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Empowering conservation practice with efficient and economical genotyping from poor quality samples

机译:通过对劣质样品进行有效而经济的基因分型来加强保护实践

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摘要

class="enumerated" style="list-style-type:decimal" id="L2">Moderate- to high-density genotyping (100 + SNPs) is widely used to determine and measure individual identity, relatedness, fitness, population structure and migration in wild populations.However, these important tools are difficult to apply when high-quality genetic material is unavailable. Most genomic tools are developed for high-quality DNA sources from laboratory or medical settings. As a result, most genetic data from market or field settings is limited to easily amplified mitochondrial DNA or a few microsatellites.To enable genotyping in conservation contexts, we used next-generation sequencing of multiplex PCR products from very low-quality DNA extracted from faeces, hair and cooked samples. We demonstrated utility and wide-ranging potential application in endangered wild tigers and tracking commercial trade in Caribbean queen conch.We genotyped 100 SNPs from degraded tiger samples to identify individuals, discern close relatives and detect population differentiation. Co-occurring carnivores do not amplify (e.g. Indian wild dog/dhole) or are monomorphic (e.g. leopard). Sixty-two SNPs from conch fritters and field-collected samples were used to test relatedness and detect population structure.We provide proof of concept for a rapid, simple, cost-effective and scalable method (for both samples and number of loci), a framework that can be applied to other conservation scenarios previously limited by low-quality DNA samples. These approaches provide a critical advance for wildlife monitoring and forensics, open the door to field-ready testing, and will strengthen the use of science in policy decisions and wildlife trade.
机译:class =“ enumerated” style =“ list-style-type:decimal” id =“ L2”> <!-list-behavior =枚举前缀word = mark-type = decimal max-label-size = 0- -> 中度到高密度基因分型(100 + SNP)被广泛用于确定和测量野生种群中的个体身份,相关性,适应性,种群结构和迁移。 但是,这些重要当无法获得高质量的遗传材料时,很难使用这些工具。大多数基因组工具都是为从实验室或医疗机构获得高质量DNA来源而开发的。结果,来自市场或现场的大多数遗传数据仅限于容易扩增的线粒体DNA或少数微卫星。 为了在保护环境中实现基因分型,我们使用了从从粪便,头发和煮熟的样品中提取的低质量DNA。我们证明了在濒临灭绝的野生老虎中的实用性和广泛的潜在应用前景,并跟踪了加勒比海皇后海螺的商业交易。 我们从退化的老虎样本中对100个SNP进行了基因分型,以识别个体,辨别近亲并检测种群分化。共同出现的食肉动物不会扩增(例如印度野狗/洞),或者是单态的(例如豹子)。使用来自海螺油条和现场采集的样本的62个SNP来测试相关性和检测种群结构。 我们提供了一种快速,简单,经济高效且可扩展的方法(对于两个样本)的概念验证和基因座数量),该框架可应用于以前受低质量DNA样品限制的其他保护方案。这些方法为野生动植物的监测和取证提供了重要的进展,为现场测试提供了方便,并将在决策和野生动植物贸易中加强科学的应用。

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