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高尔基驻留 PAP 特异性 3'-磷酸酶偶联硫酸转移酶测定。

Golgi-resident PAP-specific 3'-phosphatase-coupled sulfotransferase assays.

机构信息

R&D Systems, Inc., Minneapolis, MN 55413, United States.

出版信息

Anal Biochem. 2012 Apr 1;423(1):86-92. doi: 10.1016/j.ab.2012.01.003. Epub 2012 Jan 17.

DOI:10.1016/j.ab.2012.01.003
PMID:22289690
Abstract

Sulfotransferases are a large group of enzymes that transfer a sulfonate group from the donor substrate, 3'-phosphoadenosine-5'-phosphosulfate (PAPS)(1), to various acceptor substrates, generating 3'-phosphoadenosine-5'-phosphate (PAP) as a by-product. A universal phosphatase-coupled sulfotransferase assay is described here. In this method, Golgi-resident PAP-specific 3'-phosphatase (gPAPP) is used to couple to a sulfotransferase reaction by releasing the 3'-phosphate from PAP. The released phosphate is then detected using malachite green reagents. The enzyme kinetics of gPAPP have been determined, which allows calculation of the coupling rate, the ratio of product-to-signal conversion, of the coupled reaction. This assay is convenient, as it eliminates the need for radioisotope labeling and substrate-product separation, and is more accurate through removal of product inhibition and correction of the results with the coupling rate. This assay is also highly reproducible, as a linear correlation factor above 0.98 is routinely achievable. Using this method, we measured the Michaelis-Menten constants for recombinant human CHST10 and SULT1C4 with the substrates phenolphthalein glucuronic acid and α-naphthol, respectively. The activities obtained with the method were also validated by performing simultaneous radioisotope assays. Finally, the removal of PAP product inhibition by gPAPP was clearly demonstrated in radioisotope assays.

摘要

磺基转移酶是一大类酶,可将磺酸盐基团从供体底物 3'-磷酸腺苷-5'-磷酸硫酸(PAPS)(1)转移到各种受体底物上,生成 3'-磷酸腺苷-5'-磷酸(PAP)作为副产物。本文描述了一种通用的磷酸酶偶联磺基转移酶测定法。在该方法中,高尔基驻留的 PAP 特异性 3'-磷酸酶(gPAPP)用于通过从 PAP 释放 3'-磷酸来偶联磺基转移酶反应。然后使用孔雀绿试剂检测释放的磷酸盐。已经确定了 gPAPP 的酶动力学,这允许计算偶联反应的耦合速率、产物与信号的比值以及产物抑制的校正。该测定方法方便,因为它不需要放射性同位素标记和底物产物分离,并且通过去除产物抑制和用耦合速率校正结果更准确。该测定方法也具有高度可重复性,通常可实现线性相关系数大于 0.98。使用该方法,我们分别用苯芴酮葡萄糖醛酸和 α-萘酚作为底物测量了重组人 CHST10 和 SULT1C4 的米氏常数。该方法获得的活性也通过同时进行放射性同位素测定得到了验证。最后,通过 gPAPP 清楚地证明了放射性同位素测定中 PAP 产物抑制的消除。

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