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大肠杆菌呼吸型NADH脱氢酶的特性及ndh突变体膜囊泡中NADH氧化酶的重组。

Characterization of the respiratory NADH dehydrogenase of Escherichia coli and reconstitution of NADH oxidase in ndh mutant membrane vesicles.

作者信息

Jaworowski A, Mayo G, Shaw D C, Campbell H D, Young I G

出版信息

Biochemistry. 1981 Jun 9;20(12):3621-8. doi: 10.1021/bi00515a049.

Abstract

Highly purified preparations of the cholate-solubilized respiratory NADH dehydrogenase, isolated from genetically amplified Escherichia coli strains [Jaworowski, A., Campbell, H. D., Poulis, M. I., & Young, I. G. (1981) Biochemistry 20, 2041-2047], have been characterized. Enzyme preparations were shown to contain 70% (w/w) lipid, predominantly phosphatidylethanolamine. One mol of noncovalently bound FAD and approximately 1 mol of ubiquinone/mol of enzyme subunit were detected. The purified enzyme was shown to contain only low levels of Fe and acid-labile S, indicating the absence of iron-sulfur clusters. No Cu, Mo, W, or covalently bound P was detected, and no evidence for other chromophores was obtained from visible and ultraviolet absorption spectra of the purified enzyme or of the delipidated polypeptide prepared by gel filtration in sodium dodecyl sulfate. Protein chemical studies verified that the enzyme consists of a single polypeptide species of Mr 47 000, and the N- and C-terminal cyanogen bromide peptides were identified. The pure enzyme was shown to reconstitute membrane-bound, cyanide-sensitive NADH oxidase activity in membrane vesicles prepared from ndh mutant strains.

摘要

已对从基因扩增的大肠杆菌菌株中分离得到的经胆酸盐增溶的呼吸型NADH脱氢酶的高纯度制剂进行了表征[亚沃罗夫斯基,A.,坎贝尔,H. D.,普利西斯,M. I.,&扬,I. G.(1981年)《生物化学》20,2041 - 2047]。酶制剂显示含有70%(重量/重量)的脂质,主要是磷脂酰乙醇胺。检测到每摩尔酶亚基含有1摩尔非共价结合的FAD和约1摩尔泛醌。纯化后的酶仅含有低水平的铁和酸不稳定硫,表明不存在铁硫簇。未检测到铜、钼、钨或共价结合的磷,并且从纯化酶或通过十二烷基硫酸钠凝胶过滤制备的脱脂多肽的可见和紫外吸收光谱中未获得其他发色团的证据。蛋白质化学研究证实该酶由一种分子量为47000的单一多肽组成,并鉴定了N端和C端溴化氰肽。纯化后的酶显示能在由ndh突变株制备的膜泡中重建膜结合的、对氰化物敏感的NADH氧化酶活性。

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