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Analysis of enzyme activity regulation by non-denaturing electrophoresis and application of this regulation for enzyme reactor production

机译:非变性电泳对酶活性调节的分析及其在酶反应器生产中的应用

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Abstract Non-denaturing electrophoresis can be used to screen enzymes that self-regulate their activities by using a combination of enzymes and their inhibitors. Furthermore, this technique can be applied to develop enzyme reactors that self-regulate their activities. After separation of proteins from mouse liver cytosol by non-denaturing isoelectric focusing, lactate dehydrogense (LDH) and esterase activities were qualitatively and quantitatively examined using a combination of two-dimensional electrophoresis (2-DE) and non-denaturing stacking gel electrophoresis. Activities of mouse liver-derived LDH and carboxylesterase were reversibly inhibited by oxamate and 6,9-diamino-2-ethoxyacridine (acrinol), respectively, in the stacking gels and recovered when the enzymes migrated towards the separation gels. After separation and immobilization of the enzymes, their activities were inhibited by inhibitors and recovered after inhibitor removal. These results indicate that non-denaturing electrophoresis can be applied to select enzymes that self-regulate their activities and subsequently aid in the development of enzyme reactors that can control the enzyme activities.
机译:摘要非变性电泳可用于筛选通过结合酶及其抑制剂来自我调节酶活性的酶。此外,该技术可用于开发能自我调节其活性的酶反应器。通过非变性等电聚焦从小鼠肝细胞质中分离出蛋白质后,结合二维电泳(2-DE)和非变性堆叠凝胶电泳,定性和定量检查了乳酸脱氢酶(LDH)和酯酶活性。草酸和6,9-二氨基-2-乙氧基ac啶(acrinol)分别可逆性抑制小鼠肝脏衍生的LDH和羧酸酯酶的活性,当酶向分离凝胶迁移时,其活性得以恢复。分离和固定化酶后,它们的活性被抑制剂抑制,并在去除抑制剂后恢复。这些结果表明非变性电泳可用于选择能自我调节其活性并随后有助于开发可控制酶活性的酶反应器的酶。

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