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地塞米松处理的绵羊肝脏和肠黏膜中细胞色素P450 3A的表达及功能

Cytochrome P450 3A expression and function in liver and intestinal mucosa from dexamethasone-treated sheep.

作者信息

Maté M L, Lifschitz A, Sallovitz J, Ballent M, Muscher A S, Wilkens M R, Schröder B, Lanusse C, Virkel G

机构信息

Laboratory of Veterinary Pharmacology, Faculty of Veterinary Sciences, UNCPBA, Tandil, Argentina.

出版信息

J Vet Pharmacol Ther. 2012 Aug;35(4):319-28. doi: 10.1111/j.1365-2885.2011.01334.x. Epub 2011 Sep 12.

Abstract

The effects of repeated administrations of dexamethasone (DEX) (3 mg/kg/day by i.m. route for 7 days) on the gene expression profile of a cytochrome P450 (CYP) 3A28-like isoenzyme, on the expression of a CYP3A-immunoreactive protein and on CYP3A-dependent metabolic activities in sheep liver and small intestinal mucosa were evaluated in the current work. CYP 3A-dependent metabolic activities (erythromycin and triacetyl-oleandomycin N-demethylations) were assessed in microsomal fractions. The mRNA expression of CYP3A28-like, glucocorticoid receptor, constitutive androstane receptor, pregnane X receptor and retinoic X receptor alpha (RXRα) was determined by quantitative real-time PCR. The expression of a CYP3A-immunoreactive protein was measured by Western blot analyses. In the liver, DEX treatment increased CYP3A28-like mRNA levels (2.67-fold, P<0.01) and CYP3A apoprotein expression (1.34-fold, P<0.05) and stimulated CYP3A-dependent metabolism. High and significant correlation coefficients between CYP3A-dependent activities and CYP3A28-like gene (r=0.835-0.856, P<0.01) or protein (r=0.728-0.855, P<0.05) expression profiles were observed. Among the transcriptional factors, DEX only stimulated (2.1-fold, P<0.01) the mRNA expression of RXRα. In sheep small intestine, DEX caused a slight increment (34.6%, P<0.05) in erythromycin N-demethylase activity in the jejunal mucosa and a significant enhancement (P<0.05) of CYP3A apoprotein level in the duodenal mucosa.

摘要

在当前研究中,评估了反复给予地塞米松(DEX)(通过肌肉注射途径,3mg/kg/天,持续7天)对绵羊肝脏和小肠黏膜中细胞色素P450(CYP)3A28样同工酶的基因表达谱、CYP3A免疫反应性蛋白的表达以及CYP3A依赖性代谢活性的影响。在微粒体组分中评估了CYP 3A依赖性代谢活性(红霉素和三乙酰竹桃霉素N-去甲基化)。通过定量实时PCR测定CYP3A28样、糖皮质激素受体、组成型雄烷受体、孕烷X受体和视黄酸X受体α(RXRα)的mRNA表达。通过蛋白质免疫印迹分析测量CYP3A免疫反应性蛋白的表达。在肝脏中,DEX处理增加了CYP3A28样mRNA水平(2.67倍,P<0.01)和CYP3A载脂蛋白表达(1.34倍,P<0.05),并刺激了CYP3A依赖性代谢。观察到CYP3A依赖性活性与CYP3A28样基因(r=0.835-0.856,P<0.01)或蛋白质(r=0.728-0.855,P<0.05)表达谱之间存在高度显著的相关系数。在转录因子中,DEX仅刺激了RXRα的mRNA表达(2.1倍,P<0.01)。在绵羊小肠中,DEX导致空肠黏膜中红霉素N-去甲基酶活性略有增加(34.6%,P<0.05),十二指肠黏膜中CYP3A载脂蛋白水平显著提高(P<0.05)。

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