Direct molecular detection of the pinewood nematode, Bursaphelenchus xylophilus, from pine wood, bark and insect vector

Cardoso, Joana M. S.; Fonseca, Luís; Abrantes, Isabel

doi:10.1007/s10658-011-9915-y

Cited by 30 publications

(38 citation statements)

References 27 publications

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“…Although this satDNA family has been recurrently used for species diagnosis (François et al, 2007;Cardoso et al, 2012), the available information regarding the structure and variation of this satDNA family is still scantily studied (Tarès et al, 1993;Castagnone-Sereno et al, 2008). Despite the recent release of the genome sequence of B. xylophilus (Kikuchi et al, 2011), no output was provided for such highly repetitive regions.…”

Section: Introductionmentioning

confidence: 99%

Sequence variability of the MspI satellite DNA family of the pinewood nematode Bursaphelenchus xylophilus at different geographic scales

Vieira

Castagnone

Mallez

et al. 2014

Molecular Phylogenetics and Evolution

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a b s t r a c tTandemly repeated sequences known as satellite DNA (satDNA) generally exhibit complex evolutionary patterns of concerted evolution in which mutations are homogenized and fixed in a stochastic process of molecular drive. Here, the nucleotidic variability of the MspI satDNA family of the pinewood nematode Bursaphelenchus xylophilus is analyzed in order to understand the evolutionary dynamics of satDNA at the intraspecific level. A total of 425 MspI monomer units, either PCR-amplified from isolates of local (Peninsula of Setúbal, Portugal) or worldwide origin, or retrieved from the B. xylophilus genome sequence, were characterized and compared. Whatever their origin, sliding window analysis of sequence variability patterns among monomers revealed low, moderate and highly variant domains, indicating that variable levels of evolutionary constraint may act upon the entire monomers. The phylogenetic inference based on the different sets of MspI satDNA family for this species shows a broad polymorphism of the individual monomers, which were distributed into four main clusters. However, such clustering appeared independent from the geographic origin of the nematodes, and could not discriminate isolates or groups of geographically close isolates. Rather, the formation of different phylogenetic groups within this satDNA family suggests an a priori embodying of a set of diverging repeats from a common ancestor satDNA library, which have been differently amplified along the evolutionary pathway of this species. The present work improves knowledge on the evolutionary dynamics of satDNA at the intraspecific level, and provides new information on satDNA sequence variability among natural populations sampled at a local geographic scale.

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Section: Introductionmentioning

confidence: 99%

Sequence variability of the MspI satellite DNA family of the pinewood nematode Bursaphelenchus xylophilus at different geographic scales

Vieira

Castagnone

Mallez

et al. 2014

Molecular Phylogenetics and Evolution

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“…Additionally, PWN morphological identification can sometimes be difficult or impossible when only juvenile stages are detected or owing to the variation in the female tail of some isolates (Fonseca et al, 2008). Therefore, several molecular methods have been developed that frequently use species-specific primers by targeting several genomic regions such as satellite DNA (Castagnone et al, 2005;Cardoso et al, 2012), the heat shock protein 70 gene (Leal et al, 2005(Leal et al, , 2007, the topoisomerase I gene (Huang et al, 2010), and internal transcribed spacer (ITS) regions of ribosomal DNA (rDNA) (Cao et al, 2005;Takeuchi et al, 2005) or by using nonspecific primers for polymerase chain reaction (PCR) amplification of the ITS regions and subsequent analysis with restriction fragment length polymorphism (RFLP) (Iwahori et al, 2000;Burgermeister et al, 2009). The ITS regions are located between the repeating array of nuclear 18S, 5.8S, and 28S ribosomal RNA genes and have 100-200 copies/genome.…”

Section: Introductionmentioning

confidence: 99%

Genetic diversity of ITS sequences of Bursaphelenchus xylophilus

Cardoso

Fonseca²,

Abrantes³

2012

Genet. Mol. Res.

