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肝雌激素反应基因与鳜鱼卵子发生的关系:原代培养肝细胞中的转录诱导和对雌二醇-17β的体外启动子转录激活。

Hepatic estrogen-responsive genes relating to oogenesis in cutthroat trout (Oncorhynchus clarki): The transcriptional induction in primary cultured hepatocytes and the in vitro promoter transactivation in responses to estradiol-17β.

机构信息

Division of Marine Life Science, Faculty of Fisheries Sciences, Hokkaido University, 3-1-1 Minato, Hakodate, Hokkaido 041-8611, Japan.

Institute for East China Sea Research, Organization for Marine Science and Technology, Nagasaki University, 1551-7 Taira, Nagasaki 851-2213, Japan.

出版信息

Gen Comp Endocrinol. 2021 Sep 1;310:113812. doi: 10.1016/j.ygcen.2021.113812. Epub 2021 May 13.

Abstract

Estradiol-17β (E2) regulates transcription of estrogen-responsive genes via estrogen receptors (Esr). In many teleost species, choriogenin (chg), vitellogenin (vtg) and esr genes are transactivated by E2 in the liver. This study aimed i) to compare expression properties of all subtypes of these genes (chg: chgHα, chgHβ, chgL; vtg: vtgAs, vtgC; esr: esr1a, esr1b, esr2a, esr2b) in response to estrogen stimulation, and ii) to confirm how each of four Esr subtypes is involved in the transcriptional regulation of these estrogen-responsive genes in cutthroat trout hepatocytes. In hepatocytes in primary culture, all chg and vtg subtype mRNA levels, and those of esr1a, were increased by E2 treatment (10 M) at 24 and 72 h post initiation (hpi), but esr1b, esr2a and esr2b mRNA levels were not. Treatment of hepatocytes with various concentrations of E2 (10-10 M) induced dose-dependent increases in the levels of all chg and vtg subtype mRNAs at 24 and 72 hpi. At both time points, the lowest dose that induced a significant increase in the expression levels of mRNAs (LOEC) for E2 differed among the genes; LOECs were estimated as 10 M for chgHα at 24 hpi, as 10 M for vtgC at 72 hpi, and as 10 M for other mRNAs at both 24 and 72 hpi. Meanwhile, the levels of esr1a mRNA exhibited a dose-dependent increase at 24 and 72 hpi, but the LOEC shifted from 10 M at 24 hpi to 10 M at 72 hpi because of a decrease in mRNA levels at treatment groups exposed to high concentrations of E2. All Esr subtypes transactivated chg, vtg and esr1a promoters in the presence of E2 in vitro. The activation levels indicated that promoter activity of chgHα ≥ vtgAs > chgHβ > chgL ≥ vtgC ≥ esr1a when mediated by Esr1a, chgHβ > chgHα > chgHL > vtgAs ≥ vtgC ≥ esr1a by Esr1b, chgHβ ≥ chgL > chgHα ≥ vtgAs > vtgC > esr1a by Esr2a, and chgHβ ≥ chgHα ≥ vtgAs > chgL ≥ vtgC > esr1a by Esr2b. Collectively, different Esr subtypes were distinctly different in their ability to transactivate estrogen-responsive target genes, resulting in differential expression of chg, vtg and esr1a genes in the estrogen-exposed hepatocytes.

摘要

雌二醇-17β(E2)通过雌激素受体(Esr)调节雌激素反应基因的转录。在许多鱼类物种中,卵黄蛋白原(chg)、卵黄蛋白(vtg)和 esr 基因在肝脏中被 E2 转激活。本研究旨在:i)比较这些基因(chg:chgHα、chgHβ、chgL;vtg:vtgAs、vtgC;esr:esr1a、esr1b、esr2a、esr2b)所有亚型在雌激素刺激下的表达特性,ii)确认四个 Esr 亚型中的每一个如何参与卵黄蛋白原、卵黄蛋白和 esr1a 这些雌激素反应基因在虹鳟肝细胞中的转录调控。在原代培养的肝细胞中,所有 chg 和 vtg 亚型的 mRNA 水平以及 esr1a 的 mRNA 水平在 24 和 72 小时起始后(hpi)均被 E2 处理(10 μM)所增加,但 esr1b、esr2a 和 esr2b 的 mRNA 水平未增加。用不同浓度的 E2(10-10 M)处理肝细胞在 24 和 72 hpi 时诱导所有 chg 和 vtg 亚型 mRNA 水平的剂量依赖性增加。在这两个时间点,诱导 mRNA 水平显著增加的最低剂量(LOEC)因基因而异;E2 对 chgHα 的 LOEC 在 24 hpi 时估计为 10-10 M,对 vtgC 的 LOEC 在 72 hpi 时估计为 10-10 M,对其他 mRNAs 的 LOEC 在 24 和 72 hpi 时均为 10-10 M。与此同时,esr1a mRNA 的水平在 24 和 72 hpi 时呈剂量依赖性增加,但由于暴露于高浓度 E2 的实验组中 mRNA 水平降低,LOEC 从 24 hpi 时的 10-10 M 转移到 72 hpi 时的 10-10 M。所有 Esr 亚型在体外 E2 存在的情况下均转激活 chg、vtg 和 esr1a 启动子。激活水平表明,当由 Esr1a 介导时,chgHα≥vtgAs>chgHβ>chgL≥vtgC≥esr1a 的启动子活性,当由 Esr1b 介导时,chgHβ>chgHα>chgHL>vtgAs≥vtgC≥esr1a 的启动子活性,当由 Esr2a 介导时,chgHβ>chgL>chgHα≥vtgAs>vtgC≥esr1a 的启动子活性,当由 Esr2b 介导时,chgHβ≥chgHα≥vtgAs>chgL≥vtgC≥esr1a 的启动子活性。总之,不同的 Esr 亚型在转激活雌激素反应靶基因的能力上有明显的差异,导致暴露于雌激素的肝细胞中 chg、vtg 和 esr1a 基因的差异表达。

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