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Identification and sensitive endophytic detection of the fire blight pathogen Erwinia amylovora with 23S ribosomal DNA sequences and the polymerase chain reaction
Author(s) -
MAES M.,
GARBEVA P.,
CREPEL C.
Publication year - 1996
Publication title -
plant pathology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.928
H-Index - 85
eISSN - 1365-3059
pISSN - 0032-0862
DOI - 10.1046/j.1365-3059.1996.d01-186.x
Subject(s) - erwinia , fire blight , biology , polymerase chain reaction , bacteria , microbiology and biotechnology , 16s ribosomal rna , ribosomal dna , pantoea , virulence , pathogen , ribosomal rna , phytoplasma , blight , botany , gene , restriction fragment length polymorphism , genetics , phylogenetics
Two short sequences, situated in the bacterial 23S rDNA gene, were used as primers for the PCR detection of Erwinia amylovora bacteria. All 34 E. amylovora strains tested, coming from different geographical and host plant origins and of different virulence, produced a 565‐bp PCR fragment. The E. amylovora bacteria could be discriminated from all other phytobacteria with which no PCR product was observed. Only Escherichia coli bacteria were cross‐recognized by the production of a weaker PCR band of similar size to E. amylovora . In a fast PCR protocol, where two temperatures were cycled, E. amylovora in pure culture could be detected on gel at concentrations as low as 3 × 10 2 cfu mL –1 . This corresponds to a detection limit of 1.5 bacteria per PCR. However, reliable PCR detection in woody host plant tissue was only obtained with PVP/PVPP‐treated sample extracts. Using E. amylovora ‐spiked plant extracts and extracts of fruit tree shoots artificially infected with E. amylovora , the PCR detection sensitivity was determined to be 6.6 × 10 2 cfu mL –1 of extract. Starting from the plant samples, the PCR detection results were visualized on gels within 5 h.