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ζ蛋白激酶C在神经生长因子诱导的PC12细胞分化中的作用。

A role for zeta protein kinase C in nerve growth factor-induced differentiation of PC12 cells.

作者信息

Wooten M W, Zhou G, Seibenhener M L, Coleman E S

机构信息

Department of Zoology, Auburn University, Alabama 36849.

出版信息

Cell Growth Differ. 1994 Apr;5(4):395-403.

PMID:8043513
Abstract

Studies were undertaken to compare the signal-induced redistribution of conventional protein kinase C (cPKC) to nonclassical protein kinase C (nPKC) family members in response to phorbol 12-myristate 13-acetate (PMA) or nerve growth factor (NGF) treatment of PC12 cells. cPKC-alpha and -beta and nPKC-delta and -epsilon were predominantly cytoplasmic, whereas PKC-zeta displayed approximately equal distribution between the cytoplasm and membrane fraction. Treatment of PC12 cells with PMA induced rapid translocation of both c- and nPKC isoforms to the membrane fraction, although the kinetics varied between isoforms with epsilon being most sensitive, followed by delta > zeta > alpha. Both PKC-epsilon and delta translocated in the presence of minute concentrations of PMA, whereas cPKC was less sensitive, and PKC-zeta was least sensitive. NGF treatment, on the other hand, induced translocation of cPKCs and delta and epsilon nPKC, albeit with differential magnitude, whereas PKC-zeta was found predominantly in the cytoplasm. Chronic treatment of PC12 cells with PMA (1 microM) caused a rapid disappearance of alpha, beta, delta, and epsilon PKC isoforms, whereas the expression of PKC-zeta was unaltered over 4 days. NGF induced an increase in cytoplasmic PKC-zeta in control, or PMA down-regulated PC12 cells. Moreover, the increase in cytoplasmic PKC-zeta was blocked by pretreatment with sphingosine (2.5 microM). Furthermore, PKC-zeta was activated by NGF in PMA down-regulated PC12 cells, as determined by the extent of epsilon-peptide phosphorylation using a permeabilized cell assay. In addition, the zeta-pseudosubstrate peptide inhibited NGF-induced activation of PKC-zeta.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

开展了多项研究,以比较在佛波醇12 - 肉豆蔻酸酯13 - 乙酸酯(PMA)或神经生长因子(NGF)处理PC12细胞后,信号诱导的传统蛋白激酶C(cPKC)与非经典蛋白激酶C(nPKC)家族成员的重新分布情况。cPKC - α和 - β以及nPKC - δ和 - ε主要位于细胞质中,而PKC - ζ在细胞质和膜部分的分布大致相等。用PMA处理PC12细胞会诱导cPKC和nPKC亚型快速转位至膜部分,尽管不同亚型的动力学有所不同,其中ε最敏感,其次是δ > ζ > α。PKC - ε和δ在微量浓度的PMA存在下就会转位,而cPKC较不敏感,PKC - ζ最不敏感。另一方面,NGF处理会诱导cPKC以及δ和ε nPKC转位,尽管程度有所不同,而PKC - ζ主要存在于细胞质中。用PMA(1微摩尔)长期处理PC12细胞会导致α、β、δ和ε PKC亚型迅速消失,而PKC - ζ的表达在4天内未改变。在对照或PMA下调的PC12细胞中,NGF诱导细胞质中PKC - ζ增加。此外,用鞘氨醇(2.5微摩尔)预处理可阻断细胞质中PKC - ζ的增加。此外,在PMA下调的PC12细胞中,通过使用透化细胞测定法检测ε - 肽磷酸化程度,发现PKC - ζ被NGF激活。此外,ζ - 假底物肽可抑制NGF诱导的PKC - ζ激活。(摘要截短于250字)

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