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无法产生短杆菌酪肽的短短芽孢杆菌突变体的分离与特性

Isolation and properties of Bacillus brevis mutants unable to produce tyrocidine.

作者信息

Symons D C, Hodgson B

出版信息

J Bacteriol. 1982 Aug;151(2):580-90. doi: 10.1128/jb.151.2.580-590.1982.

DOI:10.1128/jb.151.2.580-590.1982
PMID:6284703
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC220298/
Abstract

Mutants of Bacillus brevis ATCC 10068 were isolated which produced less than 1/100 of the amount of tyrocidine produced by the parent strain. These mutants produced spores at the same frequency and which were as resistant to heating at 80 degrees C for up to 3 h as were those produced by the parent strain. A partially purified tyrocidine synthetase from strain ATCC 10068 catalyzed [32P]PPi-ATP exchange reactions dependent on added tyrocidine-constituent amino acids. These activities were separated into three groups (I, II, and III) by fractionation on an Ultrogel AcA34 column. Each group was similar to one of the three components (heavy, intermediate, and light, respectively) found previously for strain ATCC 8185 except that glutamate-dependent activity was not detected in the group I activities and some amino acyl-tRNA synthetase activities were associated with the group III activities. Some of the mutants were shown to have defective tyrocidine synthetase enzymes. Mutant BH30 was defective in two of the group II amino acid-dependent [32P]PPi-ATP exchange reactions, mutant BH16 was defective in one of the group I and one of the group II reactions, and mutant BH34 had alterations to activities in all of the groups. It is unlikely that any of these mutants could synthesise tyrocidine. We conclude that tyrocidine is not involved in either the sporulation process or the resistance of spores of B. brevis ATCC 10068 to heating at 80 degrees C for up to 3 h.

摘要

已分离出短短芽孢杆菌ATCC 10068的突变体,其产生的短杆菌肽量不到亲本菌株的1/100。这些突变体产生孢子的频率与亲本菌株相同,且其孢子对80℃加热长达3小时的耐受性与亲本菌株产生的孢子相同。来自菌株ATCC 10068的部分纯化的短杆菌肽合成酶催化依赖于添加的短杆菌肽组成氨基酸的[32P]PPi-ATP交换反应。通过在Ultrogel AcA34柱上分级分离,这些活性被分为三组(I、II和III)。每组分别类似于先前在菌株ATCC 8185中发现的三种组分(重、中、轻)之一,不同之处在于在I组活性中未检测到依赖谷氨酸的活性,并且一些氨酰-tRNA合成酶活性与III组活性相关。一些突变体显示出短杆菌肽合成酶有缺陷。突变体BH30在II组中两种依赖氨基酸的[32P]PPi-ATP交换反应中有缺陷,突变体BH16在I组中的一种反应和II组中的一种反应中有缺陷,突变体BH34在所有组的活性中都有改变。这些突变体中任何一个都不太可能合成短杆菌肽。我们得出结论,短杆菌肽不参与短短芽孢杆菌ATCC 10068的孢子形成过程或孢子对80℃加热长达3小时的抗性。

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本文引用的文献

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Biosynthesis of tyrocidine by a cell-free enzyme system of Bacillus brevis ATCC 8185. 3. Further purification of components I and II and their functions in tyrocidine synthesis.短短芽孢杆菌ATCC 8185无细胞酶系统合成短杆菌酪肽。3. 组分I和II的进一步纯化及其在短杆菌酪肽合成中的作用。
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