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牛红细胞中泛素的分离、特性鉴定以及酯酶和二氧化碳水合酶活性

Isolation, characterization, and esterase and CO2 hydration activities of ubiquitin from bovine erythrocytes.

作者信息

Matsumoto H, Taniguchi N, Deutsch H F

出版信息

Arch Biochem Biophys. 1984 Nov 1;234(2):426-33. doi: 10.1016/0003-9861(84)90289-3.

DOI:10.1016/0003-9861(84)90289-3
PMID:6093699
Abstract

Ubiquitin was isolated from bovine erythrocytes by a relatively simple procedure involving extraction with chloroform and ethanol, chromatography on DEAE-cellulose, and gel filtration. Amino acid and partial sequence analyses showed it to be identical to previously isolated material. Ubiquitin released p-nitrophenolate from p-nitrophenyl acetate, but did not cleave other esterase substrates that were tested. It had a turnover number of 116 mmol for p-nitrophenyl acetate at pH 7.7 and 30 degrees C, and this activity was relatively stable to heat treatment. Electrophoretic studies indicated that the ubiquitin was sequentially acetylated by p-nitrophenyl acetate, as judged by the appearance of more anodically migrating components. The reactions of ubiquitin with p-nitrophenyl acetate at pH 7.0 were biphasic and consisted of (a) an initial phase, during which the release of p-nitrophenol resulted from monoacetylation of the ubiquitin and from ubiquitin-catalyzed hydrolysis of the ester; and (b) a second phase, during which the release of p-nitrophenol resulted only from the breakdown and reformation of the acetyl-enzyme complex. Ubiquitin also showed CO2 hydration activity and could be localized following gel electrophoresis by the CO2-bromthymol blue staining method. The strong inhibitor of carbonic anhydrase, acetazolamide, also inhibited the CO2 hydration activity and p-nitrophenyl acetate activity of ubiquitin. An antibody against this protein did not precipitate bovine carbonic anhydrase II. The esterase activity of ubiquitin was much higher than those previously reported for the carbonic anhydrases.

摘要

通过一种相对简单的程序从牛红细胞中分离出泛素,该程序包括用氯仿和乙醇萃取、在DEAE - 纤维素上进行色谱分离以及凝胶过滤。氨基酸和部分序列分析表明它与先前分离的物质相同。泛素能从对硝基苯乙酸中释放出对硝基苯酚盐,但不能裂解所测试的其他酯酶底物。在pH 7.7和30℃下,它对对硝基苯乙酸的转换数为116 mmol,并且该活性对热处理相对稳定。电泳研究表明,根据更多向阳极迁移的组分的出现判断,泛素被对硝基苯乙酸依次乙酰化。泛素与对硝基苯乙酸在pH 7.0下的反应是双相的,包括:(a) 初始阶段,在此期间对硝基苯酚的释放是由于泛素的单乙酰化以及泛素催化的酯水解;(b) 第二阶段,在此期间对硝基苯酚的释放仅源于乙酰酶复合物的分解和重新形成。泛素还表现出二氧化碳水合活性,并且在凝胶电泳后可以通过二氧化碳 - 溴百里酚蓝染色法进行定位。碳酸酐酶的强抑制剂乙酰唑胺也抑制泛素的二氧化碳水合活性和对硝基苯乙酸活性。针对这种蛋白质的抗体不会沉淀牛碳酸酐酶II。泛素的酯酶活性比先前报道的碳酸酐酶的酯酶活性高得多。

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Isolation, characterization, and esterase and CO2 hydration activities of ubiquitin from bovine erythrocytes.牛红细胞中泛素的分离、特性鉴定以及酯酶和二氧化碳水合酶活性
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J Enzyme Inhib Med Chem. 2024 Dec;39(1):2291336. doi: 10.1080/14756366.2023.2291336. Epub 2023 Dec 11.
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