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Development and validation of a 1 K sika deer
by
Xing, Xiumei
, Fan, Huanhuan
, Wang, Tianjiao
, Wang, Hongliang
, Liu, Huitao
, Li, Yang
, Dong, Yimeng
, Zhang, Ranran
, Shang, Liyuan
in
Analysis
/ Biological diversity
/ Deer
/ Diseases
/ Examinations
/ Genetic aspects
/ Growth
/ Single nucleotide polymorphisms
/ Validity
2021
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Development and validation of a 1 K sika deer
by
Xing, Xiumei
, Fan, Huanhuan
, Wang, Tianjiao
, Wang, Hongliang
, Liu, Huitao
, Li, Yang
, Dong, Yimeng
, Zhang, Ranran
, Shang, Liyuan
in
Analysis
/ Biological diversity
/ Deer
/ Diseases
/ Examinations
/ Genetic aspects
/ Growth
/ Single nucleotide polymorphisms
/ Validity
2021
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Do you wish to request the book?
Development and validation of a 1 K sika deer
by
Xing, Xiumei
, Fan, Huanhuan
, Wang, Tianjiao
, Wang, Hongliang
, Liu, Huitao
, Li, Yang
, Dong, Yimeng
, Zhang, Ranran
, Shang, Liyuan
in
Analysis
/ Biological diversity
/ Deer
/ Diseases
/ Examinations
/ Genetic aspects
/ Growth
/ Single nucleotide polymorphisms
/ Validity
2021
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Journal Article
Development and validation of a 1 K sika deer
2021
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Overview
China is the birthplace of the deer family and the country with the most abundant deer resources. However, at present, China's deer industry faces the problem that pure sika deer and hybrid deer cannot be easily distinguished. Therefore, the development of a SNP identification chip is urgently required. In this study, 250 sika deer, 206 red deer, 23 first-generation hybrid deer (F1), 20 s-generation hybrid deer (F2), and 20 third-generation hybrid deer (F3) were resequenced. Using the chromosome-level sika deer genome as the reference sequence, mutation detection was performed on all individuals, and a total of 130,306,923 SNP loci were generated. After quality control filtering was performed, the remaining 31,140,900 loci were confirmed. From molecular-level and morphological analyses, the sika deer reference population and the red deer reference population were established. The Fst values of all SNPs in the two reference populations were calculated. According to customized algorithms and strict screening principles, 1000 red deer-specific SNP sites were finally selected for chip design, and 63 hybrid individuals were determined to contain red deer-specific SNP loci. The results showed that the gene content of red deer gradually decreased in subsequent hybrid generations, and this decrease roughly conformed to the law of statistical genetics. Reaction probes were designed according to the screening sites. All candidate sites met the requirements of the Illumina chip scoring system. The average score was 0.99, and the MAF was in the range of 0.3277 to 0.3621. Furthermore, 266 deer (125 sika deer, 39 red deer, 56 F1, 29 F2,17 F3) were randomly selected for 1 K SNP chip verification. The results showed that among the 1000 SNP sites, 995 probes were synthesized, 4 of which could not be typed, while 973 loci were polymorphic. PCA, random forest and ADMIXTURE results showed that the 1 K sika deer SNP chip was able to clearly distinguish sika deer, red deer, and hybrid deer and that this 1 K SNP chip technology may provide technical support for the protection and utilization of pure sika deer species resources. We successfully developed a low-density identification chip that can quickly and accurately distinguish sika deer from their hybrid offspring, thereby providing technical support for the protection and utilization of pure sika deer germplasm resources.
Publisher
BioMed Central Ltd
Subject
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