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一种原核尿素羧化酶的酶学特性分析

Enzymatic characterization of a prokaryotic urea carboxylase.

作者信息

Kanamori Takeshi, Kanou Norihisa, Atomi Haruyuki, Imanaka Tadayuki

机构信息

Department of Synthetic Chemistry and Biological Chemistry, Graduate School of Engineering, Kyoto University, Katsura, Nishikyo-ku, Kyoto 615-8510, Japan.

出版信息

J Bacteriol. 2004 May;186(9):2532-9. doi: 10.1128/JB.186.9.2532-2539.2004.

Abstract

We identified the first prokaryotic urea carboxylase (UCA) from a member of the alpha subclass of the class Proteobacteria, Oleomonas sagaranensis. This enzyme (O. sagaranensis Uca) was composed of 1,171 amino acids, and its N-terminal region resembled the biotin carboxylase domains of various biotin-dependent carboxylases. The C-terminal region of the enzyme harbored the Met-Lys-Met motif found in biotin carboxyl carrier proteins. The primary structure of the enzyme was 45% identical to that of the urea carboxylase domain of urea amidolyase from Saccharomyces cerevisiae. O. sagaranensis Uca did not harbor the allophanate hydrolase domain found in the yeast enzyme, but a separate gene with structural similarity was found to be adjacent to the uca gene. Purified recombinant O. sagaranensis Uca displayed ATP-dependent carboxylase activity towards urea (V(max) = 21.2 micro mol mg(-1) min(-1)) but not towards acetyl coenzyme A (acetyl-CoA) and propionyl-CoA, indicating that the gene encoded a bona fide UCA and not an acetyl-CoA or propionyl-CoA carboxylase. The enzyme also exhibited high levels of activity towards acetamide and formamide. Kinetic parameters of the enzyme reaction were determined with ATP, urea, acetamide, and formamide. O. sagaranensis could grow on urea, acetamide, and formamide as sole nitrogen sources; moreover, ATP-dependent urea-degrading activity was found in cells grown with urea but not in cells grown with ammonia. The results suggest that the UCA of this organism may be involved in the assimilation of these compounds as nitrogen sources. Furthermore, orthologues of the O. sagaranensis uca gene were found to be widely distributed among Bacteria. This implies that there are two systems of urea degradation in Bacteria, a pathway catalyzed by the previously described ureases and the UCA-allophanate hydrolase pathway identified in this study.

摘要

我们从变形菌门α亚类成员萨嘎拉油单胞菌(Oleomonas sagaranensis)中鉴定出首个原核尿素羧化酶(UCA)。这种酶(萨嘎拉油单胞菌Uca)由1171个氨基酸组成,其N端区域类似于各种生物素依赖性羧化酶的生物素羧化酶结构域。该酶的C端区域含有生物素羧基载体蛋白中发现的Met-Lys-Met基序。该酶的一级结构与酿酒酵母尿素酰胺酶的尿素羧化酶结构域的一级结构有45%的同一性。萨嘎拉油单胞菌Uca不具有酵母酶中发现的脲基甲酸水解酶结构域,但发现一个结构相似的单独基因与uca基因相邻。纯化的重组萨嘎拉油单胞菌Uca对尿素表现出ATP依赖性羧化酶活性(Vmax = 21.2微摩尔毫克-1分钟-1),但对乙酰辅酶A(乙酰-CoA)和丙酰-CoA无活性,这表明该基因编码的是一种真正的UCA,而不是乙酰-CoA或丙酰-CoA羧化酶。该酶对乙酰胺和甲酰胺也表现出高水平的活性。用ATP、尿素、乙酰胺和甲酰胺测定了酶反应的动力学参数。萨嘎拉油单胞菌能够以尿素、乙酰胺和甲酰胺作为唯一氮源生长;此外,在用尿素培养的细胞中发现了ATP依赖性尿素降解活性,而在用氨培养的细胞中未发现。结果表明,该生物体的UCA可能参与这些化合物作为氮源的同化作用。此外,发现萨嘎拉油单胞菌uca基因的直系同源物在细菌中广泛分布。这意味着细菌中存在两种尿素降解系统,一种是由先前描述的脲酶催化的途径,以及本研究中鉴定的UCA-脲基甲酸水解酶途径。

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