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Raf足以促使海马神经元细胞分化,但MEK或ERK则不然。

Raf, but not MEK or ERK, is sufficient for differentiation of hippocampal neuronal cells.

作者信息

Kuo W L, Abe M, Rhee J, Eves E M, McCarthy S A, Yan M, Templeton D J, McMahon M, Rosner M R

机构信息

Ben May Institute, University of Chicago, Ilinois 60637, USA.

出版信息

Mol Cell Biol. 1996 Apr;16(4):1458-70. doi: 10.1128/MCB.16.4.1458.

Abstract

To elucidate signal transduction pathways leading to neuronal differentiation, we have investigated a conditionally immortalized cell line from rat hippocampal neurons (H19-7) that express a temperature sensitive simian virus 40 large T antigen. Treatment of H19-7 cells with the differentiating agent basic fibroblast growth factor at 39 degrees C, the nonpermissive temperature for T function, resulted in the activation of c-Raf-1, MEK, and mitogen-activated protein (MAP) kinases (ERK1 and -2). To evaluate the role of Raf-1 in neuronal cell differentiation, we stably transfected H19-7 cells with v-raf or an oncogenic human Raf-1-estrogen receptor fusion gene (deltaRaf-1:ER). deltaRaf-1:ER transfectants in the presence of estradiol for 1 to 2 days expressed a differentiation phenotype only at the nonpermissive temperature. However, extended exposure of the deltaRaf-1:ER transfectants to estradiol or stable expression of the v-raf construct yielded cells that extended processes at the permissive as well as the nonpermissive temperature, suggesting that cells expressing the large T antigen are capable of responding to the Raf differentiation signal. deltaRaf-1:ER, MEK, and MAP kinase activities in the deltaRaf-1:ER cells were elevated constitutively for up to 36 h of estradiol treatment at the permissive temperature. At the nonpermissive temperature, MEK and ERKs were activated to a significantly lesser extent, suggesting that prolonged MAP kinase activation may not be sufficient for differentiation. To test this possibility, H19-7 cells were transfected or microinjected with constitutively activated MEK. The results indicate that prolonged activation of MEK or MAP kinases (ERK1 and -2) is not sufficient for differentiation of H19-7 neuronal cells and raise the possibility that an alternative signaling pathway is required for differentiation of H19-7 cells by Raf.

摘要

为阐明导致神经元分化的信号转导途径,我们研究了一种来自大鼠海马神经元的条件永生化细胞系(H19-7),该细胞系表达温度敏感的猿猴病毒40大T抗原。在39摄氏度(T功能的非允许温度)下用分化剂碱性成纤维细胞生长因子处理H19-7细胞,导致c-Raf-1、MEK和丝裂原活化蛋白(MAP)激酶(ERK1和-2)的激活。为评估Raf-1在神经元细胞分化中的作用,我们用v-raf或致癌性人Raf-1-雌激素受体融合基因(deltaRaf-1:ER)稳定转染H19-7细胞。在存在雌二醇的情况下,deltaRaf-1:ER转染子在1至2天内仅在非允许温度下表现出分化表型。然而,deltaRaf-1:ER转染子长时间暴露于雌二醇或v-raf构建体的稳定表达产生了在允许温度和非允许温度下都能延伸突起的细胞,这表明表达大T抗原的细胞能够响应Raf分化信号。在允许温度下,用雌二醇处理deltaRaf-1:ER细胞长达36小时,其deltaRaf-1:ER、MEK和MAP激酶活性持续升高。在非允许温度下,MEK和ERK的激活程度明显较低,这表明延长的MAP激酶激活可能不足以实现分化。为检验这种可能性,用组成型激活的MEK转染或显微注射H19-7细胞。结果表明,MEK或MAP激酶(ERK1和-2)的延长激活不足以使H19-7神经元细胞分化,并增加了Raf诱导H19-7细胞分化需要另一种信号通路的可能性。

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