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从虹鳟红细胞中纯化的一种高活性碳酸酐酶同工酶的特性分析。

Characterization of a high activity carbonic anhydrase isozyme purified from erythrocytes of Salmo gairdneri.

作者信息

Hall G E, Schraer R

出版信息

Comp Biochem Physiol B. 1983;75(1):81-92. doi: 10.1016/0305-0491(83)90043-3.

Abstract
  1. A single, high specific activity carbonic anhydrase (CA) isozyme was present in erythrocytes of the teleostean species Salmo gairdneri (rainbow trout). 2. Purification of trout CA to homogeneity was accomplished using chloroform ethanol extraction, Sephadex G-75 gel filtration, and DEAE Bio-Gel anion exchange chromatography. 3. Trout CA was a zinc metalloenzyme of mol. wt 28,300 and pI9.3. 4. Amino acid analysis indicated the presence of 6 half-cystine residues per enzyme molecule, and the presence of a sulfhydryl reducing agent was required to maintain full activity in vitro. 5. Sulfhydryl modification with both N-ethylmaleimide and acrylonitrile indicated the presence of 3 reactive sulfhydryl groups per CA molecule. Modification of those groups had no direct effect on enzyme activity, but modified CA was no longer subject to inactivation by oxidizing conditions.
摘要
  1. 硬骨鱼虹鳟(Salmo gairdneri)的红细胞中存在一种单一的、高比活性的碳酸酐酶(CA)同工酶。2. 通过氯仿乙醇提取、Sephadex G - 75凝胶过滤和DEAE Bio - Gel阴离子交换色谱法,将鳟鱼CA纯化至同质。3. 鳟鱼CA是一种分子量为28,300且等电点为9.3的锌金属酶。4. 氨基酸分析表明每个酶分子存在6个半胱氨酸残基,并且需要巯基还原剂来在体外维持完全活性。5. 用N - 乙基马来酰亚胺和丙烯腈进行的巯基修饰表明每个CA分子存在3个反应性巯基基团。这些基团的修饰对酶活性没有直接影响,但修饰后的CA不再受氧化条件失活的影响。

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Purification and properties of carbonic anhydrase from salmon erythrocytes.
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Carbonic anhydrase inhibitor in trout plasma.
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