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用于群体研究的灵活且可扩展的测序基因分型策略。

Flexible and scalable genotyping-by-sequencing strategies for population studies.

作者信息

Heffelfinger Christopher, Fragoso Christopher A, Moreno Maria A, Overton John D, Mottinger John P, Zhao Hongyu, Tohme Joe, Dellaporta Stephen L

机构信息

Department of Molecular, Cellular, and Developmental Biology, Yale University, New Haven, CT 06511, USA.

出版信息

BMC Genomics. 2014 Nov 18;15(1):979. doi: 10.1186/1471-2164-15-979.

Abstract

BACKGROUND

Many areas critical to agricultural production and research, such as the breeding and trait mapping in plants and livestock, require robust and scalable genotyping platforms. Genotyping-by-sequencing (GBS) is a one such method highly suited to non-human organisms. In the GBS protocol, genomic DNA is fractionated via restriction digest, then reduced representation is achieved through size selection. Since many restriction sites are conserved across a species, the sequenced portion of the genome is highly consistent within a population. This makes the GBS protocol highly suited for experiments that require surveying large numbers of markers within a population, such as those involving genetic mapping, breeding, and population genomics. We have modified the GBS technology in a number of ways. Custom, enzyme specific adaptors have been replaced with standard Illumina adaptors compatible with blunt-end restriction enzymes. Multiplexing is achieved through a dual barcoding system, and bead-based library preparation protocols allows for in-solution size selection and eliminates the need for columns and gels.

RESULTS

A panel of eight restriction enzymes was selected for testing on B73 maize and Nipponbare rice genomic DNA. Quality of the data was demonstrated by identifying that the vast majority of reads from each enzyme aligned to restriction sites predicted in silico. The link between enzyme parameters and experimental outcome was demonstrated by showing that the sequenced portion of the genome was adaptable by selecting enzymes based on motif length, complexity, and methylation sensitivity. The utility of the new GBS protocol was demonstrated by correctly mapping several in a maize F2 population resulting from a B73×Country Gentleman test cross.

CONCLUSIONS

This technology is readily adaptable to different genomes, highly amenable to multiplexing and compatible with over forty commercially available restriction enzymes. These advancements represent a major improvement in genotyping technology by providing a highly flexible and scalable GBS that is readily implemented for studies on genome-wide variation.

摘要

背景

农业生产和研究中的许多关键领域,如植物和家畜的育种及性状定位,都需要强大且可扩展的基因分型平台。简化基因组测序(GBS)就是一种非常适合非人类生物的方法。在GBS方案中,基因组DNA通过限制性酶切进行片段化,然后通过大小选择实现代表性降低。由于许多限制性位点在一个物种中是保守的,基因组的测序部分在群体内高度一致。这使得GBS方案非常适合需要在群体中检测大量标记的实验,例如那些涉及遗传图谱构建、育种和群体基因组学的实验。我们在多个方面对GBS技术进行了改进。定制的、酶特异性接头已被与平端限制性酶兼容的标准Illumina接头所取代。通过双条形码系统实现多重化,基于磁珠的文库制备方案允许在溶液中进行大小选择,并且无需使用柱子和凝胶。

结果

选择了一组八种限制性酶对B73玉米和日本晴水稻的基因组DNA进行测试。通过鉴定出每种酶的绝大多数 reads 与计算机预测的限制性位点对齐,证明了数据的质量。通过表明基于基序长度、复杂性和甲基化敏感性选择酶可以使基因组的测序部分具有适应性,证明了酶参数与实验结果之间的联系。通过正确定位B73×Country Gentleman测交产生的玉米F2群体中的几个基因座,证明了新GBS方案的实用性。

结论

该技术易于适应不同的基因组,高度适合多重化,并且与四十多种市售限制性酶兼容。这些进展代表了基因分型技术的重大改进,提供了一种高度灵活且可扩展的GBS,可轻松用于全基因组变异研究。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/315b/4253001/12bea9596c09/12864_2014_6697_Fig1_HTML.jpg

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