Abstract
BackgroundCharacterization of molecular markers and the development of better assays for precise and rapid detection of wildlife species are always in demand. This study describes a set of seven novel heminested PCR assays using specific primers designed based on species-specific polymorphism at the mitochondrial 16S rRNA gene for identification of Blackbuck, Goral, Nilgai, Hog deer, Chital, Sambar and Thamin deer.ResultsThe designed heminested PCR assays are two consecutive amplifications of the mitochondrial 16S rRNA gene. In the first stage, ~550 bp region of the 16S rRNA gene was amplified by PCR using template DNA and universal primers. In the second stage, a species-specific internal region of the 16S rRNA gene was amplified by PCR using the amplicon of the first PCR along with one universal primer and another species-specific primer as the reverse or forward primer. The amplicon generated after two consecutive amplifications was highly unique to target species. These assays were successfully validated for sensitivity, specificity, and ruggedness under a wide range of conditions.ConclusionThe validation experiments confirm that the designed heminested PCR assays for identification of the seven species are highly specific, sensitive, reliable and provide a reproducible method allowing analysis of low copy number DNA recovered from decomposed or highly processed tissues. The assays for identification of other species could be devised by extrapolating the principle of designed heminested PCR.
Highlights
Characterization of molecular markers and the development of better assays for precise and rapid detection of wildlife species are always in demand
We report a set of seven novel heminested PCR assays based on the amplification of a species-specific internal sequence region of mitochondrial 16s rRNA gene for identification of the species Blackbuck, Goral, Nilgai, Chital, Thamin, Sambar and Hog deer with their respective specific primers
In this study we have designed and validated seven novel heminested mitochondrial 16s rRNA gene-targeted PCR assays for identification of seven species using designed species-specific primers listed in table 1
Summary
Characterization of molecular markers and the development of better assays for precise and rapid detection of wildlife species are always in demand. This study describes a set of seven novel heminested PCR assays using specific primers designed based on species-specific polymorphism at the mitochondrial 16S rRNA gene for identification of Blackbuck, Goral, Nilgai, Hog deer, Chital, Sambar and Thamin deer. Characterization of species-specific molecular markers and designing of species-specific assays for identification of wildlife species are essential to prevent illegal trade of parts and products for better conservation and management of endangered species. Bone, horn, tail-hair, meat, antlers of Pecora family prevalent in India and have considerable trading value worldwide [1]. The protected members of Pecora family extensively hunted in India, e.g. Blackbuck, Goral, Nilgai, Chital, Thamin, Sambar, Hog deer, and Musk deer. The Cervidae family comprises (page number not for citation purposes)
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