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细胞黏菌盘基网柄菌中嘧啶代谢的特征分析。

Characterization of pyrimidine metabolism in the cellular slime mold, Dictyostelium discoideum.

作者信息

Wales M E, Mann-Dean M G, Wild J R

机构信息

Department of Biochemistry and Biophysics, Texas A&M University System, College Station 77843-2128.

出版信息

Can J Microbiol. 1989 Apr;35(4):432-8. doi: 10.1139/m89-066.

DOI:10.1139/m89-066
PMID:2568162
Abstract

The arginine-independent, de novo biosynthetic pathway of pyrimidines in Dictyostelium discoideum is initiated by a class II carbamoyl-phosphate synthetase (EC 6.3.5.5) specific for pyrimidine biosynthesis which utilized L-glutamine as its N donor and was partially inhibited by both UTP and CTP. The second step in the de novo pathway was provided by an unregulated aspartate transcarbamoylase (EC 2.1.3.2) which primarily appeared as a multimeric enzyme of 105 kilodaltons. The next enzyme, dihydroorotase (EC 3.5.2.3), was approximately 90-100 kilodaltons. Although the early enzymatic activities of the pyrimidine pathway appeared to reside in independent protein complexes, various unstable molecular species were observed. These structural variants may represent proteolytic fragments of a multienzyme complex. In addition to de novo synthesis, the amoeba demonstrated the capacity for salvage utilization of uracil, uridine, and cytidine. Upon starvation on a solid substratum, axenically grown amoebas began a concerted developmental program accompanied by a restructuring of nucleotide metabolism. The absolute levels of the ribonucleotide pools droppedby 98% within 30 h; however, both the adenylate energy charge and the GTP/ATP ratios were maintained for 50 h after the initiation of development. The maintenance of these metabolic energy parameters required the tight cell-cell contact necessary for development, and the capacity for pyrimidine metabolism was maintained throughout developmental morphogenesis.

摘要

盘基网柄菌中嘧啶的不依赖精氨酸的从头生物合成途径由一种II类氨甲酰磷酸合成酶(EC 6.3.5.5)启动,该酶对嘧啶生物合成具有特异性,以L-谷氨酰胺作为其氮供体,并受到UTP和CTP的部分抑制。从头合成途径的第二步由一种不受调控的天冬氨酸转氨甲酰酶(EC 2.1.3.2)提供,该酶主要以105千道尔顿的多聚体形式出现。下一种酶二氢乳清酸酶(EC 3.5.2.3)的分子量约为90 - 100千道尔顿。尽管嘧啶途径的早期酶活性似乎存在于独立的蛋白质复合物中,但观察到了各种不稳定的分子形式。这些结构变体可能代表多酶复合物的蛋白水解片段。除了从头合成外,变形虫还表现出对尿嘧啶、尿苷和胞苷的补救利用能力。在固体培养基上饥饿时,无菌培养的变形虫开始了协调的发育程序,同时伴随着核苷酸代谢的重组。在30小时内,核糖核苷酸池的绝对水平下降了98%;然而,在发育开始后的50小时内,腺苷酸能量电荷和GTP/ATP比值都得以维持。维持这些代谢能量参数需要发育所必需的紧密细胞间接触,并且嘧啶代谢能力在整个发育形态发生过程中得以维持。

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