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溶血曼氏杆菌(巴斯德氏菌)A1中一种假定的铁调节TonB依赖性受体:相变的可能机制。

A putative iron-regulated TonB-dependent receptor of Mannheimia (Pasteurella) haemolytica A1: possible mechanism for phase variation.

作者信息

Graham Morag R, Lo Reggie Y C

机构信息

Department of Microbiology, University of Guelph, Guelph, Ont., Canada N1G 2W1.

出版信息

Vet Microbiol. 2002 Jan 3;84(1-2):53-67. doi: 10.1016/s0378-1135(01)00415-1.

Abstract

A recombinant plasmid that codes for a novel iron receptor protein (Irp) of Mannheimia (Pasteurella) haemolytica A1 was isolated by the partial complementation of an Escherichia coli fur mutant. The deduced amino acid sequence of Irp exhibited characteristics typical of TonB-dependent receptors. These include: a TonB-box at the N-terminal; a 50 amino acid region homologous to the "plug" domain of the E. coli FhuA and FepA receptors; and a C-terminal TonB-dependent signature which likely functions as an outer membrane anchoring domain. Previously uncharacterized Irp homologues were detected by BLAST analysis of available databases and incomplete microbial genomes. When the irp homologues from Neisseria gonorrhoeae and N. meningitidis were cloned by PCR and expressed in E. coli, novel proteins of the predicted size (84kDa) were detected in cell lysates, demonstrating that these are functional genes. The M. haemolytica A1 irp gene undergoes phase variation at a nucleotide region which contain the sequence AAAAAAATTAAAA (7A-2T-4A) flanked by a short inverted repeat. Site-specific mutagenesis of the 7A-2T-4A sequence as well as replacement of the inverted repeats resulted in a stable construct that expressed the Irp protein without phase variation. The expression of irp in M. haemolytica A1 was regulated by iron concentrations and most likely a Fur homologue, consistent with the proposed function of Irp in iron metabolism. The irp genes may represent contingency loci that play a role in iron acquisition during infection.

摘要

通过对大肠杆菌fur突变体的部分互补作用,分离出了一种编码溶血曼氏杆菌(巴斯德氏菌)A1新型铁受体蛋白(Irp)的重组质粒。Irp推导的氨基酸序列显示出典型的依赖TonB的受体特征。这些特征包括:N端的TonB框;与大肠杆菌FhuA和FepA受体的“塞子”结构域同源的50个氨基酸区域;以及可能作为外膜锚定结构域的C端TonB依赖特征序列。通过对现有数据库和不完整微生物基因组进行BLAST分析,检测到了以前未鉴定的Irp同源物。当通过PCR克隆淋病奈瑟菌和脑膜炎奈瑟菌的irp同源物并在大肠杆菌中表达时,在细胞裂解物中检测到了预测大小(84kDa)的新型蛋白质,表明这些是功能基因。溶血曼氏杆菌A1的irp基因在一个核苷酸区域发生相变,该区域包含序列AAAAAAATTAAAA(7A - 2T - 4A),两侧是短的反向重复序列。对7A - 2T - 4A序列进行位点特异性诱变以及替换反向重复序列,产生了一个稳定的构建体,该构建体可表达Irp蛋白且无相变。溶血曼氏杆菌A1中irp的表达受铁浓度调节,很可能受Fur同源物调节,这与Irp在铁代谢中的推测功能一致。irp基因可能代表在感染期间铁获取中起作用的应急位点。

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