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从牛肝线粒体中分离并鉴定三种对异生物质具有活性的不同羧酸:辅酶A连接酶。

Isolation from bovine liver mitochondria and characterization of three distinct carboxylic acid: CoA ligases with activity toward xenobiotics.

作者信息

Vessey D A, Hu J

机构信息

Liver Study Unit, Department of Veterans' Affairs Medical Center, San Francisco, CA 94121, USA.

出版信息

J Biochem Toxicol. 1995 Dec;10(6):329-37. doi: 10.1002/jbt.2570100608.

DOI:10.1002/jbt.2570100608
PMID:8934636
Abstract

A mitochondrial freeze/thaw lysate was fractionated on a DEAE-cellulose column into four distinct acyl-CoA ligase fractions. First to elute was a 50 kDa short-chain ligase that activated only short-chain fatty acids. Next to elute were three ligases that had activity toward both medium-chain fatty acids and xenobiotic carboxylic acids; these were termed xenobiotic/medium-chain ligases (X-ligases) and labeled XL-I, XL-II, and XL-III, respectively, based on order of elution. The molecular weight of X-ligases I, II, and III were ca. 55,000, 55,500 and 53,000, respectively. Form XL-III showed no pH optimum; the rate increased steadily with pH beginning from pH 7.0. XL-I and XL-II showed the same behavior with benzoate as substrate, but with medium-chain fatty acids, both forms had a pH optimum at 8.8. The three X-ligases differed in substrate specificity. XL-I was the predominant nicotinic acid activating form and had the lowest Km for benzoate. Form XL-II was the only form with measurable salicylate activity, although it was extremely low. XL-III was the only 2,4,6,8-decatetraenoic acid activating form and also was the predominant medium-chain fatty acid-activating form. By comparison of substrate specificities, it was concluded that the two previously reported ligase preparations were mixtures of the three forms. When the ligase rates were compared to previously determined N-acyltransferase rates toward benzoyl-CoA and phenylacetyl-CoA, the data showed that ligase activities are 100-fold lower, and thus the ligase is rate limiting for the conjugation of both of these xenobiotics.

摘要

线粒体冻融裂解物在二乙氨基乙基纤维素柱上分离成四个不同的酰基辅酶A连接酶组分。首先洗脱的是一种50 kDa的短链连接酶,它仅能激活短链脂肪酸。接下来洗脱的是三种对中链脂肪酸和外源性羧酸均有活性的连接酶;这些被称为外源性/中链连接酶(X-连接酶),并根据洗脱顺序分别标记为XL-I、XL-II和XL-III。X-连接酶I、II和III的分子量分别约为55,000、55,500和53,000。XL-III没有最适pH值;从pH 7.0开始,反应速率随pH值稳步增加。以苯甲酸盐为底物时,XL-I和XL-II表现出相同的行为,但以中链脂肪酸为底物时,两种形式的最适pH值均为8.8。这三种X-连接酶在底物特异性上有所不同。XL-I是主要的烟酸激活形式,对苯甲酸盐的Km值最低。XL-II是唯一具有可测量水杨酸酯活性的形式,尽管活性极低。XL-III是唯一的2,4,6,8-癸四烯酸激活形式,也是主要的中链脂肪酸激活形式。通过比较底物特异性,得出结论:之前报道的两种连接酶制剂是这三种形式的混合物。当将连接酶的反应速率与先前测定的N-酰基转移酶对苯甲酰辅酶A和苯乙酰辅酶A的反应速率进行比较时,数据表明连接酶活性低100倍,因此连接酶是这两种外源性物质结合的限速因素。

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