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Molecular attempt to identify prey organisms of lobster phyllosoma larvae

机译:分子尝试鉴定龙虾叶状体幼虫的猎物生物

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A molecular approach was adopted to investigate the natural diets of palinurid and scyllarid lobster phyllosoma larvae. The central domain of the 18S rDNA gene was amplified using nested polymerase chain reaction (PCR) and genomic DNA extracted from the larval hepatopancreas. The resulting 18S rDNA clones were screened using restriction fragment length polymorphism (RFLP) analysis, and then FASTA homology search and phylogenetic analysis were performed on the nucleotide sequences to identify the source of the eukaryotic organisms. The feasibility of this method was confirmed using the laboratory-reared phyllosoma larvae of the Japanese spiny lobster Panulirus jap onicus that were fed either with common mussel Mytilus edulis gonads or with Artemia nauplii exclusively. Among the 804 clones isolated from five wild-caught mid-to late-stage phyllosoma larvae (three palinurids and two scyllarids), 0–132 clones per sample possessed restriction profiles distinct from those of the hosts. The Cnidaria and Urochordata DNA were identified from both the palinurid and the scyllarid larvae, which were thought to be prey animals for the mid- to late-stage phyllosoma larvae.
机译:采用分子方法研究了lin仁和圆须龙虾叶状体幼虫的自然饮食。使用巢式聚合酶链反应(PCR)和从幼虫肝胰腺提取的基因组DNA扩增18S rDNA基因的中央结构域。使用限制性片段长度多态性(RFLP)分析筛选所得的18S rDNA克隆,然后对核苷酸序列进行FASTA同源性搜索和系统发育分析,以鉴定真核生物的来源。该方法的可行性已通过实验室饲养的日本刺龙虾Panulirus jap onicus的叶状幼体得到了证实,该幼虫与普通贻贝的Mytilus edulis性腺或仅与Artemia nauplii一起饲养。从五个野生的中晚期晚期phyllosoma幼虫(三个变态和两个鞘状幼虫)中分离出的804个克隆中,每个样品的0-132个克隆具有与宿主不同的限制性谱。从pa虫和幼虫中都鉴定出了刺鼻和Urochordata DNA,它们被认为是中晚期食虫幼虫的捕食动物。

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