High-throughput screening of natural compounds for prophage induction in controlling pathogenic bacteria in food

Elizabeth Tompkins, Brigitte Cadieux, Margot Amitrano, Lawrence Goodridge
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Abstract

Introduction: The clean label trend emphasizes the need for natural approaches to combat pathogenic bacteria in food. This study explores the potential of inducing prophages within bacterial genomes as a novel strategy to control pathogenic and spoilage bacterial growth.Methods: A luminescence-based high-throughput assay was developed to identify natural compounds capable of inducing prophages. Bioactive compounds from four chemical libraries were screened at a final concentration of 10 µM. The assay measured luminescence production in Escherichia coli BR513, a genetically modified strain producing β-galactosidase upon prophage λ induction. Luminescence values were normalized to cell concentration (OD600) and the interquartile mean of each 384-well plate. A cut-off for normalized luminescence values, set at 2.25 standard deviations above the mean, defined positive prophage induction.Results: Four naturally-derived compounds (osthol, roccellic acid, galanginee, and sclareol) exhibited positive prophage induction, along with previously identified inducers, rosemary, and gallic acid. Dose-response experiments were conducted to determine optimal concentrations for prophage induction. However, the results could not distinguish between prophage-induced cell death and other mechanisms, making it challenging to identify ideal concentrations.Discussion: The high-throughput luminescent prophage induction assay serves as a valuable tool for the initial screening of natural bioactive compounds that have the potential to enhance food safety and quality by inducing prophages. Further research is required to understand the mechanism of bacterial cell death and to establish optimal concentrations for prophage induction in a food preservation context.
高通量筛选天然化合物诱导噬菌体以控制食品中的致病菌
导言:清洁标签趋势强调需要采用天然方法来对付食品中的致病菌。本研究探讨了在细菌基因组中诱导噬菌体作为控制致病菌和腐败菌生长的新策略的潜力:方法:研究人员开发了一种基于发光的高通量检测方法,以鉴定能够诱导噬菌体的天然化合物。以 10 µM 的最终浓度筛选了四个化学文库中的生物活性化合物。该检测法测量了大肠杆菌 BR513 的发光率,BR513 是一种转基因菌株,在诱导噬菌体 λ 时能产生 β-半乳糖苷酶。发光值归一化为细胞浓度(OD600)和每个 384 孔板的四分位数平均值。归一化发光值的临界值设定为高于平均值的 2.25 个标准偏差,以定义阳性噬菌体诱导:结果:四种天然提取的化合物(osthol、rocellic acid、galanginee 和 sclareol)以及之前确定的诱导剂迷迭香和没食子酸均显示出阳性噬菌体诱导作用。为了确定诱导噬菌体的最佳浓度,进行了剂量反应实验。然而,实验结果无法区分噬菌体诱导的细胞死亡和其他机制,因此确定理想浓度具有挑战性:高通量发光噬菌体诱导试验是初步筛选天然生物活性化合物的重要工具,这些化合物有可能通过诱导噬菌体来提高食品安全和质量。要了解细菌细胞死亡的机制,并确定在食品保鲜中诱导噬菌体的最佳浓度,还需要进一步的研究。
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