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首页> 外文期刊>Journal of dairy science >Screening of specific nucleic acid targets for Cronobacter sakazakii and visual detection by loop-mediated isothermal amplification and lateral flow dipstick method in powdered infant formula
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Screening of specific nucleic acid targets for Cronobacter sakazakii and visual detection by loop-mediated isothermal amplification and lateral flow dipstick method in powdered infant formula

机译:筛选婴幼儿配方粉幼述术曲崎茅草菌特异性核酸靶的筛选,术

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摘要

Due to the lack of specific genes for rapid detection methods of Cronobacter sakazakii in food samples, whole genome sequence analysis was performed in this investigation using the basic local alignment search tool. Forty-two DNA fragments unique to C. sakazakii were mined, then primers were designed and screened by PCR and loop-mediated isothermal amplification (LAMP). Two primer sets, CS1 and CS31, were found as specific and stable primers, with their corresponding nucleic acid targets the CSK29544_00235 gene and CSK29544_03484 gene, respectively. Furthermore, compared with 3 genes reported previously, these 2 genes were verified as more specific to C. sakazakii among Cronobacter species, by sequence similarity alignment using Cronobacter MLST databases (http: ∥ pubmlst .org/ cronobacter). The specificity of the LAMP reaction approached 100% by using 48 bacterial strains, which included 22 C. sakazakii strains. Subsequently, LAMP was combined with visual lateral flow dipstick (LFD) based on the above 2 nucleic acid targets, and was demonstrated as a rapid, efficient method with high specificity. Finally, the detection sensitivity of this assay system for pure cultures and artificially contaminated milk was measured as 4.5 × 10~0 cfu/mL and 5.7 × 10~1 cfu/g, respectively. Total time to detection for this assay was within 2 h. Thus, the establishment of this LAMP-LFD method shows great significance and potential for rapid detection of C. sakazakii in powdered infant formula.
机译:由于在食品样品中缺乏特异性基因,在食品样品中的阶段茅草杆菌的快速检测方法,通过基本局部对准搜索工具在本研究中进行全基因组序列分析。开采了C. Sakazakii独特的四十二个DNA片段,然后通过PCR和环形介导的等温扩增(灯)设计并筛选引物。发现两个引物组CS1和CS31作为特定且稳定的引物,其相应的核酸分别靶向CSK29544_00235基因和CSK29544_03484基因。此外,与先前报告的3个基因相比,通过使用克罗安杆菌MLST数据库的序列相似性对准,验证了这两种基因在串联物种中更具体于C. Sakazakii(http:∥pubmlst.org / clonobacter)。通过使用48种细菌菌株将灯反应的特异性接近了100%,其包括22℃甲崎菌株。随后,基于上述2个核酸靶标结合灯与视觉横向流量减少尺(LFD)组合,并被证明是具有高特异性的快速,有效的方法。最后,测定纯培养物和人工污染的乳的该测定系统的检测灵敏度分别为4.5×10〜0CFU / mL和5.7×10〜1 CFU / g。检测该测定的总时间在2小时内。因此,该灯LFD方法的建立具有良好的意义和粉状婴儿配方中C.Sakazakii的快速检测的巨大意义。

著录项

  • 来源
    《Journal of dairy science》 |2021年第5期|5152-5165|共14页
  • 作者单位

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

    Key Laboratory of Dairy Science Ministry of Education College of Food Science Northeast Agricultural University Harbin 150030 China;

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

    Cronobacter sakazakii; nucleic acid target; loop-mediated isothermal amplification; lateral flow dipstick; powdered infant formula;

    机译:cr s s cr;核酸靶;环介导的等温扩增;横向流量减少尺;粉状婴儿配方粉剂;

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