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Identification, characterization, and nucleotide sequence of the F17-G gene, which determines receptor binding of Escherichia coli F17 fimbriae.

机译:F17-G基因的鉴定,表征和核苷酸序列,该基因确定大肠杆菌F17菌毛的受体结合。

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摘要

Enterotoxigenic Escherichia coli strains express fimbriae which mediate binding to intestinal mucosal cells. The F17 fimbriae mediate binding to N-acetylglucosamine-containing receptors present on calf intestinal mucosal cells. These fimbriae consist of F17-A subunit peptides. Analysis of the F17 gene cluster indicated that at least the F17-A, F17-C, F17-D, and F17-G genes are indispensable to obtain adhesive F17 fimbriae (unpublished data). Genetic evidence is presented that the F17-G protein, a minor fimbrial component, is required for the binding of the F17 fimbriae to the intestinal villi. The F17-G gene was cloned and sequenced. An open reading frame of 1,032 bp encoding a polypeptide of 344 amino acids, starting with a signal sequence of 22 residues, was localized. The F17-G mutant strain produced F17 fimbriae which were morphologically identical to the fimbriae purified from strains which contained the intact F17 gene cluster. However, this F17-G mutant could no longer adhere to calf villi. The F17-G locus was shown to act in trans: transformation of the F17-G mutant strain, still expressing the genes F17-A, F17-C, and F17-D, with a vector expressing the F17-G gene restored the binding activity of this mutant strain.
机译:产肠毒素的大肠杆菌菌株表达菌毛,介导与肠粘膜细胞结合。 F17菌毛介导与小牛肠粘膜细胞上存在的含N-乙酰氨基葡萄糖的受体结合。这些菌毛由F17-A亚基肽组成。对F17基因簇的分析表明,至少F17-A,F17-C,F17-D和F17-G基因对于获得粘附性F17菌毛是必不可少的(未发表的数据)。遗传证据表明,F17-G蛋白是次要的纤维成分,是F17菌毛与肠绒毛结合所必需的。克隆并测序F17-G基因。定位了一个1,032 bp的开放阅读框,该编码框包含344个氨基酸,从22个残基的信号序列开始。 F17-G突变菌株产生的F17菌毛在形态上与从含有完整F17基因簇的菌株中纯化的菌毛形态相同。但是,此F17-G突变体不再能附着在小牛绒毛上。 F17-G基因座显示出反式作用:仍表达F17-A,F17-C和F17-D基因的F17-G突变株转化,表达F17-G基因的载体恢复了结合突变株的活性。

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