ASAS-EAAP Talk: Low-coverage whole-genome sequencing in local livestock breeds

ASAS-EAAP Talk: Low-coverage whole-genome sequencing in local livestock breeds

Current European regulations for autochthonous livestock breeds put a special emphasis on pedigree completeness, which requires laboratory paternity testing by genetic markers in most cases. This entails significant economic expenditure for breed societies and precludes other investments in breeding...

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Veröffentlicht in:Journal of animal science 2020-11, Vol.98, p.81-81
Hauptverfasser: Casellas, Joaquim, de Hijas-Villalba, Melani Martín, Vázquez-Gómez, Marta, Lahoucine, Samir Id
Format: Artikel
Sprache:eng
Schlagworte:
Alleles
Animal husbandry
Breeding
Chromosomes
Diploids
Errors
Gene frequency
Gene sequencing
Genetic markers
Genomes
Livestock
Livestock breeding
Mutation
Mutation rates
Offspring
Paternity
Paternity testing
Population genetics
Recombination
Single-nucleotide polymorphism
Whole genome sequencing
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Zusammenfassung:Current European regulations for autochthonous livestock breeds put a special emphasis on pedigree completeness, which requires laboratory paternity testing by genetic markers in most cases. This entails significant economic expenditure for breed societies and precludes other investments in breeding programs, such as genomic evaluation. Within this context, we developed paternity testing through low-coverage whole-genome data in order to reuse these data for genomic evaluation at no cost. Simulations relied on diploid genomes composed by 30 chromosomes (100 cM each) with 3,000,000 SNP per chromosome. Each population evolved during 1,000 non-overlapping generations with effective size 100, mutation rate 10-4, and recombination by Kosambi's function. Only those populations with 1,000,000 ± 10% polymorphic SNP per chromosome in generation 1,000 were retained for further analyses, and expanded to the required number of parents and offspring. Individuals were sequenced at 0.01, 0.05, 0.1, 0.5 and 1X depth, with 100, 500, 1,000 or 10,000 base-pair reads and by assuming a random sequencing error rate per SNP between 10-2 and 10-5. Assuming known allele frequencies in the population and sequencing error rate, 0.05X depth sufficed to corroborate the true father (85,0%) and to discard other candidates (96,3%). Those percentages increased up to 99,6% and 99,9% with 0,1X depth, respectively (read length = 10,000 bp; smaller read lengths slightly improved the results because they increase the number of sequenced SNP). Results were highly sensitive to biases in allele frequencies and robust to inaccuracies regarding sequencing error rate. Low-coverage wholegenome sequencing data could be subsequently integrated into genomic BLUP equations by appropriately constructing the genomic relationship matrix. This approach increased the correlation between simulated and predicted breeding values by 1.21% (h2 = 0.25; 100 parents and 900 offspring; 0.1X depth by 10,000 bp reads). Although small, this increase opens the door to genomic evaluation in local livestock breeds.
ISSN:0021-8812
1525-3163