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Sp1和Sp3激活发动蛋白I基因表达是N1E-115细胞神经元分化所必需的。

Activation of dynamin I gene expression by Sp1 and Sp3 is required for neuronal differentiation of N1E-115 cells.

作者信息

Yoo Jiyun, Jeong Moon-Jin, Kwon Byoung-Mog, Hur Man-Wook, Park Young-Mee, Han Mi Young

机构信息

Cell Biology Laboratory, Korea Research Institute of Bioscience and Biotechnology, Taejon 305-600, Korea.

出版信息

J Biol Chem. 2002 Apr 5;277(14):11904-9. doi: 10.1074/jbc.M111788200. Epub 2002 Jan 23.

DOI:10.1074/jbc.M111788200
PMID:11809758
Abstract

Dynamin I is a key molecule required for the recycling of synaptic vesicles in neurons, and it has been known that dynamin I gene expression is induced during neuronal differentiation. Our previous studies established that neuronal restriction of dynamin I gene expression is controlled by Sp1 and nuclear factor-kappaB-like element-1. Here, using a series of deletion constructs and site-directed mutation, we found that transcription of dynamin I gene during neuronal differentiation of N1E-115 cells is controlled primarily by the Sp1 element located between -13 to -4 bp of the dynamin I promoter. Gel shift analysis demonstrated that in addition to Sp1, Sp3 could interact with this Sp1 element. The requirement for Sp family transcription factors in dynamin I gene expression was confirmed by using mithramycin, an inhibitor of Sp1/Sp3 binding. Mithramycin repressed dynamin I gene expression and resulted in blocking of neuronal differentiation of N1E-115 cells. The localization of the dynamin I protein was also restricted in the peripheral region of the nucleus by the mithramycin treatment. Thus, all of our results suggest that induction of dynamin I gene expression during N1E-115 cell differentiation is modulated by Sp1/Sp3 interactions with the dynamin I promoter, and its expression is important for neuronal differentiation of the N1E-115 cells.

摘要

发动蛋白I是神经元中突触小泡循环所需的关键分子,并且已知发动蛋白I基因表达在神经元分化过程中被诱导。我们之前的研究证实,发动蛋白I基因表达的神经元限制性受Sp1和核因子κB样元件-1控制。在此,我们使用一系列缺失构建体和定点突变,发现N1E-115细胞神经元分化过程中发动蛋白I基因的转录主要受位于发动蛋白I启动子-13至-4 bp之间的Sp1元件控制。凝胶迁移分析表明,除了Sp1外,Sp3也能与该Sp1元件相互作用。通过使用丝裂霉素(一种Sp1/Sp3结合抑制剂)证实了Sp家族转录因子在发动蛋白I基因表达中的必要性。丝裂霉素抑制发动蛋白I基因表达并导致N1E-115细胞神经元分化受阻。经丝裂霉素处理后,发动蛋白I蛋白的定位也被限制在细胞核的周边区域。因此,我们所有的结果表明,N1E-115细胞分化过程中发动蛋白I基因表达的诱导是由Sp1/Sp3与发动蛋白I启动子的相互作用调节的,并且其表达对N1E-115细胞的神经元分化很重要。

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