Isolation of InsP4 and InsP6 binding proteins from human platelets: InsP4 promotes Ca2+ efflux from inside-out plasma membrane vesicles containing 104 kDa GAP1IP4BP protein

Abstract

A low-density membrane fraction from human platelets contained the plasma membrane marker glycoprotein Ib (GpIb) and selective binding sites for InsP₄ and InsP₆. It was separated from the bulk of InsP₃-receptor-containing membranes, but was heterogeneous, probably also containing surface-connected canalicular system and some lighter elements of the internal dense tubule system. After loading with calcium oxalate and re-centrifugation on Percoll gradients, this mixed fraction was subfractionated into light membranes containing all of the GpIb, high-affinity InsP₄ binding sites (K_D = 18 nM) and phosphate-stimulated Ca²⁺ transport activity. InsP₄ (EC₅₀ 0.6 μM), but not InsP₃ or InsP₆, released up to 35% of the accumulated Ca²⁺ from these vesicles, which were shown to be inside-out plasma membrane vesicles by a biotinylation labelling technique and selective removal of right-side-out plasma membrane vesicles with streptavidin–agarose. Most of the InsP₄, and all of the InsP₆, binding was present in the much denser calcium oxalate-loaded subfractions, which were free of GpIb. InsP₆ binding activity was chromatographically purified as a 116 kDa protein (K_D for InsP₆ = 5.9 nM), with an amino acid content and two internal peptide sequences identical to those of 116 kDa vinculin. A 104 kDa InsP₄ binding protein (K_D for InsP₄ = 12 nM), probably identical to GAP1^IP4BP described by Cullen, Hsuan, Truong, Letcher, Jackson, Dawson and Irvine [(1995) Nature (London) 376, 527–530], was also isolated. This InsP₄ receptor may mediate Ca²⁺ influx in platelets that occurs subsequent to receptor-stimulated production of InsP₃ and unloading of internal Ca²⁺ stores.