4.8 Article

RJPrimers: unique transposable element insertion junction discovery and PCR primer design for marker development

期刊

NUCLEIC ACIDS RESEARCH
卷 38, 期 -, 页码 W313-W320

出版社

OXFORD UNIV PRESS
DOI: 10.1093/nar/gkq425

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资金

  1. US National Science Foundation [IOS 0701916, IOS 0822100]
  2. US Department of Agriculture, Agriculture Research Service [5325-21000-014]
  3. Direct For Biological Sciences [0701916] Funding Source: National Science Foundation
  4. Division Of Integrative Organismal Systems [0701916] Funding Source: National Science Foundation

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Transposable elements (TE) exist in the genomes of nearly all eukaryotes. TE mobilization through 'cut-and-paste' or 'copy-and-paste' mechanisms causes their insertions into other repetitive sequences, gene loci and other DNA. An insertion of a TE commonly creates a unique TE junction in the genome. TE junctions are also randomly distributed along chromosomes and therefore useful for genome-wide marker development. Several TE-based marker systems have been developed and applied to genetic diversity assays, and to genetic and physical mapping. A software tool 'RJPrimers' reported here allows for accurate identification of unique repeat junctions using BLASTN against annotated repeat databases and a repeat junction finding algorithm, and then for fully automated high-throughput repeat junction-based primer design using Primer3 and BatchPrimer3. The software was tested using the rice genome and genomic sequences of Aegilops tauschii. Over 90% of repeat junction primers designed by RJPrimers were unique. At least one RJM marker per 10 Kb sequence of A. tauschii was expected with an estimate of over 0.45 million such markers in a genome of 4.02 Gb, providing an almost unlimited source of molecular markers for mapping large and complex genomes. A web-based server and a command line-based pipeline for RJPrimers are both available at http://wheat.pw.usda.gov/demos/RJPrimers/.

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