Kinetic and functional properties of [ 3H]ZM241385, a high affinity antagonist for adenosine A 2A receptors

Kinetic and functional properties of [ 3H]ZM241385, a high affinity antagonist for adenosine A 2A receptors

We have characterized the binding of [2- 3H]-4-(2-[7-Amino-2-(2-furyl)-[1,2,4]-triazolo-[2,3-a]-[1,3,5]-triazin-5-ylamino]ethyl)phenol ([ 3H]ZM241385) to adenosine A 2A receptors in membranes of rat striatum and transfected CHO cells. Saturation experiments showed that [ 3H]ZM241385 binds to a singl...

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Veröffentlicht in:Life sciences (1973) 2005, Vol.76 (13), p.1513-1526
Hauptverfasser: Uustare, Ain, Vonk, Argo, Terasmaa, Anton, Fuxe, Kjell, Rinken, Ago
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[ 3H]ZM241385
Adenosine A 2A receptors
Adenylate cyclase
CGS 21680
Isomerization
Kinetic mechanism
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container_end_page 1526
container_issue 13
container_start_page 1513
container_title Life sciences (1973)
container_volume 76
creator Uustare, Ain
Vonk, Argo
Terasmaa, Anton
Fuxe, Kjell
Rinken, Ago
description We have characterized the binding of [2- 3H]-4-(2-[7-Amino-2-(2-furyl)-[1,2,4]-triazolo-[2,3-a]-[1,3,5]-triazin-5-ylamino]ethyl)phenol ([ 3H]ZM241385) to adenosine A 2A receptors in membranes of rat striatum and transfected CHO cells. Saturation experiments showed that [ 3H]ZM241385 binds to a single class of binding sites with high affinity (K d = 0.23 nM and 0.14 nM in CHO cell and striatal membranes, respectively). The membranes of CHO cells required pretreatment with adenosine deaminase (ADA) to achieve high-affinity binding, while ADA had no influence on the ligand binding properties in striatal membranes. The binding of [ 3H]ZM241385 was fast and reversible, achieving equilibrium within 20 minutes at all radioligand concentrations. The kinetic analysis of the [ 3H]ZM241385 interaction with A 2A receptors indicated that the reaction had at least two subsequent steps. The first step corresponds to a fast equilibrium, which also determines the antagonist potency to competitively inhibit CGS21680-induced accumulation of cAMP (first equilibrium constant K A = 6.6 nM). The second step corresponds to a slow process of conformational isomerization (equilibrium constant K i = 0.03). The combination of the two steps gives the dissociation constant K d = 0.20 nM based on the kinetic data, which is in good agreement with the directly measured value. The data obtained shed light on the mechanism of the [ 3H]ZM241385 interaction with adenosine A 2A receptors from different sources in vitro. The isomerization step of the A 2A antagonist radioligand binding has to be taken into account for the interpretation of the binding parameters obtained from the various competition assays and explain the discrepancy between antagonist affinity in saturation experiments versus its potency in functional assays.
doi_str_mv 10.1016/j.lfs.2004.10.027
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subjects [ 3H]ZM241385
Adenosine A 2A receptors
Adenylate cyclase
CGS 21680
Isomerization
Kinetic mechanism
title Kinetic and functional properties of [ 3H]ZM241385, a high affinity antagonist for adenosine A 2A receptors
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