Agonist‐sensitive binding of a photoreactive GTP analog to a G‐protein α‐subunit in membranes of HL‐60 cells

Abstract

Myeloid‐differentiated HL‐60 cells were used to study the activation of G‐proteins by receptor agonists. Following incubation of membranes with the photoreactive GTP analog. [α‐³²P]GTP azidoanilide, and subsequent exposure to ultraviolet light (254 nm), photolabeling of 40 kDa proteins comigrating with the G_i2 α‐subunit was observed. Photolabeling in the absence or presence of the chemoattractant, N‐ionnyl‐methionyl‐leucyi‐phenylalanin (FMLP), absolutely required Mg²⁺; FMLP stimulated photolabeling at all Mg²⁺ concentrations employed (up to 30 mM). Addition of GDP (3–50 μM) reduced basal photolabeling to a greater extent than photolabeling stimulated by FMLP. FMLP did not stimulate photolabeling of proteins modified by pertussis toxin. Leukotriene B₄ and C5a also stimulated photolabeling of 40 kDa proteins. The results indicate that (i) the major G‐protein in HL‐60 cells, G_i2 requires Mg²⁺ for basal and receptor‐stimulated activity, (ii) effective receptor‐mediated activation of G‐proteins is observed at mM concentrations of Mg²⁺, and (iii) receptor agonists apparently reduce the affinity of G‐proteins for GDP.