Europium-labeled melanin-concentrating hormone analogues: ligands for measuring binding to melanin-concentrating hormone receptors 1 and 2

We investigated the use of Eu 3+ chelate-labeled analogues of melanin-concentrating hormone (MCH) as ligands for both human MCH receptors (MCHR1 and MCHR2). The analogues employed were Ala 17 MCH, S36057 (Y-ADO-RC*MLGRVFRPC*W, where ADO=8-amino-3,6-dioxyoctanoyl and *=disulfide bond), and R2P (RC*ML...

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Veröffentlicht in:Analytical biochemistry 2004-05, Vol.328 (2), p.187-195
Hauptverfasser: Gao, Xiaoying, Hsu, Chiun-King, Heinz, Lawrence J, Morin, John, Shi, Yuguang, Shukla, Nikhil K, Smiley, David L, Xu, Jie, Zhong, Boyu, Slieker, Lawrence J
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container_end_page 195
container_issue 2
container_start_page 187
container_title Analytical biochemistry
container_volume 328
creator Gao, Xiaoying
Hsu, Chiun-King
Heinz, Lawrence J
Morin, John
Shi, Yuguang
Shukla, Nikhil K
Smiley, David L
Xu, Jie
Zhong, Boyu
Slieker, Lawrence J
description We investigated the use of Eu 3+ chelate-labeled analogues of melanin-concentrating hormone (MCH) as ligands for both human MCH receptors (MCHR1 and MCHR2). The analogues employed were Ala 17 MCH, S36057 (Y-ADO-RC*MLGRVFRPC*W, where ADO=8-amino-3,6-dioxyoctanoyl and *=disulfide bond), and R2P (RC*MLGRVFRPC*Y-NH 2). The peptides were readily labeled on the α-amino residue with the Eu 3+ chelate of N 1-( p-isothiocyanatobenzyl)-diethylenetriamine- N 1, N 2, N 3, N 3-tetraacetic acid and then purified by reverse-phase fast-performance liquid chromatography at neutral pH to maintain Eu 3+ chelation. Both labeled Ala 17 MCH and S36057 had high affinity for MCHR1 ( K d=0.37 and 0.059 nM, respectively) while Eu 3+-labeled S36057 and R2P had high affinity for MCHR2 ( K d=0.16 and 0.10 nM, respectively). Labeled Ala 17 MCH had little demonstrable binding affinity for MCHR2. Eu 3+-labeled S36057 and R2P were full agonists at MCHR1 when assessed by measurement of agonist-stimulated GTPγ 35S binding. Competition binding experiments with both MCHR isoforms, a series of previously characterized alanine scan MCH analogues, and a recently identified nonpeptide MCHR1-selective antagonist T-226296 confirmed the expected receptor selectivity. These studies further extend the utility of Eu 3+ chelate time-resolved fluorescence for the development of high-sensitivity, nonradioactive receptor binding assays and demonstrate the need to select the optimal ligand for labeling.
doi_str_mv 10.1016/j.ab.2004.01.017
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The analogues employed were Ala 17 MCH, S36057 (Y-ADO-RC*MLGRVFRPC*W, where ADO=8-amino-3,6-dioxyoctanoyl and *=disulfide bond), and R2P (RC*MLGRVFRPC*Y-NH 2). The peptides were readily labeled on the α-amino residue with the Eu 3+ chelate of N 1-( p-isothiocyanatobenzyl)-diethylenetriamine- N 1, N 2, N 3, N 3-tetraacetic acid and then purified by reverse-phase fast-performance liquid chromatography at neutral pH to maintain Eu 3+ chelation. Both labeled Ala 17 MCH and S36057 had high affinity for MCHR1 ( K d=0.37 and 0.059 nM, respectively) while Eu 3+-labeled S36057 and R2P had high affinity for MCHR2 ( K d=0.16 and 0.10 nM, respectively). Labeled Ala 17 MCH had little demonstrable binding affinity for MCHR2. Eu 3+-labeled S36057 and R2P were full agonists at MCHR1 when assessed by measurement of agonist-stimulated GTPγ 35S binding. Competition binding experiments with both MCHR isoforms, a series of previously characterized alanine scan MCH analogues, and a recently identified nonpeptide MCHR1-selective antagonist T-226296 confirmed the expected receptor selectivity. 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Competition binding experiments with both MCHR isoforms, a series of previously characterized alanine scan MCH analogues, and a recently identified nonpeptide MCHR1-selective antagonist T-226296 confirmed the expected receptor selectivity. 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The analogues employed were Ala 17 MCH, S36057 (Y-ADO-RC*MLGRVFRPC*W, where ADO=8-amino-3,6-dioxyoctanoyl and *=disulfide bond), and R2P (RC*MLGRVFRPC*Y-NH 2). The peptides were readily labeled on the α-amino residue with the Eu 3+ chelate of N 1-( p-isothiocyanatobenzyl)-diethylenetriamine- N 1, N 2, N 3, N 3-tetraacetic acid and then purified by reverse-phase fast-performance liquid chromatography at neutral pH to maintain Eu 3+ chelation. Both labeled Ala 17 MCH and S36057 had high affinity for MCHR1 ( K d=0.37 and 0.059 nM, respectively) while Eu 3+-labeled S36057 and R2P had high affinity for MCHR2 ( K d=0.16 and 0.10 nM, respectively). Labeled Ala 17 MCH had little demonstrable binding affinity for MCHR2. Eu 3+-labeled S36057 and R2P were full agonists at MCHR1 when assessed by measurement of agonist-stimulated GTPγ 35S binding. Competition binding experiments with both MCHR isoforms, a series of previously characterized alanine scan MCH analogues, and a recently identified nonpeptide MCHR1-selective antagonist T-226296 confirmed the expected receptor selectivity. These studies further extend the utility of Eu 3+ chelate time-resolved fluorescence for the development of high-sensitivity, nonradioactive receptor binding assays and demonstrate the need to select the optimal ligand for labeling.</abstract><cop>United States</cop><pub>Elsevier Inc</pub><pmid>15113696</pmid><doi>10.1016/j.ab.2004.01.017</doi><tpages>9</tpages></addata></record>
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subjects Binding, Competitive
Cell Line
Cell Membrane - metabolism
Cloning, Molecular
Disulfides - chemistry
Disulfides - metabolism
Europium - chemistry
Fluorescence
Humans
Ligands
Melanins - chemistry
Melanins - metabolism
Organometallic Compounds - chemistry
Protein Binding
Radioligand Assay
Receptors, Pituitary Hormone - metabolism
Sensitivity and Specificity
Staining and Labeling
title Europium-labeled melanin-concentrating hormone analogues: ligands for measuring binding to melanin-concentrating hormone receptors 1 and 2
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