Pharmacological characterization of the chemokine receptor, hCCR1 in a stable transfectant and differentiated HL-60 cells: antagonism of hCCR1 activation by MIP-1beta

Chuan-Chu Chou; Jay S Fine; Catherine Pugliese-Sivo; Waldemar Gonsiorek; Liza Davies; Gregory Deno; Mary Petro; Martin Schwarz; Paul J Zavodny; R William Hipkin

doi:10.1038/sj.bjp.0704907

Pharmacological characterization of the chemokine receptor, hCCR1 in a stable transfectant and differentiated HL-60 cells: antagonism of hCCR1 activation by MIP-1beta

Br J Pharmacol. 2002 Nov;137(5):663-75. doi: 10.1038/sj.bjp.0704907.

Authors

Chuan-Chu Chou¹, Jay S Fine, Catherine Pugliese-Sivo, Waldemar Gonsiorek, Liza Davies, Gregory Deno, Mary Petro, Martin Schwarz, Paul J Zavodny, R William Hipkin

Affiliation

¹ Department of Immunology, Schering-Plough Research Institute, Kenilworth, New Jersey, NJ 07033, USA.

Abstract

C-C chemokine receptor-1 (CCR1) has been implicated in mediating a variety of inflammatory conditions including multiple sclerosis and organ rejection. Although originally referred to as the MIP-1alpha/RANTES receptor, CCR1 is quite promiscuous and can be activated by numerous chemokines. We used radioligand binding and [35S]-GTPgammaS exchange assays in membranes from a cell line transfected to express CCR1 (Ba/F3-hCCR1) to characterize a panel of chemokines (HCC-1, MIP-1alpha, MIP-1beta, MIP-1delta, MPIF-1, MCP-2, MCP-3, and RANTES) as CCR1 ligands. In this recombinant model, these chemokines displaced 125I-MIP-1alpha with a wide range of potencies and, with the exception of MCP-2, acted as full agonists in stimulating [35S]-GTPgammaS exchange. We then assessed the utility of HL-60 cells cultured with known differentiating agents (PMA, DMSO, dibutyryl-cAMP or retinoic acid) for investigating CCR1 pharmacology. In [35S]-GTPgammaS exchange assays, membranes from cells cultured with retinoic acid (4-6 days) were the most responsive to activation by MIP-1alpha and MPIF-1. FACS analysis and comparative pharmacology confirmed that these activities were mediated by CCR1. Using [35S]-GTPgammaS exchange assays, intracellular calcium flux and/or whole cell chemotaxis assays in HL-60(Rx) cells, we validated that MIP-1alpha was the most potent CCR1 ligand (MIP-1alpha>MPIF-1>RANTES>or=MIP-1beta) although the ligands differed in their efficacy as agonists. MPIF-1 was the more efficacious (MPIF-1>RANTES=MIP-1alpha>>MIP-1beta). 125I-MIP-1beta binding in Ba/F3-hCCR1 and HL-60(Rx) membranes was competitively displaced by MIP-1alpha, MPIF-1 and MIP-1beta. The binding K(i) for these chemokines with 125I-MIP-1beta were essentially identical in the two membrane systems. Lastly, MIP-1beta antagonized [35S]-GTPgammaS exchange, Ca2+ flux and chemotaxis in HL-60(Rx) cells in response to robust agonists such as MIP-1alpha, RANTES and MPIF-1. Based on our results, we propose that MIP-1beta could function as an endogenous inhibitor of CCR1 function.

MeSH terms

Animals
Cell Differentiation / drug effects
Cell Differentiation / physiology
Chemokine CCL3
Chemokine CCL4
Chemokines / pharmacology
Dose-Response Relationship, Drug
HL-60 Cells / drug effects*
HL-60 Cells / metabolism*
Humans
Macrophage Inflammatory Proteins / pharmacology*
Mice
Receptors, CCR1
Receptors, Chemokine / antagonists & inhibitors*
Receptors, Chemokine / genetics
Receptors, Chemokine / metabolism*
Transfection / methods

Substances

CCR1 protein, human
Ccr1 protein, mouse
Chemokine CCL3
Chemokine CCL4
Chemokines
Macrophage Inflammatory Proteins
Receptors, CCR1
Receptors, Chemokine