Abstract
李凤娟,阚飙,王多春.非O1非O139群霍乱弧菌多重PCR和SYBR Green实时PCR检测方法的建立[J].Chinese journal of Epidemiology,2014,35(1):66-70
非O1非O139群霍乱弧菌多重PCR和SYBR Green实时PCR检测方法的建立
Development of both multiple PCR and real—time SYBR green PCR for the detection of Vibrio cholerae non.O1/O139 serogroups
Received:September 05, 2013  
DOI:
KeyWord: 非Ol非0139群霍乱弧菌  多重PCR  SYBRGreen实时PCR
English Key Word: Vibrio cholera.non—O1/0139 serogroups  Multiple PCR  Real-time sYBR greenPCR
FundProject:国家自然科学基金(30872260);国家科技重大专项(2008ZXl0004—012)
Author NameAffiliationE-mail
Li Fengjuan   
Kan Biao   
Wang Duochun  wangduochun@icdc.cN 
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Abstract:
      目的建立检测非Ol非0139群霍乱弧菌的多重PCR和SYBRGreen实时PCR方法。方法分别以霍乱弧菌的外膜蛋白基因(ompW)、01和0139群O抗原编码基因(咖)设计引物,建立多重PCR和SYBRGreen实时PCR方法,评价两种方法检测非01非0139群霍乱弧菌的特异性、重复性和一致性及最低检测菌量。结果建立了检测非01非0139群霍乱弧菌的多重PCR和SYBRGreen实时PCR方法,根据特异性条带(多重PCR)和特异性熔解温度(SYBRGreen实时PCR),两种方法均能特异性检测非01非0139群霍乱弧菌,并能鉴别其他弧菌(5种)和肠道杆菌(3种);两种方法的最低检测菌量分别为7×104 cfu/ml(多重PCR)和7×102cftdml(SYBR Green实时PCR),差异有统计学意义(P<0.05);对实时PCR的重复性检测,批内变异系数(CV)为 0.22%~0.92%,批间cv为0.27%~1.41%;经370株非01非0139群霍乱弧菌的检测,两种方法的一致性均为100%。结论建立的两种方法其特异性、敏感性及重复性均好,可适用于不同条件下非0l非0139群霍乱弧菌的检测和鉴定。
English Abstract:
      Objective To develop methodology of both multiple PCR and real-time SYBRgreen PCR for the detection of V/brio cholerae(V.choleraE)serogroups non—01 and non-0139. Methods The outer membrane protein gene(ompW)specific for V.choleraE,as well as O antigen rfb genes specific for both O I and O 1 39.were used for the design of the PCR primers.Both multiple PCR and real—time SYBR green PCR systems were used to detect both 01 and 0139.Specific rfb genes and ompW were developed to evaluate their specificity,limit of detection,reproducibility and consistency.Results We established multiple PCR and real.time SYBR green PCR methods.According to the specific electrophoretic bands(multiple PCR)and the specific melt curve temperature(real-time SYBR green PCR).both methods could specifically detect the non一0 l,non-O l 39矿cholerae,and to differentiate them from O 1.O l 39矿cholerae.other five Vibrios and 3 intestinal bacteria.The detection limits were 7×104 cfu/ml(multiple PCR)and 7×102 cfu/m1(real—time SYBR green PCR),with statistically significant difference seen(P<0.05).For the reproducibility of real-time SYBR green PCR.the external COC:mcient variation ranging from 0.22%to 0.92%while the internal coefficient variation ranging from 0.27%to 1.41%.370 strains ofnon.0l,non.0139 V.cholerae,were detected。with both consistency rates as 1 00%.Conelusion Both multiple PCR and real—time SYBR green PCR could detectnon.01。non一O139V.cholerae,rapidly,specifically,and reproducibly,that could all be used for the detection and identification ofnon.Ol。non一0139 under different conditions.
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