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通过亲和色谱法纯化葡糖神经酰胺酶。

Purification of glucosylceramidase by affinity chromatography.

作者信息

Strasberg P M, Lowden J A, Mahuran D

出版信息

Can J Biochem. 1982 Nov;60(11):1025-31. doi: 10.1139/o82-132.

Abstract

Glucosylceramide: beta-glucosidase (glucocerebrosidase, EC 3.2.1.45) has been purified 12 900-fold from human placenta using a specific affinity column. The ligand, glucosyl sphingosine, prepared from glucocerebroside by alkaline hydrolysis, was attached to epoxy-activated Sepharose 6B. The enzyme was applied to the column in citrate--butanol or citrate--ethylene glycol solution at its pH optimum (5.6). No enzyme was bound in the presence of detergent. Glucocerebrosidase was eluted with citrate--taurocholate buffer at low pH or with citrate--taurocholate buffer containing D-gluconolactone at the pH optimum. Citrate--taurocholate solution alone at the pH optimum would not elute the enzyme. The enzyme hydrolyzed both the natural substrate, glucocerebroside, and the artificial substrate, 4-methylumbelliferyl glucopyranoside. Glucocerebrosidase migrated as a single band on 10% sodium dodecyl sulfate--polyacrylamide tube and (or) slab gels, corresponding to a molecular weight of 75 000. It also ran as a single zone of enzyme activity or protein on native gels, composed of 2.2% polyacrylamide--0.4% agarose containing sodium taurocholate. This is the first reported use of this gel system for the examination of glucocerebrosidase. Overall recovery is 30%. The procedure represents a more rapid and specific technique for purification of glucocerebrosidase than those previously reported.

摘要

葡萄糖神经酰胺

β-葡萄糖苷酶(葡糖脑苷脂酶,EC 3.2.1.45)已通过特定亲和柱从人胎盘中纯化了12900倍。配体葡萄糖基鞘氨醇由葡糖脑苷脂经碱性水解制备,连接到环氧活化的琼脂糖凝胶6B上。酶在其最适pH(5.6)下以柠檬酸盐 - 丁醇或柠檬酸盐 - 乙二醇溶液上样到柱中。在洗涤剂存在下没有酶结合。葡糖脑苷脂酶在低pH下用柠檬酸盐 - 牛磺胆酸盐缓冲液洗脱,或在最适pH下用含有D-葡糖酸内酯的柠檬酸盐 - 牛磺胆酸盐缓冲液洗脱。单独的最适pH的柠檬酸盐 - 牛磺胆酸盐溶液不能洗脱该酶。该酶能水解天然底物葡糖脑苷脂和人工底物4-甲基伞形酮基吡喃葡萄糖苷。葡糖脑苷脂酶在10%十二烷基硫酸钠 - 聚丙烯酰胺管形和(或)平板凝胶上迁移为单一条带,对应分子量为75000。在由含牛磺胆酸钠的2.2%聚丙烯酰胺 - 0.4%琼脂糖组成的天然凝胶上,它也以单一酶活性或蛋白质区带形式迁移。这是首次报道使用这种凝胶系统检测葡糖脑苷脂酶。总回收率为30%。该方法代表了一种比先前报道的方法更快速、更特异的葡糖脑苷脂酶纯化技术。

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