Development of a One-Step Real-Time Polymerase Chain Reaction Assay for Diagnosis of Phytophthora ramorum

Hughes, Kelvin; Tomlinson, J. A.; Griffin, R. L.; Boonham, Neil; Inman, A. J.; Lane, Charles R.

doi:10.1094/phyto-96-0975

Cited by 82 publications

(96 citation statements)

References 28 publications

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“…Diagnostic PCR methods and specific primers have been developed for Phytophthora species including P. nicotianae (12, 18, 22, 28) and P. cactorum (2, 5, 21, 30), but most of these studies aimed at the detection of a single pathogen. Multiplex PCR assays allow the simultaneous detection of several species, and facilitate large-scale sample processing (25); however, multiplex PCR has been applied rarely in plant pathology (13, 14, 24, 31, 34, 35). This is partially due to the difficulties related to the development of quantitative multiplex assays and to the reduced sensitivity of multiplex PCR compared with simplex PCR (31).…”

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confidence: 99%

Simultaneous Detection and Quantification of Phytophthora nicotianae and P. cactorum, and Distribution Analyses in Strawberry Greenhouses by Duplex Real-time PCR

Inada

Watanabe³

et al. 2013

Microb. Environ.

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Phytophthora nicotianae and P. cactorum cause Phytophthora rot of strawberry. A duplex real-time PCR technique for simultaneous detection and quantification of the two pathogens was developed. Species-specific primers for P. nicotianae and P. cactorum were designed based on the internal transcribed spacer regions (ITS) of rDNA and the ras-related protein gene Ypt1, respectively. TaqMan probes were labeled with FAM for P. nicotianae and HEX for P. cactorum. Specificities were demonstrated using 52 isolates, including various soil-borne pathogens. Sensitivities for P. nicotianae and P. cactorum DNAs were 10 fg and 1 pg, respectively. The technique was applied to naturally infested soil and root samples; the two pathogens were detected and the target DNA concentrations were quantified. Significant correlations of DNA quantities in roots and the surrounding soils were found. The minimum soil DNA concentration predicting the development of disease symptoms was estimated as 20 pg (g soil)−1. In three strawberry greenhouses examined, the target DNA concentrations ranged from 1 to 1,655 pg (g soil)−1 for P. nicotianae and from 13 to 233 pg (g soil)−1 for P. cactorum. The method proved fast and reliable, and provides a useful tool to monitor P. nicotianae and P. cactorum in plants or soils.

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confidence: 99%

Simultaneous Detection and Quantification of Phytophthora nicotianae and P. cactorum, and Distribution Analyses in Strawberry Greenhouses by Duplex Real-time PCR

Inada

Watanabe³

et al. 2013

Microb. Environ.

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“…Some aspects of our existing TaqMan method (33), such as the run time and the complexity of the equipment required, are not ideally suited to on-site testing. The assay on which this work is based was itself adapted from a laboratory TaqMan assay (12) which is better suited to large-scale use in a routine diagnostic setting. The original assay uses "universal" thermal cycling conditions which are often used for TaqMan real-time PCR (many TaqMan primers and probes are designed to have melting temperatures which allow universal cycling conditions to be used).…”

Section: Discussionmentioning

confidence: 99%

“…P. ramorum-specific primers (Pram-114F and Pram-190R) and a TaqMan probe (Pram probe), designed based on the ITS sequence of a range of Phytophthora spp. as previously described (12), were used as the basis for the design of a duplex scorpion primer, molecular beacon, and alternative reverse primer (Pram-199R) (Fig. 1).…”

Section: Methodsmentioning

confidence: 99%

“…In particular, real-time PCR methods have the advantages of speed, accuracy, and sensitivity over other methods (7,28,30,43) and can be closedtube systems involving no postamplification steps. TaqMan (11,16) is the most widely used real-time PCR system, and assays using this detection chemistry have been described for a range of plant pathogens (3,4,14,39,38,40), including assays for the detection of Phytophthora ramorum both in the laboratory (8,12,34) and in the field (33). A single round of real-time PCR has been found to be sufficiently sensitive to achieve the detection of 10 to 100 fg P. ramorum DNA in plant material (8,33).…”

