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Multiplex PCR for identification of two butterfly sister species: Eurema mandarina and Eurema hecabe

机译:多重PCR用于鉴定两种蝴蝶姐妹种类:Eurema Mandarina和Eurema Hecabe

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摘要

Abstract Objective In insects, closely related species are often difficult or impossible to distinguish solely by morphological traits. Mitochondrial DNA (mtDNA) markers are often useful and reliable for distinguishing closely related species. However, useful mtDNA markers can be unavailable, particularly when such species pairs experienced hybrid introgression in the past. Although polymorphic nuclear DNA markers would be necessary to distinguish such species pairs, recombination, multiple copies, and slower mutation rates of the nuclear DNA compared with those of mtDNA often make it challenging. The objective of this study was to develop a multiplex polymerase chain reaction that can reliably amplify and distinguish the Tpi sequences of Eurema mandarina and Eurema hecabe. Results We successfully analyzed the nucleotide sequences of the Z chromosome-linked triose phosphate isomerase (Tpi) gene to develop a multiplex polymerase chain reaction (PCR) that amplified ca. 120-bp products for E. mandarina and ca. 375-bp products for E. hecabe. We suggest that multiplex PCR using Tpi with appropriately designed primers can be used to accurately and reliably distinguish between other closely related Lepidoptera species.
机译:摘要目的昆虫,密切相关的物种往往难以或不可能通过形态特征完全区分开来。线粒体DNA(mtDNA)标记往往是区分近缘种有用和可靠。然而,有用的线粒体DNA标记可以是不可用的,特别是当这些物种对经历了过去混合渗入。虽然多态性核DNA标记,有必要区分这些物种对,重组,多个副本,以及核DNA的慢突变率与线粒体DNA的比较往往成为一个难题。本研究的目的是开发一种多重聚合酶链式反应能够可靠地放大和区分黄粉蝶属桑蚕和黄蝶的TPI序列。结果我们成功地分析在Z染色体连锁的磷酸丙糖异构酶(TPI)基因的核苷酸序列来开发扩增约多重聚合酶链式反应(PCR) 120-bp的产物为E.桑蚕和约375-BP产品E. hecabe。我们建议使用TPI与适当设计引物的多重PCR可以用来精确地等密切相关鳞翅目可靠地区分。

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