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Discovery of 20,000 RAD-SNPs and development of a 52-SNP array for monitoring river otters

机译:发现了20,000种RAD-SNP,并开发了用于监测水獭的52-SNP阵列

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摘要

Many North American river otter (Lontra canadensis) populations are threatened or recovering but are difficult to study because they occur at low densities, it is difficult to visually identify individuals, and they inhabit aquatic environments that accelerate degradation of biological samples. Single nucleotide polymorphisms (SNPs) can improve our ability to monitor demographic and genetic parameters of difficult to study species. We used restriction site associated DNA (RAD) sequencing to discover 20,772 SNPs present in Montana, USA, river otter populations, including 14,512 loci that were also variable in at least one other population range-wide. After applying careful filtering criteria meant to minimize ascertainment bias and identify high quality, highly heterozygous (H (o) = 0.2-0.50) SNPs, we developed and tested 52 independent SNP qPCR genotyping assays, including 41 that performed well with diluted DNA. The 41 loci provided high power for population assignment tests with only 1 misassignment (1.6 %) between closely neighboring populations. Our SNPs showed high power to differentiate individuals and assign them to population of origin, as well as strong concordance of genotypes from high and diluted concentrations of DNA, and between original RAD and the SNP qPCR array.
机译:许多北美水獭(Lontra canadensis)种群正在受到威胁或正在恢复,但由于其密度低,难以从视觉上识别个体以及居住在水生环境中而加速了生物样品的降解,因此难以研究。单核苷酸多态性(SNP)可以提高我们监测难以研究的物种的人口统计和遗传参数的能力。我们使用限制酶切位点相关DNA(RAD)测序发现了在美国蒙大纳州的水獭种群中存在的20,772个SNP,包括14512个基因座,它们在至少一个其他种群范围内也是可变的。在应用了旨在最小化确定性偏倚并识别高质量,高度杂合(H(o)= 0.2-0.50)SNP的仔细过滤标准后,我们​​开发并测试了52个独立的SNP qPCR基因分型测定,其中41个在稀释的DNA上表现良好。这41个位点为人口分配测试提供了强大的功能,在紧密相邻的人口之间只有1个分配错误(1.6%)。我们的SNP具有很高的区分个体并将其分配给起源人群的能力,以及高浓度和稀释浓度的DNA以及原始RAD和SNP qPCR阵列之间的基因型高度一致。

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