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酿酒酵母中鲨烯-2,3-环氧化酶的表征与部分纯化

Characterization and partial purification of squalene-2,3-oxide cyclase from Saccharomyces cerevisiae.

作者信息

Balliano G, Viola F, Ceruti M, Cattel L

机构信息

Istituto di Chimica Farmaceutica Applicata, Torino, Italy.

出版信息

Arch Biochem Biophys. 1992 Feb 14;293(1):122-9. doi: 10.1016/0003-9861(92)90374-6.

DOI:10.1016/0003-9861(92)90374-6
PMID:1731628
Abstract

The membrane nature of squalene oxide cyclase from Saccharomyces cerevisiae was investigated by comparing properties of the enzyme recovered from both microsomes and the soluble fraction of the yeast homogenate. The "apparent soluble" form and microsomal form of the enzyme were both stimulated by the presence of mammalian soluble cytoplasm and corresponded to one another in response to detergents Triton X-100 and Triton X-114. The observed strong dependence of the enzyme activity on the presence of detergents and the behavior of the enzyme after Triton X-114 phase separation were peculiar to a lipophilic membrane-bound enzyme. A study of the conditions required to extract the enzyme from microsomes confirmed the lipophilic character of the enzyme. Microsomes, exposed to ipotonic conditions to remove peripheral membrane proteins, retained most of the enzyme activity within the integral protein fraction. Quantitative dissociation of the enzyme from membranes occurred only if microsomes were treated with detergents (Triton X-100 or octylglucoside) at concentrations which alter membrane integrity. The squalene oxide cyclase was purified 140 times from yeast microsomes by (a) removal of peripheral proteins, (b) extraction of the enzyme from the integral protein fraction with octylglucoside, and (c) separation of the solubilized proteins by DEAE Bio-Gel A chromatography. Removal of the peripheral proteins seemed to be a key step necessary for obtaining high yields.

摘要

通过比较从微粒体和酵母匀浆可溶性部分回收的酶的特性,研究了酿酒酵母中氧化角鲨烯环化酶的膜性质。该酶的“表观可溶性”形式和微粒体形式均受到哺乳动物可溶性细胞质的刺激,并且在去污剂Triton X-100和Triton X-114作用下表现一致。观察到该酶活性对去污剂的强烈依赖性以及Triton X-114相分离后该酶的行为是亲脂性膜结合酶所特有的。对从微粒体中提取该酶所需条件的研究证实了该酶的亲脂特性。微粒体在等渗条件下处理以去除外周膜蛋白后,大部分酶活性保留在整合蛋白部分。只有当微粒体用改变膜完整性的浓度的去污剂(Triton X-100或辛基葡糖苷)处理时,该酶才会从膜上定量解离。通过(a)去除外周蛋白,(b)用辛基葡糖苷从整合蛋白部分提取该酶,以及(c)通过DEAE Bio-Gel A柱层析分离溶解的蛋白,将氧化角鲨烯环化酶从酵母微粒体中纯化了140倍。去除外周蛋白似乎是获得高产率的关键步骤。

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