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采用两步高效疏水和凝胶渗透柱色谱法纯化人胎盘葡萄糖脑苷脂酶。

Purification of human placental glucocerebrosidase using a two-step high-performance hydrophobic and gel permeation column chromatography method.

作者信息

Choy F Y

出版信息

Anal Biochem. 1986 Aug 1;156(2):515-20. doi: 10.1016/0003-2697(86)90287-3.

Abstract

Glucocerebrosidase was purified from human placenta approximately 10,600-fold to apparent homogeneity with an overall yield of 37% using cholate extraction, ammonium sulfate fractionation, butanol delipidation, and a two-step high-performance hydrophobic and gel permeation column chromatography method. A Phenyl-5PW (21.5 X 150 mm) column was used in the first step. Approximately one litre of delipidated and dialysed extract containing 3.7 X 10(6) units of enzyme activity from 1 kg of placental tissue was processed by the column at a flow rate of 5 ml/min. Glucocerebrosidase was eluted using a linear cholate gradient (2-3%). There was a 50-fold purification and 89% recovery. The run was completed in about 7 h. In the second step, the concentrated enzyme preparation from the phenyl column was run through two Bio-Sil TSK 250 gel permeation columns (21.5 X 600 mm) connected in series at a flow rate of 1.5 ml/min. A symmetrical peak of glucocerebrosidase activity (Ve = 253 ml) which had constant specific activity (47,000 units/h/mg protein) was noted. There was a 17-fold purification and 80% recovery in this run which was completed in 4 h. Sodium dodecylsulfate-polyacrylamide gel electrophoresis and protein staining with silver compounds of the purified preparation revealed the presence of one band of Mr 68,000.

摘要

采用胆酸盐提取、硫酸铵分级分离、丁醇脱脂以及两步高效疏水和凝胶渗透柱色谱法,从人胎盘中纯化葡萄糖脑苷脂酶,纯化倍数约为10600倍,达到表观均一性,总产率为37%。第一步使用苯基-5PW(21.5×150mm)柱。将约1升来自1千克胎盘组织的含3.7×10⁶单位酶活性的脱脂和透析提取物以5毫升/分钟的流速通过该柱。使用线性胆酸盐梯度(2 - 3%)洗脱葡萄糖脑苷脂酶。纯化倍数为50倍,回收率为89%。该运行约7小时完成。第二步,将苯基柱的浓缩酶制剂以1.5毫升/分钟的流速通过两个串联的Bio - Sil TSK 250凝胶渗透柱(21.5×600mm)。观察到葡萄糖脑苷脂酶活性的对称峰(Ve = 253毫升),其比活性恒定(47000单位/小时/毫克蛋白质)。该运行4小时完成,纯化倍数为17倍,回收率为80%。纯化制剂的十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳和银染蛋白质显示存在一条分子量为68000的条带。

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