低濃度に感染した野外試料からCandidatus Liberibacter asiaticusを検出する場合における遺伝子増幅法による陽性率の違い
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概要
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Polymerase chain reaction (PCR), loop-mediated isothermal amplification (LAMP), and quantitative PCR (qPCR) were used to detect low-level <I>Candidatus</I> Liberibacter asiaticus infection in citrus trees, and their results were compared. Sample DNA was prepared from the developing shoots of <I>Citrus depressa</I> and <I>Citrus tankan</I> that were spontaneously infected with <I>Ca</I>. L. asiaticus. The concentrations of the homologous region of the <I>tufB</I> gene of <I>Ca</I>. L. asiaticus were estimated by qPCR analysis using serially diluted plasmid DNA containing the <I>tufB</I> gene region as a calibration standard. All DNA samples from which the specific amplification product was detected by PCR also gave positive results in the LAMP analysis, and qPCR gave positive results for all samples that were positive in the LAMP analysis. Therefore, we concluded that qPCR is the most sensitive method for detecting low-level <I>Ca</I>. L. asiaticus infection.
- 九州病害虫研究会の論文
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