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淋球菌转铁蛋白结合蛋白A中对配体结合和铁摄取功能必需的离散结构域的鉴定。

Identification of discrete domains within gonococcal transferrin-binding protein A that are necessary for ligand binding and iron uptake functions.

作者信息

Boulton I C, Yost M K, Anderson J E, Cornelissen C N

机构信息

Department of Microbiology and Immunology, Medical College of Virginia Campus of Virginia Commonwealth University, Richmond, Virginia 23298, USA.

出版信息

Infect Immun. 2000 Dec;68(12):6988-96. doi: 10.1128/IAI.68.12.6988-6996.2000.

Abstract

The availability of free iron in vivo is strictly limited, in part by the iron-binding protein transferrin. The pathogenic Neisseria spp. can sequester iron from this protein, dependent upon two iron-repressible, transferrin-binding proteins (TbpA and TbpB). TbpA is a TonB-dependent, integral, outer membrane protein that may form a beta-barrel exposing multiple surface loops, some of which are likely to contain ligand-binding motifs. In this study we propose a topological model of gonococcal TbpA and then test some of the hypotheses set forth by the model by individually deleting three putative loops (designated loops 4, 5, and 8). Each mutant TbpA could be expressed without toxicity and was surface exposed as assessed by immunoblotting, transferrin binding, and protease accessibility. Deletion of loop 4 or loop 5 abolished transferrin binding to whole cells in solid- and liquid-phase assays, while deletion of loop 8 decreased the affinity of the receptor for transferrin without affecting the copy number. Strains expressing any of the three mutated TbpAs were incapable of growth on transferrin as a sole iron source. These data implicate putative loops 4 and 5 as critical determinants for receptor function and transferrin-iron uptake by gonococcal TbpA. The phenotype of the DeltaL8TbpA mutant suggests that high-affinity ligand interaction is required for transferrin-iron internalization.

摘要

体内游离铁的可用性受到严格限制,部分原因是铁结合蛋白转铁蛋白。致病性奈瑟菌属细菌能够从这种蛋白质中螯合铁,这依赖于两种铁抑制性转铁蛋白结合蛋白(TbpA和TbpB)。TbpA是一种依赖TonB的整合外膜蛋白,可能形成一个暴露多个表面环的β桶,其中一些环可能包含配体结合基序。在本研究中,我们提出了淋球菌TbpA的拓扑模型,然后通过分别删除三个假定的环(指定为环4、环5和环8)来测试该模型提出的一些假设。每个突变型TbpA都可以无毒表达,并且通过免疫印迹、转铁蛋白结合和蛋白酶可及性评估表明其暴露于表面。在固相和液相试验中,删除环4或环5消除了转铁蛋白与全细胞的结合,而删除环8降低了受体对转铁蛋白的亲和力,但不影响拷贝数。表达三种突变型TbpA中任何一种的菌株都不能以转铁蛋白作为唯一铁源生长。这些数据表明,假定的环4和环5是淋球菌TbpA受体功能和转铁蛋白-铁摄取的关键决定因素。DeltaL8TbpA突变体的表型表明,转铁蛋白-铁内化需要高亲和力配体相互作用。

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