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三种特异性焦磷酸水解酶催化的二腺苷多磷酸水解的区域特异性

Regiospecificity of the hydrolysis of diadenosine polyphosphates catalyzed by three specific pyrophosphohydrolases.

作者信息

Guranowski A, Brown P, Ashton P A, Blackburn G M

机构信息

Department of Chemistry, Krebs Institute, University of Sheffield, U.K.

出版信息

Biochemistry. 1994 Jan 11;33(1):235-40. doi: 10.1021/bi00167a031.

DOI:10.1021/bi00167a031
PMID:8286347
Abstract

The different patterns of enzymatic cleavage of diadenosine polyphosphates, ApnAs, where n = 3-5, have been established by fast atom bombardment mass spectrometry, FAB MS, of the nucleotide products formed in the presence of H2(18)O. The three specific pyrophosphohydrolases, Ap3A hydrolase (EC 3.6.1.29) and (asymmetrical) Ap4A hydrolase (EC 3.6.1.17) from lupin and the (symmetrical) Ap4A hydrolase (EC 3.6.1.41) from Escherichia coli, manifest three different regiospecificities. The Ap3A hydrolase cleaves all four substrates tested, Ap3A, Ap4A, ApCH2ppA, and ApCHFppA, to give [18O]AMP and the corresponding unlabeled adenosine nucleotide. In each case, the enzyme cleaves at the phosphate proximate to the bound adenosine moiety. The (asymmetrical) Ap4A hydrolase cleaves both Ap4A and Ap5A to give unlabeled ATP plus [18O]AMP and [18O]ADP, respectively, and is thus seen to add water at the fourth phosphate from the bound adenosine moiety. Lastly, the (symmetrical) Ap4A hydrolase from E. coli gives beta-[18O]ADP from Ap3A, Ap4A, and Ap5A along with the unlabeled nucleotide coproducts. In addition, with Ap4A alpha S (ApspppA) as substrate for the bacterial enzyme, the products are beta-[18O]ADP and unlabeled ADP alpha S. This symmetrical enzyme is thus characterized as cleaving the polyphosphate chain at the second phosphate from the bound adenosine moiety.

摘要

通过对在H₂¹⁸O存在下形成的核苷酸产物进行快原子轰击质谱分析(FAB MS),已确定了二腺苷多磷酸(ApnAs,其中n = 3 - 5)的不同酶促裂解模式。来自羽扇豆的三种特异性焦磷酸水解酶,即Ap3A水解酶(EC 3.6.1.29)和(不对称)Ap4A水解酶(EC 3.6.1.17)以及来自大肠杆菌的(对称)Ap4A水解酶(EC 3.6.1.41),表现出三种不同的区域特异性。Ap3A水解酶可裂解所有四种测试底物,即Ap3A、Ap4A、ApCH₂ppA和ApCHFppA,生成[¹⁸O]AMP和相应的未标记腺苷核苷酸。在每种情况下,该酶都在靠近结合腺苷部分的磷酸处裂解。(不对称)Ap4A水解酶可裂解Ap4A和Ap5A,分别生成未标记的ATP以及[¹⁸O]AMP和[¹⁸O]ADP,因此可以看出它是在距结合腺苷部分的第四个磷酸处加水。最后,大肠杆菌的(对称)Ap4A水解酶可从Ap3A、Ap4A和Ap5A生成β-[¹⁸O]ADP以及未标记的核苷酸副产物。此外,以Ap4AαS(ApspppA)作为细菌酶的底物时,产物为β-[¹⁸O]ADP和未标记的ADPαS。因此,这种对称酶的特征是在距结合腺苷部分的第二个磷酸处裂解多磷酸链。

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