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仓鼠顶体蛋白酶的辐射失活表明,其生物活性单位的分子大小较低。

Radiation inactivation of hamster acrosin reveals that the biologically active unit is of low molecular size.

作者信息

Antaki P, Vigneault N, Beauregard G, Potier M, Roberts K D

机构信息

Department of Biochemistry, University of Montreal, Maisonneuve-Rosemont Hospital Research Center, Quebec, Canada.

出版信息

Biol Reprod. 1987 Aug;37(1):249-56. doi: 10.1095/biolreprod37.1.249.

Abstract

The relationship between structure and activity of acid-extracted and purified acrosin obtained from cauda epididymal hamster spermatozoa was studied. A four-step purification procedure of acrosin was used; it included 1.) acid extraction, 2.) gel filtration over Sephadex G-100 resin, 3.) ion exchange on CM-Sepharose CL-6B, and 4.) affinity chromatography on proflavin-Sepharose 4B. Analysis of the purified enzyme by high-performance liquid chromatography (300 SW + I-125) revealed a molecular weight of 44,000, which was identical to that obtained for acid-extracted acrosin. Slab-gel electrophoresis under nondenaturing conditions showed only one active band, as revealed with a highly sensitive assay using N alpha-benzyloxycarbonyl-L-lysine thiobenzyl ester as substrate. The radiation inactivation size of acid extracted acrosin was calculated to be 8400. This small unit could represent the active polypeptide portion of a larger monomer molecule or could represent the size of active subunits. Because acrosin is autocatalytic and highly active during fertilization, it is suggested that the active portion of the completely processed form of the enzyme is of small molecular weight.

摘要

研究了从附睾尾部仓鼠精子中提取并纯化的酸性顶体蛋白酶的结构与活性之间的关系。采用了一种顶体蛋白酶的四步纯化程序;包括1.) 酸提取,2.) 在Sephadex G - 100树脂上进行凝胶过滤,3.) 在CM - Sepharose CL - 6B上进行离子交换,以及4.) 在黄素 - Sepharose 4B上进行亲和层析。通过高效液相色谱法(300 SW + I - 125)对纯化酶进行分析,结果显示分子量为44,000,这与酸提取的顶体蛋白酶所得到的分子量相同。在非变性条件下进行的平板凝胶电泳仅显示一条活性带,这是使用Nα - 苄氧羰基 - L - 赖氨酸硫代苄酯作为底物的高灵敏度测定所揭示的。计算得出酸提取的顶体蛋白酶的辐射失活大小为8400。这个小单元可能代表较大单体分子的活性多肽部分,或者可能代表活性亚基的大小。由于顶体蛋白酶在受精过程中具有自催化作用且活性很高,因此有人认为该酶完全加工形式的活性部分分子量较小。

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