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相对受体表达是异源物质介导的大鼠和人类细胞中CYP3A诱导的一个决定因素。

Relative receptor expression is a determinant in xenobiotic-mediated CYP3A induction in rat and human cells.

作者信息

Swales K, Plant N, Ayrton A, Hood S, Gibson G

机构信息

School of Biomedial and Life Sciences, University of Surrey, Guildford, UK.

出版信息

Xenobiotica. 2003 Jul;33(7):703-16. doi: 10.1080/0049825031000121626.

Abstract
  1. Species differences in xenobiotic-mediated transcriptional activation of CYP3A genes are known to exist. These differences are proposed to be due, in part, to host cell differences. 2. Host cell effects were investigated by trans-species transient transfection of reporter genes containing either the rat CYP3A23 or human CYP3A4 proximal promoters into human HepG2 and rat FaO and H4IIEC3 hepatoma cells. HepG2 and FaO cells supported activation of both CYP3A constructs by xenobiotics in a species-specific manner, whereas H4IIEC3 cells were non-permissive. 3. The mRNA complement of the cell lines was then quantified by semiquantitative RT-PCR for adult CYP3As (CYP3A23, CYP3A4/5), steroid hormone receptors (constitutive androstane receptor, glucocorticoid receptor-alpha, pregnane X receptor) and transcription factors (Hepatic nuclear factor 4alpha, retinoid X receptor). 4. Principal component analysis of absolute receptor levels demonstrated a wide scattering, with no coherent pattern. In contrast, PCA of relative receptor ratios segregated H4IIEC3 cells from all other samples. 5. The observation is confirmed that species differences in response to xenobiotics are a result of host cell environment. In addition, new evidence is provided to support the hypothesis that in addition to individual receptor activation profiles, the relative abundance of steroid hormone receptors that control CYP3A gene expression play an important role in this observed species difference.
摘要
  1. 已知在异生物介导的CYP3A基因转录激活方面存在物种差异。这些差异部分归因于宿主细胞的差异。2. 通过将含有大鼠CYP3A23或人CYP3A4近端启动子的报告基因跨物种瞬时转染到人HepG2细胞、大鼠FaO细胞和H4IIEC3肝癌细胞中,研究宿主细胞的影响。HepG2细胞和FaO细胞以物种特异性方式支持异生物对两种CYP3A构建体的激活,而H4IIEC3细胞则不支持。3. 然后通过半定量RT-PCR对成年CYP3A(CYP3A23、CYP3A4/5)、类固醇激素受体(组成型雄烷受体、糖皮质激素受体-α、孕烷X受体)和转录因子(肝细胞核因子4α、视黄酸X受体)的细胞系mRNA互补物进行定量。4. 对绝对受体水平的主成分分析显示出广泛的离散,没有连贯的模式。相比之下,相对受体比率的主成分分析将H4IIEC3细胞与所有其他样品区分开来。5. 这一观察结果证实,对外源生物的反应中的物种差异是宿主细胞环境的结果。此外,提供了新的证据来支持这一假设,即除了个体受体激活谱外,控制CYP3A基因表达的类固醇激素受体的相对丰度在这种观察到的物种差异中起重要作用。

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