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Multiplex PCR for detection of the heat-labile toxin gene and shiga-like toxin I and II genes in Escherichia coli isolated from natural waters.

机译:多重PCR用于检测从天然水体分离出的大肠杆菌中的热不稳定毒素基因以及志贺样毒素I和II基因。

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摘要

A triplex PCR method was developed to simultaneously amplify a heat-labile toxin sequence (LT) of 258 bp, a shiga-like toxin I sequence (SLT I) of 130 bp, and a shiga-like toxin II sequence (SLT II) of 346 bp from toxigenic strains of Escherichia coli. This method was used to screen 377 environmental E. coli isolates from marine waters or estuaries located in Southern California and North Carolina for enterotoxigenic or enterohemorrhagic E. coli strains. Of the 377 E. coli screened, one isolate was found to belong to the enterotoxigenic group, since it contained a LT homologous sequence, and one isolate was found to belong to the enterohemorrhagic group, since it contained a SLT I homologous sequence. None was found to contain SLT II homologous sequences. The pathogenicity of the positive environmental E. coli isolates was confirmed by standard bioassays with Y-1 adrenal cells and Vero cells to confirm toxin production. Our results suggest that toxigenic E. coli occurs infrequently in environmental waters and that there is a low public health risk from toxigenic E. coli in coastal waters.
机译:开发了一种三重PCR方法,可同时扩增258 bp的不耐热毒素序列(LT),130 bp的志贺样毒素I序列(SLT I)和109 bp的志贺样毒素II序列(SLT II)。来自大肠杆菌的产毒菌株的346bp。该方法用于从位于南加利福尼亚州和北卡罗来纳州的海水或河口中筛选出377种环境大肠杆菌分离株,以检测产肠毒素或肠出血性大肠杆菌。在所筛选的377株大肠杆菌中,发现一种分离物属于产肠毒素组,因为它含有LT同源序列;发现一种分离物属于肠出血性组,因为它含有SLT I同源序列。没有发现包含SLT II同源序列。通过使用Y-1肾上腺细胞和Vero细胞的标准生物测定法确认了阳性环境大肠杆菌分离株的致病性,以确认毒素的产生。我们的研究结果表明,在环境水域中,产毒素大肠杆菌很少发生,在沿海水域中,产毒素大肠杆菌的公共健康风险较低。

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