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首页> 美国卫生研究院文献>Biochemical Journal >Purkinje cell protein-2 (Pcp2) stimulates differentiation in PC12 cells by Gβγ-mediated activation of Ras and p38 MAPK
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Purkinje cell protein-2 (Pcp2) stimulates differentiation in PC12 cells by Gβγ-mediated activation of Ras and p38 MAPK

机译:Purkinje细胞蛋白2(Pcp2)通过Gβγ介导的Ras和p38 MAPK激活刺激PC12细胞分化

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Purkinje cell protein-2 (Pcp2 or L7) is highly expressed in cerebellar Purkinje cells and retinal bipolar neurons and interacts with the Gαi/o family of G-proteins. Although the expression pattern of Pcp2 in the developing central nervous system suggests a role in differentiation, its function remains unknown. We established Tet-off inducible expression of Pcp2 in PC12 cells (rat pheochromocytoma cells) to determine whether Pcp2 regulates neuronal differentiation. Utilizing a polyclonal antibody, Pcp2 was localized in the cell body and throughout neurites of differentiated PC12 cells, similar to its localization in cerebellar Purkinje cells. Pcp2 expression in PC12 cells stimulated process formation (5-fold) and NGF (nerve growth factor)-stimulated neurite length (2-fold). Under basal conditions, Pcp2-PC12 cells demonstrated a 5-fold increase in Ras activation relative to non-induced PC12 cells and there was no change in extracellular-signal-regulated kinase 1/2 activity with Pcp2 expression. However, Pcp2 induction led to a >3-fold increase in basal p38 MAPK (mitogen-activated protein kinase) activity and the addition of NGF significantly stimulated both Ras and p38 MAPK in Pcp2-PC12 cells relative to the controls. Pretreatment of Pcp2-PC12 cells with the p38-specific inhibitor SB203580 blocked both the increased neurite formation and NGF-stimulated neurite growth. Pertussis toxin treatment had no effect on neurite growth in control cells, but completely blocked Pcp2-mediated increased neurite growth. Transient transfection of the β-adrenergic receptor kinase C-terminus to prevent signalling through Gβγ in Pcp2-PC12 cells also inhibited the Pcp2-induced phenotype and reduced the Pcp2-stimulated Ras activation. Taken together, these findings demonstrate that Pcp2 induces differentiation in PC12 cells, in part through Gβγ-mediated Ras and p38 MAPK activation and suggest the potential for similar signalling mechanisms in Purkinje cells.
机译:Purkinje细胞蛋白2(Pcp2或L7)在小脑Purkinje细胞和视网膜双极神经元中高表达,并与G蛋白的Gαi/ o家族相互作用。尽管Pcp2在发育中的中枢神经系统中的表达模式提示其在分化中的作用,但其功能仍然未知。我们在PC12细胞(大鼠嗜铬细胞瘤细胞)中建立了Pcp2的Tet-off诱导表达,以确定Pcp2是否调节神经元分化。利用多克隆抗体,Pcp2定位在分化的PC12细胞的细胞体内和整个神经突中,类似于其在小脑浦肯野细胞中的定位。 PC12细胞中的Pcp2表达刺激过程形成(5倍),而NGF(神经生长因子)刺激神经突长度(2倍)。在基础条件下,相对于未诱导的PC12细胞,Pcp2-PC12细胞的Ras激活增加了5倍,并且细胞外信号调节的激酶1/2活性与Pcp2表达没有变化。但是,Pcp2诱导导致基底p38 MAPK(促分裂原激活的蛋白激酶)活性增加> 3倍,并且添加NGF相对于对照组显着刺激Pcp2-PC12细胞中的Ras和p38 MAPK。用p38特异性抑制剂SB203580预处理Pcp2-PC12细胞可同时阻止增加的神经突形成和NGF刺激的神经突生长。百日咳毒素处理对对照细胞中的神经突生长没有影响,但是完全阻断了Pcp2介导的神经突生长的增加。为了防止Pcp2-PC12细胞中通过Gβγ的信号传导,β-肾上腺素受体激酶C末端的瞬时转染也抑制了Pcp2诱导的表型并降低了Pcp2刺激的Ras激活。综上所述,这些发现表明,Pcp2部分地通过Gβγ介导的Ras和p38 MAPK激活诱导PC12细胞分化,并暗示了Purkinje细胞中类似信号机制的潜力。

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