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禽博德特氏菌野生型和突变型fur基因的遗传特征分析

Genetic characterization of wild-type and mutant fur genes of Bordetella avium.

作者信息

Murphy E R, Dickenson A, Militello K T, Connell T D

机构信息

Center for Microbial Pathogenesis and Department of Microbiology, School of Medicine and Biomedical Sciences, State University of New York at Buffalo, Buffalo, New York 14214, USA.

出版信息

Infect Immun. 1999 Jun;67(6):3160-5. doi: 10.1128/IAI.67.6.3160-3165.1999.

Abstract

For most, if not all, organisms, iron (Fe) is an essential element. In response to the nutritional requirement for Fe, bacteria evolved complex systems to acquire the element from the environment. The genes encoding these systems are often coordinately regulated in response to the Fe concentration. Recent investigations revealed that Bordetella avium, a respiratory pathogen of birds, expressed a number of Fe-regulated genes (T. D. Connell, A. Dickenson, A. J. Martone, K. T. Militello, M. J. Filiatraut, M. L. Hayman, and J. Pitula, Infect. Immun. 66:3597-3605, 1998). By using manganese selection on an engineered strain of B. avium that carried an Fe-regulated alkaline phosphatase reporter gene, a mutant was obtained that was affected in expression of Fe-regulated genes. To determine if Fe-dependent regulation in B. avium was mediated by a fur-like gene, a fragment of the B. avium chromosome, corresponding to the fur locus of B. pertussis, was cloned by PCR. Sequencing revealed that the fragment from B. avium encoded a polypeptide with 92% identity to the Fur protein of B. pertussis. In vivo experiments showed that the cloned gene complemented H1780, a fur mutant of Escherichia coli. Southern hybridizations and PCRs demonstrated that the manganese mutant had a deletion of 2 to 3 kbp of nucleotide sequence in the region located immediately 5' of the fur open reading frame. A spontaneous PCR-derived mutant of the B. avium fur gene was isolated that encoded a Fur protein in which a histidine was substituted for an arginine at amino acid position 18 (R18H). Genetic analysis showed that the R18H mutant gene when cloned into a low-copy-number vector did not complement the fur mutation in H1780. However, the R18H mutant gene was able to complement the fur mutation when cloned into a high-copy-number vector. The cloned wild-type fur gene will be useful as a genetic tool to identify Fur-regulated genes in the B. avium chromosome.

摘要

对于大多数(如果不是所有的话)生物体而言,铁(Fe)是一种必需元素。为响应铁的营养需求,细菌进化出复杂系统以从环境中获取该元素。编码这些系统的基因通常会根据铁浓度进行协调调控。最近的研究表明,鸟类呼吸道病原体鸟博德特氏菌表达了许多铁调控基因(T.D.康奈尔、A.迪金森、A.J.马托内、K.T.米利泰洛、M.J.菲利阿特劳、M.L.海曼和J.皮图拉,《感染与免疫》66:3597 - 3605,1998年)。通过在携带铁调控碱性磷酸酶报告基因的鸟博德特氏菌工程菌株上进行锰选择,获得了一个在铁调控基因表达方面存在缺陷的突变体。为确定鸟博德特氏菌中铁依赖性调控是否由类fur基因介导,通过PCR克隆了鸟博德特氏菌染色体上对应百日咳博德特氏菌fur位点的一个片段。测序显示,来自鸟博德特氏菌的片段编码一种与百日咳博德特氏菌Fur蛋白具有92%同一性的多肽。体内实验表明,克隆的基因可互补大肠杆菌的fur突变体H1780。Southern杂交和PCR证明,锰突变体在fur开放阅读框紧邻上游5'区域有2至3kbp核苷酸序列的缺失。分离出一个源自PCR的鸟博德特氏菌fur基因自发突变体,其编码的Fur蛋白在氨基酸位置18处精氨酸被组氨酸取代(R18H)。遗传分析表明,当克隆到低拷贝数载体中时,R18H突变基因不能互补H1780中的fur突变。然而,当克隆到高拷贝数载体中时,R18H突变基因能够互补fur突变。克隆的野生型fur基因将作为一种遗传工具,用于鉴定鸟博德特氏菌染色体中受Fur调控的基因。

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