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Better primer design for metagenomics applications by increasing taxonomic distinguishability

机译:通过提高分类学的可区分性,为宏基因组学应用提供更好的引物设计

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Current methods of understanding microbiome composition and structure rely on accurately estimating the number of distinct species and their relative abundance. Most of these methods require an efficient PCR whose forward and reverse primers bind well to the same, large number of identifiable species, and produce amplicons that are unique. It is therefore not surprising that currently used universal primers designed many years ago are not as efficient and fail to bind to recently cataloged species. We propose an automated general method of designing PCR primer pairs that abide by primer design rules and uses current sequence database as input. Since the method is automated, primers can be designed for targeted microbial species or updated as species are added or deleted from the database. In silico experiments and laboratory experiments confirm the efficacy of the newly designed primers for metagenomics applications.
机译:当前了解微生物组组成和结构的方法依赖于准确估计不同物种的数量及其相对丰度。这些方法大多数都需要有效的PCR,其正向和反向引物与相同的大量可识别物种良好结合,并产生独特的扩增子。因此,毫不奇怪的是,许多年前设计的当前使用的通用引物效率不高,并且无法与最近分类的物种结合。我们提出了一种设计PCR引物对的自动化通用方法,该方法应遵守引物设计规则,并使用当前序列数据库作为输入。由于该方法是自动化的,因此可以针对目标微生物物种设计引物,也可以在数据库中添加或删除物种时对其进行更新。在计算机实验和实验室实验中证实了新设计的引物在宏基因组学应用中的功效。

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