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用于醋酸发酵的醋酸杆菌的遗传组织。

Genetic organization of Acetobacter for acetic acid fermentation.

作者信息

Beppu T

机构信息

Department of Agricultural Chemistry, Faculty of Agriculture, University of Tokyo, Japan.

出版信息

Antonie Van Leeuwenhoek. 1993;64(2):121-35. doi: 10.1007/BF00873022.

Abstract

Plasmid vectors for the acetic acid-producing strains of Acetobacter and Gluconobacter were constructed from their cryptic plasmids and the efficient transformation conditions were established. The systems allowed to reveal the genetic background of the strains used in the acetic acid fermentation. Genes encoding indispensable components in the acetic acid fermentation, such as alcohol dehydrogenase, aldehyde dehydrogenase and terminal oxidase, were cloned and characterized. Spontaneous mutations at high frequencies in the acetic acid bacteria to cause the deficiency in ethanol oxidation were analyzed. A new insertion sequence element, IS1380, was identified as a major factor of the genetic instability, which causes insertional inactivation of the gene encoding cytochrome c, an essential component of the functional alcohol dehydrogenase complex. Several genes including the citrate synthase gene of A. aceti were identified to confer acetic acid resistance, and the histidinolphosphate aminotransferase gene was cloned as a multicopy suppressor of an ethanol sensitive mutant. Improvement of the acetic acid productivity of an A. aceti strain was achieved through amplification of the aldehyde dehydrogenase gene with a multicopy vector. In addition, spheroplast fusion of the Acetobacter strains was developed and applied to improve their properties.

摘要

从醋杆菌属和葡糖杆菌属产乙酸菌株的隐蔽质粒构建了质粒载体,并建立了高效的转化条件。该系统有助于揭示乙酸发酵所用菌株的遗传背景。克隆并鉴定了编码乙酸发酵中不可或缺成分的基因,如乙醇脱氢酶、醛脱氢酶和末端氧化酶。分析了乙酸细菌中导致乙醇氧化缺陷的高频自发突变。一种新的插入序列元件IS1380被确定为遗传不稳定性的主要因素,它会导致编码细胞色素c的基因插入失活,细胞色素c是功能性乙醇脱氢酶复合体的重要组成部分。鉴定了包括醋化醋杆菌柠檬酸合酶基因在内的几个基因赋予乙酸抗性,并克隆了组氨酸磷酸转氨酶基因作为乙醇敏感突变体的多拷贝抑制子。通过用多拷贝载体扩增醛脱氢酶基因,提高了醋化醋杆菌菌株的乙酸生产力。此外,开发并应用了醋杆菌属菌株的原生质体融合来改善其特性。

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