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cAMP‐independent and cAMP‐dependent protein phosphorylations by isolated goldfish xanthophore cytoskeletons: Evidence for the association of cytoskeleton with a carotenoid droplet protein

机译:cAMP‐independent and cAMP‐dependent protein phosphorylations by isolated goldfish xanthophore cytoskeletons: Evidence for the association of cytoskeleton with a carotenoid droplet protein

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AbstractTriton‐insoluble cytoskeleton of nonpigment cells has bound protein kinase that phosphorylates, with or without added cAMP, tubulins and the intermediate filament proteins p60, p56, p53, and p45a to give multiple charge variants. In the absence of 8‐Br‐cAMP, Triton‐insoluble cytoskeletons from xanthophores also phosphorylate p60, p56, and p45a, but not p53; tubulin phosphorylation may also be reduced. In the presence of 8‐Br‐cAMP, p53, as well as several other peptides, are phosphorylated. One of these latter peptides was identified as the carotenoid droplet (pigment organelle) protein p57, whose phosphorylation and dephosphorylation precede pigment dispersion and aggregation respectively (Lynch et al.: J. Biol. Chem. 261:4204–4211, 1986). The amount of pp57 produced depends on the state of pigment distribution in the xanthophores used to prepare the cytoskeletons for labeling. With cytoskeletons from xanthophores with aggregated pigment, pp57 is a major labeled phosphoprotein seen in two‐dimensional gels. With cytoskeletons prepared from xanthophores with dispersed pigment, the yield of labeled pp57 is greatly reduced (by at least 90). Together with earlier results, we propose that, in the aggregated state, p57 serves to bind carotenoid droplets to the cytoskeletons, most likely the microtubules. The significance of other cAMP‐dependent phosphorylation reactions is unknown but may be related to cAMP‐induced cytoskeleton rearrangement in

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