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肝脏固醇调节元件结合蛋白-1c表达对再喂养反应的体内启动子分析。

In vivo promoter analysis on refeeding response of hepatic sterol regulatory element-binding protein-1c expression.

作者信息

Takeuchi Yoshinori, Yahagi Naoya, Nakagawa Yoshimi, Matsuzaka Takashi, Shimizu Ritsuko, Sekiya Motohiro, Iizuka Yoko, Ohashi Ken, Gotoda Takanari, Yamamoto Masayuki, Nagai Ryozo, Kadowaki Takashi, Yamada Nobuhiro, Osuga Jun-Ichi, Shimano Hitoshi

机构信息

Department of Internal Medicine, Graduate School of Medicine, University of Tokyo, Tokyo 113-8655, Japan.

出版信息

Biochem Biophys Res Commun. 2007 Nov 16;363(2):329-35. doi: 10.1016/j.bbrc.2007.08.165. Epub 2007 Sep 6.

DOI:10.1016/j.bbrc.2007.08.165
PMID:17880923
Abstract

Sterol regulatory element-binding protein (SREBP)-1c is the master regulator of lipogenic gene expression in liver. The mRNA abundance of SREBP-1c is markedly induced when animals are refed after starvation, although the regulatory mechanism is so far unknown. To investigate the mechanism of refeeding response of SREBP-1c gene expression in vivo, we generated a transgenic mouse model that carries 2.2kb promoter region fused to the luciferase reporter gene. These transgenic mice exhibited refeeding responses of the reporter in liver and adipose tissues with extents essentially identical to those of endogenous SREBP-1c mRNA. The same results were obtained from experiments using adenovirus-mediated SREBP-1c-promoter-luciferase fusion gene transduction to liver. These data demonstrate that the regulation of SREBP-1c gene expression is at the transcription level, and that the 2.2kb 5'-flanking region is sufficient for this regulation. Moreover, when these transgenic or adenovirus-infected mice were placed on insulin-depleted state by streptozotocin treatment, the reporter expression was upregulated as strongly as in control mice, demonstrating that this regulation is not dominated by serum insulin level. These mice are the first models to provide the mechanistic insight into the transcriptional regulation of SREBP-1c gene in vivo.

摘要

固醇调节元件结合蛋白(SREBP)-1c是肝脏中脂肪生成基因表达的主要调节因子。饥饿后再喂食时,SREBP-1c的mRNA丰度会显著升高,但其调控机制至今仍不清楚。为了研究体内SREBP-1c基因表达的再喂食反应机制,我们构建了一个携带与荧光素酶报告基因融合的2.2kb启动子区域的转基因小鼠模型。这些转基因小鼠肝脏和脂肪组织中的报告基因呈现出再喂食反应,其程度与内源性SREBP-1c mRNA基本相同。使用腺病毒介导的SREBP-1c启动子-荧光素酶融合基因转导至肝脏的实验也得到了相同的结果。这些数据表明,SREBP-1c基因表达的调控发生在转录水平,且2.2kb的5'侧翼区域足以实现这种调控。此外,当通过链脲佐菌素处理使这些转基因或腺病毒感染的小鼠处于胰岛素缺乏状态时,报告基因的表达上调程度与对照小鼠一样强烈,这表明这种调控不受血清胰岛素水平的主导。这些小鼠是首个为深入了解体内SREBP-1c基因转录调控机制提供依据的模型。

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