Determining the Environment of the Ligand Binding Pocket of the Human Angiotensin II Type I (hAT1) Receptor Using the Methionine Proximity Assay

Clement, M.G.; Martin, Stéphane; Beaulieu, Marie-Ève; Chamberland, Caroline; Lavigne, Pierre; Leduc, Richard; Guillemette, Gaétan; Escher, Emanuel

doi:10.1074/jbc.m413653200

Cited by 63 publications

(89 citation statements)

References 46 publications

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“…Importantly, although 24 positions were probed, only 4 cross-linked. This contrasts to the observation of many cross-linking sites detected due to the "methionine magnet effect" (14)(15)(16)(17)(18)(19). The novel sites of interaction identified by this study generated a molecular model that exhibits important differences from our previous model based on Bpa photoaffinity cross-linking data.…”

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confidence: 86%

Mapping Peptide Hormone−Receptor Interactions Using a Disulfide-Trapping Approach

et al. 2008

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Efforts to elucidate the nature of the bimolecular interaction of parathyroid hormone (PTH) with its cognate receptor, the PTH receptor type 1 (PTHR1), have relied heavily on benzoylphenylalanine-(Bpa-) based photoaffinity cross-linking. However, given the flexibility, size, and shape of Bpa, the resolution at the PTH-PTHR1 interface appears to be reaching the limit of this technique. Here we employ a disulfide-trapping approach developed by others primarily for use in screening compound libraries to identify novel ligands. In this method, cysteine substitutions are introduced into a specific site within the ligand and a region in the receptor predicted to interact with each other. Upon ligand binding, if these cysteines are in close proximity, they form a disulfide bond. Since the geometry governing disulfide bond formation is more constrained than Bpa cross-linking, this novel approach can be employed to generate a more refined molecular model of the PTH-PTHR1 complex. Using a PTH analogue containing a cysteine at position 1, we probed 24 sites and identified 4 in PTHR1 to which cross-linking occurred. Importantly, previous photoaffinity cross-linking studies using a PTH analogue with Bpa at position 1 only identified a single interaction site. The new sites identified by the disulfide-trapping procedure were used as constraints in molecular dynamics simulations to generate an updated model of the PTH-PTHR1 complex. Mapping by disulfide trapping extends and complements photoaffinity cross-linking. It is applicable to other peptide-receptor interfaces and should yield insights about yet unknown sites of ligand-receptor interactions, allowing for generation of more refined models.Class II G protein-coupled receptors (GPCRs) 1 interact with physiologically important peptides. There is intense study of how these peptides associate with their cognate receptors since elucidation of these interactions should provide important insights for the rational design of ligands with enhanced pharmacological properties for use in treating an array of diseases (1,2). Over the past decade, photoaffinity cross-linking has been employed to study the interaction of a number of peptide-GPCR interactions (3). This technique involves systematically probing the receptor for regions of interaction using a peptide that incorporates a photoreactive moiety that irreversibly cross-links to the receptor. We and others have used this approach extensively to study the interaction of parathyroid hormone (PTH) with its cognate receptor, the PTH receptor type 1 (PTHR1) (4-12). This hormone-receptor system plays an integral role in calcium metabolism and bone biology. † This work was supported in part by Grants DK47490 (to M.R.) and GM54082 (to D.F.M.) from the National Institutes of Health.* Address correspondence to this author. Phone: (617) Our research is focused on studying the bimolecular interface of the PTH-PTHR1 complex in order to gain insights that will aid the design of ligands of PTHR1 for the treatment of osteoporosis and o...

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confidence: 86%

Mapping Peptide Hormone−Receptor Interactions Using a Disulfide-Trapping Approach

et al. 2008

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“…This observation was recently used by Escher and coworkers in the design of a ''Methionine Proximity Assay'' (MPA) [20]. Scanning through three transmembrane domains of the angiotensin receptor, they identified the binding groove for Bpa in position 8 of angiotensin [20]. Our study demonstrates that the preferential reactivity of Bpa for methionine over other amino acids in a target domain can be more pronounced than previously appreciated.…”

Section: Discussionsupporting

confidence: 50%

“…The characteristic low MW band corresponding to free ligand makes detection straightforward. This observation was recently used by Escher and coworkers in the design of a ''Methionine Proximity Assay'' (MPA) [20]. Scanning through three transmembrane domains of the angiotensin receptor, they identified the binding groove for Bpa in position 8 of angiotensin [20].…”

Section: Discussionmentioning

confidence: 98%

Methionine acts as a “magnet” in photoaffinity crosslinking experiments

et al. 2006

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Photoaffinity crosslinking has been utilized to probe the nature of the ligand-receptor interface for a number of G protein-coupled receptor systems. Often the photoreactive benzophenone moiety incorporated in the ligand is found to react with a methionine in the receptor. We introduced methionines one-ata-time into the region 163-176 of the parathyroid hormone receptor, and find that crosslinking occurs to the side-chain of methionine over a range of 11 amino acids. We call this the ''Magnet Effect'' of methionine. Hence, crosslinking contact points can be significantly shifted by the presence of methionine in a receptor domain.

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“…In docking to models without disul fide bond, all ligands under study were docked inside a binding pocket formed in between in the core of the receptor; large peptide ligands interact at the same time with the TM helices and extracellular loops. This characteristic binding is also postulated for other neuropeptides including NPY (Sautel et al 1995, Sjödin et al 2006, angiotensin (Clément et al 2005), and somatostatin (Strnad and Hadcock 1995). However, docking to models with this disul fide bond present yielded no good binding poses for any ligands, indicating that the reduced form must exist for ligand binding.…”

Section: Discussionmentioning

confidence: 73%

Ligand binding properties of human galanin receptors

Jurkowski

Elofsson

2012

Molecular Membrane Biology

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This is an accepted version of a paper published in Molecular membrane biology. This paper has been peer-reviewed but does not include the final publisher proof-corrections or journal pagination.Citation for the published paper: Jurkowski, W., Yazdi, S., Elofsson, A. (2013) AbstractThe galanin receptor family comprises of three members, GalR1, GalR2 and GalR3, all belonging to the G-protein-couple receptor superfamily. All three receptors bind the peptide hormone galanin, but show distinctly di erent binding properties to other molecules and e ects on intracellular signaling. To gain insight on the molecular basis of receptor subtype speci ficity, we have generated a three-dimensional model for each of the galanin receptors based on its homologs in the same family. We found significant di erences in the organization of the binding pockets among the three types of receptors, which might be the key for specific molecular recognition o igands. Through docking o ragments of the galanin peptide and a number o igands, we investigated the involvement of transmembrane and loop residues in ligand interaction.

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Determining the Environment of the Ligand Binding Pocket of the Human Angiotensin II Type I (hAT1) Receptor Using the Methionine Proximity Assay

Cited by 63 publications

References 46 publications

Mapping Peptide Hormone−Receptor Interactions Using a Disulfide-Trapping Approach

Mapping Peptide Hormone−Receptor Interactions Using a Disulfide-Trapping Approach

Methionine acts as a “magnet” in photoaffinity crosslinking experiments

Ligand binding properties of human galanin receptors

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