Purification of a Rat Liver Phenol Sulphotransferase (P-ST_G) with the Aid of Guanidine Hydrochloride Treatment
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概要
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An isoenzyme of phenol sulphotransferase, designated P-ST_G, was purified 157-fold from male rat liver cytosol by diethylaminoethyl-cellulose (DEAE-cellulose) and agarose-hexane-adenosine-3'-5'-bisphosphate affinity chromatography. The P-ST_G fraction obtained after DEAE-cellulose chromatrography rapidly lost its activity during storage at 4℃, however, the activity was recovered by the addition of 1.6M guanidine hydrochloride (Gndn HCl) followed by dialysis. Gndn HCl also substantially improved the yield of P-ST_G in a subsequent purification step using affinity chromatography, while the specific activity of the purified P-ST_G was not changed by Gndn HCl treatment. It is possible that the Gndn HCl treatment caused P-ST_G recovery from an inactivated to an active form rather than reactivating it for increased activity. Purified P-ST_G is a homodimer with a native molecular mass of 67kDa; the subunit molecular mass is 35kDa. Immunoblot analysis carried out with antibodies raised against the purified enzyme indicated that male rat liver contains a higher level of the enzyme than female rat liver. This enzyme is also expressed in the kidney and the atomach. P-ST_G reaches maximum activity when 1-naphthol, 2-naphthol and 4-nitrophenol are used as substrates at pH 5.5. Using dopamine as a substrate the pH optimum is about 9.0. P-ST_G activity is markedly inhibited by the addition of sodium chloride to the reaction mixture.
- 公益社団法人日本薬学会の論文
- 1991-12-25
著者
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松井 道夫
共立薬科大学
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松井 道夫
Kyoritsu College of Pharmacy
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本間 浩
東大薬
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本間 浩
Kyoritsu College of Pharmacy
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鎌倉 稔
Kyoritsu College of Pharmacy
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中込 泉
Kyoritsu College of Pharmacy
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