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  • 标题:ベロ毒素遺伝子の蛍光偏光法による迅速検出および遺伝子型別
  • 本地全文:下载
  • 作者:村野 勢津子 ; 伊藤 文明 ; 石村 勝之
  • 期刊名称:日本食品微生物学会雑誌
  • 印刷版ISSN:1340-8267
  • 电子版ISSN:1882-5982
  • 出版年度:2001
  • 卷号:18
  • 期号:1
  • 页码:15-19
  • DOI:10.5803/jsfm.18.15
  • 出版社:Japanese Society of Food Microbiology
  • 摘要:

    Fluorescence polarization technique can specifically detect nucleotide sequences by hybridization without separation procedures. We applied the technique to the detection of the Shiga toxin genes ( stx 1and stx 2) in enterohemorragic Escherichia coli (STEC). STEC possesses stx 1 and/or stx 2 and using MK primers, the amplification of stx 1 and/or stx 2 can be performed universally, but the band sizes for both genes are almost identical; thus the genotype is hard to determine using electrophoresis. To identify stx genotype, conventional PCR combined with electrophoresis requires a second amplification process with more than 25 temperature cycles using other genotype-specific primer pairs. However, using the newly developed method only a few temperature cycles of the asymmetric PCR using the same MK primers and two different probes for stx 1and stx 2 were needed. The incubation time for probe hybridization was 10 minutes, and the detection time for fluorescence polarization was within about 1 minute per sample. Thus, we considered that the detection method using fluorescence polarization technique was a rapid and reliable method for detecting stx 1and/or stx 2.

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