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LamB-mediated adherence of enteropathogenic Escherichia coli to HEp-2 cells

机译:LamB介导的肠致病性大肠杆菌对HEp-2细胞的粘附

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摘要

To establish the role of maltoporin (LamB) in adherence of enteropathogenic Escherichia coli (EPEC) to epithelial cells in vitro. Three strains, wild type (WT) EPEC, a maltoporin (LamB) mutant lamB, and DH5l were used to study adherence to cultured HEp-2 cells. Mutant lamB was found to be deficient in adherence compared to WT EPEC. Adherence of lamB was restored to wild type levels when complemented with the cloned lamB gene. The non-adherent strain DH5l also adhered to HEp-2 cells when it harboured the cloned lamB gene. The LamB protein was isolated from WT EPEC by electroelution and antibodies were raised in rabbits. The specificity of the antibodies was analysed by Western blotting. Anti-LamB antiserum reduced adherence of WT EPEC to HEp-2 cells. The LamB protein was coated on latex beads and the beads adhered to HEp-2 cells. Anti-LamB antiserum prevented bead adherence to HEp-2 cells. Multiple sequence alignment showed that the L9 loop of EPEC LamB had four amino acids different from the L9 loop of LamB from several other related pathogens. LamB serves as an alternative or additional adherence factor for EPEC. Adherence is an important component of the pathogenesis of noninvasive pathogens like EPEC. A putative adhesin such as LamB, which has already been found to be co-expressed with virulence factor EspB may be a potential vaccine candidate for control of EPEC and related pathogens.
机译:建立maltoporin(LamB)在肠道致病性大肠杆菌(EPEC)对上皮细胞的粘附中的作用。使用野生型(WT)EPEC,maltoporin(LamB)突变体lamB和DH51三种菌株研究对培养的HEp-2细胞的粘附性。与WT EPEC相比,发现突变型lamB缺乏依从性。当与克隆的lamB基因互补时,lamB的粘附力恢复到野生型水平。当具有克隆的lamB基因时,非贴壁菌株DH51也粘附于HEp-2细胞。通过电洗脱从WT EPEC中分离了LamB蛋白,并在兔中产生了抗体。通过蛋白质印迹分析抗体的特异性。抗LamB抗血清可降低WT EPEC对HEp-2细胞的粘附。将LamB蛋白包被在乳胶珠上,并将珠粘附在HEp-2细胞上。抗LamB抗血清可防止珠粒粘附于HEp-2细胞。多重序列比对显示,EPEC LamB的L9环具有四个氨基酸,与其他几种相关病原体的LamB的L9环不同。 LamB充当EPEC的替代或附加遵守因素。粘附是无创性病原体(如EPEC)发病机理的重要组成部分。推定的粘附素(如LamB)已被发现与毒力因子EspB共表达,可能是控制EPEC和相关病原体的潜在候选疫苗。

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