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RPA-Cas12a-FS: A frontline nucleic acid rapid detection system for food safety based on CRISPR-Cas12a combined with recombinase polymerase amplification

机译:RPA-CAS12A-FS:基于CRISPR-CAS12A结合重组酶聚合酶扩增的食品安全的前线核酸快速检测系统

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摘要

Food analysis to ensure food safety and quality are relevant to all countries. This study aimed to develop a detection technique by combining recombinase polymerase amplification with CRISPR-Cas12a for food safety (termed RPA-Cas12a-FS). Our data showed that this novel method could be detected via fluorescence intensity for the molecular identification of foodborne pathogenic bacteria, genetically modified crops, and meat adulteration. After optimization, the sensitivity and stability of RPA-Cas12a-FS was further enhanced. The RPA-Cas12a-FS system could specifically detect target gene levels as low as 10 copies in 45 min at 37 degrees C. The RPA-Cas12a-FS system was sensitive both using standard samples in the lab and using samples from the field, which indicated that this detection method was practical. In conclusion, a simple, rapid, and highly sensitive detection method based on CRISPR-Cas12a was developed for molecular identification in the food safety field without requiring technical expertise or ancillary equipment.
机译:食品分析以确保食品安全和质量与所有国家有关。本研究旨在通过将重组酶聚合酶扩增与CRISPR-CAS12A结合用于食品安全(称为RPA-CAS12A-FS)来发展检测技术。我们的数据表明,通过荧光强度可以通过用于食源性致病细菌的分子鉴定,遗传修饰的作物和肉掺杂的荧光强度来检测这种新方法。优化后,进一步提高了RPA-CAS12A-FS的灵敏度和稳定性。 RPA-CAS12A-FS系统可以在37摄氏度中特别地检测到45分钟内的靶基因水平低至10℃.RPA-CAS12A-FS系统在实验室中使用标准样品并使用来自现场的样品敏感表明该检测方法是实用的。总之,基于CRISPR-CAS12A的简单,快速和高度敏感的检测方法,用于食品安全领域的分子鉴定,无需技术专长或辅助设备。

著录项

  • 来源
    《Food Chemistry》 |2021年第1期|127608.1-127608.8|共8页
  • 作者单位

    Shanghai Acad Agr Sci Inst Biotechnol Res 2901 Beidi Rd Shanghai 201106 Peoples R China|Key Lab Agr Genet & Breeding 2901 Beidi Rd Shanghai 201106 Peoples R China|Minist Agr & Rural Affairs Crops Ecol Environm Secur Inspect & Supervis Ctr 2901 Beidi Rd Shanghai 201106 Peoples R China;

    Shanghai Acad Agr Sci Inst Biotechnol Res 2901 Beidi Rd Shanghai 201106 Peoples R China|Key Lab Agr Genet & Breeding 2901 Beidi Rd Shanghai 201106 Peoples R China|Minist Agr & Rural Affairs Crops Ecol Environm Secur Inspect & Supervis Ctr 2901 Beidi Rd Shanghai 201106 Peoples R China;

    Shanghai Acad Agr Sci Inst Biotechnol Res 2901 Beidi Rd Shanghai 201106 Peoples R China|Key Lab Agr Genet & Breeding 2901 Beidi Rd Shanghai 201106 Peoples R China|Minist Agr & Rural Affairs Crops Ecol Environm Secur Inspect & Supervis Ctr 2901 Beidi Rd Shanghai 201106 Peoples R China;

    Lanzhou Univ Technol Sch Life Sci & Engn Lanzhou 730050 Peoples R China;

    Shanghai Acad Agr Sci Inst Biotechnol Res 2901 Beidi Rd Shanghai 201106 Peoples R China|Key Lab Agr Genet & Breeding 2901 Beidi Rd Shanghai 201106 Peoples R China|Minist Agr & Rural Affairs Crops Ecol Environm Secur Inspect & Supervis Ctr 2901 Beidi Rd Shanghai 201106 Peoples R China;

    Lanzhou Univ Technol Sch Life Sci & Engn Lanzhou 730050 Peoples R China;

    Lanzhou Univ Technol Sch Life Sci & Engn Lanzhou 730050 Peoples R China;

    Shanghai Acad Agr Sci Inst Biotechnol Res 2901 Beidi Rd Shanghai 201106 Peoples R China|Key Lab Agr Genet & Breeding 2901 Beidi Rd Shanghai 201106 Peoples R China|Minist Agr & Rural Affairs Crops Ecol Environm Secur Inspect & Supervis Ctr 2901 Beidi Rd Shanghai 201106 Peoples R China;

  • 收录信息 美国《科学引文索引》(SCI);美国《生物学医学文摘》(MEDLINE);
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    CRISPR-Cas12a; Detection; Foodborne pathogenic bacteria; Genetically modified crops; Meat adulteration;

    机译:CRISPR-CAS12A;检测;食源性致病细菌;遗传修饰的作物;肉掺假;

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