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氧不稳定酶的稳定化原理:应用于一种梭菌氢化酶。

A rationale for stabilization of oxygen-labile enzymes: application to a clostridial hydrogenase.

作者信息

Klibanov A M, Kaplan N O, Kamen M D

出版信息

Proc Natl Acad Sci U S A. 1978 Aug;75(8):3640-3. doi: 10.1073/pnas.75.8.3640.

Abstract

A general procedure for stabilization of O2-labile enzymes exploiting "salting out" of oxygen from the microenvironment in the molecular layers immediately adjacent to charged surfaces of polyionic solid adsorbents has been developed. Empirical verification of this rationale is provided. The half-life of air inactivation of the O2-labile hydrogenase (EC 1.12.7.1) from Clostridium pasteurianum is increased 20- to 25-fold simply by adsorption (noncovalent binding) in dilute Tris.HCl buffer on common anion exchange supports such as DEAE-cellulose or Dowex 1-X2. Predicted increases in degree of stabilization by using more densely charged adsorbents (such as polyethyleneimine-cellulose), as well as bulkier solvent counter-anions, are found; half-lives for air inactivation for the bound hydrogenase can be increased to 3000-fold longer than that of the free enzyme. Most of the total catalytic activity, assayed as H2 evolution from dithionite mediated by methyl viologen or ferredoxin, is retained, whereas the expected suppression of H2 uptake in the reverse reaction is observed.

摘要

已开发出一种利用从紧邻聚离子固体吸附剂带电表面的分子层微环境中“盐析”出氧气来稳定对氧敏感酶的通用方法。提供了这一原理的实验验证。通过在稀Tris.HCl缓冲液中吸附(非共价结合)到常见的阴离子交换载体(如DEAE-纤维素或Dowex 1-X2)上,巴氏梭菌对氧敏感的氢化酶(EC 1.12.7.1)的空气失活半衰期简单地增加了20至25倍。发现使用电荷密度更高的吸附剂(如聚乙烯亚胺-纤维素)以及体积更大的溶剂抗衡阴离子时,预测的稳定化程度会增加;结合的氢化酶的空气失活半衰期可比游离酶的延长至3000倍。以甲基紫精或铁氧化还原蛋白介导的连二亚硫酸盐产生氢气来测定,大部分总催化活性得以保留,而在逆反应中预期的氢气摄取抑制则被观察到。

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