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Detection on Surfaces and in Caco-2 Cells of Campylobacter jejuni Cells Transformed with New gfp, yfp, and cfp Marker Plasmids

机译:新gfp,yfp和cfp标记质粒转化的空肠弯曲菌细胞表面和Caco-2细胞的检测

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摘要

We have developed two sets of Campylobacter shuttle vectors containing either the gfp (green fluorescent protein), yfp (yellow fluorescent protein), or cfp (cyan fluorescent protein) reporter gene. In one set, the reporter gene is fused to a consensus Campylobacter promoter sequence (Pc). The other set contains a pUC18 multicloning site upstream of the reporter gene, allowing the construction of transcriptional fusions using known promoters or random genomic fragments. C. jejuni cells transformed with the Pc fusion plasmids are strongly fluorescent and easily visualized on chicken skin, on plant tissue, and within infected Caco-2 cells. In each C. jejuni strain tested, these plasmids were maintained over several passages in the absence of antibiotic selection. Also, in many C. jejuni strains, >91% of the cells transformed with the Pc fusion plasmids remained fluorescent after several days. Experiments with yellow fluorescent and cyan fluorescent C. jejuni transformants suggest that aggregates containing two or more strains of C. jejuni may be present in an enrichment broth culture. Colonies arising from these aggregates would be heterologous in nature; therefore, isolation of a pure culture of C. jejuni, by selecting single colonies, from an environmental sample may not always yield a single strain.
机译:我们已经开发了两组弯曲杆菌穿梭载体,它们包含gfp(绿色荧光蛋白),yfp(黄色荧光蛋白)或cfp(蓝绿色荧光蛋白)报告基因。在一组中,报告基因与共有弯曲杆菌启动子序列(Pc)融合。另一组在报告基因上游包含一个pUC18多克隆位点,从而允许使用已知的启动子或随机基因组片段构建转录融合体。用Pc融合质粒转化的空肠弯曲杆菌细胞具有强烈的荧光,可以很容易地在鸡皮,植物组织上以及感染的Caco-2细胞内看到。在测试的每个空肠弯曲杆菌菌株中,这些质粒在没有抗生素选择的情况下经过数次传代而得以维持。同样,在许多空肠弯曲杆菌菌株中,几天后,用Pc融合质粒转化的细胞中> 91%仍保持荧光。用黄色荧光和绿色荧光的空肠弯曲杆菌转化子进行的实验表明,在富集培养液中可能存在含有两种或两种以上空肠弯曲杆菌菌株的聚集体。这些聚集体产生的菌落本质上是异源的;因此,通过从环境样品中选择单个菌落来分离空肠弯曲菌的纯培养物可能并不总是产生单个菌株。

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