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[从矛头蝮蛇毒液中分离蛋白酶阿曲毒素及其某些特性]

[Isolation and some properties of the proteinase atroxin from the venom of the snake Bothrops atrox].

作者信息

Pantigoso C, Escobar E, Málaga O, Yarlequé A

机构信息

Laboratorio de Biología Molecular, Instituto de Ciencias Biológicas Antonio Raimondi (ICBAR), Universidad Nacional Mayor de San Marcos, Lima, Perú.

出版信息

Acta Cient Venez. 1996;47(1):67-73.

PMID:9334451
Abstract

A proteolytic enzyme from the venom of Bothrops atrox snake was isolated. It was designed as Atroxin, and three chromatography steps were used to purification: ion exchange chromatography on DEAE-Sephadex A-50 equilibrated with 0.05 M Tris HCl buffer, 1 mM CaCl2 pH 7.4, followed by gel filtration on Sephadex G-50 and Sephadex G-100, respectively, using the same buffer. The enzyme was recovered with a 7.4 folds and 11% of yield. It had a high activity on casein being 7.4 optimus pH. A molecular weight was 19.9 Kd calculated by polyacrilamide gel electrophoresis, and head treatment showed that the enzyme preserves its activity in the range of 37-45 degrees C, while it was decrease when the temperature values were higher. On the other hand, 0.133 mumoles of Ca2+ and Mg2+, and Zn2+ ions (0.266 mumoles) were activators, while EDTA (0.20 mumoles) and sodium azide (0.053 mumoles) were inhibitors. The enzymatic activity was not affected by glicerol (1.33 mumoles) and phenyl methyl sulphonyl fluoride (PSMF) (0.16 mumoles). In addition, iodoacetic acid (0.08 mumoles) was slight inhibitor, but 0.16 mumoles of p-tosyl-1-lysine chloromethyl ketone (TLCK) was activator. Biological assays on mice showed that atroxin produced hemorrhagic and necrosis after 24 h of injection, which was increased by 5 mM calcium chloride.

摘要

从矛头蝮蛇毒液中分离出一种蛋白水解酶。它被命名为Atroxin,采用三步色谱法进行纯化:在以0.05 M Tris HCl缓冲液、1 mM氯化钙(pH 7.4)平衡的DEAE - Sephadex A - 50上进行离子交换色谱,随后分别在Sephadex G - 50和Sephadex G - 100上进行凝胶过滤,使用相同的缓冲液。该酶的回收率为7.4倍,产率为11%。它对酪蛋白具有高活性,最适pH为7.4。通过聚丙烯酰胺凝胶电泳计算其分子量为19.9 Kd,热处理表明该酶在37 - 45摄氏度范围内保持其活性,而当温度值更高时活性降低。另一方面,0.133微摩尔的Ca2 +、Mg2 +和Zn2 +离子(0.266微摩尔)是激活剂,而EDTA(0.20微摩尔)和叠氮化钠(0.053微摩尔)是抑制剂。酶活性不受甘油(1.33微摩尔)和苯甲基磺酰氟(PSMF)(0.16微摩尔)的影响。此外,碘乙酸(0.08微摩尔)是轻微抑制剂,但对甲苯磺酰 - 1 - 赖氨酸氯甲基酮(TLCK)(0.16微摩尔)是激活剂。对小鼠的生物测定表明,Atroxin在注射24小时后产生出血和坏死,5 mM氯化钙可增强这种作用。

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