2015
DOI: 10.1186/s12864-015-1309-7
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REDHORSE-REcombination and Double crossover detection in Haploid Organisms using next-geneRation SEquencing data

Abstract: BackgroundNext-generation sequencing technology provides a means to study genetic exchange at a higher resolution than was possible using earlier technologies. However, this improvement presents challenges as the alignments of next generation sequence data to a reference genome cannot be directly used as input to existing detection algorithms, which instead typically use multiple sequence alignments as input. We therefore designed a software suite called REDHORSE that uses genomic alignments, extracts genetic … Show more

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Cited by 6 publications
(7 citation statements)
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“…To more precisely identify SNPs and estimate the recombination intervals, we used a new utility called REDHORSE, which is described in an accompanying software methods paper [ 33 ]. In brief, the REDHORSE software identifies putative recombination breakpoints by evaluating SNPs in each progeny clone and comparing them to the genotype of the parents.…”
Section: Resultsmentioning
confidence: 99%
See 2 more Smart Citations
“…To more precisely identify SNPs and estimate the recombination intervals, we used a new utility called REDHORSE, which is described in an accompanying software methods paper [ 33 ]. In brief, the REDHORSE software identifies putative recombination breakpoints by evaluating SNPs in each progeny clone and comparing them to the genotype of the parents.…”
Section: Resultsmentioning
confidence: 99%
“…The raw reads from the parental lines as well as hybrids were aligned to the ME49 genome v 8.0 by CLC genomics ( http://www.clcbio.com ) using the following parameters- Mismatch cost: 3, Insertion cost: 3, Deletion cost: 3, Length fraction: 0.9, Similarity fraction: 0.8 and by using Global alignment. Since the ME49 genome is haploid, we extracted the alleles with frequency greater than or equal to 80% and having a minimum coverage of 5 using REDHORSE [ 33 ]. Loci that did not meet these criteria were tagged as missing data.…”
Section: Methodsmentioning
confidence: 99%
See 1 more Smart Citation
“…With the advent of microarray technology, crosses could be genotyped at over a thousand marker positions across the genome based on parental SNPs residing within probes on the array, as was done for the type 1 × type 2 cross (9). With NextGen sequencing, genomes can be completely sequenced to identify all the SNPs in the parents and progeny, yielding many thousands of markers (106). The type 2 × type 10 cross was genotyped using whole-genome sequencing allowing for the identification of recombination breakpoints and short double-crossover events in the progeny (60).…”
Section: Genetic Mapping In T Gondiimentioning
confidence: 99%
“…We utilized a previously described genetic cross between type 2 ME49-FUDR r and type 10 VAND-SNF r strains [ 25 , 28 ]. Whole-genome sequencing of 24 progeny and mapping based on genome-wide SNP analysis was previously used to identify the molecular basis of sinefungin resistance [ 29 ].…”
Section: Resultsmentioning
confidence: 99%