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新月柄杆菌色氨酸基因的遗传与物理分析

Genetic and physical analyses of Caulobacter crescentus trp genes.

作者信息

Winkler M E, Schoenlein P V, Ross C M, Barrett J T, Ely B

出版信息

J Bacteriol. 1984 Oct;160(1):279-87. doi: 10.1128/jb.160.1.279-287.1984.

Abstract

Caulobacter crescentus trp mutants were identified from a collection of auxotrophs. Precursor feeding experiments, accumulation studies, and complementation experiments resulted in the identification of six genes corresponding to trpA, trpB, trpC, trpD, trpE, and trpF. Genetic mapping experiments demonstrated that the trp genes were in two clusters, trpCDE and trpFBA, and a 5.4-kilobase restriction fragment from the C. crescentus chromosome was isolated that contained the trpFBA gene cluster. Complementation experiments with clones containing the 5.4-kilobase fragment indicated that trpF was expressed in Escherichia coli and that all three genes were expressed in Pseudomonas putida. This expression was lost in both organisms when the pBR322 tet gene promoter was inactivated, indicating that all three genes were transcribed in the same orientation from the tet promoter. Thus, the C. crescentus promoters do not seem to be expressed in E. coli or P. putida. Complementation of the C. crescentus trp mutants indicated that the tet promoter was not necessary for expression in C. crescentus and suggested that at least two native promoters were present for expression of the trpF, trpB, and trpA genes. Taken together, these results indicate that C. crescentus promoters may have structures that are significantly different from the promoters of other gram-negative species.

摘要

从一系列营养缺陷型菌株中鉴定出了新月柄杆菌色氨酸突变体。前体喂养实验、积累研究和互补实验导致鉴定出了六个与色氨酸A、色氨酸B、色氨酸C、色氨酸D、色氨酸E和色氨酸F相对应的基因。遗传图谱实验表明,色氨酸基因位于两个簇中,即色氨酸CDE和色氨酸FBA,并且从新月柄杆菌染色体中分离出了一个5.4千碱基的限制片段,该片段包含色氨酸FBA基因簇。用含有5.4千碱基片段的克隆进行的互补实验表明,色氨酸F在大肠杆菌中表达,并且所有三个基因在恶臭假单胞菌中表达。当pBR322四环素基因启动子失活时,这两种生物体中的这种表达都丧失了,这表明所有三个基因都是从四环素启动子以相同方向转录的。因此,新月柄杆菌启动子似乎在大肠杆菌或恶臭假单胞菌中不表达。新月柄杆菌色氨酸突变体的互补表明,四环素启动子对于在新月柄杆菌中的表达不是必需的,并表明至少存在两个天然启动子用于色氨酸F、色氨酸B和色氨酸A基因的表达。综上所述,这些结果表明新月柄杆菌启动子的结构可能与其他革兰氏阴性菌的启动子有显著差异。

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