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Inhibition of insulin secretion from rat islets of Langerhans is known to involve at least one pertussis toxin-sensitive guanine-nucleotide binding (G) protein. We have used antisera raised against unique antigenic determinants of different members of the family of pertussis toxin-sensitive G proteins to identify these proteins in rat islets. Antiserum SG1, which recognizes both G_i1 and G_i2, reacted with an islet protein having an approximate M_r of 40 000. Antiserum IlC (G_i1 specific) failed to recognize any islet proteins, suggesting that G_i2 is present in much greater amounts than G_i1. Indeed, G_i1 levels were below the detection limit of a sensitive immunogold/silver-staining method, indicating that it may be absent from the cells of rat islets.

Two different antisera were used to identify G_o-like G proteins in rat islet homogenates. Both antisera reacted with a protein band which, under appropriate conditions, could be resolved to reveal two separate proteins of M_r 39–40 000. Thus, at least two molecular forms of G_o are present in rat islets.

Subcellular fractionation indicated that all three G proteins identified in this study (G_i2 and two forms of G_o) are localized to islet membranes. No immunoreactivity could be detected in the cytosolic fraction.