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牛血管紧张素转换酶的纯化及底物特异性

Purification and substrate specificity of bovine angiotensin-converting enzyme.

作者信息

Rohrbach M S, Williams E B, Rolstad R A

出版信息

J Biol Chem. 1981 Jan 10;256(1):225-30.

PMID:6256346
Abstract

Angiotensin-converting enzyme was solubilized from bovine lung with detergent and purified over 2300-fold to physical homogeneity by a combination of ammonium sulfate fractionation, molecular sieve chromatography, and ion exchange chromatography. The purified enzyme had an apparent molecular weight of 126,000 in both the denatured, and reduced, denatured forms as determined by sodium dodecyl sulfate polyacrylamide gel electrophoresis. The purified enzyme had a specific activity of 13.6 units/mg. It was inhibited by EDTA and activated by chloride ion. Chloride functioned as a nonessential activator by raising the Vmax 4.26-fold and lowering the KM 5.99-fold under saturating conditions. Under these conditions, the Vmax was 1.2 mumol/min/unit and the KM was 1.3 mM. Three series of peptides having the general structures, Hip-His-X, Hip-X-Leu, and Hip-X-His-Leu were synthesized and used to examine the binding specificity and substrate specificity of the enzyme for amino acids in the COOH-terminal (P'2), penultimate COOH-terminal (P'1), and antepenultimate COOH terminal (P1) peptide positions. These studies indicated that in terms of binding specificity, the relative importance of these three positions was P'2 > P'1 > P1, while the reverse order P1 > P'1 > P'2 was observed for the relative contribution to substrate specificity. Three peptides, Hip-His-D-Leu, Hip-D-His-Leu, and Hip-D-Phe-His-Leu, were also synthesized and used to examine the stereochemical requirements of the enzyme in terms of both peptide binding and hydrolysis. Hydrolysis was found to require an L amino acid in all three positions. In contrast, all three peptides bound to the enzyme.

摘要

用去污剂从牛肺中溶解出血管紧张素转换酶,并通过硫酸铵分级分离、分子筛色谱和离子交换色谱相结合的方法将其纯化至物理纯,纯化倍数超过2300倍。通过十二烷基硫酸钠聚丙烯酰胺凝胶电泳测定,纯化后的酶在变性和还原变性形式下的表观分子量均为126,000。纯化后的酶比活性为13.6单位/毫克。它被乙二胺四乙酸(EDTA)抑制,并被氯离子激活。在饱和条件下,氯离子作为非必需激活剂,使最大反应速度(Vmax)提高4.26倍,米氏常数(KM)降低5.99倍。在这些条件下,Vmax为1.2微摩尔/分钟/单位,KM为1.3毫摩尔。合成了具有一般结构Hip-His-X、Hip-X-Leu和Hip-X-His-Leu的三个系列肽,用于研究该酶对COOH末端(P'2)、倒数第二个COOH末端(P'1)和倒数第三个COOH末端(P1)肽位置氨基酸的结合特异性和底物特异性。这些研究表明,就结合特异性而言,这三个位置的相对重要性为P'2 > P'1 > P1,而对底物特异性的相对贡献则观察到相反的顺序P1 > P'1 > P'2。还合成了三个肽Hip-His-D-Leu、Hip-D-His-Leu和Hip-D-Phe-His-Leu,用于从肽结合和水解两方面研究该酶的立体化学要求。发现水解在所有三个位置都需要L型氨基酸。相比之下,所有这三个肽都能与该酶结合。

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