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从雄性兔肝脏胞质溶胶中纯化和鉴定两种胺N-磺基转移酶,AST-RB1(ST3A1)和AST-RB2(ST2A8)。

Purification and characterization of two amine N-sulfotransferases, AST-RB1 (ST3A1) and AST-RB2 (ST2A8), from liver cytosols of male rabbits.

作者信息

Shiraga T, Iwasaki K, Hata T, Yoshinari K, Nagata K, Yamazoe Y, Ohno Y

机构信息

Biopharmaceutical and Pharmacokinetic Research Laboratories, Fujisawa Pharmaceutical Co., Ltd., 1-6, Kashima 2-chome, Yodogawa-ku, Osaka, 532-8514, Japan.

出版信息

Arch Biochem Biophys. 1999 Feb 15;362(2):265-74. doi: 10.1006/abbi.1998.1032.

DOI:10.1006/abbi.1998.1032
PMID:9989935
Abstract

Two sulfotransferases (STs), designated as AST-RB1 (ST3A1) and AST-RB2 (ST2A8), with high a amine N-sulfonating activity, were purified from male rabbit liver cytosols. AST-RB1 and AST-RB2 were purified to homogeneity by the anion-exchange, affinity, and hydroxyapatite chromatography. The N-terminus of both enzymes were blocked. The subunit molecular mass of both enzymes was estimated to be 34 kDa on SDS-PAGE. AST-RB1 efficiently catalyzed N-sulfonation of alicyclic, alkyl, and arylamines such as 4-phenyl-1,2,3, 6-tetrahydropyridine, 1-[(5-chloro-2-oxo-3(2H)-benzothiazolyl)acetyl]-piperazine, desipramine, and aniline, whereas its catalytic activities toward 2-naphthol and dehydroepiandrosterone (DHEA) were very low. On the other hand, AST-RB2 efficiently catalyzed sulfonation of desipramine and DHEA, but had no activity toward 2-naphthol. Amino acid sequences of peptide fragments derived from the purified AST-RB1 showed no significant homology with previously reported STs, but those from the purified AST-RB2 shared a high similarity with those of the ST2 family. Both enzymes were expressed specifically in the liver. The present results strongly suggest that the purified AST-RB1 is a novel enzyme in terms of structure and catalytic properties showing high selectivity for amine substrates, and AST-RB2 is a quite unique from among ST2A enzymes of other species in its substrate specificity.

摘要

从雄性兔肝脏胞质溶胶中纯化出了两种具有高胺N-磺化活性的磺基转移酶(STs),分别命名为AST-RB1(ST3A1)和AST-RB2(ST2A8)。通过阴离子交换、亲和及羟基磷灰石色谱法将AST-RB1和AST-RB2纯化至均一。两种酶的N端均被封闭。在SDS-PAGE上,两种酶的亚基分子量估计均为34 kDa。AST-RB1能高效催化脂环族、烷基和芳基胺的N-磺化反应,如4-苯基-1,2,3,6-四氢吡啶、1-[(5-氯-2-氧代-3(2H)-苯并噻唑基)乙酰基]-哌嗪、地昔帕明和苯胺,而其对2-萘酚和脱氢表雄酮(DHEA)的催化活性非常低。另一方面,AST-RB2能高效催化地昔帕明和DHEA的磺化反应,但对2-萘酚无活性。从纯化的AST-RB1衍生的肽片段的氨基酸序列与先前报道的STs无显著同源性,但从纯化的AST-RB2衍生的肽片段与ST2家族的肽片段具有高度相似性。两种酶均在肝脏中特异性表达。目前的结果有力地表明,纯化的AST-RB1在结构和催化特性方面是一种新型酶,对胺底物具有高选择性,而AST-RB2在底物特异性方面与其他物种的ST2A酶相比非常独特。

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