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流感嗜血杆菌中人转铁蛋白结合蛋白编码基因的鉴定与特性分析。

Identification and characterization of genes encoding the human transferrin-binding proteins from Haemophilus influenzae.

作者信息

Gray-Owen S D, Loosmore S, Schryvers A B

机构信息

Department of Microbiology and Infectious Diseases, Faculty of Medicine, University of Calgary, Alberta, Canada.

出版信息

Infect Immun. 1995 Apr;63(4):1201-10. doi: 10.1128/iai.63.4.1201-1210.1995.

Abstract

Haemophilus influenzae, a strict human pathogen, acquires iron in vivo through the direct binding and removal of iron from human transferrin by an as yet uncharacterized process at the bacterial cell surface. In this study, the tbpA and tbpB genes of H. influenzae, encoding the transferrin-binding proteins Tbp1 and Tbp2, respectively, were cloned and sequenced. Alignments of the H. influenzae Tbp1 and Tbp2 protein sequences with those of related proteins from heterologous species were analyzed. On the basis of similarities between these and previously characterized proteins, Tbp1 appears to be a member of the TonB-dependent family of outer membrane proteins while Tbp2 is lipid modified by signal peptidase II. Isogenic mutants deficient in expression of Tbp1 or Tbp2 or both proteins were prepared by insertion of the Tn903 kanamycin resistance cassette into cloned sequences and reintroduction of the interrupted sequences into the wild-type chromosome. Binding assays with the mutants showed that a significant reduction in transferrin-binding ability resulted from the loss of either of the Tbps and a complete loss of binding was evident when neither protein was expressed. Loss of either Tbp2 or both proteins correlated with an inability to grow on media supplemented with transferrin-bound iron as the sole source of iron, whereas the Tbp1+ Tbp2- mutant was able to grow only at high transferrin concentrations.

摘要

流感嗜血杆菌是一种严格的人类病原体,它通过一种尚未明确的过程,在细菌细胞表面直接结合并从人转铁蛋白中去除铁,从而在体内获取铁。在本研究中,分别编码转铁蛋白结合蛋白Tbp1和Tbp2的流感嗜血杆菌tbpA和tbpB基因被克隆并测序。分析了流感嗜血杆菌Tbp1和Tbp2蛋白序列与来自异源物种的相关蛋白序列的比对情况。基于这些蛋白与先前已鉴定蛋白之间的相似性,Tbp1似乎是外膜蛋白中依赖TonB的家族成员,而Tbp2经信号肽酶II进行脂质修饰。通过将Tn903卡那霉素抗性盒插入克隆序列并将中断的序列重新导入野生型染色体,制备了缺乏Tbp1或Tbp2或两种蛋白表达的同基因突变体。对这些突变体进行的结合试验表明,任何一种转铁蛋白结合蛋白(Tbp)的缺失都会导致转铁蛋白结合能力显著降低,而当两种蛋白均不表达时,结合能力则完全丧失。Tbp2缺失或两种蛋白均缺失与在以转铁蛋白结合铁作为唯一铁源的培养基上无法生长相关,而Tbp1+Tbp2-突变体仅在高浓度转铁蛋白条件下才能生长。

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