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首页> 外文期刊>Journal of Electrophoresis >Production of dye-binding esterase reactor after separation and detection using combined native isoelectric focusing and blue native electrophoresis
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Production of dye-binding esterase reactor after separation and detection using combined native isoelectric focusing and blue native electrophoresis

机译:使用组合的天然等电聚焦和蓝色天然电泳分离和检测后染料结合酯酶反应器的生产

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When cytosolic proteins from mouse liver were separated by a combined method of native isoelectric focusing (IEF) and blue native electrophoresis, spots at p I 6.7/180,000 Da, p I 6.5/100,000 Da and p I 6.4/70,000 Da were detected by Coomassie Brilliant Blue. After separation and detection, the native enzymes were extracted by native electrophoresis and immobilized on the reverse-phase chromatography media ZipTip to produce an enzyme reactor. The hydrolysis activity of 4-methylumebelliferyl acetate by the spots at p I 6.7/180,000 Da and p I 6.4/70,000 Da was 3.0 and 2.4 times, respectively, greater than that with no enzyme. The method can be applied to systematically produce biological reactors after separation and detection of enzymes by the combined method of native IEF and blue native electrophoresis.
机译:当通过天然等电聚焦(IEF)和蓝色天然电泳的组合方法分离来自小鼠肝脏的细胞溶质蛋白,P i 6.7 / 180,000da,p i 6.5 / 100,000da和p i 6.4 / 70,000da的斑点被Coomassie检测到辉煌的蓝色。分离和检测后,通过天然电泳提取天然酶并固定在反相色谱介质Ziptip上以产生酶反应器。通过P i 6.7 / 180,000da和P i 6.4 / 70,000da的斑点的4-甲基清肿的水解活性分别比没有酶的3.0和2.4倍。该方法可以应用于分离和检测酶后系统地产生生物反应器,并通过天然IEF和蓝色天然电泳的组合方法进行酶。

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