PMA结合ddPCR检测食品中沙门氏菌
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Detection of Salmonella in Food Based on PMA-ddPCR
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    摘要:

    建立一种快速、灵敏的微滴式数字PCR方法,用于检测食品中沙门氏菌活菌。利用叠氮溴化丙锭(PMA)对死菌预处理,PMA可以选择性穿过死菌细胞膜,在光照条件下与死菌DNA发生共价交联反应,进而阻止其DNA进行PCR扩增,提取细菌基因组DNA进行微滴式数字PCR(ddPCR)检测。结果表明,强烈光照15.0 min,可以使PMA与死菌DNA共价交联,同时钝化游离的PMA;PMA终质量浓度为40.0 μg/mL可以有效抑制105 CFU/mL的沙门氏菌死菌DNA的PCR扩增;不抑制活菌DNA扩增的PMA最高浓度是50.0 μg/mL。利用PMA处理死活菌混合液时,PMA-ddPCR可以在死菌存在的条件下,定量检测活菌,降低了“假阳性”结果的出现。灵敏度检测结果显示:PMA-ddPCR灵敏度是0.4 copy/μL。利用PMA-ddPCR检测人工污染的鳕鱼样品,最低可检出102 CFU/mL的沙门氏菌,精密度和稳定性良好。

    Abstract:

    The research aimed to establish a fast method to detect of live Salmonella in food with high sensitity. Propidium monoazide(PMA) permeated in the injured cells,then PMA and DNA conducted covalent cross-linking reaction,which could inhibit PCR amplification. Finally,bacterial genome DNA was extracted to detect by ddPCR. The optimization of experimental parameters showed that a final PMA concentration of 40.0 μg/mL and exposure of 15 min could restrain DNA amplification of 105 CFU/mL dead cells ,and the maximum PMA against DNA amplification from live Salmonella cells was 50.0 μg/mL. Under the different live/dead bacteria proportion,only live Salmonella cells was detected by PMA-ddPCR even in the existence of dead Salmonella cells. The detection limit was 8.0 copy/20 μL. PMA-ddPCR could detect 102 CFU/mL Salmonella cells in the codfish polluted by manual work. Furthermore,PMA-ddPCR showed better accuracy and stability. In conclusion,PMA-ddPCR showed huge potential in foodborne pathogenic bacteria detection.

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王静,秦燕,张慧敏,刘玉敏,魏玮,贾俊涛. PMA结合ddPCR检测食品中沙门氏菌[J].食品与生物技术学报,2017,36(10):1059-1063.

WANG Jing, QIN Yan, ZHANG Huimin, LIU Yumin, WEI Wei, JIA Juntao. Detection of Salmonella in Food Based on PMA-ddPCR[J]. Journal of Food Science and Biotechnology,2017,36(10):1059-1063.

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  • 在线发布日期: 2017-12-26
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