Evidence for protein kinase C in bovine adrenocortical membrane preparations using [35S] gamma-thio-ATP as a phosphate donor.

M D Coyne, H M Luszczynska, M Kunzi
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Abstract

Thio-substituted ATP is a sensitive probe for detecting protein kinase C activity as demonstrated in bovine adrenocortical cell membrane preparations. A single endogenous protein substrate with a molecular weight of approximately 47 Kd was rapidly phosphorylated with [3 5S] gamma-thio-ATP as phosphate donor. Phosphorylation was significantly increased in 30 seconds and reached a plateau by 3 minutes. The activity of the endogenous membrane kinase was unaffected by ACTH, cAMP, calmodulin or trifluoperazine but was responsive to combinations of calcium (Ca), diolein and phosphatidyl serine (PS). In addition, the kinase was activated by the tumor promoting phorbol ester, 12-0-tetradecanoylphorbol-13-acetate, indicating that the membrane contains a protein kinase C and a single 47 Kd phosphorylatable protein substrate. The same substrate is phosphorylated by Ca/diolein/PS activated kinase in membrane preparations from a broad range of rat tissues. Attempts to identify the substrate indicate that it is neither the type I regulatory subunit of cAMP dependent protein kinase nor mitochondrial cytochrome P450.

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用[35S] γ -硫代atp作为磷酸盐供体制备的牛肾上腺皮质膜中蛋白激酶C的证据。
硫代ATP是一种检测蛋白激酶C活性的灵敏探针,已在牛肾上腺皮质细胞膜制剂中得到证实。一个分子量约为47 Kd的内源性蛋白底物被[3 5S] γ -硫代atp作为磷酸供体快速磷酸化。磷酸化在30秒内显著增加,在3分钟内达到平稳期。内源性膜激酶的活性不受ACTH、cAMP、钙调素或三氟拉嗪的影响,但对钙(Ca)、二油和磷脂酰丝氨酸(PS)的组合有反应。此外,该激酶可被促肿瘤磷脂酯(12-0- tetradecanoylphobol -13-acetate)激活,表明该膜含有蛋白激酶C和单个47 Kd可磷酸化的蛋白底物。在广泛的大鼠组织的膜制剂中,同样的底物被Ca/二油苷/PS活化激酶磷酸化。鉴定底物的尝试表明,它既不是cAMP依赖性蛋白激酶的I型调节亚基,也不是线粒体细胞色素P450。
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Calmodulin is required for a full activation of the calcium slow channels in heart cells. The escape of cyclic AMP from dog thyroid slices exposed to positive and negative regulators. Do porins inhibit the macrophage phagocyting activity by stimulating the adenylate cyclase? Kinetic evidence indicating separate stimulatory and inhibitory prostaglandin receptors on platelet membranes. A micromethod for the quantitation by radioimmunoassay of cyclic AMP in samples containing immuno-cross reactive compounds and other interfering substances.
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