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鸡糖皮质激素和盐皮质激素受体的功能特征。

Functional characterization of chicken glucocorticoid and mineralocorticoid receptors.

机构信息

Department of Animal and Avian Sciences, University of Maryland, College Park, MD 20742, USA.

出版信息

Am J Physiol Regul Integr Comp Physiol. 2010 May;298(5):R1257-68. doi: 10.1152/ajpregu.00805.2009. Epub 2010 Feb 24.

Abstract

Glucocorticoid (GR) and mineralocorticoid (MR) receptors are ligand-activated transcription factors that belong to the nuclear hormone receptor superfamily. Little is known about the function of GR and MR in avian species. Recently, the chicken homologue of the GR (cGR) gene was cloned, and its tissue-specific expression was characterized, whereas the full-length sequence of the chicken MR (cMR) gene remains unknown. Therefore, the aims of this project were to clone the full-length cMR and to functionally characterize both chicken receptors. Cos-7 cells were transiently transfected with cGR or cMR expression vectors along with a glucocorticoid response element-luciferase (GRE-Luc) reporter construct. Transfected cells were then treated with increasing doses of corticosterone (CORT) or aldosterone (ALDO) alone and with GR or MR antagonists (ZK98299 and spironolactone, respectively). Transactivation of cGR or cMR was evaluated by luciferase assay. CORT and ALDO induced cGR- and cMR-driven transcriptional activity in a dose-dependent manner. Each receptor responded to both steroids, but cMR transcriptional activity was induced by lower levels of CORT and ALDO than cGR. Coexpression of both chicken corticosteroid receptors in Cos-7 cells had no synergistic or additive effect on CORT- or ALDO-induced transcriptional activity. Corticosteroid-dependent transactivation of cGR and cMR was partially blocked by antagonists. ZK98299 showed high specificity to cGR, while spironolactone had agonist properties toward both receptors. Immunocytochemistry was used to assess the cellular localization of both receptors. Corticosteroids induced translocation of both receptors into the nucleus. The functional properties of cGR and cMR determined in this study will be helpful in defining the physiological roles of GR and MR in avian species.

摘要

糖皮质激素 (GR) 和盐皮质激素 (MR) 受体是配体激活的转录因子,属于核激素受体超家族。关于 GR 和 MR 在禽类中的功能知之甚少。最近,克隆了鸡 GR(cGR)基因的同源物,并对其组织特异性表达进行了特征描述,而鸡 MR(cMR)基因的全长序列仍不清楚。因此,本项目的目的是克隆全长 cMR 并对两种鸡受体进行功能表征。将 cGR 或 cMR 表达载体与糖皮质激素反应元件-荧光素酶(GRE-Luc)报告构建体瞬时转染 Cos-7 细胞。然后用递增剂量的皮质酮(CORT)或醛固酮(ALDO)单独以及用 GR 或 MR 拮抗剂(ZK98299 和螺内酯)处理转染细胞。通过荧光素酶测定评估 cGR 或 cMR 的转导活性。CORT 和 ALDO 以剂量依赖性方式诱导 cGR 和 cMR 驱动的转录活性。每个受体都对两种类固醇有反应,但 cMR 转录活性被 CORT 和 ALDO 诱导的水平低于 cGR。两种鸡皮质类固醇受体在 Cos-7 细胞中的共表达对 CORT 或 ALDO 诱导的转录活性没有协同或相加作用。糖皮质激素依赖性 cGR 和 cMR 的转导活性部分被拮抗剂阻断。ZK98299 对 cGR 具有高度特异性,而螺内酯对两种受体均具有激动剂特性。免疫细胞化学用于评估两种受体的细胞定位。皮质类固醇诱导两种受体向核内易位。本研究中确定的 cGR 和 cMR 的功能特性将有助于定义 GR 和 MR 在禽类中的生理作用。

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