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confidence: 99%

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Faster, Simpler, More-Specific Methods for Improved Molecular Detection of Phytophthora ramorum in the Field

Tomlinson¹,

Barker²,

Boonham³

2007

Appl Environ Microbiol

138

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Phytophthora ramorum is the causal agent of sudden oak death. The pathogen also affects a wide range of tree, shrub, and herbaceous species in natural and landscaped environments as well as plants in the nursery industry. A TaqMan real-time PCR method for the detection of this pathogen in the field has been described previously; this paper describes the development of a number of assays based on this method which have various advantages for use in the field. A scorpion real-time PCR assay that is twice as fast as TaqMan was developed, allowing the detection of P. ramorum in less than 30 min. Also designed was a loop-mediated isothermal amplification (LAMP) assay, which allowed sensitive and specific detection of P. ramorum in 45 min using only a heated block. A positive reaction was identified by the detection of the LAMP product by color change visible to the naked eye.

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“…Many PCR assays were developed for P. ramorum (e.g. Tomlinson et al 2007;Bilodeau et al 2007;Tooley et al 2006;Martin et al 2004;Hughes et al 2006;Hayden et al 2006), to the point of causing some confusion in the international regulatory community as to which one should be routinely used. The international ring trial to evaluate several of these methods simultaneously with the same samples should become a model for other pathogens ).…”

Section: Diagnostics and Molecular Detectionmentioning

confidence: 99%

Fifty years of oomycetes—from consolidation to evolutionary and genomic exploration

Lévesque

2011

Fungal Diversity

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Transformative changes in biological sciences during the past 25 years have led to many significant advances in oomycete research. Before the last half century there were some hints that the oomycetes were related to some algae but it is now definitively demonstrated that they do not share an evolutionary path with kingdom Eumycota and are instead placed in a new kingdom Straminipila. Clarifying this once and for all has created many opportunities, but the rapid expansion of the research community has caused some fragmentation, probably much more so than in other groups of fungi because of a lack of a unifying forum for the members of the community working on issues such as taxonomy or phylogeny. Prior to the advent of molecular phylogenetics, mycologists working in zoosporic fungi were examining the ultrastructure of the zoospore, mainly focussing on the flagellar apparatus, and managed to generate phylogenies or define clades of zoospore producing fungi that remained for the most part valid after the advances in molecular biology. Comprehensive molecular phylogenies that have been published for some genera of the oomycetes have helped in recognising a large number of new species and in the development of a wide range of DNA-based diagnostic tools. The number of genomes available for this group is increasing rapidly, pushing further the discoveries of novel host-parasite interaction mechanisms in oomycetes. Some important plant diseases that were believed to be under control have re-emerged and many new diseases have appeared particularly in forestry and even in mammals. The research community has been able to respond rapidly and effectively to these new challenges. New ecological roles for the oomycetes were found in the suppression of plant diseases and reduction of plant invasineness in natural ecosystems. There are still many challenges ahead in the oomycete community, probably the most pressing one is to establish a robust tree of life foundation like the Assembling the Fungal Tree of Life initiative. The oomycete research community is dynamic and has put to very good use the many new technological advances.

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Development of a One-Step Real-Time Polymerase Chain Reaction Assay for Diagnosis of Phytophthora ramorum

Cited by 82 publications

References 28 publications

Simultaneous Detection and Quantification of <i>Phytophthora nicotianae</i> and <i>P. cactorum</i>, and Distribution Analyses in Strawberry Greenhouses by Duplex Real-time PCR

Simultaneous Detection and Quantification of <i>Phytophthora nicotianae</i> and <i>P. cactorum</i>, and Distribution Analyses in Strawberry Greenhouses by Duplex Real-time PCR

Faster, Simpler, More-Specific Methods for Improved Molecular Detection of Phytophthora ramorum in the Field

Fifty years of oomycetes—from consolidation to evolutionary and genomic exploration

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