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人类外周血淋巴细胞中一种新的蛋白质磷酸化可能调控系统。I. 钙激活的、磷脂依赖性蛋白激酶的特性

A new possible regulatory system for protein phosphorylation in human peripheral lymphocytes. I. Characterization of a calcium-activated, phospholipid-dependent protein kinase.

作者信息

Ogawa Y, Takai Y, Kawahara Y, Kimura S, Nishizuka Y

出版信息

J Immunol. 1981 Oct;127(4):1369-74.

PMID:7276562
Abstract

A new species of protein kinase (protein kinase C), found in human peripheral lymphocytes, is 20 times more active than adenosine 3',5'-monophosphate-dependent protein kinase (protein kinase A) with histone as phosphate acceptor. This enzyme is normally present as an inactive form in soluble fraction, but attaches to membrane to exhibit full catalytic activity. This activation process is reversible, and absolutely requires Ca++. No other divalent cations can substitute for Ca++. The enzyme is independent of cyclic nucleotides. The active factor associated with membrane is phospholipid. The protein kinase shows a m.w. of 7.7 X 10(4). The pH optimum is 7.5 to 8.5. GTP does not serve as phosphate donor. The enzyme appears to show relatively broad substrate specificity that is distinctly different from that of protein kinase A. Although both protein kinases C and A react with H1 histone, analysis of the N-bromosuccinimide-bisected fragments of this radioactive histone has revealed that protein kinase C greatly favors seryl and threonyl residues of the C-terminal portion, whereas protein kinase A reacts preferentially with seryl residues in the N-terminal portion of this histone. Protein kinase C is protentially multifunctional and may regulate various Ca++-dependent cellular processes. It is noted that protein kinase C may be alternatively activated in an irreversible manner by limited proteolysis with Ca++-dependent neutral protease. The enzyme activated in this way is independent of Ca++ and membrane.

摘要

在人外周淋巴细胞中发现的一种新型蛋白激酶(蛋白激酶C),以组蛋白作为磷酸受体时,其活性比依赖于3',5'-环磷酸腺苷的蛋白激酶(蛋白激酶A)高20倍。这种酶通常以无活性形式存在于可溶性部分,但附着于膜上时会表现出完全的催化活性。这种激活过程是可逆的,并且绝对需要Ca++。没有其他二价阳离子可以替代Ca++。该酶不依赖于环核苷酸。与膜相关的活性因子是磷脂。该蛋白激酶的分子量为7.7×10(4)。最适pH为7.5至8.5。GTP不作为磷酸供体。该酶似乎表现出相对较宽的底物特异性,这与蛋白激酶A明显不同。虽然蛋白激酶C和A都与H1组蛋白反应,但对这种放射性组蛋白经N-溴代琥珀酰亚胺切割的片段进行分析表明,蛋白激酶C极大地倾向于C末端部分的丝氨酸和苏氨酸残基,而蛋白激酶A则优先与该组蛋白N末端部分的丝氨酸残基反应。蛋白激酶C具有潜在的多功能性,可能调节各种依赖Ca++的细胞过程。值得注意的是,蛋白激酶C可能会被依赖Ca++的中性蛋白酶进行有限的蛋白水解以不可逆的方式激活。以这种方式激活的酶不依赖于Ca++和膜。

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