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通过在大肠杆菌中进行反式互补从绿豆中克隆鸟氨酸δ-氨基转移酶cDNA以及脯氨酸生物合成的调控

Cloning of ornithine delta-aminotransferase cDNA from Vigna aconitifolia by trans-complementation in Escherichia coli and regulation of proline biosynthesis.

作者信息

Delauney A J, Hu C A, Kishor P B, Verma D P

机构信息

Department of Biology, University of the West Indies, Barbados.

出版信息

J Biol Chem. 1993 Sep 5;268(25):18673-8.

PMID:8103048
Abstract

Proline prototrophy was restored to an Escherichia coli proBA proline auxotroph by ornithine and a mothbean (Vigna aconitifolia) cDNA expression library. This novel strategy, "trans-complementation," allowed isolation of a cDNA encoding ornithine delta-aminotransferase (delta-OAT). This enzyme transaminates ornithine to glutamic-gamma-semialdehyde (GSA), thereby bypassing the block in GSA synthesis from glutamate in the proBA mutant. The identity of the mothbean enzyme was confirmed by its high sequence homology to mammalian and yeast delta-OATs as well as to a family of bacterial and fungal omega-aminotransferases and an absence of significant homology to various alpha-aminotransferases. The V. aconitifolia OAT cDNA encodes a polypeptide of 48.1 kDa. The native enzyme expressed in E. coli appears to be a monomer with Km of 2 mM for ornithine and 0.75 mM for alpha-ketoglutarate. Levels of mRNA in V. aconitifolia for delta 1-pyrroline-5-carboxylate synthetase (P5CS) and delta-OAT, the two key enzymes for proline synthesis, were monitored under different physiological conditions. Salt stress and nitrogen starvation induced P5CS mRNA levels and depressed OAT mRNA levels. Conversely, OAT mRNA level was elevated in plants supplied with excess nitrogen while the P5CS mRNA level was reduced. These data suggest that the glutamate pathway is the primary route for proline synthesis in plants during conditions of osmotic stress and nitrogen limitation whereas the ornithine pathway assumes prominence under high nitrogen input.

摘要

通过鸟氨酸和一个绿豆(豇豆)cDNA表达文库,脯氨酸原养型得以恢复到大肠杆菌proBA脯氨酸营养缺陷型。这种新颖的策略“反式互补”,使得编码鸟氨酸δ-氨基转移酶(δ-OAT)的cDNA得以分离。该酶将鸟氨酸转氨生成谷氨酸γ-半醛(GSA),从而绕过了proBA突变体中从谷氨酸合成GSA的障碍。绿豆酶的身份通过其与哺乳动物和酵母δ-OAT以及细菌和真菌ω-氨基转移酶家族的高度序列同源性得以确认,并且与各种α-氨基转移酶没有显著同源性。豇豆OAT cDNA编码一个48.1 kDa的多肽。在大肠杆菌中表达的天然酶似乎是一种单体,对鸟氨酸的Km为2 mM,对α-酮戊二酸的Km为0.75 mM。在不同生理条件下监测了豇豆中脯氨酸合成的两个关键酶δ-1-吡咯啉-5-羧酸合成酶(P5CS)和δ-OAT的mRNA水平。盐胁迫和氮饥饿诱导P5CS mRNA水平升高并降低OAT mRNA水平。相反,在供应过量氮的植物中OAT mRNA水平升高,而P5CS mRNA水平降低。这些数据表明,在渗透胁迫和氮限制条件下,谷氨酸途径是植物中脯氨酸合成的主要途径,而在高氮输入下鸟氨酸途径则占主导地位。

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