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来自大肠杆菌的D-丙氨酸氧化酶:参与L-丙氨酸的氧化过程。

D-alanine oxidase from Escherichia coli: participation in the oxidation of L-alanine.

作者信息

Raunio R P, Straus L D, Jenkins W T

出版信息

J Bacteriol. 1973 Aug;115(2):567-73. doi: 10.1128/jb.115.2.567-573.1973.

Abstract

Cell wall-membrane preparations of Escherichia coli, prepared by the ethylenediaminetetraacetic acid-lysozyme method, contain enzymes which catalyze the oxidation of d-alanine and, to a lesser extent, l-alanine into pyruvate and ammonia without the formation of hydrogen peroxide. The kinetic parameters were (i) pH optima of 8.3 to 8.4 for l- and d-alanine and (ii) a K(m) value of 6.6 +/- 0.2 mM for d-alanine. Several coenzymes were without effect when added to the reaction mixture. The participation of d-alanine oxidase in the oxidation of l-alanine was demonstrated. The evidence is based on (i) results of cellular fractionation; (ii) labeling experiments; (iii) inhibition studies with aminooxyacetate and cycloserine; (iv) denaturation experiments; and (v) demonstration of the presence of an active racemase.

摘要

用乙二胺四乙酸-溶菌酶法制备的大肠杆菌细胞壁-细胞膜制剂含有能催化将d-丙氨酸以及少量l-丙氨酸氧化为丙酮酸和氨且不生成过氧化氢的酶。动力学参数为:(i)l-丙氨酸和d-丙氨酸的最适pH值为8.3至8.4;(ii)d-丙氨酸的米氏常数(K(m))值为6.6±0.2 mM。向反应混合物中添加几种辅酶均无效果。证明了d-丙氨酸氧化酶参与l-丙氨酸的氧化。证据基于:(i)细胞分级分离结果;(ii)标记实验;(iii)用氨基氧乙酸和环丝氨酸进行的抑制研究;(iv)变性实验;以及(v)活性消旋酶存在的证明。

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