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关于δ5-3-氧代类固醇异构酶的类固醇结合位点数量

On the number of steroid-binding sites of delta 5-3-oxosteroid isomerase.

作者信息

Penning T M, Westbrook E M, Talalay P

出版信息

Eur J Biochem. 1980 Apr;105(3):461-9. doi: 10.1111/j.1432-1033.1980.tb04521.x.

DOI:10.1111/j.1432-1033.1980.tb04521.x
PMID:7371643
Abstract

The number of steroid-binding sites in delta 5-3-oxosteroid isomerase of Pseudomonas testosteroni (EC 5.3.3.1) has been determined from measurements of the red shift of the ultraviolet chromophore of 19-nortestosterone upon binding to the enzyme. The experiments include spectroscopic measurements when limiting concentrations of either 19-nortestosterone or isomerase are titrated with varying concentrations of the complementary ligand. Analysis of the results indicates one binding site per subunit (Mr 13 394). Scatchard plots indicate a single family of equivalent binding sites. 5, 10-Secoestr-5-yne-3, 10, 17-trione is a suicide substrate of isomerase [Batzold & Robinson (1975) J. Am. Chem. Soc. 97, 2576]. The time course for inactivation of isomerase with an excess of 5, 10-seco[7-3H]estr-5-yne-3, 10, 17-trione was parallel to the covalent incorporation of steroid and gave a final stoichiometry of nearly one steroid molecule per subunit of enzyme. Alkylation of [14C] isomerase with excess of this 3H-labeled steroid followed by gel-filtration and dialysis gave an inactivated enzyme with a 3H/14C ratio that corresponds to one molecule of steroid bound per subunit; this stoichiometry was constant over a wide range of protein concentrations (0.1--10 mg/ml). Diffusion of [3H]progesterone into hexagonal crystals of isomerase showed that at saturation one steroid molecule was bound per protomer. Taken together these findings strongly support the conclusion that one molecule of steroid is bound per subunit of isomerase both in solution and in the crystal state.

摘要

已通过测量19-去甲睾酮与睾丸酮假单胞菌(EC 5.3.3.1)的δ5-3-氧代类固醇异构酶结合时紫外发色团的红移,确定了该酶中类固醇结合位点的数量。实验包括在用不同浓度的互补配体滴定19-去甲睾酮或异构酶的极限浓度时进行光谱测量。结果分析表明每个亚基(Mr 13394)有一个结合位点。Scatchard图表明存在一组等效的结合位点。5,10-断雌甾-5-炔-3,10,17-三酮是异构酶的自杀底物[巴佐尔德和罗宾逊(1975年)《美国化学会志》97, 2576]。用过量的5,10-断[7-3H]雌甾-5-炔-3,10,17-三酮使异构酶失活的时间进程与类固醇的共价掺入平行,最终化学计量比接近每个酶亚基一个类固醇分子。用过量的这种3H标记的类固醇对[14C]异构酶进行烷基化,然后进行凝胶过滤和透析,得到一种失活的酶,其3H/14C比值对应于每个亚基结合一个类固醇分子;在很宽的蛋白质浓度范围(0.1-10mg/ml)内,这种化学计量比是恒定的。[3H]孕酮扩散到异构酶的六方晶体中表明,在饱和时每个原体结合一个类固醇分子。这些发现共同有力地支持了这样的结论,即在溶液和晶体状态下,异构酶的每个亚基都结合一个类固醇分子。

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On the number of steroid-binding sites of delta 5-3-oxosteroid isomerase.关于δ5-3-氧代类固醇异构酶的类固醇结合位点数量
Eur J Biochem. 1980 Apr;105(3):461-9. doi: 10.1111/j.1432-1033.1980.tb04521.x.
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引用本文的文献

1
Isolation and sequencing of the gene encoding delta 5-3-ketosteroid isomerase of Pseudomonas testosteroni: overexpression of the protein.睾丸酮假单胞菌δ5-3-酮类固醇异构酶编码基因的分离与测序:该蛋白的过表达
Proc Natl Acad Sci U S A. 1987 Dec;84(24):8893-7. doi: 10.1073/pnas.84.24.8893.