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从人肝脏克隆的一种有机阴离子转运多肽的分子和功能特性

Molecular and functional characterization of an organic anion transporting polypeptide cloned from human liver.

作者信息

Kullak-Ublick G A, Hagenbuch B, Stieger B, Schteingart C D, Hofmann A F, Wolkoff A W, Meier P J

机构信息

Department of Medicine, University Hospital, Zürich, Switzerland.

出版信息

Gastroenterology. 1995 Oct;109(4):1274-82. doi: 10.1016/0016-5085(95)90588-x.

Abstract

BACKGROUND & AIMS: Based on a recently cloned rat liver organic anion transporter, we attempted to clone the corresponding human liver organic anion transporting polypeptide.

METHODS

A human liver complementary DNA library was screened with a specific rat liver complementary DNA probe. The human liver transporter was cloned by homology with the rat protein and functionally characterized in Xenopus laevis oocytes.

RESULTS

The cloned human liver organic anion transporting polypeptide consists of 670 amino acids and shows a 67% amino acid identity with the corresponding rat liver protein. Injection of in vitro transcribed complementary RNA into frog oocytes resulted in the expression of sodium-independent uptake of [35S]bromosulfophthalein (Michaelis constant [Km], approximately 20 mumol/L), [3H]cholate (Km, approximately 93 mumol/L), [3H]taurocholate (Km, approximately 60 mumol/L), [14C]glycocholate, [3H]taurochenodeoxycholate, and [3H]tauroursodeoxycholate (Km, approximately 19 mumol/L). Northern blot analysis showed cross-reactivity with messenger RNA species from human liver, brain, lung, kidney, and testes. Polymerase chain reaction analysis of genomic DNA from a panel of human-rodent somatic cell hybrids mapped the cloned human organic anion transporter to chromosome 12.

CONCLUSIONS

These studies show that the cloned human liver organic anion transporter is closely related to, but probably not identical to, the previously cloned rat liver transporter. Furthermore, its additional localization in a variety of extrahepatic tissues suggests that it plays a fundamental role in overall transepithelial organic anion transport of the human body.

摘要

背景与目的

基于最近克隆的大鼠肝脏有机阴离子转运体,我们试图克隆相应的人类肝脏有机阴离子转运多肽。

方法

用特异性大鼠肝脏互补DNA探针筛选人类肝脏互补DNA文库。通过与大鼠蛋白的同源性克隆人类肝脏转运体,并在非洲爪蟾卵母细胞中对其进行功能特性分析。

结果

克隆的人类肝脏有机阴离子转运多肽由670个氨基酸组成,与相应的大鼠肝脏蛋白有67%的氨基酸同一性。将体外转录的互补RNA注射到蛙卵母细胞中,导致[35S]溴磺酞钠(米氏常数[Km],约20μmol/L)、[3H]胆酸盐(Km,约93μmol/L)、[3H]牛磺胆酸盐(Km,约60μmol/L)、[14C]甘氨胆酸盐、[3H]牛磺鹅去氧胆酸盐和[3H]牛磺熊去氧胆酸盐(Km,约19μmol/L)的非钠依赖性摄取表达。Northern印迹分析显示与来自人类肝脏、脑、肺、肾和睾丸的信使RNA物种有交叉反应。对一组人-啮齿动物体细胞杂种的基因组DNA进行聚合酶链反应分析,将克隆的人类有机阴离子转运体定位到12号染色体。

结论

这些研究表明,克隆的人类肝脏有机阴离子转运体与先前克隆的大鼠肝脏转运体密切相关,但可能并不相同。此外,它在多种肝外组织中的额外定位表明,它在人体整体跨上皮有机阴离子转运中起重要作用。

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