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猪肠黏膜酰基转移酶I:亚细胞定位、分离、动力学研究及生物学功能

The hog intestinal mucosa acylase I: subcellular localization, isolation, kinetic studies and biological function.

作者信息

Giardina T, Biagini A, Dalle Ore F, Ferre E, Reynier M, Puigserver A

机构信息

Laboratoire de Biochimie et Biologie de la Nutrition, UPRES A 6033, Faculté des Sciences et Techniques Saint-Jérôme, Marseille, France.

出版信息

Biochimie. 1997 May;79(5):265-73. doi: 10.1016/s0300-9084(97)83514-6.

DOI:10.1016/s0300-9084(97)83514-6
PMID:9258435
Abstract

The soluble acylase I (N-acylamino acid amidohydrolase, EC 3.5.1.14) from hog intestinal mucosa was 11,000-fold purified for the first time using a new four-step procedure involving an immunoaffinity chromatography. The resulting protein, which had an isoelectric point of 5.2 and a M(r) of 90,000 was composed of two apparently identical N-acylated polypeptide chains. Its amino acid composition was comparable to that of hog kidney acylase I. The enzyme had a pH optimum at 8.0 and required Zn2+ or Co2+. The optimal temperature for the acylase reaction was 40 degrees C and the activation energy of thermodenaturation was estimated at 260 kJ mol-1. The enzyme was strongly inhibited when preincubated with chelating agents, by diethyl pyrocarbonate under histidine-modifying conditions as well as by sulfhydryl compounds. The reaction of the purified enzyme with the synthetic substrate furylacryloyl-L-methionine was partly characterized as follows: Km = 0.22 +/- 0.03 mM, kcat = 128.0 +/- 17.8 s-1 and kcat/Km = 5.8 +/- 1.6 x 10(5) M-1 s-1. The L-stereoisomer of methionine competitively inhibited the enzyme reaction with a Ki of 3.4 +/- 0.2 mM. It is suggested that acylase I might not only be involved in the catabolism of intracellular N-acylated protein but also be responsible for the biological utilization of N-acylated food proteins.

摘要

首次采用一种新的包含免疫亲和色谱的四步程序,对猪小肠黏膜中的可溶性酰基转移酶I(N-酰基氨基酸酰胺水解酶,EC 3.5.1.14)进行了11000倍的纯化。所得蛋白质的等电点为5.2,相对分子质量为90000,由两条明显相同的N-酰化多肽链组成。其氨基酸组成与猪肾酰基转移酶I的氨基酸组成相当。该酶的最适pH为8.0,需要Zn2+或Co2+。酰基转移酶反应的最适温度为40℃,热变性的活化能估计为260 kJ·mol-1。当与螯合剂预孵育时,该酶受到强烈抑制,在组氨酸修饰条件下被焦碳酸二乙酯以及巯基化合物抑制。纯化后的酶与合成底物呋喃丙烯酰-L-甲硫氨酸的反应部分特征如下:Km = 0.22±0.03 mM,kcat = 128.0±17.8 s-1,kcat/Km = 5.8±1.6×10(5) M-1·s-1。甲硫氨酸的L-立体异构体竞争性抑制酶反应,Ki为3.4±0.2 mM。有人提出,酰基转移酶I可能不仅参与细胞内N-酰化蛋白质的分解代谢,还负责N-酰化食物蛋白质的生物利用。

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