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含硫代氨基酰-脯氨酰肽键的底物对脯氨酸特异性酶的影响。

Influence on proline-specific enzymes of a substrate containing the thioxoaminoacyl-prolyl peptide bond.

作者信息

Schutkowski M, Neubert K, Fischer G

机构信息

Martin-Luther-Universität Halle-Wittenberg, Institut für Biochemie, Fachbereich Biochemie/Biotechnologie, Germany.

出版信息

Eur J Biochem. 1994 Apr 1;221(1):455-61. doi: 10.1111/j.1432-1033.1994.tb18758.x.

DOI:10.1111/j.1432-1033.1994.tb18758.x
PMID:7909521
Abstract

Dipeptidyl peptidase IV from porcine kidney and aminopeptidase P from Escherichia coli can utilize thioxoalanyl-proline 4-nitroanilide but with decreased kinetic constants compared to the normal substrates. Product analysis showed that exclusively thioxoalanyl-proline was liberated in the case of dipeptidyl peptidase IV catalysis and thioxo-alanine in the case of aminopeptidase-P-mediated thioxo peptide bond hydrolysis. For the proline-specific aminopeptidase P the kcat/Km value for the thioxo peptide is 1100-fold lower than for the corresponding oxo peptide. This difference is entirely due to kcat. Because the rotation about the thioxo amide bond is about 12.5 kJ mol-1 more difficult than rotation about an amide bond, these data support a mechanism involving rate-limiting rotation about the scissile peptide bond. It was found that the specificity rate constant for the reaction of thioxoalanyl-proline 4-nitroanilide and dipeptidyl peptidase IV is 100-1000-fold lower compared to the corresponding rate constant for alanyl-proline 4-nitroanilide. This remarkable effect is interpreted in terms of a distorted binding of the transition state for the thioxo substrate. The hydrolysis of the thioxo substrate by dipeptidyl peptidase IV is isomer-specific. The conformation about the nonscissile P2-P1 thioxo amide bond has to be in trans for successful cleavage of the scissile peptide bond. We can now directly compare the rotational energy barrier of the prolyl peptide bond for the oxo and the thioxo form.

摘要

猪肾二肽基肽酶IV和大肠杆菌氨肽酶P可以利用硫代丙氨酰 - 脯氨酸4 - 硝基苯胺,但与正常底物相比,动力学常数降低。产物分析表明,在二肽基肽酶IV催化的情况下,仅释放出硫代丙氨酰 - 脯氨酸,而在氨肽酶P介导的硫代肽键水解的情况下,释放出硫代丙氨酸。对于脯氨酸特异性氨肽酶P,硫代肽的kcat/Km值比相应的氧代肽低1100倍。这种差异完全是由于kcat。由于围绕硫代酰胺键的旋转比围绕酰胺键的旋转困难约12.5 kJ mol-1,这些数据支持一种涉及限速围绕可裂解肽键旋转的机制。发现硫代丙氨酰 - 脯氨酸4 - 硝基苯胺与二肽基肽酶IV反应的特异性速率常数比丙氨酰 - 脯氨酸4 - 硝基苯胺的相应速率常数低100 - 1000倍。这种显著的效应可以用硫代底物过渡态的扭曲结合来解释。二肽基肽酶IV对硫代底物的水解具有异构体特异性。为了成功裂解可裂解肽键,非可裂解P2 - P1硫代酰胺键的构象必须为反式。我们现在可以直接比较氧代和硫代形式的脯氨酰肽键的旋转能垒。

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