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大鼠肝脏胆汁酸磺基转移酶:催化多肽的鉴定及雌性大鼠中聚合形式的证据。

Rat hepatic bile acid sulfotransferase: identification of the catalytic polypeptide and evidence for polymeric forms in female rats.

作者信息

Collins R H, Lack L, Harman K M, Killenberg P G

出版信息

Hepatology. 1986 Jul-Aug;6(4):579-86. doi: 10.1002/hep.1840060406.

DOI:10.1002/hep.1840060406
PMID:3525366
Abstract

A monoclonal antibody, PK1B, directed against rat liver bile acid sulfotransferase was used for the purification and characterization of the enzyme. Incubation of rat liver supernatant with the antibody followed by immunoprecipitation with Staphylococcus aureus cells demonstrated that PK1B reacted with 90% of the enzymatic activity present in the liver supernatant from female rats and 40 to 50% of the activity in male liver preparations. Immunoadsorption chromatography with PK1B bound to Sepharose isolated active enzyme which was purified greater than 75-fold. Sodium dodecyl sulfate-polyacrylamide gel electrophoretic analysis of this preparation in the presence of 2-mercaptoethanol demonstrated three polypeptides: Mr 29,500; 32,500, and 34,000. Western blot analysis indicated that PK1B recognized an epitope which was found only on the Mr 29,500 polypeptide. Two-dimensional gel electrophoresis associated the enzymatic activity with this Mr 29,500 band. High-pressure liquid chromatographic analysis of immunopurified enzyme defined three distinct, enzymatically active protein populations: I (Mr 400,000 to 170,000); II (Mr 130,000), and III (Mr 43,000). An Mr 29,500 polypeptide was the sole constituent of Peaks I and III and a major constituent of Peak II. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis in the presence and absence of 2-mercaptoethanol indicated that in Peak II, catalytically active Mr 29,500 protein is associated with the other two polypeptides by disulfide bonds. In contrast, Peak I consists of a polymer of Mr 29,500 polypeptide which is independent of disulfide interaction.

摘要

一种针对大鼠肝脏胆汁酸磺基转移酶的单克隆抗体PK1B被用于该酶的纯化和特性鉴定。将大鼠肝脏上清液与该抗体孵育,随后用金黄色葡萄球菌细胞进行免疫沉淀,结果表明PK1B与雌性大鼠肝脏上清液中90%的酶活性发生反应,与雄性肝脏制剂中40%至50%的活性发生反应。用结合到琼脂糖凝胶上的PK1B进行免疫吸附色谱法分离出了活性酶,其纯化倍数超过75倍。在2-巯基乙醇存在的情况下,对该制剂进行十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分析,结果显示有三种多肽:分子量分别为29,500、32,500和34,000。蛋白质印迹分析表明PK1B识别的一个表位仅存在于分子量为29,500的多肽上。二维凝胶电泳将酶活性与这条分子量为29,500的条带联系起来。对免疫纯化酶进行高压液相色谱分析,确定了三个不同的、具有酶活性的蛋白质群体:群体I(分子量400,000至170,000);群体II(分子量130,000)和群体III(分子量43,000)。分子量为29,500的多肽是群体I和群体III的唯一成分,也是群体II的主要成分。在有和没有2-巯基乙醇的情况下进行十二烷基硫酸钠-聚丙烯酰胺凝胶电泳表明,在群体II中,具有催化活性的分子量为29,500的蛋白质通过二硫键与另外两种多肽相连。相比之下,群体I由分子量为29,500的多肽聚合物组成,该聚合物与二硫键相互作用无关。

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Biochem J. 1990 Dec 15;272(3):597-604. doi: 10.1042/bj2720597.