Mitochondrial Loci Enable Specific Quantitative Real-Time PCR Detection of the Pathogen Causing Contemporary Impatiens Downy Mildew Epidemics

Impatiens downy mildew (IDM) disease is a primary constraint on the production of Impatiens walleriana, a popular and economically important floriculture plant. IDM is caused by the biotrophic. oomycete Plasmopara destructor that emerged as a pathogen of I. walleriana in the 2000s. To enable P. dest...

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Veröffentlicht in:	Plant disease. - 1997. - 106(2022), 1 vom: 29. Jan., Seite 144-150
1. Verfasser:	LeBlanc, Nicholas (VerfasserIn)
Weitere Verfasser:	Martin, Frank, Castroagudín, Vanina, Crouch, Jo Anne
Format:	Online-Aufsatz
Sprache:	English
Veröffentlicht:	2022
Zugriff auf das übergeordnete Werk:	Plant disease
Schlagworte:	Journal Article Plasmopara downy mildew impatiens mitochondrial DNA real-time PCR


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245	1	0	\|a Mitochondrial Loci Enable Specific Quantitative Real-Time PCR Detection of the Pathogen Causing Contemporary Impatiens Downy Mildew Epidemics
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500			\|a Date Completed 09.02.2022
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520			\|a Impatiens downy mildew (IDM) disease is a primary constraint on the production of Impatiens walleriana, a popular and economically important floriculture plant. IDM is caused by the biotrophic. oomycete Plasmopara destructor that emerged as a pathogen of I. walleriana in the 2000s. To enable P. destructor detection and quantification, a hydrolysis-probe-based quantitative PCR diagnostic assay was developed based on unique orientation and order of the mitochondrial cytochrome c oxidase subunit1 (cox1) and ATP synthase subunit alpha (atp1) genes in the genus Plasmopara. Nucleotide sequences and analysis of the cox1/atp1 region distinguished P. destructor and its sister-species P. obducens, consistent with prior phylogenetic analyses using cox2 and rDNA markers. Specificity for P. destructor was incorporated into a hydrolysis probe targeting the cox1 gene and flanking primers that amplified across the cox1/atp1 intergenic region. The limit of detection was 0.5 fg/μl of P. destructor DNA (∼100 plasmid copies/μl), with amplification efficiency = 0.95. The assay was validated against a panel of target and nontarget oomycetes, which showed that the primers were specific for Plasmopara spp., while the probe was specific for P. destructor infecting both I. walleriana and I. balsamina. Testing of Impatiens tissue collected from 23 locations across 13 states indicated all samples with IDM symptoms tested positive for P. destructor. Asymptomatic plants from two locations also tested positive for P. destructor
650		4	\|a Journal Article
650		4	\|a Plasmopara
650		4	\|a downy mildew
650		4	\|a impatiens
650		4	\|a mitochondrial DNA
650		4	\|a real-time PCR
700	1		\|a Martin, Frank \|e verfasserin \|4 aut
700	1		\|a Castroagudín, Vanina \|e verfasserin \|4 aut
700	1		\|a Crouch, Jo Anne \|e verfasserin \|4 aut
773	0	8	\|i Enthalten in \|t Plant disease \|d 1997 \|g 106(2022), 1 vom: 29. Jan., Seite 144-150 \|w (DE-627)NLM098181742 \|x 0191-2917 \|7 nnas
773	1	8	\|g volume:106 \|g year:2022 \|g number:1 \|g day:29 \|g month:01 \|g pages:144-150
856	4	0	\|u http://dx.doi.org/10.1094/PDIS-05-21-0933-RE \|3 Volltext
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