Human Liver Triiodothyronine Sulfotransferase: Copurification with Phenol Sulfotransferases

Abstract

To ascertain whether triiodothyronine (T₃) sulfotransferase coeluted with the known phenol sulfotransferases (PSTs) during purification, human liver thermostable PST, thermolabile PST, and T₃ sulfotransferase were assayed with p-nitrophenol, dopamine, and T₃, respectively. Thermostable PST eluted from an ion-exchange column in two sequential peaks of activity (Peaks I and II), followed by a peak of thermolabile PST activity. There were three peaks of T₃ sulfotransferase with thermostable PST: two within thermostable PST Peak I, and one peak of T₃ sulfotransferase activity within thermostable PST Peak II. There was a minor peak of T₃ sulfotransferase with thermolabile PST. Further purification of thermostable Peak I showed coelution of T₃ sulfotransferase with thermostable PST during gel filtration and affinity chromatography. SDS-PAGE revealed a major protein band at 31 kDa. Dehydroepiandrosterone sulfotransferase comprised only 4% of the final activity. This report demonstrates coelution of T₃ sulfotransferase with thermostable PST, shows a potential additional isozyme of T₃ sulfotransferase, and points out the apparent minimal role of dehydroepiandrosterone sulfotransferase in T₃ sulfation. The findings support the hypothesis that thermostable PST is the predominant human liver T₃ sulfotransferase activity.