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实时荧光定量PCR快速检测大肠埃希菌的方法研究 被引量:4

Study of rapid method on enterotoxigenic Escherichia coli detected by real-time fluoresence quantitative PCR
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摘要 目的基于TaqMan探针建立产肠毒素大肠埃希菌实时荧光定量PCR检测方法。方法针对编码大肠埃希菌耐热肠毒素STI、不耐热性肠毒素LTI基因片段设计引物、探针,采用外标法,绘制标准曲线,进行荧光定量PCR检测。结果引物、探针特异性良好,该方法的灵敏度可达到每反应1DNA拷贝,特异性强,检测范围在100~107拷贝每反应,重复性及稳定性好,整个过程只需要2h。结论该方法能快速、灵敏、特异检出产肠毒素大肠埃希菌。 Objective To develop a real-time PCR for detecting enterotoxigenic Escherichia coli(ETEC) based on TaqMan technology.Methods Primers and probes were designed in the coding region of heat-stable enterotoxin,heat-labile enterotoxin of ETEC.ETEC were detected by real-time fluoresence quantitative PCR,making use of the exterior standard curve which was described by several different concentration.The speciality,sensitivity,accuracy,repetition,and stability of real-time fluoresence quantitative PCR system were evaluated.Results Primers and TaqMan probes were suited to the real-time fluoresence quantitative PCR.The assay showed that the method could be rapid,special,sensitive and stabile.The real-time PCR system could detect ETEC between 100-107DNA copies/reaction.The assay should be finished in two hours.Conclusion It was suggested that real-time fluoresence quantitative PCR based on TaqMan probe could be a rapid,sensitive and special method.It is significant that the excellent method could control diarrhoea caused by ETEC.
作者 代娟 李玉峰 杨潇 袁粒星 汪云利
机构地区 成都医学院医学检验系 西华大学生物工程学院 四川大学华西第二医院
出处 《卫生研究》 CAS CSCD 北大核心 2008年第5期606-608,共3页 Journal of Hygiene Research
基金 四川省科技厅项目(No.R0520503)
关键词 产肠毒素大肠埃希菌 TAQMAN探针 实时荧光定量PCR enterotoxigenic Escherichia coli,TaqMan probe,real-time fluoresence quantitative PCR
分类号 R378.2 [医药卫生—病原生物学] TS207.4 [轻工技术与工程—食品科学]
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参考文献8

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同被引文献42

  • 1蔡霞.定量PCR技术及其应用现状[J].现代诊断与治疗,2005,16(2):112-115. 被引量:25
  • 2许颂霄,王虹,尹一兵.定量PCR的荧光技术[J].生命的化学,2005,25(5):413-415. 被引量:4
  • 3张莹丹,徐维明,李健峰.大肠埃希菌不耐热肠毒素研究进展[J].动物医学进展,2007,28(2):85-88. 被引量:6
  • 4熊国华,于莉,杨海龙,曹远银,曹际娟.实时荧光PCR定量检测食品中单增李斯特菌[J].中国食品卫生杂志,2007,19(3):248-251. 被引量:12
  • 5Zhang W P,Berberov E M,Freeling J,et al.Significance ofHeat-Stable and Heat-Labile Enterotoxins in Porcine Coli-bacillosis in an Additive Model for Pathogenicity Studie[J].Infection and Immunity,2006(7):3107-3114.
  • 6Niemi R M,Heikkila M P,Lahti K,et al.Comparison ofmethods for determining the numbers and species is tribu-tion of coli form bacteria in well water samples[J].AppliedMicrobiology,2001,90:850-858.
  • 7Fu J,Li D,Xia S Y,et al.Absolute Quantification of Plas-mid DNA by Real-time PCR with Genomic DNA as Exter-nal Standard and Its Application to a Biodistribution Studyof an HIV DNA Vaccine[J].Analytical Sciences,2009,25(5):675-680.
  • 8Jin L Z,Zhao X.Intestinal receptors for adhesive fimbriae ofenterotoxigenic Escherichia coli(ETEC)K88in swine[J].Applied Microbiology and Biotechnology,2000,54:311-318.
  • 9Bela N,Peter Z F.Enterotoxigenic Escherichia coli in vet-erinary medicine[J].International Journal of Medical Mi-crobiology,2005,295:443-454.
  • 10Ronald H L P,Arnoud C F,Jan M R,et al.Sensitivity andaccuracy of quantitative real-time polymerase chain reac-tion using SYBR green I depends on cDNA synthesis con-ditions[J].Analytical Biochemistry,2002,307:63-69.

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卫生研究
2008年 第5期

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