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酿酒酵母对D-天冬酰胺的利用

Utilization of D-asparagine by Saccharomyces cerevisiae.

作者信息

Dunlop P C, Roon R J, Even H L

出版信息

J Bacteriol. 1976 Mar;125(3):999-1004. doi: 10.1128/jb.125.3.999-1004.1976.

Abstract

Yeast strains sigma1278b and Harden and Young, which synthesize only an internal constitutive form of L-asparaginase, do not grow on D-asparagine, as a sole source of nitrogen, and whole cell suspensions of these strains do not hydrolyze D-asparagine. Strains X2180-A2 and D273-10B, which possess an externally active form of asparaginase, are able to grow slowly on D-asparagine, and nitrogen-starved suspensions of these strains exhibit high activity toward the D-isomer. Nitrogen starvation of strain X218O-A2 results in coordinate increase of D- and L-asparaginase activity; the specific activity observed for the D-isomer is approximately 20% greater than that observed for the L-isomer. It was observed, in studies with cell extracts, that hydrolysis of D-asparagine occurred only with extracts from nitrogen-starved cells of strains that synthesize the external form of asparaginase. Furthermore, the activity of the extracts toward the D-isomer was always higher than that observed with the L-isomer. A 400-fold purified preparation of external asparaginase from Saccharomyces cerevisiae X218U-A2 hydrolyzed D-asparagine with an apparent Km of 0.23 mM and a Vmax of 38.7 mumol/min per mg of protein. D-Asparagine was a competitive inhibitor of L-asparagine hydrolysis and the Ki determined for this inhibition was approximately equal to its Km. These data suggest that D-asparagine is a good substrate for the external yeast asparaginase but is a poor substrate for the internal enzyme.

摘要

仅合成L-天冬酰胺酶内部组成型形式的酵母菌株sigma1278b以及哈顿和扬菌株,在以D-天冬酰胺作为唯一氮源时无法生长,并且这些菌株的全细胞悬液不能水解D-天冬酰胺。具有外部活性形式天冬酰胺酶的X2180-A2和D273-10B菌株能够在D-天冬酰胺上缓慢生长,并且这些菌株的氮饥饿悬液对D-异构体表现出高活性。X218O-A2菌株的氮饥饿导致D-和L-天冬酰胺酶活性协同增加;观察到的D-异构体的比活性比L-异构体大约高20%。在对细胞提取物的研究中观察到,仅来自合成外部形式天冬酰胺酶的菌株的氮饥饿细胞的提取物才能水解D-天冬酰胺。此外,提取物对D-异构体的活性总是高于对L-异构体观察到的活性。从酿酒酵母X218U-A2中纯化400倍的外部天冬酰胺酶制剂水解D-天冬酰胺时,表观Km为0.23 mM,Vmax为每毫克蛋白质38.7 μmol/分钟。D-天冬酰胺是L-天冬酰胺水解的竞争性抑制剂,为此抑制作用测定的Ki大约等于其Km。这些数据表明,D-天冬酰胺是外部酵母天冬酰胺酶的良好底物,但却是内部酶的不良底物。

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