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受体介导的基因递送方法证明了5'-近端DNA区域在体内赋予大鼠肝脏中CYP2B2基因苯巴比妥反应性方面的作用。

Receptor-mediated gene delivery approach demonstrates the role of 5'-proximal DNA region in conferring phenobarbitone responsiveness to CYP2B2 gene in rat liver in vivo.

作者信息

Mani S A, Harish S, Vathsala P G, Rangarajan P N, Padmanaban G

机构信息

Department of Biochemistry, Indian Institute of Science, Bangalore, 560 012, India.

出版信息

Biochem Biophys Res Commun. 2000 Feb 24;268(3):734-9. doi: 10.1006/bbrc.2000.2203.

Abstract

The phenobarbitone (PB) responsiveness of the 5'-proximal region of the CYP2B1/B2 gene was examined in detail with plasmid DNA constructs containing G-free cassette as reporter, using in vivo targeting of the same DNA constructs into rat liver as galactosylated-polylysine complexes. The contribution of the proximal region (-1 to -179 bp) and the positive element (-69 to -98 bp) identified earlier in this laboratory to PB responsiveness was assessed. The results obtained on PB treatment of rats subjected to receptor-mediated gene delivery to liver were conclusive and dramatic, with the control (saline-treated) rats manifesting very little expression of the reporter, reflecting the in vivo picture of CYP2B1/B2 gene expression. The positive element conferred PB responsiveness to homologous and heterologous promoters. Deletion of the positive element led to elimination of PB response. The entire -179 bp region was significantly more effective in responding to PB treatment than the region up to -98 bp, both containing one copy of the positive element. Thus, the positive element and its flanking sequences in the 5'-proximal region are involved in conferring PB responsiveness to the CYP2B1/B2 gene.

摘要

利用含无G盒作为报告基因的质粒DNA构建体,通过将相同的DNA构建体以半乳糖基化聚赖氨酸复合物的形式体内靶向导入大鼠肝脏,详细研究了CYP2B1/B2基因5'-近端区域对苯巴比妥(PB)的反应性。评估了本实验室先前鉴定的近端区域(-1至-179 bp)和正向元件(-69至-98 bp)对PB反应性的贡献。在经受体介导的基因传递至肝脏的大鼠中进行PB处理所获得的结果确凿且显著,对照(盐水处理)大鼠的报告基因表达极少,反映了CYP2B1/B2基因表达的体内情况。正向元件赋予同源和异源启动子PB反应性。正向元件的缺失导致PB反应的消除。整个-179 bp区域对PB处理的反应明显比直至-98 bp的区域更有效,二者均含有一个正向元件拷贝。因此,5'-近端区域中的正向元件及其侧翼序列参与赋予CYP2B1/B2基因PB反应性。

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