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使用磁性离子液体和重组酶聚合酶扩增技术捕获、浓缩和检测食品中的沙门氏菌。

Capture, Concentration, and Detection of Salmonella in Foods Using Magnetic Ionic Liquids and Recombinase Polymerase Amplification.

出版信息

Anal Chem. 2019 Jan 2;91(1):1113-1120. doi: 10.1021/acs.analchem.8b04751. Epub 2018 Dec 11.

DOI:10.1021/acs.analchem.8b04751
PMID:30499290
Abstract

We previously investigated the extraction and concentration of bacteria from model systems using magnetic ionic liquid (MIL) solvents while retaining their viability. Here, we combine MIL-based sample preparation with isothermal amplification and detection of Salmonella-specific DNA using recombinase polymerase amplification (RPA). After initial developmental work with Serratia marcescens in water, Salmonella Typhimurium ATCC 14028 was inoculated in water, 2% milk, almond milk, or liquid egg samples and extracted using one of two MILs, including trihexyl(tetradecyl)phosphonium cobalt(II) hexafluoroacetylacetonate ([P][Co(hfacac)]) and trihexyl(tetradecyl)phosphonium nickel(II) hexafluoroacetylacetonate ([P][Ni(hfacac)]). Viable cells were recovered from the MIL extraction phase after the addition of modified LB broth, followed by a 20 min isothermal RPA assay. Amplification was carried out using supersaturated sodium acetate heat packs and results compared to those using a conventional laboratory thermocycler set to a single temperature. Results were visualized using either gel electrophoresis or nucleic acid lateral flow immunoassay (NALFIA). The combined MIL-RPA approach enabled detection of Salmonella at levels as low as 10 CFU mL. MIL-based sample preparation required less than 5 min to capture and concentrate sufficient cells for detection using RPA, which (including NALFIA or gel-based analysis) required approximately 30-45 min. Our results suggest the utility of MILs for the rapid extraction and concentration of pathogenic microorganisms in food samples, providing a means for physical enrichment that is compatible with downstream analysis using RPA.

摘要

我们之前研究了使用磁性离子液体(MIL)溶剂从模型系统中提取和浓缩细菌,同时保持其活力。在这里,我们将基于 MIL 的样品制备与等温扩增和沙门氏菌特异性 DNA 的检测相结合,使用重组酶聚合扩增(RPA)。在对水培的粘质沙雷氏菌进行初步开发工作后,将鼠伤寒沙门氏菌 ATCC 14028 接种到水中、2%牛奶、杏仁奶或液体蛋样品中,并用两种 MIL 之一进行提取,包括三己基(十四烷基)膦钴(II)六氟乙酰丙酮酸盐([P][Co(hfacac)])和三己基(十四烷基)膦镍(II)六氟乙酰丙酮酸盐([P][Ni(hfacac)])。在添加改良 LB 肉汤后,从 MIL 提取阶段回收活菌,然后进行 20 分钟的等温 RPA 测定。使用过饱和的醋酸钠热包进行扩增,并将结果与使用传统实验室热循环仪设置为单一温度的结果进行比较。使用凝胶电泳或核酸侧向流动免疫分析(NALFIA)进行结果可视化。MIL-RPA 联合方法能够检测到低至 10 CFU mL 的沙门氏菌。基于 MIL 的样品制备仅需不到 5 分钟即可捕获和浓缩足够的细胞用于 RPA 检测,(包括 NALFIA 或基于凝胶的分析)大约需要 30-45 分钟。我们的结果表明,MIL 可用于从食品样品中快速提取和浓缩致病微生物,为使用 RPA 进行下游分析提供了一种与物理富集兼容的方法。

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