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PURIFICATION OF A RAT-LIVER CYTOSOLIC SULFOTRANSFERASE RESPONSIBLE FOR THE CONJUGATION OF DIGITOXIGENIN
被引:3
|
作者
:
JOHANNES, A
论文数:
0
引用数:
0
h-index:
0
机构:
UNIV HAMBURG,INST LEGAL MED,BUTENFELD 34,W-2000 HAMBURG 54,GERMANY
JOHANNES, A
VONMEYERINCK, L
论文数:
0
引用数:
0
h-index:
0
机构:
UNIV HAMBURG,INST LEGAL MED,BUTENFELD 34,W-2000 HAMBURG 54,GERMANY
VONMEYERINCK, L
SCHMOLDT, A
论文数:
0
引用数:
0
h-index:
0
机构:
UNIV HAMBURG,INST LEGAL MED,BUTENFELD 34,W-2000 HAMBURG 54,GERMANY
SCHMOLDT, A
机构
:
[1]
UNIV HAMBURG,INST LEGAL MED,BUTENFELD 34,W-2000 HAMBURG 54,GERMANY
[2]
UNIV HAMBURG,DEPT PHARMACOL,W-2000 HAMBURG 20,GERMANY
来源
:
BIOCHEMICAL PHARMACOLOGY
|
1990年
/ 39卷
/ 02期
关键词
:
D O I
:
10.1016/0006-2952(90)90029-K
中图分类号
:
R9 [药学];
学科分类号
:
1007 ;
摘要
:
Previous investigations on the digitoxin metabolism hardly considered the role of the sulfate ester conjugation. Therefore, this study examined whether digitoxin (dt-3) or one of its cleavage products might be sulfated in vitro. It was proven that digitoxigenin (dt-0) is by far the best substrate for the cytosolic sulfotransferases (ST). Digitoxigenin-monodigitoxoside (dt-1) and digitoxigenin-bisdigitoxoside (dt-2) are sulfated in trace amounts whereas dt-3 is not sulfated at all. The purification of the responsible enzyme was performed by liquid chromatography on Q-Sepharose and hydroxyapatite. During the purification procedure this enzymatic activity corresponded exactly to that towards dehydroepiandrosterone (DHEA). The 134-fold purified and gel electrophoretically homogeneous enzyme protein (Mi 33,000) showed a Vmax. of 12.5 nmoles dt-0 sulfate/min mg protein and a KM of 37 μmol/L. The purified enzyme conjugated dt-1 and dt-2 in trace amounts only and was inhibited competitively by DHEA. It can be concluded that in the rat a 3β-hydroxy-steroid sulfotransferase is responsible for the sulfation of dt-0. The purified enzyme reacts with dt-1, dt-2 and digoxigenin (dg-0) in traces only, a sulfation of dt-3 is not detectable. © 1989.
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页码:301 / 307
页数:7
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