A high-density, multi-parental SNP genetic map on apple validates a new mapping approach for outcrossing species

Pierro, Erica A. Di; Gianfranceschi, L.; Guardo, Mario Di; Putten, Herma Jj Koehorst-van; Kruisselbrink, Johannes W.; Longhi, Sara; Troggio, Michela; Bianco, Luca; Muranty, Hélène; Pagliarani, Giulia; Tartarini, Stefano; Letschka, Thomas; Lozano, Lidia; Garkava-Gustavsson, Larisa; Micheletti, Diego; Bink, M.C.A.M.; Voorrips, Roeland E.; Ebrahimi, Aziz; Velasco, Riccardo; Laurens, François; Weg, Eric van de

doi:10.1038/hortres.2016.57

Cited by 73 publications

(101 citation statements)

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“…The optical mapping then allowed us to produce scaffolds with a N50 of 5.5 Mb, which, in association with a high-density integrated linkage map, yielded highly contiguous pseudomolecules. In this new apple genome, we followed a newer convention 23 in which the orientation of Chr10 and Chr05 became aligned by the inversion of Chr05. We chose to invert Chr05 because it is the least frequently reported of the two in previous genetic studies on quantitative trait loci (QTL), gene discovery and characterization.…”

Section: Discussionmentioning

confidence: 99%

“…This consensus map was then used for the hybrid assembly with the corrected scaffolds, which, together with single-nucleotide polymorphism (SNP) markers derived from a high-density genetic linkage map 23 , allowed the construction of the 17 pseudochromosomes (Supplementary Table 2 and Supplementary Note). To estimate the genome size, we calculated different k-mer frequency distributions of the Illumina reads.…”

Section: Genome Sequencing Assembly and Scaffoldingmentioning

confidence: 99%

“…An integrated multiparental genetic linkage map of apple 23 that was composed of 15,417 SNP markers was used to organize and orientate the scaffolds into chromosomesized sequences. The probe sequences of the 15,417 markers 64 were mapped onto the genome using BWA-MEM.…”

Section: Author Contributionsmentioning

confidence: 99%

“…This assembly resulted from a combination of short High-quality de novo assembly of the apple genome and methylome dynamics of early fruit development 1 1 0 0 VOLUME 49 | NUMBER 7 | JULY 2017 Nature GeNetics A r t i c l e s (Illumina) and long sequencing reads (PacBio), along with scaffolding based on optical maps (BioNano) and a high-density integrated genetic linkage map 23 . This chromosome-scale assembly was complemented by a detailed de novo annotation of genes based on RNA sequencing (RNA-seq) data, TE annotation and small RNA alignments.…”

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High-quality de novo assembly of the apple genome and methylome dynamics of early fruit development

et al. 2017

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Using the latest sequencing and optical mapping technologies, we have produced a high-quality de novo assembly of the apple (Malus domestica Borkh.) genome. Repeat sequences, which represented over half of the assembly, provided an unprecedented opportunity to investigate the uncharacterized regions of a tree genome; we identified a new hyper-repetitive retrotransposon sequence that was over-represented in heterochromatic regions and estimated that a major burst of different transposable elements (TEs) occurred 21 million years ago. Notably, the timing of this TE burst coincided with the uplift of the Tian Shan mountains, which is thought to be the center of the location where the apple originated, suggesting that TEs and associated processes may have contributed to the diversification of the apple ancestor and possibly to its divergence from pear. Finally, genome-wide DNA methylation data suggest that epigenetic marks may contribute to agronomically relevant aspects, such as apple fruit development.

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Section: Discussionmentioning

confidence: 99%

Section: Genome Sequencing Assembly and Scaffoldingmentioning

confidence: 99%

Section: Author Contributionsmentioning

confidence: 99%

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High-quality de novo assembly of the apple genome and methylome dynamics of early fruit development

et al. 2017

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“…The red bayberry genome size is small and simple (around 320 Mb), being diploid with intermediate heterozygosity. The female and male independent assemblies, reciprocal sequence comparison at micro level in contigs and an efficient mapping approach (Di Pierro et al ., ), led to high quality of assembly, with an extended total and oriented size of the female pseudochromosome of 280 Mb (87%) and 264 Mb (82%) of the male (Table ). Due to genetic diversity of two parents, 65% of haplotype blocks (HB) in the linkage map was heterozygous (Figure S3), which is helpful to define HB and anchor scaffolds in right position and orientation.…”

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confidence: 99%

The red bayberry genome and genetic basis of sex determination

Jia

Cai³

et al. 2018

Plant Biotechnology Journal

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Morella rubra, red bayberry, is an economically important fruit tree in south China. Here, we assembled the first high-quality genome for both a female and a male individual of red bayberry. The genome size was 313-Mb, and 90% sequences were assembled into eight pseudo chromosome molecules, with 32 493 predicted genes. By whole-genome comparison between the female and male and association analysis with sequences of bulked and individual DNA samples from female and male, a 59-Kb region determining female was identified and located on distal end of pseudochromosome 8, which contains abundant transposable element and seven putative genes, four of them are related to sex floral development. This 59-Kb female-specific region was likely to be derived from duplication and rearrangement of paralogous genes and retained non-recombinant in the female-specific region. Sex-specific molecular markers developed from candidate genes co-segregated with sex in a genetically diverse female and male germplasm. We propose sex determination follow the ZW model of female heterogamety. The genome sequence of red bayberry provides a valuable resource for plant sex chromosome evolution and also provides important insights for molecular biology, genetics and modern breeding in Myricaceae family.

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Efficiency of Bayesian quantitative trait loci mapping with full‐sib progeny

et al. 2020

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Quantitative trait loci (QTL) mapping with perennial crops is based on one or more full‐sib progeny because homozygous genotypes are difficult to obtain. The objective of this study was to assess the efficiency of Bayesian QTL mapping with full‐sib progeny. The analyses used two simulated data sets, one assuming genotyping for 292 simple sequence repeats (SSR) loci (density of 10 cM) and the other assuming genotyping for 2969 single nucleotide polymorphisms (SNPs) (density of 1 cM). Each data set consisted of 50 replications of 40 full‐sib progeny of size 400. We assumed a broad sense heritability of 60%, genetic control by 10 QTLs and 90 minor genes, and positive dominance. The QTL heritability values ranged from 1 to 12%. The scenarios included one and multiple progeny. In the best scenarios for the low (four progeny of size 400) and high marker density (one progeny of size 400), the average power of detection was 52 and 67% for the low heritability QTLs, 83 and 95% for the average heritability QTLs, and 95 and 94% for the high heritability QTLs, respectively. The observed false discovery rate (FDR) was 15 and 9% with low and high density, respectively. The Bayesian QTL mapping provides a precise localization of candidate genes with a bias in the QTL position of approximately 4–6 cM. The polygenic effect is important to control the false discovery rate (FDR) and to provide a higher power of QTL detection with multiple progeny.

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A high-density, multi-parental SNP genetic map on apple validates a new mapping approach for outcrossing species

Cited by 73 publications

References 81 publications

High-quality de novo assembly of the apple genome and methylome dynamics of early fruit development

High-quality de novo assembly of the apple genome and methylome dynamics of early fruit development

The red bayberry genome and genetic basis of sex determination

Efficiency of Bayesian quantitative trait loci mapping with full‐sib progeny

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