Determination of relative proportions of <i>Globodera</i> species in mixed populations of potato cyst nematodes using PCR product melting peak analysis

Bates, J. A.; Taylor, E. J. A.; Gans, P. T.; Thomas, Jane

doi:10.1046/j.1364-3703.2002.00107.x

Cited by 35 publications

(17 citation statements)

References 5 publications

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“…However, they are impractical for use in a phytosanitary/quarantine environment as the methodologies are time-consuming relative to single-step PCR tests, thus consequently more expensive in terms of both human and financial resources. In the future, quantification PCR assays will be utilised but there are currently few such protocols for nematodes (Bates et al, 2002;Holeva et al, 2002).…”

Section: Discussionmentioning

confidence: 98%

Validation of the specificity and sensitivity of species-specific primers that provide a reliable molecular diagnostic for Xiphinema diversicaudatum, X. index and X. vuittenezi

Hübschen

Kling

Ipach

et al. 2004

European Journal of Plant Pathology

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Xiphinema diversicaudatum and X. index are vector nematode species of economic importance in viticulture regions as they can transmit Arabis Mosaic, Grapevine Fanleaf and Strawberry Latent Ringspot viruses to grapevine. Wang et al. (2003) designed species-specific diagnostic primers from ribosomal genes for both these vector species as well as a vector and a non-vector species X. italiae and X. vuittenezi, respectively. Our study aimed to confirm the specificity and determine the sensitivity and reliability of the primers for the two vector species, X. diversicaudatum and X. index when challenged with closely related longidorid species and general nematode communities typical of vineyard soil. With one exception, no PCR product was observed when the primers were tested against six Longidorus, one Paralongidorus and one Xiphinema non-target species. Occasionally (three out of eight replicate PCR reactions) a weak PCR product was noted when primers for X. index were tested with L. elongatus. Furthermore, when challenged with a range of nontarget nematode species comprising the nematode community typical of viticulture soil, no PCR product was amplified. An experimental dilution series of extracted DNA rigorously demonstrated that DNA from an equivalent single specimen of the target virus-vector species, X. diversicaudatum and/or X. index, could be detected amongst 1000 equivalent non-target X. vuittenezi. Also, extracted DNA from an equivalent single target specimen was detected when added to DNA extracted from the overall soil nematode community. The primers were assessed further by using serial mixtures of actual nematodes rather than extracted DNA to simulate field soil. Using this method, a single target nematode could be detected amongst 200 non-target specimens. Given their specificity, sensitivity and reliability, it appears that these diagnostic primers will be of great benefit to phytosanitary/quarantine services related to the viticulture industry.

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Section: Discussionmentioning

confidence: 98%

Validation of the specificity and sensitivity of species-specific primers that provide a reliable molecular diagnostic for Xiphinema diversicaudatum, X. index and X. vuittenezi

Hübschen

Kling

Ipach

et al. 2004

European Journal of Plant Pathology

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“…Various ITS-based molecular methods including recently developed qPCR assays have been proven to be valuable for identifying Globodera species (Bates et al 2002;Madani et al 2008). Although these qPCR assays offer rapid, specific, and sensitive detection, they utilize limited nucleotide polymorphisms for species differentiation.…”

Section: Discussionmentioning

confidence: 99%

“…Molecular diagnostic methods utilizing ribosomal DNA (rDNA) sequences have been developed for identifying these three important Globodera species (Bates et al 2002;Bulman and Marshall 1997;Madani et al 2008;Skantar et al 2007;Thiéry and Mugniéry 1996). The species-specific PCR primers developed by Bulman and Marshall (1997) have been found to be useful in differentiating PCN species and species-specific PCR primers for TCN identification were also recently made available (Skantar et al 2007).…”

Section: Introductionmentioning

confidence: 99%

“…The species-specific PCR primers developed by Bulman and Marshall (1997) have been found to be useful in differentiating PCN species and species-specific PCR primers for TCN identification were also recently made available (Skantar et al 2007). More recently, quantitative real-time PCR (qPCR) assays that include melting curve analysis of PCR products or TaqMan technology utilizing locked nucleic acids (LNA)-modified primers and probes, have been developed for identifying Globodera species (Bates et al 2002;Madani et al 2008). qPCR-based diagnostics offer rapid, specific, and sensitive detection compared to conventional PCR assays that require post-PCR gel analysis.…”

Section: Introductionmentioning

confidence: 99%

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Chorismate mutase: an alternatively spliced parasitism gene and a diagnostic marker for three important Globodera nematode species

Chronis

et al. 2010

Eur J Plant Pathol

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The chorismate mutase gene is widely distributed in both cyst and root-knot nematode species and believed to play a critical role in nematode parasitism. In this study, we cloned a new chorismate mutase gene (Gt-cm-1) from Globodera tabacum and further characterized the gene structure in both G. tabacum and G. pallida, a closely related species of G. rostochiensis. The genomic clones of chorismate mutase genes from these two species were found to contain three introns with the second intron having unusual 5' and 3' splice sites. A previous study revealed that the chorismate mutase gene from G. rostochiensis is subject to alternative splicing through retention of intron 2, a process that allows for the generation of multiple mRNA transcripts from a single gene. As expected, we discovered that alternative splicing of the chorismate mutase gene is a conserved event in three Globodera species, supporting an important role of alternative splicing in regulating chorismate mutase gene function in plant parasitism by these nematodes. In addition to the potential suboptimal 5' and 3' splice sites and the small size of intron 2, detailed sequence analysis also identified candidate cis-acting elements that might be responsible for regulating intron retention of Globodera chorismate mutase genes. Based on genomic sequence variations observed, we developed TaqMan qPCR assays that provided a highly specific and sensitive identification of each Globodera species, revealing a new application of using the chorismate mutase gene as a valuable diagnostic marker for plant-parasitic nematodes.

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“…A multiplex PCR was presented by Bulman and Marshal, (Figure 2), when species-speciic primers were used and combined with mixed populations of PCNs [17]. A few years later, the PCR method was named conventional PCR (CoPCR) due the appearance of quantitative real-time PCR (qPCR) [21].…”

Section: Ribosomal Dna Polymerase Chain Reaction (Rdna-pcr)mentioning

confidence: 99%

Molecular Diagnostic Tools for Nematodes

Christoforou¹,

Orford²,

Tsaltas³

2017

Nematology - Concepts, Diagnosis and Control

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Determination of relative proportions of Globodera species in mixed populations of potato cyst nematodes using PCR product melting peak analysis

Cited by 35 publications

References 5 publications

Validation of the specificity and sensitivity of species-specific primers that provide a reliable molecular diagnostic for Xiphinema diversicaudatum, X. index and X. vuittenezi

Validation of the specificity and sensitivity of species-specific primers that provide a reliable molecular diagnostic for Xiphinema diversicaudatum, X. index and X. vuittenezi

Chorismate mutase: an alternatively spliced parasitism gene and a diagnostic marker for three important Globodera nematode species

Molecular Diagnostic Tools for Nematodes

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