Research in Plant Disease (Sep 2024)

Enhancing Conventional PCR for Detection of Erwinia amylovora

  • Hyun Ju Choi,
  • Yeon Ju Kim,
  • Jeong Ho Choi,
  • Dong Hyuk Choi,
  • Duck Hwan Park

DOI
https://doi.org/10.5423/RPD.2024.30.3.294
Journal volume & issue
Vol. 30, no. 3
pp. 294 – 299

Abstract

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Polymerase chain reaction (PCR) methods, including conventional PCR (cPCR) and quantitative real-time PCR (qRT-PCR), with both plasmid- and chromosome-targeting primers, are currently the most reliable methods for detecting Erwinia amylovora due to their high sensitivity and specificity. Despite qRT-PCR's quantitative advantage, cPCR remains an attractive method to detect this bacterium in initial screenings of suspected host plants, as it is cost-effective and does not require skilled personnel in well-equipped laboratories. This study aimed to significantly improve cPCR robustness via application of bovine serum albumin (BSA) as a PCR facilitator, with a modified EaF/R primer pair, as previously reported. Experiments have shown that simple supplementation with BSA (10 mg/ml) enhances cPCR reactions using templates such as genomic DNA, bacterial cells, and infected symptomless host organs, including immature apple fruits and seedlings, with EaF/R primers. The cPCR method described in this study is simple, specific, and reliable, and can be applied in routine assays to diagnose fire blight.

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