2011
DOI: 10.1007/s11427-011-4184-8
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DNA barcoding of the fungal genus Neonectria and the discovery of two new species

Abstract: To determine a suitable DNA barcode for the genus Neonectria, the internal transcribed spacer rDNA, β-tubulin, EF-1α, and RPB2 genes were selected as candidate markers. A total of 205 sequences from 19 species of the genus were analyzed. Intraand inter-specific divergences and the ease of nucleotide sequence acquisition were treated as criteria to evaluate the feasibility of a DNA barcode. Our results indicated that any single gene among the candidate markers failed to serve as a successful barcode, while the … Show more

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Cited by 19 publications
(15 citation statements)
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“…The current study also supports the treatment of these two taxa as the same species. The species identification performance of EF-1α (84.6%) in this work was comparable with a previous identification rate of 89.5% in the genus Neonectria in Ascomycota (Zhao et al, 2011b); however, it was inferior to a previous 100% identification rate for the seven species of Pleurotus (Li et al, 2017), probably because of the greater sampling range in this study.…”
Section: Discussionsupporting
confidence: 73%
“…The current study also supports the treatment of these two taxa as the same species. The species identification performance of EF-1α (84.6%) in this work was comparable with a previous identification rate of 89.5% in the genus Neonectria in Ascomycota (Zhao et al, 2011b); however, it was inferior to a previous 100% identification rate for the seven species of Pleurotus (Li et al, 2017), probably because of the greater sampling range in this study.…”
Section: Discussionsupporting
confidence: 73%
“…In general, the PCR success rates were lower than those found by other authors (Zhao et al . , ; Schoch et al . ).…”
Section: Discussionmentioning
confidence: 99%
“…The two vital conditions for DNA barcode evaluation are sufficient intra-and inter-specific variation, as well as high PCR and sequencing success rates (Zhao et al 2011a(Zhao et al , 2011bZeng 2012;Zhu et al 2014). Taking both these standards into consideration, the use of ITS was considered to be an adequate primary Russula DNA barcode in situations of single gene analysis.…”
Section: Discussionmentioning
confidence: 99%