2011
DOI: 10.1111/j.1365-3059.2011.02430.x
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Ditylenchus gigas n. sp. parasitizing broad bean: a new stem nematode singled out from the Ditylenchus dipsaci species complex using a polyphasic approach with molecular phylogeny

Abstract: Morphologial, biochemical, molecular and karyological analyses of different populations and races of the stem and bulb nematode Ditylenchus dipsaci have suggested that it represents a species complex, of which only D. dipsaci sensu stricto and its morphologically larger variant, known as the giant race of the stem and bulb nematode, are plant parasites of economic importance. The present study singles out the giant race from this complex, herein described as a new species named Ditylenchus gigas n. sp., on the… Show more

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Cited by 88 publications
(67 citation statements)
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References 31 publications
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“…from D. gigas, D. dipsaci and other known Ditylenchus species, and are congruent with previous findings (Subbotin et al, 2004(Subbotin et al, , 2005Chizhov et al, 2010;Vovlas et al, 2011;Oliveira et al, 2013). Although D. oncogenus n. sp.…”
Section: Molecular Characterization Of Ditylenchus Oncogenus N Spsupporting
confidence: 93%
“…from D. gigas, D. dipsaci and other known Ditylenchus species, and are congruent with previous findings (Subbotin et al, 2004(Subbotin et al, , 2005Chizhov et al, 2010;Vovlas et al, 2011;Oliveira et al, 2013). Although D. oncogenus n. sp.…”
Section: Molecular Characterization Of Ditylenchus Oncogenus N Spsupporting
confidence: 93%
“…In general, the definition of cryptic species is narrower. Some plant-parasitic nematodes cryptic species have been recognized, e.g., Ditylenchus dipsaci (Kühn 1857) Filipjev 1936and D. gigas Vovlas et al 2011(Vovlas et al 2011, P. f l o r i d e n s i s D e L u c a e t a l . 2 0 1 0 a n d P. parafloridensis De Luca et al 2010(De Luca et al 2010, P. coffeae (Zimmermann 1898) Filipjev and Schuurmans Stekhoven 1941and P. speijeri De Luca et al 2012(De Luca et al 2012.…”
Section: Discussionmentioning
confidence: 98%
“…La reacción de la PCR para los iniciadores D2A y D3B comprendió 5 µl de solución amortiguadora de PCR 10X, 3 µl de MgCl 2 50mM, 1 µl mix de DNTP´s 10mM, 2 µl de cada iniciador 10 µM, 0.5 µl de Taq polimerasa 5U/µl, 5 µl de extracción de ADN y 31.5 µl de H 2 O libres de ADNasas y ARNasas. Las condiciones de la amplificación fueron las siguientes: desnaturalización inicial de 95 °C durante 3 min, seguido de 35 ciclos de 95 °C durante 0.45 min, 55 °C durante 0.45 min y 72 °C durante 1 min, y finalmente con un ciclo a 72 °C durante 5 min (Vovlas et al, 2011). Se utilizó un termociclador i-Cycler (BIO-RAD) para todas las reacciones.…”
Section: A B C Dunclassified
“…The PCR reaction for primers D2A and D3B included 5 µl of PCR buffer solution 10X, 3 µl of MgCl 2 50mM, 1 µl mix of DNTP's 10mM, 2 µl of each initiator 10 µM, 0.5 µl of Taq polymerase 5U/µl, 5 µl of DNA extraction ADN and 31.5 µl of H 2 O, free of DNAses and RNAses. The conditions for the amplification were as follows: initial denaturation at 95 °C for 3 min, followed by 35 cycles at 95 °C for 0.45 min, 55 °C for 0.45 min, and 72 °C for 1 min, and finally, one cycle at 72 °C for 5 min (Vovlas et al, 2011). An i-Cycler (BIO-RAD) thermocycler was used for all reactions.…”
Section: A B C Dmentioning
confidence: 99%