Multiplex in silico RAPD-Analysis for Genome Barcoding

Q3 Mathematics

Mathematical Biology and Bioinformatics Pub Date : 2022-09-27 DOI:10.17537/2022.17.208

O. Kiryanova, I. Kiryanov, B. Kuluev, R. Garafutdinov, A. V. Chemeris, I. Gubaydullin

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引用次数: 0

Abstract

In this work, we propose a new method for identifying organisms of multiplex polymerase chain reaction (PCR) with arbitrary primers in silico (multiplex in silico RAPD-analysis) for the unique identification of living organisms. The results of computer modeling search of possible primer annealing sites in genomic DNA, and their convertation into the genomic barcode format, are proposed. These data with information about used primers that can be unique for genomes. A comparative analysis of genomic barcodes of species of related plant species was carried out in order to classify them on the level of species and lines in the future. A pairwise analysis of the location of the same or similar amplicons within different subgenomes and genomes is presented. The genomes of wheat and Aegilops in FASTA files format are presented as the research samples. The proposed method makes possible to predict the success of the multiplex polymerase chain reaction using special primers in the laboratory. This technology allows the analysis of the entire genomic DNA, rather than fragments of the genome.

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基因组条形码的多重rapd分析

在这项工作中，我们提出了一种用任意引物在硅中鉴定多重聚合酶链反应(PCR)生物的新方法(多重硅rapd分析)，用于生物的独特鉴定。提出了基因组DNA中可能引物退火位点的计算机模拟搜索结果，并将其转换为基因组条形码格式。这些数据包含了使用过的引物的信息，这些引物对于基因组来说是独一无二的。对近缘植物种间的基因组条形码进行比较分析，以便今后在种和系的水平上进行分类。对不同亚基因组和基因组中相同或相似扩增子的位置进行了两两分析。以FASTA文件格式的小麦和羊蹄草基因组为研究样本。所提出的方法使得在实验室中使用特殊引物预测多重聚合酶链反应的成功成为可能。这项技术可以分析整个基因组DNA，而不是基因组的片段。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Mathematical Biology and Bioinformatics Mathematics-Applied Mathematics

CiteScore

1.10

自引率

0.00%

发文量