Your search keyword '"m-chitwoodi"' showing total 4 results

1. A real-time PCR assay to identify Meloidogyne minor

Subjects

m-chitwoodi, ribosomal intergenic spacer, Bioint Moleculair Phytopathology, hapla, nematodes, identification, m-fallax, dna

Abstract

Meloidogyne minor is a small root-knot nematode that causes yellow patch disease in golf courses and severe quality damage in potatoes. It was described in 2004 and has been detected in The Netherlands, England, Wales, Northern Ireland, Ireland and Belgium. The nematode often appears together with M. naasi on grasses. It causes similar symptoms on potato tubers as M. chitwoodi and M. fallax, which are both quarantine organisms in Europe. An accurate identification method therefore is required. This study describes a real-time PCR assay that enables the identification of M. minor after extraction of nematodes from soil or plant samples. Alignments of sequences of rDNA-ITS fragments of M. minor and five other Meloidogyne species were used to design a forward primer Mminor_f299, a specific primer Mminor_r362 and the specific MGB TaqMan probe P_Mm_MGB321. PCR with this primers and probe results in an amplicon of 64 bp. The analytical specificity of the real-time PCR assay was assessed by assaying it on six populations of M. minor and on 10 populations of six other Meloidogyne species. Only DNA from M. minor gave positive results in this assay. The assay was able to identify M. minor using DNA from a single juvenile independent from the DNA extraction method used

Published

2011

2. Identification of Meloidogyne incognita, M. javanica and M. arenaria using sequence characterised amplified region (SCAR) based PCR assays

Author

C. Zijlstra, Dorine T.H.M. Donkers-Venne, and Mireille Fargette

Subjects

genus meloidogyne, major meloidogyne, differentiate, identify, polymorphism, law.invention, m-chitwoodi, DIAGNOSTIC, law, mitochondrial-dna, Botany, TECHNIQUE PCR, ETUDE COMPARATIVE, Meloidogyne incognita, root-knot nematodes, Ecology, Evolution, Behavior and Systematics, Polymerase chain reaction, METHODE D'ANALYSE, IDENTIFICATION, biology, Bioint Moleculair Phytopathology, TECHNIQUE RAPD, populations, biology.organism_classification, Molecular biology, RAPD, NEMATODE PHYTOPARASITE, Genetic marker, Meloidogyne arenaria, hapla, ETUDE EXPERIMENTALE, Agronomy and Crop Science, Terra incognita, Meloidogyne javanica, Specific identification

Abstract

Three randomly amplified polymorphic DNA (RAPD) markers, OPA-12420, OPB-061200 and OPA-01700, species specific to the root-knot nematode species Meloidogyne arenaria, M. incognita and M. javanica respectively, were identified. After sequencing these RAPD-PCR products, longer primers of 18 to 23 nucleotides were designed to complement the terminal DNA sequences of the DNA fragments. This resulted in three pairs of species specific primers that were used to amplify the sequence characterised amplified regions (SCARs). The developed sets of SCAR primers were successfully used in straightforward, fast and reliable PCR assays to identify M. incognita, M. javanica and M. arenaria. The length variant SCAR markers can be amplified from DNA from egg masses, second stage juveniles and females. This species identification technique is therefore independent of the nematode's life cycle stage. Moreover the SCAR-PCR assay was successfully applied using DNA extracts from infested plant material. The method has potential to be optimised for routine practical diagnostic tests facilitating the control of these economically important pest organisms. Identification de Meloigyne incognita, M. javanica et M. arenaria au moyen de l'amplification de régions de séquences caractéristiques (SCAR) par une technique PCR - Trois marqueurs d'ADN polymorphique amplifiée au hasard (RAPD) OPA-12420, OPB-O61200 et OPA-OI700, respectivement spécifiques des espèces de nématodes Meloidogyne arenaria, M. incognita et M. javanica, ont été identifiés. Après le séquençage de ces produits RAPD-PCR, les amorces les plus longues de 18 à 23 nucléotides ont été choisies pour compléter les séquences terminales d'ADN des fragments d'ADN. Cela a conduit à trois paires d'amorces spécifiques de l'espèce, utilisées pour amplifier les régions des séquences caractéristiques (SCAR). Les lots d'amorces SCAR mis au point ont été utilisés avec succès lors d'essais directs, rapides et surs pour identifier M. incognita, M. javanica et M. arenia. Les marqueurs peuvent être amplifiés à partir de l'ADN des masses d'oeufs, des juvéniles de deuxième stade ou des femelles. Cette technique d'identification spécifique est donc indépendante des différents états de développement du nématode. De plus la technique SCAR-PCR a été appliquée avec succès à l'ADN extrait du matériel végétal infesté. Cette méthode présente des potentialités d'amélioration permettant d'envisager des tests pratiques d'identification de routine, facilitant ainsi le contrôle de ces parasites économiquement importants.

Published

2000

3. A real-time PCR assay to identify Meloidogyne minor

Author

de Weerdt, M., Kox, L., Wayenberge, L., Viaene, N., and Zijlstra, C.

Subjects

m-chitwoodi, ribosomal intergenic spacer, Bioint Moleculair Phytopathology, hapla, nematodes, identification, m-fallax, dna

Abstract

Meloidogyne minor is a small root-knot nematode that causes yellow patch disease in golf courses and severe quality damage in potatoes. It was described in 2004 and has been detected in The Netherlands, England, Wales, Northern Ireland, Ireland and Belgium. The nematode often appears together with M. naasi on grasses. It causes similar symptoms on potato tubers as M. chitwoodi and M. fallax, which are both quarantine organisms in Europe. An accurate identification method therefore is required. This study describes a real-time PCR assay that enables the identification of M. minor after extraction of nematodes from soil or plant samples. Alignments of sequences of rDNA-ITS fragments of M. minor and five other Meloidogyne species were used to design a forward primer Mminor_f299, a specific primer Mminor_r362 and the specific MGB TaqMan probe P_Mm_MGB321. PCR with this primers and probe results in an amplicon of 64 bp. The analytical specificity of the real-time PCR assay was assessed by assaying it on six populations of M. minor and on 10 populations of six other Meloidogyne species. Only DNA from M. minor gave positive results in this assay. The assay was able to identify M. minor using DNA from a single juvenile independent from the DNA extraction method used

Published

2011

4. A PCR test to detect the cereal root-knot nematode Meloidogyne naasi

Author

Richard Van hoof, Dorine T.H.M. Donkers-Venne, and C. Zijlstra

Subjects

differentiate, m-hapla, Plant Science, Horticulture, Meloidogyne naasi, Crop, m-chitwoodi, ribosomal intergenic spacer, Pcr test, Root-knot nematode, Forward primer, Biointeracties and Plant Health, biology, business.industry, Crop rotation, biology.organism_classification, Experimental research, Biotechnology, Nematode, mixtures, Agronomy, PRI Biointeractions en Plantgezondheid, identification, m-fallax, business, Agronomy and Crop Science

Abstract

The cereal root-knot nematode Meloidogyne naasi can cause serious cereal crop losses. The nematode is also found in agricultural fields where non-host crops are grown. Control of M. naasi can be based on preventing its spread, host resistance and crop management as well as on the design of crop rotation systems. Detection methods are required for these purposes and can also be helpful for inspection services and experimental research. This study describes the development of a simple PCR test that enables the detection of M. naasi. Alignment of sequences of rDNA-ITS fragments of M. naasi and five other Meloidogyne species was used to design the M. naasi specific forward primer N-ITS. Together with the reverse primer R195 M. naasi specific amplification was achieved.

Published

2004