Human Bile Salt Export Pump Promoter Is Transactivated by the Farnesoid X Receptor/Bile Acid Receptor

法尼甾体X受体 胆盐出口泵 交易激励 胆汁酸 G蛋白偶联胆汁酸受体 孕烷X受体 核受体 视黄醇X受体 雄激素受体 化学 小异二聚体伴侣 生物 生物化学 突变体 肝细胞核因子4 转录因子 运输机 基因
作者
Meenakshisundaram Ananthanarayanan,Natarajan Balasubramanian,Makoto Makishima,David J. Mangelsdorf,Frederick J. Suchy
出处
期刊:Journal of Biological Chemistry [Elsevier BV]
卷期号:276 (31): 28857-28865 被引量:729
标识
DOI:10.1074/jbc.m011610200
摘要

The bile salt excretory pump (BSEP, ABCb11) is critical for ATP-dependent transport of bile acids across the hepatocyte canalicular membrane and for generation of bile acid-dependent bile secretion. Recent studies have demonstrated that the expression of this transporter is sensitive to the flux of bile acids through the hepatocyte, possibly at the level of transcription of the BSEP gene. To determine the mechanisms underlying the regulation of BSEP by bile acids, the promoter of the BSEP gene was cloned. The sequence of the promoter contained an inverted repeat (IR)-1 element (5′-GGGACA T TGATCCT-3′) at base pairs −63/−50 consisting of two nuclear receptor half-sites organized as an inverted repeat and separated by a single nucleotide. This IR-1 element has been shown in several recent studies to serve as a binding site for the farnesoid X receptor (FXR), a nuclear receptor for bile acids. FXR activity requires heterodimerization with RXRα, and when bound by bile acids, the complex effectively regulates the transcription of several genes involved in bile acid homeostasis. Gel mobility shift assays demonstrated specific binding of FXR/RXRα heterodimers to the IR-1 element in the BSEP promoter. In HepG2 cells, co-transfection of FXR and RXRα is required to attain full transactivation of the BSEP promoter by bile acids. Two FXR transactivation-deficient mutants (an AF-2 deletion and a W469A point mutant) failed to transactivate, indicating that the effect of bile acids is FXR-dependent. Further, mutational analysis confirms that the FXR/RXRα heterodimer activates transcription through the IR-1 site in the human BSEP promoter. These results demonstrate a mechanism by which bile acids transcriptionally regulate the activity of the bile salt excretory pump, a critical component involved in the enterohepatic circulation of bile acids.
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