPC)/water membrane mimic before the resulting binding pocket was used for high-throughput docking using the program GOLD. Alternatively, a pharmacophore-based procedure was carried out where the alleged bioactive conformations of three different potent hH 3 R antagonists were used as templates for the generation of pharmacophore models. A pharmacophore-based screening was then carried out using the program Catalyst. Based upon a database of 418 validated hH 3 R antagonists both strategies could be validated in respect of their performance. Seven hits obtained during this screening procedure were commercially purchased, and experimentally tested in a [ 3 H]N a -methylhistamine binding assay. The compounds tested showed affinities at hH 3 R with K i values ranging from 0.079 to 6.3 lM.

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Section: Resultssupporting

confidence: 88%

Section: Resultsmentioning

confidence: 92%

Generation of a homology model of the human histamine H3 receptor for ligand docking and pharmacophore-based screening

Schlegel

Laggner

Meier

et al. 2007

J Comput Aided Mol Des

View full text Add to dashboard Cite

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“…The mAChR agonists developed to date, such as xanomeline and sabcomeline, improve cognition preclinically, although evidence of clinical efficacy has been confounded by peripheral effects such as sweating, nausea and diarrhoea, which are believed to be attributed to the relatively non-selective mAChR activity profile of these compounds (Wood et al, 1999). This lack of selectivity is believed to be due to binding to the orthosteric ACh binding site that is highly conserved across the mAChR family (Spalding et al, 1994;Baldwin et al, 1997;Gether, 2000;Lu et al, 2001).…”

Section: Discussionmentioning

confidence: 99%

Characterization of a CNS penetrant, selective M₁muscarinic receptor agonist, 77‐LH‐28‐1

Langmead

Austin

Branch

et al. 2008

British J Pharmacology

122

137

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Background and purpose: M 1 muscarinic ACh receptors (mAChRs) represent an attractive drug target for the treatment of cognitive deficits associated with diseases such as Alzheimer's disease and schizophrenia. However, the discovery of subtypeselective mAChR agonists has been hampered by the high degree of conservation of the orthosteric ACh-binding site among mAChR subtypes. The advent of functional screening assays has enabled the identification of agonists such as AC-42 (4-nbutyl-1-[4-(2-methylphenyl)-4-oxo-1-butyl]-piperidine), which bind to an allosteric site and selectively activate the M 1 mAChR subtype. However, studies with this compound have been limited to recombinantly expressed mAChRs. Experimental approach: In this study, we have compared the pharmacological profile of AC-42 and a close structural analogue, 77-LH-28-1 (1-[3-(4-butyl-1-piperidinyl)propyl]-3,4-dihydro-2(1H)-quinolinone) at human recombinant, and rat native, mAChRs by calcium mobilization, inositol phosphate accumulation and both in vitro and in vivo electrophysiology. Key results: Calcium mobilization and inositol phosphate accumulation assays revealed that both AC-42 and 77-LH-28-1 display high selectivity to activate the M 1 mAChR over other mAChR subtypes. Furthermore, 77-LH-28-1, but not AC-42, acted as an agonist at rat hippocampal M 1 receptors, as demonstrated by its ability to increase cell firing and initiate gamma frequency network oscillations. Finally, 77-LH-28-1 stimulated cell firing in the rat hippocampus in vivo following subcutaneous administration. Conclusions and implications: These data suggest that 77-LH-28-1 is a potent, selective, bioavailable and brain-penetrant agonist at the M 1 mAChR and therefore that it represents a better tool than AC-42, with which to study the pharmacology of the M 1 mAChR. (2008) 154, 1104-1115 doi:10.1038/bjp.2008 published online 5 May 2008 Keywords: muscarinic receptors; selective agonist; allosteric; AC-42; 77-LH-28-1; calcium mobilization; inositol phosphate; cell firing; network oscillations There is a wide array of pharmacological tools with which to study mAChRs. For example, N-methyl scopolamine, quinuclidinylbenzilate, pirenzepine and darifenacin are among numerous mAChR antagonists, and ACh and oxotremorine-M among mAChR agonists, which have been used in unlabelled and radiolabelled forms to characterize the localization, pharmacology and function of mAChRs. Unfortunately, most of these pharmacological tools exhibit poor selectivity between mAChR subtypes (Caulfield and Birdsall, 1998;Ellis, 2002). Those agents that do display high degrees of mAChR subtype selectivity are few in number and when discovered are often shown to interact with an allosteric, rather than the orthosteric, site as exemplified by the highly selective M 1 receptor peptide antagonist MT-7 (muscarinic toxin 7; Olianas et al., 2000). British Journal of PharmacologyTherefore, the identification of selective M 1 mAChR agonists would represent a significant advance in mAChR pharmacology and could offer t...

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“…This deletion did not modify ligand binding activity and shows good signaling activity [10][11][12]. The accuracy of the structure and the protonation states were analyzed with the program WHAT IF [13].…”

Section: Protein Setupmentioning

confidence: 99%

Identification of multiple allosteric sites on the M₁ muscarinic acetylcholine receptor

Espinoza-Fonseca

Trujillo‐Ferrara

2005

FEBS Letters

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Staurosporine and four staurosporine derivatives were docked on the rhodopsin-based homology model of the M 1 muscarinic acetylcholine receptor in order to localize the possible allosteric sites of this receptor. It was found that there were three major allosteric sites, two of which are located at the extracellular face of the receptor, and one in the intracellular domain of the receptor. In the present study, the localization of these binding sites is described for the first time. The present study confirms the existence of multiple allosteric sites on the M 1 muscarinic receptor, and lays the ground for further experimental and computational analysis to better understand how muscarinic receptors are modulated via their allosteric sites. These findings will also help to design and develop novel drugs acting as allosteric modulators of the M 1 receptor, which can be used in the treatment of the AlzheimerÕs disease.

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Transmembrane Domains 4 and 7 of the M1Muscarinic Acetylcholine Receptor Are Critical for Ligand Binding and the Receptor Activation Switch

Cited by 87 publications

References 36 publications

Generation of a homology model of the human histamine H3 receptor for ligand docking and pharmacophore-based screening

Generation of a homology model of the human histamine H3 receptor for ligand docking and pharmacophore-based screening

Characterization of a CNS penetrant, selective M₁muscarinic receptor agonist, 77‐LH‐28‐1

Identification of multiple allosteric sites on the M₁ muscarinic acetylcholine receptor

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Transmembrane Domains 4 and 7 of the M1Muscarinic Acetylcholine Receptor Are Critical for Ligand Binding and the Receptor Activation Switch

Cited by 87 publications

References 36 publications

Generation of a homology model of the human histamine H3 receptor for ligand docking and pharmacophore-based screening

Generation of a homology model of the human histamine H3 receptor for ligand docking and pharmacophore-based screening

Characterization of a CNS penetrant, selective M1muscarinic receptor agonist, 77‐LH‐28‐1

Identification of multiple allosteric sites on the M1 muscarinic acetylcholine receptor

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Characterization of a CNS penetrant, selective M₁muscarinic receptor agonist, 77‐LH‐28‐1

Identification of multiple allosteric sites on the M₁ muscarinic acetylcholine receptor