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首页> 外文期刊>Annals of Applied Biology >Development of species-specific primers for the ectoparasitic nematode species Xiphinema brevicolle, X. diffusum, X. elongatum, X. ifacolum and X. longicaudatum (Nematoda: Longidoridae) based on ribosomal DNA sequences.
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Development of species-specific primers for the ectoparasitic nematode species Xiphinema brevicolle, X. diffusum, X. elongatum, X. ifacolum and X. longicaudatum (Nematoda: Longidoridae) based on ribosomal DNA sequences.

机译:根据核糖体DNA序列,开发用于外寄生线虫物种Xiphinema brevicolle,X。diffusum,X。elongatum,X。ifacolum和X. longicaudatum(Nematoda:Longidoridae)的物种特异性引物。

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摘要

The objective of this study was to develop single-step PCR species-specific primers that reliably discriminate four economically important Xiphinema species (X. brevicolle, X. elongatum, X. ifacolum and X. longicaudatum) and X. diffusum that is taxonomically very similar to X. brevicolle. Each species-specific reverse primer was located in the ITS-1 rDNA region and was used in combination with a universal forward primer located in the 18S rDNA gene. Primer reliability was confirmed by screening seven and 11 populations, respectively of X. diffusum and X. elongatum. Potential species-specific primers were also identified for X. brevicolle, X. longicaudatum and X. ifacolum, however too few populations of these species were available to thoroughly assess their reliability. For all species-specific primers, specificity was demonstrated by the absence of cross-reactions with 14 non-target Xiphinema species. Multiplex PCR was effective and reproducible for two (X. longicaudatum and X. ifacolum) or three (X. brevicolle, X. diffusum and X. elongatum) of the target nematode species, thus improving the applicability of the diagnostic primers.
机译:这项研究的目的是开发单步PCR物种特异性引物,该引物能够可靠地区分在分类学上非常相似的四种经济上重要的剑兰属物种(X. brevicolle,X。elongatum,X。ifacolum和X. longicaudatum)和X.扩散。到X. brevicolle。每个物种特异性的反向引物位于ITS-1 rDNA区域,并与位于18S rDNA基因中的通用正向引物结合使用。引物的可靠性通过分别筛选7个和11个弥漫性X.和长形X.种群来确认。还鉴定了潜在的物种特异引物,用于短小X.brevicolle,X.longicaudatum和X.ifacolum,但是这些物种的种群太少,无法全面评估其可靠性。对于所有物种特异性引物,通过与14种非目标Xiphinema物种之间没有交叉反应来证明其特异性。多重PCR对于靶线虫种类的两个(X. longicaudatum和X. ifacolum)或三个(X. brevicolle,X。diffusum和X. elongatum)有效且可重现,从而提高了诊断引物的适用性。

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