AMP-activated protein kinase activation reduces the transcriptional activity of the murine luteinizing hormone β-subunit gene

R. Moriyama, Koichi Iwamoto, Teruki Hagiwara, S. Yoshida, T. Kato, Y. Kato
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引用次数: 2

Abstract

Malnutrition is one of the factors that induces reproductive disorders. However, the underlying biological processes are unclear. AMP-activated protein kinase (AMPK) is an enzyme that plays crucial role as a cellular energy sensor. In the present study, we examined the effects of AMPK activation on the transcription of the murine gonadotropin subunit genes Cga, Lhb, and Fshb, and the gonadotropin-releasing hormone receptor Gnrh-r. Real-time PCR and transcription assay using LβT2 cells demonstrated that 5-amino-imidazole carboxamide riboside (AICAR), a cell-permeable AMP analog, repressed the expression of Lhb. Next, we examined deletion mutants of the upstream region of Lhb and found that the upstream regulatory region of Lhb (–2527 to –2198 b) was responsible for the repression by AICAR. Furthermore, putative transcription factors (SP1, STAT5a, and TEF) that might mediate transcriptional control of the Lhb repression induced by AICAR were identified. In addition, it was confirmed that both AICAR and a competitive inhibitor of glucose metabolism, 2-deoxy-D-glucose, induced AMPK phosphorylation in LβT2 cells. Therefore, the upstream region of Lhb is one of the target sites for glucoprivation inducing AMPK activation. In addition, AMPK plays a role in repressing Lhb expression through the distal –2527 to –2198 b region.
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amp激活的蛋白激酶激活降低了小鼠黄体生成素β-亚基基因的转录活性
营养不良是引起生殖障碍的因素之一。然而,潜在的生物学过程尚不清楚。amp活化蛋白激酶(AMPK)是一种作为细胞能量传感器起重要作用的酶。在本研究中,我们检测了AMPK激活对小鼠促性腺激素亚基基因Cga、Lhb和Fshb以及促性腺激素释放激素受体Gnrh-r转录的影响。利用LβT2细胞进行的实时PCR和转录实验表明,5-氨基咪唑羧酰胺核苷(AICAR),一种可渗透细胞的AMP类似物,抑制了Lhb的表达。接下来,我们检查了Lhb上游区域的缺失突变体,发现Lhb的上游调控区域(-2527至- 2198b)负责AICAR的抑制。此外,还鉴定了可能介导AICAR诱导的Lhb抑制的转录控制的转录因子(SP1、STAT5a和TEF)。此外,AICAR和竞争性葡萄糖代谢抑制剂2-脱氧-d -葡萄糖(2-deoxy-D-glucose)均可诱导LβT2细胞AMPK磷酸化。因此,Lhb上游区域是葡萄糖活化诱导AMPK活化的靶点之一。此外,AMPK通过远端-2527 ~ - 2198b区抑制Lhb的表达。
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