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ABSTRACT. The sequence variation of internal transcribed spacer (ITS) regions of ribosomal DNA has been routinely used for species identification and species-level phylogeny of the pinewood nematode, Bursaphelenchus xylophilus. In this study, the intraspecies ITS genetic diversity of B. xylophilus was evaluated. Three pinewood nematode isolates from the United States, Japan, and Portugal were used for polymerase chain reaction (PCR) ITS region amplification and sequencing. Multiple peaks were observed in sequencing chromatograms from ITS regions of American and Japanese isolates, suggesting the presence of more than one ribosomal sequence for each isolate. PCR products were further cloned and 10 clones of each isolate were subsequently sequenced. Additionally, the ITS regions of individual nematodes from each isolate were amplified, cloned and sequenced. Among the 3 B. xylophilus isolates analyzed, an intraspecific and intra-isolate molecular variability was found. The intra-isolate ITS molecular diversity in the American isolate was higher than that in the Japanese and Portuguese isolates. However, the level of sequence variation observed within isolates was about the same as that described among ITS repeats within individuals.

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“…Several gDNA extraction methods using CTAB buffer, Chelex-100 resin and proteinase K have been developed for extracting total gDNA from B. xylophilus in infected pinewood (Cardoso et al, 2012;Francois et al, 2007;Hu et al, 2011;Kikuchi et al, 2009;Takeuchi et al, 2005). These methods, however, take a long time and the processes includes freezing, boiling, precipitation and filtering to increase extraction efficiency of gDNA extraction (Gou et al, 2015;Kikuchi et al, 2009;Takeuchi & Futai, 2007).…”

Section: Discussionmentioning

confidence: 99%

“…Identification of Bursaphelenchus species based on the morphological characteristics is therefore problematic. Some of the methods were attractive since they are not using Baermann funnel method and are extracting gDNA of B. xylophilus directly from the wood samples using various gDNA extraction buffer such as CTAB, Chelex-100 and proteinase K (Cardoso et al, 2012;Hu et al, 2011;Kikuchi et al, 2009;Takeuchi et al, 2005). such as several PCR, quantitative real-time PCR and loop-mediated isothermal amplification (LAMP) based methods with species-specific primers by targeting either rDNA-ITS (Iwahori et al, 2000;Kikuchi, Aikawa, Oeda, Karim, & Kanzaki, 2009;Takeuchi, Kanzaki, & Futai, 2005), rDNA-IGS (Kang et al, 2004), hsp70 (Leal, Green, Allen, Humble, & Rott, 2007), satDNA (Cardoso, Fonseca, & Abrantes, 2012;Castagnone, Abad, & Castagnone-Sereno, 2005;Francois et al, 2007), DNA topoisomerase I (Huang et al, 2010), pectate lyase 3 (Kang, Kim, Han, Moon, & Koh, 2015) and expansin-like gene (Leal et al, 2015).…”

Section: Introductionmentioning

confidence: 99%

A new on‐site detection method for Bursaphelenchus xylophilus in infected pine trees

et al. 2019

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The pinewood nematode (PWN), Bursaphelenchus xylophilus, is the causal agent of pine wilt disease (PWD), which is a major problem in East Asia and West Europe. Quick identification of PWN is needed to prevent the dispersal of PWD to healthy forests. Various detection methods of PWN have been developed using anatomical characters and molecular markers. These methods are not suitable for rapid diagnosis because it is difficult to distinguish B. xylophilus from the non‐pathogenic species Bursaphelenchus mucronatus based on morphological characters without expertise in nematode taxonomy and most PCR or isothermal amplification detection methods require time‐consuming processes. In this study, we developed an on‐site PWN detection method using a recombinase polymerase amplification (RPA) assay with a novel extraction buffer (DAP buffer). This new PWN detection method is able to extract genomic DNA from PWN in pinewood by simple buffer consisting of sodium hydrate, polyethylene glycol 200 and dimethyl sulfoxide in 10 min without using the experimental devices and able to distinguish between B. xylophilus and other Bursaphelenchus spp. by amplifying the species‐specific 5S rDNA fragment of B. xylophilus in 10 min. Taken together, our protocol can obtain the result for the detection of PWN in pine tree samples within 30 min. This result suggests that RPA/DAP assay is much faster, easier and cheaper than the conventional methods for detecting PWN.

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Direct molecular detection of the pinewood nematode, Bursaphelenchus xylophilus, from pine wood, bark and insect vector

Cited by 30 publications

References 27 publications

Sequence variability of the MspI satellite DNA family of the pinewood nematode Bursaphelenchus xylophilus at different geographic scales

Sequence variability of the MspI satellite DNA family of the pinewood nematode Bursaphelenchus xylophilus at different geographic scales

Genetic diversity of ITS sequences of Bursaphelenchus xylophilus

A new on‐site detection method for Bursaphelenchus xylophilus in infected pine trees

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