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Molecular discrimination of toxic and non-toxic Alexandrium species (Dinophyta) in natural phytoplankton assemblages from the Scottish coast of the North Sea

机译:来自北海苏格兰海岸的天然浮游植物群落中有毒和无毒亚历山大藻(Dinophyta)的分子鉴别

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摘要

Molecular methods provide promising tools for routine detection and quantification of toxic microalgae in plankton samples. To this end, novel TaqMan minor groove binding probes and primers targeting the small (SSU) or large (LSU) ribosomal subunit (rRNA) were developed for two species of the marine dinoflagellate genus Alexandrium (A. minutum, A. tamutum) and for three groups/ribotypes of the A. tamarense species complex: Group I/North American (NA), Group II/Mediterranean (ME) and Group III/Western European (WE). Primers and probes for real-time quantitative PCR (qPCR) were speciesspecific and highly efficient when tested in qPCR assays for cross-validation with pure DNA from cultured Alexandrium strains. Suitability of the qPCR assays as molecular tools for the detection and estimation of relative cell abundances of Alexandrium species and groups was evaluated from samples of natural plankton assemblages along the Scottish east coast. The results were compared with inverted microscope cell counts (Utermo¨ hl technique) of Alexandrium spp. and associated paralytic shellfish poisoning (PSP) toxin concentrations. The qPCR assays indicated that A. tamarense (Group I) and A. tamutum were the most abundant Alexandrium taxa and both were highly positively correlated with PSP toxin content of plankton samples. Cells of A. tamarense (Group III) were present at nearly all stations but in low abundance. Alexandrium minutum and A. tamarense (Group II) cells were not detected in any of the samples, thereby arguing for their absence from the specific North Sea region, at least at the time of the survey. The sympatric occurrence of A. tamarense Group I and Group III gives further support to the hypothesis that the groups/ribotypes of the A. tamarense species complex are cryptic species rather than variants belonging to the same species.
机译:分子方法为常规检测和定量浮游生物样品中的有毒微藻提供了有前途的工具。为此,针对两种海洋鞭毛鞭毛藻亚历山大藻(A. minutum,A. tamutum)和针对两种物种的新型TaqMan小沟结合探针和针对小(SSU)或大(LSU)核糖体亚基(rRNA)的引物进行了开发。 tamarense物种复合体的三类/核型:I类/北美(NA),II类/地中海(ME)和III类/西欧(WE)。用于实时定量PCR(qPCR)的引物和探针在qPCR分析中与培养的Alexandrium菌株的纯DNA进行交叉验证时具有物种特异性和高效性。从苏格兰东海岸的天然浮游生物组合样本中评估了qPCR分析作为分子工具检测和评估亚历山大藻物种和群体的相对细胞丰度的适用性。将结果与亚历山大藻的倒置显微镜细胞计数(Utermohl技术)进行比较。以及相关的麻痹性贝类中毒(PSP)毒素浓度。 qPCR分析表明,塔玛链霉菌(第一类)和塔玛曲霉是最丰富的亚历山大类群,并且都与浮游生物样品中PSP毒素含量高度正相关。 tamarense(第三组)的细胞几乎存在于所有站中,但数量很少。在任何样品中均未检测到亚历山大细小球菌和塔玛色曲霉(第II组)细胞,因此至少在调查时就没有从特定的北海区域中发现它们。 tamarense A.组和III。a。共同发生的现象进一步支持了tamarense物种复合体的组/核型是隐性物种而不是属于同一物种的变体的假说。

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