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大肠杆菌中嘧啶途径的酶。II. 二氢乳清酸脱氢酶的细胞内定位及特性

ENZYMES OF THE PYRIMIDINE PATHWAY IN ESCHERICHIA COLI. II. INTRACELLULAR LOCALIZATION AND PROPERTIES OF DIHYDROOROTIC DEHYDROGENASE.

作者信息

TAYLOR W H, TAYLOR M L

出版信息

J Bacteriol. 1964 Jul;88(1):105-10. doi: 10.1128/jb.88.1.105-110.1964.

Abstract

Taylor, W. Herman (Portland State College, Portland, Ore.), and Mary L. Taylor. Enzymes of the pyrimidine pathway in Escherichia coli. II. Intracellular localization and properties of dihydroorotic dehydrogenase. J. Bacteriol. 88:105-111. 1964.-Intracellular localization of three enzymes of the pyrimidine pathway in Escherichia coli was studied. Dihydroorotic dehydrogenase was found to be associated with the membrane portion of lysed spheroplasts. Centrifugal fractionation of cell-free extracts showed all the dihydroorotic dehydrogenase activity to be associated with large structures, probably cell wall-membrane fragments. In contrast, all orotidylic decarboxylase activity was found in the cytoplasm in both lysed spheroplasts and cell-free extracts. Aspartate transcarbamylase activity appeared to be particulate in repressed cells, but only 25% was particulate in derepressed cells. Dihydroorotic dehydrogenase was shown to be bound to oxidative particles by oxygen uptake and orotate production from dihydroorotate. A ferricyanide reduction assay, suitable for measuring soluble and particulate enzyme, was devised for dihydroorotic dehydrogenase. Soluble dihydroorotic dehydrogenase was prepared by use of deoxycholate. A 20-fold purification of the enzyme compared to whole-cell activity was achieved by ammonium sulfate fractionation of the deoxycholate-soluble enzyme. Although cytochromes were implicated by cyanide inhibition of aerobic orotate production by particles, the purified enzyme appeared to be separated from the cytochromes, as shown by lack of cyanide inhibition in the ferricyanide assay. The purified soluble enzyme did not react in the aerobic assay previously used by others for assay of this enzyme. In contrast to the degradative dihydroorotic dehydrogenases reported by other workers, the biosynthetic dihydroorotic dehydrogenase of E. coli did not link to pyridine nucleotides.

摘要

泰勒,W. 赫尔曼(波特兰州立学院,俄勒冈州波特兰),以及玛丽·L. 泰勒。大肠杆菌嘧啶途径的酶。II. 二氢乳清酸脱氢酶的细胞内定位及特性。《细菌学杂志》88:105 - 111。1964年。——研究了大肠杆菌嘧啶途径中三种酶的细胞内定位。发现二氢乳清酸脱氢酶与裂解原生质球的膜部分相关。对无细胞提取物进行离心分级分离显示,所有二氢乳清酸脱氢酶活性都与大的结构相关,可能是细胞壁 - 膜碎片。相比之下,在裂解原生质球和无细胞提取物中,所有乳清酸脱羧酶活性都存在于细胞质中。天冬氨酸转氨甲酰酶活性在阻遏细胞中似乎是颗粒状的,但在去阻遏细胞中只有25%是颗粒状的。通过氧摄取以及由二氢乳清酸产生乳清酸表明,二氢乳清酸脱氢酶与氧化颗粒结合。设计了一种适用于测量可溶性和颗粒状酶的铁氰化物还原测定法来检测二氢乳清酸脱氢酶。利用脱氧胆酸盐制备了可溶性二氢乳清酸脱氢酶。通过对脱氧胆酸盐可溶性酶进行硫酸铵分级分离,该酶与全细胞活性相比实现了20倍的纯化。尽管通过氰化物对颗粒需氧产生乳清酸的抑制表明细胞色素与之有关,但纯化后的酶似乎与细胞色素分离,如在铁氰化物测定中缺乏氰化物抑制所示。纯化后的可溶性酶在其他人先前用于检测该酶 的需氧测定中不发生反应。与其他研究者报道的降解性二氢乳清酸脱氢酶不同,大肠杆菌的生物合成性二氢乳清酸脱氢酶不与吡啶核苷酸相连。

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