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兔红细胞和子宫中的碳酸酐酶同工酶。

Carbonic anhydrase isoenzymes in the erythrocytes and uterus of the rabbit.

作者信息

McIntosh J E

出版信息

Biochem J. 1970 Nov;120(2):299-310. doi: 10.1042/bj1200299.

Abstract
  1. Two forms of the zinc-containing enzyme carbonic anhydrase (EC 4.2.1.1) were isolated from rabbit erythrocytes and two forms from rabbit uterine tissue (endometrium) in the progestational stage of pregnancy (days 6-8 of gestation). Separation of the isoenzymes was achieved by ion-exchange chromatography, preparative polyacrylamide-gel electrophoresis and isoelectric focusing. A comparison was made of the general properties and kinetic behaviour of the purified isoenzymes. 2. Although indistinguishable in terms of molecular weight and zinc content the isoenzymes were very different as catalysts of the hydration of carbon dioxide. The two erythrocyte isoenzymes, found in almost equal amounts, differed more than 100-fold in specific activity. Of the two isoenzymes prepared from either endometrial or entire uterine homogenates one was kinetically indistinguishable from the erythrocyte high-activity form, whereas the other, also possessing high activity, was found only in the endometrial or uterine tissue. Present evidence suggests that the former isoenzyme originated from residual blood contaminating the tissue homogenates, and that a marked rise in the content of the latter isoenzyme accounts for the increase in rabbit endometrial carbonic anhydrase activity that previously has been observed in early pregnancy. 3. Minor forms of the erythrocyte isoenzymes, having a characteristic quantitative and electrophoretic relationship to one another, were occasionally produced during purification. 4. The actions were investigated of the inhibitors acetazolamide (5-acetamido-3,4-diazole-1-thia-2-sulphonamide), 1,1-dimethylaminonaphthalene-5-sulphonamide and ethoxyzolamide (6-ethoxybenzothiazole-2-sulphonamide) on the hydration of carbon dioxide and the hydrolysis of p-nitrophenyl acetate catalysed by the isoenzymes. 5. The low-activity erythrocyte isoenzyme was superior to the high-activity form as a catalyst of beta-naphthyl acetate hydrolysis.
摘要
  1. 从兔红细胞中分离出两种含锌酶碳酸酐酶(EC 4.2.1.1),并在妊娠的孕激素期(妊娠第6 - 8天)从兔子宫组织(子宫内膜)中分离出两种形式。通过离子交换色谱法、制备性聚丙烯酰胺凝胶电泳和等电聚焦实现同工酶的分离。对纯化的同工酶的一般性质和动力学行为进行了比较。2. 尽管同工酶在分子量和锌含量方面难以区分,但作为二氧化碳水合作用的催化剂却有很大差异。两种红细胞同工酶的含量几乎相等,比活性相差100倍以上。从子宫内膜或整个子宫匀浆中制备的两种同工酶中,一种在动力学上与红细胞高活性形式无法区分,而另一种虽然也具有高活性,但仅存在于子宫内膜或子宫组织中。目前的证据表明,前一种同工酶源自污染组织匀浆的残留血液,而后一种同工酶含量的显著增加解释了先前在妊娠早期观察到的兔子宫内膜碳酸酐酶活性的增加。3. 在纯化过程中偶尔会产生红细胞同工酶的次要形式,它们彼此之间具有特征性的定量和电泳关系。4. 研究了抑制剂乙酰唑胺(5 - 乙酰氨基 - 3,4 - 二唑 - 1 - 硫杂 - 2 - 磺酰胺)、1,1 - 二甲基氨基萘 - 5 - 磺酰胺和乙氧唑胺(6 - 乙氧基苯并噻唑 - 2 - 磺酰胺)对同工酶催化的二氧化碳水合作用和对硝基苯乙酸水解作用的影响。5. 低活性红细胞同工酶作为β - 萘乙酸水解的催化剂优于高活性形式。
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/000d/1179600/3a9484496411/biochemj00666-0086-a.jpg

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