Real-time PCR, a method fit for detection and quantification of Erwinia amylovora

被引:9
|
作者
Dreo, Tanja [1 ]
Pirc, Manca [1 ]
Ravnikar, Maja [1 ]
机构
[1] Natl Inst Biol, Dept Biotechnol & Syst Biol, Ljubljana 1000, Slovenia
来源
TREES-STRUCTURE AND FUNCTION | 2012年 / 26卷 / 01期
关键词
Real-time PCR; Fire blight; Erwinia amylovora; Analytical sensitivity; FIRE BLIGHT PATHOGEN; INTERGENIC SPACER REGION; COMPLETE GENOME SEQUENCE; QUANTITATIVE PCR; PEAR; DNA; BACTERIA; PYRIFOLIAE; IDENTIFICATION; AMPLIFICATION;
D O I
10.1007/s00468-011-0654-7
中图分类号
S7 [林业];
学科分类号
0829 ; 0907 ;
摘要
Fire blight, a devastating disease of pome fruit trees continues to pose threat to agricultural production. Detection of its causative agent, bacterium Erwinia amylovora, is usually straightforward in symptomatic samples. Methods with increased sensitivity however, are sometimes needed for detection of E. amylovora and real-time PCR assays have been shown to have required sensitivity and reliability. Here we summarize our previous results on real-time PCR detection of fire blight and present new, fast and sensitive real-time PCR assay based on amsC gene performed on SmartCycler (R) instrument. The setting is optimal for analysis of small number of samples in the laboratory or for on-site detection. Many advantages of real-time PCR assays warrant their use in detection and diagnosis of E. amylovora, particularly in detection of low concentrations of target bacteria e. g. in testing for latent infections. It is to be expected that the use of real-time PCR will increase in both diagnostics and in research, as a tool for target detection and quantification as well as for gene expression analysis.
引用
收藏
页码:165 / 178
页数:14
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