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雌二醇通过雌激素受体α刺激孤束核中载脂蛋白A-IV基因的表达。

Estradiol stimulates apolipoprotein A-IV gene expression in the nucleus of the solitary tract through estrogen receptor-α.

作者信息

Shen Ling, Liu Yin, Wang David Q H, Tso Patrick, Woods Stephen C, Liu Min

机构信息

Departments of Pathology and Laboratory Medicine (L.S., Y.L., P.T., M.L.) and Psychiatry and Behavioral Neuroscience (S.C.W.), University of Cincinnati College of Medicine, Cincinnati, Ohio 45237-0507; and Department of Internal Medicine (D.Q.H.W.), St Louis University School of Medicine, St Louis, Missouri 63104-1008.

出版信息

Endocrinology. 2014 Oct;155(10):3882-90. doi: 10.1210/en.2014-1239. Epub 2014 Jul 22.

Abstract

Although estrogens have been implicated in the regulation of apolipoprotein A-IV (apo A-IV) gene expression in the nucleus tractus solitarius, previous studies have not defined the molecular mechanism. The aim of this study was to examine the transcriptional mechanisms involved in regulation of apo A-IV gene expression. Using cultured primary neuronal cells from rat embryonic brainstems, we found that treatment with 10nM 17β-estradiol-3-benzoate (E2) or 4,4',4″-(4-propyl-[1H]-pyrazole-1,3,5-triyl) trisphenol (an estrogen receptor [ER]α agonist), but not 2,3-bis(4-hydroxyphenyl)-propionitrile (an ERβ agonist), significantly increased apo A-IV gene expression, compared with vehicle treatment. This effect of E2 was abolished when the cells were incubated with E2 linked to BSA, which prevents E2 from entering cells, implying that a nongenomic mechanism of E2 is not involved. Two putative estrogen response elements were identified at the 5'-upstream region of the apo A-IV gene promoter, but only 1 of them was able to recruit ERα, leading to increased apo A-IV gene expression, as determined by chromatin immunoprecipitation assay and luciferase activity analysis. A cyclic regimen of E2 or 4,4',4″-(4-propyl-[1H]-pyrazole-1,3,5-triyl) trisphenol treatment for 8 cycles (4 d/cycle, mimicking the ovarian cycle of female rats) in ovariectomized female rats significantly reduced food intake and body weight gain and increased apo A-IV gene expression in the nucleus tractus solitarius, relative to vehicle. These data collectively demonstrate that nuclear ERα is the primary mediator of E2's action on apo A-IV gene expression and suggest that increased signaling of endogenous apo A-IV may at least partially mediate E2-induced inhibitory effect on feeding.

摘要

尽管雌激素被认为参与孤束核中载脂蛋白A-IV(apo A-IV)基因表达的调控,但以往研究尚未明确其分子机制。本研究旨在探讨参与apo A-IV基因表达调控的转录机制。使用来自大鼠胚胎脑干的原代培养神经元细胞,我们发现用10nM 17β-雌二醇-3-苯甲酸酯(E2)或4,4',4″-(4-丙基-[1H]-吡唑-1,3,5-三基)三苯酚(一种雌激素受体[ER]α激动剂)处理,而非2,3-双(4-羟基苯基)-丙腈(一种ERβ激动剂),与溶剂处理相比,显著增加了apo A-IV基因表达。当细胞与与牛血清白蛋白结合的E2孵育时,E2的这种作用被消除,这阻止了E2进入细胞,这意味着E2的非基因组机制不参与其中。在apo A-IV基因启动子的5'-上游区域鉴定出两个假定的雌激素反应元件,但通过染色质免疫沉淀分析和荧光素酶活性分析确定,其中只有1个能够募集ERα,导致apo A-IV基因表达增加。在去卵巢雌性大鼠中,用E2或4,4',4″-(4-丙基-[1H]-吡唑-1,3,5-三基)三苯酚进行8个周期(4天/周期,模拟雌性大鼠的卵巢周期)的循环处理,相对于溶剂,显著降低了食物摄入量和体重增加,并增加了孤束核中apo A-IV基因的表达。这些数据共同表明,核ERα是E2对apo A-IV基因表达作用的主要介导因子,并表明内源性apo A-IV信号增加可能至少部分介导E2诱导的对进食的抑制作用。

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