Veronese M E, Burgess W, Zhu X, McManus M E
Department of Clinical Pharmacology, Flinders University of South Australia, Adelaide.
Biochem J. 1994 Sep 1;302 ( Pt 2)(Pt 2):497-502. doi: 10.1042/bj3020497.
The present paper describes the functional characterization of two human aryl sulphotransferase (HAST) cDNAs, HAST1 and HAST3, previously isolated by us from liver and brain, respectively [Zhu, Veronese, Sansom, and McManus (1993) Biochem. Biophys. Res. Commun. 192, 671-676; Zhu, Veronese, Bernard, Sansom and McManus (1993) Biochem. Biophys. Res. Commun. 195, 120-127]. These appear to encode the two major forms of phenol sulphotransferase (PST) characterized in a number of human tissue cytosols, these being the phenolsulphating (P-PST) and monoamine-sulphating (M-PST) forms of phenol sulphotransferase. HAST1 and HAST3 cDNAs were functionally expressed in COS-7 cells and kinetically characterized using the model substrates for P-PST and M-PST, p-nitrophenol and dopamine (3,4-dihydroxyphenethylamine) respectively. COS-expressed HAST1 was shown to be enzymatically active in sulphating p-nitrophenol with high affinity (Km 0.6 microM), whereas dopamine was the preferred substrate for HAST3 (Km 9.7 microM). HAST1 could also sulphate dopamine, as could HAST3 sulphate p-nitrophenol, but the Km for these reactions were at least two orders of magnitude greater than for the preferred substrates. COS-expressed HAST1 and HAST3 displayed inhibition profiles with the ST inhibitor 2,6-dichloro-4-nitrophenol (DCNP), identical with human liver cytosolic P-PST and M-PST activities respectively. Thermal-stability studies with the expressed enzymes showed that HAST1 was considerably more thermostable (TS) than HAST3, which is consistent with P-PST being termed the TS PST and M-PST being termed the thermolabile (TL) PST. Western immunoblot analyses of the expressed PST proteins using an antibody generated to a bacterially expressed rat liver aryl/phenol ST showed that HAST1 and HAST3 migrated as single proteins with different electrophoretic mobilities (32 versus 34 kDa). This is consistent with the differences in electrophoretic mobilities observed for P-PST and M-PST in a variety of tissues reported by other workers. This report on the functional characterization of P-PST and M-PST cDNAs provides important information on the structural as well as functional relationships of human PSTs, which sulphate a vast array of exogenous and endogenous compounds.
本文描述了两个人类芳基硫酸转移酶(HAST)cDNA,即HAST1和HAST3的功能特性,它们分别是我们之前从肝脏和大脑中分离得到的[朱、韦罗内塞、桑森和麦克马纳斯(1993年)《生物化学与生物物理学研究通讯》192,671 - 676;朱、韦罗内塞、伯纳德、桑森和麦克马纳斯(1993年)《生物化学与生物物理学研究通讯》195,120 - 127]。这些cDNA似乎编码了在许多人体组织胞质溶胶中所鉴定出的两种主要形式的酚硫酸转移酶(PST),即酚硫酸化(P - PST)形式和单胺硫酸化(M - PST)形式的酚硫酸转移酶。HAST1和HAST3 cDNA在COS - 7细胞中进行了功能表达,并分别使用P - PST和M - PST的模型底物对硝基苯酚和多巴胺(3,4 - 二羟基苯乙胺)进行了动力学特性分析。结果表明,COS细胞表达的HAST1对硫酸化对硝基苯酚具有酶活性,且亲和力较高(Km为0.6微摩尔),而多巴胺是HAST3的首选底物(Km为9.7微摩尔)。HAST1也能硫酸化多巴胺,HAST3也能硫酸化对硝基苯酚,但这些反应的Km值比对首选底物的Km值至少高两个数量级。COS细胞表达的HAST1和HAST3对硫酸转移酶(ST)抑制剂2,6 - 二氯 - 4 - 硝基苯酚(DCNP)的抑制谱,分别与人肝脏胞质溶胶中的P - PST和M - PST活性相同。对表达的酶进行热稳定性研究表明,HAST1比HAST3的热稳定性高得多(TS),这与P - PST被称为热稳定型PST以及M - PST被称为热不稳定型(TL)PST是一致的。使用针对细菌表达的大鼠肝脏芳基/酚硫酸转移酶产生的抗体对表达的PST蛋白进行Western免疫印迹分析表明,HAST1和HAST3以单一蛋白形式迁移,具有不同的电泳迁移率(分别为32 kDa和34 kDa)。这与其他研究人员报道的在多种组织中观察到的P - PST和M - PST的电泳迁移率差异一致。这份关于P - PST和M - PST cDNA功能特性的报告提供了关于人类PSTs的结构以及功能关系的重要信息,PSTs可硫酸化大量的外源性和内源性化合物。
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