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作 者:刘斯奇[1,2] 卢义钦[1,2] Das BALLABH Satish K.SRIVASTAVA
机构地区:[1]湖南医科大学生化教研室 [2]德克萨斯大学医学院人类生化与遗传学系
出 处:《生命科学研究》1999年第2期118-127,共10页Life Science Research
摘 要:联合采用DEAE-纤维素层析、色谱聚焦、NADP亲和层析与SephadexG-100的凝胶过滤,对人脑醛糖还原酶(EC1.1.1.21;ALR)进行纯化.现测得该酶的等电点pH值为5.85.经聚丙烯酰胺凝胶盘状电泳和Western印迹证实,获得了满意的酶纯度.同葡萄糖,葡糖-6-磷酸与NADPH保温后,人脑ALR纯品的活性与对照酶组相似,且不被糖酵解途径的一些磷酸化中间产物抑制.苯基硼酸琼脂糖柱层析洗脱谱峰和氢硼化钠还原反应提示,当同葡萄糖保温时,人脑ALR(特别是其均一态)可能未被进一步糖基化.在糖尿病并发症和按结构完成药物设计的研究工作中。Aldose reductase(EC1.1.1.21;ALR)from human brain was purified by combination of DEAE cellulose chromatography,chromatofocusing,NADP affinity chromatography and Sephadex G 100 gel filtration.The isoelectric pH for this enzyme was determined to be 5.85.The high purity of the enzyme was confirmed by disc PAGE and Western blotting.The purified human brian ALR after incubation with glucose,glucose 6 phosphate and NADPH was comparable to the control enzyme in activity,and was not inhibited by several phosphorylated intermediates of glycolytic pathway.Phenylboronate agarose column profile and sodium borohydride reduction imply that human brain ALR,especially at the homogenous state,is possibly not further glycosylated during incubation with glucose. Application of purified ALR is important for studying the pathogenesis of diabetic complications and structure based drug design.
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