Parasitism effects on white clover by root-knot and cyst nematodes and molecular separation of Heterodera daverti from H. trifolii

Vovlas, N.; Vovlas, Alessio; Leonetti, Paola; Liébanas, Gracia; Castillo, Pablo; Subbotin, Sergei A.; Palomares-Rius, Juan E.

doi:10.1007/s10658-015-0735-3

Cited by 21 publications

(10 citation statements)

References 32 publications

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“…DNA sequence analysis (n=10) of two population was done at GenoTech Corporation (Dajeon, Korea). Outgroup taxa for each dataset was taken based on references from previous studies (Sekimoto et al, 2017; Subbotin et al, 2001; Vovlas et al, 2015). The newly obtained sequences of ITS rRNA and CO I gene were aligned using ClustalX 1.83 program with datasets of ‘Schachtii’ group species, registered in National center for biotechnology information.…”

Section: Methodsmentioning

confidence: 99%

“…The newly obtained sequences of ITS rRNA and CO I gene were aligned using ClustalX 1.83 program with datasets of ‘Schachtii’ group species, registered in National center for biotechnology information. Bayesian analysis of the sequence datasets was performed using MrBayes 3.1.2 (Kang et al, 2016; Sekimoto et al, 2017; Vovlas et al, 2015). The general time reversible substitution model (GTR+I+G) was chosen for this analysis and was run with four chains for 1 × 10 6 generations.…”

Section: Methodsmentioning

confidence: 99%

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Morphological and Molecular Characterization of Heterodera schachtii and the Newly Recorded Cyst Nematode, H. trifolii Associated with Chinese Cabbage in Korea

Mwamula

Kim

et al. 2018

Plant Pathol J

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Morphological and Molecular Characterization of Heterodera schachtii and the Newly Recorded Cyst Nematode, H. trifolii Associated with Chinese Cabbage in Korea

Mwamula

Kim

et al. 2018

Plant Pathol J

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“…For this reason, a qPCR assay based on the differences of another gene sequence was developed to discriminate between the Heterodera avenae group species ( H. avenae , H. filipjevi , and H. latipons ) by targeting the CO I gene (Toumi et al, 2013, 2015). Several studies have adopted the CO I gene for the DNA barcoding of the Heteroderidae family (Powers et al, 2018; Subbotin et al, 2018; Vovlas et al, 2015). According to Subbotin et al (2018), the CO I gene is a powerful barcoding marker because each species of Heterodera has a unique sequence.…”

Section: Discussionmentioning

confidence: 99%

“…Recently, research has been carried out in several countries on various diagnostic techniques for H . glycines using DNA barcode and quantitative PCR (qPCR); however, these techniques have not been studied in Korea (Vovlas et al, 2015; Ye, 2012). qPCR with species-specific primers can allow for the rapid diagnosis of H. glycines since the amplified results of the target sequences can be confirmed in real time and because the electrophoresis of PCR products is not necessary.…”

mentioning

confidence: 99%

Identification of Heterodera glycines (Tylenchida; Heteroderidae) Using qPCR

Kang

Eun-Hyoung

et al. 2019

Plant Pathol J

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“…Usually, several adjacent cells, not directly penetrated by the nematode stylet, exhibit cytological features such as a granulated cytoplasm with hypertrophied nuclei and nucleoli. These cells could be called nurturing cells and they proliferate amongst pith parenchyma and vascular bundles in some plants close to the feeding sites formed by the cavity within the gall (Watson and Shorthouse, 1979 ; Vovlas et al, 2015a ). Some authors as early as Goodey ( 1935 ), Krusberg ( 1961 ), and Watson and Shorthouse ( 1979 ), related this specific plant morphogenesis to the number of meristematic cells, as cortical parenchyma is associated with cell separation only, while meristematic cells are more commonly related with gall formation.…”

Section: Plant Morphogenesis Induced By Nematodesmentioning

confidence: 99%

Anatomical Alterations in Plant Tissues Induced by Plant-Parasitic Nematodes

et al. 2017

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Plant-parasitic nematodes (PPNs) interact with plants in different ways, for example, through subtle feeding behavior, migrating destructively through infected tissues, or acting as virus-vectors for nepoviruses. They are all obligate biotrophic parasites as they derive their nutrients from living cells which they modify using pharyngeal gland secretions prior to food ingestion. Some of them can also shield themselves against plant defenses to sustain a relatively long lasting interaction while feeding. This paper is centered on cell types or organs that are newly induced in plants during PPN parasitism, including recent approaches to their study based on molecular biology combined with cell biology-histopathology. This issue has already been reviewed extensively for major PPNs (i.e., root-knot or cyst nematodes), but not for other genera (viz. Nacobbus aberrans, Rotylenchulus spp.). PPNs have evolved with plants and this co-evolution process has allowed the induction of new types of plant cells necessary for their parasitism. There are four basic types of feeding cells: (i) non-hypertrophied nurse cells; (ii) single giant cells; (iii) syncytia; and (iv) coenocytes. Variations in the structure of these cells within each group are also present between some genera depending on the nematode species viz. Meloidogyne or Rotylenchulus. This variability of feeding sites may be related in some way to PPN life style (migratory ectoparasites, sedentary ectoparasites, migratory ecto-endoparasites, migratory endoparasites, or sedentary endoparasites). Apart from their co-evolution with plants, the response of plant cells and roots are closely related to feeding behavior, the anatomy of the nematode (mainly stylet size, which could reach different types of cells in the plant), and the secretory fluids produced in the pharyngeal glands. These secretory fluids are injected through the stylet into perforated cells where they modify plant cytoplasm prior to food removal. Some species do not produce specialized feeding sites (viz. Ditylenchus, Subanguina), but may develop a specialized modification of the root system (e.g., unspecialized root galls or a profusion of roots). This review introduces new data on cell types and plant organs stimulated by PPNs using sources varying from traditional histopathology to new holistic methodologies.

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Parasitism effects on white clover by root-knot and cyst nematodes and molecular separation of Heterodera daverti from H. trifolii

Cited by 21 publications

References 32 publications

Morphological and Molecular Characterization of Heterodera schachtii and the Newly Recorded Cyst Nematode, H. trifolii Associated with Chinese Cabbage in Korea

Morphological and Molecular Characterization of Heterodera schachtii and the Newly Recorded Cyst Nematode, H. trifolii Associated with Chinese Cabbage in Korea

Identification of Heterodera glycines (Tylenchida; Heteroderidae) Using qPCR

Anatomical Alterations in Plant Tissues Induced by Plant-Parasitic Nematodes

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