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首页> 外文期刊>Journal of Neurochemistry: Offical Journal of the International Society for Neurochemistry >NO-cGMP mediated galanin expression in NGF-deprived or axotomized sensory neurons.
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NO-cGMP mediated galanin expression in NGF-deprived or axotomized sensory neurons.

机译:NO-cGMP介导的NGF缺乏或轴突切除的感觉神经元中甘丙肽的表达。

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Leukaemia inhibitory factor (LIF) and nerve growth factor (NGF) are well characterized regulators of galanin expression. However, LIF knockout mice containing the rat galanin 5' proximal promoter fragment (- 2546 to + 15 bp) driving luciferase responded to axotomy in the same way as control mice. Also, LIF had no effect on reporter gene expression in vitro, neither in the presence or absence of NGF, suggesting that other factors mediate an axotomy response from the galanin promoter. We then addressed the role of nitric oxide (NO) using NGF-deprived rat dorsal root ganglion (DRG) neuron cultures infected with viral vectors containing the above-mentioned construct, and also studied endogenous galanin expression in axotomized DRG in vivo. Blocking endogenous NO in NGF-deprived DRG cultures suppressed galanin promoter activity. Consistent with this, axotomized/NGF-deprived DRG neurons expressed high levels of neuronal NO synthase (nNOS) and galanin. Further, using pharmacological NOS blockers, or adenoviral vectors expressing dominant-negative either for nNOS or soluble guanylate cyclase in vivo and in vitro, we show that the NO-cGMP pathway induces endogenous galanin in DRG neurons. We propose that both LIF and NO, acting at different promoter regions, are important for the up-regulation of galanin, and for DRG neuron survival and regeneration after axotomy.
机译:白血病抑制因子(LIF)和神经生长因子(NGF)是甘丙肽表达的良好调节因子。但是,包含驱动荧光素酶的大鼠甘丙肽5'近端启动子片段(-2546至+ 15 bp)的LIF基因敲除小鼠对轴切的反应与对照小鼠相同。同样,无论是否存在NGF,LIF均不影响报告基因的体外表达,表明其他因素介导了甘丙肽启动子的轴突切开反应。然后,我们探讨了使用含有上述构建体的病毒载体感染的NGF剥夺的大鼠背根神经节(DRG)神经元培养物对一氧化氮(NO)的作用,并且还研究了在体内被切除的DRG中内源性甘丙肽的表达。在NGF缺乏的DRG培养物中阻断内源性NO可抑制甘丙肽启动子活性。与此一致的是,轴突切除/ NGF剥夺的DRG神经元表达高水平的神经元一氧化氮合酶(nNOS)和甘丙肽。此外,在体内外使用药理性NOS阻断剂或表达对nNOS或可溶性鸟苷酸环化酶显性阴性的腺病毒载体,我们显示NO-cGMP途径在DRG神经元中诱导内源性甘丙肽。我们建议,LIF和NO,分别作用于不同的启动子区域,对于甘丙肽的上调以及对于轴切术后DRG神经元的存活和再生很重要。

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