Boyd J, Oza M N, Murphy J R
Evans Department of Clinical Research, Boston University Medical Center, MA 02118.
Proc Natl Acad Sci U S A. 1990 Aug;87(15):5968-72. doi: 10.1073/pnas.87.15.5968.
Although the structural gene for diphtheria toxin, tox, is carried by a family of closely related corynebacteriophages, the regulation of tox expression is controlled, to a large extent, by its bacterial host Corynebacterium diphtheriae. Optimal yields of tox gene products are obtained only when iron becomes the growth-rate-limiting substrate. Previous studies suggest that regulation of tox expression is mediated through an iron-binding aporepressor. To facilitate molecular cloning of the tox regulatory element from genomic libraries of C. diphtheriae, we constructed a tox promoter/operator (toxPO)-lacZ transcriptional fusion in Escherichia coli strain DH5 alpha. We report the molecular cloning and nucleic acid sequence of a diphtheria tox iron-dependent regulatory element, dtxR, and demonstrate that expression of beta-galactosidase from the toxPO-lacZ fusion is regulated by dtxR-encoded protein in an iron-sensitive manner. In addition, we show that expression of the toxPO-lacZ fusion is not affected by the E. coli iron-regulatory protein Fur and that the dtxR protein does not inhibit expression of fur-regulated outer-membrane proteins.
尽管白喉毒素的结构基因tox由一系列密切相关的棒状噬菌体携带,但tox表达的调控在很大程度上由其细菌宿主白喉棒状杆菌控制。只有当铁成为生长速率限制底物时,才能获得tox基因产物的最佳产量。先前的研究表明,tox表达的调控是通过一种铁结合无辅基阻遏物介导的。为了便于从白喉棒状杆菌基因组文库中分子克隆tox调控元件,我们在大肠杆菌菌株DH5α中构建了一个tox启动子/操纵子(toxPO)-lacZ转录融合体。我们报道了白喉毒素铁依赖性调控元件dtxR的分子克隆和核酸序列,并证明来自toxPO-lacZ融合体的β-半乳糖苷酶表达受dtxR编码蛋白以铁敏感方式调控。此外,我们表明toxPO-lacZ融合体的表达不受大肠杆菌铁调控蛋白Fur的影响,并且dtxR蛋白不抑制Fur调控的外膜蛋白的表达。
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