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纯化兔肝酯酶ES-1的底物特异性

Substrate specificity of purified rabbit liver esterase ES-1.

作者信息

Van Lith H A, Haller M, Van Zutphen B F, Beynen A C

机构信息

Department of Laboratory Animal Science, Faculty of Veterinary Medicine, State University, Utrecht, The Netherlands.

出版信息

Eur J Biochem. 1992 Jun 1;206(2):527-35. doi: 10.1111/j.1432-1033.1992.tb16956.x.

DOI:10.1111/j.1432-1033.1992.tb16956.x
PMID:1597192
Abstract
  1. Substrate hydrolysis by two purified rabbit liver esterase-1 allozymes (ES-1A and ES-1B) was compared under conditions differing in substrate, pH and temperature. ES-1A and ES-1B activities had a similar pH and temperature dependency and similar thermal stability profile. 2. There were marked differences in specific activity of ES-1A and ES-1B. ES-1A hydrolysed procaine more rapidly than ES-1B, but was less active towards aspirin. The acetate and propionate esters of p-nitrophenyl were hydrolysed slower by ES-1A than by ES-1B. 3. The effect of substrate concentration on ES-1A activity did not comply with the Michaelis-Menten kinetics, which may be due to so-called substrate activation. 4. At identical substrate concentration, pH and temperature, selected artificial esters were better substrates for ES-1A than selected physiological substrates. Beta-Naphthyloctanoate was found to be a suitable substrate for ES-1A. 1,3-Dioctanoylglycerol was hydrolysed at a rate of only 2% of that of beta-naphthyloctanoate. 5. With methyl, p-nitrophenyl, beta-naphthyl and 4-methylumbelliferyl esters as substrates, ES-1A activity is influenced by length and structure of the acyl moiety. Likewise, ES-1A activity is influenced by the nature of the alkyl moiety of acetate esters. With acetate and methyl esters, branched chains when compared with unbranched chains reduced the esterase activity of ES-1A. Elongation of the acyl moiety up to four or five C atoms gradually raised the velocity of methyl, p-nitrophenyl, and 4-methylumbelliferyl ester hydrolysis by ES-1A. A similar pattern was found for the length of the alkyl moiety of acetate esters. 6. The high degree of similarity between the observed substrate specificity of rabbit ES-1A and that reported earlier for rat ES-10, suggests that these two esterases have a common evolutionary origin.
摘要
  1. 在底物、pH值和温度不同的条件下,比较了两种纯化的兔肝酯酶-1同工酶(ES-1A和ES-1B)对底物的水解作用。ES-1A和ES-1B的活性具有相似的pH值和温度依赖性以及相似的热稳定性曲线。2. ES-1A和ES-1B的比活性存在显著差异。ES-1A比ES-1B更快速地水解普鲁卡因,但对阿司匹林的活性较低。对硝基苯的乙酸酯和丙酸酯被ES-1A水解的速度比被ES-1B水解的速度慢。3. 底物浓度对ES-1A活性的影响不符合米氏动力学,这可能是由于所谓的底物激活。4. 在相同的底物浓度、pH值和温度下,所选的人工酯对ES-1A而言是比所选的生理底物更好的底物。发现β-萘辛酸酯是ES-1A的合适底物。1,3-二辛酰甘油的水解速率仅为β-萘辛酸酯水解速率的2%。5. 以甲基、对硝基苯基、β-萘基和4-甲基伞形酮基酯作为底物时,ES-1A的活性受酰基部分的长度和结构影响。同样,ES-1A的活性受乙酸酯烷基部分的性质影响。对于乙酸酯和甲酯,与直链相比,支链降低了ES-1A的酯酶活性。酰基部分延长至四或五个碳原子逐渐提高了ES-1A对甲基、对硝基苯基和4-甲基伞形酮基酯的水解速度。对于乙酸酯烷基部分的长度也发现了类似的模式。6. 观察到的兔ES-1A底物特异性与先前报道的大鼠ES-10的底物特异性高度相似,这表明这两种酯酶有共同的进化起源。

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