Rapid identification of deer products by multiplex PCR assay |
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| Authors: | Dai-Ming Zha Xiu-Mei Xing Fu-He Yang |
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| Affiliation: | 1. Institute of Special Economic Animal and Plant Science, Chinese Academy of Agricultural Sciences, Jilin 132109, China;2. School of Biotechnology and Environmental Engineering, Jiangsu University of Science and Technology, Zhenjiang 212018, China;3. State Key Laboratory of Special Economic Animal Molecular Biology, Jilin 132109, China;4. Key Laboratory of Special Economic Animal Germplasm Resources and Genetic Improvement, Jilin 132109, China |
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| Abstract: | Attempts were made to establish one-step multiplex PCR assay for the identification of the widely used species in deer products (sika deer, wapiti, red deer and reindeer). Primers were designed from tandem repeat region of D-loop and well-conserved region of 16S rDNA after alignment of the available sequences in the GenBank database. The primers generated specific fragments of 307 bp in length for sika deer, 307 and 246 bp for wapiti, 272 bp for Tarim red deer, 230 bp for red deer and 141 bp for reindeer, respectively. The detection limit was 0.05 ng for sika deer and wapiti, 0.1 ng for Tarim red deer, 0.5 ng for red deer and 0.02 ng for reindeer. The results demonstrated that the fraudulent phenomenon is epidemic in the substitution of deer products, in especially antler, penis, foetus and tendon products. Hence, this multiplex PCR provided a useful and sensitive technique to identify the sources of deer products. |
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| Keywords: | Multiplex PCR Deer products Species identification D-loop region 16S rDNA |
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